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Structural and Functional Characteristics of a Soluble Form of Endoglin in the Context of Preeclampsia
by
Allison Gregory
A thesis submitted in conformity with the requirements for the degree of Master of Science
Graduate Department of Immunology University of Toronto
© Copyright by Allison Gregory 2011
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Structural and Functional Characteristics of a Soluble Form of Endoglin in the Context of Preeclampsia
Allison Gregory
Master of Science
Graduate Department of Immunology University of Toronto
2011
Abstract Endoglin is an auxiliary receptor for ligands of TGF-β receptor superfamily. It is an integral
membrane protein highly expressed in the vascular endothelium. It is also present in the placental
syncytiotrophoblast layer, and up-regulated during pregnancy. The expression of membrane
endoglin (mEng) is further increased in the placenta during preeclampsia, a pregnancy-specific
hypertensive syndrome. We hypothesize that the soluble form of endoglin (sEng) released from
the placenta leads to endothelial dysfunction and hypertension by disrupting normal BMP-9
signaling. We first analyze the ligand specificity of mEng by comparing endoglin-deficient and
normal endothelial cells. We show that the presence of mEng at the cell surface inhibits TGF-β1,
BMP-2, and BMP-7 induced Smad1,5,8 phosphorylation while potentiating BMP-9 induced
signaling. sEng has been shown to be elevated in the sera of preeclamptic women several weeks
before the onset of clinical signs of preeclampsia and is postulated to interfere with endothelial
cell function. We engineered a soluble form of sEng for both structural and functional studies.
We show that sEng binds to BMP-9 with a 2 nM affinity, much higher than observed for other
ligands. We also show that sEng can compete for BMP-9 binding to endothelial cells, resulting in
inhibition of downstream Smad1,5,8 phosphorylation. Our results suggest that sEng is
contributing to endothelial dysfunction and hypertension by dysregulating BMP-9 signaling in
the maternal vasculature.
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Dedication
To my family and friends for their love,
faith in me and constant support during the completion of my Master’s Degree.
&
Pete Mason for all his help, confidence, support and enthusiasm
he provided while I wrote my thesis.
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Acknowledgments I would like to thank my supervisor, Dr. Michelle Letarte, for giving me the opportunity to work
in her lab, and for all her guidance and support. Without her push and belief in me, I would have
never realized my potential in research as well as life in general. I would like to thank Dr. Luca
Jovine, from the Karolinska Institutet in Stockholm, Sweden, for allowing me to work in his lab
for 6 months. He gave me such an amazing opportunity and experience at the same time as
renewing my passion for protein biochemistry. I am also grateful to the members of my graduate
supervisory committee Drs. James Rini and Stuart Berger for all their help on this project.
I owe special thanks to Dr. Guoxiong Xu and Ling Han for getting me on my feet in both labs
and their willingness to answer my endless stream of questions. As well, I would like to express
my strong appreciation to Dr. Mirjana Jerkic for her constant positive reinforcement and for
giving me a motivational push when needed. I also extend my most sincere thanks to Zhijie Li,
from the Rini Lab, for all his time, guidance and involvement in performing the surface plasmon
resonance experiments.
My graduate studies would not have been the same without all the students from the Letarte lab;
Madonna, Josh, Daniella, Valentin and Niousha. I was also blessed to have the experience to
work with two amazing summer students, Joyce Li and Arvind Devanabanda. I was also
incredibly lucky to work with extremely welcoming and talented students in the Jovine Lab;
Amy, Elisa and Hamed.
Last but not least, I extend my most sincere thanks to the Ontario Graduate Scholarship and the
Heart and Stroke Foundation for their generous financial support.
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Acknowledgement of Contributions
Ling Han in Dr. Luca Jovine’s Research Team Supervised and assisted in the generation of stable cell lines, large scale protein expression and protein purification. This data was used to generate Figures 9 and 10. Dr. Guoxiong Xu
Performed TGF-β1, BMP-2 and BMP-9 stimulation experiments. The data was used to generate Figures 11A, 11B and 11D. Zhijie Li in Dr. James Rini’s Research Team Supervised and assisted with all surface plasmon resonance experiments. The data was used to generate Figures 14 and 15, as well as Table 3. Valentin Sotov Assisted with all the surface Plasmon resonance experiments. The data was used to generate Figures 14 and 15, as well as Table 3.
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Table of Contents 1 Introduction ................................................................................................................................ 1
1.1 TGF-β superfamily.............................................................................................................. 1
1.1.1 Ligands and receptors ............................................................................................. 1
1.1.2 Signalling pathways and downstream effects ......................................................... 2
1.2 Endoglin distribution, structure and function ..................................................................... 9
1.2.1 Endoglin expression profile .................................................................................... 9
1.2.2 Structural features of endoglin ................................................................................ 9
1.2.3 Association of endoglin with multiple members of the TGF-β superfamily ........ 12
1.2.4 Functional role of endoglin within the cell and the organism .............................. 13
1.3 Endoglin and disease ......................................................................................................... 14
1.3.1 Hereditary hemorrhagic telangiectasia ................................................................. 14
1.3.2 Cancer ................................................................................................................... 16
1.3.3 Preeclampsia ......................................................................................................... 18
1.4 Thesis objectives ............................................................................................................... 22
1.4.1 Rationale ............................................................................................................... 22
1.4.2 Hypothesis ............................................................................................................. 23
1.4.3 Specific objectives ................................................................................................ 23
2 Materials and Methods ............................................................................................................. 24
2.1 DNA Constructs ................................................................................................................ 24
2.2 Cell Culture ....................................................................................................................... 26
2.3 Transient transfection and small-scale protein expression ............................................... 26
2.4 Generation of protein and subsequent deglycosylation .................................................... 26
2.5 Cell-based stimulation and inhibition assays .................................................................... 27
2.6 Generation of stable cell lines and large-scale protein expression ................................... 27
2.7 Protein Purification ........................................................................................................... 28
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2.8 SDS-PAGE and Western blotting ..................................................................................... 28
2.9 BIAcore Biosensor Analysis ............................................................................................. 29
2.10 Analysis of Biosensor Data ............................................................................................... 30
2.11 Statistical Analysis ............................................................................................................ 30
3 Results : Generation of Materials for Structural and Functional Studies ................................. 31
3.1 The complete extracellular and orphan domains of endoglin are readily expressed and secreted as soluble proteins ............................................................................................... 31
3.2 Generation of deglycosylated forms of soluble endoglin ................................................. 34
3.3 Sub-cloning endoglin constructs into high-expression CHO vectors ............................... 38
3.4 Large-scale expression and purification of Eng1-586-His and Eng1-357-His proteins ... 40
4 Results : Functional Studies of Soluble Endoglin .................................................................... 44
4.1 Endoglin modulates the signaling of multiple TGF-β superfamily ligands ...................... 44
4.2 The soluble extracellular domain of endoglin can inhibit BMP-9 induced Smad1 phosphorylation ................................................................................................................. 47
4.3 Relative binding of immobilized purified soluble endoglin to ligands of the TGF-β superfamily ....................................................................................................................... 49
5 Discussion ................................................................................................................................ 57
5.1 Biochemical characterization of sEng .............................................................................. 57
5.1.1 Expression of sEng ............................................................................................... 57
5.1.2 Potential multiple forms of sEng .......................................................................... 58
5.1.3 Disulphide linkages ............................................................................................... 59
5.2 Functional understanding of sEng .................................................................................... 59
5.2.1 mEng role in modulating Smad1,5,8 signaling ..................................................... 59
5.2.2 sEng role in binding ligand and modulating Smad1,5,8 signaling ....................... 60
5.2.3 sEng in the context of PE ...................................................................................... 62
5.3 Concluding remarks .......................................................................................................... 64
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List of Tables Table 1 TGF-β superfamily of signaling components
Table 2 Primers used for cloning, site-directed mutagenesis and sub-cloning
Table 3 Kinetic and thermodynamic constants for the interaction of multiple ligands with
the extracellular domain of selected receptors using a simple computer generated
binding model
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List of Figures Figure 1 TGF-β signaling pathways in endothelial cells.
Figure 2 BMP signaling pathways in endothelial cells.
Figure 3 Schematic diagram of the endoglin protein.
Figure 4 Model of the angiotensin II type I receptor agonistic antibodies (AT1-AA)
mediated release of placental factors.
Figure 5 Cloning and expression of endoglin fragments.
Figure 6 Generation of deglycosylated endoglin fragments by site-directed mutagenesis.
Figure 7 Generation of deglycosylated endoglin fragments by kifunensine and EndoH
treatment.
Figure 8 Expression of endoglin fragments in vectors designed for large scale protein
generation.
Figure 9 Analysis of purified endoglin samples using coomassie blue stained SDS-PAGE
gels.
Figure 10 Size exclusion chromatography analysis of eluted Eng1-586-His.
Figure 11 Smad1 phosphorylation in response to stimulation by TGF-β superfamily
members.
Figure 12 Blocking of Smad1 phosphorylation by soluble ligand-binding receptors.
Figure 13 Analysis of the ability of sEng to inhibit ligand induced Smad1 phosphorylation.
Figure 14 Kinetic analysis of TGF-β1 and BMP-9 binding to their receptors, TBRII and
Alk1, respectively.
Figure 15 Kinetic analysis of TGF-β1, BMP-7 and BMP-9 binding to sEng.
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Figure 16 Model of the mechanism through which sEng contributes to endothelial cell
dysfunction in the context of PE
Abbreviations ActRII : Activin receptor type II
ACVRL1 : ALK1 gene (human)
ALK : Activin receptor-like kinase
AT1 : Angiotensin II type I receptor
AT1-AA : Angiotensin II type I receptor agonistic autoantibodies
AVM : Arteriovenous malformation
BMP : bone morphogenic protein
BMPRII : bone morphogenic protein receptor type II
CHO : Chinese hamster ovary
EndoH : endoglycosidase H
ENG : ENDOGLIN gene (human)
Eng : endoglin protein
Eng+/+ : Endoglin wild-type
Eng+/- : Endoglin heterozygous
Eng-/- : Endoglin homozygous null
eNOS : endothelial nitric oxide synthase
ET1 : endothelin-1
GDF : growth differentiation factor
GlcNAc : glucosamine
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HEK 293T : human embryonic kidney 293T cell
HHT : Hereditary Hemorrhagic Telangiectasia
HHT1 : Hereditary Hemorrhagic Telangiectasia type 1
HHT2 : Hereditary Hemorrhagic Telangiectasia type 2
HELLP : hemolysis, elevated liver enzymes, low platelets
HRE : hypoxia-responsive element
HUVEC : Human umbilical vein endothelial cells
I-Smads : Inhibitory Smads
Id-1 : Inhibitors of differentiation-1
IMAC : Ni2+ immobilized metal affinity chromatography
KD : affinity constant
mEng : membrane endoglin
MISRII : Mullerian inhibitory substance type II receptor
MT1-MMP : membrane-type 1 matrix metalloproteinase
PAI-1 : Plasminogen activator inhibitor-1
PE : Preeclampsia
R-Smads : Receptor activated Smads
sEng : soluble endoglin
sFlt1 : soluble fms-like kinase (soluble VEGF receptor type 1)
SPR : surface plasmon resonance
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TBRII : Transforming growth factor β receptor II
TGF-β : Transforming growth factor β
TNF-α : Tumor necrosis factor α
VEGF : vascular endothelial growth factor
ZP : Zona pellucida
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Chapter 1
Introduction
1 Introduction The transforming growth factor β (TGF-β) superfamily of cytokines is one of the most
ubiquitous regulators of embryonic development and of physiological and cellular processes. The
superfamily is composed of multiple ligands and receptors that lead to a complex signaling
network. Endoglin, an accessory receptor, has been shown to be a critical member of this family.
This transmembrane glycoprotein is predominately expressed on proliferating endothelial cells.
Through modulating the cellular response to multiple ligands from the TGF-β superfamily,
endoglin has a critical role in embryonic development and angiogenesis. Endoglin has also been
implicated in the pathogenesis of multiple diseases. Mutations in endoglin have been linked to
hereditary hemorrhagic telangictasia (HHT), an autosomal dominant vascular disorder. Endoglin
has also been implicated in tumor angiogenesis and a soluble form of the membrane protein has
been shown to be released in cancer. A similar form of soluble endoglin has been implicated in
the pathogenesis of preeplampsia, a pregnancy-related condition resulting in maternal
hypertension. The introduction will summarize briefly our knowledge of the TGF-β superfamily
with a particular emphasis on endoglin in terms of structure and function and its soluble form in
the context of preeclampsia.
1.1 TGF-β superfamily The TGF-β superfamily is a large family of evolutionarily conserved cytokines that include
transforming growth factor β (TGF-β), bone morphogenetic proteins (BMPs) and activins to
name a few (1-3). Also included in this family are all the corresponding membrane receptors (1-
3).
1.1.1 Ligands and receptors
The TGF-β superfamily of cytokines contain more than 30 structurally related polypeptide
growth factors, which include: TGF-β1, -β2, -β3; activins A and B; inhibins A and B; BMP-1 to
BMP-10; nodal and growth differentiation factors (GDFs) (1-3). These proteins all share a
conserved cystine knot structure (4). All are initially translated as a precursor protein, composed
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of a N-terminal pro-region and a C-terminal ligand (4). These precursors form covalently-linked
dimeric structures in the endoplasmic reticulum, and then the pro-region is cleaved (5). In most
cases, such as for BMPs, the pro-domain dissociates and the active ligand is released from the
cell (5). However, in the case of the TGF-βs, the pro-region remains non-covalently attached to
the ligand after secretion, requiring further steps for generation of an active ligand (6).
Briefly, ligands of the TGF-β superfamily initiate their cellular effects by interacting with a
heteromeric receptor complex at the cell surface (7). All individual receptors exist as disulphide
linked homodimers (7). The TGF-β superfamily of receptors can be divided into three broad
categories: type I, type II and type III (7). The subsequent information is summarized in Table 1.
The type I family, also known as Activin-like kinases (ALK), has seven members (ALK1 to
ALK7), which are serine/threonine kinases (8). The type I receptors can be separated into 3 main
groups based on sequence similarity: the ALK5 group which, includes the TGF-β type I receptor,
ALK5, the Activin receptor, ALK4, and the Nodal receptor ALK7; the ALK3 group, consisting
of the BMP type I receptors, ALK3 and ALK6; and the ALK1 group, with ALK1 and ALK2
interacting with different BMP/TGF-β/Activin family members (8, 9).
The kinase function of these receptors only becomes activated when phosphorylated by a type II
receptor (8, 9). The type II sub-family of receptors contains 5 members, which are all
constitutively active serine/threonine kinases (3). Type II receptors include the TGF-β type II
receptor, TBRII, the Activin and BMP/GDF type II receptors, ActRII and ActRIIB and BMPRII,
and the Mullerian inhibitory substance type II receptor, MISRII. The third category of receptors
(type III) is commonly referred to as accessory or co-receptors (10). The two main members of
this group are betaglycan and endoglin. These receptors function by modulating the signaling of
multiple members of the TGF-β superfamily.
1.1.2 Signalling pathways and downstream effects
TGF-β superfamily ligands interact with a heteromeric receptor complex on the cell surface
consisting of one of each of the type I and II receptors (11). The ligands have different affinities
for different type I and II receptor combinations, that can be modulated by the presence of a type
III receptor (3, 10). The ligand initially binds the ligand-binding receptor, type II for TGF-βs as
opposed to type I for BMPs, and initiates a conformational change (3, 12-14). This results in the
recruitment and binding of the appropriate second receptor, in turn resulting in receptor complex
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Table 1. TGF-β Superfamily Signaling Components
Receptor gene/protein
Ligands, binding partners Receptor Smad
Type I receptors
ACVRL1/ALK1 ACVR1/ALK2 BMPRIA/ALK3 ACVR1B/ALK4 TGFBR1/ALK5 BMPR1B/ALK6 ACR1C/ALK7
Activin A, BMP-9, TGF-β1, TGF-β3 Activin A, BMP-6, BMP-7, MIS, TGF-β1, TGF-β2, TGF-β3 BMP-2, BMP-4, BMP-6, BMP-7 Activin A, GDF-1, GDF-11, Nodal TGF-β1, TGF-β2, TGF-β3 BMP-2, BMP-4, BMP-6, BMP-7, GDF-5, GDF -8, GDF-9b, MIS, Nodal
1,5,8 1,5,8 1,5,8 2,3 2,3 1,5,8 2,3
Type II receptors
ACVR2/ActRII ACVR2B/ActRIIb BMPR2/BMPRII AMHR2/MISRII TGFBR2/TBRII
Activin A, BMP-2, BMP-6, BMP-7, GDF-5, GDF -8, GDF-9b, GDF-11, Inhibins A and B Activin A, BMP-2,BMP-6,BMP-7, GDF-5, GDF -8, GDF-11 Inhibins A and B, Nodal, BMP-2, BMP-4, BMP-6, BMP-7, GDF-5, GDF-6, GDF-9b MIS TGF-β1, TGF-β2, TGF-β3
Type III receptors (co-receptors)
Betaglycan Endoglin CRIPTO RGMA RGMB (DRAGON) HJV/RGMc (hemojuvelin)
Inhibins, TGF-β1, TGF-β2, TGF-β3 BMP-2,BMP4, BMP-7, GDF-5 Activin A, BMP-2, BMP -7, BMP -9, BMP-10, TGF-β1, TGF-β3 GDF-1, GDF-3, Nodal, TGF-β1 BMP-2, BMP-4 BMP-2, BMP-4 BMP-2, BMP-4
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formation (7, 15). The type II receptor then phosphorylates the type I receptor, causing activation
of the serine/threonine kinase activity (13, 16, 17).
The activated type I receptors mediate their cellular effects through phosphorylation of the Smad
proteins, a family of conserved dimeric transcriptional factors (18, 19). Phosphorylation of the
receptor Smads (R-Smads: Smad1, Smad2, Smad3, Smad5, Smad8) by the type I receptor results
in R-Smad activation (19). Phoshorylated R-Smads complex with the common Smad4,
translocate to the nucleus, and regulate gene expression (20, 21). Negative feedback in these
pathways is mediated by the inhibitory Smads (I-Smads): Smad6 and Smad7 (22, 23). While it
might seem like an infinite possibility of signalling pathways, commonly each type I receptor
only activates a defined subset of R-Smads. ALK4, ALK5 and ALK7 are specific for induction
of Smad2,3 phosphorylation, while ALK1, ALK2, ALK3 and ALK6 interact and activate
Smad1,5,8 (10) (Table 1).
In most cell types, TGF-β1 and -β3 signal via ALK5 and TBRII resulting in Smad2,3
phosphorylation (Fig. 1) (24). This pathway is known to inhibit cellular proliferation, induce
apoptosis, facilitate cellular adhesion, as well as promote homotypic cell aggregation. The
Smad2,3 pathway induces expression of plasminogen activator inhibitor-1 (PAI-1), a negative
regulator of cell migration and angiogenesis. TGF-β-induced Smad2,3 activation has also been
shown to increase expression of extracellular matrix components such as collagen and
fibronectin. However, in endothelial cells, TGF-β1,3 can also signal through ALK1, another type
I receptor only expressed in this cell type (Fig. 1). Although TGF-β/ALK5/Smad2,3 signalling
antagonizes TGF-β/Alk1/Smad1,5,8 signaling, ALK5 is essential for recruitment and activation
of ALK1 (25). Just as the receptors are antagonistic, so are the pathways, ALK1 and ALK5 have
opposite effects on endothelial cell migration and proliferation. The BMPs signal via multiple
type I receptors (ALK1, ALK2, ALK3, ALK6), resulting in Smad1,5,8 phosphorylation (Fig. 2)
(24, 26). While each BMP elicits its own unique cellular effect, in general, activation of the
Smad1,5,8 pathway induces expression of Id-1, an inhibitor of basic helix-loop-helix proteins
that promotes cell proliferation and migration (27). The complexity of these signaling pathways
is further complicated by the modulating effects of TGF-β superfamily type III accessory
receptors.
