5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2-...

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5.1 Mitochondrial structure and function • 1. Living fibroblast • 2. TEM • 3. Sperm midpiece • 1-4μm, 0.2- 1.0μm
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Transcript of 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2-...

Page 1: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

5.1 Mitochondrial structure and function

• 1. Living fibroblast

• 2. TEM

• 3. Sperm midpiece

• 1-4μm, 0.2- 1.0μm

Page 2: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

1. Mitochondrial membranes

• The outer membrane is thought to be homologous to an outer membrane present as part of the cell wall of certain bacterial cells.

• The inner membrane is highly impermeable; all molecules and ions require special membrane transporters to gain entrance to the matrix.

Page 3: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

5.1 Mitochondrial structure and function

• 1. Living fibroblast

• 2. TEM

• 3. Sperm midpiece

• 1-4μm, 0.2- 1.0μm

Page 4: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

1. Mitochondrial membranes

• The outer membrane is thought to be homologous to an outer membrane present as part of the cell wall of certain bacterial cells.

• The inner membrane is highly impermeable; all molecules and ions require special membrane transporters to gain entrance to the matrix.

Page 5: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

2. The mitochondrial matrix

• Possess ribosomes, circular DNA to manufacture their own RNAs and proteins

Page 6: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

5.2 Oxidative metabolism in the mitochondrion

Page 7: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

• Pyruvate + HS-CoA + NAD+ → acetyl CoA + CO2 + NADH + H+

Page 8: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

1. The Tricarboxylic Acid (TCA) cycle

• Acetyl CoA + 2 H2O + FAD + 3 NAD+ + GDP + Pi → 2 CO2 + FADH2 + 3 NADH + 3H+ + GTP +HS-CoA

Page 9: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

The glycerol phosphate shuttle

• Electrons are transferred from NADH to dihydroxyacetone phosphate (DHAP) to form glycerol 3-phosphate, which shuttles them into the mitochondrion. These electrons then reduce FAD at the inner membrane, forming FADH2 which can transfer the electrons to a carrier of the electron-transport chain.

Page 10: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

2. The importance of reduced coenzymes in the formation of ATP

(Chemiosmosis)• 1. High-energy electrons are passed from

FADH2 or NADH to the first of a series of electron carriers in the electron transport chain.

• 2. The controlled movement of protons back across the membrane through an ATP-synthesizing enzyme provides the energy required to form ATP from ADP.

Page 11: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

5.3 The role of mitochondria in the formation of ATP

• 1. Oxidation-reduction potentials

• 2. Electron transport

• 3. Types of electron carriers

Page 12: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

1. Oxidation –reduction potential

Oxidizing agents can be ranked in a series according to their affinity for electrons:

the greater the affinity, the stronger the oxidizing agent.

Page 13: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Reducing agents can also be ranked according to their affinity for electrons:

• The lower the affinity, the stronger the reducing agent

• Reducing agents are ranked according to electron-transfer potential, such as NADH is strong reducing agent, whereas those with low electron-transfer potential such as H2O, are weak reducing agents.

Page 14: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Oxidizing and reducing agents occur as couples such as NAD+ and NADH which differ in their electrons.Strong reducing agents are coupled to weak oxidizing agents and vice versa. For example, in NAD+ - NADH, NAD + is a weak oxidizing agent, in O2 – H2O, O2 is a strong oxidizing agent

Page 15: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

The affinity of substances for electrons can be measured by instruments that detect voltage—oxidation-reduction (redox) potential.

Page 16: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

2. Electron transport

• 1. Five of the nine reactions in Fig. 5.7 are catalyzed by dehydrogenases that transfer pairs of electrons fron substrates to coenzymes, NADH and FADH2 → electron-transport chain

• 2. NADH and FADH2 dehydrogenase are located in the inner membrane of mitochondria.

