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Transcript
Fatty acid synthesis Source of acetyl-CoA: food carbohydrates, some amino acids But mitochondrial reactions are required too! NADPH producing enzymes: glu-6P dehydrogenase 6P-gluconate dehydr. malic enzyme cytoplasmic isocitrate deh. Acetyl-CoA is the precursor of all kind of lipids. First, commited, regulated, rate-limiting step of fatty acid synthesis is catalyzed by: acetyl CoA carboxylase summary mixed acidic anhydride is formed then carboxyl group is transfered to biotin from carboxy-biotin to acetyl coA the carboxyl group is transfered to form malonyl CoA Acetyl CoA carboxylase domains It is a monomer here, but it is active only as polymer. Fatty acid synthase is a multifunctional dimer in humans: two proteins, each has 7 enzyme activity and one carrier arm called ACP domains: transferase reductase thioesterase Just the dimer is functional, because the synthesis of one fatty acid requires both proteins. Two fatty acids are produced at the same time. not a separate protein, but part of transferase domain R-C-S-CH2-CH2-N-pantothenate-R ║ │ O H THIOESTER BOND between fatty acid and CoA or ACP 1st cycle: then C4 (6-14) is translocated from ACP to ketoacyl synthase SH instead of acetyl-CoA acyl group translocation from ACP to ketoacyl synthase (KS) 2nd, 3rd...7th cycle of the FA synthesis till 16 C long palmityl-ACP, or in lactating mammary gland till C 6-12 long fatty acid After 7 cycles of elongation the very last step: palmitoyl-S-ACP + H2O → palmitate + H+ + HS-ACP thioesterase last domain palmitate = C 16, saturated fatty acid The overall fatty acid synthase equation for seven cycles acetyl-CoA + 7 malonyl-CoA + 14 NADPH + 14 H+ → palmitate + 7 CO2 + 8 HSCoA + 14 NADP + 6 H2O Energy cost of fatty acid synthesis: acetyl CoA carboxylase 7 acetyl-CoA + 7 ATP + 7 CO2 + 7 H2O → 7 malonyl-CoA + 7 H+ + 7 ADP + 7 Pi citrate lyase 8 citrate + 8 ATP + 8 HSCoA → 8 acetyl-CoA + 8 oxaloacetate + 8 ADP + 8 Pi REGULATION OF FATTY ACID SYNTHESIS AMP functions as an energy sensor and regulator of metabolism. When ATP production does not keep up with needs, a higher portion of a cell's adenine nucleotide pool is in the form of AMP. AMP promotes catabolic pathways that lead to synthesis of ATP, while inhibiting energy-utilizing synthetic pathways. For example, AMP regulates fatty acid synthesis and catabolism by controlling availability of malonyl-CoA. AMP-Activated Kinase catalyzes phosphorylation of Acetyl-CoA Carboxylase causing inhibition of the ATP-utilizing production of malonyl-CoA . Fatty acid synthesis is diminished by lack of the substrate malonyl-CoA. Fatty acid oxidation is stimulated due to decreased inhibition by malonyl-CoA of transfer of fatty acids into mitochondria (see section fatty acid oxidation ). A cyclic-AMP cascade, activated by the hormones glucagon and epinephrine when blood glucose is low, may also result in phosphorylation of Acetyl-CoA Carboxylase via cAMP-Dependent Protein Kinase. With Acetyl-CoA Carboxylase inhibited, acetyl-CoA remains available for synthesis of ketone bodies, the alternative metabolic fuel used when blood glucose is low. The antagonistic effect of insulin, produced when blood glucose is high, is attributed to activation of Protein Phosphatase. Regulation of Acetyl-CoA Carboxylase by local metabolites: Palmitoyl-CoA, the product of Fatty Acid Synthase, promotes the inactive conformation of Acetyl-CoA Carboxylase (diagram above), diminishing production of malonyl-CoA, the precursor of fatty acid synthesis. This is an example of feedback inhibition. Citrate allosterically activates Acetyl-CoA Carboxylase. Citrate concentration is high when there is adequate acetyl-CoA entering Krebs Cycle. Excess acetyl-CoA is then converted via malonyl-CoA to fatty acids for storage. Fatty Acid Synthase is transcriptionally regulated. •In liver: •Fatty Acid Synthase expression is stimulated by insulin, a hormone produced when blood glucose is high. Thus excess glucose is stored as fat. Transcription factors that that mediate the stimulatory effect of insulin include USFs (upstream stimulatory factors) and SREBP-1. SREBPs (sterol response element binding proteins) were first identified for their role in regulating cholesterol synthesis. •Polyunsaturated fatty acids diminish transcription of the Fatty Acid Synthase gene in liver cells, by suppressing production of SREBPs. •In fat cells: Expression of SREBP-1 and of Fatty Acid Synthase is inhibited by leptin, a hormone that has a role in regulating food intake and fat metabolism. Leptin is produced by fat cells in response to excess fat storage. Leptin regulates body weight by decreasing food intake, increasing energy expenditure, and inhibiting fatty acid synthesis.
