thorax trauma-induced experimental lung injury
TRANSCRIPT
Thorax trauma-induced experimental
lung injury
DISSERTATION
zur Erlangung des akademischen Grades eines
Doktors der Naturwissenschaften (Dr. rer. nat.) des Fachbereiches für Biologie
an der Universität Konstanz
vorgelegt
von
Katja Eichert
Konstanz, im Juli 2003
Dissertation der Universität Konstanz
Datum der mündlichen Prüfung: 16.10.2003
1. Referent: Prof. Dr. Albrecht Wendel
2. Referent: Prof. Dr. Klaus Schäfer
Table of Contents
I
Table of Contents 1. Introduction....................................................................................................... 1
1.1 The lung.................................................................................................................. 1 1.1.1 Lung morphology and aerodynamics.................................................................... 1 1.1.2 Physiological parameters of the lung .................................................................... 2
1.2 Pulmonary oedema ................................................................................................ 3 1.2.1 Alveolar liquid clearance....................................................................................... 4
1.3 Mechanisms of host defence ................................................................................ 5 1.4 Multiple trauma..................................................................................................... 11
1.4.1 Impact of trauma on patients and society ........................................................... 11 1.4.2 Blast injury.......................................................................................................... 11 1.4.3 Chest trauma...................................................................................................... 12 1.4.4 Molecular injury .................................................................................................. 15 1.4.5 Management of pulmonary blast injury ............................................................... 16 1.4.6 Immunomodulation after trauma......................................................................... 16
2. Aims of the Study ........................................................................................... 18
3. Materials and Methods ................................................................................... 19 3.1 Animals................................................................................................................. 19 3.2 Chemicals ............................................................................................................. 19
3.2.1 Chemicals used in the isolated perfused rat lung experiments ........................... 19 3.2.2 Chemicals used in the in vitro experiments......................................................... 20 3.2.3 Other chemicals ................................................................................................. 20 3.2.4 Solutes ............................................................................................................... 21 3.2.5 Anaesthesia and analgesic................................................................................. 21 3.2.6 Cell culture material............................................................................................ 21
3.3 Laboratory equipment and technical devices .................................................... 21 3.4 The in vivo blast wave thorax trauma in rats ..................................................... 22
3.4.1 The blast wave generator apparatus .................................................................. 22 3.4.2 Pressure wave monitoring .................................................................................. 23 3.4.3 Protocol of anaesthesia and analgesic ............................................................... 24 3.4.4 Experimental protocol......................................................................................... 25 3.4.5 Determination of an injury score and validation .................................................. 26
3.5 The isolated ex vivo perfused and ventilated rat lung....................................... 27 3.5.1 Isolated perfused rat lung preparation ................................................................ 27 3.5.2 Experimental Setup ............................................................................................ 27 3.5.3 Experimental design of the perfused lung studies............................................... 28
3.6 In vitro stimulation of primary rat alveolar macrophages ................................. 29
Table of Contents
II
3.6.1 Preparation and culturing of rat alveolar macrophages....................................... 29 3.6.2 Stimulation with dead, fluorescent bacteria......................................................... 30 3.6.3 Stimulation with endotoxin.................................................................................. 30 3.6.4 Fluorescence labelled E. coli/ S. aureus phagocytosis assay ............................. 30 3.6.5 Assay for superoxide production ........................................................................ 31 3.6.6 Preparation of washed and haemolysed erythrocytes and haemolysat............... 32 3.6.7 Lysis of erythrocytes........................................................................................... 32 3.6.8 Experimental design of the in vitro experiments.................................................. 33
3.7 Lung lavage .......................................................................................................... 33 3.8 Determination of the alveolar haemorrhage....................................................... 34 3.9 Total and differential cell counts and cell viability ............................................ 34 3.10 Determination of total protein content................................................................ 34 3.11 Cytokines determinations.................................................................................... 34 3.12 Measurement of eicosanoids .............................................................................. 35 3.13 Determination of NO production......................................................................... 35 3.14 Measurement of lactate dehydrogenase ............................................................ 36 3.15 Measurement of CINC-3....................................................................................... 36 3.16 Gelatin zymograpy ............................................................................................... 36 3.17 Lung Wet/ Dry-Ratio............................................................................................. 37 3.18 Histological examinations ................................................................................... 37 3.19 Statistics............................................................................................................... 37
4. Results............................................................................................................. 38 4.1 System characteristics ........................................................................................ 38
4.1.1 Variability and influence of physical parameters ................................................. 38 4.2 Functional changes of alveolar macrophages and interaction with blood in vitro after trauma ............................................................................................................. 43
4.2.1 Trauma-induced impairment in host defence mechanisms ................................. 43 4.2.2 Role of the trauma-induced alveolar haemorrhage in impaired macrophage
functions......................................................................................................................... 48 4.2.3 Influence of different blood components on the macrophage function ................ 50 4.2.4 Summary of the in vitro findings ......................................................................... 53
4.3 Functional consequences and endogenous modulation in vivo ...................... 55 4.3.1 Blast injury-induced disruption of the alveolar capillary barrier............................ 55 4.3.2 Blast injury-related mediator release .................................................................. 60 4.3.3 Infiltration of inflammatory cells .......................................................................... 64
4.4 Ex vivo lung perfusion: Trauma-induced changes in lung function................. 69 4.4.1 Interrelationships between physical and physiological injury .............................. 69
Table of Contents
III
4.4.2 Time-dependent recovery of the lung function after trauma................................ 73 4.4.3 Pharmacological intervention.............................................................................. 76
5. Discussion....................................................................................................... 83 5.1 A laboratory model for studying primary blast injury ....................................... 84
5.1.1 Rationale for the development of the blast thorax trauma rat lung model ........... 84 5.1.2 Standardization and monitoring of the blast pressure wave................................ 84 5.1.3 Standardization of the blast thorax trauma in rats............................................... 86
5.2 Combination of the in vivo thorax trauma model with ex vivo lung perfusion 86 5.2.1 Match of physical and biological impact.............................................................. 87 5.2.2 Time-dependence of the lung dysfunction .......................................................... 88 5.2.3 Pharmacological modulation of the injury ........................................................... 89
5.3 Thorax trauma-related pathophysiological changes in vivo over time ............ 91 5.3.1 Structural integrity of the lung tissue after blast injury......................................... 91 5.3.2 Mediator release in response to primary blast injury........................................... 93 5.3.3 Thorax trauma-related chemokine release and inflammatory cell infiltration ....... 97 5.3.4 Oedema generation and resorption after thorax trauma: Comparison of the ex
vivo and in vivo results.................................................................................................... 98 5.4 Thorax trauma-related impairment of alveolar macrophage function in vitro . 98
5.4.1 Alveolar macrophage population after trauma .................................................... 98 5.4.2 Phagocytic capacity, microbial killing and TNF release....................................... 99 5.4.3 Involvement of trauma-related alveolar haemorrhage in impaired macrophage
functions....................................................................................................................... 103
6. Summary ....................................................................................................... 105
7. Deutsche Zusammenfassung ...................................................................... 107
8. References .................................................................................................... 110
9. Abbreviatons................................................................................................. 120
Introduction
1
1. Introduction
1.1 The lung
The lung is the central organ for gas exchange of land-living animals, including mammals. The
respiratory system is one of the primary interfaces between the organism and the
environment. As a result of air circulating through the respiratory system, the latter represents
a target for toxic gases, airborne particulates, and infectious agents. Because the entire output
of the right heart also passes through the vascular bed of the lung, this organ is also a target
for blood-borne toxicants and pathogens. Therefore, the lung also has many non-respiratory
functions, such as metabolism, mediator synthesis, host defence and the clearance of
substances from the pulmonary circulation. The respiratory system, especially the conducting
airways and gas exchange area of the lungs, is organized in a highly polarized fashion. As a
consequence, most of the pathological responses within the lung tend to be highly focal and
generally target one or more small subpopulations of the over 40 different cell types found in
this organ. Thus, the cellular composition and architectural organization of airway and gas
exchange tissue have major impacts on the pathological responses within the system. This
chapter will only focus on physiological aspects and metabolic functions pertinent to the
present study.
1.1.1 Lung morphology and aerodynamics
Most of the thoracic cavity is occupied by the right and the left lungs, which are divided into
three and two lobes, respectively. The anatomical structure of the lung combines the
respiratory system and the blood circulation. During breathing, the inhaled air enters the lung
via the trachea and flows towards the respiratory zone driven by pressures, generated by
constriction of the inspiratory muscles. The airways divide about 25 times, depending on the
species. The trachea branches out into the two main bronchi, which then further divide in the
lobular bronchioles, the respiratory bronchioles and the alveolar ducts, which end blindly in the
alveoli. The upper airways are stabilized by cartilage; towards the lower airways less cartilage
but more contractile muscle fibers and elastic fibers are found. The total number of airways
grows exponentially and with each division the total diameter increases, while the diameter of
the single airways decreases. The total area of the 300 million alveoli is estimated to vary
between 80 and 140 m2 (depending on the publication) in the adult lung. The alveoli are 0.2 –
0.3 mm in diameter and are surrounded by a net of capillaries with 5 µm in diameter. Here, at
the very thin alveolar-capillary membrane (0.2 – 0.6 µm), oxygen and carbon dioxide
Introduction
2
exchange occurs. This membrane consists of capillary epithelial cells, a very narrow
interstitium and endothelial cells. Two different systems ensure the blood supply of the lung:
i) the pulmonary circulation (low pressure system), which starts at the right ventricle,
leaving the heart via the pulmonary artery which carries the oxygen-poor blood to
the lung. After saturation with oxygen, the blood leaves the lung by the pulmonary
vein, which ends in the left atrium of the heart.
ii) The bronchial circulation (high pressure system) supplies the central airways and
vessels as well as lung nymph nodes with blood.
The alveolar epithelium is composed mainly of cuboidal type II pneumocytes and large, flat
type I pneumocytes. Alveolar type II pneumocytes synthesize, store and secrete the highly
surface active pulmonary surfactant, a heterogeneous mixture of lipids and proteins, that
reduces surface tension along the air-liquid interface and prevents alveolar collapse upon
expiration. The main function of the type I pneumocytes is the formation of the air-blood
barrier and therefore they facilitate the gas exchange. Alveolar and interstitial macrophages,
eosinophils and neutrophils are also located in the lung, in order to maintain its immunological
functions.
1.1.2 Physiological parameters of the lung
The functional properties of the lung, i.e. the airway and vascular mechanics, are
characterized by different lung function parameters, including the tidal volume, the pulmonary
compliance, the airway resistance, the vascular resistance, and the extent of extravascular
lung water (oedema). The determination of these parameters is not only interesting for the
diagnosis used by the medical specialist, but also for the scientist. Various experimental
approaches in whole animals or in isolated organs, such as the isolated perfused rat lung, 1
have been done to investigate these lung parameters.
1.1.2.1 Airway mechanics
The tidal volume is the amount of air which enters the lung during a single breathing cycle of
inspiration and expiration. It can be calculated by integrating the airflow velocity during
respiration. The driving force for the airflow in the airways is the transpulmonary pressure, e.g.
the difference between the alveolar and the pleural pressure. During inspiration, the thorax
expands, thus the pleural pressure decreases, and the transpulmonary pressure increases,
causing inspiratory airflow from the outside into the alveoli. During expiration, the thorax
relaxes forcing expiratory airflow back into the atmosphere. At a given transpulmonary
pressure, tidal volume depends mainly on two parameters: airway resistance and lung
compliance. The airway resistance is an index for the resistive forces against the airflow in the
Introduction
3
airways and depends on the diameter and the length of the airways. Because the total
diameter is lowest in the upper airways, this region accounts for the major part of the airway
resistance. The airway resistance can be calculated from the relation between transpulmonary
pressure and airflow velocity. The airway resistance increases, as a consequence of
narrowing the airways due to bronchoconstriction or obstructive processes, e.g. bronchial
oedema or enhanced mucus deposition.
The pulmonary compliance is a marker for the functional stiffness of the lung and thus
depends on properties of the peripheral lung tissue, such as elastic fibers. The compliance
can be calculated from the relation between tidal volume and transpulmonary pressure and
thus is also affected by the air volumes at which it is calculated and the lung volume history.
The pulmonary compliance decreases during restrictive pathological changes e.g. atelectasis,
fibrosis, loss of elastic fibers, pulmonary oedema or disturbed surfactant secretion.
1.1.2.2 Vascular mechanics
The pulmonary blood flow is regulated by contractile elements of the pulmonary vasculature
and depends mainly on the smooth muscle tone of the small arteries. The vascular resistance
is calculated from the ratio between the blood pressure difference (Part - Pven) and blood flow
rate. This parameter is increased as a consequence of vasoconstriction, but also of air emboli
and vascular obliteration, due to thrombus formation or blood cell aggregation.
1.2 Pulmonary oedema
The term oedema denotes the presence of abnormally high amounts of water in the
interstitium (interstitial oedema) or in the alveoli (alveolar oedema). Under physiological
conditions, the positive hydrostatic blood pressure, interstitial pressure and oncotic forces are
in balance and small amounts of excess water are drained of by the lymphatic system. Only
when the lymph`s capacity is exceeded e.g. due to massive interstitial fluid accumulation or
loss of the alveolar-capillary barrier integrity, water gets access into the alveoli. The
consequences are impaired gas exchange and a loss of pulmonary compliance. Depending
on the cause, two different kinds of oedema formation can be determined: Cardiogenic or
hydrostatic oedema and non-cardiogenic or high permeability oedema. The former is due to
enhanced capillary pressure, leading to subsequent water influx into the interstitial space,
whereas the latter is independent of the hydrostatic pressure and is related to an impaired
permeability for water and/ or proteins. Non-cardiogenic oedema and hypotension represent
the hallmarks of ARDS (adult respiratory distress syndrome).
Introduction
4
1.2.1 Alveolar liquid clearance
Sodium and fluid transport across the intact respiratory epithelium
Although, for many years, Starling forces (hydrostatic and protein osmotic pressures) were
thought to play a major role in maintaining the alveolar space free of fluid 2, there is now
strong evidence that active ion transport across the alveolar epithelium creates an osmotic
gradient that leads to water reabsorption both during the perinatal period 3 and in adulthood 4
(reviewed by Matthay and coworkers, 5; Sartori and Matthay, 6). Despite significant species
differences in the basal rates of sodium and fluid transport 7-12, the basic mechanisms seem to
be comparable. On the apical membrane of alveolar type II cells there is a sodium uptake by
amiloride-sensitive cation channels, such as the amiloride-sensitive epithelial sodium channel
(ENaC) as well as by several other non-selective cation channels 3,4,13. On the basolateral
surface of the cell, sodium is discharged into the interstitium by the ouabain-sensitive sodium/
potassium adenosine triphosphatase (Na+/ K+-ATPase) 14,15. In addition to the sodium
transport, a pathway for chloride transport, involving CFTR (cystic fibrosis transmembrane
regulator chloride channel) is suggested to play an important role in fluid resorption 16. CFTR
activation was recently suggested to regulate ENaC 17. Due to the osmotic gradient, water
follows passively, probably through water channels (the aquaporins, AQPs) 18,19, although the
presence of these water channels is not required for maximal alveolar epithelial transport in
the lung 20. This process can be upregulated by several catecholamine-dependent and
independent mechanisms.
Regulation of alveolar transepithelial fluid transport
Beta2-adrenergic agonists can upregulate alveolar fluid clearance in isolated perfused rat
lungs 21,22, ventilated rats 8, sheep 7 and dogs 23 as well as in mice 24, partly due to cyclic
adenosine monophosphate (cAMP)-dependent mechanisms 25. Furthermore β1-adrenergic
stimulation is reported to be also effective in upregulating fluid resorption. Both β1- and
β2-receptors are detectable on both the apical and basolateral surface of the alveolar
epithelium 26.
Hormones like epidermal growth factor (EGF) 27, keratinocyte growth factor (KGF) 28 or TGFα 29 are capable of inducing a catecholamine-independent increase of the alveolar fluid
clearance, primarily by stimulating alveolar type II cell proliferation.
Introduction
5
Sodium and fluid transport across the respiratory epithelium in acute lung injury
A profound injury to the alveolar epithelium can disrupt the integrity of the alveolar barrier and/
or downregulate ion transport pathways, thus reducing net alveolar fluid reabsorption and
enhancing the extent of alveolar oedema. Endogenous catecholamines in experimental rat
models of hyperoxia 30, haemorrhagic shock 31, septic shock 32 and in a canine model of
neurogenic pulmonary oedema 33 were reported to stimulate the alveolar fluid clearance.
Alternatively, catecholamine-independent stimulation of the fluid transport may occur due to a
mechanism involving the lectin-like domain of TNF 34,35.
Pharmacological stimulation of the alveolar fluid clearance
Beta2-agonists are attractive therapeutic agents because of their minimal side effects even in
critically ill patients 36. They accelerate not only the resolution of experimental induced alveolar
oedema, e.g. aerosolized salmeterol in sheep 37, moderate injury due to hyperoxia in rats 38,
but also increase the secretion of surfactant and perhaps exert an anti-inflammatory effect 39,
thus helping to restore the vascular permeability of the lung 40. With regard to accelerate re-
epithelialization of the alveolar barrier in the case of acute lung injury 41, benefits with KGF
pre-treatment 42 have been achieved. The combination of KGF and β2-agonist treatment
results in an additive upregulation of fluid clearance 43. This suggests that there may be
mechanisms for providing both short-term (β2-agonist) and long-term (growth factors)
upregulation of fluid transport, that might hasten the resolution of clinical pulmonary oedema.
1.3 Mechanisms of host defence
The respiratory tract is situated at the interface between the environmental air and the internal
tissues of the organism. During normal ventilation or as a result of aspiration, noxious
materials, including infectious agents, are deposited on mucosal surfaces of the airways and
penetrate into the depths of the lung parenchyma. Foreign material encounters a highly
integrated system of natural and acquired defence mechanisms, that prevent injury, infections,
and invasion of host tissue 44-46. This system of host defence includes mechanical (filtration,
cough, mucociliary clearance), molecular (airway secretions), phagocytic, and antigen-specific
immune mechanisms (B- and T-cell-mediated reactions) of resistance (reviewed in 47).
Introduction
6
1.3.1.1 The alveolar macrophage
The alveolar macrophage (AM) is the primary resident respiratory cell responsible for
maintaining the sterility of the alveolar space and thus represents the first line of defence. As a
mobile cell and representative of the mononuclear phagocyte system, the AM is believed to be
the central modulator, as both regulator and effector of the degree of inflammation and anti-
inflammation within the alveolar space 48. This metabolically highly active cell scavenges
particulate matter, removes macromolecular debris, kills microorganisms, functions as an
accessory cell in immune response, maintains and repairs the lung parenchyma and provides
surveillance against neoplasms 49. Since the pulmonary alveolar macrophages are enveloped
by surfactant in vivo, and since their lysosomes contain hydrolytic enzymes necessary for
surfactant degradation 50, it is believed that alveolar macrophages are also involved in the
clearance of surfactant from the alveoli. When confronted with a particularly large inoculum of
microorganisms, the AM supplements its direct antimicrobial capabilities by recruiting and
activating polymorphonuclear leukocytes (PMN) from the bloodstream, which may represent
the second line of defence. Approximately 40% of the body’s PMN’s are marginated within the
microvasculature of the lungs, facilitating the recruitment to the alveolus, or to other sides of
the body 51.
1.3.1.2 Location and origin
Pulmonary macrophages constitute the most abundant non-parenchymal cell type in the lung 52. Macrophages are present in the alveoli (alveolar macrophages, AM), interstitial spaces
(interstitial macrophages), intravascular spaces (intravascular macrophages), conducting
airways (airway macrophages), pleura (pleural macrophages), and lymph nodes (lymph note
macrophages) 53,54.
Alveolar macrophages initially encounter materials, that reach gas exchange units and
subsequently perform phagocytosis and microbial killing. Interstitial macrophages serve as
precursors for physiologic renewal of alveolar macrophages and for their expansion during
pulmonary inflammation 53. Adhering to the pulmonary endothelial cells, intravascular
macrophages remove circulating particles, but may also contribute to pathogenesis during
sepsis 48,55. Airway macrophages are responsible for the reactivity of the conductive airways in
response to inhaled stimuli in patients with asthma 47.
The ultimate source of pulmonary macrophages are monocyte progenitor cells in the bone
marrow 56, which enter the lung from the vascular bed, and adapt to the local environment by
maturation into tissue macrophages. Maturation results in an increase in cell size, in the
number of cytoplasmatic organelles, lysosomal enzyme activity, phagocytosis capacity, and
expression of Fc, complement and cytokine receptors on surface membranes 54. Alveolar
Introduction
7
macrophages vary considerable in size and morphologic features. They represent both
phenotypically and functionally a heterogenous population of cells 57. Pulmonary macrophages
live for weeks to months and possess some limited replicative potential 58. It is believed that
the effector arm of the cell-mediated immune response depends on both the activation of
resident macrophages as well as on the recruitment of circulating monocytes into the alveoli 58. However, the proportion of monocyte influx and local replication during the pulmonary
inflammation has to be defined.
Chemotactic factors like complement component C5a, transforming growth factor beta (TGF-
β), formylated peptides and monocyte-chemotactic peptide (MCP-1), stimulate the influx of
monocytes into the lung (reviewed in 50). To exert their effector functions, alveolar
macrophages have to be either activated non-specifically by adherence 59 or usually through
ligand-to-receptor coupling. Among a large number of receptors expressed on alveolar
macrophages 57, immunoglobulin (Ig) and complement (C) receptors (CR1, CR3) participate in
receptor-mediated phagocytosis. The former bind to the Fc portion of Ig molecules (IgG, IgA,
IgE), whereas the latter are important natural opsonins for microbial organisms and
particulates 60. Macrophages further express C5a, a potent chemotactic, cell-activating and
pro-inflammatory molecule, as well as various cytokine receptors for interleukin-1 (IL-1), tumor
necrosis factor (TNF), interferon γ (INF-γ), growth factor receptors and cell activation factors
e.g. lectins, lipoproteins and glucocorticoids (reviewed in 50,57).
CD14, a 55-kDa phosphatidylinositiol-anchored membrane glycoprotein expressed on the
surface of monocytes, macrophages, and, to a lesser extent on neutrophils 61 has been
identified as an important receptor for LPS, in association with LPS-binding protein (LBP). The
stimulation of CD14 triggers a concentration-dependent macrophage activation 62. This
activation results in the release of TNF, IL-6 and IL-8 63,64 and has been described as both
LBP-dependent and -independent 63. Haugen and coworkers reported a higher expression of
CD14 on monocytes (MO) than on AM, with AM of different size and maturity having different
CD14 expression levels. The expression of CD14 can be modulated in response to LPS, but
the LPS binding capacity of AM and MO does not correlate with their CD14 levels 65. Indeed,
several other macrophage receptors that function as LPS receptors have been described 66.
1.3.1.3 Secretory function
Macrophages are pluripotent cells. The range of products secreted by alveolar macrophages
is broad, with over 100 molecular species having been identified, including reactive oxygen
species, proteases and anti-proteases, bioactive lipids, cytokines as well as growth factors
(reviewed in 50).
Introduction
8
Reactive oxygen radicals are generated via the “respiratory burst”. Together with several
proteases and other enzymes that function intracellularly, reactive oxygen species are
involved in microbial killing. Secreted proteinases (metalloproteinases, serine proteinases)
affect fibrinolysis and extracellular matrix remodelling 50. Stimulation of alveolar macrophages
with IgG or IgE immune-complexes leads to the production of both cyclooxygenase-derived
(thromboxane A2 and prostaglandin E2 and D2) and lipoxygenase-derived (leukotriene B4)
compounds 67. In the IgG immune complex animal model of acute lung injury 68,
bronchoalveolar lavage fluids contain large amounts of biologically active TNF and IL-1. These
“early response cytokines” function in a pro-inflammatory manner, by playing a key role in the
upregulation or induction of adhesion molecules in the lung vasculature, such as ICAM-1 and
E-selectin, which are critically necessary for neutrophil recruitment. In this regard, the α-
chemokine family (IL-8 or its family relatives such as MIP-2, CINC) are described to have
chemotactic activity primarily for neutrophils and to a lesser extent for T-cell subsets, while the
β-chemokines (e.g. MIP-1a, b; MCP-1, 2 and 3) are thought to be predominantly chemotactic
for monocytes and lymphocytes. In contrast, there are various anti-inflammatory cytokines
such as IL-10, IL-4, IL-6 or IL-13 produced by alveolar macrophages to suppress the cytokine
production and therefore regulate the intensity of the inflammatory response (reviewed in 69).
In addition to cytokines, also lipid mediators such as leukotrienes (LT) upregulate directly the
antimicrobial potential of macrophages as well as PMN’s from different species against both
bacteria and fungi (reviewed in 70). Leukotriene levels have been shown to be elevated in
bronchoalveolar lavage fluid from patients with bacterial pneumonia and also in lung tissue in
animal models of pneumonia 70.
1.3.1.4 Phagocytic function
Macrophages remove materials present in the local environment through both pinocytosis and
phagocytosis. In contrast to pinocytosis, phagocytosis is an energy-dependent process,
characterized by adherence through receptors and engulfment, leading further to
internalisation of the particulates and finally to digestion in phagolysosomal vacuoles. Efficient
phagocytosis depends on opsonization. Opsonins defined in the lung include IgG1, IgG3, C3b,
surfactant protein A/ D (SP-A/ D) 71,72, mannose and lipopolysaccharide-binding proteins 60.
Furthermore, SP-A has been reported to enhance the phagocytosis of C1q-coated particles by
alveolar macrophages 73. However, binding of inhaled environmental particles must be
accomplished without the benefit of opsonization by specific antibodies. The identities of
receptors on AM’s that mediate unopsonized particle binding are not fully known, whereas the
role of some scavenger receptors (SR) have been recently reported 66,74,75.
Introduction
9
1.3.1.5 Microbicidal function
The production of reactive oxygen species (ROS) upon receptor-mediated stimulation of
phagocytosis was first recognized in phagocytes such as macrophages, a process
determining their microbicidal activity and referred to as respiratory burst. This process results
from the assembly and activation of the nicotinamide dinucleotide phosphate (NADPH)
oxidase, a multicomponent enzyme that catalyses the one-electron reduction of molecular
oxygen to superoxide 76, which is subsequently converted to other oxygen-derived species, by
either spontaneous or enzyme-mediated reduction. ROS generated in an inflammatory milieu
act in an autocrine and paracrine manner, in order to rapidly amplify the effector potential of
Fcγ R on quiescent phagocytes, by means of altering signal transduction (reviewed by Pricop
and Salmon, 77). Controlled upregulation of oxygen generation is important, since
dysregulation or overproduction results in acute tissue injury 78,79. With regard to this, it has
been reported that during the respiratory burst of phagocytic cells in vitro, the superoxide
anion production per cell shows an inverse correlation with the cell density, a phenomenon
described as autoregulation 80. Furthermore, it has been shown that the decrease in individual
cell response is due to a significant increase in the amount of basal responses of the
macrophages, thus, concomitantly, the number of reactive cells remains unchanged,
irrespective of the cell density of the population 78.
In vitro, the respiratory burst can be triggered e.g. by certain soluble (PMA) or particulate
opsonized zymosan (OZ) agents. Both agents produce an intense oxidative burst, although
mediated by different signal transduction pathways: PMA is soluble and associated to cell
membrane perturbations that is dependent on protein kinase C (PKC) activation, whereas
particulate OZ reflects processes related to PKC-independent phagocytic mechanisms 81.
Moreover both stimuli utilize more than one activation pathway to stimulate NADPH-oxidase 82, revealing that different stimuli produce the same reaction in terms of respiratory burst
autoregulation at the single cell level. Together with the LPS-induced oxidative burst (CD14
receptor-dependent) these pathways depend on ERK 1/ 2 activation. Activated ERK kinases
also control the production of TNF in both LPS and PMA membrane activation of human
alveolar macrophages. Whereas LPS activates NFκB nuclear translocation, PMA does not,
but rather activates alveolar macrophages through the ERK 1/ 2 MAP kinase pathway. It has
been shown that IgA, a predominant Ig isotype of respiratory secretions, regulates LPS-and
PMA-induced oxidative burst and TNF through both dependent and independent modulation
of ERK pathways, revealing a role of IgA in both lung protection and inflammation 83. The LPS-
related oxidative burst, TNF and IL-10 release of human monocytes can also be modulated by
IL-9, through an upregulation of TGF-β 84. In contrast, ADP stimulates the respiratory burst,
without activation of ERK in rat alveolar macrophages 85.
Introduction
10
The physiological generation of ROS production has now been clearly implicated in the
activation of signalling pathways, resulting in a broad array of physiological responses ranging
from cell proliferation to gene expression and apoptosis 79,86. In this regard, and as reviewed
by Forman and Torres, 79, it has been suggested that: 1. hydrogen peroxide and superoxide
act as second messengers; 2. anti-oxidant enzymes are implicated in the “turn-off” phase of
signal transduction; 3. the primary physiological role of the respiratory burst in macrophages
may be redox signalling, rather than microbicidal activity.
In contrast to neutrophils, oxygen-dependent killing by macrophages is myeloperoxidase–
independent because they lose this enzyme during maturation 47.
In macrophages from rodents, a second oxidant-generating pathway features inducible nitric
oxide synthase (iNOS), that is inducible by TNF, IL-1, and interferon-γ 69.
