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通过定点诱变评估氨基酸不变量在MurG活性位点中的作用。

Role of the amino acid invariants in the active site of MurG as evaluated by site-directed mutagenesis.

作者信息

Crouvoisier Muriel, Auger Geneviève, Blanot Didier, Mengin-Lecreulx Dominique

机构信息

Enveloppes Bactériennes et Antibiotiques, Institut de Biochimie et Biophysique Moléculaire et Cellulaire, UMR 8619 du CNRS, Université Paris-Sud, Bâtiment 430, 91405 Orsay Cedex, France.

出版信息

Biochimie. 2007 Dec;89(12):1498-508. doi: 10.1016/j.biochi.2007.06.011. Epub 2007 Jul 5.

Abstract

To evaluate their role in the active site of the MurG enzyme from Escherichia coli, 13 residues conserved in the sequences of 73 MurG orthologues were submitted to site-directed mutagenesis. All these residues lay within, or close to, the active site of MurG as defined by its tridimensional structure [Ha et al., Prot. Sci. 9 (2000) 1045-1052, and Hu et al., Proc. Natl. Acad. Sci. USA 100 (2003) 845-849]. Thirteen mutants proteins, in which residues T15, H18, Y105, H124, E125, N127, N134, S191, N198, R260, E268, Q288 or N291 have been replaced by alanine, were obtained as the C-terminal His-tagged forms. The effects of the mutations on the activity were checked: (i) by functional complementation of an E. coli murG mutant strain by the mutated genes; and (ii) by the determination of the steady-state kinetic parameters of the purified proteins. Most mutations resulted in an important loss of activity and, in the case of N134A, in the production of a highly unstable protein. The results correlated with the assigned or putative functions of the residues based on the tridimensional structure.

摘要

为了评估它们在大肠杆菌MurG酶活性位点中的作用,对73个MurG直系同源物序列中保守的13个残基进行了定点诱变。所有这些残基都位于根据其三维结构所定义的MurG活性位点内或附近[Ha等人,《蛋白质科学》9 (2000) 1045 - 1052,以及Hu等人,《美国国家科学院院刊》100 (2003) 845 - 849]。获得了13种突变蛋白,其中残基T15、H18、Y105、H124、E125、N127、N134、S191、N198、R260、E268、Q288或N291已被丙氨酸取代,均为C端带有组氨酸标签的形式。检查了这些突变对活性的影响:(i) 通过突变基因对大肠杆菌murG突变菌株进行功能互补;(ii) 通过测定纯化蛋白的稳态动力学参数。大多数突变导致活性大幅丧失,对于N134A突变体,还产生了一种高度不稳定的蛋白。这些结果与基于三维结构对这些残基所赋予的或推测的功能相关。

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