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Pyruvate dehydrogenase
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Pyruvate dehydrogenase

Pyruvate dehydrogenase (E1) is the first component enzyme of pyruvate dehydrogenase complex (PDC). It thus contributes to transforming pyruvate into acetyl-CoA by a process called pyruvate decarboxylation. Acetyl-CoA may then be used in the citric acid cycle to carry out cellular respiration, so pyruvate dehydrogenase contributes to linking the glycolysis metabolic pathway to the citric acid cycle. .

Contents


Function

E1 performs the first two reactions within the complex. They are:

Regulation

Phosphorylation of E1 by pyruvate dehydrogenase kinase (PDK) inactivates E1 and subsequently the entire PDC.

This is reversed by pyruvate dehydrogenase phosphatase.

Genes

E1 is a multimeric protein:

  • Mammalian E1s, including human E1, are tetrameric, composed of two ?- and two ?- subunits.[1]
  • Some bacterial E1s, including E1 from Escherichia coli, are composed of two similar subunits, each being as large as the sum of molecular masses of ?- and ?- subunits.[2]

Catalytic sites

E1 has two catalytic sites, each providing thiamine pyrophosphate (TPP) and magnesium ion as cofactors.

  • The ?- subunit binds magnesium ion and pyrophosphate fragment.
  • The ?-subunit binds pyrimidine fragment of TPP, forming together a catalytic site at the interface of subunits.

Conformation and reactions

Biochemical and structural data for E1s revealed a mechanism of activation of TPP cofactor by forming the conserved hydrogen bond with glutamate residue (Glu59 in human E1) and by imposing a V-conformation that brings the N4? atom of the aminopyrimidine to the distance required for the intramolecular hydrogen bonding with the thiazolium C2 atom.

This unique combination of contacts and conformation of TPP leads eventually to formation of the reactive C2-carbanion.

After the cofactor TPP reacts with pyruvate, which undergoes decarboxylation, the acetyl portion becomes a hydroxyethyl derivative covalently attached to TPP.

In the second reaction, E1 transfers two electrons and the acetyl group to the second substrate, lipoic acid. This reduces the oxidized lipoic acid and transfers the acetyl group to the lipollyl group to form an acetyl thioester.

Stimulation and inhibition

Pyruvate dehydrogenase is stimulated by insulin, PEP, and AMP, but competitively inhibited by ATP, NADH, and Acetyl-CoA.

Pathology

Pyruvate dehydrogenase is an autoantigen recognized in primary biliary cirrhosis, a form of acute liver failure. These antibodies appear to recognize oxidized protein that has resulted from inflamatory immune responses. Some of these inflamatory responses are explained by gluten sensitivity.[3] Other mitochondrial autoantigens include oxoglutarate dehydrogenase and branched-chain alpha-keto acid dehydrogenase complex, which are antigens recognized by anti-mitochondrial antibodies.

Other forms

In bacteria, a form of pyruvate dehydrogenase (also called pyruvate oxidase, EC 1.2.2.2) exists that links the oxidation of pyruvate into acetate and carbon dioxide to the reduction of ferrocytochrome. In E. coli this enzyme is encoded by the pox B gene and the protein has a flavin cofactor.[4] This enzyme increases the efficiency of growth of E. coli under aerobic conditions.[5]

See also

References

External links

de:Pyruvat-Dehydrogenase-Komplex es:Piruvato deshidrogenasa fr:Pyruvate déshydrogénase it:Piruvato deidrogenasi he:?????? ?????????? pt:Piruvato desidrogenase





Source: Wikipedia | The above article is available under the GNU FDL. | Edit this article


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