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b 3
O C
1
O H2 C HC H2 C OH OH HO OH O C R H2 C O H2 C HC O O C O C O C R R R
glycerol
fatty acid
triacylglycerol
Triacylglycerols (triglycerides) are the most abundant dietary lipids. They are the form in which we store reduced C for energy. Each triacylglycerol has a glycerol backbone to which are esterified 3 fatty acids Most triacylglycerols are mixed. The 3 fatty acids differ in chain length & number of double bonds.
O H2 C HC H2 C OH OH HO OH O C R H2 C O H2 C HC O O C O C O C R R R
glycerol
fatty acid
triacylglycerol
CH2 OH HO CH CH2 OH
ATP 1
ADP
HO
CH2 OH CH CH2 O
NAD
PO3
H + CH OH 2 NADH
C O PO3
CH2 O
glycerol
glycerol-3-P
dihydroxyacetone-P
Glycerol, arising from hydrolysis of triacylglycerols, is converted to the Glycolysis intermediate dihydroxyacetone phosphate, by reactions catalyzed by: 1 Glycerol Kinase 2 Glycerol Phosphate Dehydrogenase.
b 3
O C
1
Acyl-CoA Synthases Exergonic PPi (P~P) hydrolysis, catalyzed by Pyrophosphatase, makes the coupled reaction spontaneous. 2 ~P bonds of ATP are cleaved. The acyl-CoA product includes one "~" thioester linkage.
NH2 N N
fatty acid
O
C O
O N O CH2 H H OH O H H OH N
O O
P O
P O
P O
ATP
NH2 N N
2 Pi O R C
PPi O O P O O CH2 H H OH O H
acyladenylate
CoA
SH AMP O R C S
H OH
CoA
acyl-CoA
PPi 2 Pi
acyladenylate + HS-CoA acyl-CoA + AMP Overall: fatty acid + ATP + HS-CoA acyl-CoA + AMP + 2 Pi
Mitochondrion
b-Oxidation pathway in matrix
b-Oxidation pathway:
Fatty acids are degraded in the mitochondrial matrix via the b-Oxidation Pathway.
For most steps of the pathway there are multiple enzymes specific for particular fatty acid chain lengths.
Many of the constituent Mitochondrion enzymes are soluble proteins located in the b-Oxidation mitochondrial matrix. pathway in
But enzymes specific for very long chain fatty acids are associated with the inner membrane, facing the matrix.
matrix
Fatty acyl-CoA formed outside can pass through the outer mitochondrial membrane (which has large VDAC channels), but cannot penetrate the inner membrane.
OH CH CH2 COO +
R C O
carnitine
SCoA
Transfer of the fatty acid moiety across the mitochondrial inner membrane involves carnitine.
Carnitine Palmitoyl Transferases catalyzes transfer of a fatty acid between the thiol of Coenzyme A and the hydroxyl on carnitine.
Carnitine-mediated transfer of the fatty acyl moiety into the mitochondrial matrix is a 3-step process: 1. Carnitine Palmitoyl Transferase I, an enzyme on the cytosolic surface of the outer mitochondrial membrane, transfers a fatty acid from CoA to the OH on carnitine. 2. An antiporter in the inner mitochondrial membrane mediates exchange of carnitine for acylcarnitine.
3. Carnitine Palmitoyl Transferase II, an enzyme within the matrix, transfers the fatty acid from carnitine to CoA. (Carnitine exits the matrix in step 2.) The fatty acid is now esterified to CoA in the matrix.
O H3C C SCoA
acetyl-CoA
O
OOC
CH2
SCoA
malonyl-CoA
Control of fatty acid oxidation is exerted mainly at the step of fatty acid entry into mitochondria. Malonyl-CoA (which is also a precursor for fatty acid synthesis) inhibits Carnitine Palmitoyl Transferase I.
AMP-Activated Kinase, H3C C a sensor of cellular energy acetyl-CoA levels, is allosterically ATP + HCO3 activated by AMP, which is high in concentration ADP + Pi when [ATP] is low.
SCoA
Acetyl-CoA Carboxylase OOC CH2 C SCoA is inhibited when malonyl-CoA phosphorylated by AMPActivated Kinase, leading to decreased malonyl-CoA.
The decrease in malonyl-CoA concentration leads to increased activity of Carnitine Palmitoyl Transferase I.
Increased fatty acid oxidation then generates acetyl-CoA, for entry into Krebs cycle with associated ATP production.