1.3.1.6 Immune function
Macrophages contribute importantly to the induction, expression and regulation of immune
responses 47. Alveolar macrophages possess the capacity to serve as antigen presenting cells
(APC’s) and secrete co-stimulatory cytokines, both required for T-cell activation. In contrast to
resting macrophages, alveolar macrophages activated by chronic pulmonary inflammation or
by T-lymphocyte-derived cytokines are more effective in antigen presentation 48. Furthermore,
pulmonary macrophages are important effector cells for T-cell mediated immunity and regulate
immune responses. Thus IFN-γ, secreted by activated T-lymphocytes potently activates
resting macrophages and upregulates these host defence functions 87. The balance between
macrophage-derived enhancing and -suppressive signals determines the degree with which
antigen presentation and induction of immune responses occur. Therefore, not only T-cells,
but also dendritic cells (DCs), another antigen-presenting cell, are maintained in a down-
modulated state in the airways, tightly controlled by high numbers of nearby macrophages 47.
Immuno-modulatory factors involved in this process include among others: AM-derived nitric
oxide (NO) 88, prostaglandin E2 (PGE2) 89,90, TGFβ 91 and IL-10 92.
Introduction
11
1.4 Multiple trauma
1.4.1 Impact of trauma on patients and society
Trauma is generally the third leading cause of death in the United States and specifically the
leading cause of death in men under 40 years of age 93, due to accidents and military causes.
Speed limits combined with improvements in seatbelts, airbags, and vehicle constructions
lead to a decline in the number of accidental deaths, but also result in an increase in the
number of accidental victims suffering from blunt chest trauma. Trauma further represents the
second leading cause of life-threatening acute lung injury, i.e. in its severe form the Adult
Respiratory Distress Syndrome (ARDS) 41,94. Prevention and intervention are thus both a
socio-ethical and economic necessity. After initial, non-fatal injury thoracic trauma is
considered to be an important clue to single or multi-organ failure, itself making the patient
more susceptible to infections 95-97. With exception of changing the ventilation strategy 98, none
of the numerous interventions made it into clinical practice. This emphasizes the need for
further basic understanding of both pathogenesis and consequences of intervention.
1.4.2 Blast injury
Blast injuries are a special form of blunt trauma, with serious internal injuries, often without
evidence of external lesions. Blast injury occurs following a sudden change in environmental
pressure, originating from an explosion. The process of the explosion is equivalent to the
energy release which is then transmitted as a radial pressure wave, called shock-wave, from
the source into the surroundings 99,100. After a short travelling distance, a new shock front with
lower pressure peak and initial velocity is formed in the air, called the blast wave. It travels
supersonically and exerts its effects at comparably long distances from the explosion. The
simple blast wave, described as the Friedlander wave form, rises very rapidly, then decays
slowly (the vacuum phase) and may even drop below the previous ambient pressure. If the
blast is confined by reflective surfaces, then a complex wave-form is formed. Complex blast
waves contain multiple overpressure peaks 101. These wave-forms are usually expressed by
their impulse (integral of pressure changes over time, P/ dt) rather than by their maximum
peak overpressure value alone. Several factors can alter the response to the blast, such as
peak overpressure, duration of the overpressure, impulse (in case of complex wave forms),
the surrounding medium (e.g. water is a dense medium), and the distance from the explosion,
because the effect is inversely proportional to the distance and the body orientation towards
the blast wave front (reviewed by Elsayed, 102). Blast injuries are divided into 4 groups 103,104:
1. primary blast injury due to the blast wave, the effect of which is greatest at gas-liquid
Introduction
12
interfaces, 2. secondary blast injury resulting from flying debris, 3. tertiary blast injury due to
victims being thrown against an object, and 4. miscellaneous blast injuries including exposure
to dust, thermal burns or fire by the blast.
The pressure wave of the primary blast injury, encountering media of different densities in the
body, is reflected, causing turbulence and cavitation. The phenomenon termed “spalling”
describes the process where fluid is thrown from a more dense to less dense medium.
Another effect is the “secondary” explosion or implosion, as a consequence of compression
and re-expansion of gas pockets in the organs by the traversing blast wave. As the blast wave
reaches the surface of the victim’s body, a pressure difference develops between the outer
surface of the body and the internal organs. In air-containing organs like the lung, the air in the
alveoli is easily compressible and thus rupture of the alveolar capillary membrane occurs, with
blood driven from the capillaries into the alveolar space, due to the pressure differences
created. Finally, inertia is the shear created when the pressure wave moves tissues of
different densities at different speeds 105,106.
1.4.3 Chest trauma
The organs most affected by blast injuries are the hollow, gas-filled organs such as the ears,
the lungs, the gastro-intestinal tract 103,104,107-110, and to a lesser extent the cardiovascular and
central nervous system 111. The lungs are almost always affected by blast injuries 103,107-109.
Postulated explanations are: 1. The positive pressure is transmitted through the airways into
the lung, causing rupture of the alveoli and the capillaries, 2. the longer lasting negative phase
produces the alveolar capillary disruption, and 3. direct compression of the lung.
1.4.3.1 Pacemaker function of thorax trauma
Thoracic trauma seems to be an important trigger of morbidity and mortality in polytraumatic
patients and may lead itself to severe lung injury 93. Indeed, the lethality of polytrauma patients
without thorax involvement is 4%, as compared to 23% with simultaneous thorax trauma 112.
Therefore, thorax injury is a major negative determinant for the long-term consequences after
trauma 104,113. One of the major problems for clinical evaluation of the early phase after trauma
is the missing of clinical signs of pulmonary dysfunction 114,115. This means that the severity of
the consecutive injury is unpredictable at this stage.
Introduction
13
1.4.3.2 Pathology of pulmonary blast injury
Pulmonary contusion and haemorrhage
Experimental lung injury from air blast 116,117 showed that the most consistent lesion was
bilateral traumatic haemorrhage, variable in extent and distribution. Furthermore, oedema is
usually prominent 116-118. Post-mortem data of fatal blast injury in humans is rare.
Ultrastructural examination of lungs 24 hours after blast exposure, reveals haemorrhagic
areas in the lung contralateral to the side of blast exposure which initially microscopically
appeared only slightly congested 118. Loss of structure of the alveolar epithelium and changes
to the type II pneumocytes 118 and thus loss of surfactant production may be important in the
development of respiratory insufficiency.
Haemopneumothorax and air embolism
Tension pneumothorax has been observed in rats exposed to air blast under laboratory
conditions 116. Air embolism, pulmonary contusion and haemorrhage account for the majority
of immediate and early death 104,110,119,120. Whether air emboli are important in survivors is
unclear, but early and persisting neurological deficits might be the result of this phenomenon 103. Whether air-embolism is caused by mechanical ventilation is still a matter of debate 121.
However, recently it has been shown that air embolism, present in blast victims, is not a mere
ventilation-induced artefact 119.
1.4.3.3 Acute physiologic responses to primary blast
The reported physiologic responses in blast-injured patients vary considerably, largely as a
result of varying observation times and the influence of other injuries. The most consistent
physiological data is derived from animal experiments from which common cardiorespiratory
and haemodynamic changes can be determined.
Pulmonary response
Moderate to severe blast exposure in animals is usually followed by an immediate, variable
period of apnoea, lasting from a few seconds to up to more than one minute 122. This apneic
period is followed by a fast and shallow breathing for a variable time before returning to pre-
blast values 122. Blast-induced effects on gas-exchange and ventilatory function are variable
throughout different animal experiments. The reduction of arterial blood oxygen tension
(PaO2) that returns gradually to control levels, causes transient hypoxemia of varying degree
Introduction
14
of severity. Carbon dioxide tension (PaCO2) however is not affected and has been related to a
ventilation-perfusion mismatch, due to a massive pulmonary haemorrhage 116.
Cardiovascular response
The most consistent finding of experimental blast injury on the heart rate appears to be an
immediate bradycardia, which is more severe with higher intensity blast waves 116. Bomb blast
survivors are occasionally found in profound shock and hypoxia without external signs of injury 115. An immediate fall in the mean arterial pressure (MAP) to less than 50% has been shown in
various animal species following blast exposure 116. This response to blast wave injury is
sometimes bimodal 116,117 and graded with higher intensity blasts, resulting in lower MAP and
slower recovery. Recovery time to pre-blast values ranges from two hours 122 to up to several
days 123. Concomitant with the reduction in MAP, a fall in the cardiac index (CI) can be
observed. The CI response to injury, like MAP, is lower with exposure to higher intensity blast
pressure waves. Despite hypotension and low CI, no compensatory peripheral
vasoconstriction is detectable 116. This triad of apnoea, bradycardia, and hypotension 116,122 is
only seen in animals in which just the thorax is exposed to the blast, but not in animals
undergoing abdominal blast exposure 122. These changes are attributed to air embolism and
direct cardiac injury 120 and probably mediated by vagal reflexes 124,125. Experimental animal
studies 126 and clinical observations 127 following blunt chest trauma reveal a variety of EKG
disturbances, from ventricular extracystoles to ventricular fibrillation, that are usually
temporary but might account for some fatalities following blast injury and may exacerbate the
triad of apnoea, bradycardia, and hypotension.
Progressive pulmonary insufficiency (PPI)
Several different mechanisms, in addition to the pressure wave-induced disruption of the lung
architecture, are considered to be responsible for the various presentations of blast-induced
pulmonary insufficiency (“blast lung”) and delayed respiratory insufficiency. Respiratory failure
occurring 24 - 48 hours after blast exposure is unlikely to be caused solely by the primary
blast 103,128. The pulmonary results of injury, namely the combination of blast effects, inhalation
injury, tissue injury, and fluid resuscitation are frequently diagnosed as the Adult Respiratory
Distress Syndrome (ARDS) 41,94. The late mortality after trauma is related to multi-organ failure
(MOF), as a consequence of shock or sepsis 97. The pathophysiology of injury-induced organ
MOF is poorly characterized, but has been linked to systemic inflammation, as a result of
infection (either obvious or occult) or massive tissue injury (systemic inflammatory response
syndrome, SIRS). Post-traumatic immunosuppression, called the counterregulatory anti-
Introduction
15
inflammatory response syndrome (CARS), also contribute to the development of MOF
(reviewed by Cobb and coworkers, 129), 95,130.
1.4.4 Molecular injury
Recent information indicates that there is a complex cellular and molecular generic response
to injury, leading to multi-organ failure.
First of all, there is the direct tissue injury leading to interstitial or alveolar haemorrhage and
oedema formation. The intensity of pulmonary oedema was positively correlated with the
length of the survival time 119. As a result, hypoxemia and pulmonary air embolism may occur 120. Such events can also cause oxidative stress in the lung, which is characterized by an
antioxidant depletion (water soluble and lipid soluble), an increase in lipid peroxidation, an
increased methaemoglobin (metHb) content 131, and an inhibition of ATP-dependent Ca2+
transport 132. Supplementation with vitamin E and lipoic acid, but not vitamin C, increases the
Hb oxygenation 133, however the pro-oxidant action of water soluble antioxidants via redox
cycling of oxyHb and metHb may promote oxidative stress rather then prevent it 102,131.
Due to tissue trauma itself, as well as due to blood components and cell debris, an activation
of host defence mechanisms occurs, including soluble plasma factors (complement and
clotting cascades) and immunocompetent cellular components (neutrophils, monocytes,
macrophages, and endothelial cells). Such activated cells in turn produce potentially toxic host
mediators, such as tumor necrosis factor (TNF) and interleukin-1 (IL-1), as well as chemical
species such as kinins, eicosanoids, platelet-activating factor (PAF), and nitric oxide. This
sequential increase of the inflammatory response may variably lead to shock, multiple organ
failure and death. Eicosanoids have been shown to play an important role in the pathogenesis
and modulation of pulmonary oedema associated with blast injury. Significantly elevated
plasma levels of the prostanoids, thromboxane A2 (TXA2), prostacycline (PGF1a), PGF2a and
PGE2 are reported for polytrauma patients with thorax involvement 134,135 and after surgery
induced lung tissue injury 136, implying a relative prognostic value of these early mediators with
regard to the intensity and the pattern of the injury. Concomitantly elevated plasma levels of
type II a phospholipase A2 (PLA2) are suggested to bear some prognostic value 137,138.
Unchanged levels of prostaglandin M (PGM) indicate an unaltered pulmonary metabolic
capacity 136. Pharmacological inhibition of 5-lipoxygenase, immediately prior to blast exposure,
reduces oedema formation, accumulation of neutrophils and generation of lipid peroxidation
products in injured rabbit lungs 139 and permits respiratory compensation of metabolic acidosis
in the general circulation, in spite of increased hypotension and acidosis in the venous
circulation 140. Neither experimental haemorrhage alone, nor haemorrhage in combination with
blunt trauma increases circulating TNF in pigs, implying no involvement in the vasomotor
Introduction
16
collapse observed in this setting 141. Unlike TNF and IL-1, increased IL-6 levels are commonly
detected during disease 135,142, thus IL-6 serum concentrations received more attention as a
prognostic indicator for both severity and outcome.
1.4.5 Management of pulmonary blast injury
Success or failure of the treatment may depend on the judicious use of resuscitative fluids and
respiratory support 128. In trauma victims, increased interstitial and intra-alveolar oedema
impairs gas exchange. The initial ventilator settings in the trauma victim are somewhat
different from those used in other patients, because the decreased functional residual
capacity, due to oedema formation requires a lower tidal volume. Thus, modern ventilator
strategies include a low tidal volume with a positive end-expiratory pressure (PEEP) and high
inspired oxygen concentrations, in order to recruit alveoli and thus avoid atelectasis. However,
the beneficial effects of supplementary oxygen and mechanical ventilation remain
controversial and depend on the extent of the respiratory insufficiency 143. Concomitant
respiratory acidosis is thereby compensated by therapeutic bicarbonate application. Together
with pharmacological manipulations that increase the cardiac output, the function of both the
heart and the lung, as well as other organs, can be augmented. The outcome of
pharmacological interventions manipulating the reflex mechanisms and therefore altering
haemodynamic functions remains unclear 128.
Various attempts have been done to interrupt the interaction of the neutrophils, endothelial
cells, cytokines, and free radicals 133,144. Despite limited clinical and experimental success, this
approach may prove to be worthwhile in the future for treating the severely injured patient 145.
1.4.6 Immunomodulation after trauma
Besides clinical characterization, recent research data indicate that the prognosis of trauma
patients is strongly associated with a post-traumatic imbalance of the immunological system 146. For the outcome of patients with multiple injuries, it seems very important to gain an
inflammatory mediator homeostasis as fast as possible. Overwhelming immune activation,
however, can result in a systemic inflammatory response syndrome (SIRS) and septic shock.
To control the potentially harmful pro-inflammatory response, the immune system, as a
mechanism of counterregulation, releases anti-inflammatory mediators inducing the so-called
anti-inflammatory response syndrome (CARS). In addition to the autoregulatory pathways of
the immune cells, the systemic immune response is controlled by two neuroimmune
pathways: 1. the hypothalamic-pituitary-adrenal (HPA) axis and 2. the sympathic nerve system
leading to glucocorticoid and catecholamine release, respectively, that affect primarily
Introduction
17
monocytes and macrophages 130. However, if the anti-inflammatory mediators predominate,
immunosuppression (“immunoparalysis”) with ineffective eradication of microorganisms and
septic complications may follow 147. In this context, the early presence of soluble TNF
receptors (sTNFRs) 142 and interleukin 1 receptor antagonist (IL-1ra) in the circulation of
trauma patients has been reported, even with a strong correlation to mortality 148,149. Traumatic
injuries cause the liberation of various mediators such as IL-6, IL-10, and PMN elastase, with
more or less an association between anatomic injury and the pattern of mediator release 135,142. For IL-6, an anti-inflammatory role in controlling the levels of other pro-inflammatory
cytokines 150 and by inducing the release/ formation of sTNFRs has been suggested 151. In
addition, PMN elastase is thought to increase the sTNFR release by proteolytic mechanisms 152. Since PGE2 is significantly elevated in the plasma of injured patients and since the
immune cells (primarily the macrophages) from traumatized and burn patients hypersecrete
PGE2 upon stimulation 153, this potent immunosuppressive agent is regarded to be a pivotal
mediator in the post-trauma immune dyshomeostasis 154. Not only increased synthesis of
PGE2, but also decreased removal and degradation have been reported in burn injury and
trauma (reviewed in 89). Furthermore, it has been shown that trauma results in delayed
macrophage hypersecretion of inflammatory mediators, such as TNF, IL-6 and end products
of the respiratory burst, such as H2O2, that is associated with persistent functional
macrophage defects in antigen presentation 155. The paradoxical combination of suppressed
macrophage function and hypersecretion of inflammatory mediators, simultaneously renders
the host susceptible to both infectious complications and the immune-mediated sequelae of
SIRS and MOF. However, despite immunosuppression immediately after injury, a recovery
from an early impairment occurring 3 to 6 days after trauma is also reported 156.
Aims of the Study
18
2. Aims of the Study
The blast trauma model is based on a rodent model originally developed by Irwin et al. 1998, 117.
The objective of this study was to use and to improve this model, in order to reproduce the
clinical spectrum of injuries seen in blast victims, for studying the pathophysiology and
potential treatment approaches of thorax trauma in rats.
The first aim was to standardize the blast pressure wave and its application, with regard to
assessing characteristical physical blast properties, in order to study its biological correlate.
The second aim was to asses and to characterize the physiological and functional changes
after in vivo trauma by means of:
I. Assessing lung physiological parameters over time in order to characterize trauma-
induced changes, by combining our primary blast injury model with our ex vivo
isolated perfused rat lung model. These studies include the investigation of
pharmacological interventions, as to their therapeutic potential.
II. Assessing pro-and anti-inflammatory mediator release, oedema generation and
resorption, as well as pulmonary infiltrate formation in vivo over time.
The third aim represented the study aspects of local and general immunodeficiency after
thoracic trauma, that might clinically result in a higher number of infections. Due to their key
role as modulator of pulmonary inflammation, macrophage functions will be assessed in vitro,
as to their phagocytic capacity, respiratory burst and mediator release.
Materials and Methods
19
3. Materials and Methods
3.1 Animals
Female Wistar rats (230 ± 20 g) obtained from Harlan Winkelman GmbH (Borchen, Germany)
and kept under controlled conditions (24°C, 55% humidity, 12 hours day/ night rhythm) on a
standard laboratory chow and water ad libitum were used as lung donors for experiments with
isolated perfused rat lungs, for the isolation of primary alveolar macrophages and for the in
vivo experiments.
3.2 Chemicals
3.2.1 Chemicals used in the isolated perfused rat lung experiments
Substance Producer Solute in Concentration Storage
Amiloride Sigma-Aldrich, Deisenhofen, Germany
DMSO *, NaCl 10-4 M freshly prepared
Bovine serum albumin fraction V, receptor-grade; Lot No. 12353
Serva, Heidelberg, Germany
buffer 2% freshly prepared
Formoterol AstraZeneca, Zug, Switzerland
saline, 0.05% Na2S2O5
1 nM freshly prepared
Propranolol Sigma-Aldrich, Deisenhofen, Germany
saline 10-4 M freshly prepared
Terbutaline Sigma-Aldrich, Deisenhofen, Germany
NaCl 10-4 M stock at -20°C
Table 3.1 Substances used in the isolated perfused rat lung experiments. * 0.03% DMSO.
Materials and Methods
20
3.2.2 Chemicals used in the in vitro experiments
Substance Producer Solute in Concentration Storage
Escherichia coli (K-12 strain) tetramethylrhodamine conjugate
Molecular Probes, Eugene, OR, USA
PBS 250 µg/ ml 20 mg/ ml stock at 4°C
Liquemin Hoffmann-La Roche, Grenzach-Wyhlen, Germany
NaCl (1:10) 8 Units/ ml Heparin
4°C
LPS from Salmonella abortus equi
Metalon, Wusterhausen, Germany
PBS 100 µg/ ml – 10 ng/ ml
1 mg/ ml stock 4°C
LTA from Staphylococcus aureus
LS Wendel, University of Konstanz, Germany
PBS 100 µg/ ml – 2 µg/ ml
5 mg/ ml stock -70°C
SOD (superoxide dismutase)
Sigma-Aldrich, Deisenhofen, Germany
HBSS * 1000 U/ ml freshly prepared
Staphylococcus aureus (wood strain without protein A), tetramethylrhodamine conjugate
Molecular Probes, Eugene, OR, USA
PBS 250 µg/ ml 10 mg/ ml stock at 4°C
WST-1 (C19H11IN5NaO8S2, tetrazolium salt)
Probior, München, Germany
HBSS * 500 µM freshly prepared
Table 3.2 Substances used in vitro. * Hanks balanced salt solution.
3.2.3 Other chemicals
Brij, Tween 20, 0.4%Trypan blue, 3,3´,5,5´-tetramethyl-benzidine liquid substrate solution,
LPS from Salmonella abortus equi, sodium dodecylsulfate (Sigma-Aldrich Chemie GmbH, Deisenhofen, Germany); HEPES (ICN Biomedicals, Ohio, USA); OptEIATM, biotin labelled
polyclonal anti mouse/ rat TNFα (Pharmingen, Hamburg, Germany); Hoechst 33342, Sytox
green (Molecular Probes Europe BV, Leiden, Netherlands); rabbit anti-TNFα- serum, K533
(LS Wendel, Biochemical Pharmacology, University of Konstanz, Germany); Streptavidin-
peroxidase (Jackson Immuno Research, West Grove, PA, USA); MMP-2, matrix
metalloproteinase 2, human rheumatoid synovial fibroblast, MMP-9, matrix metalloproteinase
9, human neutrophil granulocyte, Eosine-methylene blue, Azur-eosine-methylene blue (Merck
KGaA, Darmstadt, Germany); Coomassi brilliant blue R250 (Serva, Heidelberg, Germany);
Materials and Methods
21
Temed (Biorad, München, Germany); APS (Amersham, Little Chalfont, UK); Pierce BCA
protein assay reagent (Bender & Hobein GmbH, Heidelberg, Germany); ELISA/ EIA: IL-6, IL-
10 (Biosource Europe SA, Nivelles, Belgium); TXB2, 6-keto-PGF1α (BioTrend GmbH, Köln,
Germany); CINC-3, mouse sTNFR1, sTNFR2 (R&D Systems, Wiesbaden-Nordenstadt,
Germany). All standard chemicals were purchased from established companies, primarily
Sigma-Aldrich Chemie GmbH (Deisenhofen, Germany).
3.2.4 Solutes
Distilled water; Dimethylsulfoxid, DMSO (Riedel de-Haen, Seelze, Germany); Ethanol; NaCl
0.9% (Delta-Pharma Boehringer-Ingelheim, Germany); Phosphate-buffered saline solution,
PBS (PAA, Germany); Triton X-100 (Sigma-Aldrich Chemie GmbH, Deisenhofen, Germany);
EDTA, ethylendiamine tetraacetic acid (Sigma-Aldrich Chemie GmbH, Deisenhofen,
Germany).
3.2.5 Anaesthesia and analgesic
• Halothane, 2-bromo-2-chloro-1, 1, 1-trifluoroethane (Sigma-Aldrich Chemie GmbH,
Deisenhofen, Germany)
• Pentobarbital sodium (Narcoren), (Wirtschaftsgenossenschaft deutscher Tierärzte,
Hannover, Germany)
• Buprenorphin (Temgesic), (Tierforschungsanlage, Universität Konstanz, Germany)
3.2.6 Cell culture material
RPMI 1640: with L-Glutamine, with/ without phenol red (PAA, Pasching, Austria); Hanks
balanced salt solution (PAA, Pasching, Austria); Penicillin-Streptomycin (Gibco BRL Life
Technologies, Eggenstein, Germany); Fetal calf serum (FCS) (Boehringer Mannheim GmbH,
Mannheim, Germany); Cell culture plates (Greiner, Frickenhausen, Germany)
3.3 Laboratory equipment and technical devices
Centrifuges: Eppendorf 5417R (Netheler & Hinz, Hamburg, Germany); Minifuge RF (Heraeus
Instruments, Hanau, Germany); ELISA reader: SLT Spektra Rainbow Photometer (SLT
Labinstruments, Grailsheim, Germany); Microplate Fluorescence Reader FL 600 (Deelux
Labortechnik, Gödenstorf, Germany); Isolated perfused rat lung (Harvard Apparatus, March-
Hugstetten, Germany); Osmometer 3MO (Advanced Instruments, Needham Heights, MA,
Materials and Methods
22
USA); Eppendorf ACP 5040 (Netheler & Hinz, Hamburg, Germany); Microscope: Zeiss
Axiovert 35 (Zeiss, Oberkochen, Germany)
3.4 The in vivo blast wave thorax trauma in rats
3.4.1 The blast wave generator apparatus
The blast wave generator was originally designed and constructed by Irwin and colleagues in
1998 117 and optimized by Liener and coworkers to discharge a global blast pressure wave in
a safe laboratory environment. We have modified this setting to our specific needs in order to
improve the pressure wave monitoring and the reproducibility of pressure wave exposure. The
blast wave generator (Wissenschaftliche Werkstätten, Universität Konstanz) consists of three
parts: a pressure reservoir, a blast nozzle, and a 190 A µm Mylar polyester film (Strohmeier,
Rheda-Wiedenbrück, Germany) that separates the two compartments. Compressed air from
the storage tank was slowly delivered by a pressure reducer to fill up a 0.75 l compressed air
bottle, that is located close to the pressure reservoir of the generator. When a working
pressure of 18 bar was reached the air supply was stopped. The valve (opening time: ≈ 25
ms) (HEE-D-MINI-24, Festo AG & CO, Esslingen, Germany) between the compressed air
bottle and the pressure reservoir was triggered by the computer. Opening of the valve resulted
in a fast pressure build-up in the reservoir. As soon as the burst strength of the Mylar
diaphragm was reached, a blast pressure wave was discharged towards the rat by the nozzle.
Figure 3.1 shows the blast wave generator.
Figure 3.1: Schematic diagram of the blast wave generator (front view). Dimension is in millimetre (mm).
Materials and Methods
23
3.4.2 Pressure wave monitoring
Different sensors at varying positions offered an exact monitoring of the exposed blast
pressure wave (Erne B., Abteilung Elektronik, Wissenschaftliche Werkstätten, Universität
Konstanz):
1. A pressure transducer (PR-6ST-80400.XX-20, sensitivity: 39.7 mV/ bar, excitation: 4 mA,
natural frequency: < 30 KHz; Keller AG, Winterthur, Switzerland) in the pressure reservoir
determined the cracking pressure meaning the rupture of the polyester film. The measured
time course of the pressure wave curve indicated the velocity of the pressure increase
followed by the decay. The fast pressure build-up and pressure decline is a requirement for
explosively discharging of the pressure wave (Fig. 3.2).
2. Two pressure transducers (2 MI PAA 110-050-020, sensitivity: 8.03/ 7.99 mV/ bar,
excitation: 1 mA, natural frequency: > 400 KHz; Keller AG, Winterthur, Switzerland) on both
sides of the rat measure the pressure peaks on rat thorax level (Fig. 3.2).
3. Another transducer (Halleffekt-IC 634-SS2, sensitivity: 7.5 – 10.6 mV/ mT; RS Components
GmbH, Mörfelden-Walldorf, Germany) records the breathing frequency of the animal.
Therefore a string connected with the breathing sensor was placed above the thoracic cage.
Via this transducer the valve was triggered automatically depending on the breathing situation
(e.g. inspiration, expiration or resting expiratory position) (Fig. 3.2). In addition the breathing
frequency of the anaesthetized animals, before and after the pressure wave exposure was
recorded.
All the measured pressure wave signals by the sensors were transmitted through a high
accuracy measuring instrumentation amplifier Burr-Brown (Texas Instruments GmbH,
Freising, Germany) either direct to the computer (cracking pressure transducer) via an A/ D-
converter (MAX 186, Maxim Corporate Headquarters, Sunnyvale, CA, USA) or first (pressure
peak transducer) to the HAMEG oscilloscope HM 407 (HAMEG instruments, distributor
VELMA, Großkrotzenburg, Germany). Then pressure wave data were analysed by a special
developed software (Heine G., Abteilung Elektronik, Wissenschaftliche Werkstätten,
Universität Konstanz) for cracking pressure of the polyester film (Rp), wave form, pressure
peaks (Pp(r), Pp(l)), impulse or area under the curve (AUC(r), AUC(l)), duration (t(r), t(l)) and
pre-and post breathing frequency (Fpre, Fpost). For calculation of these parameters the
following equations were used:
Materials and Methods
24
pressure peaks (Pp(r), Pp(l)): 12
2
1
tt
UP
mi
mii
−=
∑=
= (U = voltage; t = time), whereas the voltage U is
proportional to the pressure P (cracking pressure transducer: 0.5 bar = 1 bar, pressure peak
transducer: 0.1 bar = 1 bar);
area under the curve (AUC(r), AUC(l)): ∑=
=
=2
1
ti
tiiUAUC ,
and pre-and post breathing frequency (Fpre, Fpost): breath/ min.
As an index for variations between different experiment the variation coefficient CV was
calculated using the equation: [ ] 100% ⋅=medianSDCV .
Figure 3.2: The blast wave generator including pressure transducers at different positions. A cracking pressure transducer in the pressure reservoir, two overpressure sensors on the left and right side of the rat and a transducer for recording the breathing frequency.
3.4.3 Protocol of anaesthesia and analgesic
The rats were anaesthetized in a bell jar flooded with a Halothane®/ O2 gas mixture through a
Halothane-evaporator (flow: 2 L/ min oxygen, 4% Halothane). By the time the breathing
frequency was slow enough the animals were weighed and placed on a special immobilized
Materials and Methods
25
pad (Wissenschaftliche Werkstätten, Universität Konstanz). The rats were positioned in a
supine position and the paws were fixed with tapes on the pad. Up to the pressure wave
exposure the animals were inhalation-anaesthetized through a anaesthesia mask (flow: 1.5 L/
min oxygen, 4% Halothane). In addition the animals received the analgesic Buprenorphin
(0.03 mg/ kg BW) (Temgesic, Tierforschungsanlage, Universität Konstanz) subcutan. After
the blast exposure the animals were provided with oxygen (flow: 4 - 5 L/ min) to get them out
from the anaesthesia. The rats were terminally anaesthetised by an intraperitoneal injection of
sodium pentobarbital (Narcoren®, 160 mg/ kg BW).
