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肠炎沙门氏菌的Mg2+传感器PhoQ对Mg2+的感应

Mg2+ sensing by the Mg2+ sensor PhoQ of Salmonella enterica.

作者信息

Chamnongpol Sangpen, Cromie Michael, Groisman Eduardo A

机构信息

Department of Molecular Microbiology, Howard Hughes Medical Institute, Washington University School of Medicine, 660 S. Euclid Avenue, Campus Box 8230, St. Louis, MO 63110-1093, USA.

出版信息

J Mol Biol. 2003 Jan 24;325(4):795-807. doi: 10.1016/s0022-2836(02)01268-8.

Abstract

The PhoP/PhoQ two-component regulatory system governs the adaptation to low Mg(2+) environments and virulence in several Gram-negative species. During growth in low Mg(2+), the sensor PhoQ modifies the activity of the response regulator PhoP promoting gene transcription, whereas growth in high Mg(2+) represses transcription of PhoP-activated genes. The PhoQ protein harbors a periplasmic domain of 146 amino acid residues that binds Mg(2+) in vitro and is required for Mg(2+)-mediated repression in vivo. Here, we identify periplasmic mutants of the Salmonella PhoQ protein that allow transcription of PhoP-activated genes even under high Mg(2+) concentrations. When expressed in a strain harboring a PhoP variant that is phosphorylated from acetyl phosphate, some of the mutants failed to repress PhoP-promoted transcription in high Mg(2+), whereas others displayed a wild-type ability to do so. Mutant PhoQ proteins that allowed expression of PhoP-activated genes in high Mg(2+) displayed a pattern of iron-mediated cleavage in vitro that was different from that displayed by wild-type PhoQ, indicative of altered Mg(2+) binding. A PhoQ protein with the conserved histidine residue (H277) substituted by alanine could not promote transcription of PhoP-activated genes in low Mg(2+) but could turn off expression in response to high Mg(2+). Our studies demonstrate that residues G93, W97, H120 and T156 are required for a wild-type response to Mg(2+), and suggest that Mg(2+) binding to the periplasmic domain regulates several activities in the PhoQ protein.

摘要

PhoP/PhoQ双组分调节系统控制着几种革兰氏阴性菌对低镁(Mg²⁺)环境的适应及毒力。在低镁环境中生长时,传感器PhoQ会改变反应调节因子PhoP的活性,促进基因转录;而在高镁环境中生长则会抑制PhoP激活基因的转录。PhoQ蛋白含有一个由146个氨基酸残基组成的周质结构域,该结构域在体外可结合Mg²⁺,且在体内Mg²⁺介导的抑制过程中是必需的。在此,我们鉴定出沙门氏菌PhoQ蛋白的周质突变体,这些突变体即使在高镁浓度下也能使PhoP激活基因转录。当在携带从乙酰磷酸磷酸化的PhoP变体的菌株中表达时,一些突变体在高镁环境中无法抑制PhoP促进的转录,而其他一些则表现出野生型的抑制能力。在高镁环境中允许PhoP激活基因表达的突变PhoQ蛋白在体外显示出与野生型PhoQ不同的铁介导切割模式,这表明Mg²⁺结合发生了改变。一个保守组氨酸残基(H277)被丙氨酸取代的PhoQ蛋白在低镁环境中不能促进PhoP激活基因的转录,但能响应高镁环境关闭表达。我们的研究表明,残基G93、W97、H120和T156是对Mg²⁺野生型反应所必需的,并表明Mg²⁺与周质结构域的结合调节了PhoQ蛋白中的多种活性。

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