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Figure 1. TGF-β signaling pathways in endothelial cells.
Both ALK1 and ALK5 are functional TGF-β type I receptors in endothelial cells. The
constitutively active kinase, TβRII, binds TGF-β1 or TGF-β3 ligand, recruits ALK1 or ALK5 to
the complex and phosphorylates the type I receptor cytoplasmic domain. This signalling complex
may be modulated by endoglin, which can bind the ligand in association with TβRII. When
ALK5 is phosphorylated, it transmits signals through Smad2/3, while activated ALK1 signals
though Smad1/5/8. These receptor-activated Smads then bind the common partner Smad
(Smad4) and translocate to the nucleus, where they regulate gene transcription. It has been
proposed that TGF-β regulates the state of the endothelium via a fine balance between ALK1 and
ALK5 pathways. Activation of the ALK5 pathway could be involved in vessel homeostasis
through expression of proteinase inhibitors (eg. PAI-1), and the production of extracellular
matrix proteins. On the other hand, ALK1 activation may be involved in new vessel formation,
supported by expression of inhibitors of differentiation (Id-1) and genes involved in proliferation
and migration.
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Figure 2. BMP signalling pathways in endothelial cells.
ALK1, ALK2, ALK3 and ALK6 are all functional TGF-β type I receptors found on endothelial
cells. The ligand-binding receptors (ALK1, -2, -3, -6) bind the BMP ligand, and then recruit the
appropriate constitutively active kinase (BMPRII or ActRII). The type II receptor (constitutively
active kinase) phosphorylates the type I receptor cytoplasmic domain. This signaling complex
may be modulated by endoglin, which can only bind ligand in association with the ligand
binding receptors. Endoglin has been shown to interact with BMP-2, BMP-7 and BMP-9. When
the type I receptor is phosphorylated, it transmits signals through Smad1/5/8. These receptor-
activated Smads then bind the common partner Smad (Smad4) and translocate to the nucleus and
regulate gene transcription. Activation of the Smad1/5/8 pathway is associated with expression
of inhibitors of differentiation (Id-1) and genes involved in proliferation and migration.
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1.2 Endoglin distribution, structure and function
1.2.1 Endoglin expression profile
Endoglin, a type III accessory receptor, is a membrane protein that was first identified, cloned
and sequenced in our laboratory. It was initially discovered on a lymphoblastic cell line derived
from a pre-B acute lymphoblastic leukaemia, the HOON pre-B cell line, using the monoclonal
antibody 44G4 (28). Use of the same antibody showed strong reactivity with endothelial cells
from capillaries, arterioles and venules in a variety of tissues ranging from lymph nodes, tonsils,
thymus, spleen, kidney, liver and lungs (28-30). This predominant expression in the vascular
endothelium led to endoglin being classified as an endothelial cell marker (CD105) at the Vth
International Leukocyte Workshop (30). Endoglin expression appears to be regulated by the
activation status of the endothelium and is increased during the angiogenic process (31). In fact,
endoglin is now widely used as an immunohistochemical marker of tumor angiogenesis (32).
Endoglin expression is not only increased on blood vessels undergoing angiogenesis, but also
during an inflammatory state, in association with infiltrating cells (33). Endoglin is also highly
expressed by the syncytiotrophoblast layer, which is the outer-most layer of the placenta, bathed
in maternal blood (34). This expression is further increased if the mother is suffering from
preeclampsia, a pregnancy related condition associated with hypertension (35). Endoglin
expression is also highly upregulated on human endocardial cushion tissue mesenchyme during
heart septation and valve formation, but returns to baseline as the valves mature (36).
Endoglin is also expressed by erythroid precursors (37), leukemic cells of the lymphoid and
myeloid lineages (37, 38) and mesenchymal stem cells (39). Endoglin is induced upon activation
of peripheral blood monocytes into macrophages (40). It is also expressed by vascular smooth
muscle cells, as well as fibroblasts (41, 42).
1.2.2 Structural features of endoglin
The human CD105 gene was located to chromosome 9q34, identified using fluorescence in situ
hybridization; the coding region contains 14 exons (43, 44). This sequence codes for a type I
integral membrane protein (45). Endoglin is composed of a large extracellular domain with a
short cytoplasmic domain (45). Between species, endoglin exhibits a fair degree of similarity,
with the most highly conserved regions being the transmembrane and cytoplasmic domains. The
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human and murine proteins share overall 74% identity, with 95% sequence identity in the
transmembrane and cytoplasmic domains (42, 46). This could indicate that the cytoplasmic
domain, while having no known enzymatic activity, may be critical for endoglin function within
the cell. The closest known relative of endoglin is betaglycan, another TGF-β superfamily type
III receptor (47). Overall, they share a significant sequence homology, particularly in the
transmembrane and cytoplasmic domains (47).
Endoglin is composed of an N-terminal orphan domain followed by a zona pellucida (ZP)
domain, juxtamembrane region, transmembrane region and short cytoplasmic domain (48, 49)
(illustrated in Figure 3). The orphan domain covers amino acids 1-357 and is termed orphan
since it has no known structural or functional homologue. The ZP domain consists of
approximately 260 amino acids with 8 conserved cysteine residues (48, 50). This domain can be
divided into two ZP sub-domains (ZP-N and ZP-C). The ZP-N sub-domain is highly conserved
throughout most ZP proteins, while more variation can be observed in the ZP-C (48). Endoglin
has a very similar ZP-N region to other ZP proteins, such as betaglycan, but with a divergent ZP-
C sub-domain (48). The ZP domain can be involved in receptor oligomerization, as in the case
for the ZP proteins surrounding the oocyte; however there is no evidence showing that endoglin
forms oligomeric chains at the cell surface through the use of its ZP domain (48). As mentioned
previously, while the entire protein shares roughly 70% homology between different species, the
transmembrane and cytoplasmic domains of endoglin are highly conserved (27). The
cytoplasmic domain, while having no enzymatic activity, can be phosphorylated by
serine/threonine kinases, and likely contributes to the function of endoglin in the cell (51).
At the cell surface, endoglin exists as a 180 kD disulphide-linked homodimeric protein referred
to in this thesis as membrane endoglin (mEng) (28, 29). The exact site of the interchain
disulphide linkage remains unknown. Some believe that it is located at Cys582, however this
residue is not conserved in all species such as mice, which still express a disulphide-linked
homodimer (51). A study that utilized a chimaeric construct encoding the N-terminal sequence of
monomeric PECAM-1 (CD31) antigen fused to residues Ile281-Ala658 of endoglin was
expressed as a dimer, suggesting that cysteine residues contained within fragment Cys330-
Cys412 are involved in the intrachain disulphide bond formation (52). More work needs to be
done to elucidate the exact residues involved.
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Figure 3. Schematic diagram of the endoglin protein.
Endoglin is an integral membrane protein. It is composed on an N-terminal signal peptide (1-26),
an orphan domain (27-357), zona pellucida domain (358-586), juxtamembrane region,
transmembrane region and short cytoplasmic domain. Within the cell it exists as a disulphide
linked homodimer. The polypeptide structure is also illustrated with cysteine residues (•)
numbered according to their position in the endoglin sequence.
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Endoglin is a highly glycosylated protein with five potential sites for N-linked glycosylation
(Asn88, Asn102, Asn121, Asn134, Asn307) within the orphan domain (45). Purified endoglin
showed a reduction of 20 kD when treated with N-glycosidase or Endoglycosidase (29),
suggesting that at least some of these sites are glycosylated. It has yet to be determined if these
sites confer structural or functional importance. There is also evidence for the presence of O-
linked glycosylation (45). The extracellular region extending from amino acids 311 to 551 is rich
in serine and threonine residues, a characteristic of an area rich in O-glycans. This was
confirmed by an observed 15 kD reduction following treatment of endoglin with O-glycanase
and neuraminidase (29).
Currently little is known of the actual three-dimensional structure of endoglin (49). Using single
particle electromicroscopy, the structure of the extracellular domain was determined to a
resolution of 25Ǻ (49). The molecular reconstruction suggested that endoglin might exist as a
dome formed of two anti-parallel oriented monomers. The use of data fitting also suggested that
each endoglin monomer itself was made up of three well defined regions, one orphan domain
and two ZP domains (ZP-N and ZP-C). In contrast, recent experiments using small angle X-ray
scattering revealed that endoglin might exist in a more elongated dimeric conformation (53). The
information obtained from these structural studies has been very useful; however, a higher
resolution structure is needed to further our understanding of endoglin. The generation of a high-
resolution three-dimensional image of endoglin using X-ray crystallography is the next step in
the quest to better understand not only the biochemistry of this highly important protein but its
functional role as well.
1.2.3 Association of endoglin with multiple members of the TGF-β superfamily
Endoglin bound to ligand can be isolated as a complex with type I and type II receptors, using
cross linkers with isolated cells and radioactive ligand (54). Initially, it was determined that
endoglin binds TGF-β1 and TGF-β3 but not TGF-β2, in contrast to betaglycan, which can bind
all three isoforms (54-56). Binding of TGF-β was originally demonstrated in human umbilical
vein endothelial cells (HUVEC) (54), then in human bone marrow stromal cells (57), and
haematopoietic cells (58). In view of the much lower number of receptors type I and II, relative
to the amount of endoglin present at the cell surface, it was concluded that only a small fraction
of endoglin was part of a TGF-β receptor complex (59). In vitro co-immunoprecipitation studies
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of endoglin with type I and type II receptors indicated that endoglin can also interact with
activin-A, BMP-7, and BMP-2 (54, 59, 60). Each of these interactions required co-expression of
the ligand-binding kinase receptor (59, 60). Accordingly, endoglin binds TGF-β1 and TGF-β3 by
interacting with TBRII. It can interact with activin-A and BMP-7 via their respective ActRII and
ActRIIB receptors, and with BMP-2 via ALK3 and ALK6. More recently, it was shown in
transfection experiments that endoglin could bind with high affinity to BMP-9 and BMP-10 in
the absence of the ligand-binding kinase receptor, ALK1 (61). Over-expression of endoglin also
increased BMP-9 responses (62).
Protein-protein interaction, co-immunoprecipitation, cross-linking, phoshorylation and functional
experiments have been used to determine the interactions of endoglin with other receptors of the
TGF-β superfamily. Endoglin has been found to interact with ALK5 and TBRII through both its
extracellular and cytoplasmic domains (51). Endoglin has only been shown to interact with one
other receptor via its cytoplasmic domain, ALK1 (63). The extracellular region is much more
likely to interact with other receptors (32).
1.2.4 Functional role of endoglin within the cell and the organism
The evidence to date suggests TGF-β superfamily auxiliary receptors do not have an intrinsic
signaling function but regulate ligand access to the signalling receptors. Betaglycan has been
characterized as facilitating TGF-β binding to its kinase receptors (64). The exact mechanism
through which endoglin modulates signalling remains to be determined. Several studies suggest
endoglin functions as an ancillary receptor that contributes to the TGF-β superfamily system of
regulation (27). A significant portion of the endoglin research thus far has focused on its
involvement in TGF-β signalling. Human U937 myelomonocytic cells over-expressing endoglin
were shown to block the following normal TGF-β1 responses: inhibition of cellular proliferation,
down-regulation of c-myc mRNA, stimulation of fibronectin synthesis, cellular adhesion, and
phosphorylation of PECAM-1 (65). Rat myoblasts transfected to over-express human endoglin
showed similar effects (60). In HUVEC cells, which naturally express significant amounts of
endoglin, an antisense approach was used to reduce expression, resulting in an increase of TGF-
β1 inhibitory effects on cell proliferation and migration (66). It has also been shown that
ALK1/Smad1,5,8 activation is enhanced in endothelial cells lacking endoglin, suggesting that
endoglin may also inhibit this pathway (67). However other in vitro studies have shown that
14
endoglin promotes the effects of ALK1 in endothelial cells (63). Relatively little is known
regarding endoglin function in BMP signalling. It has been shown that expression of endoglin
can enhance BMP-7 and BMP-9-induced Smad1,5 activation and responses, although the
mechanism by which this occurs is largely unknown (62, 68).
Endoglin is important in development since endoglin null (Eng-/-) mice are embryonic lethal at
E10.5 with cardiac and vascular defects (69-71). There is vessel rupturing and a lack of
endothelial-mesenchymal transition. Failed endocardial cushion formation, essential for valve
development and heart septation, and pericardial edema were also detected (69). However the
vasculature appears normal before E8.5. In vitro angioblast differentiation in Eng-/- embryonic
stem cells was found to be unaffected by the loss of endoglin expression. The endothelial cell
network in Eng-/- embryos also appeared to be normal. Endoglin has been implicated in early
hematopoietic development. In vitro differentiation assays showed that Eng-/- mouse embryonic
stem cells have reduced myelopoiesis and erythropoiesis, whereas generation of lymphoid and
vascular precursors was unaffected (72).
1.3 Endoglin and disease The importance of endoglin in normal function is highlighted by the fact that alterations in
normal endoglin expression have been associated with multiple disease states (73). Mutations in
the ENG gene lead to a vascular disease called hereditary hemorrhagic telangiectasia 1 (HHT1),
also known as Rendu-Osler-Weber syndrome (43). The observation that endoglin expression is
strongly up-regulated in the endothelium of various tumor tissues led to the discovery that
endoglin is important, and even critical, in tumor angiogenesis (32). A soluble form of endoglin
(sEng) has also been seen to be shed in cancer (32). A circulating form of sEng has also been
implicated in preeclampsia, contributing to hypertension, one of the trademark symptoms (35).
This section will explore the role of endoglin in these disease states.
1.3.1 Hereditary hemorrhagic telangiectasia
HHT is an autosomal dominant disorder with variable penetrance that is characterized by
aberrant vascular development (74). HHT is not constrained by race or ethnicity, having a wide
geographic distribution. Epidemiological studies have revealed an incidence of one in 5000
people (75, 76). Generally, clinical symptoms present during puberty. Classical symptoms
15
include spontaneous epistaxis (nosebleeds) and mucocutaneous telangiectases, which are
generally the first disease manifestations (74). In addition, arteriovenous malformations (AVMs)
in lung, brain, and liver and gastrointestinal telangiectases are the most severe consequences of
this vascular disease. AVMs, like telangiectases, are direct connections between arteries and
veins, bypassing the capillary bed (77). The shunting of blood through these lesions can lead to
serious complications such as gastrointestinal bleeding, high cardiac output heart failure,
hypoxemia, stroke, brain abscess and fatal haemorrhage (77, 78). Pulmonary AVMs are
generally the first to become apparent, starting at puberty, with other characteristics of HHT
developing with age (79).
Genetic linkage studies of families with HHT identified two disease associated loci, the ENG
gene coding for the co-receptor endoglin (HHT1), and the ACVRLI gene coding for the ALK1
receptor (HHT2) (43, 80). In HHT1, 311 unique mutations in ENG, all contained within the
extracellular domain, have been identified (74). These mutations are generally unique to a
particular family, and include deletions, insertions, missense, and nonsense mutations (77, 81).
ENG mutations result in unstable mRNA and protein, such that mutant proteins are rarely
detectable (81-85). Our laboratory has characterized HHT1 as a haploinsufficiency-related
condition, as opposed to a dominant negative genetic disease, since we demonstrated that
endothelial cells from HHT1 patients express half the normal amount of endoglin. Further
support for the haploinsufficiency model is obtained from the fact that multiple unique mutations
of different types result in the same HHT phenotype (86). In the case of HHT2, 249 unique
mutations in ACVRL1 have been identified (74). In contrast to ENG mutations, ACVRL1
mutations, largely missense, can be located in any of the extracellular, transmembrane or
cytoplasmic domains. The majority of mutations affect protein folding and stability (74). Studies
from our laboratory have demonstrated that HHT2 is also characterized by haploinsufficiency.
There were reduced ALK1 protein levels in HUVEC samples of newborns with an ALK1
mutation (87, 88).
HHT is therefore due to a loss of function of endoglin and ALK1 in endothelial cells, where both
genes are expressed. However, the mechanisms through which these receptors normally function
are still being explored. This pursuit is impeded by the level of complexity associated with the
TGF-β superfamily signalling in endothelial cells. Firstly, TGF-β can signal through both the
ALK5/Smad2,3 pathway as well as the ALK1/Smad1,5,8 pathway, having opposing effects on
16
endothelial cell proliferation and migration (25, 89). The presence of these two pathways may
allow TGF-β to function in a dose-dependent manner in endothelial cells, promoting
proliferation and migration at low concentrations, while inhibiting these responses at higher
ligand concentrations (25). The intricacies of this potentially functional balance are still to be
determined.
It has been proposed that endoglin may have a protective effect against hypoxia and/or TGF-β
induced apoptosis (90). The reduced endoglin expression in HHT may lead to massive apoptosis
in capillary ECs, resulting in the loss of capillaries and ultimately development of an
arteriovenous shunt. These malformations may appear only at distinct locations because of the
need for an external trigger such as inflammation or injury, which are known to cause an
upregulation in endoglin expression in known disease states (27, 91). This two hit model stresses
the importance of the protective effects of endoglin. However, this model does not highlight the
importance of ALK1, which is also implicated in HHT. ALK1 has been identified as the true
type I receptor for BMP-9 (61). This ligand has also been shown to interact with endoglin in the
absence of the ligand-binding kinase receptor (61). This suggests that the HHT phenotype is
associated with decreased ALK1/Smad1,5,8 signalling. The potential role of BMP-9 in HHT
must be considered. Clearly, further investigation is required to understand the role of endoglin
and ALK1 in the pathobiology of HHT.
1.3.2 Cancer
It has been established that endoglin is expressed at low levels in resting endothelial cells but is
upregulated in the vascular endothelium at sites of active angiogenesis (32). While angiogenesis
is a normal physiological event, it is also critical for tumour growth, which is dependent on a
continuous supply of oxygen and nutrients (27). As in the case of normal angiogenesis, the role
of endoglin in tumor angiogenesis is shrouded by the complexity of the TGF-β superfamily. In
tumors, enhancement of endoglin expression in endothelial cells is likely due to hypoxic
microenvironments (32). In support of this view, a hypoxia-responsive element (HRE) has been
characterized downstream of the main transcription start site in the ENG gene. Under low-
oxygen conditions, the HIF-1 transcription factor complex binds the HRE and effectively
increases endoglin promoter activity (92). This elevated endoglin expression is correlated with
the proliferation of tumor endothelial cells (93). This has been shown to have a physiological
17
effect with Eng+/- mice having reduced angiogenic responses and consequently reduced tumor
angiogenesis (94).
