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A role for the Rcs phosphorelay in regulating expression of plant cell wall degrading enzymes in Pectobacterium carotovorum subsp. carotovorum

机译:RCS磷酸磷在植物细胞段患者植物细胞壁降解酶的调节中的作用。 Carotovorum.

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The Rcs phosphorelay is a signal transduction system that influences the virulence phenotype of several pathogenic bacteria. In the plant pathogen Pectobacterium carotovorum subsp. carotovorum (Pcc) the response regulator of the Rcs phosphorelay, RcsB, represses expression of plant cell wall degrading enzymes (PCWDE) and motility. The focus of this study was to identify genes directly regulated by the binding of RcsB that also regulate expression of PCWDE genes in Pcc. RcsB-binding sites within the regulatory regions of the flhDC operon and the rprA and rsmB genes were identified using DNase I protection assays, while in vivo studies using flhDC?:?:?gusA, rsmB?:?:?gusA and rprA?:?:?gusA gene fusions revealed gene regulation. These experiments demonstrated that the operon flhDC, a flagellar master regulator, was repressed by RcsB, and transcription of rprA was activated by RcsB. Regulation of the rsmB promoter by RcsB is more complicated. Our results show that RcsB represses rsmB expression mainly through modulating flhDC transcription. Neverthless, direct binding of RcsB on the rsmB promoter region is possible in certain conditions. Using an rprA-negative mutant, it was further demonstrated that RprA RNA is not essential for regulating expression of PCWDE under the conditions tested, whereas overexpression of rprA increased protease expression in wild-type cells. Stationary-phase sigma factor, RpoS, is the only known target gene for RprA RNA in Escherichia coli; however, in Pcc the effect of RprA RNA was found to be rpoS-independent. Overall, our results show that the Rcs phosphorelay negatively affects expression of PCWDE by inhibiting expression of flhDC and rsmB.
机译:RCS磷酸是一种信号转导系统,其影响几种致病细菌的毒力表型。在植物病原体胶杆Carotovorum subsp中。 Carotovorum(PCC)RCS磷的响应调节器,RCSB,抑制植物细胞壁降解酶(PCWDE)和运动的表达。本研究的重点是鉴定通过RCSB的结合直接调节的基因,该基因还调节PCC中PCWDE基因的表达。使用FLHDC的体内研究中鉴定了FLHDC操纵子和RPRA和RSMB基因的调节区域内的RCSB结合位点?:?:?GUSA,RSMB?:?:?GUSA和RPRA ?: ?:?Gusa基因融合揭示了基因调控。这些实验证明,通过RCSB抑制了操纵子FLHDC,鞭毛母稳压器,并通过RCSB激活RPRA的转录。 RCSB对RSMB启动子的调节更复杂。我们的结果表明,RCSB主要通过调制FLHDC转录来压制RSMB表达。在某些情况下,RCSB对RSMB启动子区域的直接结合是可能的。使用RPRA阴性突变体,进一步证明RPRA RNA对于在测试的条件下调节PCWDE的表达至关重要,而RPRA的过度表达增加野生型细胞中的蛋白酶表达。静止相思σ因子,RPO是大肠杆菌中唯一已知的RPRA RNA靶基因;然而,在PCC中,发现RPRA RNA的效果是RPOS的。总体而言,我们的结果表明,RCS磷脂通过抑制FLHDC和RSMB的表达而对PCWDE的表达产生负面影响。

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