首页> 美国卫生研究院文献>Applied and Environmental Microbiology >Identification of the mcpA and mcpM Genes Encoding Methyl-Accepting Proteins Involved in Amino Acid and l-Malate Chemotaxis and Involvement of McpM-Mediated Chemotaxis in Plant Infection by Ralstonia pseudosolanacearum (Formerly Ralstonia solanacearum Phylotypes I and III)
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Identification of the mcpA and mcpM Genes Encoding Methyl-Accepting Proteins Involved in Amino Acid and l-Malate Chemotaxis and Involvement of McpM-Mediated Chemotaxis in Plant Infection by Ralstonia pseudosolanacearum (Formerly Ralstonia solanacearum Phylotypes I and III)

机译:mcpA和mcpM基因的鉴定编码涉及氨基酸和l-苹果酸趋化性的甲基受体蛋白以及McpM介导的趋化性参与拟南芥(Ralstonia pseudosolanacearum)植物感染(以前为Ralstonia solanacearum型I和III)。

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摘要

Sequence analysis has revealed the presence of 22 putative methyl-accepting chemotaxis protein (mcp) genes in the Ralstonia pseudosolanacearum GMI1000 genome. PCR analysis and DNA sequencing showed that the highly motile R. pseudosolanacearum strain Ps29 possesses homologs of all 22 R. pseudosolanacearum GMI1000 mcp genes. We constructed a complete collection of single mcp gene deletion mutants of R. pseudosolanacearum Ps29 by unmarked gene deletion. Screening of the mutant collection revealed that R. pseudosolanacearum Ps29 mutants of RSp0507 and RSc0606 homologs were defective in chemotaxis to l-malate and amino acids, respectively. RSp0507 and RSc0606 homologs were designated mcpM and mcpA. While wild-type R. pseudosolanacearum strain Ps29 displayed attraction to 16 amino acids, the mcpA mutant showed no response to 12 of these amino acids and decreased responses to 4 amino acids. We constructed mcpA and mcpM deletion mutants of highly virulent R. pseudosolanacearum strain MAFF106611 to investigate the contribution of chemotaxis to l-malate and amino acids to tomato plant infection. Neither single mutant exhibited altered virulence for tomato plants when tested by root dip inoculation assays. In contrast, the mcpM mutant (but not the mcpA mutant) was significantly less infectious than the wild type when tested by a sand soak inoculation assay, which requires bacteria to locate and invade host roots from sand. Thus, McpM-mediated chemotaxis, possibly reflecting chemotaxis to l-malate, facilitates R. pseudosolanacearum motility to tomato roots in sand.
机译:序列分析揭示了假单胞菌GMI1000基因组中存在22个假定的甲基接受趋化蛋白(mcp)基因。 PCR分析和DNA测序表明,高能动假单胞菌菌株Ps29具有所有22个假单胞菌GMI1000 mcp基因的同源物。我们通过未标记的基因缺失构建了完整的假单胞菌Ps29 mcp基因缺失突变体集合。突变体集合的筛选显示,RSp0507和RSc0606同源物的假单胞菌Ps29突变体分别对L-苹果酸和氨基酸趋化性有缺陷。 RSp0507和RSc0606同源物称为mcpM和mcpA。野生型假单胞菌菌株Ps29对16个氨基酸表现出吸引力,而mcpA突变体对其中12个氨基酸无反应,而对4个氨基酸反应却减少。我们构建了高毒性假单胞菌菌株MAFF106611的mcpA和mcpM缺失突变体,以研究趋化性对l-苹果酸和氨基酸对番茄植物感染的贡献。当通过根浸接种试验进行测试时,单个突变体均未表现出对番茄植物的改变的毒力。相比之下,用沙浸接种法进行测试时,mcpM突变体(而不是 mcpA 突变体)的感染力明显低于野生型,这需要细菌从沙子中定位并侵入宿主根。因此,McpM介导的趋化性,可能反映了对L-苹果酸的趋化性,促进了R。 pseudosolanacearum 对沙子中番茄根的运动。

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