AMP-Activated Kinase functions under a variety of conditions that lead to depletion of cellular ATP (reflected as increased AMP), including: glucose deprivation, exercise, hypoxia & ischaemia.
AMP-Activated Kinase in the hypothalamus of the brain is involved also in regulation of food intake.
H H O b-Oxidation 3 2 1 H3C (CH2)n C C C SCoA Pathway: b fatty acyl-CoA Step 1. Acyl-CoA H H FAD Dehydrogenase Acyl-CoA Dehydrogenase FADH2 catalyzes oxidation H O of the fatty acid H3C (CH2)n C C C SCoA moiety of acyl-CoA trans-2-enoyl-CoA H to produce a double 2 bond between carbon atomsH2O& 3. H O There are different Acyl-CoA Dehydrogenases for short (4-6 C), medium (6-10 3C), (CH2)n and CH2 C SCoA H C long C very long (12-18 C) chain fatty acids. OH Very Long Chain Acyl-CoA Dehydrogenase is bound to H+ + NADH the inner mitochondrial membrane. The others are soluble O O NAD+ enzymes located in the mitochondrial matrix.
H
2 C
O C
1
SCoA
glutamate
H H3N+ C CH2 CH2 COO
fatty acyl-CoA
Acyl-CoA Dehydrogenase
H C O C
2
SCoA
O
trans- -enoyl-CoA
FAD is the prosthetic group that functions as e acceptor H O for Acyl-CoA Dehydrogenase. Proposed mechanism:
H3C (CH2)n C CH2carboxyl extracts A Glu side-chain C SCoA
a proton from the -carbon ofOH substrate, facilitating transfer of 2 e the with H+ (a hydride) from the b position to FAD. H+ + NADH The reduced FAD accepts a 2nd H+, yielding FADH2. + O O
NAD
H C H
2
O C
1
SCoA
fatty acyl-CoA
Acyl-CoA Dehydrogenase
H C O C SCoA
trans-2-enoyl-CoA
The carbonyl O of the thioester substrate is hydrogen H O bonded to the 2'-OH C the ribityl moiety of FAD, giving of CH C SCoA H3C (CH2)n 2 this part of FAD a role in positioning the substrate and increasing acidity of OH substrate -proton. the
H+ + NADH
dimethylisoalloxazine
H C H3C H3C C C C H C C N CH2 HC OH OH N C C
O C NH C N O
2e +2H
H C H3C H3C C C C H C C
H N C C N CH2 HC OH OH
C NH C N H O
FAD
HC HC H2C
OH O O P OO
O P OO
Adenine Ribose
FADH2
HC HC H2C
OH O O P OO
O P OO
Adenine Ribose
The carbonyl O of the thioester substrate is hydrogen bonded to the 2'-OH of the ribitol moiety of FAD, giving the sugar alcohol a role in positioning the substrate and increasing acidity of the substrate -proton.
H C H
2
O C
1
SCoA
fatty acyl-CoA
Acyl-CoA Dehydrogenase
H C O C SCoA
trans-2-enoyl-CoA
H O The reactive Glu and FAD are on opposite sides of the substrateHat the active site. C SCoA 3C (CH2)n C CH2 Thus the reaction is OH stereospecific, yielding a trans double bond in enoyl-CoA. H+ + NADH
Matrix
H+ + NADH NAD+ + 2H+ 2H+ + O2 H2O
2 e Q
III IV
++
4H
+
4H
cyt c
2H+
Intermembrane Space
FADH2 is reoxidized by transfer of 2 electrons to an electron transfer flavoprotein (ETF), which in turn passes the electrons to coenzyme Q of the respiratory chain.
H C H
2
O C
1
Step 2. Enoyl-CoA Hydratase catalyzes stereospecific hydration of the trans double bond produced in the 1st step, yielding L-hydroxyacylCoenzyme A.
SCoA
fatty acyl-CoA
Acyl-CoA Dehydrogenase
H C O C SCoA
trans-2-enoyl-CoA
Enoyl-CoA Hydratase
O SCoA
3-L-hydroxyacyl-CoA
H H2O H O SCoA
Step 3. Hydroxyacyl-CoA Dehydrogenase catalyzes oxidation of the hydroxyl in the b position (C3) to a ketone. NAD+ is the electron acceptor.