As well as being functionally important for tumor angiogenesis, this increased endoglin
expression on tumor vessels has a multifaceted clinical value (32). Endoglin staining in
microvessels has important prognostic value (32). Monoclonal antibodies to endoglin show
greater specificity for tumor microvasculature, a prognostic indicator for multiple human tumors,
than other endothelial markers such as CD31, CD34 or vWF (31, 95-98). This has been
confirmed in multiple types of solid tumors such as breast carcinoma, prostate cancer and non-
small cell lung cancer to name a few (97-99). As well as having prognostic value, endoglin
expression has diagnostic value (32). Labelled antibodies to endoglin were shown to effectively
accumulate in tumor specific tissue and were detectable with a high signal to noise ratio,
suggesting that endoglin is a good target for tumor imaging (100-102). Using a similar
mechanism, endoglin was found to be an exceptional target for anti-angiogenic therapy, aimed at
preventing the development of new blood vessels within the tumor (32). In vivo studies revealed
that injecting naked antibodies to endoglin in mice with human breast or colon cancer
xenographs was associated with significantly smaller tumors and greater survival rates as
compared to controls (103, 104). Taken together, these findings indicate that while endoglin
promotes tumor angiogenesis, it also has potentially great prognostic, diagnostic and therapeutic
value as a targeted marker.
Endoglin expression has also been detected on tumor cells of human sarcoma, melanoma,
carcinoma and leukemia origin (105, 106). Endoglin expression is differentially regulated in a
variety of tumors and correlates differently with tumor progression and metastatis, depending on
cancer type. Endoglin expression is downregulated on malignant or metastatic prostate cancer
cell lines as compared to the non-tumorigenic counterparts (107). Similarly, downregulation of
endoglin expression in esophageal cancer cells is correlated with disease progression (108).
Endoglin’s ability to antagonize TGF-β-mediated cell migration has been suggested as a possible
mechanism. However, recently, endoglin was shown to have a pro-invasive role in metastatic
breast cancer cells (109). Ectopic overexpression of endoglin enhanced migration and
invasiveness in breast cancer cells. Endoglin clearly can play an important role in sporadic
cancer, however, it may be context-dependent and the mechanism still needs to be determined.
18
A number of laboratories have also reported the detection of increased levels of a soluble,
circulating form of endoglin (sEng) in serum, plasma or other fluids from cancer patients (110).
Recently, it was shown that an 80 kD form of sEng was released from the surface of HUVEC
cells after proteolytic cleavage by membrane-type 1 matrix metalloproteinase (MT1-MMP)
(111). Using cleavage site mutants, it was shown that MT1-MMP cleaved endoglin between
amino acids 586 and 587. Cleavage at this site results in the release of a nearly full-length
endoglin extracellular domain (~80 kD) into circulation. There is still a significant amount of
information to be determined regarding the cleaved protein. Its exact origin is unclear, being
either the neovasculature or the cancer cells themselves, or both (110, 112, 113). Its influence on
tumor development remains to be elucidated, but sEng has been identified as a marker of poor
prognosis in cancer patients (110, 112). The measured serum levels of sEng were significantly
higher in individuals with metastatic solid malignancies, mainly breast and colorectal, as
compared to controls (112, 113). Increased levels of sEng in serum and urine have also been
detected in patients with prostate cancer, making sEng a marker for the potential diagnosis of
prostate cancer (114).
1.3.3 Preeclampsia
Both membrane (mEng) and soluble (sEng) forms of endoglin have been implicated in another
disease termed preeclampsia. Preeclampsia is a major obstetric problem leading to substantial
maternal, fetal and neonatal morbidity (and mortality) in 5-7% of pregnancies worldwide,
especially in developing countries (115). This disease can manifest in two non-mutually
exclusive ways, as fetal and maternal syndromes (116). The fetal syndrome can be characterized
by fetal growth restriction, reduced amniotic fluid and abnormal oxygenation (117-119). This
placental dysfunction is thought to give rise to the maternal syndrome that can be further divided
into severe, early-onset (that develops before 34 weeks) and mild, late-onset (that appears after
week 34) (115, 118). Mild, late-onset is characterized by hypertension and proteinurea. Severe
preeclampsia can lead to the appearance of the HELLP (hemolysis, elevated liver enzymes, low
platelets) syndrome and seizures (eclampsia) (115, 120). There are many theories concerning the
pathogenesis of preeclampsia, but very little is understood about the patho-mechanism of this
pregnancy-related condition.
19
The importance of the fetus and placenta in the development of PE can be seen by the fact that
symptoms of disease rapidly disappear upon delivery (115). Currently, this is the only known
treatment resulting in total relief of symptoms. It is presently believed that PE is induced by
placental ischemia that results in fetal distress and dysfunction (121, 122). This ultimately results
in the placenta releasing soluble factors into the maternal blood stream and causing the
symptoms associated with PE (35, 123). In normal pregnancy, the extravillous trophoblasts of
the placenta penetrate the maternal decidua and invade the maternal spiral arteries (124). The
spiral arteries then become extensively remodelled by the invasive trophoblasts. The once high-
resistance vessels become dilated, high-capacitance vascular channels that allow for fetal
perfusion. In preeclampsia, it has been shown that the trophoblasts do not invade the spiral
arteries to the same extent (124). This results in failure to convert the high-resistance vessels to
high-capacitance vessels (125). This causes decreased fetal circulation and ultimately leads to
placental and fetal ischemia. The exact events that lead to this improper vascular remodelling
remain to be determined.
This placental ischemia is thought to lead to fetal and placental distress, resulting in multiple
physiological changes. One such change is the increased expression of mEng. Expression of this
protein is naturally upregulated on the syncitiotrophoblast during pregnancy; however, women
with PE experience on average a fourfold increase in both mRNA and protein levels of mEng in
the placenta (35). This change is thought to be brought on by the hypoxic environment created
by the placental ischemia. As previously stated, endoglin expression can be upregulated by
hypoxia in endothelial cells (92). The HIF-1 transcription factor, known to be induced by
hypoxic conditions, has been shown to enhance endoglin promoter activity (92). It has also
recently been shown that levels of endoglin are up-regulated by low oxygen both in vitro, using
villous explants, and in vivo, using models of placental hypoxia pathology (126). The effect of
this increased expression, however, remains to be determined.
Placental ischemia has also been linked to the release of multiple factors into the maternal
circulation (121). These factors then target maternal endothelial cells resulting in endothelial cell
dysfunction, which in turn leads to hypertension and other clinical manifestations of the maternal
syndrome. It has been shown that two of these factors are sFlt-1 (soluble fms-like kinase, also
known as soluble VEGF receptor type I) and sEng, which can both be detected in the circulation
20
6-8 weeks before the onset of clinical symptoms (35, 123, 127-130). Elevated levels of these
factors have been shown to correlate with disease severity (35, 131).
Adenoviral expression of sEng in pregnant rats indicated that sEng can induce a significant
increase in arterial pressure, further increased by the presence of sFlt1 (35). Low levels of
proteinurea were also detected in sEng-treated rats, but nephritic damage was much more severe
in sFlt1-treated rats (35). sEng and sFlt1 in combination lead to proteinurea, severe hypertension
and the HELLP syndrome (35). While it is obvious that sEng plays an important role in disease
pathogenesis, the means through which it is released and the mechanism leading to endothelial
dysfunction are still largely unknown.
While sFlt1 is a splice variant, the 65 kD sEng is believed to be generated by cleavage of mEng
by a metalloproteinase (35). The exact form of sEng released into circulation is unknown, since
insufficient amounts of this soluble protein could be purified from maternal serum to perform C-
terminal sequencing (35). MT1-MMP has been implicated in mEng cleavage from endothelial
cells in the context of cancer; however, the product predicted to be Eng1-586 is larger (80kD)
than the sEng detected in PE (111).
Multiple mechanisms have been proposed to explain the release of sEng. Similar to mEng, the
levels of sEng are also positively correlated with hypoxic conditions. Low oxygen levels have
also been shown to upregulate multiple proteases, such as MT1-MMP; combined with increased
mEng expression, this may ultimately lead to increased release of sEng. A significant amount of
work has also linked this increased expression to a more immunological pathogenesis model
(115) (Fig. 4). Walluket et al. showed that women with PE have autoantibodies that stimulate the
angiotensin II type I receptor (ATI), which is an important component of the renin-angiotensin
system (132). Through activation of the ATI receptor, angiotensin II type I receptor agonistic
autoantibodies (ATI-AA) have been shown to produce preeclamptic symptoms in pregnant
women (133-135). It is suggested that placental ischemia leads to production of ATI-AA.
Pregnant rats exposed to chronic reduced uterine perfusion pressure (RUPP) showed the
presence of ATI-AA (136). These antibodies were also detectable between 18-22 weeks of
pregnancy in women with abnormal uterine perfusion determined by Doppler ultrasound (137).
ATI-AA from preeclamptic patients were shown to effectively interact with the ATI receptors in
pregnant mice and induce symptoms of disease, hypertension and proteinurea (138). The
21
Figure 4. Model of the angiotensin II type I receptor agonistic antibodies (AT1-AA)
mediated release of placental factors.
This diagram represents a possible signaling cascade by which placental ischemia leads to the
generation and release of AT1-AA. These antibodies are free to activate the angiotensin II type I
receptor (AT1R) which results in an increased expression of tumor necrosis factor-α (TNF-α).
This leads to the increased release of soluble factors into the maternal circulation. Soluble
endoglin (sEng), soluble VEGF receptor 1 (sFlt-1) and endothelin-1 have all be shown to
contribute to maternal hypertension in preeclampsia.
22
hypertension is thought to be partially mediated by the ability of ATI-AA to induce endothelin-1
(ET1) expression, a well-known vasoconstrictor. Injection of IgG from women with PE into
pregnant mice also showed that ATI-AA lead to increased placental sEng expression by ATI
activation (139). The mechanism is mediated by increased TNF-α expression in the placenta.
Both membrane and soluble endoglin expression were increased in human extravillous explants
treated with IgG from preeclamptic women, as compared to controls, and this was prevented by
the presence of a TNF-α inhibitor. Increased shedding of endoglin could also be mediated by the
ability of TNF-α to upregulate multiple proteases. Both hypoxia and agonistic antibodies
represent viable means of inducing the expression of both forms of endoglin, and are likely not
mutually exclusive (115).
While a significant amount of progress has been made in understanding the release of sEng,
these is still a large amount of work to be done in regards to the role of sEng in endothelial
dysfunction and ultimately hypertension. It has been shown that sEng inhibits TGF-β-mediated
eNOS-dependent vasodilatation (35). Both TGF-β1 and TGF-β3 induced vasodilatation in
isolated rat renal microvessels (35). sEng was able to attenuate these effects. TGF-β mediates
this effect via eNOS dephosphorylation at Thr495, which precedes activation of eNOS via
Ser1177 phosphorylation. TGF-β could act synergistically with VEGF, since VEGF induces
eNOS Ser1177 phosphorylation (140, 141). sFlt1 leads to hypertension by binding VEGF and no
longer allowing for eNOS activation or its downstream vasodilation (131). It is logical to
suggest sEng works in a similar manner. With the use of a radio-labelled binding assay, it was
found sEng significantly reduced the ability of TGF-β1 to bind TBRII (35). This would
effectively limit the ability of TGF-β to allow for eNOS activation. sEng also inhibited TGF-β1-
induced activation of the Smad2,3 pathway (35). Taken together, these data suggested that sEng
competes for TGF-β binding to its receptor; however, there is no direct evidence indicating that
sEng binds TGF-β in the absence of the ligand-binding receptor, TBRII.
1.4 Thesis objectives
1.4.1 Rationale
For a long time, it has been known that endoglin modulates the signalling of multiple members
of the TGF-β superfamily. Endoglin effects differ based on cell type and environmental milieu,
and are therefore context-dependent. The significant amount of research conducted thus far has
23
allowed us a basic understanding of endoglin biochemistry and function. Structural studies have
provided a globular image of endoglin; however, a higher resolution structure is needed to
further our understanding in both physiological and pathological settings.
Within the context of preeclampsia, a soluble form of endoglin is released from the
syncytiotrophoblast into the maternal blood stream. This soluble protein has been shown to
contribute to the development of high blood pressure, a characteristic symptom of preeclampsia;
however, the exact mode of action has yet to be understood. The current dogma is that soluble
endoglin sequesters TGF-β1,3, resulting in endothelial dysfunction and ultimately leading to
hypertension. However, it was shown that endoglin can only bind TGF-β1,3 in the presence of
TBRII. Interestingly, preliminary results have shown that endoglin may have the capacity to bind
BMP-9 in the absence of its ligand-binding receptor and this specificity may be more relevant to
the role of endoglin in preeclampsia.
1.4.2 Hypothesis
Soluble endoglin contributes to endothelial dysfunction within the context of preeclampsia by
binding and effectively competing for BMP-9.
1.4.3 Specific objectives
Our main objectives were:
I) To generate soluble and stable endoglin proteins that could be produced in large-scale
quantities for the generation of protein crystals for X-ray crystallography and for
functional studies.
II) To determine if soluble endoglin can interact with various ligands of the TGF-
β superfamily, in order to better understand how sEng leads to preeclampsia.
24
Chapter 2
Materials and Methods
2 Materials and Methods
2.1 DNA Constructs Constructs containing the full-length endoglin coding sequence (Eng1-658) and the extracellular
domain (Eng1-586) had been previously generated in the laboratory. They were inserted between
Kpn1 and Xba1 restriction sites in a modified version of the mammalian pCMV5 vector
(Invitrogen), with a C-terminal Flag-tag. All subsequent endoglin constructs (Eng1-357, Eng358-
581, Eng358-586) were generated by PCR amplifying segments of the full length human
endoglin sequence (accession number: NM_001114753) to contain Kpn1 and Xba1 restriction
sites to facilitate their subcloning into the pCMV5 vector with the C-terminal Flag-tag. The
forward (F) and reverse (R) primers used for cloning are shown in Table 2.
Glycosylation mutants were obtained by sequential sit- directed mutagenesis of glycosylation
sites from asparagine (Asn;N) to glutamine (Gln;Q) residues. Site-directed mutagenesis was
performed using the GeneTailor Site-Directed Mutagenesis kit (Invitrogen) along with KOD XL
DNA polymerase (Novagen). The protocol was optimized from the manufacturer’s
specifications. The primers are shown in Table 2.
Wild-type and glycosylation mutant forms of Eng1-586 and Eng1-357 were sub-cloned into
Chinese Hamster Elongation Factor 1 (CHEF1) plasmids pDEF28 and pNEF38 (CMC
Biologics) with a C-terminal 6xHis tag. The desired endoglin sequences were inserted between
Sal1 and Xba1, with the cut sites added to the inserts during PCR amplification. The primers are
shown in Table 2.
All constructs were confirmed by DNA sequencing and aligned to control sequence using Vector
NTI.
25
Table 2: Primers used for cloning, site-directed mutagenesis and sub-cloning
Purpose Construct Direction Cut Site
Primer
cloning Eng1-357 F Kpn1 5’-CCGGGTACCATGGACCGC GGCACGCTCCCTCTG-3’
R Xba1 5’-TAGTCTAGAGGACATGAGCA GCTCCGGGCTACA-3’
cloning Eng358-581 F Kpn1 5’-CCGGGTACCATGTTGATCCAGA CAAAGTGTGCCGAC-3’
R Xba1 5’-TAGTCTAGAACCAGACAGGTCA GGGCTGATGAT-3’
cloning Eng358-586 F Kpn1 5’-CCGGGTACCATGTTGATCCAGA CAAAGTGTGCCGAC-3’
R Xba1 5’-TAGTCTAGAGCCTTTGCTTGT GCAACCAGACAG-3’
mutagenesis Eng1-586-N-88-Q F n/a 5’-CTCTCCAGGCATCCAAGCAAC AAGGCACCTGGCCCCGA-3’
R n/a 5’-GCCTTGTTGCTTGGATGCCTG GAGAGTCAG-3’
mutagenesis Eng1-586-N-102-Q F n/a 5’-TGCTTCTGGTCCTCAGTGTAC AAAGCAGTGTCT-3’
R n/a 5’-TACACTGAGGACCAGAAGCA CCTCTCGGGG-3’
mutagenesis Eng1-586-N-121-Q F n/a 5’-TCCCACTGCACTTGGCCTACC AATCCAGCTTGG-3’
R n/a 5’-GTAGGCCAAGTGCAGTGGGA TTCCCAGGGC-3’
mutagenesis Eng1-586-N-134-Q F n/a 5’-TCCAAGAGCCCCCGGGGGTC CAAACCACAGAGC-3’
R n/a 5’-GACCCCCGGGGGCTCTTGGA AGGTGACCAG-3’
mutagenesis Eng1-586-N-307-Q F n/a 5’-TGGGGGAGGCCCGGATGCTC CAAGCCAGCATTG-3’
R n/a 5’-GAGCATCCGGGCCTCCCCCA GGAGGCCTTG-3’
sub-cloning All pDEF38-Eng1-586
F Sal1 5’-CCGCCGGTCGACATGGACCG CGGCACGCTCCCTCTG-3’
R Xba1 5’-TAGTAGTCTAGACTAGTGATG GTGATGGTGATGGCCTTTGCTTGTGCAACCAGACAG-3’
sub-cloning All pDEF38-Eng1-357
F Sal1 5’-CCGCCGGTCGACATGGACCG CGGCACGCTCCCTCTG-3’
R Xba1 5’-TAGTAGTCTAGACTAGTGATG GTGATGGTGATGGGACATGAGCAGCTCCGGGCTACA-3’
sub-cloning All pNEF38-Eng1-586
F Sal1 5’-CCGCCGGTCGACATGGACCG CGGCACGCTCCCTCTG-3’
R Xba1 5’-TAGTAGTCTAGACTAGTGATG GTGATGGTGATGGCCTTTGCTTGTGCAACCAGACAG-3’
sub-cloning All pNEF38-Eng1-357
F Sal1 5’-CCGCCGGTCGACATGGACCG CGGCACGCTCCCTCTG-3’
R Xba1 5’-TAGTAGTCTAGACTAGTGATG GTGATGGTGATGGGACATGAGCAGCTCCGGGCTACA-3’
26
2.2 Cell Culture Human renal epithelial (HEK) 293T cells (ATCC: CRL-1573) were cultured in DMEM medium
(GIBCO) and supplemented with 10% fetal bovine serum (GIBCO) and 5% antibiotics
(Penicillin/Streptomycin solution, GIBCO).
Immortalized mouse embryonic endothelial cells expressing either wild-type levels of membrane
endoglin (Eng+/+) or no membrane endoglin (Eng-/-) were originally developed in Letarte
laboratory from murine embryo and yolk sacs harvested at E9.0 of gestation (67). These cells are
cultured in MCDB 131 medium (GIBCO) supplemented with 15% fetal bovine serum (GIBCO),
5% glutamine solution (GIBCO), 5% antibiotics (Penicillin/Streptomycin solution, GIBCO) and
25 μg/ml endothelial mitogen (Biomedical Technologies Inc.).
