topic 3 the neuronal membrane at rest lange biology 463 - neurobiology
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Topic 3
The Neuronal Membrane at Rest
Lange
Biology 463 - Neurobiology
Introduction
Resting Potential – the chemical makeup of the neuron when it is at “rest”…. meaning there is no message present
Action Potential – the chemical makeup of the neuron when it is “active”…. meaning there is a message present
Please note that the image above displays neurons in a way that can perpetuate a misconception: The Action Potential does NOT occur throughout the entire neuron instantly, but instead… the Action Potential will exist in a small portion of the neuron and will travel along the length of the neuron.
The Cast of Chemicals Involved the Generation of an Action Potential
• Cytosolic and Extracellular Fluids– water is a polar solvent– Various cations (+) and anions (-)
• The Phospholipid Membrane– Hydrophilic (Polar) Head
• Materials that dissolve in water will pass through – Hydrophobic (Nonpolar) Tails
• Materials that dissolve in water will NOT pass through• Materials that dissolve in non-polar solvents (such as oils)
will pass through
– The phospholipids will aggregate in a water media to create what is known as the Phospholipid Bilayer
With the phospholipid molecule having the polar head region and the nonpolar tail region, when the phospholipid bilayer (PLB) is formed, the property that is seen is a PLB that serves as a selectively permeable membrane… a crucial feature for message transport both in the “electrical message” and the chemical message aspect of the neuron.
• Proteins
– Molecules
• Enzymes
• Cytoskeletal elements
• Receptors
• Specialized transmembrane proteins
– Control resting and action potentials
It is estimated that there can be hundreds of billions of different types of proteins that can be made, and our best estimate is that there are roughly 100,000 different proteins produced and used in the human body.
• Protein structure is enormously diverse:
• The 20 different amino acids consisting of an alpha carbon, a carboxyl group, hydrogen, and some sort of R (residue) group
• Diversity is due to the variation in the R group
In the neuron, proteins are synthesized by ribosomes in two primary areas:
– Neuronal cell body (soma)– Axon terminals
In both places, the ribosomes assemble amino acids into polypeptide chains (connected by polypeptides)
Levels of protein structure.
Secondary structure:The primary chain formsspirals (-helices) andsheets (-sheets).
Tertiary structure:Superimposed on secondary structure.
-Helices and/or -sheets are folded upto form a compact globular moleculeheld together by intramolecular bonds.
Quaternary structure:Two or more polypeptide chains, eachwith its own tertiary structure, combineto form a functional protein.
Tertiary structure of prealbumin(transthyretin), a protein thattransports the thyroid hormonethyroxine in serum and cerebro-spinal fluid.
Quaternary structure of afunctional prealbumin molecule.Two identical prealbumin subunitsjoin head to tail to form the dimer.
Amino acid Amino acid Amino acid Amino acid Amino acid
-Helix: The primary chain is coiledto form a spiral structure, which isstabilized by hydrogen bonds.
-Sheet: The primary chain “zig-zags” backand forth forming a “pleated” sheet. Adjacentstrands are held together by hydrogen bonds.
(a) Primary structure: The sequence of amino acids forms the polypeptide chain.
(b)
(c)
(d)
(a) Primary structure: The sequence of amino acids forms the polypeptide chain.
Amino acid Amino acid Amino acid Amino acid Amino acid
-Helix: The primary chain is coiledto form a spiral structure, which isstabilized by hydrogen bonds.
-Sheet: The primary chain “zig-zags” backand forth forming a “pleated” sheet. Adjacentstrands are held together by hydrogen bonds.
(b) Secondary structure:The primary chain forms spirals (-helices) and sheets (-sheets).
Tertiary structure of prealbumin(transthyretin), a protein thattransports the thyroid hormonethyroxine in serum and cerebro-spinal fluid.
(c) Tertiary structure: Superimposed on secondary structure. -Helices and/or -sheets are folded up to form a compact globular molecule held together by intramolecular bonds.
Levels of protein structure.
Quaternary structure ofa functional prealbuminmolecule. Two identicalprealbumin subunitsjoin head to tail to formthe dimer.
(d) Quaternary structure: Two or more polypeptide chains, each with its own tertiary structure, combine to form a functional protein.
An example of the progression in complexity of structure in proteins with the final quaternary structure being that of hemoglobin.