NAD+ H+ + NADH
OH
3-L-hydroxyacyl-CoA
Hydroxyacyl-CoA Dehydrogenase
O O SCoA
b-Ketothiolase
b-ketoacyl-CoA
O
SCoA + CH3 C
SCoA
acetyl-CoA
O SCoA
b-ketoacyl-CoA
O
cysteine
SCoA + CH3 C
SCoA
Step 4. fatty acyl-CoA acetyl-CoA (2 C shorter) b-Ketothiolase b-Ketothiolase catalyzes thiolytic cleavage. A cysteine S attacks the b-keto C. Acetyl-CoA is released, leaving the fatty acyl moiety in thioester linkage to the cysteine thiol. The thiol of HSCoA displaces the cysteine thiol, yielding fatty acyl-CoA (2 C less).
A membrane-bound trifunctional protein complex with two subunit types expresses the enzyme activities for steps 2-4 of the b-oxidation pathway for long chain fatty acids. Equivalent enzymes for shorter chain fatty acids are soluble proteins of the mitochondrial matrix.
Summary of one round of the b-oxidation pathway: fatty acyl-CoA + FAD + NAD+ + HS-CoA fatty acyl-CoA (2 C less) + FADH2 + NADH + H+ + acetyl-CoA
The b-oxidation pathway is cyclic. The product, 2 carbons shorter, is the input to another round of the pathway. If, as is usually the case, the fatty acid contains an even number of C atoms, in the final reaction cycle butyryl-CoA is converted to 2 copies of acetyl-CoA.
Matrix
H+ + NADH NAD+ + 2H+
F1 Fo
2 e Q
III IV
++
4H
+
4H
cyt c
2H
3H+
Intermembrane Space
NADH produced during fatty acid oxidation is reoxidized by transfer of 2e to respiratory chain complex I. Transfer of 2e from complex I to oxygen causes sufficient proton ejection to yield approximately 2.5 ATP.
Recall that 4H+ enter the matrix per ATP synthesized, taking into account transmembrane flux of ADP, ATP & Pi.
Matrix
H+ + NADH NAD+ + 2H+
F1 Fo
2 e Q
III IV
++
4H+ 4H+
cyt c
2H+
3H+
Intermembrane Space
FADH2 of Acyl-CoA Dehydrogenase is reoxidized by transfer of 2e via ETF to CoQ of the respiratory chain. H+ ejection from the matrix that accompanies transfer of 2e from coenzyme Q to oxygen, leads to production of approximately 1.5 ATP.
Acetyl-CoA can enter Krebs cycle, yielding additional NADH, FADH2, and ATP.
Fatty acid oxidation is a major source of cell ATP.
Matrix
H+ + NADH NAD+ + 2H+
F1 Fo
2 e Q
III IV
++
4H+ 4H+
cyt c
2H+
3H+
Intermembrane Space
Catabolism of two 6-C glucose through Glycolysis, Krebs, & ox phos yields about 60 ~P bonds of ATP (30/glucose).
Compare energy yield oxidizing a 12-C fatty acid. Assume: 1.5 ATP produced per FADH2 reoxidized in the respiratory chain (via coenzyme Q). 2.5 ATP produced per NADH reoxidized in the respiratory chain.
How many "high energy" (~) bonds are utilized in activating the fatty acid, by 2 esterifying it to coenzyme A? ()________ How many times is the b-oxidation pathway repeated during oxidation of a 12-C 5 fatty acid? _________ 5 6 5 How many each of NADH______, FADH2______, and Acetyl CoA______ are produced, per 12-carbon fatty acid, in the b-oxidation pathway? Oxidation of each acetyl CoA in Krebs cycle yields 3 NADH and one FADH2 (from succinate), resulting in additional production of _______NADH and 18 6 _______FADH2. 23 11 Thus the yield is a total of _______NADH and _______FADH2. In the respiratory chain, approx. 2.5 ~ bonds of ATP are produced per NADH and 1.5 ~ bonds of ATP per FADH2 (electrons entering the respiratory chain via 74 coenzyme Q). Thus from reoxidation of NADH and FADH2 a total of _______ ~ bonds of ATP are produced per 12-C fatty acid. Add to this the ~P bonds of GTP produced in Krebs Cycle (one GTP per acetyl80 CoA) for a total of _______ ~P bonds produced. 78 Summing input and output yields a total of _______ ~P bonds per 12-C fatty acid YES oxidized. Does fat yield more energy than carbohydrate? _______
Human genetic diseases have been identified that involve mutations in: the plasma membrane fatty acid transporter CD36 Carnitine Palmitoyltransferases I & II (required for transfer of fatty acids into mitochondria) Acyl-CoA Dehydrogenases for various chain lengths of fatty acids Hydroxyacyl-CoA Dehydrogenases for medium & short chain length fatty acids Medium Chain b-Ketothiolase the trifunctional protein complex Electron Transfer Flavoprotein (ETF).
