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σ因子 FliA、ppGpp 和 DksA 协调调控假单胞菌 aer2 基因的转录。

The sigma-factor FliA, ppGpp and DksA coordinate transcriptional control of the aer2 gene of Pseudomonas putida.

机构信息

Department of Molecular Biology, Umeå University, SE-901 87 Umeå, Sweden.

出版信息

Environ Microbiol. 2010 Jun;12(6):1439-51. doi: 10.1111/j.1462-2920.2009.02139.x. Epub 2010 Jan 18.

DOI:10.1111/j.1462-2920.2009.02139.x
PMID:20089044
Abstract

Here the sigma-factor requirement for transcription of three similar, but differentially regulated, aer genes of Pseudomonas putida KT2440 is investigated. Previous work has shown that the three Aer proteins, like chemoreceptors, colocalize to a single pole in a CheA-dependent manner. Lack of Aer2 - the most abundant of these three proteins - mediates defects in metabolism-dependent taxis and aerotaxis, while lack of Aer1 or Aer3 has no apparent phenotype. We show, using wild-type and mutant P. putida derivatives combined with P. putida reconstituted FliA- (sigma(28)) and sigma(70)-dependent in vitro transcription assays, that transcription of aer2 is coupled to motility through the flagella sigma-factor FliA, while sigma(70) is responsible for transcription of aer1 and aer3. By comparing activities of the wild-type and mutant forms of the aer2 promoter, we present evidence (i) that transcription from FliA-dependent Paer2 is enhanced by changes towards the Escherichia coli consensus for FliA promoters rather than towards that of P. putida, (ii) that the nature of the AT-rich upstream region is important for both output and sigma(70) discrimination of this promoter, and (iii) that Paer2 output is directly stimulated by the bacterial alarmone ppGpp and its cofactor DksA.

摘要

本文研究了假单胞菌 KT2440 中三个相似但受差异调控的 aer 基因的转录所需的 sigma 因子。先前的工作表明,这三种 Aer 蛋白与化学感受器一样,以 CheA 依赖的方式共定位到一个单一的极点。缺乏 Aer2(这三种蛋白质中最丰富的一种)会导致代谢依赖性趋化性和趋气性缺陷,而缺乏 Aer1 或 Aer3 则没有明显的表型。我们使用野生型和突变型假单胞菌衍生物,并结合假单胞菌重建的 FliA-(sigma(28))和 sigma(70)依赖性体外转录测定,表明 aer2 的转录通过鞭毛 sigma 因子 FliA 与运动相关,而 sigma(70)负责 aer1 和 aer3 的转录。通过比较 aer2 启动子的野生型和突变型的活性,我们提供了以下证据:(i) 依赖于 FliA 的 Paer2 转录的增强是通过向 FliA 启动子的大肠杆菌共识而不是向假单胞菌的共识发生变化,(ii) 富含 AT 的上游区域的性质对于该启动子的输出和 sigma(70)识别都很重要,以及 (iii) Paer2 的输出直接受到细菌警报素 ppGpp 和其共因子 DksA 的刺激。

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