3.4.4 Experimental protocol
After positioning and fixing the rat in the supine position and starting the inhalation-
anaesthesia through the anaesthesia mask, the string connected with the breathing
transducer was placed above the thoracic cage detecting the breathing frequency. Triggered
by the breathing sensor the rats were subjected to the pressure wave at the top of expiration.
The blast pressure wave was centered on the xiphoid with the tip of the blast nozzle located
either 3.5, 5, 7 cm away from the sternum. The blast animals were provided with oxygen (flow:
4 - 5 L/ min) to get out from the anaesthesia afterwards and the reset of the breathing was
recorded for one minute via the breathing sensor. For studies immediately after blast exposure
the animals were directly, terminally anaesthetised by an intraperitoneal injection of sodium
pentobarbital (Narcoren®, 160 mg/ kg BW). In case of long-time studies the animals were
sacrificed at 1.5, 3, 6, 12, 24 and 96 hours following the blast respectively. If necessary these
animals got a second injection of the analgesic Buprenorphin (0.03 mg/ kg BW) (Temgesic,
Tierforschungsanlage, Universität Konstanz) subcutan. Control animals were subjected to the
same experimental protocol but did not receive a blast.
Subsequently either the bronchoalveolar lavage (BAL) was performed (3.7) to determine total
and differential BAL cell counts (cytospin) (3.9), total protein content (3.10), erythrocyte counts
(3.8) and the release of different mediators and enzymes (3.11 - 3.16) or the wet/ dry ratio
(3.17) of the lung was assessed.
Figure 3.3 shows the timescale of the in vivo experiments.
Materials and Methods
26
Figure 3.3: Timescale of the in vivo experiments.
3.4.5 Determination of an injury score and validation
3.4.5.1 Haemorrhage score
The different lung lobes were each examined macroscopically for areas of pleural and
subpleural bleeding using an injury score:
0 = no haemorrhage,
1 = < 30% haemorrhage,
2 = 30 – 60% haemorrhage,
3 = > 60% haemorrhage
the total score resulted from the summation of the scores of each lobe whereas the score of
the upper left lobe (≈ double size) was duplicated. The inter-observer agreement was 93%.
3.4.5.2 Oedema score
Analogous to the haemorrhage score an oedema score was defined depending on the amount
of macroscopically visible oedematous areas. The same score scale (3.4.5.1) was used. The
inter-observer agreement was also > 90%.
in vivo
in vivo• thorax trauma (3.5 cm distance)• sham controls
~ + 10 min ~ + 6 h~ + 3 h
lung wet/ dry ratio
~ + 1.5 h ~ + 12 h ~ + 24 h ~ + 96 h
• BAL: - mediator measurement- cytospin- protein content- erythrocyte counts - LDH- MMP-2, -9
histological examination
in vivo
in vivo• thorax trauma (3.5 cm distance)• sham controls
~ + 10 min ~ + 6 h~ + 3 h
lung wet/ dry ratio
~ + 1.5 h ~ + 12 h ~ + 24 h ~ + 96 h
• BAL: - mediator measurement- cytospin- protein content- erythrocyte counts - LDH- MMP-2, -9
histological examination
Materials and Methods
27
3.5 The isolated ex vivo perfused and ventilated rat lung
3.5.1 Isolated perfused rat lung preparation
The lungs were perfused and prepared essentially as described previously 1. Briefly, female
Wistar rats were anaesthetized by intraperitoneal injection of 160 mg/ kg pentobarbital sodium
(Narcoren®). The positive pressure ventilation was performed through a tracheal cannula.
After exsanguination, two catheters were placed in the pulmonary artery and the left atrium
and then the non-recirculating perfusion was started to remove the blood from the pulmonary
circulation. The heart-lung block was excised and put in the artificial thorax chamber (38°C). In
order to obtain a correct continuous assessment of the lung weight via the weight transducer
integrated into the chamber lid 157, it was checked that the lung is suspended without contact
between catheters and water-jacked glass chamber wall.
3.5.2 Experimental Setup
The apparatus and technical equipment was purchased from Hugo Sachs Electronics-
Harvard Apparatus GmbH, Germany. The Setup is almost the same as described previously 1.
Excised lungs are perfused at constant hydrostatic pressure (14 cm H2O) in a recirculating
fashion, with a total volume of about 100 ml. For perfusion a Krebs-Henseleit buffer (305 - 315
mosm, 37°C) containing 2% bovine serum albumin (BSA), 0.1% glucose and 0.3% HEPES
was used. The pH value of the perfusate before entering the lung was kept at 7.35 by
automatic bubbling of the buffer with carbon dioxide as soon as the pH exceeded this value.
The perfusate flow (NarcomaticTM RT 500, Narco Biosystems, Texas, USA), the arterial
pressure PA, the venous pressure PV (both Isotec™ transducer, Quest Medical, Dallas, USA)
and pH (WTW pMX 3000) were continuously monitored.
The suspended lungs were ventilated by the trachea with a rotary vane compressor pump
(ventilation control module VCM) with negative pressure and ambient air. Breathing frequency
was 80 breaths/ min. The pulmonary end-expiratory (PEEP), –inspiratory (PIP) pressures
were set to 2 and 7 cm H2O reaching a tidal volume between 1.8 – 2.2 ml in untreated control
lungs. To avoid the generation of atelectasis as well as to recruit collapsed lung areas an
hyperinflation of -16 cm H2O was triggered automatically every 5 minutes (timer counter
module, TCM). Pulmonary ventilation pressure was measured with a differential pressure
transducer (Validyne DP 45-24, Northridge, Ca, USA) and air flow velocity was measured with
a pneumotachograph connected to a differential pressure transducer (Validyne DP 45 - 14,
Northridge, Ca, USA).
Materials and Methods
28
All data were transmitted to a computer and analysed by a special software (Pulmodyn
software): pulmonary pressure (P), tidal volume (Tv), airway resistance (RA), dynamic lung
compliance (CL), perfusate flow (Q), pulmonary arterial pressure (PA), pulmonary vein
pressure (PV), vascular resistance (RV), perfusate temperature, perfusate pH and lung weight
(G). For calculation of lung mechanics the following equation was used:
LL
RTvC
P +⋅
= 1
⋅dtdTv ; t = time.
Vascular resistance RV was calculated from the equation: ( )QPP vA −
.
In order to obtain a minimal vital ventilation of 1ml in injured lungs, it was necessary to
increase the standard ventilation pressure, depending on the extent (3.4.4) of blast injury.
The Setup of the isolated perfused rat lung is shown in Figure 3.4.
Figure 3.4: The Setup of the isolated perfused rat lung. The isolated rat lung is perfused in a recirculating fashion, blood-free under constant pressure conditions and with a negative pressure ventilation.
3.5.3 Experimental design of the perfused lung studies
After the lungs were fixed in the artificial thorax chamber, the ventilation and perfusion
parameters were controlled and adjusted. If procurable the injured lungs were perfused over
150 minutes like the untreated control lungs. The experimental design of the ex vivo studies is
shown in Figure 3.5.
Materials and Methods
29
Figure 3.5: Experimental design of the ex vivo studies.
3.6 In vitro stimulation of primary rat alveolar macrophages
3.6.1 Preparation and culturing of rat alveolar macrophages
Anaesthetised rats were exposed to the blast pressure wave as already described previously
(3.4). The animals were sacrificed 10 minutes (min), 24 and 96 hours following this
experimental induced blunt chest trauma, non-traumatized animals served as sham controls.
The alveolar macrophages were harvested by bronchoalveolar lavage (BAL). Therefore lungs
were tracheotomized and five times rinsed with 10 ml cold NaCl: The latter three times while
softly massaging the thoracic cage to increase the amount of the isolated BAL cells. Recovery
of the NaCl was always > 75%. The lavage fluids were pooled and centrifuged (4°C) for 10
min at 270 x g, and the pellet was resuspended in 20 - 50 ml cold RPMI 1640 and centrifuged
for another 5 min (190 x g, 4°C). The pellet was again resuspended in RPMI 1640 with phenol
red, 10% heat-inactivated FCS and 1% penicillin/ streptomycin. BAL cells were cultured at an
initial density of 5 x 105/ ml (except 3.6.3/ 3.11) on 96-well plates in 200 µl/ well RPMI 1640
(phenol red, 10% FCS, 1% penicillin/ streptomycin) for two hours at 37°C. The non-adherent
in vivo ex vivo
end of perfusion
in vivo• thorax trauma (3.5, 5, 7 cm distance)• sham controls
rat lung preparation
~ - 15 min~ - 6 h ~ - 3 h
start of perfusion
0 min 4 min
infusion of:• terbutaline (10-4 M),• formoterol (1 nM),• amiloride (10-4 M),• propranolol (10-4 M)into the perfusate.
150 min
• lung wet/ dry ratio• BAL
~ - 10 min
in vivo ex vivo
end of perfusion
in vivo• thorax trauma (3.5, 5, 7 cm distance)• sham controls
rat lung preparation
~ - 15 min~ - 6 h ~ - 3 h
start of perfusion
0 min 4 min
infusion of:• terbutaline (10-4 M),• formoterol (1 nM),• amiloride (10-4 M),• propranolol (10-4 M)into the perfusate.
150 min
• lung wet/ dry ratio• BAL
~ - 10 min
Materials and Methods
30
BAL cells were removed by washing the cells three times with fresh medium. The remaining
adherent alveolar macrophages were cultured in 200 µl/ well RPMI 1640 (without phenol red,
10% FCS, 1% penicillin/ streptomycin) either non-stimulated, with endotoxin or whole, dead
bacteria (3.6.2, 3.6.3). Depending on the isolated BAL-cell counts all experiments were run at
least in duplicate.
3.6.2 Stimulation with dead, fluorescent bacteria
The experiments were started by incubating the alveolar macrophages with either
fluorescence labelled Staphylococcus aureus (S. aureus) or Escherichia coli (E. coli)
(Molecular Probes) in a final concentration of 250 µg/ ml. Both reagents were stored as
concentrated stocks at 4°C and diluted with medium after sonicating (2 min) immediately
before use. After three hours incubation at 37°C the cells and supernatant were either
harvested and analysed (3.11) or subjected to different assays as described below (3.6.4,
3.6.5).
3.6.3 Stimulation with endotoxin
The cells were cultured at an initial density of 106 cells/ ml (100 µl/ well) (3.11) or 5 x 105/ ml
(200 µl/ well) (3.6.5) in the presence of various concentrations of lipopolyssacharide (LPS)
from salmonella abortus equi (Metalon) (0, 10, 100 ng/ ml, 1, 10, 100 µg/ ml) or lipoteichoic
acid (LTA) from staphylococcus aureus (Konstanz) (0, 2, 10, 50, 100 µg/ ml). Both reagents
were stored as concentrated stocks at 4°C and –20°C respectively and diluted with medium
immediately before use. Restored endotoxin was sonified for 2 minutes before use. After three
(3.6.5) or four (3.11) hours incubation at 37°C the supernatant was either harvested and
analysed (3.11) or subjected to another assay as described below (3.6.5).
3.6.4 Fluorescence labelled E. coli/ S. aureus phagocytosis assay
This assay measures the ability of phagocytes to engulf fluorescence labelled E. coli/ S.
aureus particles. Prepared BAL cells were cultured in 96-well plates (5 x 105 cells/ ml, 200 µl/
well), allowed to adhere for 2 hours and stimulated with dead, labelled E. coli/ S. aureus (final
concentration: 250 µg/ ml) as described in 3.6.5. After 3 hours incubation the phagocytosis
was stopped by washing the cells three times with PBS (room temperature) to remove non-
phagocytosed bacteria. The remaining PBS was removed by quickly turning the plate and
gently pushing it on a lint-free paper towel. Then cells were lysed by addition of 100 µl/ well
PBS + 0.1% Triton X-100. Fluorescence was determined at 530 nm excitation and 590 nm
Materials and Methods
31
emission wavelengths using a fluorescence microplate reader. Cells without bacteria were
used to determine the background fluorescence. From every experiment a digital photograph
was taken (Nikon Coolpix 995 through a special ocular with a Zeiss Axiovert 50).
Viability assays like Trypan blue or Sytox/ Hoechst staining at different steps during the assay
procedure were used as an index for physiological culture conditions.
The used particle concentration of 250 µg/ ml as well as the incubation time of 3 hours is
based on previous experiments, were the concentration signal relation and kinetic of particle
phagocytosis was measured. Furthermore complete inhibition of ingestion at 0°C was a
criteria for a quantitative phagocytic assay 158.
3.6.5 Assay for superoxide production
The production of superoxide after stimulation with either endotoxin or whole, dead bacteria
was performed by assaying the superoxide sensitive reduction of the water soluble and cell
impermeable tetrazolium salt WST-1. The advantage of this system is the higher sensitivity
and lower background in comparison to the method using the reduction of ferrycytochrome C 159. Isolated BAL cells were seeded in 96-well plates as described in 3.6.1. After 2 hours
adhesion the non-adhered BAL cells were removed by washing. Then 200 µl of 500 µM WST-
1 in Hanks balanced saline solution (HBSS) were added to each well.
In the experiments with whole, dead bacteria (see 3.6.2) to half of the wells either 250 µg/ ml
E. coli or S. aureus were added respectively. If endotoxin was used for stimulation to half of
the wells 0.1 µg/ ml LPS or 100 µg/ ml LTA was added. Therefore, three different groups (non-
stimulated, stimulated with endotoxin or bacteria) can be defined. To one well of each of these
groups 1000 U/ ml superoxide dismutase (SOD) was added. Then the plates were incubated
at 37°C for 3 hours.
After 3 hours, the extinction of the single wells was read by a plate reader at a wavelength of
λ = 450 nm. The concentration of superoxide and the rate of its production was calculated
considering the following facts:
The number of moles n is defined by the product of volume V of the sample ( 610100 ⋅=V l)
and its molar concentration C: CVn ⋅=
According to Lambert/ Beer, the molecular concentration C is calculated by dividing E∆
(change in WST-1 extinction caused by its reduction by superoxide) through the product of
WST-1`s molar extinction coefficient ε (37000 M-1 cm-1) and the diameter d of the sample (d =
0.3cm): dEVn⋅
∆⋅=ε
Materials and Methods
32
The difference in extinction E∆ was calculated for each group by forming the difference
between extinction En of each single well of a group and the average extinction SODE for the
appropriate wells containing SOD: SODn EEE −=∆
Since superoxide – in contrast to cytochrome C – is reduced by two electrons, 2 moles of
superoxide are needed to reduce 1 mol of WST-1, the formula has to be multiplied by the
factor 2, resulting in the final equation: dEVn⋅
∆⋅⋅=ε
2
The rate of production of superoxide R is the quotient of the number of molecules produced
during a certain time t, which was 180 minutes in these experiments:
⋅⋅⋅⋅∆==td
VEtnR
ε2
After inserting the known constants, the average rate for one group can be expressed as:
∑ ⋅∆⋅= 2.2001 En
R [pmol superoxide/ minute].
3.6.6 Preparation of washed and haemolysed erythrocytes and haemolysat
Peripheral venous blood was drawn from rats. To prevent coagulation Liquemin in NaCl (1 :
10) was added. The blood was diluted 10-fold in ice-cold NaCl and centrifuged for 5 minutes
at 270 x g and 4°C. The supernatant was carefully removed and the washing procedure was
repeated twice. Then a 10-fold volume of RPMI 1640 (without phenol red) was added and the
erythrocyte cell count was determined using the Neubauer counting chamber. After another 5
minutes centrifugation step at 270 x g and 4°C, cell pellet was diluted in RPMI 1640 (without
phenol red) to a final concentration of 8 x 109 erythrocytes/ ml corresponding approximately to
whole blood erythrocyte counts. The experiments were performed with 1.25 % washed
erythrocytes. To determine the impureness with leukocytes the leukocyte counts were
assessed (3.9). To get haemolysed erythrocytes the washed erythrocytes were frozen in liquid
nitrogen and then thawed at RT. This procedure was repeated three times. The haemolysat
was obtained after centrifugation for 10 minutes at 10600 x g and 4°C.
3.6.7 Lysis of erythrocytes
BAL fluid was centrifuged for 10 minutes at 270 x g and 4°C and the pellet was resuspended
in medium (1:20) containing 0.17 M ammonium chloride to lyse the erythrocytes and
incubated for 5 minutes at RT. To stop the lysis a five-fold excess of fresh medium was added,
pellet was resuspended and centrifuged again for 5 minutes at 190 x g and 4°C.
Materials and Methods
33
3.6.8 Experimental design of the in vitro experiments
Anaesthetised rats were exposed to blast wave thorax trauma (3.5 cm distance from the
nozzle). Animals were sacrificed 10 min, 24 and 96 hours after trauma, non-traumatized
animals served as sham controls (3.4.4). The alveolar macrophages were harvested by BAL
(3.6.1) and cultured either non-stimulated, with endotoxin (LPS or LTA) (3.6.3) or whole, dead
bacteria (E. coli or S. aureus) (3.6.2) for four and three hours, respectively.
Supernatants were either harvested for TNF measurement (3.11) or subjected to a
phagocytosis (3.6.4) and superoxide (3.6.5) production assay respectively.
In some experiments either whole blood, plasma, washed erythrocytes, haemolysed
erythrocytes or haemolysat (3.6.6) was added together with the bacterial stimulus.
In addition total and differential BAL cell counts (3.9) were determined.
Figure 3.6 summarizes schematic the experimental design of the in vitro experiments.
Figure 3.3: Timescale of the in vitro experiments.
3.7 Lung lavage
Lungs were tracheotomized and gently rinsed with 6 ml ice-cold NaCl. Recovery of the buffer
was always > 50%. The BAL fluids were centrifuged at 340 x g for 8 min and the supernatants
were stored at -70°C.
• phagocytosis assay• superoxide production• TNF release
in vitroin vivo
in vivothorax trauma/ sham controls
isolation/ culturingof thealveolar macrophages, 4°C
~ + 10 min, ~ + 24 h, ~ + 96 h
2 h adhesion, 37°C
in vitro stimulation:• dead, fluorescent E. coli/ S. aureus• LPS/ LTA
3 h or 4 h stimulation, 37°C
3 x washing
in case of oxidative burst measurement:• WST-1(500 µM) • SOD (1000 U/ ml)
cytospin
viability control
viability control
0 min
• phagocytosis assay• superoxide production• TNF release
in vitroin vivo
in vivothorax trauma/ sham controls
isolation/ culturingof thealveolar macrophages, 4°C
~ + 10 min, ~ + 24 h, ~ + 96 h
2 h adhesion, 37°C
in vitro stimulation:• dead, fluorescent E. coli/ S. aureus• LPS/ LTA
3 h or 4 h stimulation, 37°C
3 x washing
in case of oxidative burst measurement:• WST-1(500 µM) • SOD (1000 U/ ml)
cytospin
viability control
viability control
0 min
Materials and Methods
34
3.8 Determination of the alveolar haemorrhage
Pulmonary haemorrhage was quantified using the total erythrocyte count in the BAL fluid. The
erythrocyte number was assayed in a Neubauer counting chamber.
3.9 Total and differential cell counts and cell viability
To determine the total BAL cell count, the BAL fluid was mixed with Trypan blue solution (1:2)
and incubated for 1 minute at RT. Cell number was assayed using a Neubauer counting
chamber. Cells that excluded the Trypan dye were regarded as viable, blue cells as being
dead.
Cytospin preparations were used to determine the BAL cell differential. Depending on the total
cell counts the BAL samples were first diluted (2 – 4 folds) in isolation medium before pipetting
200 µl in the cytospin inserts. The samples were centrifuged at 90 x g (Minifuge RF (Heraeus
Instruments, Hanau, Germany) for 7 min at RT. The cells were fixed and stained with May-
Grünwald/ Giemsa solution (Merck KGaA, Darmstadt, Germany). From every experiment two
cytospins were made and a digital photograph was taken (Nikon Coolpix 995 through a
special ocular with a Zeiss Axiovert 50). The numbers of alveolar macrophages, lymphocytes
and infiltrated PMN were assessed by using standard morphological criteria for differentiation.
Total blood leucocytes were determined in the Neubauer counting chamber mixing heparin
blood (Liquemin in NaCl, 1:10) with Türk solution (1:10). For the differential blood count 10 -
15 µl whole blood were dispensed on a microscope slide, dried and stained with May-
Grünwald/ Giemsa solution.
3.10 Determination of total protein content
The BAL supernatants were stored at -70°C. The standard 2 mg/ ml BSA was diluted (2000,
1000, 500, 250, 125, 62.5, 31.25, 0 µg/ ml). 10 µl sample and standard were added on a
microtiter plate respectively. 190 µl/ well Pierce BCA protein assay reagent was added and
incubated for 30 min at 37°C. The extinction was measured at 550 nm in an ELISA reader.
Protein content was calculated using the BSA standard curve.
3.11 Cytokines determinations
For TNF measurements, BAL samples or cell culture supernatants were stored at –70°C and
quantified by sandwich ELISA. Antibody pairs (polyclonal rabbit anti-rat/ mouse Ab) and
recombinant TNF used as standard were purchased from Pharmingen (San Diego, CA, USA).
Materials and Methods
35
ELISA plates were coated over night at 4°C with 50 µl/ well with coat Ab (0.5% rabbit anti-TNF
serum) diluted in coating buffer (1:200). After blocking with 200 µl/ well PBS/ 3% BSA, pH 7.0
for 2 hours at room temperature (RT), the plates were washed twice with PBS/ 0.05% Tween
20. Samples and standard (50 µl/ well) were added and incubated for 3 hours at RT. After four
wash cycles, 100 µl/ well 0.5 mg/ ml tracer antibody in PBS/ 3% BSA were added and
incubated for 45 minutes. After another six wash cycles, plates were incubated for 30 minutes
with 100 µl/ well 50 ng/ ml streptavidin-peroxidase (Jackson Immuno Research, West Grove,
PA, USA) in PBS/ 3% BSA. Following eight wash cycles, 100 µl/ well TMB liquid substrate
solution (Sigma, Deisenhofen, Germany) was added and incubated at RT for 5 – 15 minutes.
After addition of 50 µl/ well stop solution (1 M H2SO4), absorption was measured at 450 nm
using a reference wavelength of 690 nm in an ELISA reader. The detection limit of the assay
was 10 pg/ ml.
IL-10 and IL-6 were determined using a commercially available ELISA kit (Biosource Europe
SA, Nivelles, Belgium). The detection limits of the assays were 15.6 pg/ ml for IL-10 and 31
pg/ ml for IL-6. Assay and analysis were performed according to the instructions of the
supplier.
3.12 Measurement of eicosanoids
BAL samples were stored at –70°C. Thromboxane A2 (t1/2 = 30 sec) was assessed as the
stable by-product thromboxane B2 (TXB2). Both TXB2 and and prostacycline (6-keto-PGF1α)
were determined by EIA (BioTrend GmbH, Köln, Germany) according to the manufacturer`s
instructions. The detection limits of the assays were 13.7 pg/ ml TXB2 and 3.2 pg/ ml for 6-
keto-PGF1α. The cross reactivity of the detecting antibody was TXB2 100%, 2,3-dinor TXB2
7.1%, prostaglandins < 0.01% and 6-keto-PGF1α 100%, 2,3-dinor 6-keto-PGF1α 3.17 %,
PGF2α 1.67%, prostaglandins 0.2-0.6% respectively.
3.13 Determination of NO production
The NO release into the alveolar space was determined indirectly by measuring the nitrate
level in the BAL fluid. Therefore 350 µl BAL fluid was filtrated by centrifugation in a microcon
concentrater (cut off 10 KD) at 470 x g and 4°C until a filtrate volume of approximately 300 µl
was reached. The nitrate reduction was performed in Eppendorf cups by mixing 300 µl BAL
filtrate with Nitrate reductase (0.1 U/ ml), FAD (5 µM), and NADPH (30 µM), incubating at
37°C for 15 minutes. For the NADPH oxidation, LDH (0.1 KU/ ml) and Na-pyruvat (0.3 mM)
were added and incubated at 37°C for 10 minutes. For di-azzo cuppling reaction, one part
sulfanilamide (1 mM) was mixed with one part HCL (6 N) and incubated for 15 minutes at 4°C.
Materials and Methods
36
A standard curve with different concentrations of NaNO3 (0 to 10 µM) was performed to
calculate the concentration of nitrate in the BAL fluid. After adding of N-naphtylethyldiamine
(NEDA) (0.8 mM) the absorption was measured at 560 nm to the reference at 690 nm.
3.14 Measurement of lactate dehydrogenase
Lactate dehydrogenase (LDH) was measured in BAL fluids according to Bergmeyer 160.
Measurement of LDH activity was performed in an Eppendorf ACP 5040 Analyser (Netheler &
Hinz, Hamburg, Germany). The reduction of nicotinamid adenine dinucleotide (NAD) to NADH
was measured at 340 nm.
3.15 Measurement of CINC-3
Samples taken from bronchoalveolar lavages were stored at -20°C. Rat CINC-3 was
assessed with a Duo Set ELISA Kit (Cat. No. DY525) and performed according to the
manufacturers instructions (R&D Systems Europe).
3.16 Gelatin zymograpy
To detect the gelatinolytic activity of matrix metalloproteinase-2 and –9 in BAL fluids, the
samples were evaluated by gelatin zymography 161. 300 µl BAL fluid were concentrated by
centrifuge in a microcon concentrater (cut off 10 KD) at 470 x g and 4°C until a volume of
approximately 50 µl was reached. The supernatant were treated under non-reducing
conditions and subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-
PAGE) in 10% acrylamide gels containing 1.2% gelatin (300 Bloom, pig) at a constant current
of 120 V at RT. After electrophoresis, the gels were washed three times for 15 minutes with
TNCA buffer (40 mM Tris-HCL (pH 7.6), 10 mM CaCl2, 2 µM ZnCl2, and 0.1% Brij) including
3% Triton X-100 and then once for 5 minutes with TNCA buffer without Triton X-100 to remove
all trace of SDS. The gels were then incubated over night at 37°C in the TCNA buffer (without
Triton X-100). Following incubation, the gels were fixed in a solution of 10% acetic acid and 40
% methanol and stained with 0.2% Coomassie brilliant blue R250 for 15 minutes. The gels
were decolorized in a solution of 5% acetic acid, 25% methanol and 70% water. Gelatin
digestion was identified as a clear lytic zone against a blue background. The gels were
scanned and converted to digital images by scanner.
As markers we used the purified pro-matrix metalloproteinase-2 (1 ng MMP-2, isolated from
human rheumatoid synovial fibroblasts) and pro-matrix metalloproteinase-9 (0.1 ng MMP-9,
isolated from human neutrophil granulocytes) (Merck KGaA, Darmstadt, Germany).
Materials and Methods
37
3.17 Lung Wet/ Dry-Ratio
After the animal was sacrificed and exsanguinated the lungs were excised “en bloc”, cleaned
of extraneous tissue and blood. The different lung lobes were carefully separated from the
bronchi. The lung wet weight (LWW [g]) and the lung wet weight to body weight ratio (LWR)
was determined before drying the lung tissue in an oven at 50°C. The mean LWR for the
animals exposed to blast was expressed as a multiple of the LWR of non-traumatized
controls; this ratio was designed the injury quotient (Qi). Thus Qi = LWR (injured animals)
divided by LWR (controls). The extent of injury was determined as minor or uninjured for Qi <
1.2, moderate for Qi = 1.2 to 1.5, severe for Qi = 1.5 to 1.9, and very severe for Qi > 1.9 162.
After three days a stable dry weight of the lungs was achieved and the wet-to-dry weight ratio
was calculated.
3.18 Histological examinations
After exsanguination and opening of the thoracic cage the cardiac apex was cut and a
catheters was placed in the pulmonary artery. Then a non-recirculating perfusion (30 ml/ min)
with ice-cold PBS was started to remove the blood from the pulmonary circulation. The heart-
lung block was excised, cleaned and infused intratracheally with 4% buffered formalin (15 cm
H20). The paraffin embedded lung tissues were cut in five-micrometer sections and stained
with haematoxylin and eosin (H & E) and examined by light microscopy. Representative
sections are shown (in the chapter “Results”).
3.19 Statistics
Data in the figures are given as means ± SEM, data in the tables as mean ± SD. The entire
curves data from two experiments were compared by a Two-way ANOVA design. This test,
determines how a response is affected by different factors e.g. drug treatment. Values of p <
0.05 were considered statistically significant. Data from end- or other time-points were
analysed by One-way ANOVA. In case of differences among the groups, post-tests were
performed as indicated in the legends (Dunnet’s Multiple Comparison Test, Tukey’s Multiple
Comparison Test or Bonferroni's Multiple Comparison Test); Statistics were performed with
the Graph Pad Prism 3.0 software (Graph Pad Software, San Diego, CA, USA).
Results
38
4. Results
4.1 System characteristics
Since it turned out that the blast wave generator originally designed and constructed by Irwin
and coworkers in 1998, 117 and modified by our colleagues in Ulm (U.C. Liener, F. Gebhard, L.
Kinzl) was lacking reproducibility concerning the variability of the measured lung function
parameters, we tried to modify this setting to our specific needs in order to optimise the
reproducibility of pressure wave exposure and the monitoring of the pressure wave.
4.1.1 Variability and influence of physical parameters
A well-defined pressure wave exposure requires a standardized rupture of the Mylar
polyester film. There is a good correlation between the speed of the air supply of the pressure
reservoir, the rupture of the diaphragm and the degree of standardization of the expansion of
the pressure wave. In order to obtain a fast air supply from the storage tank into the pressure
reservoir of the blast wave generator, we installed a 0.75 l compressed air bottle in between.
