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首页> 外文期刊>Molecular Microbiology >GENETIC ANALYSIS OF PERTUSSIS TOXIN PROMOTER ACTIVATION IN BORDETELLA PERTUSSIS
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GENETIC ANALYSIS OF PERTUSSIS TOXIN PROMOTER ACTIVATION IN BORDETELLA PERTUSSIS

机译:百日咳百日咳中百日咳毒素启动子的遗传分析

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摘要

Bordetella pertussis regulates expression of its virulence factors such as pertussis toxin (Ptx) via the bvg locus, which encodes a two-component system composed of a sensor protein, BvgS, and a transcription activator, BvgA. We used a ptx-lac fusion on the B. pertussis chromosome to analyse promoter activation by alteration of specific sequences upstream of and within the promoter. Our data demonstrate that a pair of heptanucleotide inverted repeats separated by a turn of the DNA helix within the upstream repeat region (centred around nucleotide -136.5) are crucial cis-activating elements, and probably represent the initial BvgA-binding site. In addition, we demonstrate that the sequence between these repeats and the promoter plays a role in activation. Our data are most consistent with a model of co-operative binding of BvgA dimers to this intervening region and interaction with RNA polymerase at the promoter to activate ptx transcription. In the core promoter region both the non-consensus 21 bp spacing and the specific sequence between the -35 and -10 elements are crucial for promoter activity. [References: 34]
机译:百日咳博德特氏菌通过bvg基因座调节其毒力因子(例如百日咳毒素)的表达,该基因编码由传感器蛋白BvgS和转录激活剂BvgA组成的两组分系统。我们在百日咳博德特氏菌染色体上使用了ptx-lac融合体,通过改变启动子上游和内部的特定序列来分析启动子的激活。我们的数据表明,一对被上游重复区域(以核苷酸-136.5为中心)中的DNA螺旋旋转隔开的七核苷酸反向重复序列是至关重要的顺式激活元件,可能代表了最初的BvgA结合位点。另外,我们证明了这些重复序列与启动子之间的序列在激活中起作用。我们的数据与BvgA二聚体与该中间区域的合作结合以及在启动子处与RNA聚合酶相互作用以激活ptx转录的模型相一致。在核心启动子区域中,非共有的21 bp间隔以及-35和-10元件之间的特定序列对于启动子活性至关重要。 [参考:34]

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