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铜绿假单胞菌群体感应转录因子LasR的全局定位分析

Global position analysis of the Pseudomonas aeruginosa quorum-sensing transcription factor LasR.

作者信息

Gilbert Kerrigan B, Kim Tae Hoon, Gupta Rashmi, Greenberg E Peter, Schuster Martin

机构信息

Department of Microbiology, Oregon State University, Corvallis, OR 97331, USA.

出版信息

Mol Microbiol. 2009 Sep;73(6):1072-85. doi: 10.1111/j.1365-2958.2009.06832.x. Epub 2009 Aug 11.

Abstract

In Pseudomonas aeruginosa quorum sensing (QS), the transcriptional regulator LasR controls the expression of more than 300 genes. Several of these genes are activated indirectly via a second, subordinate QS regulator, RhlR. Conserved sequence elements upstream of individual other genes have been shown to bind LasR in vitro. To comprehensively identify all regions that are bound by LasR in vivo, we employed chromatin immunoprecipitation in conjunction with microarray analysis. We identified 35 putative promoter regions that direct the expression of up to 74 genes. In vitro DNA binding studies allowed us to distinguish between cooperative and non-cooperative LasR binding sites, and allowed us to build consensus sequences according to the mode of binding. Five promoter regions were not previously recognized as QS-controlled. Two of the associated transcript units encode proteins involved in the cold-shock response and in Psl exopolysaccharide synthesis respectively. The LasR regulon includes seven genes encoding transcriptional regulators, while secreted factors and secretion machinery are the most over-represented functional categories overall. This supports the notion that the core function of LasR is to co-ordinate the production of extracellular factors, although many of its effects on global gene expression are likely mediated indirectly by regulatory genes under its control.

摘要

在铜绿假单胞菌群体感应(QS)中,转录调节因子LasR控制着300多个基因的表达。其中一些基因通过第二个从属的QS调节因子RhlR间接激活。已表明单个其他基因上游的保守序列元件在体外可与LasR结合。为了全面鉴定体内与LasR结合的所有区域,我们采用了染色质免疫沉淀结合微阵列分析的方法。我们鉴定出35个推定的启动子区域,这些区域指导多达74个基因的表达。体外DNA结合研究使我们能够区分协同和非协同的LasR结合位点,并根据结合模式构建共有序列。五个启动子区域以前未被认为受QS控制。其中两个相关的转录单元分别编码参与冷休克反应和Psl胞外多糖合成的蛋白质。LasR调控子包括七个编码转录调节因子的基因,而分泌因子和分泌机制是总体上代表性最强的功能类别。这支持了LasR的核心功能是协调细胞外因子产生的观点,尽管它对全局基因表达的许多影响可能是由其控制下的调节基因间接介导的。

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