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高分辨率晶体结构的氟化物抑制有机磷降解金属水解酶。

High resolution crystal structure of a fluoride-inhibited organophosphate-degrading metallohydrolase.

机构信息

School of Chemistry and Molecular Biosciences, The University of Queensland, St. Lucia, Queensland 4072, Australia.

Research School of Chemistry, Australian National University, Canberra, ACT 0200, Australia.

出版信息

J Inorg Biochem. 2017 Dec;177:287-290. doi: 10.1016/j.jinorgbio.2017.06.013. Epub 2017 Jun 27.

Abstract

Metal ion-dependent, organophosphate-degrading enzymes (OP hydrolases) have received increasing attention due to their ability to degrade and thus detoxify commonly used pesticides and nerve agents such as sarin and VX. These enzymes thus garner strong potential as bioremediators. The OP hydrolase from Agrobacterium radiobacter (OpdA) is one of the most efficient members of this group of enzymes. Previous studies have indicated that the choice of the hydrolysis-initiating nucleophile may depend on the pH of the reaction, with a metal ion-bridging hydroxide being preferred at lower pH (i.e. pH≤8.5), and a terminally coordinated hydroxide at higher pH (i.e. pH>9.0). Furthermore, fluoride was shown to be a potent inhibitor of the reaction, but only at low pH. Here, the crystal structure (1.3Å, pH6) of OpdA in presence of fluoride is described. While the first coordination sphere in the active site displays minimal changes in the presence of fluoride, the hydrogen bonding network that connects the dimetallic metal center to the substrate binding pocket is disrupted. Thus, the structure of fluoride-inhibited OpdA demonstrates the significance of this hydrogen bond network in controlling the mechanism and function of this enzyme.

摘要

由于能够降解常用农药和神经毒剂(如沙林和 VX),金属离子依赖的有机磷水解酶(OP 水解酶)受到越来越多的关注。这些酶因此具有很强的生物修复潜力。土壤农杆菌来源的 OP 水解酶(OpdA)是该酶组中最有效的成员之一。先前的研究表明,水解起始亲核试剂的选择可能取决于反应的 pH 值,在较低 pH 值(即 pH≤8.5)下,金属离子桥连的氢氧化物是首选,而在较高 pH 值(即 pH>9.0)下,末端配位的氢氧化物是首选。此外,氟化物被证明是该反应的一种有效抑制剂,但仅在低 pH 值下。本文描述了氟化物存在下 OpdA 的晶体结构(1.3Å,pH6)。虽然活性位点的第一配位球在氟化物存在下变化很小,但连接双金属金属中心和底物结合口袋的氢键网络被破坏。因此,氟化物抑制的 OpdA 结构证明了该氢键网络在控制该酶的机制和功能方面的重要性。

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