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Identification of Direct Transcriptional Target Genes of ExoS/ChvI Two-Component Signaling in Sinorhizobium meliloti

机译:苜蓿根瘤菌ExoS / ChvI两组分信号转导的直接转录靶基因的鉴定

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摘要

The Sinorhizobium meliloti ExoS/ChvI two-component signaling pathway is required for the development of a nitrogen-fixing symbiosis between S. meliloti and its plant hosts. ExoS/ChvI also has important roles in regulating succinoglycan production, biofilm formation, motility, nutrient utilization, and the viability of free-living bacteria. Previous microarray experiments with an exoS96::Tn5 mutant indicated that ExoS/ChvI influences the expression of a few hundred genes, complicating the investigation of which downstream genes respond directly or indirectly to ExoS/ChvI regulation. To focus our study of ExoS/ChvI transcriptional target genes, we performed transcriptional profiling with chvI gain-of-function and reduced-function strains. The chvI gain-of-function strain that we used contains a dominant gain-of-function chvI allele in addition to wild-type chvI. We identified genes that, relative to their expression level in the wild type, are both upregulated in the chvI gain-of-function strain and downregulated in the reduced-function strain or vice versa. Guided by this focused set of genes, we performed gel mobility shift assays and demonstrated that ChvI directly binds the intergenic regions upstream of ropB1, , and . Furthermore, DNase I footprint analysis of the region upstream of identified a specific DNA sequence bound by ChvI and allowed the discovery of a possible motif for ChvI binding. Our results provide insight into the mechanism of how ExoS/ChvI regulates its downstream targets and lay a foundation for studying this conserved pathway with critical roles in free-living and symbiotic bacteria.
机译:苜蓿中华根瘤菌ExoS / ChvI两组分信号传导途径是苜蓿链球菌与其植物宿主之间固氮共生发展的必需条件。 ExoS / ChvI在调节琥珀聚糖的产生,生物膜形成,运动性,养分利用和自由生存细菌的活力方面也起着重要作用。以前使用exoS96 :: Tn5突变体进行的微阵列实验表明,ExoS / ChvI影响数百个基因的表达,这使得对哪些下游基因直接或间接响应ExoS / ChvI调节的研究变得复杂。为了专注于我们对ExoS / ChvI转录靶基因的研究,我们使用chvI功能获得和功能降低的菌株进行了转录谱分析。我们使用的chvI功能获得性菌株除野生型chvI外还包含主要的功能获得性chvI等位基因。我们鉴定了相对于其在野生型中的表达水平在chvI功能获得性菌株中上调而在功能降低的菌株中下调的基因,反之亦然。在这一集中的基因指导下,我们进行了凝胶迁移率迁移分析,并证明ChvI直接结合ropB1,和上游的基因间区域。此外,对上游区域的DNase I足迹分析确定了与ChvI结合的特定DNA序列,并发现了与ChvI结合的可能基序。我们的结果提供了关于ExoS / ChvI如何调节其下游目标的机制的见解,并为研究这种在自由生存和共生细菌中起关键作用的保守途径奠定了基础。

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