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线粒体甘氨酸裂解系统:在甘氨酸-二氧化碳交换中,二价阳离子对甘氨酸合成和甘氨酸脱羧的差异抑制作用。

The mitochondrial glycine cleavage system: differential inhibition by divalent cations of glycine synthesis and glycine decarboxylation in the glycine-CO2 exchange.

作者信息

Hiraga K, Kikuchi G

出版信息

J Biochem. 1982 Sep;92(3):937-44. doi: 10.1093/oxfordjournals.jbchem.a134009.

Abstract

The exchange of glycine carboxyl carbon with CO2 catalyzed by the combination of chicken liver glycine decarboxylase (P-protein) and aminomethyl carrier protein (H-protein) was markedly inhibited by various divalent cations, although extents of inhibition by individual metal ions varied considerably. Cu2+ and Zn2+, at 100 microM, inhibited the reaction almost completely, and the inhibitions by Co2+ and Ni2+ were also significant, while Mg2+ and Mn2+ did not appreciably affect the reaction. The inhibition by Zn2+ was competitive with both bicarbonate and H-protein and non-competitive with glycine. Of the two reactions involved in the glycine-CO2 exchange, decarboxylation of glycine yielding the H-protein-bound aminomethyl moiety was not significantly affected by 100 microM Zn2+ or Cu2+, but carboxylation of the H-protein-bound aminomethyl moiety to form glycine was strongly inhibited by either Zn2+ or Cu2+. Various degrees of inhibition of the glycine-CO2 exchange by other divalent metal ions could also be accounted for by the inhibition of the carboxylation step of the exchange reaction. The primary site of the action of divalent metal ions is likely to be not P-protein but H-protein, and the binding of metal ions with the H-protein-bound intermediate of glycine decarboxylation was assumed to account for the observed marked inhibition.

摘要

鸡肝甘氨酸脱羧酶(P蛋白)和氨甲基载体蛋白(H蛋白)联合催化的甘氨酸羧基碳与二氧化碳的交换反应受到多种二价阳离子的显著抑制,尽管不同金属离子的抑制程度差异很大。100微摩尔的Cu2+和Zn2+几乎完全抑制了该反应,Co2+和Ni2+的抑制作用也很显著,而Mg2+和Mn2+对反应没有明显影响。Zn2+的抑制作用对碳酸氢盐和H蛋白均表现为竞争性,对甘氨酸则为非竞争性。在甘氨酸-二氧化碳交换所涉及的两个反应中,甘氨酸脱羧生成与H蛋白结合的氨甲基部分的反应不受100微摩尔Zn2+或Cu2+的显著影响,但H蛋白结合的氨甲基部分羧化形成甘氨酸的反应则受到Zn2+或Cu2+的强烈抑制。其他二价金属离子对甘氨酸-二氧化碳交换反应的不同程度抑制作用也可以通过对交换反应羧化步骤的抑制来解释。二价金属离子的主要作用位点可能不是P蛋白而是H蛋白,并且金属离子与甘氨酸脱羧反应中与H蛋白结合的中间体的结合被认为是观察到的显著抑制作用的原因。

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