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Site-directed mutagenesis of the Klebsiella pneumoniae nifL and nifH promoters and in vivo analysis of promoter activity

机译:肺炎克雷伯菌nifL和nifH启动子的定点诱变和启动子活性的体内分析

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The role of conserved nucleotides in nitrogen-fixation promoter function has been examined using both oligonucleotide and chemical mutagenesis to introduce base changes in the Klebsiella pneumoniae nifL and nifH promoters. Among ten mutations analysed, including six spontaneous mutations, base changes at -12, -13, -14, and -26, located in previously identified conserved sequences, perturbed the activity of the promoters, demonstrating that these sequences are required for transcription. Not all base changes produced similar strong promoter down phenotypes when the nifL and nifH promoters were compared: activation of the nifH promoter by the nifA gene product was less sensitive to base changes in conserved nucleotides than was activation of the equivalently altered nifL promoter by the nifA or ntrC products. We have found that the nifH promoter can be weakly activated by the ntrC product; this activation shows the same down response to base changes seen with ntrC activation of the nifL promoter. We present evidence that the efficient activation of the nifH promoter by nifA (but not ntrC) can be attributed to specific upstream sequences present in the nifH promoter.
机译:使用寡核苷酸和化学诱变法在肺炎克雷伯氏菌nifL和nifH启动子中引入碱基变化,已经检查了保守核苷酸在固氮启动子功能中的作用。在分析的十个突变中,包括六个自发突变,位于先前确定的保守序列中的-12,-13,-14和-26处的碱基变化干扰了启动子的活性,表明这些序列是转录所必需的。比较nifL和nifH启动子时,并非所有碱基改变都产生相似的强启动子下降表型:与通过nifA等效改变的nifL启动子激活相比,由nifA基因产物激活nifH启动子对保守核苷酸的敏感性较低。或ntrC产品。我们发现nifC启动子可以被ntrC产物弱激活。这种激活对nifL启动子的ntrC激活所见的碱基变化显示出相同的下降反应。我们提供的证据表明,由nifA(而非ntrC)对nifH启动子进行的有效激活可以归因于nifH启动子中存在的特定上游序列。

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