Regulation of methionine synthesis in Escherichia coli: Effect of the MetR protein on the expression of the metE and metR genes

M. E. Maxon, B. Redfield, X. Y. Cai, R. Shoeman, K. Fujita, W. Fisher, G. Stauffer, H. Weissbach, N. Brot

研究成果: Article同行評審

67 引文 斯高帕斯(Scopus)

摘要

A plasmid (pRSE562) containing the metE and metR genes of Escherichia coli was used to study the expression of these genes and the role of the MetR protein in regulating metE expression. DNA sequence analysis of the 236-base-pair region separating these genes showed the presence of seven putative met boxes. When this plasmid was used to transform either wild-type E. coli, metE mutant, or metR mutant, MetE enzyme activity increased 5- to 7-fold over wild-type levels. The metR gene was subcloned from pRSE562, and this plasmid, pMRIII, relieved the methionine auxotrophy of a metR mutant after transformation. The metR gene was also cloned into a vector containing the λP(L) promoter, and the MetR protein was overexpressed and purified to near homogeneity. This protein, when added to an in vitro DNA-dependent protein synthesis system in which the MetE and/or MetR proteins were synthesized, caused a large increase in the expression of the metE gene but a decrease in the expression of the metR gene. The in vitro expression of both genes was inhibited by the MetJ protein and S-adenosylmethionine in the presence or absence of MetR protein. These results provide evidence that the product of the metR gene is a trans-activator of the expression of the metE gene and that the expression of the metR gene is under autogenous regulation and is repressed by the MetJ protein.

原文English
頁(從 - 到)85-89
頁數5
期刊Proceedings of the National Academy of Sciences of the United States of America
86
發行號1
DOIs
出版狀態Published - 1989

指紋

深入研究「Regulation of methionine synthesis in Escherichia coli: Effect of the MetR protein on the expression of the metE and metR genes」主題。共同形成了獨特的指紋。

引用此