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大肠杆菌中的跨膜信号转导与渗透调节:I. 对EnvZ和OmpR这两个调节成分之间磷酸转移所涉及的氨基酸残基进行定点诱变分析。

Transmembrane signal transduction and osmoregulation in Escherichia coli: I. Analysis by site-directed mutagenesis of the amino acid residues involved in phosphotransfer between the two regulatory components, EnvZ and OmpR.

作者信息

Kanamaru K, Aiba H, Mizuno T

机构信息

Laboratory of Microbiology, School of Agriculture, Nagoya University, Aichi.

出版信息

J Biochem. 1990 Sep;108(3):483-7. doi: 10.1093/oxfordjournals.jbchem.a123225.

DOI:10.1093/oxfordjournals.jbchem.a123225
PMID:2277041
Abstract

Previously, the transfer of a phosphoryl group between the EnvZ and OmpR proteins, which are involved in expression of the ompF and ompC genes in response to the medium osmolarity, was demonstrated in vitro. In this study, the histidine (His) residue at position 243 of the EnvZ protein, and the aspartate (Asp) residues at positions 12 and 55 of the OmpR protein were changed, respectively, by means of site-directed mutagenesis. We characterized the mutant proteins in terms of not only their in vitro phosphotransfer reactions but also their in vivo osmoregulatory phenotypes. The mutant EnvZ protein was defective in its in vitro ability not only as to EnvZ-autophosphorylation but also OmpR-phosphorylation and OmpR-dephosphorylation. This particular mutant EnvZ protein seemed to exhibit null functions as to the in vivo osmoregulatory phenotype. The mutant OmpR protein with the amino acid change at position 12 was clearly phosphorylated in vitro, but at a very low rate as compared with the wild-type OmpR protein. In vitro phosphorylation of the mutant OmpR protein with the amino acid change at position 55 was more severely affected. This mutant OmpR protein appeared to exhibit null functions as to the in vivo osmoregulatory phenotype. These results suggest that the histidine residue at position 243 of the EnvZ protein and the aspartate residues at positions 12 and 55 of the OmpR protein are deeply involved in the phosphotransfer between the EnvZ and OmpR proteins.

摘要

先前已在体外证明,参与响应培养基渗透压而表达ompF和ompC基因的EnvZ和OmpR蛋白之间存在磷酰基转移。在本研究中,通过定点诱变分别改变了EnvZ蛋白第243位的组氨酸(His)残基以及OmpR蛋白第12位和第55位的天冬氨酸(Asp)残基。我们不仅根据突变蛋白的体外磷转移反应,还根据其体内渗透调节表型对它们进行了表征。突变的EnvZ蛋白在体外不仅在EnvZ自身磷酸化方面存在缺陷,而且在OmpR磷酸化和OmpR去磷酸化方面也存在缺陷。这种特定的突变EnvZ蛋白在体内渗透调节表型方面似乎表现出无效功能。第12位氨基酸发生变化的突变OmpR蛋白在体外明显被磷酸化,但与野生型OmpR蛋白相比,磷酸化速率非常低。第55位氨基酸发生变化的突变OmpR蛋白的体外磷酸化受到的影响更大。这种突变OmpR蛋白在体内渗透调节表型方面似乎表现出无效功能。这些结果表明,EnvZ蛋白第243位的组氨酸残基以及OmpR蛋白第12位和第55位的天冬氨酸残基与EnvZ和OmpR蛋白之间的磷转移密切相关。

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