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蛋白质动力学控制大肠杆菌DNA修复酶AlkB催化反应循环的进程和效率。

Protein dynamics control the progression and efficiency of the catalytic reaction cycle of the Escherichia coli DNA-repair enzyme AlkB.

作者信息

Ergel Burçe, Gill Michelle L, Brown Lewis, Yu Bomina, Palmer Arthur G, Hunt John F

机构信息

From the Department of Biological Sciences, Columbia University, New York, New York 10027-6601 and.

the Department of Biochemistry and Molecular Biophysics, Columbia University, New York, New York 10032-3702.

出版信息

J Biol Chem. 2014 Oct 24;289(43):29584-601. doi: 10.1074/jbc.M114.575647. Epub 2014 Jul 20.

Abstract

A central goal of enzymology is to understand the physicochemical mechanisms that enable proteins to catalyze complex chemical reactions with high efficiency. Recent methodological advances enable the contribution of protein dynamics to enzyme efficiency to be explored more deeply. Here, we utilize enzymological and biophysical studies, including NMR measurements of conformational dynamics, to develop a quantitative mechanistic scheme for the DNA repair enzyme AlkB. Like other iron/2-oxoglutarate-dependent dioxygenases, AlkB employs a two-step mechanism in which oxidation of 2-oxoglutarate generates a highly reactive enzyme-bound oxyferryl intermediate that, in the case of AlkB, slowly hydroxylates an alkylated nucleobase. Our results demonstrate that a microsecond-to-millisecond time scale conformational transition facilitates the proper sequential order of substrate binding to AlkB. Mutations altering the dynamics of this transition allow generation of the oxyferryl intermediate but promote its premature quenching by solvent, which uncouples 2-oxoglutarate turnover from nucleobase oxidation. Therefore, efficient catalysis by AlkB depends upon the dynamics of a specific conformational transition, establishing another paradigm for the control of enzyme function by protein dynamics.

摘要

酶学的一个核心目标是了解使蛋白质能够高效催化复杂化学反应的物理化学机制。最近的方法学进展使人们能够更深入地探索蛋白质动力学对酶效率的贡献。在这里,我们利用酶学和生物物理研究,包括对构象动力学的核磁共振测量,来为DNA修复酶AlkB建立一个定量的机制方案。与其他铁/2-氧代戊二酸依赖性双加氧酶一样,AlkB采用两步机制,其中2-氧代戊二酸的氧化产生一个高反应性的酶结合氧铁中间体,就AlkB而言,该中间体缓慢地将烷基化的核碱基羟基化。我们的结果表明,微秒到毫秒时间尺度的构象转变促进了底物与AlkB结合的正确顺序。改变这种转变动力学的突变允许氧铁中间体的产生,但促进其被溶剂过早淬灭,从而使2-氧代戊二酸的周转与核碱基氧化解偶联。因此,AlkB的有效催化取决于特定构象转变的动力学,这为通过蛋白质动力学控制酶功能建立了另一个范例。

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