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The cabABC Operon Essential for Biofilm and Rugose Colony Development in Vibrio vulnificus

机译:cabABC Operon对创伤弧菌生物膜和毛糖菌落发育至关重要

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摘要

A transcriptome analysis identified Vibrio vulnificus cabABC genes which were preferentially expressed in biofilms. The cabABC genes were transcribed as a single operon. The cabA gene was induced by elevated 3′,5′-cyclic diguanylic acid (c-di-GMP) and encoded a calcium-binding protein CabA. Comparison of the biofilms produced by the cabA mutant and its parent strain JN111 in microtiter plates using crystal-violet staining demonstrated that CabA contributed to biofilm formation in a calcium-dependent manner under elevated c-di-GMP conditions. Genetic and biochemical analyses revealed that CabA was secreted to the cell exterior through functional CabB and CabC, distributed throughout the biofilm matrix, and produced as the biofilm matured. These results, together with the observation that CabA also contributes to the development of rugose colony morphology, indicated that CabA is a matrix-associated protein required for maturation, rather than adhesion involved in the initial attachment, of biofilms. Microscopic comparison of the structure of biofilms produced by JN111 and the cabA mutant demonstrated that CabA is an extracellular matrix component essential for the development of the mature biofilm structures in flow cells and on oyster shells. Exogenously providing purified CabA restored the biofilm- and rugose colony-forming abilities of the cabA mutant when calcium was available. Circular dichroism and size exclusion analyses revealed that calcium binding induces CabA conformational changes which may lead to multimerization. Extracellular complementation experiments revealed that CabA can assemble a functional matrix only when exopolysaccharides coexist. Consequently, the combined results suggested that CabA is a structural protein of the extracellular matrix and multimerizes to a conformation functional in building robust biofilms, which may render V. vulnificus to survive in hostile environments and reach a concentrated infective dose.
机译:转录组分析确定了在生物膜中优先表达的创伤弧菌cabABC基因。 cabABC基因被转录为单个操纵子。 cabA基因由升高的3',5'-环二鸟苷酸(c-di-GMP)诱导并编码钙结合蛋白CabA。使用结晶紫染色在微量滴定板上比较cabA突变体及其亲本菌株JN111产生的生物膜,结果表明CabA在升高的c-di-GMP条件下以钙依赖性方式有助于生物膜形成。遗传和生化分析表明,CabA通过功能性CabB和CabC分泌到细胞外部,分布在整个生物膜基质中,并随着生物膜的成熟而产生。这些结果,再加上CabA也有助于皱纹菌落形态发展的观察,表明CabA是生物膜成熟所需的基质相关蛋白,而不是最初附着生物膜的粘附力。由JN111和cabA突变体产生的生物膜结构的微观比较表明,CabA是细胞外基质成分,对于在流通池和牡蛎壳上成熟的生物膜结构的发育至关重要。当有钙时,外源提供纯化的CabA可以恢复cabA突变体的生物膜和皱纹菌落形成能力。圆二色性和尺寸排阻分析表明,钙结合诱导CabA构象变化,可能导致多聚化。细胞外互补实验表明,只有胞外多糖共存时,CabA才能组装功能性基质。因此,综合结果表明,CabA是细胞外基质的结构蛋白,可以多聚化为构象,在构建坚固的生物膜中起作用,这可能使创伤弧菌能够在恶劣的环境中生存并达到集中的感染剂量。

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