R Max Wynn, Mischa Machius, Jacinta L Chuang, Jun Li, Diana R Tomchick, David T Chuang
Index: J. Biol. Chem. 278(44) , 43402-10, (2003)
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We report here that alterations of either His291-alpha or His146-beta' in the active site of human branched-chain alpha-ketoacid dehydrogenase (E1b) impede both the decarboxylation and the reductive acylation reactions catalyzed by E1b as well as the binding of cofactor thiamin diphosphate (ThDP). In a refined human E1b active-site structure, His291-alpha, which aligns with His407 in Escherichia coli pyruvate dehydrogenase and His263 in yeast transketolase, is on a largely ordered phosphorylation loop. The imidazole ring of His291-alpha in E1b coordinates to the terminal phosphate oxygen atoms of bound ThDP. The N3 atom of wild-type His146-beta', which can be protonated, binds a water molecule and points toward the aminopyrimidine ring of ThDP. Remarkably, the H291A-alpha mutation results in a complete order-to-disorder transition of the loop region, which precludes the binding of the substrate lipoyl-bearing domain to E1b. The H146A-beta' mutation, on the other hand, does not alter the loop structure, but nullifies the reductive acylation activity of E1b. Our results suggest that: 1) His291-alpha plays a structural rather than a catalytic role in the binding of cofactor ThDP and the lipoyl-bearing domain to E1b, and 2) His146-beta' is an essential catalytic residue, probably functioning as a proton donor in the reductive acylation of lipoamide on the lipoyl-bearing domain.
| Structure | Name/CAS No. | Molecular Formula | Articles | 
|---|---|---|---|
                        ![]()  | 
                    Lipoamide
                     CAS:940-69-2  | 
                    C8H15NOS2 | 
| 
                                
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                                 1996-08-05 [Biochem. Biophys. Res. Commun. 225(1) , 268-74, (1996)]  | 
                        
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