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Structural basis for the binding of succinate to succinyl-CoA synthetase

机译:绑定的琥珀酸结构依据琥珀酰辅酶合成酶

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Succinyl-CoA synthetase catalyzes the only step in the citric acid cycle that provides substrate-level phosphorylation. Although the binding sites for the substrates CoA, phosphate, and the nucleotides ADP and ATP or GDP and GTP have been identified, the binding site for succinate has not. To determine this binding site, pig GTP-specific succinyl-CoA synthetase was crystallized in the presence of succinate, magnesium ions and CoA, and the structure of the complex was determined by X-ray crystallography to 2.2 angstrom resolution. Succinate binds in the carboxy-terminal domain of the beta-subunit. The succinate-binding site is near both the active-site histidine residue that is phosphorylated in the reaction and the free thiol of CoA. The carboxy-terminal domain rearranges when succinate binds, burying this active site. However, succinate is not in position for transfer of the phosphoryl group from phosphohistidine. Here, it is proposed that when the active-site histidine residue has been phosphorylated by GTP, the phosphohistidine displaces phosphate and triggers the movement of the carboxylate of succinate into position to be phosphorylated. The structure shows why succinyl-CoA synthetase is specific for succinate and does not react appreciably with citrate nor with the other C4-dicarboxylic acids of the citric acid cycle, fumarate and oxaloacetate, but shows some activity with l-malate.
机译:琥珀酰辅酶合成酶催化唯一的一步提供的三羧酸循环作用物水平磷酸化。磷酸为底物结合位点辅酶a,,核苷酸ADP和ATP或GDP和三磷酸鸟苷已确定,绑定网站琥珀酸。网站,猪GTP-specific琥珀酰辅酶合成酶在琥珀酸的结晶,镁离子和辅酶a,和结构复杂的是由x射线晶体学2.2埃分辨率。beta-subunit carboxy-terminal域。succinate-binding站点附近的活性部位组氨酸残基磷酸化反应和自由硫醇农委会。当琥珀酸结合,埋葬这活跃的站点。然而,琥珀酸不到位磷酰基集团的转移phosphohistidine。活性位点的组氨酸残基三磷酸鸟苷磷酸化的phosphohistidine取代磷酸和触发器的运动琥珀酸的羧酸盐的位置磷酸化。琥珀酸琥珀酰辅酶合成酶是特定的与柠檬酸也反应不明显与其他C4-dicarboxylic酸的三羧酸循环、延胡索酸酯和草酰乙酸,但是与l-malate显示了一些活动。

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