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大肠杆菌磷酸调节子中的信号转导涉及PhoR和PhoB蛋白之间的磷酸转移。

Signal transduction in the phosphate regulon of Escherichia coli involves phosphotransfer between PhoR and PhoB proteins.

作者信息

Makino K, Shinagawa H, Amemura M, Kawamoto T, Yamada M, Nakata A

机构信息

Department of Experimental Chemotherapy, Osaka University, Japan.

出版信息

J Mol Biol. 1989 Dec 5;210(3):551-9. doi: 10.1016/0022-2836(89)90131-9.

Abstract

PhoB protein is the transcriptional activator for genes in the phosphate regulon of Escherichia coli, such as phoA and pstS, that are induced by phosphate deprivation. PhoR protein activates PhoB when phosphate is limiting and inactivates it when phosphate is in excess. We constructed a plasmid with a mutant phoR gene (phoR1084), which encoded a PhoR protein (PhoR1084) lacking the amino-terminal hydrophobic region of the intact protein. The cells carrying the plasmid overproduced PhoR1084, which was recovered in the soluble fraction of the cell lysate. We purified the Phor1084 protein and showed that it was autophosphorylated in the presence of ATP, and the phosphate group on the protein was rapidly transferred to PhoB. The phosphorylation of PhoB protein occurred concurrently with the acquisition of the ability to activate transcription from the pstS promoter. On the basis of these findings, we propose that phosphorylated PhoB protein activates transcription from the promoters of the phosphate regulon, and that the role of PhoR is to catalyze the formation and breakdown of phosphorylated PhoB in response to phosphate concentrations in the medium.

摘要

PhoB蛋白是大肠杆菌磷酸盐调节子中基因(如phoA和pstS)的转录激活因子,这些基因在磷酸盐缺乏时被诱导表达。当磷酸盐有限时,PhoR蛋白激活PhoB,而当磷酸盐过量时则使其失活。我们构建了一个携带突变型phoR基因(phoR1084)的质粒,该基因编码一种缺少完整蛋白氨基末端疏水区域的PhoR蛋白(PhoR1084)。携带该质粒的细胞过量产生PhoR1084,其存在于细胞裂解物的可溶部分中。我们纯化了PhoR1084蛋白,并表明它在ATP存在下会自动磷酸化,且蛋白上的磷酸基团会迅速转移到PhoB上。PhoB蛋白的磷酸化与获得激活pstS启动子转录的能力同时发生。基于这些发现,我们提出磷酸化的PhoB蛋白激活磷酸盐调节子启动子的转录,并且PhoR的作用是响应培养基中磷酸盐浓度催化磷酸化PhoB的形成和分解。

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