In addition, the bottle was located as close as possible to the pressure reservoir. The working
pressure of 18 bar in the air bottle was determined higher than the burst strength of the Mylar
diaphragm (≈ 8.5 bar). Thus a complete rupture of the polyester film was reached, as
compared to the incomplete rupture in the case of a slow air supply via a compressed-air hose
directly to the valve and the pressure reservoir. By pressing the diaphragm along a
predetermined breaking point between pressure reservoir and nozzle instead of only fixing it
with screws, the rupture of the film was further optimised (Fig. 4.1).
Figure 4.1: The nozzle of the blast wave generator in A) the top view and in B) the predetermined breaking point in detail.
Results
4.1.1.1 Monitoring and standardization of the blast pressure wave
For an exact monitoring of the blast pressure wave as the basis of comparability between
different experiments, we assessed the pressure wave data by different sensors at different
positions. As exemplarily presented in Figure 4.2 the pressure measurement by the
transducer in the reservoir revealed a fast pressure increase of up to 8.7 bar within 19.2 ms,
depending on and limited by the opening time of the valve, an immediate decay to zero
indicating a fast rupture of the diaphragm and therefore a fast exposure of the pressure wave
by the nozzle, and a negative phase or suction.
P
l
(
a
w
ressure curves over time measured at the thorax level by two transducers on the right and
eft side of the rat revealed a nearly instantaneous 100 percent rise time of 85 and 295 µs
Pp(r), Pp(l)) to the pressure peaks 3.4 and 3 bar (Pp(r), Pp(l)) and a duration (t(r), t(l)) of 654
nd 625 µs respectively (Fig. 4.3). The calculated area under the curves (AUC(r), AUC(l))
ere 101.35 and 100.37 V*s, respectively.
Figure 4.2: Time course of pressure increase in the pressure reservoir until rupture of the diaphragm. The working pressure in the compressed air bottle was 18 bar. Under control of a valve the pressure charged the pressure reservoir. The time course of the rupture pressure (Rp) was measured by the transducer in the reservoir. 0 5 10 15 20 25
-10123456789
10
t [ms]
Rp
[bar
]
4.0
39
Figure 4.3: Pressure wave monitoring at rat thorax level. The pressure wave data were measured over time by two sensors on the right Pp(r) and left side Pp(l) of the rat. Pp(r): , n = 1; Pp(l): ---, n = 1. 0 250 500 750 1000 1250 1500
0.0
0.5
1.0
1.5
2.0
2.5
3.0
3.5
t [µs]
Pp [b
ar]
Results
40
Table 4.1 summarizes the pressure wave data and the calculated area under the curves at a
3.5 cm distance from the nozzle measured in the present study.
Table 4.1: Pressure wave data measured by different transducers at various positions.
Rp
[bar]
Pp(r)
[bar]
AUC(r)
[V*s]
t(r)
[µs]
Pp(l)
[bar]
AUC(l)
[V*s]
t(l)
[µs]
mean±SD 8.56 ± 0.21 2.69 ± 0.37 95.04 ± 5.81 612.6 ± 17.42 3.63 ± 0.94 101.73 ± 10.4 644.71 ± 55.01
n 218 219 220 219 220 218 217
CV [%] 2 14 6 3 26 10 9
Pressure wave data were measured at a distance of 3.5 cm from the nozzle by three different transducers at different positions: cracking pressure in the pressure reservoir (Rp), pressure peaks at thorax level with two transducers on the left and the right side (Pp(r), Pp(l)). The corresponding area under the curves (AUC(r), AUC(l)) and the duration of the pressure wave t(r), t(l) were calculated. Data are expressed as mean ± SD, number of individual experiments (n), variation coefficient (CV).
The mean values of the pressure wave data measured and calculated from the right and left
transducer were assumed to be the pressures obtained above the rat thorax (Tab. 4.2).
Table 4.2 Assumed pressure conditions above the rat thorax.
3.5 cm
distance
Pp(r+l)
[bar]
AUC(r+l)
[V*s]
t(r+l)
[µs]
mean ± SD 3.16 ± 0.43 98.35 ± 6.18 628.78 ± 29.31
n 219 220 216
CV [%] 14 6 5
Pressure wave data were measured at a distance of 3.5 cm from the nozzle by three different transducers at different positions: mean of the pressure peaks at thorax level (Pp(r+l)), mean of the calculated area under the curve: (AUC(r+l)) and mean of the duration of the pressure wave (t(r+l)). Data are expressed as mean ± SD, number of individual experiments (n), variation coefficient (SD/ median) (CV).
To further improve the reproducibility of the setting, the animals were always blasted in the
same breathing situation during spontaneous breathing at halothane anaesthesia, namely at
top of expiration. This was achieved by a string above thorax that allows respiratory
monitoring and which triggers automatically the time point of valve opening and thus of the
blast. Figure 4.4 shows exemplarily the breathing frequency at halothane anaesthesia that
was uniformly 36 breaths per minute compared to physiological 100 - 130 breaths/ minute
indicating a deep anaesthesia (Fig. 4.4 A). The animals had a low breathing frequency
Results
immediately after blast exposure (Fig. 4.4 B), which was sometimes only transient in nature
depending on anaesthesia.
FBA
T
±
4
T
e
0
s
m
c
a
A) B)
41
igure 4.4: Respiratory monitoring before and after pressure wave exposure. reathing frequency was monitored with a string above the rat thorax connected with a sensor: ) before and B) after pressure wave exposure, exemplary for n = 1.
he mean respiratory rate before blast at 3.5 cm distance throughout the experiments was 38
12 breath/ minute (n = 224).
.1.1.2 Distance dependency of the pressure wave parameters
he mean pressure peak (Pp(r+l)) measured at rat thorax level decayed rapidly as it
xpanded from the blast wave generator. This pressure decrease correlated significantly (r = -
.58) with the distance (Fig. 4.5 A), allowing rats` exposure to different blast intensities by
imply varying the distance between the blast wave generator and the rat. Moreover, the
ean duration of the pressure wave (t(r+l)) and therefore the impact on the rat and the
alculated area under the curve (AUC (r+l)) correlated significantly with the distance (r = 0.24
nd r = 0.51) respectively (Fig. 4.5 B+C).
0.0 0.5 1.0 1.5 2.0 2.5 3.0
insp
iratio
nex
pira
tion
t [s]0 10 20 30 40 50
insp
iratio
nex
pira
tion
t [s]
Results
A)
2.5 3.5 4.5 5.5 6.5 7.5 8.5 9.5
1
2
3
4
5
distance below nozzle [cm]
Pp (r
+l) [
bar]
B)
2.5 4.5 6.5 8.5 10.5
0
250
500
750
1000
distance below nozzle [cm]
time
(r+l
) [µs
]
C)
42
Figure 4.5: Correlation between pressure wave parameters and distance below the nozzle. The pressure wave data were measured at different distances below the nozzle: A) mean pressure peak (Pp(r+l); B) mean duration of the pressure wave (t(r+l)) and C) mean calculated area under the curve (AUC(r+l)). The number of experiments (n) was n = 220. The statistical analysis was done by correlating A) - C) with the distance and linear regression revealing a Pearson r of r = 0.58 (p < 0.0001), r = 0.24 (p = 0.0003) and r = 0.51 (p < 0.0001), respectively.
2.5 3.5 4.5 5.5 6.5 7.5 8.5 9.5
0
25
50
75
100
125
150
distance below nozzle [cm]
AUC
(r+l
) [Vs
]
Results
4.1.1.3 Pressure wave data of survivors versus non-survivors
The mortality was about 14.46% in the group exposed to the blast at a distance of 3.5 cm,
mostly due to vessel rupture. Comparing the pressure wave data of the survivors versus the
non-survivors, the latter showed a higher rupture pressure (Rp, p = 0.0004) resulting in a
pressure wave curve with no significant higher pressure peak at rat thorax level (Pp(r+l), p =
0.89) but a longer duration (t(r+l), p = 0.025) and therefore an increased area under the curve
(AUC(r+l), p = 0.025) (Tab. 4.3). Since the Mylar polyester films show differences in their
physical characteristics (supplier information) and since different lots of Mylar polyester film
were used in the present study, the differences in the necessary rupture pressures may be
explained. A relationship between mortality and pre-blast breathing frequency with regard to a
prolonged recovery time from anaesthesia, could not be observed (survivors: 38 ± 12 breath/
minute (n = 224); non-survivors: 44 ± 16 breath/ min (n = 36)).
Table 4.3: Comparison of the pressure wave data from survivors versus non-survivors.
The presrighttwo the cData
4.2
4.2.
Alth
com
impa
func
imm156,16
sur
non
sur
distance
[cm] n
Rp
[bar]
Pp(r+l)
[bar]
AUC(r+l)
[V*s]
t(r+l)
[µs]
vivors 235
8.56 ± 0.21
(218)
3.16 ± 0.43
(219)
98.35 ± 6.18
(220)
628.78 ± 29.31
(216)
-3.5
34 8.72 ± 0.39 3.17 ± 0.33 101.05 ± 7.34 642.31 ± 45.18
43
animals were exposed to the pressure wave at a distance of 3.5 cm below the nozzle. The sure wave data were recorded by a transducer in the pressure reservoir (Rp), two sensors at the and left side at rat thorax level (Pp(r), Pp(l)). The data represent the recorded mean values of the transducers: mean pressure peak (Pp(r+l)), mean duration (t(r+l)) and mean calculated area under urve (AUC(r+l)). Data represent mean ± SD, number of individual experiments (n) in parentheses. were analysed by an unpaired t-test (* p < 0.05, *** p < 0.0001).
Functional changes of alveolar macrophages and interaction with blood in vitro after trauma
1 Trauma-induced impairment in host defence mechanisms
ough it is reported that severe trauma contributes to an increase in infectious
plications through an impairment of host defence mechanisms 163, the cause of such
irment remains unknown 164. Most studies have focused on the suppression of immune
tion determined during the first few hours after trauma, implying that this
unosuppression may be responsible for an impairment of host defence mechanisms 5. Since the alveolar macrophage, mobile representative of the mononuclear phagocyte
vivors (34) *** (33) (32) * (32) *
Results
system, is believed to be the central modulator as both regulator and effector of inflammation/
anti-inflammation within the alveolar space 48, macrophage function following experimental
blunt chest trauma with regards to phagocytotic capacity, respiratory burst and mediator
release was assessed.
4.2.1.1 Differences in the amount of isolated macrophages depending on the time after trauma
The macrophage is by far the most abundant non-parenchymal lung cell: about 50 to 100
macrophages are found per alveolus, and they dominate lymphocytes by a ratio of
approximately 5 to 10 49. The number of macrophages recruited from the alveolar space of
rats after thoracic trauma, ranging from 3.11 ± 1.08 x 106 cells/ ml (10 minutes after trauma) to
9.86 ± 0.34 x 106 cells/ ml (96 hours after trauma) of bronchoalveolar lavage exudates
depending on the time after blast exposure (Fig. 4.6), was significantly different from that of
non-traumatized controls (6.32 ± 0.92 x 106 cells/ ml). The observed increase after 96 hours
may be due to an excess of macrophages recruited into the alveolar space.
4
I
d
c
S
0
***
44
.2.1.2 Trauma-related modulation of phagocytosis of dead, fluorescence labelled E. coli and S. aureus by alveolar macrophages
nitially after the blast pressure wave exposure, the alveolar macrophage phagocytosis rate of
ead, fluorescence labelled Escherichia coli (E. coli) was reduced by 82% (Fig. 4.7) and
ontrol levels were reached 96 hours after the blast. In contrast, the phagocytic capacity for
taphylococcus aureus (S.aureus) particles was not significantly impaired after trauma (p =
.075).
Figure 4.6: Thoracic trauma-induced changes in the amount of resident alveolar macrophages. Animals were sacrificed 10 min (n = 37), 24 (n = 23) and 96 (n = 13) hours after trauma, non-traumatized animals served as sham controls (n = 57). The alveolar macrophages were harvested by BAL. Data represent means ± SD, number of individual experiments (n) in parentheses. Data were statistically analysed by One-way ANOVA and Tukey's Multiple Comparison Test: ***p < 0.001 vs. sham control, 96 hours.
sham
contro
l
+10m
in+2
4h+9
6h
2.5×1006
5.0×1006
7.5×1006
1.0×1007
time after blast exposure
*** ***
BA
L ce
ll co
unt [
cells
/ml]
Results
4
N
r
t
“
s
S
S
p
o
b
t
T
s
400
FcTcncaD
45
.2.1.3 Oxidative burst capacity after trauma induced by Gram positive and Gram negative stimuli
ext, we investigated whether the oxidative burst capacity of the alveolar macrophages in
esponse to either whole, dead bacteria or endotoxin was impaired, following experimental
horax trauma, using the superoxide sensitive dye WST-1 (as described in the chapter
Materials and Methods”). Thoracic trauma yielded a marked decrease in the production of
uperoxide within the first 24 hours after trauma, both with or without the addition of E. coli or
. aureus, with recovery only after 96 hours (Fig. 4.8 A).
imilarly, the trauma-related initial decrease of superoxide generation was independent of the
resence of lipopolysaccharide (LPS) or lipoteichoic acid (LTA) (Fig. 4.8 B). Superoxide levels
f non-traumatized controls were reached already at 24 hours. Furthermore, 96 hours after the
last the superoxide production was significantly increased in all groups, as compared to non-
raumatized controls.
aken together, these results indicate that thoracic trauma decreases the production of
uperoxide by primary rat alveolar macrophages.
E. coli S. aureus0
100
200
300
sham controltrauma: +10mintrauma: +24htrauma: +96h
**
rela
tive
units
igure 4.7: Thorax-trauma related modulation of phagocytosis of dead, fluorescence labelled E. oli/ S. aureus by primary alveolar macrophages. he alveolar macrophages (AM) were cultured either non-stimulated or stimulated with fluorescent E. oli and S. aureus particles (250 µg/ ml) for three hours respectively. Data represent means ± SEM, umber of individual experiments (n) in parentheses: AM harvested either from non-traumatized sham ontrols (n = 10); from recently (10 min) traumatized rats (n = 7) and from rats traumatized 24 h (n = 8) nd 96 h (n = 6) in advance. Data were analysed by One-way ANOVA (on log-transformed data) and unnett's Multiple Comparison Test: * p < 0.05, ** p < 0.01 vs. control.
Results
Fmd(t(stO
A)
non-stim
ulated
E. coli
S. aureu
s0
20
40
60
***
****
***
sham controltrauma: +10mintrauma: +24htrauma: +96h
supe
roxi
de p
rodu
ctio
n [p
mol
/min
]
*
B)
46
igure 4.8: Thoracic trauma decreases the production of superoxide by primary rat alveolar acrophages. The alveolar macrophages were seeded either non-stimulated or stimulated with whole,
ead bacteria or endotoxin for three hours. Data are means ± SEM, number of individual experiments n) in parentheses: A) E. coli or S. aureus stimulation (250 µg/ ml) of alveolar macrophages from non-raumatized sham controls (n = 8); from recently traumatized rats (10 min) n = 9) or 24 h (n = 7) and 96 h after trauma (n = 5), and B) LPS (0.1µg/ ml) or LTA (100 µg/ ml) timulation of alveolar macrophages either from non-traumatized sham controls (n = 5); from recently raumatized rats (n = 4) or from rats 24 h (n = 4) and 96 h (n = 3) after trauma. Data were analysed by ne-way ANOVA and Dunnett's Multiple Comparison Test: * p < 0.05, ** p < 0.01 vs. control.
non-stim
ulated LTA
LPS0
50
100
150
200
250
sham controltrauma: +10mintrauma: +24htrauma: +96h
**
**
**
**
**
**
supe
roxi
de p
rodu
ctio
n [p
mol
/min
]
Results
4.2.1.4 Trauma-related modulation of TNF release after Gram positive and Gram
negative stimulation
Due to the key role of alveolar macrophages (AM) as modulators of pulmonary inflammation,
we further investigated macrophage-induced tumor necrosis factor α (TNF α) release after
experimental thorax trauma alone and in response to Gram-positive and Gram-negative
stimuli. The TNF release of non-stimulated AM was more than 3-fold increased 96 hours after
blast, indicating that the AM are primed to release TNF following thoracic trauma. Additional
stimulation of the AM with whole, dead E. coli or S. aureus induced a marked TNF release
already 24 hours after trauma. In contrast, initially after trauma the stimulation with bacteria
did not increase the TNF release as compared to sham controls. In the case of E. coli
stimulation, the TNF release was even decreased at this time point (Fig. 4.9 A). In these
experiments E. coli stimulation was more potent in inducing TNF release from AM than S.
aureus.
I
T
t
a
t
i
t
A)
47
n line with the results described above, there was a more than 1.5-fold and 3-fold increase in
NF release in response to LPS and LTA stimulation (100 µg/ ml), respectively, 24 hours after
rauma. In contrast, no endotoxin-induced increase in TNF release could be detected initially
fter trauma, as compared to non-traumatized sham controls (Fig. 4.9 B+C). With regard to
he TNF release, the AM are more susceptible towards LPS than LTA stimulation. These data
ndicate that 24 hours after blast injury the AM showed an increased TNF release in response
o both whole bacteria or endotoxin.
non-stim
ulated
E. coli
S. aureu
s0
1000
2000
3000
4000
5000
6000
sham controltrauma: +10mintrauma: +24htrauma: +96h
**
**
**
**
TNF α ααα
[pg/
ml]
Results
48
4.2.2 Role of the trauma-induced alveolar haemorrhage in impaired macrophage functions
The most frequent and obvious injury, detected in our rat blast model, was bilateral pulmonary
haemorrhage, due to a disruption of the alveolar parenchyma and capillaries, with exudation
of blood into the interstitial and alveolar spaces. Therefore, we tested whether the observed
macrophage dysregulation after trauma is due to the accompanying alveolar haemorrhage.
Thus, we lysed the red blood cells (RBCs) in the harvested BAL fluids (as described in the
chapter “Materials and Methods”) before seeding, stimulation and assessing the macrophage
function. This manipulation did not lead to any changes in macrophage functions (data not
shown).
4.2.2.1 Role of alveolar haemorrhage in reduced phagocytosis
Based on the total reduction of 70 ± 26% of the phagocytic capacity for labelled E. coli
particles of alveolar macrophages from traumatized animals, as compared to non-traumatized
sham controls, the removal of red blood cells (RBCs) resulted in a more than 2-fold increase
in phagocytic capacity of AM from traumatized rat lungs (p = 0.0078). These experiments
Figure 4.9: Thoracic trauma leads to alterations in TNF release. The alveolar macrophages were seeded either non-stimulated or stimulated with E. coli and S. aureus particles (250 µg/ ml) or with LPS (100, 10, 1, 0.1 and 0.01 µg/ ml) and LTA (100, 50, 10, and 2 µg/ ml) for three and four hours, respectively: A) E. coli and S. aureus stimulation of alveolar macrophages harvested either from non-traumatized sham controls (n = 8); from recently traumatized rats (n = 7) and from rats 24 h (n = 7) and 96 h (n = 5) after trauma, B) LPS and C) LTA stimulation of alveolar macrophages either from non-traumatized sham controls (n = 6); from recently traumatized rats (n = 7) and from rats 24 h (n = 5) after trauma. Data were analysed by One-way ANOVA and Dunnett's Multiple Comparison Test: * p < 0.05, ** p < 0.01 vs. control. Data represent means ± SEM, number of individual experiments (n) in parentheses.
100 10 1
0.1
0.01
non-
stim
ulat
ed
0
2500
5000
7500
10000 sham controltrauma: +10mintrauma: +24h
TNF α ααα
[pg/
ml]
LPS [µg/ml]
**
*
**
*
B)
100 50 10 2
non-
stim
ulat
ed
0
500
1000
1500
2000
2500 sham controltrauma: +10mintrauma: +24h
LTA [µg/ml]
TNF α ααα
[pg/
ml]
**
***
C)
Results
Fptntr
suggested that the massive alveolar haemorrhage is at least in part responsible for the
impaired phagocytic capacity after trauma in this model (Fig. 4.10).
4
A
o
(
p
T
i
100
Figure 4.10: Impairment of phagocytosis upon thorax trauma is partly due to the accompanying alveolar haemorrhage. E. coli (250 µg/ ml) stimulation of alveolar macrophages from non-traumatized sham controls (n = 6) and recently traumatized rats (10 min) (n = 6) with or without lysis of the red blood cells (RBCs) respectively. Data were analysed by an unpaired t-test: ** p < 0.01 trauma (lysed RBCs) vs. trauma. Data represent means ± SEM, number of individual experiments (n) in parentheses.
.2.2.2 Role of alveolar haemorrhage in reduced oxidative burst
s already mentioned in 4.2.1.3 thoracic trauma yielded a marked decrease in the production
f superoxide, as compared to non-traumatized sham controls. Lysis of the red blood cells
RBCs) showed an up to 6-fold (p = 0.0248) and 8-fold (p < 0.0001) increase in superoxide
roduction of AM from traumatized rat lungs with or without E. coli stimulation, respectively.
hese data provided further evidence that alveolar haemorrhage plays a role in the trauma-
nduced decrease in superoxide production by alveolar macrophages (Fig. 4.11).
25
50
75
trauma: +10mintrauma: +10min(lysed RBCs)
sham controlsham control(lysed RBCs)
sham control trauma: +10min
**
rela
tive
units
100 sham control]
49
igure 4.11: Alveolar haemorrhage plays a role in thorax trauma-related decrease in superoxide roduction. Alveolar macrophages from non-traumatized sham controls (n = 4) and recently
raumatized rats (10 min) (n = 3) with or without lysis of the red blood cells (RBCs) and cultured either on-stimulated or stimulated with E. coli (250 µg/ ml) respectively. Data were analysed by an unpaired -test: * p < 0.05 vs. trauma (E. coli stimulation), *** p < 0.0001 vs. trauma (non-stimulated). Data epresent means ± SEM, number of individual experiments (n) in parentheses.
0
25
50
75
non-stimulatedE. coli
no RB
Cs
trauma: +10min
no RB
Cs
*** *
supe
roxi
de p
rodu
ctio
n [p
mol
/min
Results
50
Figure 4.12: Alveolar haemorrhage plays a minor role in TNF release after trauma. Alveolar macrophages were harvested from non-traumatized sham controls (n = 6) and recently traumatized rats (10 min) (n = 6) with or without lysis of the red blood cells (RBCs) and cultured either non-stimulated or stimulated with E. coli (250 µg/ ml) respectively. Cells without bacteria were used to determine the background and were subtracted. Data were analysed by an unpaired t-test. Data represent means ± SEM, number of individual experiments (n) in parentheses.
4.2.2.3 Role of alveolar haemorrhage in diminished TNF release
Next, we investigated whether the trauma-associated alveolar haemorrhage affects the TNF
release from alveolar macrophages in response to E. coli particles. Figure 4.12 shows that in
the presence of RBCs the TNF release was reduced by 48 ± 21% in consequence of pressure
wave exposure. However, in the absence of RBCs, the TNF release from AM from
traumatized animals was not significantly increased (p = 0.0887). In contrast to the
phagocytosis and oxidative burst capacity, these data exclude a major role of the alveolar
haemorrhage in trauma-related diminished TNF release.
1000
2000
3000
4000
sham control(lysed RBCs)
trauma: +10mintrauma: +10min(lysed RBCs)
sham control
TNF α ααα
[pg/
ml]
4.2.3 Influence of different blood components on the macrophage function
Since at least a part of the trauma-induced macrophage dysregulation was shown to be due to
the associated alveolar haemorrhage, we tested different blood components, which could be
responsible for the observed effects. For this purpose, we prepared washed and haemolysed
red blood cells (RBCs), haemolysate of RBCs, and plasma from peripheral venous blood (as
described in the chapter “Materials and Methods”) and tested whether these different blood
components impaired the macrophage functions. To preserve the in vivo conditions after
thorax trauma, whole blood and the prepared components were used in a final concentration
of 1.25%, corresponding to the red blood cell counts found in bronchoalveolar lavage fluids
from traumatized rats (data not shown).
4.2.3.1 Influence on phagocytosis
The phagocytic activity was significantly diminished in the presence of whole blood and
washed red blood cells (RBCs), whereas the addition of haemolytic blood, plasma, haemolytic
RBCs and RBC haemolysate had no effect (Fig. 4.13). These results indicate that only intact
blood cells, but neither cellular debris nor plasma components decreased phagocytosis.
Results
250
FmsnnaE
51
E. coli
+ whole
blood
+ hae
molytic
blood
+ plas
ma
+ was
hed RBCs
+ hae
molytic
RBCs
+ RBC hae
molysate
0
50
100
150
200
* *
rela
tive
units
igure 4.13: Blood cells attenuate phagocytosis of fluorescent E. coli particles by alveolar acrophages. Alveolar macrophages harvested from non-traumatized sham controls (n = 8) were
timulated with fluorescent E. coli (250 µg/ ml) particles together with either whole blood (1.25%, = 4), haemolytic blood (1.25%, n = 5), plasma (1.25%, n = 3), washed red blood cells (RBCs) (1.25%, = 5), haemolytic RBCs (1.25%, n = 5) or RBC haemolysate (1.25%, n = 5). Data were statistically nalysed by One-way ANOVA and Dunnett's Multiple Comparison Test: * p < 0.05 vs. . coli control. Data represent means ± SEM, number of individual experiments (n) in parentheses.
Results
4.2.3.2 Influence on oxidative burst
In contrast to the reduced phagocytosis by whole, intact blood cells, the oxidative burst
capacity was significantly reduced by haemolytic blood, both with or without the addition of E.
coli (Fig. 4.14). Furthermore, the addition of plasma yielded a decrease of superoxide
generation, although to a lesser extent than with E. coli and afflicted by variations between the
individual experiments. The plasma-related effect may be explained by a plasma
contamination with intracellular components due to centrifugation.
Fmcb(r*S
70
52
igure 4.14: Intracellular blood cell components decrease the oxidative burst by alveolar acrophages. Alveolar macrophages harvested from non-traumatized sham controls (n = 8) and
ultured either non-stimulated or stimulated with whole, dead E. coli (250 µg/ ml), together with whole lood (1.25%, n = 4), haemolytic blood (1.25%, n = 5), plasma (1.25%, n = 3), washed red blood cells RBCs) (1.25%, n = 5), haemolytic RBCs (1.25%, n = 5) and RBC haemolysate (1.25%, n = 5) espectively. Data were analysed by One-way ANOVA and Dunnett's Multiple Comparison Test: p < 0.05, ** p < 0.01 vs. non-stimulated and E. coli-stimulated control, respectively. Data are means ± EM, number of individual experiments (n) in parentheses.
+ whole
blood
+ hae
molytic
blood
+ plas
ma
+ was
hed RBCs
+ hae
molytic
RBCs
+ RBC hae
molysate
0
10
20
30
40
50
60
non-stimulatedE. coli
** ****
supe
roxi
de p
rodu
ctio
n [p
mol
/min
]
Results
4.2.3.3 Influence on TNF release
In line with the reduced oxidative burst capacity by haemolytic blood, the E. coli-induced TNF
release was also significantly reduced, whereas the addition of the other blood components
was without effect (Fig. 4.15).
T
c
s
d
t
s
4
T
5000
Fmsnndan
53
he experiments described above were also assessed with whole blood and prepared blood
omponents in a final concentration of 5%. Compared to 1.25% there were no statistically
ignificant differences in the phagocytotic- and oxidative burst activity or TNF release
etectable (data not shown). Whole intact blood cells as well as cellular debris seeded
ogether with harvested macrophages interfered with the macrophage adhesion (data not
hown).
.2.4 Summary of the in vitro findings
he results of the different in vitro experiments are summarized in the Table 4.4.
E. coli
+ whole
blood
+ hae
molytic
blood
+ plas
ma
+ was
hed RBCs
+ hae
molytic
RBCs
+ RBC hae
molysate
1000
2000
3000
4000
**
TNFα ααα
[pg/
ml]
igure 4.15: Haemolytic blood decreases E coli-induced TNF release by macrophages. Alveolar acrophages from non-traumatized sham controls (n = 8) were cultured either non-stimulated or
timulated with E. coli (250 µg/ ml) together with whole blood (1.25%, n = 4), haemolytic blood (1.25%, = 5), plasma (1.25%, n = 3), washed red blood cells (RBCs) (1.25%, n = 5), haemolytic RBCs (1.25%, = 5) and RBC haemolysate (1.25%, n = 5) respectively. Cells without bacteria were used to etermine the background TNF levels and were subtracted. Data were analysed by One-way ANOVA nd Dunnett's Multiple Comparison Test: ** p < 0.01 vs. E.coli control. Data represent means ± SEM, umber of individual experiments (n) in parentheses.
Results
54
A) Thorax trauma-related changes in macrophage functions.
time after blast exposure
stimulus read out sham control 10min 24h 96h
phagocytosis
oxidative burst non-stimulated
TNF release
phagocytosis / / / /
oxidative burst / / / / E. coli/ S. aureus
TNF release / / / /
oxidative burst / / / / LPS/ LTA
TNF release / / / -
B) Influence of different blood components on macrophage functions.
Table 4.4: no change, upregulation, downregulation (compared to sham control A) and non-stimulated and E. coli stimulation B), respectively), and - not measured.
non-traumatized controls
non-stimulated E. coli
addition of: phagocytosis oxidative
burst
TNF
release phagocytosis
oxidative
burst
TNF
release
cell culture
medium
whole blood
haemolytic
blood
plasma
washed
RBCs
haemolytic
RBCs
RBC
haemolysate
Results
55
4.3 Functional consequences and endogenous modulation in vivo
After an initial non-fatal injury, thoracic trauma is considered to play a pivotal role in the
development of single-or multi-organ failure 97, probably making the patient more susceptible
to infections 95. The initial physiologic responses to thoracic trauma have not been adequately
investigated and none of the numerous interventions studied until today made it into clinical
practice. Therefore, we investigated the pathophysiological consequences occurring in rat
lungs in response to primary blast exposure in vivo over time.