2.3 Transient transfection and small-scale protein expression HEK 293T cells were transiently transfected with 1 μg of the indicated plasmids using
FUGENE6 (Roche) as described by the manufacturer. 24 h after transfection, cells were washed
with PBS (Invitrogen), and cultured for 24 h in DMEM without supplements. Culture media was
then collected, debris removed by centrifugation (4˚C, 15800xg, 5 min) and the media
concentrated 10-fold using an UltracelTM 10kD centrifugal filter unit (Millipore). Lysate
fractions were prepared by scraping cells and solubilizing in lysis buffer (50mM Tris-HCl pH
7.4, 100mM NaCl, 1mM EDTA, 1% Triton X-100, 10mM sodium pyrophosphate, 25mM NaF,
1mM Na3VO4, 1% ProteoBlockTM protease inhibitor cocktail (Fermentas)). Protein concentration
was determined by the Dc protein assay, a modified Lowry assay (Bio-rad), and samples
solubilised in SDS sample buffer (60 mM Tris-HCl pH 6.8, 2% Sodium dodecyl sulfate, 5%
glycerol, 10mM Dithiothreitol, 0.005% Bromophenol blue). Samples intended for non-reducing
gels were solubilised in the same SDS sample buffer only lacking the reducing agent,
Dithiothreitol.
2.4 Generation of protein and subsequent deglycosylation
HEK 293T cells were transiently transfected with the indicated plasmids using FUGENE6
(Roche) as described by the manufacturer. Cells were grown in complete medium (lacking
antibiotics) supplemented with 5 μM kifunensine (Toronto Research Chemicals). After 24 h,
cells were washed with PBS and cultured for 24 h in DMEM supplemented with 5 μM
27
kifunensine. Tissue culture supernatant containing the secreted proteins was harvested, debris
removed by centrifugation (4˚C, 15800xg, 5 min) and then concentrated 10-fold using an
UltracelTM 10kD centrifugal filter unit. Proteins contained in the media were deglycosylated with
EndoH (New England Biolabs). The EndoH was initially prepared by serial dilutions in 0.1 M
sodium acetate pH 5.2. Samples of concentrated media (20μl) were exposed to a range of EndoH
(100U, 200U, 400U) concentrations, and incubated for 3h at 4˚C (control) or 37˚C. The extent of
deglycosylation was monitored by immunoblot.
2.5 Cell-based stimulation and inhibition assays
In stimulation studies, equivalent numbers of endothelial cells were seeded in complete medium.
After 48 h, cells were starved for 3 h in serum-free medium and treated with increasing
concentrations of ligand (TGF-β1, BMP-2,7,9; R&D) for 30 min. Lysates were prepared by
scraping the cells and solubilizing in lysis buffer as described above. Protein concentration was
estimated and samples were further solubilized in SDS sample buffer (60 mM Tris-HCl pH 6.8,
2% Sodium dodecyl sulfate, 5% glycerol, 10mM Dithiothreitol, 0.005% Bromophenol blue).
Samples intended for non-reducing gels were solubilised in the same SDS sample buffer only
lacking the reducing agent, Dithiothreitol.
In inhibition studies, 5.0x105 endothelial cells were seeded in complete medium. After 48 h, cells
were starved for 2 h in serum-free medium, exposed to increasing concentrations of soluble
receptors (sAlk1, sEng, sTBRII ; R&D) for 1 hour and then treated with a defined concentration
of each ligand (TGF-β1, BMP-2,7,9; R&D). Lysates were collected as previously described.
Protein concentration was determined by the Dc protein assay, a modified Lowry assay (Bio-
rad), and samples were solubilized in SDS sample buffer (60 mM Tris-HCl pH 6.8, 2% Sodium
dodecyl sulfate, 5% glycerol, 10mM Dithiothreitol, 0.005% Bromophenol blue). Samples
intended for non-reducing gels were solubilised in the same SDS sample buffer only lacking the
reducing agent, Dithiothreitol.
2.6 Generation of stable cell lines and large-scale protein expression
For stable expression, dihydrofolate reductase-deficient CHO DG44 cells (Invitrogen), grown in
α-MEM medium (Invitrogen) supplemented with 10% fetal bovine serum (Invitrogen), were co-
28
transfected with the pDEF38 and pNEF38 CHEF1 vector pairs containing wild-type and triple
glycosylation mutant forms of Eng1-586 and Eng1-357 using the LipofectamineTM 2000 system.
Stably transfected clones were grown in α-MEM medium lacking hypoxanthine/thymidine, and
supplemented with 8% dialyzed fetal bovine serum (Invitrogen) and 0.8mg/ml G418
(Invitrogen). 96 single cell colonies per cell line were selected and plated at constant density.
Clones expressing high levels of the C-terminally histidine-tagged endoglin constructs were
identified by immunoblot. The 8 clones (12 for Eng1-357-N-121,134,307-Q-His) expressing the
highest levels of C-terminally histidine-tagged endoglin constructs were selected, plated at
constant density, media analyzed via immunoblot and cells counted at time of harvest. The 3 best
clones for each cell line, selected based on endoglin production and low cell number at time of
harvest, were amplified and stored.
For large scale protein expression, selected stable cell lines were grown in 3L spinner flasks at
initial concentrations of 0.3x106 cells/ml in serum-free medium HyQ SFM4CHO-utility medium
(HyClone). Cells were grown until they reached 60% viability (roughly 2-3 weeks), then the
media was harvested.
2.7 Protein Purification
Secreted sEng proteins were captured from conditioned medium by batch binding with Ni-NTA
Superflow beads (QIAGEN) overnight. The IMAC column was gravity packed and then
equilibrated with Buffer A (20 mM NaHEPES [pH 7.8], 150 mM NaCl, 20 mM Imidazole).
Bound protein was eluted using a 20 mM to 500 mM imidazole gradient for 100 min at 1ml/min.
Subsequently, the eluted peak was concentrated and then dialyzed for 24 h against gel filtration
buffer (10mM Tris-HCl pH 7.2, 50mM NaCl). Samples were subjected to size exclusion
chromatography using a 10/300 Superdex-200 column (GE Healthcare) equilibrated against gel
filtration buffer and fractionated at 0.3 ml/min in 10mM Tris-HCl pH 7.2, 50 mM NaCl.
2.8 SDS-PAGE and Western blotting
All protein samples were run on NuPAGE Bis-Tris 4-12% SDS-PAGE gels (Invitrogen) for
approximately 60 min at 170V, followed by electrophoretic transfer to nitrocellulose (Millipore)
for 90 min at 200 mA. Blocking proceeded for 90 min at room temperature in blocking solution
[5% milk powder (Bio-Rad) in Tris-buffered saline/0.1% Tween-20 (TBS-T)]. The blots were
29
stripped using a 1M glycine solution (pH2.5) and washed with TBS-T. Western blot (or
immunoblots) were used to detect expression of endoglin constructs using a primary antibody,
rabbit polyclonal H300 (Santa Cruz; 1:1000), that recognizes both reduced and non-reduced
endoglin. Dot blot and Western blot experiments, for analysis of stably transfected clones, used
the primary mouse monoclonal antibody to the 5His tag (QIAGEN; 1:1000). For functional
studies, rabbit polyclonal anti-phospho-Smad1/5/8 (Cell Signalling; 1:1000), and mouse
monoclonal anti-Smad1(Santa Cruz; 1:1000). Secondary antibodies were horseradish
peroxidase-conjugated AffiniPure sheep anti-mouse and donkey anti-rabbit (GE Healthcare,
1:10,000). Bands were visualized using Western LightingTM Chemiluminescent Reagent Plus
(PerkinElmer) followed by exposure to HyperfilmTM ECLTM (Amersham Biosciences). All
immunoblots were performed in duplicate.
2.9 BIAcore Biosensor Analysis
All analyses were carried out on a BIAcore X (BIAcore, Uppsala, Sweden) at 25̊ C. Research
grade CM5 sensor chips, N-hydroxysuccinimide (NHS), N-ethyl-N’-(3-diethylaminopropyl)
carbodiimide (EDC), and ethanol-amine hydrochloride were purchased from the manufacturer
(BIAcore Inc.). sALK1-Fc and sTBRII-Fc were purchased from R&D. sEng was generated and
purified as previously described. All ligand/analytes (TGF-β1, BMP-2,7,9) were purchased from
R&D and prepared according to the manufacturers specifications. All buffers were filtered and
degassed.
For amine coupling, carboxymethylated dextran surfaces on CM5 chips were activated using the
standard NHS/EDC procedure. Soluble receptors were diluted to 20 nM in 10 nM sodium acetate
buffer, pH 6. The receptor solutions were injected over the activated surface until the desired
surface densities were achieved. Activated coupled surfaces were then quenched of reactive sites
with 1 M ethanolamine, pH 8.5, for 7 min. Reference surfaces were activated as described above
and then quenched with 1M ethanolamine, pH 8.5, for 7 min.
All data was collected at 10 Hz using at least 5 injections for each receptor/ligand pair. Flow
rates during each injection were maintained, and ranged from 2-20 μL/min based on usable
sample volume. Regeneration of sALK1 chip was carried out with a 5 μL injection of 3M
MgCl2. Regeneration of all other active surfaces (when necessary) was carried out with a 5 μL
30
injection of regeneration buffer (0.4M urea, 0.9M MgCl2, 25mM EDTA, 0.9M guanidine-HCl,
10mM glycine pH 9.5).
2.10 Analysis of Biosensor Data BIAevaluation 4.1 software was used to measure and plot the kon and koff values directly, which
were then used to calculate the affinity (KD). We confirmed the BIAevaluation 4.1 software
affinities using the plateau method. In this method we plotted RU difference vs. analyte
concentration. Hyperbolic curve fitting was used to determine the hyperbolic equation describing
the relationship between RU difference and analyte concentration. The concentration that
generated the half-maximal RU difference represents the affinity of the interaction (KD). The
highest RU difference observed was assumed to be the maximal RU difference.
2.11 Statistical Analysis Data was evaluated by one-way analysis of variance (ANOVA). Paired t-test was used to
compare two sets of data determine significant difference. Statistical significance was accepted
at P<0.05.
31
Chapter 3 Generation of Materials for Structural and Functional Studies
3 Results : Generation of Materials for Structural and Functional Studies
Despite two reports of the low resolution structure of endoglin (49, 53), its biochemical nature
remains mostly unresolved. We therefore generated stable and soluble forms of the extracellular
domain of endoglin for the purpose of X-ray crystallography and functional studies.
3.1 The complete extracellular and orphan domains of endoglin are readily expressed and secreted as soluble proteins
The membrane form of endoglin consists of a N-terminal orphan domain followed by the zona
pellucida (ZP) domain, juxtamembrane region, transmembrane region and a short cytoplasmic
domain (48, 49). Full-length endoglin was previously cloned into the mammalian pCMV5 vector
with a C-terminal Flag-tag (Fig. 5A), and used as a template to generate multiple constructs of
endoglin delineating different domains. pCMV5-Eng1-586-Flag codes for the complete
extracellular domain, encompassing both the orphan and ZP domains (Fig. 5A). pCMV5-Eng1-
357-Flag codes for the endoglin N-terminal orphan domain (Fig. 5A). Two different constructs
coding for the ZP domain were generated, one terminating at residue 581 (pCMV5-Eng358-581-
Flag) and the other at residue 586 (pCMV5-Eng358-586-Flag) (Fig. 5A). These two forms were
generated to test the role of Cys-582 in the structure and stability of endoglin ZP domain.
Expression levels and solubility of each construct were evaluated using transfected HEK 293T
cells. Twenty-four hours after transfection, cells were washed and then cultured in serum-free
medium, after which the cell lysate and medium were collected and analyzed by SDS-PAGE and
immunoblotting (Fig. 5B). Within the lysates, Eng1-586 (80 kD) and Eng1-357 (55kD) were
readily identified, whereas both ZP domain constructs (27 kD) were barely detectable, despite
loading five times more material, relative to the other constructs (Fig. 5B). This implies that both
ZP domain constructs are expressed poorly relative to the orphan or complete extracellular
domain. Within the media, Eng1-586 (95 kD) and Eng1-357 (75 kD) were easily detectable,
32
33
Figure 5. Cloning and expression of endoglin fragments.
(A) Schematic representation of the full length endoglin cDNA and the engineered extracellular
domain constructs containing a FLAG tag. Human endoglin cDNA codes for full length endoglin
(L-Eng) (Met1-Ala658). Select endoglin fragments were cloned into the pCMV5 vector. The five
glycosylation sites (Asn88, 102, 121, 134, 307) are marked (•). (B) Immunoblotting of endoglin
constructs expressed in HEK 293T Cell Lysate and Media using a polyclonal antibody to
endoglin (H300) that reacts with both monomers and dimers. 5 µg of cell lysate proteins were
loaded for the empty vector control (1), L-Eng (2), Eng1-586 (3) and Eng1-357 (4) while 25 µg
protein was used for Eng358-581 (5) and Eng358-586 (6). Culture media, concentrated 10-fold,
was loaded with three times the volume loaded for the equivalent cell lysate samples. Samples
were run under reducing (R) and non-reducing (NR) conditions.
34
demonstrating that both constructs are expressed and secreted in a soluble form (Fig. 5B).
Neither ZP domain was detectable in the media.
Western blot analysis also provided useful information regarding the oligomeric structure of the
endoglin constructs. Full-length endoglin is a transmembrane disulfide-linked dimer of 180,000
Da as previously reported (45), and resolved as monomers under reducing conditions (Fig. 5B).
In cell lysates, Eng1-586 was found in both dimeric and monomeric forms under non-reducing
conditions while Eng1-357 was mostly monomeric. Since the disulphide bond is likely within the
1-357 region (52), the decreased presence of dimeric protein can likely be attributed to improper
orientation due to no longer being tethered to the membrane. Both forms of the ZP domain exist
only in monomeric form under both reducing and non-reducing conditions. In the culture media,
Eng1-586 was also present as dimer and monomer under non-reducing conditions, whereas
Eng1-357 was mostly monomeric. Taken together these results indicated that both Eng1-586 and
Eng1-357 were expressed and secreted as stable forms of the extracellular domain of endoglin
(142) and could be used for susbsequent studies aimed at determining endoglin structure and
function.
3.2 Generation of deglycosylated forms of soluble endoglin
Since these soluble proteins were intended for X-ray crystallography we needed to ensure that
they would be suitable. Some of the most difficult proteins to crystallize are glycoproteins,
owing to the fact that crystallization is usually inhibited by the chemical and conformational
heterogeneity of carbohydrate moieties (142). In an attempt to facilitate protein crystallization, it
was decided that glycosylation mutants would be generated using site-directed mutagenesis.
Human endoglin contains 5 putative N-linked glycosylation sites (Asn 88, 102, 121, 134, 307)
based on sequence analysis (45). These sites were altered sequentially by site-directed
mutagenesis and converted to Gln residues. The corresponding constructs were analyzed for
expression and secretion in HEK 293T cells (Fig. 6A). Progressively mutating glycosylation sites
resulted in a progressive downward shift in molecular weight. This observation gives the first
evidence that each of these sites are in fact glycosylated.
While removal of glycosylation sites is beneficial in the context of crystallography it may come
at the cost of protein expression (142). When one or two of the five sites (N-134-Q and N-
35
Figure 6. Generation of deglycosylated endoglin fragments by site-directed mutagenesis.
(A) Expression of Eng1-586 glycosylation mutants. cDNA (1 μg) corresponding to Eng1-586
(WT) and its glycosylation mutants were transfected into HEK 293T cells and equivalent
amounts of culture media samples analyzed by SDS-PAGE and anti-FLAG Western blot. This is
a representative image of 7 experiments. Eng1-586-N134Q (88kD) and Eng1-586-N121,134Q
(82kD) showed 80% expression relative to WT (95kD) while Eng1-586-N121,134,307Q (72kD)
and Eng1-586-N88,121,134,307Q (67kD) showed 50% expression. Eng1-586-
N102,121,134,307Q (66kD) was only expressed at 10% and the completely deglycosylated
(45kD) form was not detectable, indicating that Asn102, and to a lesser extent Asn307,
glycosylation sites are important for protein folding/stability. (B) Generation of Eng1-357 triple
(N121,134,307Q) and quadruple (N88,121,134,307Q) mutants. Eng1-357-N121,134,307Q and
Eng1-357-N88,121,134,307Q mutants were generated by sub-cloning from the equivalent Eng1-
586 constructs. cDNA (1 μg) was transfected into HEK 293T cells and equivalent amounts of
culture media samples were run under reducing conditions and immublotted with anti-endoglin
(H300).
36
121,134-Q, respectively) of Eng1-586 were mutated, protein expression was reduced to 80%
relative to wild-type (WT) (Fig. 6A). On average, the triple (N-121,134,307-Q) and quadruple
(N-88,121,134,307-Q) mutant forms of Eng1-586 showed 50% expression relative to WT. An
alternate form of the quadruple mutant (N-102,121,134,307-Q) had drastically reduced
expression, 10% relative to WT, while a completely deglycosylated mutant was not detectable in
the media. The large loss of protein stability and subsequent expression experienced by mutating
residue 102 suggests that glycosylation at this site is required for endoglin stability. We decided
that the triple (N-121,134,307-Q) and quadruple (N-88,121,134,307-Q) mutant forms of Eng1-
586 were the most viable options to pursue since they were partially deglycosylated, expressed
and secreted, and may yield enough protein for functional and structural studies.
These mutants were then used as templates for the generation of the deglycosylated forms of the
orphan domain, Eng1-357 (Fig. 6B). On average, the triple mutant form of Eng1-357 (N-
121,134,307-Q) had approximately 70% expression relative to WT, while the quadruple mutant
(N-88,121,134,307-Q) was not detectable in the media. This suggests that the ZP domain may
offer some shielding near residue 88, thereby allowing the quadruple (N-88,121,134,307-Q)
mutant forms of Eng1-586 to be expressed.
Due to decreased protein expression with mutation of glycosylation sites, an alternate means of
deglycosylation was explored. Within mammalian cells, once a glycoprotein reaches the Golgi,
all glycosylation sites contain a high-mannose chain (Fig. 7A) (142). This chain is then trimmed
by mannosidase I, forming the substrate needed for the generation of complex glycosylation
chains. However, growing cells in the presence of kifunensine, a potent inhibitor of mannosidase
I, blocks its action, leaving only high-mannose chains. These high-mannose chains, as opposed
to complex chains, can be cleaved by endoglycosidase (Endo) H leaving a single glucosamine
(GlcNAc) residue.
To test the suitability of removing glycosylated side-chains by kifunensine treatment and EndoH
digestion on endoglin expression, HEK 293T cells were transfected with either wild-type Eng1-
586 or Eng1-357 and grown in the absence or presence of 50 μM kifunensine for 24 h. The cell
media was then concentrated 10-fold and incubated with increasing concentrations of EndoH.
Growing cells in the presence of kifunensine did not affect protein expression and secretion (Fig.
37
Figure 7. Generation of deglycosylated endoglin fragments by kifunensine and EndoH
treatment.
(A) Pictorial representation of complex glycosylation pathways and their inhibition by
kifunensine and cleavage of high-mannose glycosyl groups by EndoH. Immunoblotting of
kifunensine and EndoH treated Eng1-586 (B) and Eng1-357 (C). Transfected HEK 293T cells
were grown in either the absence (lanes 1-5) or presence (lanes 6-10) of 50 μM kifunensine. The
concentrated culture media were then treated with varying concentrations of EndoH for 3 h at
37˚C (lanes 3-5, 7-10). Protein stability was assessed in relation to temperature, 4̊C (lanes 1 and
6) and 37̊C (lanes 2 and 7). EndoH dependent deglycosylation was only apparent when cells
were grown in the presence of kifunensine.
