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Cold Shock Response and Major Cold Shock Proteins of Vibrio cholerae

机译:霍乱弧菌的冷激反应和主要冷激蛋白

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摘要

When exponentially growing Vibrio cholerae cells were shifted from 37°C to various lower temperatures, it was found that the organism could adapt and grow at temperatures down to 15°C, below which the growth was completely arrested. There was no difference between the patterns of the cold shock responses in toxinogenic and nontoxinogenic strains of V. cholerae. Gel electrophoretic analyses of proteins of cold-exposed cells revealed significant induction of two major cold shock proteins (Csps), whose molecular masses were 7.7 kDa (CspAVC) and 7.5 kDa (CspV), and six other Csps, most of which were much larger. We cloned, sequenced, and analyzed the cspV gene encoding the CspV protein of V. cholerae O139 strain SG24. Although CspAVC and CspV have similar kinetics of synthesis and down-regulation, the corresponding genes, cspA and cspV, which are located in the small chromosome, are not located in the same operon. A comparative analysis of the kinetics of synthesis revealed that the CspV protein was synthesized de novo only during cold shock. Although both CspAVC and CspV were stable for several hours in the cold, the CspV protein was degraded rapidly when the culture was shifted back to 37°C, suggesting that this protein is probably necessary for adaptation at lower temperatures. Northern blot analysis confirmed that the cspV gene is cold shock inducible and is regulated tightly at the level of transcription. Interestingly, the cspV gene has a cold shock-inducible promoter which is only 12 nucleotides from the translational start site, and therefore, it appears that no unusually long 5′ untranslated region is present in its mRNA transcript. Thus, this promoter is an exception compared to other promoters of cold shock-inducible genes of different organisms, including Escherichia coli. Our results suggest that V. cholerae may use an alternative pathway for regulation of gene expression during cold shock.
机译:当呈指数增长的霍乱弧菌细胞从37°C转变为各种较低的温度时,发现该生物体可以适应并在低至15°C的温度下生长,在此温度以下,该生长被完全阻止。在霍乱弧菌的产毒和非产毒菌株中,冷休克反应的模式之间没有差异。凝胶电泳分析的冷暴露细胞蛋白揭示了两种主要冷激蛋白(Csps)的显着诱导,其分子质量分别为7.7 kDa(CspAVC)和7.5 kDa(CspV),以及其他六种Csps,其中大多数都更大。我们克隆,测序,并分析编码霍乱弧菌O139菌株SG24 CspV蛋白的cspV基因。尽管CspAVC和CspV具有相似的合成和下调动力学,但是位于小染色体上的相应基因cspA和cspV不在同一操纵子中。合成动力学的比较分析表明,CspV蛋白仅在冷休克期间从头合成。尽管CspAVC和CspV都在寒冷中稳定了几个小时,但当培养物移回37°C时,CspV蛋白迅速降解,这表明该蛋白可能是在较低温度下适应所必需的。 Northern印迹分析证实cspV基因是冷休克诱导的,并且在转录水平上受到严格调节。有趣的是,cspV基因具有一个冷休克诱导型启动子,该启动子距离翻译起始位点仅12个核苷酸,因此,似乎在其mRNA转录物中没有异常长的5'非翻译区。因此,与包括大肠杆菌在内的不同生物体的冷休克诱导基因的其他启动子相比,该启动子是一个例外。我们的结果表明,霍乱弧菌可能在冷休克期间使用一条替代途径来调节基因表达。

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