4.3.1 Blast injury-induced disruption of the alveolar capillary barrier
As already mentioned in 4.2.2, histological examinations of the blasted rat lungs showed
characteristic signs of pressure wave-induced injury (Fig. 4.16 A-E). The non-traumatized
sham controls showed a normal lung structure (Fig. 4.16 D+E). In contrast, at 10 minutes, i.e.
immediately after blast pressure wave exposure, a massive alveolar haemorrhage and
exudation of fluid into the interstitial and alveolar spaces was detectable (Fig. 4.16 A).
Disruption of the alveolar septa was also observed (not shown in the present visual field). At 3
hours after blast exposure, there was a marked focal alveolar haemorrhage, but there were
virtually no PMN infiltrates yet observed (Fig. 4.16 B). On the contrary, erythrocyte-laden huge
alveolar macrophages were observed 24 hours after the blast accompanying by a few
detectable PMN in the alveolar space (Fig. 4.16 C).
Figure 4.16: Histopathology of rat blast injury. Rats were exposed to the pressure wave at 3.5 cm distance from the nozzle. Animals were sacrificed either 10 min A), 3 hours B) or 24 hours C) after blast exposure, non-traumatized animals served as sham controls E) + D). Visualized at an original magnification of 40-fold A) – C) + E) and 10-fold in D).
Results
10
4.3.1.1 Thorax trauma-related BAL protein accumulation
In order to determine pressure-induced cell destruction, we assessed the total protein content
in the bronchoalveolar lavage fluids. Figure 4.17 illustrates a significant protein accumulation
in the alveolar space of traumatized lungs, as compared to non-traumatized controls (p <
0.0001). From 12 hours on, the protein levels decreased and returned to control levels 96
hours after trauma, indicating that some kind of repair and/ or active protein transport took
place 166.
4
I
t
f
d
a
FmedCe
56
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
2
4
6
8
time after blast exposure
****
**
prot
ein
cont
ent [
mg/
ml]
.3.1.2 Thorax trauma-induced pulmonary haemorrhage
ntra-alveolar haemorrhage quantified by red blood cell (RBC) counts in BAL fluids of
raumatized rat lungs (Fig. 4.18) showed a massive increase within the first 10 minutes,
ollowed by a decrease from 3 hours on. At 96 hours after blast exposure no RBCs were
etectable. These results provided evidence for an enormous clearance over time, which is
lso reported for clinical situations of alveolar haemorrhage 167.
igure 4.17: Blast injury-related protein accumulation in BAL fluids. Animals were sacrificed 10 in (n = 5), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours (n = 3) after blast
xposure, non-traumatized animals served as sham controls (n = 9). Protein concentration was etermined in the BAL fluid. Data were analysed by One-way ANOVA and Dunnett's Multiple omparison Test: ** p < 0.01 vs. control. Data represent means ± SEM, number of individual xperiments (n) in parentheses.
Results
10.0
4
T
m
b
0
T
e
a
h
i
F(efa
57
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0.0
2.5
5.0
7.5
time after blast exposure
*
** **R
BC
s [1
07 /ml]
.3.1.3 Trauma-induced cell destruction
he release of the cytosolic enzyme lactate dehydrogenase (LDH) into the BAL was used as a
arker for cellular integrity after blast. In accordance with the protein accumulation and red
lood cell counts, LDH activity was significantly increased upon pressure wave exposure (p =
.0047) (Fig. 4.19). This also confirmed the mechanical-induced cell damage in this setting.
he levels were still elevated 24 hours after the blast, probably due to the long half-life of the
nzyme and/ or possible delayed cell death. The activity returned to control levels 96 hours
fter blast. Thus, the BAL LDH activity, in contrast to the different kinetics of the alveolar
aemorrhage and total protein content, may be a suitable marker for the extent of the initially
nduced injury.
igure 4.18: Blast injury-related pulmonary haemorrhage. The animals were sacrificed 10 min n = 5), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 3), 24 h (n = 3) or 96 hours (n = 3) after blast xposure, non-traumatized animals served as sham controls (n = 8). RBCs were determined in BAL luids. Data were analysed by One-way ANOVA and Dunnett's Multiple Comparison Test: *p < 0.05 nd ** p < 0.01 vs. control. Data are means ± SEM, number of experiments (n) in parentheses.
Results
200
4
P
s
o
e
(
w
q
6
d
v
58
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
50
100
150
time after blast exposure
**
**
*LD
H ac
tivity
[uni
ts/l]
.3.1.4 Thorax trauma related pulmonary oedema formation
ulmonary injury, quantified by the lung wet to dry weight ratio (wet WT/ dry WT ratio), was
ignificantly increased within the first 90 minutes after blast (p < 0.001), indicating pulmonary
edema formation (Fig. 4.20). The reduced ratios assessed from three hours after blast
xposure on may suggest that oedema generation stopped and/ or fluid resorption increased
1.5 h vs. 6 h: p < 0.001). However, although not significant different, the calculated lung wet
eight (LWW) to body weight (BW) ratio (LWR) (p = 0.27) and the corresponding injury
uotient (Qi) (described in detail in the chapter Material and Methods, 162) examined between
and 24 hours after blast exposure may indicate a secondary deterioration (Tab. 4.5). This
iscrepancy may be explained by pulmonary infiltrates in these lungs, which were not obvious
isible in the lung wet to dry weight ratios.
Figure 4.19: LDH release after thoracic trauma. The animals were sacrificed 10 min (n = 5), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours (n = 3) after blast exposure, non-traumatized animals served as sham controls (n = 8). LDH activity was determined in BAL fluids. Data were analysed by One-way ANOVA and Dunnett's Multiple Comparison Test: *p < 0.05 and ** p < 0.01 vs. control. Data are means ± SEM, number of experiments (n).
Results
T
TM
FaDv
** **
59
able 4.5: Time course of wet WT/ dry WT ratio and LWR
time after blast n BW [g] wet Wt/ dry WT
ratio LWR Qi
sham control 3 250 ± 13 5.32 ± 0.21 0.0045 ± 0.0006
10 min 4 234 ± 11 6.58 ± 0.99 0.0082 ± 0.0034 1.84
1.5 h 6 246 ± 6 6.77 ± 0.49 ** 0.0083 ± 0.0022 1.85
3 h 4 234 ± 7 5.64 ± 0.72 0.0064 ± 0.0017 1.44
6 h 4 233 ± 10 5.05 ± 0.34 0.0065 ± 0.0011 1.46
12 h 3 243 ± 4 5.15 ± 0.44 0.0081 ± 0.0033 1.82
24 h 3 237 ± 2 4.66 ± 0.13 0.0073 ± 0.0014 1.63
able 4.5: Data represent mean ± SD. Data were analysed by One-way ANOVA and Bonferroni's ultiple Comparison Test: **p < 0.01 1.5 h vs. sham control and 6 h after blast, respectively.
igure 4.20: Thorax trauma-induced weight gain. Lung wet weight and dry weight was determined t different time points after pressure wave exposure. The wet to dry weight ratios were calculated. ata were analysed by One-way ANOVA and Bonferroni's Multiple Comparison Test: **p < 0.01 1.5 h s. sham control and 6 h after blast, respectively.
sham
contro
l
10min
1.5h 3h 6h 12
h24
h
4
5
6
7
8
time after blast exposure
wet
WT/
dry
WT
ratio
Results
Fs(aTS
4.3.2 Blast injury-related mediator release
Besides clinical characterization, recent research data indicate that the prognosis of trauma
patients is strongly associated with a posttraumatic imbalance of the immune system 146. Post-
traumatic immunosuppression (“immunoparalysis”) 95,130 is a highly complex interplay of cell
interactions, cytokines, central nervous and humoral system, cell demise, and further factors.
Thus we focused on a restricted list of mediators that may explain the observed mitigation of
immune defence (described in 4.2).
4.3.2.1 Eicosanoid release
Since it is reported that there is a pattern-related release of prostanoids in patients suffering
from thoracic trauma 134, we examined the release of thromboxane and prostacycline into the
alveolar space over 96 hours, following blast pressure wave exposure. As expected and in
line with clinical data obtained from polytrauma patients with thorax involvement 138, there was
a marked immediate release of both thromboxane and prostacycline within the first 10 minutes
after blast followed by a significant decrease by 90 minutes. Within 96 hours after blast
exposure, we could not detect a secondary increase at the time points investigated (Fig. 4.21
A+B). Together with the lack of COX-2 induction, determined by RT-PCR analysis (data not
shown) within the first 6 hours after blast exposure, an inflammatory reaction, involving these
mediators during this time appeared to be rather unlikely.
A) B)
60
igure 4.21: Prostanoid release in the early phase after thoracic trauma. The animals were acrificed 10 min (n = 6), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours n = 3) after blast exposure, non-traumatized animals served as sham controls (n = 9). A) TxB2 release nd B) 6-keto PGF1α were determined in BAL fluids. Data were analysed by One-way ANOVA and ukey's Multiple Comparison Test. *** p < 0.001: 10min vs. all other groups. Data represent means ± EM, number of experiments (n) in parentheses.
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
200
400
600
800
1000
1200
1400
1600
1800
time after blast exposure
***
TxB
2[p
g/m
l]
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
500
1000
1500
2000
2500
3000
time after blast exposure
***
6-ke
to P
GF1
α ααα [p
g/m
l]
Results
61
4.3.2.2 Nitric oxide release
Since there was no COX-2 induction detectable, we were further interested whether there is
an induction of the NO-synthases (NOS) after thoracic trauma. Figure 4.22 may suggest a
two-phase release of nitric oxide related nitrite and nitrate with a delayed maximum 12 hours
after trauma. However, RT-PCR analysis revealed no induction of the inducible NOS within 12
hours (data not shown). These results indicate rather an initial trauma-induced NO release
due to the constitutive endothelial NOS, than an involvement of the iNOS during the first four
days following blast exposure in this setting.
4.3.2.3 Cytokine release
High synthesis of pro-inflammatory cytokines after trauma has been correlated with poor
outcome 168,169. Therefore, we examined the release of TNF-α and interleukin (IL)-6 after
thoracic trauma over time. Increasing BAL TNF-α levels were detectable from 3 hours after
trauma on, reaching a maximum 12 hours after blast exposure, followed by a continuous
decrease over 96 hours (Fig. 4.23 A). Plasma TNF-α was not detectable within 96 hours after
trauma, neither by ELISA nor by WEHI-assay (data not shown). In addition to TNF-α, IL-6
levels seemed to increase within 3 hours after trauma and reached significant peak levels
after six hours (Fig. 4.23 B). This early increase is in accordance with plasma IL-6 levels
obtained from polytrauma patients 142.
Figure 4.22: Thoracic trauma-induced nitric oxide release. The animals were sacrificed 10 min (n = 5), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours (n = 3) after blast exposure, non-traumatized animals served as sham controls (n = 8). Nitric oxide release was determined as nitrate in BAL fluids. Data were statistically analysed by One-way ANOVA (p = 0.0054) and Dunnett's Multiple Comparison Test: * p < 0.05 vs. sham control. Data are means ± SEM, number of experiments (n) in parentheses.
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
1
2
3
4
5 *
time after blast exposure
nitr
ate
[µM
]
Results
F
c
l
p
Fs(Bam
A) B)
urthermore, we measured interleukin (IL)-10, as a possible indicator for an anti-inflammatory
ounterregulation after trauma. In comparison to non-traumatized sham controls, the IL-10
evels in BAL fluids of traumatized animals were significantly decreased at any measured time
oint within 24 hours and returned to reference ratios 96 hours after blast (Fig. 4.24).
igure 4.23: Time course of TNF and IL-6 release after thoracic trauma. The animals were acrificed 10 min (n = 6), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours n = 3) after blast exposure, non-traumatized animals served as sham controls (n = 9). A) TNF-α and ) IL-6 release were determined in BAL fluids. Data were statistically analysed by One-way ANOVA nd Dunnett's Multiple Comparison Test: * p < 0.05 and ** p < 0.01 vs. sham control. Data represent eans ± SEM, number of experiments (n) in parentheses.
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
15
30
45
60
75
time after blast exposure
**
****
*TNFα ααα
[pg/
ml]
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
250
500
750
1000 **
time after blast exposure
IL- 6
[pg/
ml]
75
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
15
30
45
60
time after blast exposure
***
IL-1
0 [p
g/m
l]
Figure 4.24: Decrease in BAL IL-10 after thoracic trauma. The animals were sacrificed 10 min (n = 6), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours (n = 3) after blast exposure, non-traumatized animals served as sham controls (n = 9). IL-10 release was assessed in BAL fluids. Data were statistically analysed by One-way ANOVA and Dunnett's Multiple Comparison Test: * p < 0.05 and ** p < 0.01 vs. sham control. Data are means ± SEM, number of experiments (n) in parentheses.
62
Results
63
4.3.2.4 Measurement of soluble tumor necrosis factor receptors
Some publications have provided evidence for the presence of 55- and 75-k Da soluble tumor
necrosis factor receptors (sTNFRs) in injured patients, with a strong correlation with mortality 148,149. Because of the lack of detectable plasma TNF, together with the relatively moderate
levels of secreted TNF into the BAL after blast exposure, we examined sTNF R1 - and
sTNFR2-BAL levels in response to blast injury, in order to test whether the TNF is bound to
the soluble TNF receptors and therefore not active and possibly not detectable. Patterns of
BAL 55 and 75 kDa sTNFR at serial intervals after injury are illustrated in Figure 4.25 A. Both
soluble receptors were significantly elevated 90 minutes after blast. Then levels declined,
followed by a second marked increase within the first 6 to 12 hours, and reaching near
baseline levels within 24 hours. Within the first 12 hours after blast there were no remarkable
differences between 55 and 75 kDa sTNFR release. In contrast, 24 and 96 hours after trauma
the sTNFR p75 levels were significantly higher than the sTNFR p55 levels (p = 0.0074 and p =
0.04, respectively). Comparison of the 55 and 75 kDa sTNFR levels of non-traumatized
control lungs showed higher levels of sTNFR p75 than of p55 (p = 0.0113). The soluble tumor
necrosis factor receptor p55/ p75 ratio was significantly elevated within 6 hours of trauma and
returned to reference ratios after 12 hours (Fig. 4.25 B). A high correlation between both
sTNFR subtypes could be shown over 96 hours (r = 0.96; p < 0.0001). Correlation between
different detected plasma mediators revealed a correlation between both soluble TNF
receptors and IL-6 levels (4.3.2.3) over 96 hours after blast exposure (r = 0.595; p = 0.0002
and r = 0.557; p = 0.0006 for p55 and p75 to IL-6, respectively).
0 3 6 9 12
0
25
50
75
100
125
0
50
100
150
200
250
300
24 48 72 96
trauma: sTNFR p55trauma: sTNFR p75sham control: sTNFR p55sham control: sTNFR p75
**** **
**
**
**
A)
time after blast exposure [h]
sTNF
R p5
5 [p
g/m
l] sTNFR p75 [pg/ml]
Results
B)
64
4.3.3 Infiltration of inflammatory cells
To further elucidate a possible inflammatory response to blast injury, we investigated whether
an infiltration of inflammatory cells into the BAL took place.
4.3.3.1 PMN infiltration
The analysis of the amount of different cell types in lavage fluids from traumatized rats,
isolated at different time points, may suggest an permanent increase in neutrophil (PMN)
infiltration into the alveoli, starting from 90 minutes after trauma on. However, significant
amounts of neutrophils were detected not until 6 and 12 hours after blast exposure followed
by a continuous decay within 96 hours (Fig. 4.26). The number of lymphocytes in the BAL fluid
did not vary significantly over time (data not shown). Figure 4.27 shows the corresponding
cytospins of the different BAL fluids. The cytospins of the non-traumatized sham controls
showed a quite homogeneous population of alveolar macrophages. Only very few
lymphocytes can be found, and no PMN (Fig. 4.27 A). At 24 hours post-trauma the PMN were
as frequent as the alveolar macrophages. The alveolar macrophages were carrying
Figure 4.25: Time course of sTNFR p55 and p75 BAL concentrations in A) as well as the p55/ p75 ratio in B). The animals were sacrificed 10 min (n = 6), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours (n = 3) after blast exposure, non-traumatized animals served as sham controls (n = 9). Levels of sTNFR p55 and p75 were assessed in BAL fluids. Data were analysed by One-way ANOVA and Dunnett's Multiple Comparison Test: * p < 0.05 and ** p < 0.01 vs. sham control. Unpaired t-test was performed to compare differences in p55 and p75 levels at different time points: **p = 0.0074 for p75 vs. p55 and * p = 0.04 for p75 versus p55 at 24 hours and 96 hours after blast, respectively. Data are means ± SEM, number of experiments (n) in parentheses. Linear regression between p55 and p75 release revealing a Pearson r of r = 0.96; p < 0.0001.
0 3 6 9 12
0.0
0.1
0.2
0.3
0.4
0.5
24 48 72 96
sham
con
trol
****
** *
time after blast exposure [h]
ratio
sTN
FR p
55/ p
75
Results
intracellularly high amounts of erythrocytes due to the important alveolar haemorrhage (Fig.
4.27 B).
Fe
W
c
e
4
T
w
C
i
I
i
100
65
igure 4.27: Cytospin pictures after blast exposure. A) sham control, B) 24 hours after blast xposure. AM: alveolar macrophages; PMN: neutrophils; Lym: lymphocytes; RBC: red blood cells.
ith respect to a possible post-traumatic immunosuppression, we quantified the white blood
ell counts, revealing no statistically significant differences within 96 hours following blast
xposure (data not shown).
.3.3.2 CINC-3 measurement in the BAL fluids
o elucidate the role of chemokines in the thoracic trauma-induced infiltration of neutrophils,
e measured the α-chemokine CINC-3 (chemokine-induced neutrophil chemotactic factor,
INC). CINC-3 is one of three functional rat homologues to human IL-8 and plays an
mportant role in an animal model of acute lung injury induced by intrapulmonary deposition of
gG immune complexes 170. The CINC-3 levels in the BAL fluids of traumatized rat lungs were
ncreased 6 hours after trauma and returned to sham control levels after 96 hours. The time
Figure 4.26: Time-course of PMN infiltration into the alveoli after thoracic trauma. The animals were sacrificed 10 min (n = 6), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours (n = 3) after blast exposure, non-traumatized animals served as sham controls (n = 9). Statistical analysis was performed by One-way ANOVA and Dunnett's Multiple Comparison Test: * p < 0.05 vs. sham control. Data are expressed as mean ± SEM, number of experiments (n).
A)
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
20
40
60
80
time after blast exposure
**
% B
AL n
eutro
phils
Results
course of the CINC-3 release correlated with the infiltration of neutrophils into the alveolar
space (r = 0.63, p = 0.0007) (Fig. 4.28).
4
W
i
o
k
l
r
b
G
l
b
a
N
f
T
t
e
Fp(wv
500 **
66
.3.3.3 Matrix metalloproteinase activity
ith regard to the observed neutrophil infiltration and extracellular matrix remodelling, we
nvestigated the release and activation of the matrix metalloproteinases (MMP)-2 and MMP-9
ver time after thoracic trauma. Gelatinolytic bands of approximately 134, 92, 85, 72, and 66
Da were detected in BAL fluids (Fig. 4.29). These bands correspond to the pro-MMP-9
ipocalin complex, pro-MMP-9, active form of MMP-9, pro-MMP-2, and active form of MMP-2,
espectively (according to Moritaka and coworkers, 161). Within the first 24 hours following
last exposure, intense lytic bands corresponding to pro – and active MMP-2 were detected.
elatinolytic bands corresponding to MMP-9 and coexpressed bands of the pro-MMP-9
ipocalin complex were detected after six hours and weak after 12 and 24 hours, whereas lytic
ands equivalent to active MMP-9 were only barely detected at these time points. In addition,
weak gelatinolytic band corresponding to active MMP-9 appeared initially after trauma.
either pro- nor active MMP-2 or MMP-9 were detectable after 96 hours and in BAL fluids
rom non-traumatized sham controls, respectively.
he MMP-9 activity after six hours correlated with the increased neutrophil infiltration at this
ime point (4.3.3.1). MMP-2 is reported to be preferentially secreted by fibroblasts and
pithelial cells 171 and may therefore be released after trauma-induced cellular damage.
igure 4.28: CINC-3 measurement in the BAL fluid of traumatized rat lungs at different time oints after blast exposure: 10 min (n = 6), 1.5 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n=3), 24 h n = 3) and 96h (n = 3). Non-traumatized animals served as sham controls (n = 9). Statistical analysis as performed by One-way ANOVA (p = 0.0014) and Dunnett's Multiple Comparison Test: ** p < 0.01 s. sham control. Data are expressed as mean ± SEM, number of experiments (n).
sham
contro
l
10min
1.5h 3h 6h 12
h24
h96
h0
100
200
300
400
time after blast exposure
CIN
C-3
[pg/
ml]
Results
67
Furthermore, increased neutrophil related myeloperoxidase (MPO) activity was determined in
BAL fluid investigated 12 after blast exposure (p < 0.01), as compared to non-traumatized
controls (12 h: 0.43 ± 0.24 relative units, n = 4 and sham controls: 0.07 ± 0,004 relative units,
n = 9). This elevated MPO activity may related with the infiltration of neutrophils into the
alveolar space (4.3.3.1).
Figure 4.29: Gelatin zymograms of BAL fluids from traumatized rats and controls. Gelatin zymogram of BAL fluids from animals sacrificed 10 min (n = 5), 1.5 h (n = 3), 3 h (n = 3), 6 h (n = 3), 12 h (n = 4), 24 h (n = 3) or 96 hours (n = 3) after blast exposure, and from non-traumatized sham controls (n = 8). Gelatinolytic bands of approximately 134, 92, 85, 72, and 66 kDa correspond to the pro MMP-9 lipocalin complex, pro-MMP-9, active form of MMP-9, pro-MMP-2, and active form of MMP-2, respectively. Purified pro-MMP-9 and pro-MMP-2 were used in the concentrations of 0.1 ng and 1 ng, respectively were used simultaneously as positive controls for gelatin zymographic analysis of BAL fluid samples to standardize the measurement results.
pro-MMP-2 (72kDa)active MMP-2 (66kDa)
pro-MMP-9 (92kDa)/ active MMP-9 (85kDa)
lipocalin complex (134kDa)
pro-
MM
P-9
pro-
MM
P-2
6h3h1.5
h
10m
in
sham
con
trol
12h
24h
96h Mw
(kDa)
time after blast exposure
pro-MMP-2 (72kDa)active MMP-2 (66kDa)
pro-MMP-9 (92kDa)/ active MMP-9 (85kDa)
lipocalin complex (134kDa)
pro-
MM
P-9
pro-
MM
P-2
6h3h1.5
h
10m
in
sham
con
trol
12h
24h
96h Mw
(kDa)
time after blast exposure
Results
68
4.3.3.4 Summary of time-dependent BAL-findings
time course in vivo after blast injury
read out peak/
minimum
maximal
recovery conclusions
total protein content 1.5 h 96 h
alveolar
haemorrhage 1.5 h 96 h
LDH activity 10 min 96 h
disrupted alveolar-
capillary barrier/
cell death
wet/ dry ratio 1.5 h 6 h pulmonary infiltrates
TxB2 10 min 3 h
6-keto PGF1α 10 min 3 h early prostanoid release
nitrite/ nitrate 12 h > 96 h constitutive NO release
TNF α 12 h 96 h
IL-6 6 h 96 h
pro-inflammatory
cytokine release
IL-10 10 min 96 h early decrease
CINC-3 6 h 96 h pro-inflammatory
chemokine release
sTNFR p55/ p75
ratio 10 min 24 h
anti-inflammatory
counterregulation
neutrophil infiltration 6 - 12 h > 96 h
10 min 96 h MMP-2
MMP-9 6 h 96 h
MPO 12 h 96 h
inflammation
time-
depe
nden
t rec
over
y
Table 4.6: upregulation, downregulation (compared to non-traumatized sham controls).
Results
69
4.4 Ex vivo lung perfusion: Trauma-induced changes in lung function
To further assess and to characterize the physiological and functional changes after in vivo
thorax trauma, we combined our blast trauma model with our ex vivo isolated perfused rat
lung model, allowing the assessment of physiological lung function parameters without
interference of other organs.
4.4.1 Interrelationships between physical and physiological injury
The pressure peak decayed rapidly as it expanded from the blast wave generator (described
in the chapter 4.1.1.2) and therefore theoretically allowing rats exposure to different blast
intensities by varying the distance between the blast wave generator and the rat. Therefore,
we investigated whether physical and biological impact match in this setting.
Pathological evaluation:
The animals were subjected to a blast pressure wave with the tip of the blast nozzle located
either 3.5, 5, or 7 cm above the sternum. The alveolar haemorrhage showed a marked
increase in rats positioned at 3.5 cm distance below the nozzle, as compared to non-
traumatized control lung (Fig. 4.30 A, Tab. 4.8). The red blood cell counts correlated not only
with the distance between the animal and the nozzle (r = - 0.49, p = 0.033), but also with the
particular defined injury score (p = 0.011, r = 0.565) for each group (described in 3.4.5). The
latter correlation underscores the validity of this macroscopically examined injury score (Fig.
4.30 B, Tab. 4.8).
Results
sham
contro
l7 c
m5 c
m3.5
cm
2.0×10 06
4.0×10 06
6.0×10 06
8.0×10 06
1.0×10 07
**
distance belowthe nozzle
A)R
BC
s/ m
l BA
L flu
id
2 4 6 8 10 12 14
5.0×10 06
1.0×10 07
1.5×10 07
2.0×10 07
B)
haemorrhage score
RB
Cs/
ml
Figure 4.30: Distance-dependent alveolar haemorrhage. A) alveolar haemorrhage expressed as red blood cells (RBCs) per ml BAL fluid and assessed after 150 minutes perfusion time and B) RBCs/ haemorrhage score correlation. The animals were located either 3.5 (n = 12), 5 (n = 4), or 7 cm (n = 3) distance from the nozzle, non-traumatized animals served as sham controls (n = 5). Statistical analysis was performed on A) by One-way ANOVA and Dunnett's Multiple Comparison Test: ** p < 0.01 vs. sham control. Linear regression revealed a Pearson r of r = - 0.49, p = 0.033. Data are expressed as mean ± SD, number of experiments (n) and B) by correlating RBCs with the score and linear regression revealing a Spearman r of r = 0.565.
F
(
f
s
c
t
s
T
Ov
70
urthermore pulmonary injury, quantified by lung wet weight (LWW)/ body weight (BW) ratio
LWR), was significantly increased at 3.5 cm distance below the nozzle, indicating oedema
ormation (Tab. 4.7) in these lungs. In addition, the individually defined oedema score showed
ignificant higher values in the 3.5 and 5 cm group compared to non-traumatized sham
ontrols (Tab. 4.8). Comparison of the calculated injury quotients (Qi) revealed a Qi of 1.94 for
he 3.5 cm group, 1.31 for the 5 cm group and 1.20 for the 7 cm group, indicating “very
evere“, “moderate” and “minor” lung injury, respectively (Tab. 4.7) 162.
able 4.7: Lung wet weight to body weight ratio at varying distances from the nozzle.
distance n BW [g] LWW [g] LWR Qi
sham control 4 269 ± 30 1.83 ± 0.13 0.0069 ± 0.0013
3.5 cm 3 243 ± 6 3.21 ± 1.25 * 0.0130 ± 0.0053 * 1.94
5 cm 5 241 ± 6 2.14 ± 0.23 0.0089 ± 0.0009 1.31
7 cm 3 238 ± 12 1.94 ± 0.06 # 0.0082 ± 0.0006 # 1.20
ne-way ANOVA and Tukey's Multiple Comparison Test: # p < 0.05 vs. 3.5 cm and * p < 0.05 s. sham control. Data are expressed as mean ± SD, number of experiments (n).
Results
Table 4.8: Selected results from exposure to graded blast waves.
distance RBCs x 106/ ml haemorrhage score oedema score
sham control 0.12 ± 0.15 (5) 0 ± 0 (5) 0 ± 0 (4)
3.5 cm 7.13 ± 4.72 (12) ** 9.6 ± 2.2 (12) *** 10.0 ± 3.6 (3) ***
5 cm 4.68 ± 3.11(4) 8.3 ± 2.1 (4) *** 7.2 ± 1.9 (5) **
7 cm 1.33 ± 0.44 (3) 5.7 ± 3.1 (3) ** # 4.0 ± 1.4 (3) #
Lung function parameters:
The initial tidal volume (Tv) and therefore the compliance (CL) (data not shown) of the lungs
immediately after blast, obtained with standard ventilation pressures (PEEP/ PIP: -2/ -7 cm
H2O) was significantly decreased in the 3.5 and 5 cm distance group. (Tv: 3.5 cm: 0.98 ± 0.35
ml, 5 cm: 1.33 ± 0.52 ml, and 7 cm: 1.72 ± 0.5 ml), as compared to the non-traumatized sham
controls (1.95 ± 0.33 ml) (Fig. 4.31). The decrease in initial Tv correlated with the distance
below the nozzle (r = 0.58, p = 0.0005), indicating that thoracic trauma deteriorates the lung
function depending on the pressure wave intensity.
