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活化的枯草芽孢杆菌 Pho 应答调节因子 PhoP~P 的衰变涉及 PhoR~P 中间体。

Decay of activated Bacillus subtilis pho response regulator, PhoP approximately P, involves the PhoR approximately P intermediate.

作者信息

Shi L, Liu W, Hulett F M

机构信息

Laboratory for Molecular Biology, Department of Biological Sciences, University of Illinois at Chicago 60607, USA.

出版信息

Biochemistry. 1999 Aug 3;38(31):10119-25. doi: 10.1021/bi990658t.

Abstract

PhoR of Bacillus subtilis is a histidine sensor-kinase belonging to the family of two-component signal transduction systems. PhoR is responsible for processing the phosphate-starvation signal and providing phosphate input to regulate the level of phosphorylated response regulator, PhoP, which activates/represses Pho regulon gene transcription. The catalytic domain of PhoR is sufficient for the low-phosphate inducible expression of Pho regulon genes since removing the N-terminal membrane-associated domain did not alter the kinetics of Pho induction, albeit the total level of induction was decreased (1). In this study we showed that the complete B. subtilis PhoR protein produced in Escherichia coli can be reverse phosphorylated by PhoP-phosphate. We also used a C-terminal fragment of the PhoR protein, PhoR, to demonstrate that the phosphoryl group on phospho-PhoP was transferred back to PhoR in the reverse phosphorylation reaction or released as inorganic phosphate to the reaction mixture. The reverse phosphorylation of the PhoR protein likely occurs at the same histidine residue (His360) that is utilized for the autokinase reaction by the same protein. In the presence of ADP, the phosphoryl group is further transferred to ADP to form ATP. While the autokinase reaction, the forward phosphotransfer reaction from PhoR approximately P to PhoP, and the release of inorganic phosphate from PhoP approximately P in the presence of PhoR require Mg(2+), the reverse phosphotransfer from PhoP approximately P to PhoR does not. These results indicate that the energy levels of the phosphoryl groups on PhoP and PhoR are very similar. The reversible autokinase reaction and/or the reversible phosphotransfer reaction between PhoR approximately P and PhoP may have a role in PhoP approximately P decay thus influencing the PhoP approximately P concentration in the cell.

摘要

枯草芽孢杆菌的PhoR是一种组氨酸传感器激酶,属于双组分信号转导系统家族。PhoR负责处理磷酸盐饥饿信号,并提供磷酸盐输入以调节磷酸化反应调节因子PhoP的水平,PhoP可激活/抑制Pho调控子基因转录。PhoR的催化结构域足以实现Pho调控子基因的低磷酸盐诱导表达,因为去除N端膜相关结构域不会改变Pho诱导的动力学,尽管诱导的总水平有所降低(1)。在本研究中,我们表明在大肠杆菌中产生的完整枯草芽孢杆菌PhoR蛋白可被PhoP-磷酸盐反向磷酸化。我们还使用了PhoR蛋白的C端片段PhoR,以证明磷酸化PhoP上的磷酰基在反向磷酸化反应中转移回PhoR或作为无机磷酸盐释放到反应混合物中。PhoR蛋白的反向磷酸化可能发生在与同一蛋白自激酶反应相同的组氨酸残基(His360)上。在ADP存在的情况下,磷酰基进一步转移到ADP上形成ATP。虽然自激酶反应、从PhoRP到PhoP的正向磷转移反应以及在PhoR存在下PhoPP释放无机磷酸盐都需要Mg(2+),但从PhoPP到PhoR的反向磷转移则不需要。这些结果表明PhoP和PhoR上磷酰基的能量水平非常相似。PhoRP和PhoP之间的可逆自激酶反应和/或可逆磷转移反应可能在PhoPP衰变中起作用,从而影响细胞中PhoPP的浓度。

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