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鞘氨醇单胞菌 Fr1 PhyR-NepR-σEcfG 级联在一般应激反应中的作用及 PhyR 负调控因子的鉴定。

Role of Sphingomonas sp. strain Fr1 PhyR-NepR-σEcfG cascade in general stress response and identification of a negative regulator of PhyR.

机构信息

Institute of Microbiology, ETH Zurich, Wolfgang-Pauli-Strasse 10, 8093 Zurich, Switzerland.

出版信息

J Bacteriol. 2011 Dec;193(23):6629-38. doi: 10.1128/JB.06006-11. Epub 2011 Sep 23.

DOI:10.1128/JB.06006-11
PMID:21949070
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3232908/
Abstract

The general stress response in Alphaproteobacteria was recently described to depend on the alternative sigma factor σ(EcfG), whose activity is regulated by its anti-sigma factor NepR. The response regulator PhyR, in turn, regulates NepR activity in a partner-switching mechanism according to which phosphorylation of PhyR triggers sequestration of NepR by the sigma factor-like effector domain of PhyR. Although genes encoding predicted histidine kinases can often be found associated with phyR, little is known about their role in modulation of PhyR phosphorylation status. We demonstrate here that the PhyR-NepR-σ(EcfG) cascade is important for multiple stress resistance and competitiveness in the phyllosphere in a naturally abundant plant epiphyte, Sphingomonas sp. strain Fr1, and provide evidence that the partner switching mechanism is conserved. We furthermore identify a gene, designated phyP, encoding a predicted histidine kinase at the phyR locus as essential. Genetic epistasis experiments suggest that PhyP acts upstream of PhyR, keeping PhyR in an unphosphorylated, inactive state in nonstress conditions, strictly depending on the predicted phosphorylatable site of PhyP, His-341. In vitro experiments show that Escherichia coli inner membrane fractions containing PhyP disrupt the PhyR-P/NepR complex. Together with the fact that PhyP lacks an obvious ATPase domain, these results are in agreement with PhyP functioning as a phosphatase of PhyR, rather than a kinase.

摘要

α变形菌中的一般应激反应最近被描述为依赖于替代 sigma 因子 σ(EcfG),其活性受其反 sigma 因子 NepR 调节。响应调节剂 PhyR 又根据伴侣切换机制调节 NepR 的活性,根据该机制,PhyR 的磷酸化触发 NepR 被 PhyR 的 sigma 因子样效应结构域隔离。尽管经常可以找到与 phyR 相关的预测组氨酸激酶基因,但它们在调节 PhyR 磷酸化状态中的作用知之甚少。我们在这里证明,PhyR-NepR-σ(EcfG)级联对于自然丰富的植物附生菌 Sphingomonas sp. strain Fr1 的叶际中的多种应激抗性和竞争力很重要,并提供证据表明伴侣切换机制是保守的。我们还鉴定了一个基因 phyP,它在 phyR 基因座上编码一个预测的组氨酸激酶,是必需的。遗传上位性实验表明,PhyP 在上游作用于 PhyR,使 PhyR 在非应激条件下保持未磷酸化、无活性状态,严格依赖于 PhyP 的预测可磷酸化位点 His-341。体外实验表明,含有 PhyP 的大肠杆菌内膜部分破坏了 PhyR-P/NepR 复合物。由于 PhyP 缺乏明显的 ATP 酶结构域,这些结果与 PhyP 作为 PhyR 的磷酸酶而不是激酶的功能一致。

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