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铜绿假单胞菌AlgR以生物膜特异性方式抑制Rhl群体感应系统。

Pseudomonas aeruginosa AlgR represses the Rhl quorum-sensing system in a biofilm-specific manner.

作者信息

Morici Lisa A, Carterson Alexander J, Wagner Victoria E, Frisk Anders, Schurr Jill R, Höner zu Bentrup Kerstin, Hassett Daniel J, Iglewski Barbara H, Sauer Karin, Schurr Michael J

机构信息

Tulane University Health Sciences Center, Department of Microbiology and Immunology, New Orleans, LA 70112, USA.

出版信息

J Bacteriol. 2007 Nov;189(21):7752-64. doi: 10.1128/JB.01797-06. Epub 2007 Aug 31.

Abstract

AlgR controls numerous virulence factors in Pseudomonas aeruginosa, including alginate, hydrogen cyanide production, and type IV pilus-mediated twitching motility. In this study, the role of AlgR in biofilms was examined in continuous-flow and static biofilm assays. Strain PSL317 (DeltaalgR) produced one-third the biofilm biomass of wild-type strain PAO1. Complementation with algR, but not fimTU-pilVWXY1Y2E, restored PSL317 to the wild-type biofilm phenotype. Comparisons of the transcriptional profiles of biofilm-grown PAO1 and PSL317 revealed that a number of quorum-sensing genes were upregulated in the algR deletion strain. Measurement of rhlA::lacZ and rhlI::lacZ promoter fusions confirmed the transcriptional profiling data when PSL317 was grown as a biofilm, but not planktonically. Increased amounts of rhamnolipids and N-butyryl homoserine lactone were detected in the biofilm effluent but not the planktonic supernatants of the algR mutant. Additionally, AlgR specifically bound to the rhlA and rhlI promoters in mobility shift assays. Moreover, PAO1 containing a chromosomal mutated AlgR binding site in its rhlI promoter formed biofilms and produced increased amounts of rhamnolipids similarly to the algR deletion strain. These observations indicate that AlgR specifically represses the Rhl quorum-sensing system during biofilm growth and that such repression is necessary for normal biofilm development. These data also suggest that AlgR may control transcription in a contact-dependent or biofilm-specific manner.

摘要

AlgR调控铜绿假单胞菌中的多种毒力因子,包括藻酸盐、氰化氢的产生以及IV型菌毛介导的颤动运动。在本研究中,通过连续流和静态生物膜试验检测了AlgR在生物膜中的作用。菌株PSL317(ΔalgR)产生的生物膜生物量是野生型菌株PAO1的三分之一。用algR而非fimTU - pilVWXY1Y2E进行互补,可使PSL317恢复到野生型生物膜表型。对生物膜生长的PAO1和PSL317的转录谱进行比较,发现许多群体感应基因在algR缺失菌株中上调。对rhlA::lacZ和rhlI::lacZ启动子融合体的检测证实了PSL317作为生物膜生长时的转录谱数据,但浮游生长时则不然。在algR突变体的生物膜流出物中检测到鼠李糖脂和N - 丁酰高丝氨酸内酯的量增加,而浮游上清液中未检测到。此外,在迁移率变动分析中,AlgR特异性结合rhlA和rhlI启动子。而且,在其rhlI启动子中含有染色体突变AlgR结合位点的PAO1形成生物膜并产生与algR缺失菌株类似的增加量的鼠李糖脂。这些观察结果表明,AlgR在生物膜生长过程中特异性抑制Rhl群体感应系统,并且这种抑制对于正常生物膜发育是必要的。这些数据还表明,AlgR可能以接触依赖或生物膜特异性方式控制转录。

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