Human genetic diseases: Symptoms vary depending on the specific genetic defect but may include: hypoglycemia and failure to increase ketone body production during fasting fatty degeneration of the liver heart and/or skeletal muscle defects maternal complications of pregnancy sudden infant death (SIDS). Hereditary deficiency of Medium Chain Acyl-CoA Dehydrogenase (MCAD), the most common genetic disease relating to fatty acid catabolism, has been linked to SIDS.
The reactions presented accomplish catabolism of a fatty acid with an even number of C atoms & no double bonds. Additional enzymes deal with catabolism of fatty acids with an odd number of C atoms or with double bonds. The final round of b-oxidation of a fatty acid with an odd number of C atoms yields acetyl-CoA & propionyl-CoA. Propionyl-CoA is converted to the Krebs cycle intermediate succinyl-CoA, by a pathway involving vitamin B12 (to be presented later).
Most double bonds of naturally occurring fatty acids have the cis configuration.
As C atoms are removed two at a time, a double bond may end up in the wrong position or wrong configuration to be the correct substrate for EnoylCoA Hydratase.
The reactions that allow unsaturated fatty acids to be fully catabolized by the b-oxidation pathway are summarized in the textbook.
Peroxisome
Single membrane Crystalline inclusion often present
Enzymes, some of which produce H2O2 , & always including Catalase, that degrades H2O2.
FAD is e acceptor for peroxisomal Acyl-CoA Oxidase, which catalyzes the 1st oxidative step of the pathway.
Within the peroxisome, FADH2 generated by fatty acid oxidation is reoxidized producing hydrogen peroxide: FADH2 + O2 FAD + H2O2 The peroxisomal enzyme Catalase degrades H2O2: 2 H2O2 2 H2O + O2 These reactions produce no ATP.
Once fatty acids are reduced in length within the peroxisomes they may shift to the mitochondria to be catabolized all the way to CO2. Carnitine is involved in transfer of fatty acids into and out of peroxisomes.
Serious genetic diseases are associated with defects in or deficiency of enzymes of the peroxisomal b-oxidation system.
Peroxisomes also contain enzymes for an essential -oxidation pathway that degrades fatty acids having methyl branches, such as phytanic acid, a breakdown product of chlorophyll.
During fasting acetyl CoA ketone bodies or carbohydrate cholesterol starvation, oxaloacetate citrate oxaloacetate is depleted in Krebs Cycle liver due to gluconeogenesis. This impedes entry of acetyl-CoA into Krebs cycle.
Acetyl-CoA in liver mitochondria is converted then to ketone bodies, acetoacetate & b-hydroxybutyrate.
Ketone body synthesis: b-Ketothiolase. The final step of the boxidation pathway runs backward. HMG-CoA Synthase catalyzes condensation with a 3rd acetate moiety (from acetyl-CoA). HMG-CoA Lyase cleaves HMG-CoA to yield acetoacetate & acetyl-CoA.
O H3 C C SCoA + H3C
O C SCoA
acetyl-CoA
HSCoA
Thiolase
O O H2 C C
acetyl-CoA
O H3C C
H3C SCoA
SCoA
acetoacetyl-CoA
acetyl-CoA HSCoA
O
HMG-CoA Synthase
OH O H2 C C SCoA
H2 C
C CH3
HMG-CoA
O
HMG-CoA Lyase
O
O H2 C C CH3 + H3C
SCoA
acetoacetate
acetyl-CoA
b-Hydroxybutyrate CH3 + H Dehydrogenase C O NADH catalyzes reversible interconversion of CH2 the ketone bodies COO acetoacetate & acetoacetate b-hydroxybutyrate.
b-Hydroxybutyrate Dehydrogenase
CH3
NAD HO
CH CH2 COO
D-b-hydroxybutyrate
Ketone bodies are transported in the blood to other cells, where they are converted back to acetyl-CoA for catabolism in Krebs cycle, to generate ATP. While ketone bodies thus function as an alternative fuel, amino acids must be degraded to supply input to gluconeogenesis when hypoglycemia occurs, since acetate cannot be converted to glucose.