38
7B,C). As expected, incubation of proteins obtained from kifunensine untreated but EndoH
treated cells did not alter the degree of glycosylation. However, proteins obtained from
kifunensine treated cells allowed for nearly complete deglycosylation by EndoH for both Eng1-
586 and Eng1-357. Therefore, treatment with kifunensine and EndoH represents a viable
alternate means of generating deglycosylated endoglin for structural studies.
This method is very useful since it allows for proper folding due to glycosylated side-chains,
which can be removed later. Also, the single GlcNAc residue left behind at each glycosylation
sites allows for partial shielding of the potentially hydrophobic regions of the protein surface.
This method is now being implemented in the laboratory of our collaborator in order to produce
deglycosylated Eng1-586 and ultimately to perform X-ray crystallography.
3.3 Sub-cloning endoglin constructs into high-expression CHO vectors
In order to generate stable CHO cell lines expressing endoglin for structural and functional
studies, the constructs of interest must be sub-cloned into specialized vectors for stable
transformation. The vectors chosen were the CHEF1 vectors (pDEF38 and pNEF38) since they
were designed for high-level protein expression in CHO cells (Fig. 8A) (143). These vectors
contain the 5’ and 3’ UTR regions of a highly expressed CHO gene, EF1-α, and the
dihydrofolate reductase gene, as well as the AmpR selection marker. It was decided that the
wild-type, triple (N-121,134,307-Q) and quadruple (N-88,121,134,307-Q) mutant forms of both
Eng1-586 and Eng1-357 would be inserted into the high-expression vectors, pDEF38 and
pNEF38. All of the desired endoglin fragments were successfully sub-cloned into the proper
vectors with a C-terminal His-tag. The expression and secretion of the pDEF38 vector constructs
were compared to that of the pCMV5 constructs (Fig. 8B, C). For both Eng1-586 and Eng1-357,
each high-expression construct was readily expressed and secreted in HEK 293T cells; however,
protein expression was slightly lower relative to expression of the same protein fragment in the
pCMV5 vector. This decreased expression can be explained due to the fact that the CHEF1
vectors are designed for use in CHO cell lines, and we were testing them in HEK 293T cells to
simply verify expression of the constructs. Increased protein expression in CHO cells of these
vectors is due to desired sequences being flanked by the 5’ and 3’ UTR regions of a highly
expressed CHO gene.
39
Figure 8. Expression of endoglin fragments in vectors designed for large scale protein
generation.
(A) Schematic of high-expression vectors (pDEF38/pNEF38). These vectors are engineered for
high expression in CHO cells by containing the 5’ and 3’ flanking sequences of a highly
expressed CHO gene (EF-1α). The wild-type and triple mutant (N-121,134,307-Q) forms of both
Eng1-586-His and 1-357-His were sub-cloned into both pDEF38 and pNEF38 and then used in
the generation of stable CHO cell lines. The WT, triple (GS3, N121,134,307Q) and quadruple
(GS4, N88,121,134,307Q) mutant forms of both Eng1-586 (B) and Eng1-357 (C) in either
pCMV5 (P) or pDEF38 (D) were transfected into HEK 293T cells. Equivalent amounts of
culture media samples were run under reducing conditions and immunoblotted with anti-
endoglin (H300).
40
3.4 Large-scale expression and purification of Eng1-586-His and Eng1-357-His proteins
With the ultimate goal being the production of sufficient quantities of protein for structural and
functional studies, four stable cell lines were generated, each expressing one of the following
constructs: Eng1-586-His, Eng1-586-N-121,134,307-Q-His, Eng1-357-His and Eng1-357-N-
121,134,307-Q-His. Due to resource and space limitations, only the cells expressing Eng1-586
and Eng1-357 were used for large scale protein expression since they are the most
physiologically relevant forms for functional studies. Each cell line was grown in a spinner flask
for 2-3 weeks. Secreted proteins were purified via Ni2+ immobilized metal affinity
chromatography (IMAC).
The initial Eng1-586-His preparation yielded ~2mg of protein from a 1.5 L culture volume.
Purity of the endoglin preparations was evaluated by SDS-PAGE followed by Coomassie blue
staining. The Eng1-586-His samples had very high purity after IMAC with little visible protein
contaminates (Fig. 9A). This protein was subsequently dialyzed against the desired buffer for
functional studies.
Unfortunately the cells expressing Eng1-357-His responded poorly to the serum-free medium
and failed to produce detectable levels of protein. With adjustments to the production protocol,
3.1L of Eng1-357-His culture yielded ~2.2mg of protein. The Eng1-357-His samples had very
high purity after IMAC, with some visible protein contaminates based on the Coomassie blue
stained SDS-PAGE gel (Fig. 9B). This protein was subsequently dialyzed against the desired
buffer for future functional studies.
Based on the Coomassie blue stained SDS-PAGE gels, Eng1-586-His was found in both
monomeric and dimeric forms under non-reducing conditions (Fig. 9A). There was a greater
proportion of dimeric protein (~80%), as compared to Eng1-586-Flag obtained from transient
transfection in HEK 293T cells (~50%) (Fig. 5B vs. Fig. 1B). The proportion of dimeric form of
purified Eng1-357 (~50%) was also higher than observed for the transiently expressed Eng1-
357-Flag (~2%) (Fig. 5B vs. Fig. 1B). Evidence from other research has shown that the presence
of a His-tag may actually increase the likelihood of dimerization, giving a possible explanation
for the differences observed in this research (144).
41
Figure 9. Analysis of purified endoglin samples using coomassie blue stained SDS-PAGE
gels.
Eng1-586-His and Eng1-357-His in the high expression vectors (pDEF38/pNEF38) were stably
expressed in CHO cell lines. Secreted proteins were purified from the media by Ni2+-IMAC
purification and resolved by SDS-PAGE and analyzed by coomassie blue staining. (A) Under
reducing (R) conditions, Eng1-586-His exists as a monomer; under non-reducing (NR)
conditions it exists in both monomeric and dimeric forms. (B) Under reducing conditions, Eng1-
357-His is resolved as a monomer; under non-reducing conditions it exists as a mixture of
monomers and dimers. Both samples are of high purity.
42
Once we had obtained protein samples for functional studies, we then optimized the procedures
to increase production of Eng1-586-His for the generation of protein crystals for X-ray
crystallography. With adjustments to the growing protocol such as addition of more cells, 2.8L
of Eng1-586-His culture yielded ~15mg of protein following IMAC fractionation. The IMAC
fractions containing Eng1-586 were further subjected to gel filtration chromatography using a
Hi-Load Superdex-200 gel filtration column, separated into monomer and dimer samples and
then used for crystallography screens.
Another important criterion for the generation of protein crystals suitable for crystallography is a
pure homogenous protein solution. Based on Coomassie-stained SDS-PAGE gels (Fig. 9), the
proteins eluted from the IMAC column were very pure, with few visible contaminants. Another
possible form of contamination is the heterogeneity of monomeric and dimeric proteins in
solution. In order to analyze the relative stability of purified Eng1-586-His, IMAC eluted
samples from the second preparation, were run on a small 10/300 Superdex-200 column. It was
resolved mostly as a dimer (eluting at 10.07 mL) and with an additional peak corresponding to
the monomer (eluting at 11.93 mL) (Fig. 10A). Monomeric and dimeric Eng1-586-His initially
separated using the Hi-Load Superdex-200 column were subsequently run on a 10/300 Superdex-
200 column. Monomeric Eng1-586-His remained in monomeric form, eluting at 11.94mL, with
only slight dimer contamination, eluting at 10.05mL (Fig. 10B). Conversely, Eng1-586-His
dimer remained stable eluting at 10.08mL (Fig. 10C). This successfully demonstrates that the
two oligomeric forms of Eng1-586-His are stable and do not readily interconvert. Taken
together, these results indicate that we have generated and purified a sufficient amount of
structurally stable and highly pure proteins to be used in structural and functional studies.
43
Figure 10. Size exclusion chromatography analysis of eluted Eng1-586-His.
Eng1-586-His was expressed in CHO cell lines using high-expression CHEF1 vectors
(pDEF38/pNEF38) and purified by Ni2+-IMAC. Fractions containing Eng1-586 were pooled and
100 μg subjected to gel filtration chromatography using a 10/300 Superdex-200 column. (A) UV
absorbance of eluted fractions of Eng1-586-His displaying a mixture of oligomeric states. The
eluted fractions were subjected to a second round of gel filtration chromatography to assess their
stability. UV absorbance chromatograph of purified monomers (B) and dimers (C) of Eng1-586-
His.
44
Chapter 4
Functional Studies of Soluble Endoglin
4 Results : Functional Studies of Soluble Endoglin
4.1 Endoglin modulates the signaling of multiple TGF-β superfamily ligands
While a significant amount of research has been focused on the role of endoglin, much remains
to be understood about its mechanisms of action. It is generally accepted that endoglin does not
bind ligand on its own, but is able to modulate the downstream signaling of multiple members of
the TGF-β superfamily, in a context-dependent manner. Our interests lie in better understanding
the role of endoglin in endothelial cells. We first determined the effect of membrane endoglin,
mEng, on signaling for multiple members of the TGF-β superfamily. We then tested if a soluble
form of endoglin, sEng, could disrupt ligand-induced Smad activation as a first step towards
elucidating how sEng leads to endothelial cell dysfunction and ultimately hypertension in the
context of preeclampsia.
To better define the role of mEng in response to specific ligands acting via the BMP pathways,
we measured Smad1,5,8 phosphorylation as a surrogate for downstream signaling. Smad 1,5,8
phosphorylation was examined in the presence or absence of membrane endoglin, in
immortalized E ng+/+ and E ng-/- mouse embryonic endothelial cells respectively (Fig. 11). We
first tested Smad1 phosphorylation in response to increasing doses of TGF-β1 using a phospho-
specific antibody that recognizes activated Smad1. Levels of Smad1 phosphorylation were
higher in E ng-/- cells compared to their wild-type counterpart, E ng+/+ cells with increasing
concentrations of TGF-β1 (Fig. 11A). This is in agreement with previous studies from this
laboratory (67) and suggests that membrane endoglin inhibits Smad- mediated TGF-β1 responses
in endothelial cells.
Next we examined Smad1 activation in response to BMP-2 stimulation and observed higher
phosphorylation with increasing ligand concentration, being close to saturation at 400 pM, the
highest dose tested (Fig. 11B). Similar to the case of TGF-β1, the level of Smad1
45
46
Figure 11. Smad1 phosphorylation in response to stimulation by TGF-β superfamily
ligands.
Eng+/+ and Eng-/- cells were serum-starved for 30 min, and stimulated for 30 min with varying
concentrations of TGF-β1 (A), BMP-2 (B), BMP-7 (C) and BMP-9 (D). Cell lysates were
resolved by SDS-PAGE and analyzed by Western blot with an antibody to phosphorylated
Smad1,5,8 (PSmad1) and to total Smad1,5,8 (Smad1). The amount of PSmad1 was quantified
relative to total Smad1 levels. The graphs represent the mean ± s.e.m. of 3 experiments, except
for panel A which is a representative experiment of a previously published observation (67).
Panels (A), (B) and (D) were generated by Dr. Guoxiong Xu. Based on ANOVA analysis both
the Eng+/+ and Eng-/- curves were statistically different for Panels B and D. Time points
showing statistically different values between Eng+/+ and Eng-/- samples are illustrated by *; P
< 0.05.
47
phosphorylation was consistently higher in E ng-/- than control cells, suggesting that endoglin also
inhibited BMP-2 induced signaling. We next investigated the response of endothelial cells to
BMP-7 and found that higher concentrations were needed to activate Smad 1 phosphorylation,
reaching near saturation at 1200 pM, the highest dose tested (Fig. 11C). Membrane endoglin
gave a small but not statistically significant inhibition of the BMP-7 response. However,
membrane endoglin significantly potentiated the BMP-9 induced Smad1 phosphorylation (Fig.
11D). Near maximal activation of Smad1 was obtained at 25 pM BMP-9 for E ng+/+ cells as
compared to 400 pM for E ng-/- cells.
In summary, mEng inhibits Smad1,5,8 dependent signaling induced by TGF-β 1, BMP-2, and to
some degree BMP-7 while it potentiates BMP-9 signaling.
4.2 The soluble extracellular domain of endoglin can inhibit BMP-9 induced Smad1 phosphorylation
Soluble forms of endoglin are cleaved from the placental surface in patients with preeclampsia
and released into the maternal bloodstream, contributing to endothelial dysfunction and
ultimately hypertension. While an increase in circulating soluble endoglin is associated with
preeclampsia (35), its mechanism of action remains elusive. One proposed model is that soluble
endoglin alters endothelial homeostasis via competitive binding of TGF-β1, thus preventing its
binding to membrane-tethered receptors on endothelial cells. However, endoglin has been
proposed to bind TGF-β1 in association with TBRII. It therefore remains unclear how sEng
elicits its effects within the context of preecplampsia.
Towards this end, we determined if commercially available soluble endoglin (sEng; Eng 1-586)
alters downstream Smad1 activation by TGF-β1 or BMP-2, -7 and -9 in wild-type (E ng+/+)
endothelial cells. As proof of principle, we tested if Smad1 phosphorylation was inhibited by
known soluble receptors, such as TBRII in the case of TGF-β1, or ALK1 in the case of BMP-9.
Therefore, we first incubated endothelial cells with increasing concentrations of soluble receptors
and after 1 h stimulated the cells with a constant amount of the cognate ligand for 30 min in the
presence of the soluble receptors. (Fig. 12). Incubation of TGF-β1-stimulated cells with soluble
TBRII reduced Smad1 phosphorylation by 90% at 10 nM, the highest concentration tested (Fig.
12A). Similarly, a soluble form of ALK1 (sALK1), was able to reduce BMP-9-induced Smad1
phosphorylation by approximately 50% at 10 nM (Fig. 12B). Therefore, competitive binding of
48
Figure 12. Blocking of Smad1 phosphorylation by soluble ligand-binding receptors.
Eng+/+ cells were serum-starved for 2h, incubated for 1h with varying concentrations of soluble
TGF-β receptor II (sTBRII) (A) or soluble type I receptor ALK1 (B) as indicated and stimulated
for 30 min with 100 pM TGF-β1 (A) or 25 pM BMP9 (B) respectively. Cell lysates were
resolved by SDS-PAGE and analyzed by Western blot with anti-phospho-Smad1 or anti-Smad1.
The amount of phospho-Smad1 was quantified relative to total Smad1 levels. The data represent
the average of two experiments.
49
soluble receptors to either TGF-β1 or BMP-9 leads to inhibition of Smad1 phosphorylation,
which can be detected by immunoblot. We then tested if sEng affects Smad1 signaling by TGF-
β1, BMP-2, -7 and -9 (Fig. 13). No detectable changes in TGF-β1- or BMP-2-induced Smad1
phosphorylation were observed when endothelial cells were incubated with up to 10nM sEng
(Fig. 13A and B, respectively). In contrast, sEng inhibited BMP-7-induced Smad1 signaling by
nearly 50% at a 500 nM concentration (Fig. 13C). A more potent inhibition of BMP-9 induced
Smad1 phosphorylation was observed when cells were co-incubated with sEng and BMP-9, with
nearly 50% inhibition obtained with 10 nM sEng (Fig. 13D). Taken together, these data indicate
that sEng can effectively compete with the membrane receptor complex for binding to BMP-9,
and to a lesser extent BMP-7, but not to TGF-β1 and BMP-2.
4.3 Relative binding of immobilized purified soluble endoglin to ligands of the TGF-β superfamily
Activation of Smad1 by BMP-7 and BMP-9 can be inhibited by sEng. To determine if this
inhibition is mediated by direct binding of sEng to ligands and effective competition with
membrane bound receptors, surface plasmon resonance (SPR) was used to determine binding
affinities. To ensure that our experimental system was working properly, SPR was used to
delineate the KD for known interactions between TGF-β1/TBRII and BMP-9/ALK1 (145, 146).
Binding of increasing concentrations of TGF-β1 (0.1 nM – 200 nM) to a soluble dimeric TBRII
immobilized on a sensor chip was analyzed using a BIAcore X (Fig. 14A). We were unable to
remove bound TGF-β1 from the chip, implying a strong interaction. Therefore, kinetic analyses
were accomplished using a combination of the plateau method and values generated using the
BIAevaluation software. Due to the very tight nature of this interaction resulting in incomplete
ligand dissociation, the initial base-line was used to determine the actual RU difference that
could be obtained had the TBRII chip been free of bound ligand. The results from kinetic
analyses revealed a KD of approximately 100 pM, weaker than previously described values (5
pM) (Table 3 and Fig. 14A) (145). We next tested the binding of BMP-9 at concentrations
ranging from 0.5 nM to 400 nM to immobilized dimeric sALK1-Fc (Fig. 14B). BIAevaluation-
based kinetic analysis, verified by the plateau method, gave a KD = 1.8 nM, a value in agreement
with a previously reported study (146).
50
51
Figure 13. Analysis of the ability of sEng to inhibit ligand induced Smad1 phosphorylation.
Eng+/+ cells were serum-starved for 2 h, incubated for 1 h with varying concentrations of sEng
and stimulated for 30 min with (A) 100 pM TGF-β1, (B) 100 pM BMP-2, (C) 300 pM BMP-7,
(D) or 25 pM BMP-9. Cell lysates were resolved by SDS-PAGE and analyzed by Western blot
with anti-PSmad1 or anti-Smad1. The amount of PSmad1 was quantified relative to total Smad1
levels. The graphs represent the mean ± s.e.m. of 3 experiments. Inhibition with sEng versus
untreated was significant for points denoted by an asterisk; P < 0.05.
52
Figure 14. Kinetic analysis of TGF-β1 and BMP-9 binding to their respective TBRII and
Alk1 receptors.
Commercially available forms of TBRII-Fc (A) and ALK1-Fc (B) were amine-coupled to a CM5
chip and different concentrations of (A) TGF-β1 (50-200 nM) or (B) BMP-9 (20-400 nM) were
injected over the captured receptors. The raw data (coloured lines) are overlaid with a global fit
1:1 model (black lines) obtained by the BIAevaluation software. The difference in resonance
signal was plotted against concentration and the data was overlaid with a hyperbolic fit curve
(insets).
53
Table 3. Kinetic and thermodynamic constants for the interaction of multiple ligands of the
TGF-β superfamily with the extracellular domain of selected receptors using the BIAevaluation
software.
Receptor Ligand ka
(M-1s-1)
kd
(s-1)
KD
(nM)
sTBRII TGF-β1 - - 0.1
sALK1 BMP-9 2.5x105 4.6x10-4 1.8
sEng BMP-9 9.9x105 4.9x10-3 5
BMP-7 4.9x104 2.9x10-3 60
TGF-β1 4.5x103 5.6x10-3 1,230
BMP-2 26.1 4.9x10-3 186,000
54
We then estimated the sEng binding affinities for TGF-β1, BMP-2, -7, and -9 (Fig. 15 and Table
3). The sEng was obtained from stably transfected CHO cell lines, purified and characterized as
described in Chapters 3. The dimeric form of sEng, retrieved after size exclusion
chromatography was coupled to the chip. Binding of increasing concentrations of ligand (TGF-
β1 (1 nM – 800 nM), BMP-7 (1 nM – 300 nM), BMP-9 (0.1 nM – 500 nM) and BMP-2 (1 nM –
300 nM), to sEng immobilized on a sensor chip was analyzed using a BIAcore X instrument.
Kinetic and equilibrium analysis were performed using the BIAevaluation software and then
confirmed using the plateau method where possible.
