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1,10-菲咯啉对鸡肝丙酮酸羧化酶的失活作用。

Inactivation of chicken liver pyruvate carboxylase by 1,10-phenanthroline.

作者信息

Carver J A, Baldwin G S, Keech D B, Bais R, Wallace J C

机构信息

Department of Biochemistry, University of Adelaide, South Australia.

出版信息

Biochem J. 1988 Jun 1;252(2):501-7. doi: 10.1042/bj2520501.

Abstract

Inactivation of chicken liver pyruvate carboxylase by the chelating agent 1,10-phenanthroline follows pseudo-first-order kinetics. The hyperbolic dependence of the apparent first-order rate constant on 1,10-phenanthroline concentration is consistent with a two-step inactivation mechanism, in which 1,10-phenanthroline binds firstly to the enzyme, and secondly to the enzyme-bound Mn(II) ion. Binding of 1,10-phenanthroline to pyruvate carboxylase results in complete loss of ATP/Pi exchange activity, but only a 61% decrease in pyruvate/oxaloacetate exchange activity. The rate of inactivation is greater at low enzyme concentrations, implying that binding of 1,10-phenanthroline to monomers and dimers is preferred relative to that of tetramers. Furthermore, in the presence of acetyl-CoA, which stabilizes the tetrameric structure, no dependence of inactivation on enzyme concentration is observed. As monitored by gel-permeation liquid chromatography, formation of the enzyme-Mn(II)-phenanthroline complex results in loss of the tetrameric structure of the enzyme. From atomic-absorption measurements, inactivation by 1,10-phenanthroline also causes some loss of Mn(II) from the enzyme. It is concluded that the Mn(II) atom does not participate directly in the reaction mechanism, but may play a structural role essential to the integrity of the enzyme's tetrameric structure.

摘要

螯合剂1,10 - 菲咯啉使鸡肝丙酮酸羧化酶失活遵循准一级动力学。表观一级速率常数对1,10 - 菲咯啉浓度的双曲线依赖性与两步失活机制一致,其中1,10 - 菲咯啉首先与酶结合,其次与酶结合的Mn(II)离子结合。1,10 - 菲咯啉与丙酮酸羧化酶的结合导致ATP/Pi交换活性完全丧失,但丙酮酸/草酰乙酸交换活性仅降低61%。在低酶浓度下失活速率更快,这意味着相对于四聚体,1,10 - 菲咯啉与单体和二聚体的结合更受青睐。此外,在稳定四聚体结构的乙酰辅酶A存在下,未观察到失活对酶浓度的依赖性。通过凝胶渗透液相色谱监测,酶 - Mn(II) - 菲咯啉复合物的形成导致酶的四聚体结构丧失。通过原子吸收测量,1,10 - 菲咯啉引起的失活还导致酶中Mn(II)的一些损失。得出的结论是,Mn(II)原子不直接参与反应机制,但可能对酶的四聚体结构的完整性起至关重要的结构作用。

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