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细胞壁抑制性抗生素激活铜绿假单胞菌中的藻酸盐生物合成操纵子:σ因子(AlgT)以及AlgW和Prc蛋白酶的作用。

Cell wall-inhibitory antibiotics activate the alginate biosynthesis operon in Pseudomonas aeruginosa: Roles of sigma (AlgT) and the AlgW and Prc proteases.

作者信息

Wood Lynn F, Leech Andrew J, Ohman Dennis E

机构信息

Department of Microbiology and Immunology, Medical College of Virginia Campus of Virginia Commonwealth University, Richmond, VA 23298-0678, USA.

出版信息

Mol Microbiol. 2006 Oct;62(2):412-26. doi: 10.1111/j.1365-2958.2006.05390.x.

DOI:10.1111/j.1365-2958.2006.05390.x
PMID:17020580
Abstract

A bioassay was developed to identify stimuli that promote the transcriptional induction of the algD operon for alginate biosynthesis in Pseudomonas aeruginosa. Strain PAO1 carried the algD promoter fused to a chloramphenicol acetyl-transferase cartridge (PalgD-cat), and > 50 compounds were tested for promoting chloramphenicol resistance. Most compounds showing PalgD-cat induction were cell wall-active antibiotics that blocked peptidoglycan synthesis. PalgD-cat induction was blocked by mutations in the genes for sigma22 (algT/algU) or regulators AlgB and AlgR. Anti-sigma factor MucA was the primary regulator of sigma22 activity. A transcriptome analysis using microarrays verified that the algD operon undergoes high induction by D-cycloserine. A similar sigma(E)-RseAB complex in Escherichia coli responds to envelope stress, which requires DegS protease in a regulated intramembrane proteolysis (RIP) cascade to derepress the sigma. Mutant phenotypic studies in P. aeruginosa showed that AlgW (PA4446) is likely to be the DegS functional homologue. A mutation in algW resulted in a complete lack of PalgD-cat induction by D-cycloserine. Overexpression of algW in PAO1 resulted in a mucoid phenotype and alginate production, even in the absence of cell wall stress, suggesting that AlgW protease plays a role in sigma22 activation. In addition, a mutation in gene PA3257 (prc), encoding a Prc-like protease, resulted in poor induction of PalgD-cat by D-cycloserine, suggesting that it also plays a role in the response to cell wall stress.

摘要

已开发出一种生物测定法,用于鉴定促进铜绿假单胞菌中藻酸盐生物合成的algD操纵子转录诱导的刺激因素。菌株PAO1携带与氯霉素乙酰转移酶盒融合的algD启动子(PalgD-cat),并测试了50多种化合物促进氯霉素抗性的能力。大多数显示PalgD-cat诱导的化合物是阻断肽聚糖合成的细胞壁活性抗生素。sigma22(algT/algU)或调节因子AlgB和AlgR基因中的突变可阻断PalgD-cat诱导。抗sigma因子MucA是sigma22活性的主要调节因子。使用微阵列进行的转录组分析证实,algD操纵子受到D-环丝氨酸的高度诱导。大肠杆菌中类似的sigma(E)-RseAB复合物对包膜应激作出反应,这需要DegS蛋白酶参与调节性膜内蛋白水解(RIP)级联反应来解除对sigma的抑制。铜绿假单胞菌的突变表型研究表明,AlgW(PA4446)可能是DegS的功能同源物。algW中的突变导致D-环丝氨酸完全缺乏PalgD-cat诱导。在PAO1中过表达algW会导致黏液样表型和藻酸盐产生,即使在没有细胞壁应激的情况下也是如此,这表明AlgW蛋白酶在sigma22激活中起作用。此外,编码Prc样蛋白酶的基因PA3257(prc)中的突变导致D-环丝氨酸对PalgD-cat的诱导不佳,表明它也在对细胞壁应激的反应中起作用。

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