As already mentioned above (described in d
used a negative pressure ventilation (PEEP/
With these ventilation pressures tidal volu
sham
contro
l7 c
m5 c
m3.5
cm0.0
0.5
1.0
1.5
2.0
2.5
distance belowthe nozzle
**
*
Tv [m
l]
One-way ANOVA and Tukey's Multiple Comparison Test: ** p < 0.01, *** p < 0.001 vs. sham control; # p < 0.05 vs. 3.5 cm. Data are expressed as mean ± SD, number of experiments (n) in parentheses.
Figure 4.31: Pressure wave intensity-related decrease in initial tidal volume after thoracic trauma. Rats were exposed to the pressure wave at different distances from the nozzle (3.5 cm, n = 9; 5 cm, n = 16; 7 cm, n = 7). The rat lungs were perfusedimmediately after blast. Non-traumatized animals served as sham controls (n = 7). The initial tidal volume (Tv) was assessed with standard ventilation pressures (PEEP/ PIP: -2/ -7 cm H2O). Data are expressed as mean ± SD, number of experiments (n). Statistical analysis was performed by One-way ANOVA and Dunnett's Multiple Comparison Test: * p < 0.05 and ** p < 0.01 vs. sham control. Correlation between distance and Tv was performed by linear regression revealing a Pearson r of r = 0.58, p = 0.0005.
71
etail in the chapter “Materials and Methods”) we
PIP: -2/ -7 cm H2O) in our lung perfusion model.
mes of 1.95 ± 0.33 ml are obtained in non-
Results
72
traumatized control lungs (Fig. 4.31). The ventilation pressures in traumatized lungs were
adjusted in order to obtain a minimal vital ventilation of 1 ml tidal volume. Rats exposed to
blast pressure wave at a distance of 3.5 cm needed a significantly higher inspiratory pressure
PIP) to achieve 1 ml tidal volume than non-traumatized controls (Tab. 4.9).
Lung function parameters of traumatized rat lungs measured at the end of 150 minutes
perfusion time were significantly deteriorated in the 3.5 cm distance group, as compared to
non-traumatized controls with respect to tidal volume (TV) (Tab. 4.9), airway resistance (RA)
(Fig. 4.32, Tab. 4.9), and also lung weight gain (ΔW) (Fig. 4.32, Tab. 4.9). The vascular
parameters showed no significant differences (data not shown). The comparison of the airway
resistance and the lung weight gain of the different groups revealed a distance-dependency
(Tab. 4.9). This was not the case for the tidal volume; despite the correlation between distance
and initial tidal volume deterioration, at the end of perfusion no distance-dependency could be
measured. The following experiments were all done at a distance of 3.5 cm below the nozzle.
Figure 4.32: Bronchoconstriction and pulmonary oedema ex vivo as a function of distance between rat thorax and blaster nozzle. Rats were exposed to the pressure wave at different distances from the nozzle (3.5 cm, 5 cm, and 7 cm). Immediately after blast the lung perfusion was started. Non-traumatized animals served as sham controls. Data are expressed as mean ± SEM. A) RA/ RA0min: airway resistance and B) ΔW: weight gain were all normalized to the value at t = 0 min.
0 20 40 60 80 100 120 140
1.0
1.2
1.4
1.6
1.8
trauma: 5 cm distancetrauma: 7 cm distance
trauma: 3.5 cm distance
sham control
A)
time [min]
RA/R
A0m
in
0 20 40 60 80 100 120 140
0
250
500
750
1000
1250
trauma: 5 cm distancetrauma: 7 cm distance
trauma: 3.5 cm distance
sham control
B)
time [min]
∆ ∆∆∆W
[mg]
Results
73
Table 4.9: Thoracic trauma-induced deterioration of lung function parameters.
in vivo trauma ex vivo perfusion
~ -15 min ~ 3 min 150 min 150 min 150 min
distance PIP
(cm H2O)
Tv
(ml)
RA
(cm H2O*s/ ml)
ΔW
(mg)
sham
control
7 ± 0
(7)
1.60 ± 0.15
(7)
0.33 ± 0.05
(7)
579 ± 184
(6)
3.5 cm 8.36 ± 1.36 *
(16)
0.66 ± 0.21 ***
(13)
0.47 ± 0.15 *
(15)
1099 ± 441 **
(15)
5 cm 7.31 ± 0.64 #
(11)
0.68 ± 0.23 ***
(11)
0.34 ± 0.05 #
(10)
723 ± 158 #
(9)
7 cm 7.07 ± 0.07 #
(7)
0.90 ± 0.31 ***
(7)
0.29 ± 0.02 ##
(7)
789 ± 114
(6)
4.4.2 Time-dependent recovery of the lung function after trauma
With regard to the reduced wet to dry weight ratios assessed in vivo from three hours after
blast exposure on, we further investigated whether the pulmonary oedema formation and the
deteriorated lung function observed ex vivo initially after blast is also a function of time.
Therefore, the animals were subjected to a blast wave injury at a distance of 3.5 cm, and
sacrificed 10 minutes, three hours and six hours after trauma. Subsequently lungs were
perfused over 150 minutes.
Pathological evaluation:
As expected and in accordance with the results obtained in vivo (4.3.1.2), the red blood cell
counts examined after 150 minutes perfusion time did not significantly differ within the three
Rats were exposed to the pressure wave at different distances from the nozzle (3.5 cm, 5 cm,
and 7 cm). Immediately after blast, lung perfusion was started and the lung function parameters
were recorded. Non-traumatized animals served as sham controls. Inspiratory pressure (PIP),
tidal volume (Tv), airway resistance (RA) or weight gain (ΔW). Data are expressed as mean ± SD,
number of experiments (n) in parentheses. One-way ANOVA and Tukey's Multiple Comparison
Test was performed: * p < 0.05, ** p < 0.01, *** p< 0.001 vs. sham control, and # p < 0.05, ## p <
0.01 vs. 3.5 cm, respectively
Results
10 m
in 3 h 6 h0.0
0.5
1.0
1.5
2.0
time after blastexposure
**
**
Tv [m
l]
groups (10 minutes: 7.13 ± 4.72 x 106/ ml (n = 12), 3 h: 6.74 ± 2.71 x 106/ ml (n = 4), 6 h: 10.9
± 7.65 x 106/ ml (n = 3)).
Lung function parameters:
Linear correlation showed that the initial tidal volume (Tv) obtained with standard ventilation
pressures (PEEP/ PIP: -2/ -7 cm H2O) was improved depending on the time after blast
exposure (r = 0.74, p < 0.0001). Thus, the initial tidal volume was significantly improved 3 and
6 hours after blast exposure, as compared to immediately perfused traumatized lungs (10min:
0.98 ± 0.35 ml, 3 h: 1.60 ± 0.29 ml, 6 h: 1.85 ± 0.35 ml) (Fig. 4.33). Within six hours after the
blast the tidal volume recovered and reached sham control levels (1.95 ± 0.33 ml), indicating
that some kind of repair takes place in vivo over time. These data are in line with the improved
compliance (CL) over time (data not shown).
Due to this time-dependent amelioratio
necessary inspiratory pressure (PIP) to
and 6 hours after blast as compared to
significant improved initial tidal volume
compared to immediately perfused lung
volume (Tv) nor in airway resistance (R
of perfusion (Tab. 4.10).
Figure 4.33: Time-dependent improvement of tidal volume after thoracic trauma. Rats were exposed to the pressure wave at a distance of 3.5 cm from the nozzle. The rats were sacrificed either 10 minutes (n = 16), 3 hours (n = 7) or 6 hours (n = 7) following the blast. Subsequently lung perfusion was started. The initial tidal volume (Tv) was assessed at standard ventilation pressures (PEEP/ PIP: -2/ -7 cm H2O). Data are expressed as mean ± SD, number of experiments (n). Statistical analysis was performed by One-way ANOVA and Dunnett's Multiple Comparison Test: ** p < 0.01 vs. 10 min. Correlation between time after blast and Tv was performed by linear regression revealing a Pearson r of r = 0.74, p < 0.0001.
74
n of the respiratory mechanics following blast injury, the
achieve 1 ml tidal volume was significantly reduced 3
immediately perfused lungs (Tab. 4.10). Despite of the
(Tv) in lungs perfused three and six hours after trauma
s (10 minutes), no significant difference neither in tidal
A) between the groups could be measured at the end
Results
75
Table 4.10: Lung function assessed ex vivo at different time points after blast injury.
in vivo trauma ex vivo perfusion
~ -15 min 0 min 150 min 150 min 150 min
time
after blast
PIP
(cm H2O)
Tv
(ml)
RA
(cm H2O*s/ ml)
ΔW
(mg)
10 min 8.36 ± 1.36
(16)
0.66 ± 0.21
(13)
0.47 ± 0.15
(15)
1099 ± 441
(15)
3 h 7.07 ± 0.11
** (8)
0.83 ± 0.31
(7)
0.36 ± 0.07
(7)
826 ± 293
(8)
6 h 7.09 ± 0.08
* (8)
0.76 ± 0.34
(6)
0.38 ± 0.09
(6)
855 ± 311
(8)
Comparison of the entire curves data from the different groups showed a reduced weight gain
3 and 6 hours after blast, as compared to immediately perfused lungs (Fig. 4.34, Tab. 4.11).
However, analysis of the lung weight values assessed at the end of perfusion (Tab. 4.10)
revealed no significant differences between the groups. Whether the decrease of the weight
gain is due to an increased oedema resorption and / or a stop in oedema generation over time
in these lungs can not be determined by the used setting. Nevertheless, the reduced weight
gain did not reach control levels (∆ W: 579 mg ± 184 mg). The macroscopically defined
oedema score correlated with the time after blast exposure (r = - 0.85, p < 0.0001) and was
significantly decreased three and six hours after blast compared to recently injured lungs (3 h:
1.1 ± 1.9, n = 8; 6 h: 0.6 ± 1.5, n = 7; and 10 minutes: 10.1 ± 2.4, n = 16), thus suggesting a
recovery in vivo over time.
Rats were exposed to the pressure wave at a distances of 3.5 cm from the nozzle. The rats were sacrificed either 10 minutes, 3 hours or 6 hours following the blast. Subsequently lung perfusion was started. Inspiratory pressure (PIP), tidal volume (TV), airway resistance (RA), weight gain (ΔW). Data are expressed as mean ± SD, number of experiments (n). One-way ANOVA and Dunnett's Multiple Comparison Test were performed: * p < 0.05, ** p< 0.01 vs. 10min.
Results
4
W
in
w
is
4
D
s
a17
1250
76
ex vivo ΔW
in vivo blast 3 h 6 h
+ 10 min *** ***
+ 3 h *
.4.3 Pharmacological intervention
ith regard to the observed time-dependent “mixed” oedema generation and fluid resorption
vivo after pressure wave exposure, we further examined whether active sodium transport,
hich is reported to be the primary mechanism that activates alveolar fluid clearance in vivo,
involved (reviewed by Matthay and coworkers, 2002, 172).
.4.3.1 The role of the amiloride-sensitive sodium channels after trauma
epending on the species investigated, amiloride–sensitive sodium channels on the apical
ide of alveolar epithelial cells account for 40 to 80% of the sodium uptake 173. Since
miloride, in a species-dependent manner, inhibited 40 - 70% of basal alveolar fluid clearance 2 we used amiloride to examine the role of these sodium channels after trauma.
Figure 4.34, Table 4.11: Pulmonary oedema ex vivo as a function of time. Rats were exposed to the pressure wave at a distances of 3.5 cm from the nozzle. The rats were sacrificed either 10 minutes (n = 15), 3 hours (n = 8) or 6 hours (n = 8) following the blast. Subsequently lung perfusion was started. Data are expressed as mean ± SEM. Lung weight gain ΔW: was assessed over 150 minutes perfusion time. Statistical analysis of the entire curve data from different groups were compared by a Two-way ANOVA design. The p value represents the time dependent recovery after trauma: * p < 0.05 and *** p < 0.0001.
0 20 40 60 80 100 120 140
0
250
500
750
1000trauma: +3htrauma: +6h
trauma: +10min
time [min]
∆ ∆∆∆W
[mg]
Results
P
t
b
c
w
m
b
w
A) B)
Fdlpvf
77
erfusion of blasted rats` lungs with amiloride inhibited the endogenous fluid resorption in
hese lungs, resulting in a further increase of oedema formation, as compared to untreated
lasted lungs (Fig. 4.35 A, Tab. 4.12+13). These data suggest an involvement of sodium
hannels in fluid resorption during trauma. Similarly, tidal volume (Tv), airway resistance (RA)
ere deteriorated upon amiloride treatment (Fig. 4.35 B+C, Tab. 4.12+13). This aggravation is
aybe related to the massive oedema formation. The software only allows to calculate data
etween a defined minimal and maximal value. Therefore, the increase in airway resistance
as only recordable up to 80 minutes after start of perfusion (Fig. 4.35 C).
0 20 40 60 80 100 120 140
0
500
1000
1500
2000
2500
3000
3500trauma (+10min)trauma (+10min) + amiloride
***
time [min]
∆ ∆∆∆ W
[mg]
0 20 40 60 80 100 120 140
0.2
0.4
0.6
0.8
1.0
trauma (+10min)trauma (+10min) + amiloride
***
time [min]
Tv/T
v 0m
in
0 20 40 60 80 100 120 140
1.0
1.2
1.4
1.6
1.8
2.0
trauma (+10min)trauma (+10min) + amiloride
***
C)
time [min]
RA/R
A0m
in
igure 4.35: Role of sodium-channels after trauma. Rats were exposed to the pressure wave at a istance of 3.5 cm from the nozzle. The rats were sacrificed 10 minutes (n = 24) after the blast. The
ungs were treated either with (n = 8) or without (n = 16) amiloride (10-4 M) 4 minutes after start of erfusion. Data are expressed as mean ± SEM. A) ΔW: weight gain, B) Tv/ Tv0min: normalized tidal olume, and C) RA/ RA0min: normalized airway resistance. Statistical analysis of the entire curve data rom two groups were compared by a Two-way ANOVA design: *** p < 0.0001 (Tab. 4.13).
Results
78
4.4.3.2 The role of 2-adrenergic receptors after trauma
Stimulation of β2-adrenergic receptors in intact lungs, in vivo and ex vivo by synthetic agonists
(terbutaline, salmeterol, isoproterenol) and endogenous or exogenous epinephrine
respectively, was reported to increase fluid clearance 7,10,11. In addition, this effect is reported
to occur rapidly after administration of the substances and is completely blocked by unspecific
(propranolol) or specific β2-receptor antagonists 7,22. Therefore, we used the β2-adrenergic
receptor agonists terbutaline and formoterol to examine on the one hand the role of β2-
adrenergic receptors after blunt chest trauma and on the other hand the possible therapeutic
potential of these substances.
In these experiments, thoracic trauma-related deterioration of the lung parameters was
markedly improved by terbutaline and formoterol with respect to tidal volume (Tv), airway
resistance (RA) and weight gain (∆W) (Fig. 4.36 A-C, Tab. 4.12+13). With regard to the weight
gain of blasted rat lungs during perfusion, the terbutaline-induced reduction reached control
levels of non-traumatized lungs (∆W: 559 ± 368 mg and 579 ± 184 mg for traumatized rat
lungs plus terbutaline treatment and sham controls, respectively) (Tab. 4.12).
Taken together, these data indicate that β2-agonist treatment improves the lung weight and
the lung function parameters after blast exposure.
The terbutaline-induced amelioration in tidal volume (Tv) and airway resistance (RA) was
completely blocked by the unspecific β-receptor antagonists propranolol (Tab. 4.12+13). The
oedema formation was even more impaired than in non-treated blasted rat lungs (Tab.
4.12+13).
Amiloride blocked the terbutaline-related decrease in lung weight (Tab. 4.12+13), indicating
that β2-receptor related stimulation is dependent on amiloride-sensitive sodium transport, as
also proposed by several publications 8,22. However, statistical analysis by Two-way ANOVA
yielded also a significant difference between terbutaline plus amiloride versus amiloride
treatment alone, suggesting the implication of an amiloride-insensitive sodium transport.
As expected, and in contrast to the weight gain, amiloride did not influence the terbutaline-
induced improvement of the tidal volume (Tv), airway resistance (RA) (Tab. 4.12+13) which
thus may be considered as sodium channel independent β2-adrenergic effects.
Results
Ffw(4Ar*
A) B)
79
igure 4.36: Modulation of the trauma-induced pulmonary dysfunction by terbutaline and ormoterol. Rats were exposed to the pressure wave at a distances of 3.5 cm from the nozzle. The rats ere sacrificed 10 minutes (n = 37) following the blast. The lungs were perfused either untreated
n = 16) or treated with terbutaline (100 µM ) (n = 9) and formoterol (1 nM) (n = 12), respectively minutes after start of perfusion. Data are expressed as mean ± SEM. ) ΔW: weight gain, B) Tv/ Tv0min: normalized tidal volume and C) RA/ RA0min: normalized airway
esistance were monitored over 150 minutes perfusion time. Two-way ANOVA analysis: ** p < 0.0001 vs. trauma (+ 10 min) (Tab. 4.13).
0 20 40 60 80 100 120 140
0
250
500
750
1000
1250
1500trauma (+10min)trauma (+10min) + terbutalinetrauma (+10min) + formoterol
***
***
time [min]
∆ ∆∆∆W
[mg]
0 20 40 60 80 100 120 140
0.4
0.6
0.8
1.0
trauma (+10min)trauma (+10min) + terbutalinetrauma (+10min) + formoterol
***
***
time [min]
Tv/T
v 0m
in
0 20 40 60 80 100 120 140
0.8
1.0
1.2
1.4
1.6
1.8
trauma (+10min)trauma (+10min) + terbutalinetrauma (+10min) + formoterol
***
***
C)
time [min]
R A/R
A0m
in
Results
80
Table 4.12: Pharmacological intervention: Role of amiloride-sensitive sodium channels and 2-adrenergic receptor modulation.
in vivo trauma ex vivo perfusion
~ -15 min ~ 4 min 150 min 150 min 150 min
treatment Tv
(ml)
RA
(cm H2O*s/ ml)
ΔW
(mg)
sham control 1.60 ± 0.15
(7)
0.33 ± 0.05
(7)
579 ± 184
(6)
0.66 ± 0.21
(13) §§§
0.47 ± 0.15
(15) §
1099 ± 441
(15) §
+ amiloride 0.56 ± 0.09
(4)
1.60 ± 0.46
(5) *** ⊗
2429 ± 2265
(8) *
+ terbutaline 1.08 ± 0.26
(9) ***
0.33 ± 0.04
(9) **
559 ± 368
(8) **
+ formoterol 1.12 ± 0.34
(12) ***
0.32 ± 0.04
(12) **
827 ± 381
(12)
+ terbutaline
+ propranolol
0.89 ± 0.51
(3)
0.40 ± 0.12
(3) #
3378 ± 2779
(5) ***, #
trauma
+ terbutaline
+ amiloride
1.09 ± 0.61
(4) *
0.35 ± 0.12
(4)
1534 ± 799
(4) #
Rats were exposed to the pressure wave at a distances of 3.5 cm from the nozzle. The rats were sacrificed 10 minutes (n = 55) following the blast. After preparation of the lungs, the blood-free perfusion was started and the lung function parameters were recorded. The lungs were perfused either untreated (n = 16) or treated with amiloride (10-4 M) (n = 8), terbutaline (10-4 M ) (n = 9), formoterol (1 nM) (n = 12), terbutaline + propranolol (10-4 M) (n = 5) and terbutaline + amiloride (n = 5) respectively 4 minutes after start of perfusion. Non-traumatized animals served as sham controls (n = 7). Data are expressed as mean ± SD and represent the values assessed after t = 150 minutes perfusion time (except ⊗: value at t = 80 minutes). Data were analysed by an unpaired t-test: § p < 0.05 and §§§ p < 0.001 vs. sham control; * p < 0.05, ** p < 0.01 and *** p < 0.001 vs. trauma; # p < 0.05, ## p < 0.01 and ### p < 0.001 vs. trauma + terbutaline.
Results
81
Table 4.13: Statistical analysis of different pharmacological interventions.
Tv
(ml)
RA
(cm H2O*s/ ml)
ΔW
(mg)
treatment tra
uma
+ te
rbut
alin
e
+ am
ilorid
e
traum
a
+ te
rbut
alin
e
+ am
ilorid
e
traum
a
+ te
rbut
alin
e
+ am
ilorid
e
+ amiloride *** *** ***
+ terbutaline *** *** ***
+ formoterol *** *** *** *** *** ***
+ terbutaline
+ propranolol ns *** ns *** *** ***
+ terbutaline
+ amiloride *** ns *** *** ns *** *** *** **
Statistical analysis of the entire curve data from two groups were compared by a Two-way ANOVA design: The analysed condition was the pharmacological modulation during perfusion: ** p < 0.01, *** p < 0.0001 and p > 0.05 was considered to be not significantly different.
Results
82
Table 4.14 illustrates the role of amiloride-sensitive sodium channels and 2-adrenergic
receptor modulation during trauma.
in vivo trauma ex vivo perfusion
~ -15 min ~ 4 min 150 min 150 min 150 min
treatment Tv
(ml)
RA
(cm H2O*s/ ml)
ΔW
(mg)
sham control ↔ ↔ ↔
+ amiloride ↔
+ terbutaline
+ formoterol
+ terbutaline
+ propranolol ↔ ↔
trauma
+ terbutaline
+ amiloride ↔ ↔
Table 4.14: ↔ no change, upregulation, downregulation (compared to sham
control or trauma without treatment respectively).
Discussion
83
5. Discussion
The present study consists of three parts, with the primary aim to optimise a blast wave injury
model in order to study primary lung injury in terms of lung physiology, biochemistry and
immunology. The blast trauma model is intended to reproduce the clinical spectrum of injuries
seen in blast victims and is therefore used for studying the pathophysiology and the potential
treatment of thorax trauma in rats. Three approaches for studying the correlation between
clinically relevant physical blast properties and its biological impact were taken.
In the first approach, we assessed and characterized the functional consequences of in vivo
thorax trauma by means of combining the in vivo trauma model with the ex vivo isolated
perfused rat lung model. These studies included the investigation of pharmacological
interventions as to their therapeutic potential.
In the second approach, we examined the pathophysiological consequences including
biochemical responses of the lung following blast injury in vivo over time.
The third approach addresses immunodeficiency after thoracic trauma, which results in a high
number of infections. Due to its key role as modulator of pulmonary inflammation, the function
of the alveolar macrophage was assessed in vitro as to its phagocytic capacity, respiratory
burst and mediator release. These different approaches will be discussed separately
(summarized in Figure 5).
in vivo blast thorax trauma• standardization• monitoring• pressure wave intensity injury
ex vivo lung perfusion• lung function• weight gain• therapeutical
interventionin vivometabolism
in vitroimmune status
primary alveolar macrophage function
pathophysiological consequences
5.1
5.2 5.35.4
in vivo blast thorax trauma• standardization• monitoring• pressure wave intensity injury
ex vivo lung perfusion• lung function• weight gain• therapeutical
interventionin vivometabolism
in vitroimmune status
primary alveolar macrophage function
pathophysiological consequences
5.1
5.2 5.35.4
Discussion
84
5.1 A laboratory model for studying primary blast injury
Recently, the management of blast injured patients has become a problem not only for civilian
trauma surgeons, but also for military physicians, due to both an increase in the number of
accident-related blunt trauma and an increase in terrorist activity. Blast wave injury leads to a
unique but poorly understood spectrum of injuries 119. One of the cardinal clinical problems in
the early posttraumatic phase are the missing clinical signs of injury 114,115 and therefore the
outcome at this stage is unpredictable. Thus, some patients may present acute damage, while
others appear uninjured, but develop respiratory failure after 12 - 24 hours 128. Damage
caused by the pressure wave alone (primary blast injury) is not commonly seen after air-blast,
since most of the casualties are additionally affected by secondary and tertiary injuries.
However, primary blast injuries are estimated to contribute to 47 - 57% of the injuries in
survivors and to 86% of fatal injuries 99. Therefore, studying primary blast injury implies the
following demands: 1. discharge of high energy pressure waves comparable with high energy
chemical explosives, 2. practicable in a safe laboratory environment, 3. high reproducibility
and 4. reproducing the spectrum of injuries seen in blast victims.
5.1.1 Rationale for the development of the blast thorax trauma rat lung model
As already described in the chapter “Introduction”, the lungs are almost always affected by
blast injuries 103,107-109. Furthermore, it has been widely shown that the involvement of the
thorax in polytrauma patients is a major negative determinant for the long-term consequences
after trauma 93,104,112. This emphasizes the need for further basic understanding of the
pathogenesis especially of the lung. Therefore, we used the primary blast injury model
previously developed by Irwin and coworkers 117 to study primary lung injury (the blast wave
generator is described in detail in the chapter “Materials and Methods”). This model develops
a mechanical explosive that simulates blast pressure waves from high explosives and
produces the types of injuries commonly seen in blast victims.
5.1.2 Standardization and monitoring of the blast pressure wave
Attempts to further standardize the pressure wave-induced injury were successfully
undertaken to improve the reproducibility.
Different wave types, characterized by the rate of energy application at the impact side and
the degree of compression produced, have different capacities to injure internal organs 106.
Thus, we further modified the blast wave generator to guarantee a standardized, fast and
complete rupture of the diaphragm and therefore a fast discharge of the blast pressure wave.
Discussion
85
This was achieved by two modifications: First, by using an additional compressed air bottle
located as close as possible to the pressure reservoir, and second by pressing the diaphragm
along a predetermined breaking point between the pressure reservoir and the nozzle, instead
of only fixing it with screws.
We further installed pressure transducers at different positions, including the pressure
reservoir, at the right and left side at the rat thorax level. This Setup allowed a thorough
monitoring and evaluation of the key physical blast wave properties and a comparison of the
data over time. Our blast waves are comparable in form and duration to blast waves from
other groups using such a Setup 116,117,124,174. However, our pressure wave monitoring at the
rat thorax level revealed a complex wave rather than a simple wave form (Friedlander wave
form) possibly due to reflections from the rat surface. Furthermore, a comparison of the data
from the two sensors situated on the right and left side of the rat suggests that the type of
turbulences of the pressure wave may be due to the confinement of the blast wave by
reflective surfaces of the nozzle. In addition, the achieved pressure peaks at comparable
distances and the similar spectrum of injuries are lower as compared to those obtained by
others 116,117,124,174. Because the exact position of the pressure transducer is not mentioned in
these studies, we can only speculate on another position than the one directly about the
thorax e.g. in the nozzle. Since complex wave forms are usually expressed by their impulse
(integral of pressure change over time) rather than by their maximum peak overpressure
values alone 102, we calculated the area under the pressure wave curve. The pressure
measured at the rat thorax level decayed rapidly as it expanded from the nozzle. Our
measured mean overpressure, i.e. the duration of the impact and the area under the curve
correlated significantly with the distance. This allows an exposure of the rats to different blast
intensities by simply varying the distance between the blast wave generator and the animals 116,117,124,174. The necessity of such a thorough monitoring becomes further apparent when
comparing the pressure wave data from survivors versus non-survivors, blasted at the same
distance from the nozzle. In the non-survivor group the rupture pressure of the diaphragm was
significantly higher than in the survivor group, resulting in a higher impact on the animal. Since
the Mylar polyester films show differences in their physical characteristics (supplier
information) and since different lots of the Mylar polyester films were used in the present
study, the observed variances in the rupture pressures may be attributed to these material
differences.
Discussion
86
5.1.3 Standardization of the blast thorax trauma in rats
Our rats were inhalation-anaesthetized and non-intubated during the blast pressure wave
exposure. This Setup is not only easy to handle but also displays the clinical situation and
avoids additional ventilation-related modulations during blast exposure. In addition, the
vagolytic response from the blast wave injury can be investigated. The disadvantage is the
lack of respiratory control and therefore the risk of prolonged apnoea and probably death.
With regard to a possible involvement of the breathing situation in the extent of the induced
lung injury, the animals were all blasted at the top of expiration. This was achieved by an
automatic triggering of the valve during spontaneous breathing at halothane anaesthesia.
However, the anesthetic has been shown to affect the cardiopulmonary physiology 175 and a
modulation of the autonomous nervous system cannot be ruled out. In some animals,
anaesthesia could not be achieved maybe because of stressing of the animals in advance.
Nevertheless, no correlation between the mortality and the reduced pre-blast breathing
frequency, with regard to a prolonged time of apnoea was observed. Mortality occurring
immediately after the blast pressure wave exposure was mostly due to vessel rupture.
Furthermore, air embolism is thought to be the predominant cause of the immediate death
after the blast wave injury 104,119,120. Because of the rapid air absorption in the capillaries, air
embolism is difficult to detect but was seen histologically in some cases. Recently it was
shown that air embolism presenting in blast victims is not a mere ventilation-induced artefact 119. Blast exposure was usually followed by an immediate period of apnoea. In line with the
findings of others our rats had a low breathing frequency immediately after the blast pursued
by fast shallow breathing 116,117,122,124,125,174. The characteristic triad of apnoea, bradycardia,
and hypotension has been attributed to a vagal reflex 124,125.
Taken together, despite technical variances we succeeded in establishing a reproducible,
standardized and well-monitored pressure wave exposure. Thus, this blast wave generator
allows a safe method to study primary blast injury without contact with the thoracic cage.
5.2 Combination of the in vivo thorax trauma model with ex vivo lung perfusion
The direct functional consequences of an in vivo thoracic trauma were assessed in our ex vivo
isolated perfused rat lung model, which has, to the best of our knowledge, not been described
previously. This model is a standardized and well-established tool in our laboratory 1,157,176. In
order to study primary lung injury, the isolated perfused rat lung represents a system much
less complicated than the whole animal, while preserving most of the integrity of the organ. As
an experimental approach it stands between in vivo and in vitro experiments.
Discussion
87
5.2.1 Match of physical and biological impact
The most striking pathological changes were pulmonary haemorrhage and oedema,
sometimes called “blast lung” 177, as determined by BAL red blood cell counts and ex vivo
weight gain or lung wet to lung body weight ratio and confirmed by histological examinations.
