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双组分遗传开关的顺序作用调控枯草芽孢杆菌中的PHO调节子。

Sequential action of two-component genetic switches regulates the PHO regulon in Bacillus subtilis.

作者信息

Hulett F M, Lee J, Shi L, Sun G, Chesnut R, Sharkova E, Duggan M F, Kapp N

机构信息

Department of Biological Sciences, University of Illinois at Chicago 60607-7020.

出版信息

J Bacteriol. 1994 Mar;176(5):1348-58. doi: 10.1128/jb.176.5.1348-1358.1994.

Abstract

Bacillus subtilis has an alkaline phosphatase (APase) gene family composed of at least four genes. All members of this gene family are expressed postexponentially, either in response to phosphate starvation or sporulation induction or, in some cases, in response to both. The phoA gene (formerly called phoAIV) and the phoB gene (formerly called phoAIII) products have both been isolated from phosphate-starved cells, and a mutation in either gene decreased the total APase expressed under phosphate starvation conditions. Data presented here show that a phoA phoB double mutant reduced APase production during phosphate starvation by 98%, indicating that these two genes are responsible for most of the APase activity during phosphate-limited growth. The promoter for phoA was cloned and used, with the phoB promoter, to examine phosphate regulation in B. subtilis. phoA-lacZ reporter gene assays showed that the expression of the phoA gene commences as the culture enters stationary phase as a result of limiting phosphate concentrations in the growth medium, thereby mimicking the pattern of total APase expression. Induction persists for approximately 2 h and is then turned off. phoA is transcribed from a single promoter which initiates transcription 19 bp before the translation initiation codon. PhoP and PhoR are members of the two-component signal transduction system believed to regulate gene expression in response to limiting phosphate. The expression of phoA or phoB in response to phosphate starvation was equally dependent on PhoP and PhoR for induction. lacZ-promoter fusions showed that both phoA and phoB were hyperinduced, or failed to turn off induction after 2 h, in a spo0A strain of B. subtilis. Mutations in genes which are required for phosphorylation of Spo0A, spo0B and spo0F, also resulted in phoA and phoB hyperinduction, suggesting that phosphorylation of Spo0A is required for the repression of both APases in wild-type strains. The hyperinduction of either APase gene in a spo0A strain was dependent on PhoP and PhoR. Analysis of a phoP-lacZ promoter fusion showed that the phoPR operon is hyperinduced in a spo0A mutant strain, suggesting that Spo0A approximately P represses APases by repressing phoPR transcription. We propose a model for PHO regulation in B. subtilis whereby the phoPR operon is transcribed in response to limiting phosphate concentration, resulting in activation of the PHO regulon transcription, including transcription of phoA and phoB. When the phosphate response fails to overcome the nutrient deficiency, signals for phosphorylation of Spo0A result in production of Spo0A approximately P, which represses transcription of phoPR, thereby repressing synthesis of the PHO regulon.

摘要

枯草芽孢杆菌拥有一个由至少四个基因组成的碱性磷酸酶(APase)基因家族。该基因家族的所有成员在指数期后表达,要么是对磷酸盐饥饿或芽孢形成诱导的响应,在某些情况下,是对两者的响应。phoA基因(以前称为phoAIV)和phoB基因(以前称为phoAIII)的产物都已从磷酸盐饥饿的细胞中分离出来,并且任一基因中的突变都会降低在磷酸盐饥饿条件下表达的总APase。此处呈现的数据表明,phoA phoB双突变体在磷酸盐饥饿期间使APase产量降低了98%,表明这两个基因负责磷酸盐限制生长期间的大部分APase活性。phoA的启动子被克隆并与phoB启动子一起用于研究枯草芽孢杆菌中的磷酸盐调节。phoA - lacZ报告基因检测表明,由于生长培养基中磷酸盐浓度受限,phoA基因的表达在培养进入稳定期时开始,从而模仿了总APase表达的模式。诱导持续约2小时,然后关闭。phoA从单个启动子转录,该启动子在翻译起始密码子前19 bp处启动转录。PhoP和PhoR是双组分信号转导系统的成员,据信它们响应有限的磷酸盐来调节基因表达。phoA或phoB对磷酸盐饥饿的响应在诱导方面同样依赖于PhoP和PhoR。lacZ - 启动子融合表明,在枯草芽孢杆菌的spo0A菌株中,phoA和phoB都被超诱导,或者在2小时后未能关闭诱导。Spo0A磷酸化所需基因spo0B和spo0F中的突变也导致phoA和phoB超诱导,这表明野生型菌株中Spo0A的磷酸化是两种APase抑制所必需的。spo0A菌株中任一APase基因的超诱导依赖于PhoP和PhoR。对phoP - lacZ启动子融合的分析表明,phoPR操纵子在spo0A突变菌株中被超诱导,这表明Spo0AP通过抑制phoPR转录来抑制APase。我们提出了一个枯草芽孢杆菌中PHO调节的模型,即phoPR操纵子响应有限的磷酸盐浓度进行转录,导致PHO调节子转录的激活,包括phoA和phoB的转录。当磷酸盐响应未能克服营养缺乏时,Spo0A磷酸化的信号导致Spo0AP的产生,它抑制phoPR的转录,从而抑制PHO调节子的合成。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3e6f/205199/b93c696bcdb1/jbacter00023-0159-a.jpg

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