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赖氨酰氧化酶作用机制中的α-质子提取与碳负离子形成

Alpha-proton abstraction and carbanion formation in the mechanism of action of lysyl oxidase.

作者信息

Williamson P R, Kagan H M

出版信息

J Biol Chem. 1987 Jun 15;262(17):8196-201.

PMID:2885317
Abstract

Tetranitromethane (TNM) was employed as an electrophilic reagent to probe for the lysyl oxidase-catalyzed processing of n-butylamine to an intermediate carbanion during the oxidation of this amine to n-butyraldehyde according to a prior description of the use of TNM to trap enzyme-generated carbanion intermediates (Christen, P. and Riordan, J. F. (1968) Biochemistry 7, 1531-1538). The addition of n-butylamine to assay mixtures containing lysyl oxidase and TNM markedly increased the background rate of nitroform release. The Km for n-butylamine was essentially the same whether determined from the rate of lysyl oxidase-catalyzed nitroform release or from the rate of n-butyraldehyde production in the absence of TNM, the latter assessed by measurements of the rate of H2O2 formation. The initial rate of substrate- and enzyme-dependent nitroform production was linearly related to functional active site content. These data are consistent with the enzyme-dependent abstraction of an alpha-proton from the substrate to form an intermediate enzyme-bound carbanion. Kinetic analyses of the oxidation of n-butylamine and 1,1-dideutero-n-butylamine by lysyl oxidase revealed kinetic isotope effects on Vmax and Vmax/Km parameters, consistent with a rate-contributing alpha-proton abstraction step. These and other available data are incorporated into a proposal for the mechanism of action of this enzyme.

摘要

根据之前使用四硝基甲烷(TNM)捕获酶生成的碳负离子中间体的描述(克里斯滕,P.和里奥丹,J.F.(1968年)《生物化学》7,1531 - 1538),四硝基甲烷(TNM)被用作亲电试剂,以探测赖氨氧化酶催化正丁胺氧化为正丁醛过程中,正丁胺向中间碳负离子的转化情况。向含有赖氨氧化酶和TNM的测定混合物中添加正丁胺,显著提高了硝基仿释放的背景速率。无论从赖氨氧化酶催化的硝基仿释放速率,还是从在无TNM情况下正丁醛生成速率(通过测量过氧化氢生成速率来评估后者)来测定,正丁胺的米氏常数(Km)基本相同。底物和酶依赖性硝基仿生成的初始速率与功能性活性位点含量呈线性相关。这些数据与酶从底物中夺取α - 质子以形成中间的酶结合碳负离子的情况一致。对赖氨氧化酶催化正丁胺和1,1 - 二氘代正丁胺氧化的动力学分析揭示了对最大反应速率(Vmax)和Vmax/Km参数的动力学同位素效应,这与一个对速率有贡献的α - 质子夺取步骤一致。这些以及其他现有数据被纳入了关于该酶作用机制的提议中。

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