These two characteristics of “blast lung” were macroscopically quantified by lung injury scores
(haemorrhage and oedema score) that have been shown to posses high validity. Because the
air in the alveoli is easily compressible, blast pressure waves disrupt the alveolar capillary
membrane and blood is driven from the capillaries into the alveolar space by two mechanisms:
direct compression of the lung and transfer of the blast wave through the body, causing injury
by spalling, implosion and inertia 105,106. Alveolar haemorrhage and oedema formation are
common findings 117,118,122,174 and occurred regularly in our model with increasing intensities
with higher pressure wave intensities.
The ex vivo perfusion of the blasted rat lungs showed that thoracic trauma deteriorates the
lung function with respect to the airway parameters and leads to oedema formation,
depending on the distance from the nozzle and therefore on the pressure wave intensity. This
included not only the tidal volume measured immediately after the onset of the ventilation, but
also an increase of the airway resistance and the weight gain over the perfusion time. The
closer the animals were positioned to the nozzle, e.g. 3.5 cm versus 5 cm, the higher was the
necessary inspiratory pressure (PIP) to ventilate these lungs in order to achieve a vital tidal
volume of at least 1 ml. However, despite the correlation between the distance and the initial
tidal volume (Tv), at the end of the perfusion no distance-dependency could be measured.
Thus, we cannot exclude an involvement of the ex vivo ventilation in the observed changes
during perfusion. Our ventilatory strategy was based on the hypothesis that a minimal vital
tidal volume of 1 ml is necessary for survival of the animals. One has to take into account that
the isolated perfused rat lung model has been optimised for uninjured lungs, in terms of both
negative pressure ventilation (overpressure ventilation during surgical procedure) and
constant pressure perfusion 1,157. This is of importance, since the mechanical ventilation of an
injured lung may induce a secondary injury called “ventilator-associated lung injury”.
Mechanical ventilation is one of the ultimate life-supporting technologies in the therapy of
critically ill patients with respiratory failure. However, data accumulated over the past decade
provide strong evidence that ventilatory strategies associated with excessive end-inspiratory
stretch and/ or collapse/ recruitment of lung units can cause further injury and perhaps
promote the development of multi-organ failure 178-180. Forms of the ventilator-associated lung
injury are barotrauma, volutrauma, atelectotrauma, and biotrauma. In a clinical trial it has been
shown that mechanical ventilation with a lower tidal volume than the one traditionally used
results in decreased mortality and increases the number of days without ventilator use 98.
Discussion
88
Different ventilatory strategies (high PEEP versus low PEEP, conventional mechanical
ventilation versus high frequency ventilation) have been investigated by many authors in
different lung injury models 181-183. However, especially the interpretation of results from ex
vivo perfused lung models must take into account the fact that the degree of collapse and
reopening is magnified, because there is no chest wall and hence at a PEEP of 0,
transpulmonary pressure is also 0. This is not comparable with the in vivo situation.
Taken together, the correlation of pressure wave monitoring together with the injury score, the
BAL red blood cell counts and the ex vivo data collected in the isolated traumatized and
perfused lung indicate that physical and biological impact may be matched
5.2.2 Time-dependence of the lung dysfunction
In addition to the distance-injury correlation, we could also show a time-dependence of
oedema generation. Isolation and perfusion of the lung immediately after blast led to much
more weight gain than 3 and 6 hours after blast exposure. These results provide evidence that
the alveolar capillary barrier membrane is at least in part intact and that oedema resorption
and/ or stop of oedema generation took place in these lungs (discussed in detail in 5.3.4).
Interestingly, no further improvement could be seen between 3 and 6 hours after blast,
indicating that the main resorption capacity and/ or repair occurred within the first 3 hours.
Indeed, many experimental studies indicate that the alveolar epithelium is remarkable
resistant to injury, particularly compared to the adjacent lung endothelium. Even when mild to
moderate alveolar epithelial injury occurs e.g. hyperosmolar injury 184 or leukotriene B4-
induced PMN infiltration 185, the capacity of the alveolar epithelium to transport salt and water
is often preserved.
Also, the tidal volume (Tv) measured immediately after the onset of ventilation was
significantly improved 3 and 6 hours following the blast, reaching almost control levels of non-
traumatized animals. This improvement is accompanied by lower necessary inspiration
pressure (PIP) to achieve 1 ml (see 5.2.1) and may be due to the reduced weight gain.
Despite gentle standard ventilation of these lungs (3 and 6 hours after blast) there was also a
measurable decline of the lung mechanics over time. This observation provided further
evidence for a higher susceptibility of injured lungs towards ventilator-associated lung injury,
even at standard ventilation-pressures. This is important since the success or failure of the
clinical treatment of primary blast injury may depend not only on the judicious use of
resuscitative fluids but also on the respiratory support 128.
Discussion
89
5.2.3 Pharmacological modulation of the injury
The present study suggests that even after severe mechanical injury such as blast injury, the
alveolar-capillary barrier capacity together with the alveolar epithelial fluid transport is at least
in part maintained.
5.2.3.1 Role of the amiloride-sensitive sodium channels
Several studies have shown that transport of sodium is a primary mechanism driving alveolar
fluid clearance (reviewed by Matthay and coworkers 5,172, Sartory and Matthay, 6), although
further work is needed to determine the role of chloride in vectorial transport across the
alveolar epithelium 16. Thus, the objective of the present study was to test the effect of the
known sodium transport inhibitor amiloride on alveolar liquid clearance in our primary blast
injury model. Amiloride was given into the perfusate in a commonly used concentration of 10-4
M 7,22,186. The results of our amiloride studies demonstrate a more than double increase in
oedema formation during perfusion in blasted lungs perfused with amiloride, as compared to
non-treated blasted lungs. Thus, even if limited, a partial integrity of the sodium channels and
therefore a fluid resorption capacity after trauma has been suggested. Such an amiloride-
sensitive fluid resorption could be the underlying mechanism for the reduced weight gain
observed ex vivo 3 and 6 hours after blast exposure (discussed in detail in 5.2.2 and 5.3.4).
The presence of regulable, amiloride-sensitive sodium channels leading to fluid resorption in
the intact mammalian alveolar epithelium has been reported by many authors using different
models and different species 7,8,21. Inhibition of the endogenous fluid resorption in traumatized
rat lungs by amiloride furthermore resulted in a marked deterioration of the airway mechanics.
This may be due to the massive oedema formation rather than to a negative effect of amiloride
itself.
5.2.3.2 Role of ββββ-adrenergic receptors
Upon infusion of terbutaline (10-4 M) or formoterol (1 nM) in the perfusate of blasted rat lungs,
the weight gain during perfusion was significantly reduced. Upon terbutaline treatment, almost
control levels of non-traumatized rat lungs were reached. In rats the response to β-adrenergic
agonists included an increase in sodium unidirectional flux out of the alveoli and stimulation of
fluid absorption 21,186,187. These observations are in line with others, that report that terbutaline
increased sodium transport in alveolar type II cell monolayers 188,189 as well as in vivo 8.
Terbutaline must have stimulated the transport through amiloride-sensitive pathways, since
amiloride reduced the terbutaline-related fluid resorption in this setting. This result is in
accordance with prior studies of the effect of amiloride on the terbutaline-induced increase in
alveolar liquid clearance 7,8,22. With regard to the increased but not complete fluid resorption
Discussion
90
and/ or stop in oedema generation in vivo within the first six hours after blast exposure (5.2.2),
these data further indicate that the fluid transport capacity after traumatic injury may be
upregulated by β-adrenergic agonists. However, infusion of amiloride plus terbutaline resulted
in decreased oedema formation in this injury model than amiloride treatment alone. The most
reasonable explanation for this finding is that terbutaline stimulates sodium transport through
both amiloride-sensitive and insensitive pathways. Similar findings were reported by Goodman
and colleagues 21 and confirmed by others 7,8. In the isolated perfused rat lung, amiloride
alone reduced sodium transport by 30%, terbutaline increased it by 59%, but terbutaline plus
amiloride decreased clearance only by 14%. Another explanation could be a permeability
decreasing action of terbutaline, leading to a reduction of oedema generation after trauma. It
has been reported that isoproterenol attenuates the thrombin-induced increase in endothelial
permeability in vitro 190.
Thoracic trauma-related deterioration of the airway mechanics was markedly reduced by β-
adrenergic agonist treatment, with respect to tidal volume (Tv) and airway resistance (RA). The
reduced airway resistance is probably due to the β2-receptor-mediated airway smooth muscle
relaxation. Improved pulmonary mechanics upon β2-agonist treatment have also been shown
in fetal lambs 191. Particularly, the “longer”-acting β2-agonists such as salmeterol and
formoterol represent a therapeutic advance in the management of asthma 192, especially in
combination with inhaled corticosteroids 193. Furthermore, the positive influence on the airway
compliance (data not shown) and therefore on the tidal volume observed in these studies may
be due to β-agonist-related modulation of the pulmonary surfactant synthesis 191,194,195. In
contrast to the weight gain, amiloride did not affect the terbutaline-related effects on airway
mechanics, which therefore may be considered as sodium-channel independent β2-agonist
effects.
The experiments with the unspecific β-receptor antagonist propranolol indicate that the effect
of terbutaline on airway mechanics in blasted rat lungs is mediated through β-receptors.
However, oedema formation and vascular resistance (data not shown) were even more
impaired upon terbutaline plus propranolol treatment, as compared to non-treated blasted rat
lungs. The block of β2-receptors causes the well known side effects, e.g. vasoconstriction,
delayed response to hypoglycemia in diabetic patients, and bronchoconstriction (reviewed by
Pozzi, 196), which could be involved in the observed effects. A propranolol-related
vasoconstriction in turn might be a possible explanation for the observed increase in oedema
formation. Because propranolol also blocks possible endogenous epinephrine-related-effects
during trauma, this might at least in part explain the observed deterioration. We did not
specifically attempt to block possible trauma-related epinephrine effects, thus we can only
speculate about this. However, the basal β-adrenergic tone in anaesthetized sheep 7 and rats
Discussion
91
8 is probably not an important factor in the normal fluid clearance, because propranolol alone
did not have an effect on lung liquid clearance.
Taken together, these results demonstrate that the integrity of the sodium channels is at least
in part maintained after blast injury in this model. Thus, increased alveolar fluid clearance
might be the underlying mechanism for the observed fluid resorption in vivo within the first six
hours after trauma (discussed in detail in 5.2.2 and 5.3.4). Furthermore, β2-adrenergic therapy
increased not only the oedema resorption and/ or the oedema generation after trauma, but
also improved the airway mechanics by direct β2-adrenergic effects independent of β-receptor-
related fluid resorption. Thus β2-adrenergic substances like terbutaline or formoterol appear to
be beneficial after primary blast injury in this model.
5.3 Thorax trauma-related pathophysiological changes in vivo over time
After an initial non-fatal injury, thoracic trauma is considered to play a pivotal role in the
development of single-or multi-organ failure 93,112, probably making the patient more
susceptible to infections 95. However, the aetiology of pulmonary contusions following
exposure to blast is not clear 118. In the present study, we investigated the sequence of
alveolar injury in vivo over time, with regard to pathological findings and molecular responses
to injury as e.g. inflammatory mediator release.
5.3.1 Structural integrity of the lung tissue after blast injury
At autopsy, none of our rats showed external signs of injury 116,117,122,124. The pulmonary
contusion produced after blast exposure was evident as areas of haemorrhage on gross
inspection of the lungs immediately after blast, with increasing intensities with higher pressure
wave intensities (5.2.1). Clinically, these contusions may be difficult to detect in the absence of
overt symptoms such as breathlessness, haemoptysis or a decreased PaO2, and the lung may
continue to accumulate extravascular lung haemorrhagic or oedema fluid, that may lead to
deterioration in lung function and in the condition of the patient. The implication of these
clinical sequelae is that haemorrhage may continue within the injured lung and that areas of
the lung initially apparently undamaged may later bleed and show other signs of damage 118.
However, our experiments showed that after an initial massive blast-induced alveolar
bleeding, the bronchoalveolar lavage (BAL) red blood cell counts continuously decreased over
time and were no longer detectable after 96 hours. Together with the time-dependent
resolution of the trauma-related alveolar protein content, these results suggested an
enormous clearance capacity and/ or repair of the lung, despite of the mechanically induced
Discussion
92
cell damage in this setting. In this context, Kim and coworkers 166 reported a net absorption of
intact albumin via saturable receptor-mediated transcellular endocytotic processes in primary
cultured rat alveolar epithelial cell monolayers. The resolution of the alveolar haemorrhage is
also in line with clinical situations of alveolar haemorrhage 167 and may be related to the
increasing amounts of alveolar macrophages detected in this “later” phase after blast
exposure (discussed in detail in 5.4.1). Indeed, after haemorrhage, large quantities of
haemoglobin and ingested red blood cells can be detected in alveolar macrophages 197, in
accordance with our observations on the microscopic level (data not shown). Furthermore,
haemosiderin-laden alveolar macrophages are a common finding in patients with alveolar
bleeding 197,198.
Markers of endothelial injury such as the von Willebrand`s factor (vWF) antigen have been
used to reflect systemic endothelial cell activation and/ or damage in patients with acute lung
injury 199. Because of the lack of an available commercial kit for the detection of rat von
Willebrand`s factor (vWF), in the present study the profound release of the cytosolic enzyme
lactate dehydrogenase (LDH) into the BAL was used as a marker for the cellular integrity after
blast. Thanks to the long half life of the enzyme, LDH release may be a suitable marker for
trauma-induced cell lysis. A recent study demonstrated a strong haemoglobin
immunoreactivity of the oedema fluid within the alveolar space of blast victims 119.
Erythrocytes are known to express the LDH-1 isoform and thus may also be considered as a
source for the observed LDH release. Sustained elevated LDH levels might also be an
indication for a delayed cell death after trauma. Morphologic changes from haematoma to
necrosis to gangrene have been observed after primary non-perforative intestinal blast injuries
in rats 200.
Based on the determined wet to dry weight ratios, maximal oedema formation was detected
within the first 90 minutes after blast exposure. The reduced wet to dry weight ratios assessed
from 3 hours after blast exposure on might suggest oedema resorption and/ or a stop in
oedema generation. In contrast, although not significant, our calculated lung wet to body
weight ratios (LWR) and thus the corresponding injury quotient (Qi) indicated a secondary
deterioration between 6 and 24 hours after blast. This was attributed to a secondary increase
in lung wet weight resulting in an increased LWR and Qi. This increase may be explained by
increasing amounts of infiltrating neutrophils during this time (discussed in 5.3.3). Thus, we
can not discriminate between an increased oedema resorption and an increase in pulmonary
infiltrates (discussed in detail in 5.3.4).
Discussion
93
5.3.2 Mediator release in response to primary blast injury
A generalized host inflammatory response is necessary to orchestrate the maintenance or
recovery of tissue repair and immune competence, following severe injury or infection.
Besides clinical characterization, recent research data indicate that the prognosis of trauma
patients is strongly associated with a post-traumatic imbalance of the immunologic system 146.
For the outcome of patients with multiple injuries it seems very important to gain an
inflammatory mediator homeostasis as fast as possible. If the pro-inflammatory potential
predominates, systemic inflammatory response syndrome (SIRS) may be the consequence; if
the counter-regulatory, anti-inflammatory mediators predominate (CARS), immunosuppression
(“immunoparalysis”) with ineffective eradication of microorganisms and septic complications
may follow 142.
There were three major reasons for us to study the involvement of mediator release after
primary blast injury in this setting: First, to gain more knowledge about the pathogenesis of the
injury; second, to determine whether the balance between pro- and anti-inflammatory mediator
release is maintained in this setting; and third, to identify markers, either in the early or in the
“late” posttraumatic phase, that may be suitable predictors of the overall outcome.
Since measurement of mediators directly in the lungs has been shown to be more valuable
than measurement in plasma or serum 201, we determined the release of different mediators in
the bronchoalveolar lavage (BAL) fluid of traumatized rat lungs.
5.3.2.1 Thorax trauma-related eicosanoid release
Brückner and colleagues 134,138 reported a pattern-related release of prostanoids which was
rather pronounced in polytrauma associated with damage of the lung. A similar pattern has
been found in patients who underwent thoracotomy plus additional surgical damage to the
lung 136. Therefore, these authors suggested the prostanoid release to be specific for the
involvement of the lung. In line with these results, we detected a significant immediate release
of both thromboxane and prostacycline within the first 10 minutes after blast exposure,
followed by a marked decrease reaching control levels within 90 minutes. Prostanoids are
synthesized from arachidonic acid by the constitutively expressed cyclooxygenase (COX)-1
and the inducible COX-2 enzymes. Among others, the activity of phospholipase A2 regulates
prostanoid production in many cell types 202. Elevated plasma levels of type II a phospholipase
A2 (PLA2) have been found in inflammatory diseases and trauma and are suggested to bear
prognostic value for outcome 137,138. Thromboxane and prostacycline play an important role in
the control of haemodynamics. Prostacycline is predominately released from endothelial cells
as a result of endothelial injury or mediator stimulation. In contrast to prostacycline, the
release of thromboxane from alveolar macrophages, platelets or endothelial cells is believed
Discussion
94
to require specific stimulation 203,204. Thromboxane-induced platelet aggregation and
vasoconstriction are antagonized by prostacycline, and thus the ratio of thromboxane to
prostacycline is of importance. In addition, thromboxane acts as a potent bronchoconstrictor.
Thus, increasing release of thromboxane in polytrauma patients with thorax involvement has
been suggested to be a predictive marker for the development of pulmonary dysfunction after
trauma 136. Despite of pressure wave-induced lung injury, the crucial metabolic activities of the
lung, such as thromboxane degradation as well as extrapulmonary clearance of 6-keto PGF1α
seemed unaltered in the present study, which is in accordance with other reports 136. The
metabolic clearance occurs via two steps: 1. selective, carrier-mediated prostaglandin uptake
across the plasma membrane and 2. non-selective oxidation inside the cell. However, only
TXA2, PGE1, PGE2, PGD2, and PGF2α are transported across the cell membrane. There is
substantially less clearance of PGA2 and essentially none of PGI2 or 6-keto PGF1α (reviewed
by Schuster, 205). With regard to the lack of COX-2 induction within the first 6 hours after blast
(RT-PCR analysis, data not shown), a secondary increase of these mediators in the “late”
posttraumatic phase in this setting appeared rather unlikely.
5.3.2.2 Thorax trauma-related cytokine release
Trauma, shock, and infection initiate a complex inflammatory response in which the pro-
inflammatory cytokines tumor necrosis factor (TNF)-α, interleukin (IL-1)-β, and interleukin (IL-)
6 are thought to play a pivotal role. Overwhelming synthesis of pro-inflammatory cytokines
after trauma has been correlated with poor outcome 168,169.
In the present study IL-6 levels in bronchoalveolar lavage (BAL) fluids were significantly
elevated 6 hours after trauma, as compared to non-traumatized control lungs, returning to
baseline between 12 and 96 hours. This early increase is in accordance with plasma IL-6
levels obtained from polytrauma patients 135,142. IL-6 production is induced in part by TNF-α
and IL-1β, and it has been proposed that IL-6 “integrates” signals produced early in the
inflammatory response 206. Some data support the concept that the production of TNF-α and
IL-6 is regulated independently 168. In contrast to TNF, IL-6 has been reported to be a marker
of the intensity of the injury, bearing some prognostic value for the survival in the early
posttraumatic phase 135. Recent reports support a crucial anti-inflammatory role for IL-6 by
controlling the levels of other pro-inflammatory cytokines 150 and by inducing significant
release/ formation of soluble tumor necrosis factor receptors (sTNFR) 151.
In comparison to non-traumatized control lungs, the BAL TNF-α levels of traumatized lungs
were significantly elevated from 3 hours after trauma on and returned to basal values after 96
hours. Most likely, the TNF-α found in BAL was produced by activated pulmonary
macrophages. A major function of TNF-α in the lung appears to be upregulation and induction
Discussion
95
of endothelial adhesion molecules ICAM-1 and E-selectin, respectively, both of which are
critical for the early steps required in neutrophil adhesion to the activated endothelium and
eventually in transmigration of neutrophils into the alveolar compartiment 69. Indeed, a marked
increase in neutrophil infiltration into the alveoli was observed 6 and 12 hours after blast
exposure in this setting (discussed in 5.3.3).
Simultaneous determination of TNF-α in plasma showed a striking difference from levels in
BAL fluids; plasma TNF-α was not detectable within 96 hours after trauma neither by ELISA
nor by the WEHI-bioassay (data not shown). This suggests that TNF-α is secreted locally in
the lung by pulmonary macrophages. The lack of any increase in plasma TNF-α levels is in
line with clinical data obtained from trauma patients suffering from different traumatic injuries 135. Even in patients with ARDS after trauma, shock or sepsis, plasma cytokines were neither
increased in most patients nor did they correlate with the development or severity of ARDS 169.
Since experimental haemorrhage and blunt trauma do not lead to increased circulating TNF-α
levels in pigs, the authors of this study have suggested that TNF-α plays no role in the
pathogenesis of shock in their model 141. In contrast to sepsis, where bacteremia and
endotoxemia result in the systemic appearance of cytokines 207, blunt trauma may cause the
release of cell-associated TNF-α only at the local side of trauma. However, other animal 208 as
well as clinical studies 168 reported that the induction of TNF-α release after trauma is
significantly enhanced when haemorrhagic shock is also present. These authors suggested
that shock is the main factor leading to the production and release of TNF-α by macrophages.
Nevertheless, the levels of secreted BAL TNF-α after primary blast injury in this setting were
relatively moderate. Some publications have provided evidence for the presence of 55- and
75-k Da soluble tumor necrosis factor receptors (sTNFRs) in injured patients in the absence of
measurable plasma TNF-α, with a strong correlation with mortality 148,149,209. Although it has
been reported that sTNFRs affect TNF functions even at low TNF concentrations by stabilizing
and augmenting some of its activities by a kind of controlled release 210, it is assumed that
shedding of sTNFRs in response to high TNF concentrations could serve as a mechanism for
binding and inhibiting overwhelming TNF levels and localizing the inflammatory response 211.
In the present study, sTNFR (p55 and p75) levels in BAL fluids of traumatized rat lungs were
significantly elevated within 90 minutes after trauma. This early release is in accordance with
plasma sTNFR levels obtained in polytrauma patients 142,149. This suggests that thoracic
trauma initiates the rapid release of preformed receptors on the cell surface of injured tissues
or activated leukocytes, or both. Similarly to the measured BAL TNF levels, also sTNFR levels
were comparatively low as compared to plasma sTNFR levels measured in trauma patients 142,148,209. This may be in part explained by a dilution effect due to the BAL method (for
cytokines by about 100-fold, 206). In contrast to other studies 142,148, data from the present
Discussion
96
study showed that receptor levels return to non-traumatized control levels, indicating a peak-
like profile of sTNFR instead of sustained elevation. Since clinical studies reported declined
sTNFR levels in patients who recovered from injury 149, the decrease in BAL sTNFR levels in
the present study may be correlated with a recovery from primary blast injury. The correlation
between each p55 and p75 with IL-6 release within 96 hours after blast supports the
hypothesis that IL-6 may be involved in the regulation of both sTNFR p55 and p75 levels. This
hypothesis is supported by the report of Tilg and coworkers 151, who observed elevated
sTNFR p55 levels in cancer patients after administration of recombinant IL-6. In the present
study the 55-kDa and 75-kDa sTNFR levels were both significantly elevated within 90 minutes
after trauma, which is in agreement with clinical data obtained from severely injured patients
described by Tan and colleagues 212. In contrast, other authors reported an early shift towards
sTNFR p55 release 142. The factors that may be responsible for increased or prolonged
release of sTNFR after trauma have not been determined yet, although proteases and IL-6
have been discussed 151,152. Neutrophil-derived proteases have been shown to be elevated,
predominantly in patients with isolated thorax trauma 135. With regard to our results, we can
only speculate about an involvement of locally produced IL-6 in the early appearance of
sTNFR subtypes in the injured lung after primary blast injury. Whether sTNFR levels in the
BAL fluids may be the response to local TNF production and/ or the reason why BAL TNF
levels were relatively moderate and plasma levels were even not measurable, can not be
explained in the present study.
Furthermore, we measured IL-10 as a counterregulatory cytokine that inhibits cytokine
production by stimulated macrophages 213. IL-10 is detectable in ARDS BAL fluids, but the
concentrations are very low (10 - 20 pg/ ml), as compared to other cytokines 206. In agreement
with this, our data demonstrated low and even significantly decreased BAL IL-10 levels at any
measured time point within 24 hours after blast exposure, as compared to base line levels of
non-traumatized control lungs, and with recovery only after 96 hours. Such low IL-10 levels
may favour cytokine production in the alveolar environment in this setting. In contrast,
Henseler and colleagues 142, showed elevated plasma IL-10 values within 3 hours after
trauma in patients suffering from multiple injuries. It has also been reported that the lung
perpetuates a constitutive level of anti-inflammatory cytokine IL-10, which is not enhanced
after aerosol exposure of endotoxin, whereas systemically, intraperitoneal delivery of
endotoxin resulted in an increase in circulating IL-10 150. Initiation of coagulation by tissue
factor (TF) has been shown to be a powerful regulator of local inflammatory responses 214.
With regard to this, Miller and colleagues 215 reported that blockade of TF-FVIIa complex
protects the lung from injury by LPS in part by reducing local expression of pro-inflammatory
cytokines and local elaboration of interleukin (IL)-1beta, IL-6, and IL-10. Furthermore, it has
Discussion
97
been shown that trauma induces TF expression on monocytes 216 which may be one reason
for the observed decline in BAL IL-10 after blast injury in this model.
5.3.2.3 Thorax trauma-related NO release
Following blast exposure we could detect nitric oxide related nitrite and nitrate with a
significant maximum 12 hours after trauma. However, RT-PCR analysis revealed no induction
of the inducible nitric oxide synthase (iNOS) within 12 hours (data not shown). These results
indicate an initial trauma-induced NO release due to the constitutive endothelial NOS rather
than due to an involvement of the iNOS during the first four days following blast exposure in
this setting. Whether this increase reflects injury or a signal mechanism to initiate repair
process remains to be established.
5.3.3 Thorax trauma-related chemokine release and inflammatory cell infiltration
Thoracic trauma resulted in a pronounced CINC-3 production and neutrophil infiltration into
the alveolar space after 6 hours, whereas these hallmarks of inflammation were absent in the
bronchoalveolar lavage (BAL) fluids of non-traumatized control lungs. Alveolar macrophages
are thought to be the major source of α-chemokines such as CINC-3 in the airspaces 170,206
and produce CINC in response to LPS, both in vitro 217 and in vivo 218,219. Thus, CINC has
been reported to contribute to the influx of neutrophils and their activation during acute lung
injury 170,220.
Likewise, matrix metalloproteinase (MMP)-9 release was detectable in BAL fluids 6 hours after
blast exposure. MMP-9 is preferentially expressed by inflammatory cells 171 and thus may be
correlate with the observed neutrophil infiltration at this time. In addition, the release and
activation of MMP-2 was measurable within 24 hours after blast, whereas no MMP-2 was
detectable after 96 hours and in BAL fluids from non-traumatized rats. MMP-2 has been
reported to be preferentially secreted by fibroblasts and epithelial cells 171 and may therefore
be released after trauma-induced cell damage and/ or participate in tissue remodeling
associated with pathological situations such as thoracic injury. Recently, matrix
metalloproteinases (MMPs) and the specific tissue inhibitors of metalloproteinases (TIMPs)
have been shown to participate in both parenchymal destruction and repair process resulting,
in extracellular matrix (ECM) remodeling 161,221-223.
Discussion
98
5.3.4 Oedema generation and resorption after thorax trauma: Comparison of the ex vivo and in vivo results
Based on the increasing wet to dry weight ratios, maximal oedema formation was detected
within the first 90 minutes after blast exposure. The reduced wet to dry weight ratios
determined from 3 hours after trauma on might suggest, but were not inevitably due to, an
oedema resorption and thus may result from pulmonary infiltrates, protein sediments,
membrane regeneration and others. Although not significant, the calculated lung wet to body
weight ratios (LWR) and therefore the corresponding injury quotient (Qi) indicated a secondary
deterioration between 6 and 24 hours after blast, arguing against an increased oedema
resorption during this time. This is further supported by an increased infiltration of neutrophils
into the alveolar space starting from 6 hours after trauma on. However, our ex vivo results
demonstrated that the alveolar capillary fluid resorption capacity is at least in part maintained
after blast pressure wave exposure since β2-adrenergic therapy stimulated and amiloride
treatment inhibited the fluid resorption in this model. The reduced weight gain assessed 3 and
6 hours after blast, as compared to the immediately perfused lungs can therefore be related to
both an increased repair, a stop in oedema generation and elevated oedema resorption.
Whether these effects are related to possible endogenous epinephrine-induced actions can
not be explained because we did not specifically attempt to block possible trauma-related
epinephrine effects in this setting.
5.4 Thorax trauma-related impairment of alveolar macrophage function in vitro
5.4.1 Alveolar macrophage population after trauma
The number of alveolar macrophages (AM) recruited from the alveolar space after thoracic
trauma was significantly different when compared to non-traumatized controls. Whereas the
number of AM was decreased within the first 24 hours after trauma, there was an up to 1.5-
fold increase after 96 hours. Since we measured elevated LDH levels after trauma (discussed
in 5.3.1), the decrease in the AM number may be the consequence of increased cell death
due to blast exposure. Furthermore, increased trauma-related adhesion of the AM to the
endothelium/ epithelium would lead to lower amounts of AM in isolated BAL fluids. With regard
to the increasing amounts of AM isolated in the “later” post-traumatic phase, it has been
shown that an increased number of mononuclear phagocytes, characteristic for the chronic 58
and acute inflammatory 224,225 state, can result from an increased rate of recruitment of these
cells from the blood 225, from a decreased rate of efflux (including cell death) from the lung, or
from local replication 58,225.
