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利用同源建模和定点突变分析土曲霉顺式-环氧琥珀酸水解酶的活性位点。

Active site analysis of cis-epoxysuccinate hydrolase from Nocardia tartaricans using homology modeling and site-directed mutagenesis.

机构信息

Centre for Biotechnology, Anna University, Guindy, Chennai, India.

出版信息

Appl Microbiol Biotechnol. 2012 Mar;93(6):2377-86. doi: 10.1007/s00253-011-3548-0. Epub 2011 Sep 1.

Abstract

Cis-epoxysuccinate hydrolase (CESH, EC 3.3.2.3) from Nocardia tartaricans is known to catalyze the opening of an epoxide ring of cis-epoxysuccinate (CES), thereby converting it to corresponding vicinal diol, L(+)-tartaric acid. An attempt has been made to build a 3D homology model of CESH to investigate the structure-function relationship, and also to understand the mechanism of the enzymatic reaction. Using a combination of molecular-docking simulation and multiple sequence alignment, a set of putative residues that are involved in the CESH catalysis has been identified. Functional roles of these putative active-site residues were further evaluated by site-directed mutagenesis. Interestingly, the mutants D18A, D18E, Q20E, T22A, R55E, N134D, K164A, H190A, H190N, H190Q, D193A, and D193E resulted in complete loss of activity, whereas the mutants Y58F, T133A, S189A, and Y192D retained partial enzyme activity. Furthermore, the active-site residues responsible for the opening of CES were analyzed, and the mechanism underlying the catalytic triad involved in L(+)-tartaric acid biosynthesis was proposed.

摘要

来源于北美的土曲霉的顺式-环氧琥珀酸水解酶(CESH,EC 3.3.2.3),已知能够催化顺式-环氧琥珀酸(CES)的环氧环打开,从而将其转化为相应的顺式-二醇,L(+)-酒石酸。我们尝试构建 CESH 的 3D 同源模型,以研究结构-功能关系,并深入了解酶促反应的机制。通过分子对接模拟和多重序列比对的组合,我们确定了一组可能参与 CESH 催化的残基。通过定点突变进一步评估了这些假定的活性位点残基的功能作用。有趣的是,突变体 D18A、D18E、Q20E、T22A、R55E、N134D、K164A、H190A、H190N、H190Q、D193A 和 D193E 导致完全失去活性,而突变体 Y58F、T133A、S189A 和 Y192D 保留了部分酶活性。此外,还分析了负责 CES 开口的活性位点残基,并提出了参与 L(+)-酒石酸生物合成的催化三联体的机制。

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