Analyses revealed that sEng (Eng1-586) binds TGF-β1 with an affinity of 1.23 μM. The kinetic
studies indicated rapid on and off rates (4.5x103 M-1s-1 and 5.6x10-3 s-1, respectively) (Figure 15A
and Table 3). We were unable to reach plateau values using the available ligand concentrations,
meaning that we could not confirm the binding affinity using the plateau method. The interaction
of BMP-7 with immobilized sEng is considerably stronger (KD = 60 nM) with a faster on rate
(4.9x104 M-1s-1) but a comparable off rate (2.9x10-3 s-1) (Fig 15B and Table 3). sEng interacts
most strongly with BMP-9, having an affinity of 5 nM (Fig 15C and Table 3). This higher
affinity results from the fast on rate (9.9x105 M-1s-1)as the off rate (4.9x10-3 s-1)is similar to those
observed for sEng and TGF-β1 and BMP-7. The interaction between sEng and BMP-2 was much
weaker (KD = 186 μM) with a slow on rate (26.1 M-1s-1) but an off rate (4.9x10-3 s-1) comparable
to that of sEng with other ligands (Table 3). Due to resource limitations, only the two highest
ligand concentrations tested produced a change in the RU and neither reached a plateau. This
means that the determined KD will likely change with a complete SPR analysis with more
concentrated ligand samples.
Together, these data demonstrate that sEng can in fact bind directly to ligands of the
TGF-β superfamily but with different affinities. The strongest binding of sEng is with BMP-9
(KD = 5nM), implying that BMP-9 is functionally the most relevant ligand for endoglin. The
interaction of sEng with BMP-7 is one order of magnitude less and likely also of biological
relevance. The interaction of TGF-β1 with sEng is in the μM range and 10,000 times less than its
binding to TBRII, implying that sEng is unable to compete effectively for binding of TGF-β1 to
cells. The weakest interaction observed for sEng was with BMP-2 with an estimated KD close to
200 μM, leading us to propose that sEng cannot compete with surface receptors for BMP-2
effects.
55
56
Figure 15. Kinetic analysis of TGF-β1, BMP-7 and BMP-9 binding to sEng.
The dimeric fraction of purified Eng 1-586 (sEng) produced in CHO cells was amine coupled to
a CM5 chip and different concentrations of (A) TGF-β1 (25-800 nM), (B) BMP-7 (3-300 nM)
and (C) BMP-9 (1-500 nM) were injected over the captured receptors. The raw data (coloured
lines) are overlaid with a global fit 1:1 model (black lines) obtained by the BIAevaluation
software. The difference in resonance signal was plotted against concentration and the data was
overlaid with a hyperbolic fit curve (insets).
57
Chapter 5 Discussion
5 Discussion Both forms of endoglin, mEng and sEng, have been implicated in preeclampsia. There has been
shown to be an increased mEng expression in placenta of women with preeclampsia. We have
shown in this thesis that the presence of mEng in endothelial cells inhibits TGF-β1, BMP-2 and
BMP-7-induced Smad1,5,8 phosphorylation. On the other hand, the presence of mEng
potentiates BMP-9 Smad1,5,8 signaling. Research has also shown that there are increased levels
of sEng in the sera of women with PE and it correlates with disease severity. Our results show
that sEng can bind BMP-9 with high enough affinity to inhibit downstream Smad1,5,8
phosphorylation. However, the affinity between sEng and multiple TGF-β superfamily ligands
(TGF-β1, BMP-2, BMP-7) was not sufficient to inhibit Smad1,5,8 signaling within the
physiological range.
5.1 Biochemical characterization of sEng
Currently the exact nature of sEng associated with preeclampsia is unknown. Very small
amounts could be purified from the serum of women with PE. Mass spectrometry allowed the
identification of several peptides and indicated that the N-terminal region extended at least as far
as Arg406, however, there was insufficient protein to resolve the C-terminal sequence. This
means that we could not generate the exact fragment corresponding to the circulating form of
endoglin found in PE. However, we chose to express the Eng1-586 construct, corresponding to
the extracellular domain of endoglin.
5.1.1 Expression of sEng
To fulfill our ultimate goal of determining how sEng contributes to endothelial cell dysfunction
and hypertension in PE, we first needed to engineer components of the extracellular domain that
could be readily expressed and soluble. Previous studies of endoglin truncation mutations have
shown that most variants are unstable and would not generate soluble fragments (85). Our
construct expressing the entire extracellular domain (Eng1-586) was in fact readily expressed
58
and secreted into the media. This protein fragment containing the complete extracellular domain
had been shown to be expressed and secreted previously (111). This fragment may also have a
physiological role. Hawinkels et al. showed that HUVEC cells released a large amount of a
soluble form of endoglin into the media (111). Through the use of protease inhibitors and
cleavage site mutants, they were able to determine that this 80 kD form of sEng was generated
by MT1-MMP cleavage at residues 586-587. This further supports our choice of Eng1-586 as a
soluble protein that may permit the study of the role of sEng in a physiological context.
We found that the isolated orphan domain (Eng1-357) was readily expressed, stable, and
secreted from HEK 293T cells. The stability could be due to the domain being self-contained.
Thus Eng1-357 represents an alternate soluble fragment for structural and functional studies. The
isolated ZP domains were only weakly expressed and not released from the cell, suggesting that
the orphan domain confers some stability to the ZP domain. While we were unable to readily
express the isolated ZP domain, although another group was able to transiently express Eng360-
586 in HEK 293T cells (147). The increased expression and stability of this particular protein
fragment may be due to the use of the pAID-4 vector or the presence of a C-terminal Fc,
fragment which may confer some degree of stability (147).
5.1.2 Potential multiple forms of sEng
The physiologically relevant form of sEng associated with PE remains to be determined. While
MT1-MMP was shown to cleave mEng, resulting in the release of a soluble form, there are
discrepancies to suggest that sEng fragments of different size may also exist. The protein
released by MT1-MMP in HUVEC cells was approximately 80 kD based upon Western blot
analysis. However, the sEng purified from the sera of women with PE was 65 kD, based upon
Western blot analysis. Thus, there might be different forms of sEng likely generated through
cleavage by different proteases. The true form of sEng in PE needs to be identified to obtain a
better understanding of its nature and function. With the development of more sensitive C-
terminal sequencing techniques, it should be possible to identify the placenta-derived sEng and
its mechanism of release, and to generate the appropriate constructs for structural and functional
studies.
59
5.1.3 Disulphide linkages
Another critical piece of information that is yet to be resolved is the location of the interchain
disulphide bond(s) that maintain the dimeric structure of endoglin. Our work and that of others
have shown that Eng1-586 can exist as a disulphide linked homodimer. As previously stated,
work done by Raab et al. (52) has suggested that the location of the cysteine residues involved
are likely to reside between residues 330 and 412. Within this region there are six cysteine
residues (Cys330, Csy350, Cys363, Cys382, Cys394 and Cys412) that could potentially be
involved. The possibilities could be narrowed down based on our observation that Eng1-357,
generated and expressed in our laboratory, can exist in dimeric form. Taken together, these data
suggest that the cysteine residues involved in maintaining the dimeric structure of endoglin are
either Cys330 or Cys350. Based on sequence analysis from the sEng found in PE (to Arg406),
both these cysteine residues were within the cleaved section of the extracellular domain,
suggesting that the physiological sEng in PE is dimeric.
5.2 Functional understanding of sEng The mechanisms involved in the contribution of sEng to endothelial dysfunction and
hypertension remain to be determined. Our research was aimed at increasing our understanding
of the physiological and pathological role of endoglin.
5.2.1 mEng role in modulating Smad1,5,8 signaling
It is well known that ligands of the TGF-β superfamily induce intracellular Smad signaling by
interacting with a heteromeric receptor complex, composed of both a type I and type II receptor,
at the cell surface. While mEng is not an essential component of this receptor complex it has
been shown to modulate the signaling of multiple members of this family. In this study, we
demonstrate that mEng inhibits the ability of TGF-β1 to stimulate Smad1,5,8 phosphorylation.
This inhibition is not surprising, as similar results have been reported using the same endothelial
cell lines (67). In addition, L6E9 myoblast cells, lacking endoglin expression, also showed
decreased Smad signaling when transfected with a mEng-expressing construct (60). The exact
mechanism involved in this inhibition is unknown, since endoglin has not been shown to bind
and effectively sequester ligand. It is possible that the presence of endoglin changes the
conformation of the ligand-binding receptor present in the receptor complex. The cytoplasmic
60
domain of endoglin could also be interfering with signal transduction. The mechanism involved
in the ability of mEng to modulate signal remains to be determined.
We also tested other TGF-β superfamily ligands that have been shown to interact with endoglin,
namely BMP-2, BMP-7, and BMP-9. We show for the first time that mEng inhibits BMP-2-
induced Smad1,5,8 signalling. We also see that mEng slightly inhibits, however not
significantly, BMP-7-induced Smad1,5,8 activation. This is contrary to what is seen in mEng
overexression studies in a rat myoblast cell line, where the presence of mEng actually
strengthens BMP-7 signaling (68). This difference could be due to the different cell type, as the
mode of action of endoglin has been shown to be very context dependent.
Interestingly, we found that mEng significantly potentiates BMP-9-induced Smad1,5,8 signaling.
Similarly, overexpression of mEng in NIH-3T3 fibroblast cells was shown to lead to increased
BMP-9-induced B recognition element (BRE) promoter activity (62). This mEng-mediated
modulation may occur through a different mechanism as compared to those stated above, since
mEng has been shown to interact with BMP-9 in the absence of its ligand-binding receptor
ALK1 (61). This suggests that mEng may be binding ligand and facilitating its interaction with
its cell surface receptor complex, ALK1, similar to the means through which betaglycan has been
proposed to potentiate TGF-β2 signaling (32).
5.2.2 sEng role in binding ligand and modulating Smad1,5,8 signaling
Next, we wanted to better understand how sEng contributes to endothelial cell dysfunction in PE.
sEng has been proposed to interfere with TGF-β1,3 signaling by effectively competing for
ligand, even though it is known that sEng can only bind TGF-β1,3 in the presence of the ligand-
binding receptor, TBRII. Contrary to what was seen previously using a luciferase assay (35), the
presence of sEng did not affect TGF-β1-induced Smad1,5,8 signaling. While these results are
contrary to the current accepted model of the role of sEng in PE, they agree with reports
indicating that endoglin cannot bind TGF-β1 (59). However, incubation with a soluble
extracellular domain of TBRII resulted in a significant and almost complete inhibition of TGF-
β1-induced Smad1,5,8 phosphorylation. This is consistent with the kinetic data we obtained.
For the first time we show that sEng can in fact bind TGF-β1 with a 1.23 μM affinity; however
this would be too weak to inhibit Smad1,5,8 phosphorylation in our inhibition assay or produce a
61
physiological change. During the writing of this manuscript, another group published a study
looking at sEng binding ligand, also using BIAcore (147). They reported that the sEng/TGF-β1
interaction was in the μM range or weaker, in agreement with our observations. Consistent with
the cell-based assay, we observed that the interaction between TBRII and TGF-β1 (100 pM) was
much stronger than for sEng. This interaction has been extensively studied and our value is
similar, although weaker than published data (~5 pM) (145). Together, this data infers that
TBRII has a significantly higher affinity for TGF-β1 than sEng. This demonstrates that sEng
could not effectively compete with TBRII at the cell surface for TGF-β1 binding. Given our
results, it is unlikely that sEng is leading to endothelial dysfunction in the context of PE by
effectively competing for TGF-β1 binding and interrupting downstream signaling.
We also found that sEng was unable to inhibit BMP-2-induced Smad1,5,8 phosphorylation and
subsequent downstream signaling. This is consistent with the data suggesting that BMP-2 can
only bind endoglin in the presence of ALK3 or ALK6 (59). Our BIAcore data showed that sEng
bound BMP-2 with an estimated affinity of 186 μM. This is lower than what was seen for TGF-
β1. It can reasonably be concluded that BMP-2 is not the ligand of interest in the context of PE.
sEng was only able to inhibit BMP-7-induced Smad1,5,8 phosphorylation at high concentrations.
These sEng concentrations are 10-20 fold higher than what would be seen in PE (35). We found
that the interaction between sEng and BMP-7 has an affinity of 60 nM. This interaction is
stronger that what has recently been reported. Castonguay et al. reported that if there was any
interaction it would be in the μM range or weaker; however, they did not determine the exact
affinity (147). While we see that sEng can in fact bind BMP-7, the affinity is likely too weak to
cause a significant physiological change and the serum level of sEng in PE is approximately 1.5
nM, which is far less than what was needed to inhibit Smad signaling.
On the other hand, we showed that sEng can interfere with BMP-9-induced Smad1,5,8
phosphorylation. Roughly 50% inhibition of Smad1,5,8 signaling was obtained at 10 nM sEng.
This is consistent with studies showing that endoglin can actively interact with BMP-9 without
the ligand-binding receptor (61). These observations are supported by the binding affinities. We
determined that sEng binds BMP-9 with 5 nM affinity. This is a strong interaction; however,
Castonguay et al. reported an observed kD of 26 pM. This large discrepancy could be due to
experimental differences, such as linking sEng to the sensor chip using a C-terminal Fc, as
62
opposed to our protein with a His-tag and attached to the chip in a random orientation. Our
determined affinity for the sALK1 and BMP-9 interaction (2 nM) is similar to what we found for
sEng/BMP-9. This is consistent with a previously reported affinity of 2 nM (146). This kinetic
data is consistent with our cell-based assays. sEng and sALK1, which have been shown to have a
similar kD, both show roughly 50% inhibition of Smad1,5,8 phosphorylation at a 10 nM soluble
receptor concentration. Since sEng and ALK1 have similar affinities, it is reasonable to suggest
that sEng could effectively compete with membrane ALK1 for BMP-9 binding.
Based on this work and other binding studies that were recently done, it looks as if sEng can
effectively compete for BMP-9 binding and actually affect downstream signaling. This gives
credence to the theory that sEng may lead to endothelial cell dysfunction by interfering with
BMP-9 signalling. These results are contrary to the widely held view that sEng interferes with
TGF-β1,3 signalling. We were unable to detect a significant affinity between TGF-β1 and sEng
to allow it to effectively compete for ligand binding and subsequently disrupt signaling. We were
also unable to detect sEng interfering with mEng in the context of Smad signaling. However, we
cannot rule out the possibility that sEng may be interfering with TGF-β1 mediated Smad
independent pathways by interfering with mEng.
5.2.3 sEng in the context of PE
This new information could completely change the concept of how sEng leads to endothelial cell
dysfunction. A lot of work must now be done to elucidate how inhibition of the Smad1,5,8
pathway could lead to the symptoms associated with PE. Recent work within the field of cancer
may provide some potential mechanisms. BMP-9 stimulation causes Smad1,5,8 phosphorylation,
which can then interact with Smad4, translocate to the nucleus and increase expression of Id-1
(Fig. 16). When this pathway was disrupted by the presence of sALK1, which could mimic the
effects of sEng based on our results, this lead to decreased Id-1 expression and ultimately
decreased expression of VEGF. sFlt-1 is known to sequester VEGF in the context of PE. These
results suggest that sEng and sFlt-1 are ultimately disrupting the same pathway, namely VEGF
signalling. This explains previous results that show that sEng and sFlt-1 individually cause mild
symptoms, but together have a synergistic effect and contribute to severe PE. VEGF signaling
has been shown to increase eNOS expression as well as activation. sEng and sFlt-1 may be
inhibiting
63
Figure 16. Model of the mechanism through which sEng contributes to endothelial cell
dysfunction in the context of PE.
This diagram represents a possible mechanism by which placentally derived sEng leads to
maternal endothelial cell dysfunction in PE. sEng is released from the placenta into the maternal
circulation. sEng effectively competes for BMP-9 binding thereby decreasing the amount of
ligand available to induce downstream Smad1,5,8 phosphorylation. This would result in
decreased Id-1 expression directly resulting in decreased VEGF production. This decreased
production, along with sFlt-1 sequestering VEGF in the circulation, results in decreased VEGF
induced expression and activation of eNOS. This means that the pregnant women are no longer
able to vasodilate in response to the increased blood volume associated with normal pregnancy
resulting in hypertension.
64
production and signaling of VEGF, respectively. This could lead to less eNOS expression and
activation. This would not cause vasoconstriction, but would no longer allow for the maternal
vasculature to adjust to the increased blood volume associated with pregnancy, since the vessels
are no longer able to produce sufficient NO to allow for vasodilatation. This proposed
mechanism gives a plausible means through which sEng, in conjunction with sFlt-1, contributes
to hypertension in the context of PE. Such a model will guide future research.
5.3 Concluding remarks Our results have afforded us a better understanding of endoglin biochemistry. This protein is
highly stable as a dimer with the cystine residues involved in the interchain disulphide bond
being either Cys330 or Cys350. The sEng found in PE is likely to exist as a disulphide-linked
homodimer. While mechanisms of endoglin cleavage have been reported, the exact mechanism
and form of sEng in the context of PE remains to be determined. Based on our functional studies
we have determined that mEng can potentiate the endothelial cell response to BMP-9, while
inhibiting responsiveness to TGF-β1, BMP-2 and BMP-7. More importantly, we demonstrated
that sEng can actually bind BMP-9 with a high enough affinity to effectively compete with the
membrane receptor for ligand binding. We propose that sEng inhibits BMP-9-induced Smad1,5,8
phosphorylation, ultimately resulting in reduced VEGF expression, thereby contributing to the
maternal symptoms of PE. Reduced VEGF could lead to decreased eNOS expression and
activation, resulting in maternal vasculature that can no longer vasodilate in response to the
increased blood volume associated with pregnancy. The challenge of future research in this field
will be to investigate the merits of this proposed mechanism.
65
References
1. Heldin, C. H., K. Miyazono, and P. ten Dijke. 1997. TGF-beta signalling from cell membrane
to nucleus through SMAD proteins. Nature 390: 465-471.
2. Miyazono, K., S. Maeda, and T. Imamura. 2005. BMP receptor signaling: transcriptional
targets, regulation of signals, and signaling cross-talk. Cytokine Growth Factor Rev. 16: 251-
263.
3. de Caestecker, M. 2004. The transforming growth factor-beta superfamily of receptors.
Cytokine Growth Factor Rev. 15: 1-11.
4. Siegel, P. M. and J. Massague. 2003. Cytostatic and apoptotic actions of TGF-beta in
homeostasis and cancer. Nat. Rev. Cancer. 3: 807-821.
5. Balemans, W. and W. Van Hul. 2002. Extracellular regulation of BMP signaling in
vertebrates: a cocktail of modulators. Dev. Biol. 250: 231-250.
6. Munger, J. S., J. G. Harpel, P. E. Gleizes, R. Mazzieri, I. Nunes, and D. B. Rifkin. 1997.
Latent transforming growth factor-beta: structural features and mechanisms of activation. Kidney
Int. 51: 1376-1382.
7. Shi, Y. and J. Massague. 2003. Mechanisms of TGF-beta signaling from cell membrane to the
nucleus. Cell 113: 685-700.
8. ten Dijke, P., H. Yamashita, H. Ichijo, P. Franzen, M. Laiho, K. Miyazono, and C. H. Heldin.
1994. Characterization of type I receptors for transforming growth factor-beta and activin.
Science 264: 101-104.