Discussion
99
5.4.2 Phagocytic capacity, microbial killing and TNF release
Although it has been reported that severe trauma contributes to an increase in infectious
complications through an impairment of host defence mechanisms 163, the cause of such
impairment remains unknown 164. The alveolar macrophage, mobile representative of the
mononuclear phagocyte system, is believed to be the central modulator, both as regulator and
effector of inflammation/ anti-inflammation within the alveolar space 48.
In the present study, blast pressure wave exposure resulted in an immediate decrease in the
alveolar macrophage (AM) phagocytosis rate of Escherichia coli (E. coli) in vitro with recovery
within 96 hours after blast. Although not statistically significant, the phagocytic capacity for
Staphylococcus aureus (S. aureus) particles seemed to be reduced initially after thoracic
trauma. Disorders of the phagocytic process in alveolar macrophages have been reported
after thermal injury 226,227. These studies showed a primary decrease occurring immediately
after the burn. The discrepancy between the different phagocytosis rates of both bacterial
stimuli may be explained by experimental problems rather than by strains differences.
Whereas the E. coli particles were suspended homogenously, the S. aureus particles formed
aggregates despite of sonicating them and this may affect particle counts and therefore the
read-out of the experiment. The use of different lots of fluorescence labelled particles may
also contribute to the controversial results. Nevertheless, as macrophages are the primary
resident phagocyte of the resting human lung, it is intuitive that any functional impairment
leads to infection by micro-organisms. Thus, despite recovery within 4 days after trauma,
these data suggest an initially impaired phagocytosis capacity due to thoracic trauma, that
may result in a higher susceptibility to infections. It is possible that trauma-induced factors or
mediators may either bind to the macrophage surface or suppress macrophage activity,
thereby down-regulating phagocytosis. It is also conceivable that impairment of the pulmonary
surfactant during lung injury contributes to a decreased phagocytosis capacity. Indeed,
surfactant protein A 71 and D 72 are able to precoat bacteria and particles in order to facilitate
macrophage phagocytosis and bactericidal activities. The trauma-related, deteriorated tidal
volume and pulmonary compliance we assessed ex vivo in our lung perfusion model support
such a trauma-induced loss in surfactant.
The production of reactive oxygen species (ROS) (“respiratory burst”) upon receptor-mediated
phagocytosis was investigated to determine the microbicidal activity of the AM in vitro after in
vivo thorax trauma. Thoracic trauma yielded a marked decrease in the production of
superoxide within the first 24 hours after trauma, both with or without the addition of E. coli or
S. aureus, with recovery only after 96 hours. The respiratory burst results from the assembly
and activation of the NADPH oxidase 76. Decreased levels of superoxide can be attained
Discussion
100
either by a decrease in its production or by an increase in its elimination, be it through
interfering with one or more steps in the signal transduction pathway at either the cell
membrane level or subsequent intracellular stage such as dismutase, protein kinase (PK)-C
activation or through scavenging by other radicals, such as nitric oxide. With regard to this, it
has been shown that LPS-related oxidative burst and TNF-release by human monocytes can
be modulated by IL-9 through an upregulation of TGF-β which in turn inactivates the
extracellular signal-regulated kinases (ERK) 1/ 2 84. TGF-β is involved in bronchial wound
repair 228.
The difference between trauma and control in both the resting and the activated state, could
therefore arise from both a decreased activity of one or more oxidases and an increased
ability of the cells to eliminate superoxide, due to cellular damage and released NO (discussed
in 5.3.2.3).
Since overnight culturing of the isolated control AM reduced the spontaneous superoxide
production to about 30% of its initial value, the increased release of superoxide in non-
traumatized controls may be attributed to the activation of NADPH oxidase during the
macrophage isolation procedure. In contrast, the superoxide anion levels produced upon E.
coli stimulation were not affected by overnight culturing in these cells and thus may be related
to the bacterial stimulus (data not shown). In order to preserve the in vivo conditions after
trauma in terms of both macrophage environment and time-dependent AM behaviour, we
abstained form overnight culturing before stimulation.
Similarly, trauma-related initial decrease of superoxide generation was independent of the
presence of lipopolysaccharide (LPS) or lipoteichoic acid (LTA). In contrast to the stimulation
with whole dead bacteria, upon LPS/ LTA stimulation the superoxide levels of non-traumatized
controls were reached already at 24 hours, and were increased 96 hours after the blast. Since
the levels of superoxide produced by the non-stimulated controls were different between the
experiments, the higher respiratory burst capacity observed upon LPS/ LTA stimulation as
compared to E. coli/ S. aureus stimulation, may be due to an increased basal stimulation,
rather than to their particular specificity. In contrast to this stimulus-independent effect, the
earlier recovery together with the increased oxidative burst after 96 hours, suggests higher
susceptibility of the AM towards LPS and LTA as compared to E. coli and S. aureus
stimulation in this setting. However, the most likely explanation for this would be that the
amount of surface-bound endotoxin on E. coli and LTA on S. aureus particles is not
comparable with the amount of LPS and LTA used in these experiments. This explanation is
further supported by the fact that both whole bacteria and endotoxin, act on the same
receptors on the macrophage surface. Recent studies have identified multiple receptors for
endotoxin which has accelerated the study of signalling in macrophages (reviewed by Monick
and Hunninghake, 229, Wright, 66). Two classes of receptors, the CD18 antigens (leukocyte
Discussion
101
integrins) and the scavenger receptor (acetyl low-density lipoprotein), recognize particulate
LPS directly. Both these receptors may be involved in catabolism of LPS, because neither
receptor initiates strong secretory responses e.g. TNF synthesis to LPS. A third receptor,
CD14, recognizes LPS complexed with the serum lipoprotein binding protein (LBP) 62. CD14
appears to participate in both the ingestion of, and the responses to LPS, because a blockade
of CD 14 with monoclonal antibodies (mAbs) strongly inhibits both uptake of bacteria and
secretion of TNF by human mononuclear cells 62. A recent study suggested that the
recognition sites of CD14 for LPS and LTA are distinct, with a partial overlap 230.
Furthermore, leukocytes express three different receptors for complement protein C3, and 10
distinct receptors for the Fc region of IgG 60. With regard to possible regulatory mechanisms of
phagocytosis and oxidative burst in the present study, Pricop and Salmon 77 reported that
FcγR activation induces the NADPH oxidase and thus increases ROS formation. These
authors further demonstrated that ROS generated in an inflammatory milieu act in an
autocrine and paracrine manner in order to rapidly amplify the effector potential of FcγR on
quiescent phagocytes by altering signal transduction.
We further investigated macrophage TNF release after experimental thorax trauma, alone and
in response to either endotoxin/ LTA or whole dead bacteria. The TNF release of AM from
traumatized rat lungs was increased 96 hours after blast as compared to non-traumatized
controls, indicating that the AM are primed to release TNF following thoracic trauma. This
result is in line with increasing TNF levels measured in BAL fluids of traumatized rat lungs in
vivo over time (discussed in 5.3.2.2). However, when compared to the early TNF release
measured in BAL fluids from 3 hours after trauma on, the TNF release by isolated AM in vitro
is delayed. Additional stimulation of the AM with either endotoxin/ LTA or bacteria induced a
marked increase in TNF release 24 hours after blast exposure, whereas initially after blast the
response of the AM towards both stimuli was comparable or even decreased (E. coli
stimulation) with that from AM of non-traumatized controls. We conclude that thoracic trauma
primes AM to release TNF which can be augmented by an additional bacterial stimulus. With
regard to TNF release, AM from sham controls as well as from traumatized rats were more
susceptible to LPS than to LTA (up to 8-fold and 7-fold, respectively at the highest used
concentration) and more to E. coli than to S. aureus stimulation (up to 4.7-fold and 6.5-fold,
respectively). This is in close correlation to reports from Morath and colleagues 231, who
described LTA as a weak inducer of cytokine release in human blood compared to LPS.
Many experimental models of trauma have demonstrated a change in macrophage function as
manifested by a decreased cytokine production 155,165,232, superoxide production 155,156,232,
phagocytosis capacity 156, antigen presentation 155,156, and Candida killing 156,232 immediately
Discussion
102
after injury. The causes of abnormal macrophage function appear to be multifactorial but are
not well understood. Injury causes a stress response which in turn has been recognized as a
source of immunosuppression. Thus, physical or even psychological stresses trigger the
hypothalamic-pituitary-adrenal (HPA) axis, resulting in a marked rise in serum levels of many
hormones e.g. glucocorticoids 130. Receptors for glucocorticoids are present on macrophages 233 and have been shown to downregulate macrophage functions 232. Furthermore, not only
stress but also pro-inflammatory cytokines such as IL-1, IL-6 and TNF cause via the release of
corticotropin the release of glucocorticoids (reviewed in 130). Thus, glucocorticoid-mediated
immunosuppression following injury may represent dysfunction of normal, inhibitory feedback
pathways. With regard to this, Cech and colleagues 232 reported increased plasma
corticosterone levels one day after femure fracture in mice. In this study femur fracture
resulted also in a reduction of 1. Macrophage production of superoxide anion, 2. C. albicans
killing, 3. macrophage synthesis of IL-6 and TNF and 4. an increase in PGE2 synthesis. These
authors further demonstrated that pre-treatment with the glucocorticoid receptor antagonist,
mifepristone (RU 486) significantly prevented or reduced the observed suppression of several
macrophage functions, including oxidative burst capacity and C. albicans killing but did not
alter the increased PGE2 synthesis. However, the initially suppressed macrophage function
was supposed to be at least in part due to the trauma-related PGE2 production 155. The results
from our study demonstrated a recovery from an initially suppressed E. coli phagocytosis and
oxidative burst within 24 hours and 96 hours, respectively. Such a rebound phenomenon has
also been described for peritoneal macrophages after laparotomy 156. We further identified a
hyperactive TNF response of AM to endotoxin/ LTA and whole bacteria stimulation that is
seen 24 hours after blast exposure. This is in line with McCarter and colleagues 155 who found
increased TNF, IL-6 and H2O2 secretion of splenic macrophages in response to endotoxin or
PMA stimulation 7 days after trauma. These authors further demonstrated that inflammatory
hypersecretion does not necessary translate into improved immunologic protection, as
demonstrated by the functional impairment of macrophage antigen presentation. It is likely
that the impairment of phagocytic function and microbicidal activity after thoracic trauma
observed in this setting could contribute to a depressed antigen presentation. However,
preliminary findings showed that Keyhole Limped Hemocyanin (KLH)-sensitised rats
developed a cutaneous anergy during about four days after severe trauma, which underlines
that the intensity of the investigated trauma has systemic repercussions and seems to include
aspects of immunosupression.
The search of the signalling endotoxin receptor led to the discovery of Toll receptors (reviewed
by Monick and Hunninghake, 229): TLR 4 is the LPS-specific receptor, whereas TLR 2 has
been linked to LTA from Gram-positive bacteria. Both TLR 2 and TLR 4 have been found on
alveolar macrophages, providing the entry point for a complex cascade of LTA/ LPS signalling.
Discussion
103
Downstream of the TLR 4 complex, a number of signalling pathways are activated. These
include the MAP kinases, phosphatidylinositol (PI) 3-kinase pathway and sphingolipid
metabolites that regulate LPS-induced gene expression. Protein kinase (PK) C and PI3-kinase
have been shown to be not only involved in the phagocytosis of E.coli particles, but also in the
signalling pathway of LPS-induced TNF release. In contrast, anti-inflammatory
phosphodiesterase inhibitors prevented LPS-induced TNF release but had no effect on the
beneficial phagocytosis of E. coli by macrophages 234.
5.4.3 Involvement of trauma-related alveolar haemorrhage in impaired macrophage functions
As already discussed in 5.3.1, alveolar haemorrhage was the most frequent and obvious
injury detected in our rat blast model, thus it was of interest to examine whether the observed
initial alveolar macrophage (AM) dysregulation was due to the accompanying alveolar
bleeding. In these experiments, the removal of the red blood cells (RBCs) resulted in a
marked increase in the phagocytosis of E. coli particles and superoxide anion production (with
or without E. coli stimulation) by AM from traumatized rat lungs. Although other factors may be
implicated in the downregulation of the macrophage function, the initial suppression of
phagocytosis and oxidative burst capacity by AM may be caused at least in part by the
trauma-related alveolar bleeding. In contrast, the absence of RBC’s did not significantly alter
the E. coli-induced TNF release, thus the alveolar haemorrhage seems to play only a minor
role in the trauma-related TNF release. We could further demonstrate that different blood
components are involved. Whereas the phagocytosis capacity of control AM was significantly
reduced in the presence of intact blood cells (whole blood and washed RBC’s), the oxidative
burst and the TNF release remained unaffected. In contrast, haemolytic blood decreased the
superoxide production and the TNF release but had no effect on the phagocytosis capacity of
E. coli particles. Since previous experiments revealed no difference in superoxide production
with or without the presence of a bacterial stimulus, the plasma-related decrease in
superoxide production upon E. coli stimulation may be explained by a plasma contamination
with intracellular components, due to centrifugation during the experimental procedure. These
results suggest an anti-oxidative blood cell component that may quench the superoxide anion
production. As only haemolytic blood and neither RBC haemolysate nor plasma altered the
oxidative burst (at least without E. coli) and TNF release, one hypothesis would be that an
intracellular component and a plasma component may act together, e.g. glutathione and
glutathione peroxidase while quenching the superoxide. Because both oxidative burst and
TNF release were not affected by either whole blood or RBC’s, a steric interference between
E. coli and AM as the cause for the diminished phagocytosis seemed rather unlikely. Thus
Discussion
104
there are two possible explanations: 1. Intact blood cells bind on the macrophage surface,
thereby down-regulating the phagocytosis of E. coli particles and/ or 2. a preferential
phagocytic engulfment of RBC’s as compared to E. coli. The latter hypothesis is supported by
the finding that after haemorrhage large quantities of haemoglobin, haemosiderin and
ingested red blood cells can be detected in alveolar macrophages 197,198. However, further
work is needed to differentiate these possibilities.
In summary, the in vitro study has demonstrated a phasic response in alveolar macrophage
response to Gram-positive and Gram-negative stimuli that is a function of time after thoracic
trauma. The paradoxical combination of suppressed macrophage function such as
phagocytosis and oxidative burst, and hypersecretion of inflammatory mediators such as TNF,
may simultaneously render the host susceptible to both infectious complications and the
immune-mediated sequelae of SIRS and MOF.
Summary
105
6. Summary
Despite of variations in injury, due to animal as well as technical variabilities, we could
establish a reproducible in vivo model of blast thorax trauma. This includes not only a
standardized discharge of the blast pressure wave, but also a thorough monitoring of the blast
pressure wave parameters and an exact triggering depending on the respiratory cycle, to
monitor key blast wave properties and thus to be able to compare data over time. Our blast
wave generator develops a mechanical explosive that simulates blast pressure waves from
high explosives and produces pulmonary injuries in rats which tend to reproduce the spectrum
of injuries seen in blast victims and previous animal experiments. This model allows to study
primary blast injury without direct contact with the thoracic cage in a safe laboratory
environment.
The direct functional consequences of in vivo thoracic trauma were assessed in our ex vivo
isolated perfused rat lung model which has, to the best of our knowledge, not been described
previously. The correlation of pressure wave monitoring together with a validated injury score,
the BAL red blood cell counts and the ex vivo data collection in the isolated, traumatized and
perfused rat lung indicate that physical and biological impact may be matched in this setting.
Our present results illustrate that thoracic trauma deteriorates lung function, leads to important
oedema formation due to a loss of alveolar-capillary barrier function, depending on the trauma
intensity. The observation that especially the airway mechanics of traumatized rat lungs
appear to be more susceptible towards ex vivo mechanical ventilation and perfusion, provided
evidence for the possible development of a secondary injury called “ventilator-associated lung
injury”. This is of importance, since mechanical ventilation is one of the ultimate life-supporting
technologies in the therapy of critically ill patients with respiratory failure.
Pharmacological modulation during ex vivo lung perfusion indicated that the integrity of the
sodium channels is at least in part maintained after blast injury in this model. Thus, an
increased alveolar fluid clearance might be an underlying mechanism for the postulated fluid
resorption in vivo within the first six hours after trauma and assessed as decreased ex vivo
weight gain. Furthermore, β2-adrenergic therapy increased not only the oedema resorption
and/ or the oedema generation after trauma, but also improved the airway mechanics by direct
β2-adrenergic effects, possible independent of β-receptor-related fluid resorption. Thus β2-
adrenergic substances like terbutaline or formoterol appear to be beneficial after primary blast
injury in this model.
The sequelae of important alveolar haemorrhage and protein accumulation followed by a time-
dependent resolution, reflects not only a disrupted alveolar-capillary barrier induced by the
blast pressure wave, but also an enormous clearance capacity and/ or repair of the lung. One
Summary
106
biochemical response of the lung to the blast pressure wave was an immediate release of the
eicosanoids thromboxane and prostacycline, which have been reported in clinical studies to
be rather specific for the involvement of the lung in polytrauma patients. Thoracic trauma
resulted not only in an increased TNF and IL-6 release after 6 hours but also in a pronounced
CINC-3 production and neutrophil infiltration into the alveolar space. Likewise, matrix
metalloproteinase (MMP)-9/ –2 release and myeloperoxidase activity were detectable during
this time. The low IL-10 levels measured up to 24 hours after blast may favour cytokine
production in the alveolar environment in this setting. The appearance of increasing amounts
of the soluble TNF receptors (p55 and p75) in BAL fluids within the first 12 hours suggest an
early anti-inflammatory counterregulation, which in turn could be the cause for the “delayed”
and moderate TNF release after blast exposure.
With regard to the post-traumatic immune status, our in vitro results demonstrate a phasic
response of alveolar macrophages to endotoxin and whole bacteria stimulation, in terms of
both initially suppressed phagocytosis capacity, superoxide production (independent of
stimulation) and a delayed increase in TNF secretion. The dysregulation was shown to be at
least in part due to the accompanying alveolar haemorrhage and more precisely to different
blood components. However, also with respect to the in vivo results, this response may
represent a state of dysregulation, rather than a purely suppressed or hyperactive state.
Although the rats in our study appear to recover from the injury - confirmed by the parameters
we investigated in vivo, ex vivo and in vitro - the observed dysregulation in the lung, especially
in macrophage function may in fact increase their susceptibility to an infectious challenge or to
the development of multi-organ failure.
In conclusion, the present study demonstrates that the trauma model gives valid and
reproducible results, which in turn underscore the importance to address further questions on
the modulation of this injury in view of the major impact of trauma on especially young patients
and thus on the society.
Deutsche Zusammenfassung
107
7. Deutsche Zusammenfassung
Ein vorrangiges Ziel dieser Studie war die Erzeugung einer reproduzierbaren, isolierten in vivo
Druckwellenverletzung („Blast Injury“) des Thorax der Ratte. Trotz materialbedingter
Variationen und Schwankungen, die auf die verwendeten Tiere zurückgeführt wurden, ist uns
dies weitgehend gelungen. Die standardisierte Generierung der Druckwelle zusammen mit
einer reproduzierbaren Erfassung der Druckwellenparameter unter Berücksichtigung der
Atemlage des Tieres waren hierfür die Voraussetzung. Das für diese Versuche gewählte
Rattenmodell, welches ursprünglich zur Untersuchung von Explosionstraumen entwickelt
wurde, erlaubt die experimentelle Erzeugung einer isolierten Druckwellenverletzung der
Lunge, ohne direkten Kontakt mit den Strukturen des Brustkorbes. Die hierbei entstehende
Schädigung entspricht den beim Menschen auftretenden Verletzungen nach Exposition einer
Druckwelle, und ist vergleichbar mit zahlreichen tierexperimentellen Untersuchungen.
Durch die Verknüpfung zweier Modellsysteme, der in vivo erzeugten Druckwellenverletzung
des Thorax und der anschliessenden ex vivo Perfusion der isolierten Rattenlunge, konnten
erstmals die direkten Auswirkungen der Druckwelle auf die Physiologie und den Metabolismus
der Lunge untersucht werden. Hierbei konnte ein deutlicher Zusammenhang zwischen der
Intensität des auf die Ratte einwirkenden Druckes, also den physikalischen Eigenschaften und
dem daraus resultierenden Ausmass der Lungenschädigung gezeigt werden. Die
zugrundeliegenden Schädigungsparameter waren der Gehalt an roten Blutkörperchen im
Alveolarraum, der makroskopisch berechnete und validierte „Injury score“ als auch die ex vivo
erfasste Lungenfunktion. Basierend auf den Ergebnissen der ex vivo Perfusion konnte eine
direkte pulmonale Funktionsstörung nach Druckwelleneinwirkung gezeigt werden. Diese
beinhaltet eine Verschlechterung der Atemparameter gemessen an einem reduzierten
Atemzugvolumen und einem erhöhten Atemwegswiderstand der Lunge. Des weiteren kann,
aufgrund der Flüssigkeitseinlagerung (Ödembildung) in der Lunge, eine alveloär-kapilläre
Schrankenstörung postuliert werden. Der zur initialen Ödembildung vergleichsweise geringe
ex vivo Gewichtsanstieg zu einem späteren Zeitpunkt nach Trauma (drei und sechs Stunden),
legte die Vermutung einer Flüssigkeitsresorption und/ oder Verminderung der Ödemgenese in
vivo nach Thoraxverletzung nahe. Die Beobachtung, dass die Atemparameter traumatisierter
Tiere sich gegenüber derer „gesunder“ Lungen aus Tieren der Kontrollgruppe innerhalb der
Perfusion verschlechtern, lässt auf eine zusätzliche, ventilationsbedingte Verletzung
schliessen. Dies ist insofern von Bedeutung, als dass die mechanische Beatmung eine häufig
angewendete, lebenserhaltende klinische Maßnahme bei Patienten mit respiratorischer
Insuffizienz darstellt. Mit Hilfe ex vivo eingesetzter pharmakologischer Substanzen konnte
gezeigt werden, dass die Integrität der für die Flüssigkeitsresorption notwendigen Natrium-
Deutsche Zusammenfassung
108
Kanäle, nach einem Trauma zumindest teilweise besteht. Diese Erkenntnis führte zu der
Hypothese, dass die bereits erwähnte, postulierte Flüssigkeitsresorption in vivo,
möglicherweise auf die Aktivierung solcher Kanäle zurückzuführen ist. Des weiteren konnte
gezeigt werden, dass sich der Einsatz beta-2-adrenerger Substanzen nicht nur positiv auf
Ödemresorption und/ oder die Hemmung der Ödemgenese auswirkt, sondern auch beta-
rezeptor-abhängig die Atemparameter der Lunge nach Trauma verbessern. Beta-2-adrenerge
Substanzen wie Terbutalin und Formoterol, können daher im Modell der ex vivo
Lungenperfusion nach in vivo Druckwellenverletzung als therapeutisch wirksam angesehen
werden. Die traumabedingten Folgeerscheinungen wie die starke Einblutung und
Proteinakkumulation in der Lunge machen eine Zerstörung der Lungenarchitektur deutlich.
Dennoch konnte eine zeitabhängige Verbesserung dieser initialen Schadensparameter
innerhalb von 96 Stunden nach Druckwelleneinwirkung beobachtet werden. Aufgrund dessen
kann von einer enormen Regenerationsleistung der Lunge ausgegangen werden.
Die Analyse biochemischer Parameter nach einem in vivo Thoraxtrauma, ergab eine direkte
Freisetzung der Eikosanoide Thromboxan und Prostazyklin. Eine derartige Freisetzung dieser
Metabolite wird in der Literatur als relativ spezifisch für die Beteiligung der Lunge im
Polytrauma angesehen. Weiterhin konnten ansteigende Mengen der Mediatoren Tumor-
Nekrose Faktor (TNF)-α und Interleukin (IL)-6, innerhalb von sechs Stunden nach Trauma
gemessen werden. Zusammen mit einer Freisetzung des chemotaktisch wirksamen
Metaboliten CINC-3 und einer Infiltration neutrophiler Granulozyten in die Lunge, deutete dies
klar auf eine traumabedingte Entzündungsreaktion hin. Unterstützt wurde diese Vermutung
durch die Messung von Enzymen, wie den Matrixmetalloproteinasen (MMP)-2/ -9, welche als
charakteristisch für eine Einwanderung bzw. das Vorhandensein neutrophiler Granulozyten
angesehen werden können. Die geringen Mengen an messbarem Interleukin (IL)-10, einem
anti-entzündlichen Mediator, könnten das Gleichgewicht zwischen pro-und anti-entzündlichen
Mediatoren nach Druckwellenverletzung zugunsten der pro-entzündlichen Metabolite
verschoben haben. Im Gegensatz dazu, konnten innerhalb der ersten zwölf Stunden
steigende Mengen der löslichen Tumor-Nekrose Faktor (sTNF)-Rezeptoren in der broncho-
alveolären Lavegeflüssigkeit (BAL) gemessen werden, was auf eine anti-inflammatorische
Gegenregulation nach einem Thoraxtrauma hindeutet. Über einen möglichen Zusammenhang
zwischen dem Auftauchen löslicher TNF Rezeptoren, von welchen eine TNF neutralisierende
Wirkung bekannt ist, und der verzögerten (TNF)-α Freisetzung nach einem Thoraxtrauma
kann spekuliert werden.
Im Hinblick auf eine mögliche post-traumatische Immunsuppression wurden isolierte, primäre
Alveolarmakrophagen aus traumatisierten Rattenlungen auf ihre Funktionalität hin untersucht.
Entscheidend für die Beurteilung waren die Fähigkeit zur Phagozytose, zur Bildung reaktiver
Deutsche Zusammenfassung
109
Sauerstoffmetabolite, wie Superoxidanionen als auch die Freisetzung des pro-entzündlichen
Metaboliten TNF. In diesen in vitro Versuchen konnte eine phasische Antwort der
Alveolarmakrophagen sowohl auf die Stimulation mit bakteriellen Bestandteilen
(Lipopolyssacharid (LPS) und Lipoteichonsäure (LTA)) als auch auf ganze Gram-positive und
Gram-negative Bakterien (Escherichia Coli/ Staphylococcus aureus) hin beobachtet werden:
Initial nach einem Trauma war sowohl die Phagozytosekapazität als auch die Fähigkeit zur
Generierung von Superoxidanionen deutlich vermindert. Im Gegensatz dazu waren diese
Funktionen zu späteren Zeitpunkten nach Trauma wieder vergleichbar mit denen der
Kontrolltiere, wohingegen die TNF Freisetzung der Alveolarmakrophagen traumatisierter Tiere
24 Stunden nach Setzen des Traumas deutlich erhöht war. In der vorliegenden Arbeit konnte
gezeigt werden, dass die beobachteten Veränderungen der Alveolarmakrophagen Funktionen
zumindest teilweise auf die traumainduzierte, massive, alveoläre Einblutung zurückgeführt
werden kann. Weiterführende Untersuchungen lassen unterschiedliche Blutkomponenten als
Ursache für die Störung der jeweiligen Funktionen vermuten. Unter Berücksichtigung der oben
beschriebenen metabolischen Konsequenzen nach einer Druckwellenverletzung der Lunge,
deuten diese in vitro Ergebnisse eher auf eine Trauma bedingte Fehlregulation, als auf eine
generelle Suppression bzw. Hyperreaktion hin.
Die Resultate dieser Arbeit machen deutlich, dass alle Parameter, gemessen in den
verschiedenen Modellsystemen (in vivo, ex vivo und in vitro), sich zeitabhängig nach einer
Druckwellenverletzung der Lunge normalisierten und auch keine offensichtlichen Anzeichen
einer Spätletalität zu verzeichnen waren. Dennoch ist eine erhöhte Empfindlichkeit gegenüber
bakterieller Infektionen, also auch die Entwicklung eines Multi-Organ Versagens (MOF) im
Zustand einer eingeschränkten Abwehr, wie die hier beobachtete durchaus vorstellbar.
Zusammenfassend konnte in der vorliegenden Studie gezeigt werden, dass das Modell des in
vivo erzeugten Thoraxtrauma ein geeignetes Modell zur Untersuchung des primären
Lungenschadens der Ratte nach Druckwelleneinwirkung darstellt. Die erzielten Ergebnisse
tragen nicht nur zum Verständnis der post-traumatischen Schädigung bei, sondern
unterstreichen auch in Anbetracht der Häufigkeit traumabedingter Todesfälle in unserer
Gesellschaft die Notwendigkeit weiterer Untersuchungen.
References
110
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9. Abbreviatons
AM alveolar macrophage ARDS acute respiratory distress syndrome AUC area under the curve BAL bronchoalveolar lavage BW body weight CINC chemokine-induced neutrophil chemotactic factor CL dynamic lung compliance COX cyclooxygenase E. coli Escherichia coli Fpre, Fpost pre-and post breathing frequency IL interleukin LDH lactate dehydrogenase LPS lipopolyssacharide LTA lipoteichoic acid LWR lung wet weight weight to body weight ratio LWW lung wet weight MMPs matrix metalloproteinases MPO myeloperoxidase NO nitric oxide PEEP positive end-expiratory pressure PGF1a prostacycline PIP positive inspiratory pressure PMN polymorphonuclear leukocytes Pp pressure peak Qi injury quotient RA airway resistance RBCs red blood cells Rp cracking pressure S. aureus Staphylococcus aureus SEM/ SD standard error of means/ standard deviation sTNFRs soluble tumor necrosis factor receptors t duration TNF tumor necrosis factor TXA2 thromboxane A2
∆W weight gain