Proteins develop in a variety of forms in neurons to form
– Ion channels using channel proteins
– Ion pumps using other proteins
The Movement of Ions
• Simple diffusion is an option for small ions and other small molecules
• Electrical current influences ion movement
• Electrical conductance (g) and resistance (R);
R = 1/g
• Electrical potential (voltage)
Electricity and Circuits
Chemicals Involved in the Conduction of Electricity• Electricity
– Electrical current can flow across a membrane
– Ohm’s law I = gV (current = conductance x electrical potential)
The Ionic Basis of The Resting Membrane Potential
• Membrane potential: Voltage across the neuronal membrane
• Equilibrium Potential (Eion) – No net movement of ions
when separated by a phospholipid membrane
– Equilibrium reached when K+ channels inserted into the phospholipid bilayer
– Electrical potential difference that exactly balances ionic concentration gradient
• Equilibrium Potential
Voltmeter
Microelectrodeinside cell
Plasmamembrane
Ground electrodeoutside cell
Neuron
Axon
Depolarizing stimulus
Mem
bra
ne
po
ten
tial
(vo
ltag
e, m
V)
Time (ms)
0–100
–70
0
–50 –50
+50
1 2 3 4 5 6 7
Hyperpolarizing stimulus
Mem
bra
ne
po
ten
tial
(vo
ltag
e, m
V)
Time (ms)
0 1 2 3 4 5 6 7–100
–70
0
+50
Insidepositive
Insidenegative
(a) (b)
Restingpotential
DepolarizationRestingpotential
Hyper-polarization
(b)
Depolarized region Stimulus
Plasmamembrane
Depolarization Spread of depolarization(a)
Distance (a few mm)
–70Resting potential
Active area(site of initialdepolarization)
Mem
bra
ne
po
ten
tial
(m
V)
Copyright © 2010 Pearson Education, Inc.
0 1 2 3 4
–70–55
0
+30
Mem
bra
ne
po
ten
tial
(m
V)
Time (ms)
Rel
ativ
e m
emb
ran
e p
erm
eab
ilit
y
Na+Na+
K+
K+
Outsidecell
Insidecell
Outsidecell
Insidecell
Depolarizing phase: Na+
channels open
Repolarizing phase: Na+
channels inactivating, K+
channels open
Action potential
PNa
PKThreshold
Na+
Na+
K+K+
Outside cell
Insidecell
Outsidecell
Insidecell
Inactivation gate
Activationgates
Potassiumchannel
Sodiumchannel
Resting state: All gated Na+
and K+ channels closed (Na+ activation gates closed; inactivation gates open)
Hyperpolarization: K+
channels remain open; Na+ channels resetting
2
2
3
4
4
1
11
3
–70
+30
(a) Time = 0 ms (b) Time = 2 ms (c) Time = 4 ms
Voltageat 2 ms
Voltageat 4 ms
Voltageat 0 ms
Resting potential
Peak of action potential
Hyperpolarization
Me
mb
ran
e p
ote
nti
al
(mV
))
Time (ms)
Vo
ltag
eM
emb
ran
e p
ote
nti
al (
mV
)
–70
0
+30
Threshold
Actionpotentials
Stimulusamplitude
Stimulus
Mem
bra
ne
po
ten
tial
(m
V)
Time (ms)
–70
0
+30
0 1 2 3 4 5
Absolute refractoryperiod
Relative refractoryperiod
Depolarization(Na+ enters)
Repolarization(K+ leaves)
After-hyperpolarization
• Equilibrium Potentials (Cont’d)– The Nernst Equation
• Calculates the exact value of the equilibrium potential for each ion in mV
• Takes into consideration:– Charge of the ion– Temperature– Ratio of the external and internal ion concentrations
• The Distribution of Ions Across The Membrane
• The sodium-potassium pump– Enzyme - breaks down ATP when Na present– Calcium pump: Actively transports Ca2+ out of
cytosol
Na+ Na+
K+
K+
K+
K+
Na+
Na+
Na+
Na+
Cell interiorNa+
15 mMK+
150 mMCl–
10 mM A–
100 mMNa+
150 mMA–
0.2 mM
Cell exterior
K+
5 mM Cl–
120 mM
Cellexterior
Cellinterior
Plasmamembrane
Na+–K+
pumpDif
fusi
on
K+ N
a+ D
iffus
ion
-70 mV
Seymour Benzer – research leader in studies of Shaker Flies. In the 1970s, his lab was able to associate this mutant’s behavior to a gene that affects potassium channel development.
Shaker Potassium Channels
Genetic approaches include screening for behavioral changes in animals with mutations in K+ channel genes. Such genetic methods allowed the genetic identification of the "Shaker" K+ channel gene in Drosophila before ion channel gene sequences were well known.
The Shaker (Sh) gene, when mutated, causes a variety of atypical behaviors in the fruit fly, Drosophila melanogaster. Under ether anesthesia, the fly’s legs will shake (hence the name); even when the fly is unanaesthetized, it will exhibit aberrant movements. Sh-mutant flies have a shorter lifespan than regular flies; in their larvae, the repetitive firing of action potentials as well as prolonged exposure to neurotransmitters at neuromuscular junctions occurs.
The Sh gene plays a part in the operation of potassium ion channels, which are integral membrane proteins and are essential to the correct functioning of the cell.
• Relative Ion Permeabilities of the Membrane at Rest – K+ channels: 4 subunits – Channel selectively permeable to K+
ions– MacKinnon—2003 Nobel Prize
• Mutations of specific K+ channels; Inherited neurological disorders
END.
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