9. ten Dijke, P., H. Ichijo, P. Franzen, P. Schulz, J. Saras, H. Toyoshima, C. H. Heldin, and K.
Miyazono. 1993. Activin receptor-like kinases: a novel subclass of cell-surface receptors with
predicted serine/threonine kinase activity. Oncogene 8: 2879-2887.
10. Kirkbride, K. C., B. N. Ray, and G. C. Blobe. 2005. Cell-surface co-receptors: emerging
roles in signaling and human disease. Trends Biochem. Sci. 30: 611-621.
66
11. Gordon, K. J. and G. C. Blobe. 2008. Role of transforming growth factor-beta superfamily
signaling pathways in human disease. Biochim. Biophys. Acta 1782: 197-228.
12. Wrana, J. L., L. Attisano, J. Carcamo, A. Zentella, J. Doody, M. Laiho, X. F. Wang, and J.
Massague. 1992. TGF beta signals through a heteromeric protein kinase receptor complex. Cell
71: 1003-1014.
13. Wrana, J. L., L. Attisano, R. Wieser, F. Ventura, and J. Massague. 1994. Mechanism of
activation of the TGF-beta receptor. Nature 370: 341-347.
14. Hart, P. J., S. Deep, A. B. Taylor, Z. Shu, C. S. Hinck, and A. P. Hinck. 2002. Crystal
structure of the human TbetaR2 ectodomain--TGF-beta3 complex. Nat. Struct. Biol. 9: 203-208.
15. Massague, J. and R. R. Gomis. 2006. The logic of TGFbeta signaling. FEBS Lett. 580: 2811-
2820.
16. Liu, F., F. Ventura, J. Doody, and J. Massague. 1995. Human type II receptor for bone
morphogenic proteins (BMPs): extension of the two-kinase receptor model to the BMPs. Mol.
Cell. Biol. 15: 3479-3486.
17. Willis, S. A., C. M. Zimmerman, L. I. Li, and L. S. Mathews. 1996. Formation and activation
by phosphorylation of activin receptor complexes. Mol. Endocrinol. 10: 367-379.
18. Huse, M., Y. G. Chen, J. Massague, and J. Kuriyan. 1999. Crystal structure of the
cytoplasmic domain of the type I TGF beta receptor in complex with FKBP12. Cell 96: 425-436.
19. Huse, M., T. W. Muir, L. Xu, Y. G. Chen, J. Kuriyan, and J. Massague. 2001. The TGF beta
receptor activation process: an inhibitor- to substrate-binding switch. Mol. Cell 8: 671-682.
20. Attisano, L. and J. L. Wrana. 2000. Smads as transcriptional co-modulators. Curr. Opin. Cell
Biol. 12: 235-243.
21. Massague, J. and D. Wotton. 2000. Transcriptional control by the TGF-beta/Smad signaling
system. EMBO J. 19: 1745-1754.
67
22. Imamura, T., M. Takase, A. Nishihara, E. Oeda, J. Hanai, M. Kawabata, and K. Miyazono.
1997. Smad6 inhibits signalling by the TGF-beta superfamily. Nature 389: 622-626.
23. Nakao, A., M. Afrakhte, A. Moren, T. Nakayama, J. L. Christian, R. Heuchel, S. Itoh, M.
Kawabata, N. E. Heldin, C. H. Heldin, and P. ten Dijke. 1997. Identification of Smad7, a
TGFbeta-inducible antagonist of TGF-beta signalling. Nature 389: 631-635.
24. Chen, Y. G., A. Hata, R. S. Lo, D. Wotton, Y. Shi, N. Pavletich, and J. Massague. 1998.
Determinants of specificity in TGF-beta signal transduction. Genes Dev. 12: 2144-2152.
25. Lebrin, F., M. Deckers, P. Bertolino, and P. Ten Dijke. 2005. TGF-beta receptor function in
the endothelium. Cardiovasc. Res. 65: 599-608.
26. Chen, Y. G. and J. Massague. 1999. Smad1 recognition and activation by the ALK1 group of
transforming growth factor-beta family receptors. J. Biol. Chem. 274: 3672-3677.
27. Lopez-Novoa, J. M. and C. Bernabeu. 2010. The physiological role of endoglin in the
cardiovascular system. Am. J. Physiol. Heart Circ. Physiol. 299: H959-74.
28. Quackenbush, E. J. and M. Letarte. 1985. Identification of several cell surface proteins of
non-T, non-B acute lymphoblastic leukemia by using monoclonal antibodies. J. Immunol. 134:
1276-1285.
29. Gougos, A. and M. Letarte. 1988. Biochemical characterization of the 44G4 antigen from the
HOON pre-B leukemic cell line. J. Immunol. 141: 1934-1940.
30. Gougos, A. and M. Letarte. 1988. Identification of a human endothelial cell antigen with
monoclonal antibody 44G4 produced against a pre-B leukemic cell line. J. Immunol. 141: 1925-
1933.
31. Burrows, F. J., E. J. Derbyshire, P. L. Tazzari, P. Amlot, A. F. Gazdar, S. W. King, M.
Letarte, E. S. Vitetta, and P. E. Thorpe. 1995. Up-regulation of endoglin on vascular endothelial
cells in human solid tumors: implications for diagnosis and therapy. Clin. Cancer Res. 1: 1623-
1634.
68
32. Bernabeu, C., J. M. Lopez-Novoa, and M. Quintanilla. 2009. The emerging role of TGF-beta
superfamily coreceptors in cancer. Biochim. Biophys. Acta 1792: 954-973.
33. Torsney, E., R. Charlton, D. Parums, M. Collis, and H. M. Arthur. 2002. Inducible
expression of human endoglin during inflammation and wound healing in vivo. Inflamm. Res.
51: 464-470.
34. Gougos, A., S. St Jacques, A. Greaves, P. J. O'Connell, A. J. d'Apice, H. J. Buhring, C.
Bernabeu, J. A. van Mourik, and M. Letarte. 1992. Identification of distinct epitopes of endoglin,
an RGD-containing glycoprotein of endothelial cells, leukemic cells, and syncytiotrophoblasts.
Int. Immunol. 4: 83-92.
35. Venkatesha, S., M. Toporsian, C. Lam, J. Hanai, T. Mammoto, Y. M. Kim, Y. Bdolah, K. H.
Lim, H. T. Yuan, T. A. Libermann, I. E. Stillman, D. Roberts, P. A. D'Amore, F. H. Epstein, F.
W. Sellke, R. Romero, V. P. Sukhatme, M. Letarte, and S. A. Karumanchi. 2006. Soluble
endoglin contributes to the pathogenesis of preeclampsia. Nat. Med. 12: 642-649.
36. Qu, R., M. M. Silver, and M. Letarte. 1998. Distribution of endoglin in early human
development reveals high levels on endocardial cushion tissue mesenchyme during valve
formation. Cell Tissue Res. 292: 333-343.
37. Buhring, H. J., C. A. Muller, M. Letarte, A. Gougos, A. Saalmuller, A. J. van Agthoven, and
F. W. Busch. 1991. Endoglin is expressed on a subpopulation of immature erythroid cells of
normal human bone marrow. Leukemia 5: 841-847.
38. Kay, N. E., N. D. Bone, R. C. Tschumper, K. H. Howell, S. M. Geyer, G. W. Dewald, C. A.
Hanson, and D. F. Jelinek. 2002. B-CLL cells are capable of synthesis and secretion of both pro-
and anti-angiogenic molecules. Leukemia 16: 911-919.
39. Kestendjieva, S., D. Kyurkchiev, G. Tsvetkova, T. Mehandjiev, A. Dimitrov, A. Nikolov,
and S. Kyurkchiev. 2008. Characterization of mesenchymal stem cells isolated from the human
umbilical cord. Cell Biol. Int. 32: 724-732.
69
40. Lastres, P., T. Bellon, C. Cabanas, F. Sanchez-Madrid, A. Acevedo, A. Gougos, M. Letarte,
and C. Bernabeu. 1992. Regulated expression on human macrophages of endoglin, an Arg-Gly-
Asp-containing surface antigen. Eur. J. Immunol. 22: 393-397.
41. Adam, P. J., G. J. Clesham, and P. L. Weissberg. 1998. Expression of endoglin mRNA and
protein in human vascular smooth muscle cells. Biochem. Biophys. Res. Commun. 247: 33-37.
42. St-Jacques, S., U. Cymerman, N. Pece, and M. Letarte. 1994. Molecular characterization and
in situ localization of murine endoglin reveal that it is a transforming growth factor-beta binding
protein of endothelial and stromal cells. Endocrinology 134: 2645-2657.
43. McAllister, K. A., K. M. Grogg, D. W. Johnson, C. J. Gallione, M. A. Baldwin, C. E.
Jackson, E. A. Helmbold, D. S. Markel, W. C. McKinnon, and J. Murrell. 1994. Endoglin, a
TGF-beta binding protein of endothelial cells, is the gene for hereditary haemorrhagic
telangiectasia type 1. Nat. Genet. 8: 345-351.
44. Fernandez-Ruiz, E., S. St-Jacques, T. Bellon, M. Letarte, and C. Bernabeu. 1993.
Assignment of the human endoglin gene (END) to 9q34-->qter. Cytogenet. Cell Genet. 64: 204-
207.
45. Gougos, A. and M. Letarte. 1990. Primary structure of endoglin, an RGD-containing
glycoprotein of human endothelial cells. J. Biol. Chem. 265: 8361-8364.
46. Ge, A. Z. and E. C. Butcher. 1994. Cloning and expression of a cDNA encoding mouse
endoglin, an endothelial cell TGF-beta ligand. Gene 138: 201-206.
47. Lopez-Casillas, F., S. Cheifetz, J. Doody, J. L. Andres, W. S. Lane, and J. Massague. 1991.
Structure and expression of the membrane proteoglycan betaglycan, a component of the TGF-
beta receptor system. Cell 67: 785-795.
48. Jovine, L., C. C. Darie, E. S. Litscher, and P. M. Wassarman. 2005. Zona pellucida domain
proteins. Annu. Rev. Biochem. 74: 83-114.
49. Llorca, O., A. Trujillo, F. J. Blanco, and C. Bernabeu. 2007. Structural model of human
endoglin, a transmembrane receptor responsible for hereditary hemorrhagic telangiectasia. J.
Mol. Biol. 365: 694-705.
70
50. Bork, P. and C. Sander. 1992. A large domain common to sperm receptors (Zp2 and Zp3)
and TGF-beta type III receptor. FEBS Lett. 300: 237-240.
51. Guerrero-Esteo, M., T. Sanchez-Elsner, A. Letamendia, and C. Bernabeu. 2002. Extracellular
and cytoplasmic domains of endoglin interact with the transforming growth factor-beta receptors
I and II. J. Biol. Chem. 277: 29197-29209.
52. Raab, U., B. Velasco, P. Lastres, A. Letamendia, C. Cales, C. Langa, E. Tapia, J. P. Lopez-
Bote, E. Paez, and C. Bernabeu. 1999. Expression of normal and truncated forms of human
endoglin. Biochem. J. 339 ( Pt 3): 579-588.
53. Van Le, B., D. Franke, D. I. Svergun, T. Han, H. Y. Hwang, and K. K. Kim. 2009. Structural
and functional characterization of soluble endoglin receptor. Biochem. Biophys. Res. Commun.
383: 386-391.
54. Cheifetz, S., T. Bellon, C. Cales, S. Vera, C. Bernabeu, J. Massague, and M. Letarte. 1992.
Endoglin is a component of the transforming growth factor-beta receptor system in human
endothelial cells. J. Biol. Chem. 267: 19027-19030.
55. Cheifetz, S., H. Hernandez, M. Laiho, P. ten Dijke, K. K. Iwata, and J. Massague. 1990.
Distinct transforming growth factor-beta (TGF-beta) receptor subsets as determinants of cellular
responsiveness to three TGF-beta isoforms. J. Biol. Chem. 265: 20533-20538.
56. Bellon, T., A. Corbi, P. Lastres, C. Cales, M. Cebrian, S. Vera, S. Cheifetz, J. Massague, M.
Letarte, and C. Bernabeu. 1993. Identification and expression of two forms of the human
transforming growth factor-beta-binding protein endoglin with distinct cytoplasmic regions. Eur.
J. Immunol. 23: 2340-2345.
57. Rokhlin, O. W., M. B. Cohen, H. Kubagawa, M. Letarte, and M. D. Cooper. 1995.
Differential expression of endoglin on fetal and adult hematopoietic cells in human bone
marrow. J. Immunol. 154: 4456-4465.
58. Zhang, H., A. R. Shaw, A. Mak, and M. Letarte. 1996. Endoglin is a component of the
transforming growth factor (TGF)-beta receptor complex of human pre-B leukemic cells. J.
Immunol. 156: 564-573.
71
59. Barbara, N. P., J. L. Wrana, and M. Letarte. 1999. Endoglin is an accessory protein that
interacts with the signaling receptor complex of multiple members of the transforming growth
factor-beta superfamily. J. Biol. Chem. 274: 584-594.
60. Letamendia, A., P. Lastres, L. M. Botella, U. Raab, C. Langa, B. Velasco, L. Attisano, and C.
Bernabeu. 1998. Role of endoglin in cellular responses to transforming growth factor-beta. A
comparative study with betaglycan. J. Biol. Chem. 273: 33011-33019.
61. Scharpfenecker, M., M. van Dinther, Z. Liu, R. L. van Bezooijen, Q. Zhao, L. Pukac, C. W.
Lowik, and P. ten Dijke. 2007. BMP-9 signals via ALK1 and inhibits bFGF-induced endothelial
cell proliferation and VEGF-stimulated angiogenesis. J. Cell. Sci. 120: 964-972.
62. David, L., C. Mallet, S. Mazerbourg, J. J. Feige, and S. Bailly. 2007. Identification of BMP9
and BMP10 as functional activators of the orphan activin receptor-like kinase 1 (ALK1) in
endothelial cells. Blood 109: 1953-1961.
63. Blanco, F. J., J. F. Santibanez, M. Guerrero-Esteo, C. Langa, C. P. Vary, and C. Bernabeu.
2005. Interaction and functional interplay between endoglin and ALK-1, two components of the
endothelial transforming growth factor-beta receptor complex. J. Cell. Physiol. 204: 574-584.
64. Lopez-Casillas, F., J. L. Wrana, and J. Massague. 1993. Betaglycan presents ligand to the
TGF beta signaling receptor. Cell 73: 1435-1444.
65. Lastres, P., A. Letamendia, H. Zhang, C. Rius, N. Almendro, U. Raab, L. A. Lopez, C.
Langa, A. Fabra, M. Letarte, and C. Bernabeu. 1996. Endoglin modulates cellular responses to
TGF-beta 1. J. Cell Biol. 133: 1109-1121.
66. Li, C., I. N. Hampson, L. Hampson, P. Kumar, C. Bernabeu, and S. Kumar. 2000. CD105
antagonizes the inhibitory signaling of transforming growth factor beta1 on human vascular
endothelial cells. FASEB J. 14: 55-64.
67. Pece-Barbara, N., S. Vera, K. Kathirkamathamby, S. Liebner, G. M. Di Guglielmo, E.
Dejana, J. L. Wrana, and M. Letarte. 2005. Endoglin null endothelial cells proliferate faster and
are more responsive to transforming growth factor beta1 with higher affinity receptors and an
activated Alk1 pathway. J. Biol. Chem. 280: 27800-27808.
72
68. Scherner, O., S. K. Meurer, L. Tihaa, A. M. Gressner, and R. Weiskirchen. 2007. Endoglin
differentially modulates antagonistic transforming growth factor-beta1 and BMP-7 signaling. J.
Biol. Chem. 282: 13934-13943.
69. Bourdeau, A., D. J. Dumont, and M. Letarte. 1999. A murine model of hereditary
hemorrhagic telangiectasia. J. Clin. Invest. 104: 1343-1351.
70. Li, D. Y., L. K. Sorensen, B. S. Brooke, L. D. Urness, E. C. Davis, D. G. Taylor, B. B. Boak,
and D. P. Wendel. 1999. Defective angiogenesis in mice lacking endoglin. Science 284: 1534-
1537.
71. Arthur, H. M., J. Ure, A. J. Smith, G. Renforth, D. I. Wilson, E. Torsney, R. Charlton, D. V.
Parums, T. Jowett, D. A. Marchuk, J. Burn, and A. G. Diamond. 2000. Endoglin, an ancillary
TGFbeta receptor, is required for extraembryonic angiogenesis and plays a key role in heart
development. Dev. Biol. 217: 42-53.
72. Cho, S. K., A. Bourdeau, M. Letarte, and J. C. Zuniga-Pflucker. 2001. Expression and
function of CD105 during the onset of hematopoiesis from Flk1(+) precursors. Blood 98: 3635-
3642.
73. ten Dijke, P., M. J. Goumans, and E. Pardali. 2008. Endoglin in angiogenesis and vascular
diseases. Angiogenesis 11: 79-89.
74. Abdalla, S. A. and M. Letarte. 2006. Hereditary haemorrhagic telangiectasia: current views
on genetics and mechanisms of disease. J. Med. Genet. 43: 97-110.
75. Dakeishi, M., T. Shioya, Y. Wada, T. Shindo, K. Otaka, M. Manabe, J. Nozaki, S. Inoue, and
A. Koizumi. 2002. Genetic epidemiology of hereditary hemorrhagic telangiectasia in a local
community in the northern part of Japan. Hum. Mutat. 19: 140-148.
76. Kjeldsen, A. D., P. Vase, and A. Green. 2000. Hereditary hemorrhagic telangiectasia. A
population-based study on prevalence and mortality among Danish HHT patients. Ugeskr.
Laeger 162: 3597-3601.
73
77. Shovlin, C. L. and M. Letarte. 1999. Hereditary haemorrhagic telangiectasia and pulmonary
arteriovenous malformations: issues in clinical management and review of pathogenic
mechanisms. Thorax 54: 714-729.
78. Moussouttas, M., P. Fayad, M. Rosenblatt, M. Hashimoto, J. Pollak, K. Henderson, T. Y.
Ma, and R. I. White. 2000. Pulmonary arteriovenous malformations: cerebral ischemia and
neurologic manifestations. Neurology 55: 959-964.
79. Begbie, M. E., G. M. Wallace, and C. L. Shovlin. 2003. Hereditary haemorrhagic
telangiectasia (Osler-Weber-Rendu syndrome): a view from the 21st century. Postgrad. Med. J.
79: 18-24.
80. Johnson, D. W., J. N. Berg, M. A. Baldwin, C. J. Gallione, I. Marondel, S. J. Yoon, T. T.
Stenzel, M. Speer, M. A. Pericak-Vance, A. Diamond, A. E. Guttmacher, C. E. Jackson, L.
Attisano, R. Kucherlapati, M. E. Porteous, and D. A. Marchuk. 1996. Mutations in the activin
receptor-like kinase 1 gene in hereditary haemorrhagic telangiectasia type 2. Nat. Genet. 13: 189-
195.
81. Cymerman, U., S. Vera, A. Karabegovic, S. Abdalla, and M. Letarte. 2003. Characterization
of 17 novel endoglin mutations associated with hereditary hemorrhagic telangiectasia. Hum.
Mutat. 21: 482-492.
82. Pece, N., S. Vera, U. Cymerman, R. I. White Jr, J. L. Wrana, and M. Letarte. 1997. Mutant
endoglin in hereditary hemorrhagic telangiectasia type 1 is transiently expressed intracellularly
and is not a dominant negative. J. Clin. Invest. 100: 2568-2579.
