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枯草芽孢杆菌中σ(B)转录因子的能量应激激活需要α/β水解酶的催化功能。

Catalytic function of an alpha/beta hydrolase is required for energy stress activation of the sigma(B) transcription factor in Bacillus subtilis.

作者信息

Brody M S, Vijay K, Price C W

机构信息

Department of Food Science and Technology, University of California, Davis, California 95616, USA.

出版信息

J Bacteriol. 2001 Nov;183(21):6422-8. doi: 10.1128/JB.183.21.6422-6428.2001.

Abstract

The general stress response of Bacillus subtilis is controlled by the sigma(B) transcription factor, which is activated in response to diverse energy and environmental stresses. These two classes of stress are transmitted by separate signaling pathways which converge on the direct regulators of sigma(B), the RsbV anti-anti-sigma factor and the RsbW anti-sigma factor. The energy signaling branch involves the RsbP phosphatase, which dephosphorylates RsbV in order to trigger the general stress response. The rsbP structural gene lies downstream from rsbQ in a two-gene operon. Here we identify the RsbQ protein as a required positive regulator inferred to act in concert with the RsbP phosphatase. RsbQ bound RsbP in the yeast two-hybrid system, and a large in-frame deletion in rsbQ had the same phenotype as a null allele of rsbP-an inability to activate sigma(B) in response to energy stress. Genetic complementation studies indicated that this phenotype was not due to a polar effect of the rsbQ alteration on rsbP. The predicted rsbQ product is a hydrolase or acyltransferase of the alpha/beta fold superfamily, members of which catalyze a wide variety of reactions. Notably, substitutions in the presumed catalytic triad of RsbQ also abolished the energy stress response but had no detectable effect on RsbQ structure, synthesis, or stability. We conclude that the catalytic activity of RsbQ is an essential constituent of the energy stress signaling pathway.

摘要

枯草芽孢杆菌的一般应激反应由σ(B)转录因子控制,该因子在应对各种能量和环境应激时被激活。这两类应激通过 separate 信号通路传递,这些通路汇聚于σ(B)的直接调节因子,即RsbV抗抗σ因子和RsbW抗σ因子。能量信号分支涉及RsbP磷酸酶,它使RsbV去磷酸化以触发一般应激反应。rsbP结构基因位于一个双基因操纵子中rsbQ的下游。在这里,我们将RsbQ蛋白鉴定为一种必需的正调节因子,推测它与RsbP磷酸酶协同作用。在酵母双杂交系统中,RsbQ与RsbP结合,并且rsbQ中的一个大的框内缺失与rsbP的无效等位基因具有相同的表型——无法在能量应激下激活σ(B)。遗传互补研究表明,这种表型不是由于rsbQ改变对rsbP的极性效应。预测的rsbQ产物是α/β折叠超家族的水解酶或酰基转移酶,该家族成员催化多种反应。值得注意的是,RsbQ假定催化三联体中的取代也消除了能量应激反应,但对RsbQ的结构、合成或稳定性没有可检测到的影响。我们得出结论,RsbQ的催化活性是能量应激信号通路的一个重要组成部分。

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