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Characterization of the low-pH responses of Helicobacter pylori using genomic DNA arrays

机译:使用基因组DNA阵列表征幽门螺杆菌的低pH反应

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Helicobacter pylori is unique among bacterial pathogens in its ability to persist in the acidic environment of the human stomach. To identify H. pylori genes responsive to low pH, the authors assembled a high-density array of PCR-amplified random genomic DNA. Hybridization of radiolabelled cDNA probes, prepared using total RNA from bacteria exposed to buffer at either pH?4·0 or pH?7·0, allowed both qualitative and quantitative information on differential gene expression to be obtained. A previously described low-pH-induced gene, cagA, was identified together with several novel genes that may have relevance to the survival and persistence of H. pylori in the gastric environment. These include genes encoding enzymes involved in LPS and phospholipid synthesis and secF, encoding a component of the protein export machinery. A hypothetical protein unique to H. pylori (HP0681) was also found to be acid induced. Genes down-regulated at pH?4·0 include those encoding a sugar nucleotide biosynthesis protein, a flagellar protein and an outer-membrane protein. Differential gene expression was confirmed by total RNA slot-blot hybridization.
机译:幽门螺杆菌在细菌病原体中是独一无二的,其能够持续存在于人类胃的酸性环境中。响应于低pH鉴定幽门螺杆菌基因,作者组装了高密度阵列的PCR扩增的无规基因组DNA。放射性标记的cDNA探针的杂交,使用从暴露于缓冲液的细菌的总RNA制备在pH?4·0或pH oth?7·0的细菌中制备,允许获得差异基因表达的定性和定量信息。先前描述的低pH诱导的基因Caga与几种新的基因一起鉴定在胃环境中的幽门螺杆菌的存活和持续性有关。这些包括编码参与LPS和磷脂合成的酶的基因和SECF,编码蛋白质出口机制的组分。还发现了H. Pylori(HP0681)特有的假设蛋白是酸诱导的。在pHα4·0处下调的基因包括编码糖核苷酸生物合成蛋白,鞭毛蛋白和外膜蛋白的那些。通过RNA槽印迹杂交的总RNA槽印迹证实了差异基因表达。

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