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来自 fasciculata 锥虫的黄素蛋白 trypanothione 二硫化物还原酶的底物特异性。 (注:这里“trypanothione”可能是特定名称,直接保留原文未翻译,如果它有更准确的中文译名,请根据实际情况修改)

Substrate specificity of the flavoprotein trypanothione disulfide reductase from Crithidia fasciculata.

作者信息

Henderson G B, Fairlamb A H, Ulrich P, Cerami A

出版信息

Biochemistry. 1987 Jun 2;26(11):3023-7. doi: 10.1021/bi00385a011.

Abstract

The substrate specificity of the trypanosomatid enzyme trypanothione reductase has been studied by measuring the ability of the enzyme to reduce a series of chemically synthesized cyclic and acyclic derivatives of N1,N8-bis(glutathionyl)spermidine disulfide (trypanothione). Kinetic analysis of the enzymatic reduction of these synthetic substrates indicates that the mutually exclusive substrate specificity observed by the NADPH-dependent trypanothione disulfide reductase and the related flavoprotein glutathione disulfide reductase is due to the presence of a spermidine binding site in the substrate binding domain of trypanothione reductase. Trypanothione reductase will reduce the disulfide form of N1-monoglutathionylspermidine and also the mixed disulfide of N1-monoglutathionylspermidine and glutathione. The Michaelis constants for these reactions are 149 microM and 379 microM, respectively. Since the disulfide form of N1-monoglutathionylspermidine and the mixed disulfide of N1-monoglutathionylspermidine and glutathione could be formed in trypanosomatids, the binding constants and turnover numbers for the enzymatic reduction of these acyclic disulfides are consistent with these being potential alternative substrates for trypanothione reductase in vivo.

摘要

通过测量锥虫硫醇还原酶还原一系列化学合成的N1,N8 - 双(谷胱甘肽基)亚精胺二硫化物(锥虫硫醇)的环状和非环状衍生物的能力,对锥虫的锥虫硫醇还原酶的底物特异性进行了研究。对这些合成底物的酶促还原进行动力学分析表明,NADPH依赖性锥虫硫醇二硫化物还原酶和相关黄素蛋白谷胱甘肽二硫化物还原酶所观察到的互斥底物特异性,是由于锥虫硫醇还原酶的底物结合结构域中存在亚精胺结合位点。锥虫硫醇还原酶将还原N1 - 单谷胱甘肽基亚精胺的二硫化物形式,以及N1 - 单谷胱甘肽基亚精胺和谷胱甘肽的混合二硫化物。这些反应的米氏常数分别为149 microM和379 microM。由于N1 - 单谷胱甘肽基亚精胺的二硫化物形式以及N1 - 单谷胱甘肽基亚精胺和谷胱甘肽的混合二硫化物可以在锥虫中形成,这些非环状二硫化物的酶促还原的结合常数和周转数与它们在体内作为锥虫硫醇还原酶的潜在替代底物一致。

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