Page 17: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

3. Types of electron carriers

• Flavoproteins (FMN of NADH dehydrogenase)• Cytochromes (heme group)• Three copper atoms• Ubiquinone (Coenzyme Q)• Iron-sulfur proteins• With the exception of ubiquinone, all of the redox centers

within the respiratory chain that accept and donate electrons are prosthetic groups (non-amino acid components that are tightly associated with proteins)

Page 18: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Electron-transport complexes

• 1. Complexes I, II, III, IV ----Fixed in place • 2. I, III, VI in which the transfer of electrons is ac

companied by a major release of free energy. • 2. Ubiquinone (lipid-soluble), cytochrome c (solu

ble protein in the intermembrane space)----move within or along the membrane

Page 19: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Experimental demonstration that cytochrome oxidase is a proton pump

Page 20: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Translocation of protons and the establishment of a proton-motive force

• Concentration difference between hydrogen ions between the inside and outside of the membrane (∆ pH)

• Voltage difference (Ψ)that results from the separatopn of charge across the membrane

• Electrochemical gradient → proton motive force (∆p)• ∆p = Ψ-2.3 (RT/F)∆ pH• The permeability of the inner membrane to Cl ions• Uncoupling proteins (UCP)

Page 21: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

5.5 The mechinery for ATP formation

• 1. The structure of ATP synthase

• 2. The basis of ATP formation according to the binding change mechanism

• 3. Other roles for the proton-motive force in addition to ATP synthesis

Page 22: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

RECALL THAT:

• 1. Enzymes do not affect the equilibrium constant of the reaction they catalyze

• 2. Enzymes are capable of catalyzing both the forward and reverse reactions

Page 23: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

2. The basis of ATP formation according to the binding change

mechanism

• 1979 Paul Boyer (UCLA): published a hypothesis “ binding change mechanism”

Page 24: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

“Seeing is beliving”

• Masasuke Yoshida et al. at the Tokyo Institute Technology in Japan

• They devised an system to watch the enzyme catalyze the reverse reaction from the normally operating cell.

Page 25: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Only two biological structures are known that contain rotating parts

• 1. ATP synthase• 2. Bacterial flagella• 3. Both are described as rotary “nanomac

hines”• 4. Invent nanoscale devices • 5. Someday, human may be using ATP ins

tead of electricity to power some of their most delicate instruments.

Page 26: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Using the proton gradient to drive the catalytic machinery:

• 1. What is the path taken by protons as they move through the F0 complex?

• 2. How does this movement lead to the synthesis of ATP?

• 3. The role of the F0 portion of ATP synthase

Page 27: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

All of the following presumptions were confirmed by data collection between 1995-

2001• 1. The c subunit of the F0 base were assembled into a rin

g that resides within the lipid bilayer.• 2. The c ring is physically bound to the γsubunit of the st

alk.• 3. The “downhill” movement of protons through the mem

brane drives the rotation of the ring of c subunit.

• 4. The rotation of the c ring of F0 provides the twisting force that drives the rotation of the attached γsubunit, leading to the synthesis and release of ATP.

Page 28: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Rotation of the c ring drives rotation of the attached γsubunit

H+ movements drive the rotation of the c ring

1. Each “a” subunit has two half-channels that are physically separate

2. From intermembrane space into “a” subunit

4. From the middle of the “a” subunit into the matrix

3. Binding of the H+ to the carboxyl group of aspartic acid generates a major conformational change in the c subunit to rotate 30o

in a Counter-clockwise direction.

Page 29: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

1. Movement of the ring is driven by the conformational changes associated with the sequential protonation and deprotonation of the aspartic acid residue of each “c” subunit.

2. In this case, the association/dissociation of 4 protons in the manner described would move the ring 120o.

3. This would drive a corresponding rotation of the attached γsubunit 120o and lead to release newly synthesized ATP.

4. The translocation of 12 protons would lead to the full 360orotation of the c ring and γunit and synthesis of 3 molecules of ATP.

Page 30: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

Other roles for the proton-motive force in addition to ATP synthesis

Page 31: 5.1 Mitochondrial structure and function 1. Living fibroblast 2. TEM 3. Sperm midpiece 1-4μm, 0.2- 1.0μm.

GLYOXYSOME IN PLANT SEEDLINGS

• 1. conversion of stored fatty acids to carbohydrate

• 2. disassembly of stored fatty acids generates acetyl CoA, which condenses with oxaloacetate to form citrate, which is then converted into glucose by a series of enzymes of the glyoxylate cycle localized in the glyoxysome.