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The cin and rai Quorum-Sensing Regulatory Systems in Rhizobium leguminosarum Are Coordinated by ExpR and CinS, a Small Regulatory Protein Coexpressed with CinI▿

机译:豆科根瘤菌中的cin和rai群体感应调控系统由ExpR和CinS协调,这是一种与CinI▿共表达的小调控蛋白。

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摘要

To understand how the Rhizobium leguminosarum raiI-raiR quorum-sensing system is regulated, we identified mutants with decreased levels of RaiI-made N-acyl homoserine lactones (AHLs). A LuxR-type regulator, ExpR, is required for raiR expression, and RaiR is required to induce raiI. Since raiR (and raiI) expression is also reduced in cinI and cinR quorum-sensing mutants, we thought CinI-made AHLs may activate ExpR to induce raiR. However, added CinI-made AHLs did not induce raiR expression in a cinI mutant. The reduced raiR expression in cinI and cinR mutants was due to lack of expression of cinS immediately downstream of cinI. cinS encodes a 67-residue protein, translationally coupled to CinI, and cinS acts downstream of expR for raiR induction. Cloned cinS in R. leguminosarum caused an unusual collapse of colony structure, and this was delayed by mutation of expR. The phenotype looked like a loss of exopolysaccharide (EPS) integrity; mutations in cinI, cinR, cinS, and expR all reduced expression of plyB, encoding an EPS glycanase, and mutation of plyB abolished the effect of cloned cinS on colony morphology. We conclude that CinS and ExpR act to increase PlyB levels, thereby influencing the bacterial surface. CinS is conserved in other rhizobia, including Rhizobium etli; the previously observed effect of cinI and cinR mutations decreasing swarming in that strain is primarily due to a lack of CinS rather than a lack of CinI-made AHL. We conclude that CinS mediates quorum-sensing regulation because it is coregulated with an AHL synthase and demonstrate that its regulatory effects can occur in the absence of AHLs.
机译:为了了解豆科根瘤菌(Rhizobium leguminosarum)raiI-raiR群体感应系统是如何调控的,我们鉴定了RaiI制N-酰基高丝氨酸内酯(AHLs)水平降低的突变体。 raiR表达需要LuxR型调节子ExpR,而诱导raiI则需要RaiR。由于在cinI和cinR群体感应突变体中raiR(和raiI)的表达也降低了,因此我们认为由CinI制成的AHL可能会激活ExpR来诱导raiR。但是,添加的CinI制成的AHL不会在cinI突变体中诱导raiR表达。 cinI和cinR突变体中的raiR表达降低是由于紧靠cinI下游的cinS表达不足。 cinS编码67个残基的蛋白质,翻译后与CinI偶联,而cinS在expR的下游起作用,用于raiR诱导。豆科植物念珠菌中克隆的cinS导致菌落结构异常塌陷,并且由于expR突变而被延迟。该表型看起来像是胞外多糖(EPS)完整性的丧失。 cinI,cinR,cinS和expR中的突变均降低了编码EPS聚糖酶的plyB的表达,并且plyB的突变消除了克隆的cinS对菌落形态的影响。我们得出结论,CinS和ExpR起作用以增加PlyB水平,从而影响细菌表面。 CinS在其他根瘤菌中是保守的,包括等根瘤菌。先前观察到的cinI和cinR突变降低了该菌株群的作用主要是由于缺乏CinS而非缺乏由CinI制成的AHL。我们得出的结论是,CinS介导群体感应调控,因为它与AHL合酶共调节,并证明了其调控作用可以在没有AHL的情况下发生。

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