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实用稳态酶动力学

Practical steady-state enzyme kinetics.

作者信息

Lorsch Jon R

机构信息

Department of Biophysics and Biophysical Chemistry, Johns Hopkins University School of Medicine, Baltimore, MD, USA.

出版信息

Methods Enzymol. 2014;536:3-15. doi: 10.1016/B978-0-12-420070-8.00001-5.

Abstract

Enzymes are key components of most biological processes. Characterization of enzymes is therefore frequently required during the study of biological systems. Steady-state kinetics provides a simple and rapid means of assessing the substrate specificity of an enzyme. When combined with site-directed mutagenesis (see Site-Directed Mutagenesis), it can be used to probe the roles of particular amino acids in the enzyme in substrate recognition and catalysis. Effects of interaction partners and posttranslational modifications can also be assessed using steady-state kinetics. This overview explains the general principles of steady-state enzyme kinetics experiments in a practical, rather than theoretical, way. Any biochemistry textbook will have a section on the theory of Michaelis-Menten kinetics, including derivations of the relevant equations. No specific enzymatic assay is described here, although a method for monitoring product formation or substrate consumption over time (an assay) is required to perform the experiments described.

摘要

酶是大多数生物过程的关键组成部分。因此,在生物系统研究过程中经常需要对酶进行表征。稳态动力学提供了一种简单快速的方法来评估酶的底物特异性。当与定点诱变(见定点诱变)相结合时,它可用于探究特定氨基酸在酶的底物识别和催化中的作用。相互作用伙伴和翻译后修饰的影响也可以使用稳态动力学进行评估。本概述以实际而非理论的方式解释了稳态酶动力学实验的一般原理。任何生物化学教科书都会有关于米氏动力学理论的章节,包括相关方程的推导。这里没有描述具体的酶活性测定方法,尽管进行所述实验需要一种监测产物形成或底物随时间消耗的方法(一种测定方法)。

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