83. Pece-Barbara, N., U. Cymerman, S. Vera, D. A. Marchuk, and M. Letarte. 1999. Expression
analysis of four endoglin missense mutations suggests that haploinsufficiency is the predominant
mechanism for hereditary hemorrhagic telangiectasia type 1. Hum. Mol. Genet. 8: 2171-2181.
84. Cymerman, U., S. Vera, N. Pece-Barbara, A. Bourdeau, R. I. White Jr, J. Dunn, and M.
Letarte. 2000. Identification of hereditary hemorrhagic telangiectasia type 1 in newborns by
protein expression and mutation analysis of endoglin. Pediatr. Res. 47: 24-35.
74
85. Paquet, M. E., N. Pece-Barbara, S. Vera, U. Cymerman, A. Karabegovic, C. Shovlin, and M.
Letarte. 2001. Analysis of several endoglin mutants reveals no endogenous mature or secreted
protein capable of interfering with normal endoglin function. Hum. Mol. Genet. 10: 1347-1357.
86. Shovlin, C. L., J. M. Hughes, J. Scott, C. E. Seidman, and J. G. Seidman. 1997.
Characterization of endoglin and identification of novel mutations in hereditary hemorrhagic
telangiectasia. Am. J. Hum. Genet. 61: 68-79.
87. Abdalla, S. A., N. Pece-Barbara, S. Vera, E. Tapia, E. Paez, C. Bernabeu, and M. Letarte.
2000. Analysis of ALK-1 and endoglin in newborns from families with hereditary hemorrhagic
telangiectasia type 2. Hum. Mol. Genet. 9: 1227-1237.
88. Abdalla, S. A., U. Cymerman, R. M. Johnson, C. M. Deber, and M. Letarte. 2003. Disease-
associated mutations in conserved residues of ALK-1 kinase domain. Eur. J. Hum. Genet. 11:
279-287.
89. Goumans, M. J., G. Valdimarsdottir, S. Itoh, A. Rosendahl, P. Sideras, and P. ten Dijke.
2002. Balancing the activation state of the endothelium via two distinct TGF-beta type I
receptors. EMBO J. 21: 1743-1753.
90. Li, C., R. Issa, P. Kumar, I. N. Hampson, J. M. Lopez-Novoa, C. Bernabeu, and S. Kumar.
2003. CD105 prevents apoptosis in hypoxic endothelial cells. J. Cell. Sci. 116: 2677-2685.
91. Mahmoud, M., K. R. Allinson, Z. Zhai, R. Oakenfull, P. Ghandi, R. H. Adams, M. Fruttiger,
and H. M. Arthur. 2010. Pathogenesis of arteriovenous malformations in the absence of
endoglin. Circ. Res. 106: 1425-1433.
92. Sanchez-Elsner, T., L. M. Botella, B. Velasco, C. Langa, and C. Bernabeu. 2002. Endoglin
expression is regulated by transcriptional cooperation between the hypoxia and transforming
growth factor-beta pathways. J. Biol. Chem. 277: 43799-43808.
93. Miller, D. W., W. Graulich, B. Karges, S. Stahl, M. Ernst, A. Ramaswamy, H. H. Sedlacek,
R. Muller, and J. Adamkiewicz. 1999. Elevated expression of endoglin, a component of the
TGF-beta-receptor complex, correlates with proliferation of tumor endothelial cells. Int. J.
Cancer 81: 568-572.
75
94. Duwel, A., N. Eleno, M. Jerkic, M. Arevalo, J. P. Bolanos, C. Bernabeu, and J. M. Lopez-
Novoa. 2007. Reduced tumor growth and angiogenesis in endoglin-haploinsufficient mice.
Tumour Biol. 28: 1-8.
95. Weidner, N., J. Folkman, F. Pozza, P. Bevilacqua, E. N. Allred, D. H. Moore, S. Meli, and G.
Gasparini. 1992. Tumor angiogenesis: a new significant and independent prognostic indicator in
early-stage breast carcinoma. J. Natl. Cancer Inst. 84: 1875-1887.
96. Tanigawa, N., H. Amaya, M. Matsumura, and T. Shimomatsuya. 1997. Association of
tumour vasculature with tumour progression and overall survival of patients with non-early
gastric carcinomas. Br. J. Cancer 75: 566-571.
97. Tanaka, F., Y. Otake, K. Yanagihara, Y. Kawano, R. Miyahara, M. Li, T. Yamada, N.
Hanaoka, K. Inui, and H. Wada. 2001. Evaluation of angiogenesis in non-small cell lung cancer:
comparison between anti-CD34 antibody and anti-CD105 antibody. Clin. Cancer Res. 7: 3410-
3415.
98. Wang, J. M., S. Kumar, D. Pye, N. Haboubi, and L. al-Nakib. 1994. Breast carcinoma:
comparative study of tumor vasculature using two endothelial cell markers. J. Natl. Cancer Inst.
86: 386-388.
99. Wikstrom, P., I. F. Lissbrant, P. Stattin, L. Egevad, and A. Bergh. 2002. Endoglin (CD105) is
expressed on immature blood vessels and is a marker for survival in prostate cancer. Prostate 51:
268-275.
100. Costello, B., C. Li, S. Duff, D. Butterworth, A. Khan, M. Perkins, S. Owens, A. F. Al-
Mowallad, S. O'Dwyer, and S. Kumar. 2004. Perfusion of 99Tcm-labeled CD105 Mab into
kidneys from patients with renal carcinoma suggests that CD105 is a promising vascular target.
Int. J. Cancer 109: 436-441.
101. Fonsatti, E., A. P. Jekunen, K. J. Kairemo, S. Coral, M. Snellman, M. R. Nicotra, P. G.
Natali, M. Altomonte, and M. Maio. 2000. Endoglin is a suitable target for efficient imaging of
solid tumors: in vivo evidence in a canine mammary carcinoma model. Clin. Cancer Res. 6:
2037-2043.
76
102. Bredow, S., M. Lewin, B. Hofmann, E. Marecos, and R. Weissleder. 2000. Imaging of
tumour neovasculature by targeting the TGF-beta binding receptor endoglin. Eur. J. Cancer 36:
675-681.
103. Matsuno, F., Y. Haruta, M. Kondo, H. Tsai, M. Barcos, and B. K. Seon. 1999. Induction of
lasting complete regression of preformed distinct solid tumors by targeting the tumor vasculature
using two new anti-endoglin monoclonal antibodies. Clin. Cancer Res. 5: 371-382.
104. Tsujie, M., S. Uneda, H. Tsai, and B. K. Seon. 2006. Effective anti-angiogenic therapy of
established tumors in mice by naked anti-human endoglin (CD105) antibody: differences in
growth rate and therapeutic response between tumors growing at different sites. Int. J. Oncol. 29:
1087-1094.
105. Fonsatti, E., L. Del Vecchio, M. Altomonte, L. Sigalotti, M. R. Nicotra, S. Coral, P. G.
Natali, and M. Maio. 2001. Endoglin: An accessory component of the TGF-beta-binding
receptor-complex with diagnostic, prognostic, and bioimmunotherapeutic potential in human
malignancies. J. Cell. Physiol. 188: 1-7.
106. Postiglione, L., G. Di Domenico, M. Caraglia, M. Marra, G. Giuberti, L. Del Vecchio, S.
Montagnani, M. Macri, E. M. Bruno, A. Abbruzzese, and G. Rossi. 2005. Differential expression
and cytoplasm/membrane distribution of endoglin (CD105) in human tumour cell lines:
Implications in the modulation of cell proliferation. Int. J. Oncol. 26: 1193-1201.
107. Liu, Y., B. Jovanovic, M. Pins, C. Lee, and R. C. Bergan. 2002. Over expression of
endoglin in human prostate cancer suppresses cell detachment, migration and invasion.
Oncogene 21: 8272-8281.
108. Wong, V. C., P. L. Chan, C. Bernabeu, S. Law, L. D. Wang, J. L. Li, S. W. Tsao, G.
Srivastava, and M. L. Lung. 2008. Identification of an invasion and tumor-suppressing gene,
Endoglin (ENG), silenced by both epigenetic inactivation and allelic loss in esophageal
squamous cell carcinoma. Int. J. Cancer 123: 2816-2823.
109. Oxmann, D., J. Held-Feindt, A. M. Stark, K. Hattermann, T. Yoneda, and R. Mentlein.
2008. Endoglin expression in metastatic breast cancer cells enhances their invasive phenotype.
Oncogene 27: 3567-3575.
77
110. Fonsatti, E., M. Altomonte, M. R. Nicotra, P. G. Natali, and M. Maio. 2003. Endoglin
(CD105): a powerful therapeutic target on tumor-associated angiogenetic blood vessels.
Oncogene 22: 6557-6563.
111. Hawinkels, L. J., P. Kuiper, E. Wiercinska, H. W. Verspaget, Z. Liu, E. Pardali, C. F. Sier,
and P. ten Dijke. 2010. Matrix metalloproteinase-14 (MT1-MMP)-mediated endoglin shedding
inhibits tumor angiogenesis. Cancer Res. 70: 4141-4150.
112. Takahashi, N., R. Kawanishi-Tabata, A. Haba, M. Tabata, Y. Haruta, H. Tsai, and B. K.
Seon. 2001. Association of serum endoglin with metastasis in patients with colorectal, breast,
and other solid tumors, and suppressive effect of chemotherapy on the serum endoglin. Clin.
Cancer Res. 7: 524-532.
113. Li, C., B. Guo, P. B. Wilson, A. Stewart, G. Byrne, N. Bundred, and S. Kumar. 2000.
Plasma levels of soluble CD105 correlate with metastasis in patients with breast cancer. Int. J.
Cancer 89: 122-126.
114. Fujita, K., C. M. Ewing, D. Y. Chan, L. A. Mangold, A. W. Partin, W. B. Isaacs, and C. P.
Pavlovich. 2009. Endoglin (CD105) as a urinary and serum marker of prostate cancer. Int. J.
Cancer 124: 664-669.
115. Sibai, B., G. Dekker, and M. Kupferminc. 2005. Pre-eclampsia. Lancet 365: 785-799.
116. Myatt, L. and R. P. Webster. 2009. Vascular biology of preeclampsia. J. Thromb. Haemost.
7: 375-384.
117. Anonymous 2000. Report of the National High Blood Pressure Education Program Working
Group on High Blood Pressure in Pregnancy. Am. J. Obstet. Gynecol. 183: S1-S22.
118. Sibai, B. M. 2003. Diagnosis and management of gestational hypertension and
preeclampsia. Obstet. Gynecol. 102: 181-192.
119. Ness, R. B. and J. M. Roberts. 1996. Heterogeneous causes constituting the single syndrome
of preeclampsia: a hypothesis and its implications. Am. J. Obstet. Gynecol. 175: 1365-1370.
78
120. Weinstein, L. 1982. Syndrome of hemolysis, elevated liver enzymes, and low platelet count:
a severe consequence of hypertension in pregnancy. Am. J. Obstet. Gynecol. 142: 159-167.
121. Kanasaki, K. and R. Kalluri. 2009. The biology of preeclampsia. Kidney Int. 76: 831-837.
122. Genbacev, O., R. Joslin, C. H. Damsky, B. M. Polliotti, and S. J. Fisher. 1996. Hypoxia
alters early gestation human cytotrophoblast differentiation/invasion in vitro and models the
placental defects that occur in preeclampsia. J. Clin. Invest. 97: 540-550.
123. Vuorela, P., S. Helske, C. Hornig, K. Alitalo, H. Weich, and E. Halmesmaki. 2000.
Amniotic fluid--soluble vascular endothelial growth factor receptor-1 in preeclampsia. Obstet.
Gynecol. 95: 353-357.
124. Zhou, Y., C. H. Damsky, and S. J. Fisher. 1997. Preeclampsia is associated with failure of
human cytotrophoblasts to mimic a vascular adhesion phenotype. One cause of defective
endovascular invasion in this syndrome? J. Clin. Invest. 99: 2152-2164.
125. Redman, C. W. and I. L. Sargent. 2005. Latest advances in understanding preeclampsia.
Science 308: 1592-1594.
126. Yinon, Y., O. Nevo, J. Xu, A. Many, A. Rolfo, T. Todros, M. Post, and I. Caniggia. 2008.
Severe intrauterine growth restriction pregnancies have increased placental endoglin levels:
hypoxic regulation via transforming growth factor-beta 3. Am. J. Pathol. 172: 77-85.
127. Vuorela-Vepsalainen, P., H. Alfthan, A. Orpana, K. Alitalo, U. H. Stenman, and E.
Halmesmaki. 1999. Vascular endothelial growth factor is bound in amniotic fluid and maternal
serum. Hum. Reprod. 14: 1346-1351.
128. Helske, S., P. Vuorela, O. Carpen, C. Hornig, H. Weich, and E. Halmesmaki. 2001.
Expression of vascular endothelial growth factor receptors 1, 2 and 3 in placentas from normal
and complicated pregnancies. Mol. Hum. Reprod. 7: 205-210.
129. Zhou, Y., M. McMaster, K. Woo, M. Janatpour, J. Perry, T. Karpanen, K. Alitalo, C.
Damsky, and S. J. Fisher. 2002. Vascular endothelial growth factor ligands and receptors that
regulate human cytotrophoblast survival are dysregulated in severe preeclampsia and hemolysis,
elevated liver enzymes, and low platelets syndrome. Am. J. Pathol. 160: 1405-1423.
79
130. Levine, R. J., C. Lam, C. Qian, K. F. Yu, S. E. Maynard, B. P. Sachs, B. M. Sibai, F. H.
Epstein, R. Romero, R. Thadhani, S. A. Karumanchi, and CPEP Study Group. 2006. Soluble
endoglin and other circulating antiangiogenic factors in preeclampsia. N. Engl. J. Med. 355: 992-
1005.
131. Maynard, S. E., J. Y. Min, J. Merchan, K. H. Lim, J. Li, S. Mondal, T. A. Libermann, J. P.
Morgan, F. W. Sellke, I. E. Stillman, F. H. Epstein, V. P. Sukhatme, and S. A. Karumanchi.
2003. Excess placental soluble fms-like tyrosine kinase 1 (sFlt1) may contribute to endothelial
dysfunction, hypertension, and proteinuria in preeclampsia. J. Clin. Invest. 111: 649-658.
132. Wallukat, G., V. Homuth, T. Fischer, C. Lindschau, B. Horstkamp, A. Jupner, E. Baur, E.
Nissen, K. Vetter, D. Neichel, J. W. Dudenhausen, H. Haller, and F. C. Luft. 1999. Patients with
preeclampsia develop agonistic autoantibodies against the angiotensin AT1 receptor. J. Clin.
Invest. 103: 945-952.
133. Luft, F. C. 2000. The preeclampsia enigma and the renin-angiotensin system. J. Mol. Med.
(Berl) 78: 63-65.
134. Xia, Y., C. C. Zhou, S. M. Ramin, and R. E. Kellems. 2007. Angiotensin receptors,
autoimmunity, and preeclampsia. J. Immunol. 179: 3391-3395.
135. Xia, Y., S. M. Ramin, and R. E. Kellems. 2007. Potential roles of angiotensin receptor-
activating autoantibody in the pathophysiology of preeclampsia. Hypertension 50: 269-275.
136. LaMarca, B. D., J. Gilbert, and J. P. Granger. 2008. Recent progress toward the
understanding of the pathophysiology of hypertension during preeclampsia. Hypertension 51:
982-988.
137. Walther, T., G. Wallukat, A. Jank, S. Bartel, H. P. Schultheiss, R. Faber, and H. Stepan.
2005. Angiotensin II type 1 receptor agonistic antibodies reflect fundamental alterations in the
uteroplacental vasculature. Hypertension 46: 1275-1279.
138. Zhou, C. C., Y. Zhang, R. A. Irani, H. Zhang, T. Mi, E. J. Popek, M. J. Hicks, S. M. Ramin,
R. E. Kellems, and Y. Xia. 2008. Angiotensin receptor agonistic autoantibodies induce pre-
eclampsia in pregnant mice. Nat. Med. 14: 855-862.
80
139. Zhou, C. C., R. A. Irani, Y. Zhang, S. C. Blackwell, T. Mi, J. Wen, H. Shelat, Y. J. Geng, S.
M. Ramin, R. E. Kellems, and Y. Xia. 2010. Angiotensin receptor agonistic autoantibody-
mediated tumor necrosis factor-alpha induction contributes to increased soluble endoglin
production in preeclampsia. Circulation 121: 436-444.
140. Dimmeler, S., E. Dernbach, and A. M. Zeiher. 2000. Phosphorylation of the endothelial
nitric oxide synthase at ser-1177 is required for VEGF-induced endothelial cell migration. FEBS
Lett. 477: 258-262.
141. Fleming, I., B. Fisslthaler, S. Dimmeler, B. E. Kemp, and R. Busse. 2001. Phosphorylation
of Thr(495) regulates Ca(2+)/calmodulin-dependent endothelial nitric oxide synthase activity.
Circ. Res. 88: E68-75.
142. Chang, V. T., M. Crispin, A. R. Aricescu, D. J. Harvey, J. E. Nettleship, J. A. Fennelly, C.
Yu, K. S. Boles, E. J. Evans, D. I. Stuart, R. A. Dwek, E. Y. Jones, R. J. Owens, and S. J. Davis.
2007. Glycoprotein structural genomics: solving the glycosylation problem. Structure 15: 267-
273.
143. Running Deer, J. and D. S. Allison. 2004. High-level expression of proteins in mammalian
cells using transcription regulatory sequences from the Chinese hamster EF-1alpha gene.
Biotechnol. Prog. 20: 880-889.
144. Kaoud, T. S., A. K. Devkota, R. Harris, M. S. Rana, O. Abramczyk, M. Warthaka, S. Lee,
M. E. Girvin, A. F. Riggs, and K. N. Dalby. 2011. Activated ERK2 is a monomer in vitro with or
without divalent cations and when complexed to the cytoplasmic scaffold PEA-15. Biochemistry
50: 4568-4578.
145. De Crescenzo, G., P. L. Pham, Y. Durocher, and M. D. O'Connor-McCourt. 2003.
Transforming growth factor-beta (TGF-beta) binding to the extracellular domain of the type II
TGF-beta receptor: receptor capture on a biosensor surface using a new coiled-coil capture
system demonstrates that avidity contributes significantly to high affinity binding. J. Mol. Biol.
328: 1173-1183.
146. Mitchell, D., E. G. Pobre, A. W. Mulivor, A. V. Grinberg, R. Castonguay, T. E. Monnell, N.
Solban, J. A. Ucran, R. S. Pearsall, K. W. Underwood, J. Seehra, and R. Kumar. 2010. ALK1-Fc
81
inhibits multiple mediators of angiogenesis and suppresses tumor growth. Mol. Cancer. Ther. 9:
379-388.
147. Castonguay, R., E. D. Werner, R. G. Matthews, E. Presman, A. W. Mulivor, N. Solban, D.
Sako, R. S. Pearsall, K. W. Underwood, J. Seehra, R. Kumar, and A. V. Grinberg. 2011. Soluble
endoglin specifically binds BMP9/BMP10 via its orphan domain,inhibits blood vessel formation
and suppresses tumor growth. J. Biol. Chem.
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