首页> 外文OA文献 >Nucleotide sequence, mutational analysis, transcriptional start site, and product analysis of nov, the gene which affects Escherichia coli K-12 resistance to the gyrase inhibitor novobiocin.
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Nucleotide sequence, mutational analysis, transcriptional start site, and product analysis of nov, the gene which affects Escherichia coli K-12 resistance to the gyrase inhibitor novobiocin.

机译:nov的核苷酸序列,突变分析,转录起始位点和产物分析,该基因会影响大肠杆菌K-12对回旋酶抑制剂新霉素的抗性。

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摘要

In a previous study, we demonstrated the existence of a gene locus, nov, which affects resistance of Escherichia coli K-12 to the gyrase inhibitor novobiocin and, to a lesser degree, coumermycin (J. Rakonjac, M. Milic, D. Ajdic, D. Santos, R. Ivanisevic, and D. J. Savic, Mol. Microbiol. 6:1547-1553, 1992). In the present study, sequencing of the nov gene locus revealed one open reading frame that encodes a protein of 54,574 Da, a value. found to be in correspondence with the size of the Nov protein identified in an in vitro translation system. We also located the 5' end of the nov transcript 8 bp downstream from a classical sigma70 promoter. Transcription of the gene is in the counterclockwise direction on the E. coli chromosome. Transposon mutagenesis of nov followed by complementation analyses and replacement of chromosomal alleles with mutated nov confirmed our previous assumption that the nov gene exists in two allelic forms and that the Novr gene is an active allele while the Novs gene is an inactive form. After comparing nucleotide sequences flanking the nov gene with existing data, we conclude that the gene order in this region of the E. coli K-12 map is att phi 80-open reading frame of unknown function-kch (potassium channel protein)-nov-opp. Finally, the possible identity of the nov gene with cls, the gene that codes for cardiolipin synthase, is also discussed.
机译:在先前的研究中,我们证明了存在一个基因座nov,该基因座影响大肠杆菌K-12对回旋酶抑制剂新生生物素的耐药性,而在较小程度上影响对香豆素的耐药性(J. Rakonjac,M。Milic,D。Ajdic ,D.Santos,R.Ivanisevic和DJSavic,Mol.Microbiol.6:1547-1553,1992)。在本研究中,对nov基因基因座的测序揭示了一个开放阅读框,该框架编码一个54,574 Da的蛋白质。被发现与体外翻译系统中鉴定的Nov蛋白大小一致。我们还将位于经典sigma70启动子下游nov转录物8 bp的5'端。该基因的转录是在大肠杆菌染色体上逆时针方向进行的。 nov的转座子诱变,然后进行互补分析和用突变的nov替换染色体等位基因,证实了我们先前的假设,即nov基因以两种等位基因形式存在,Novr基因是活跃等位基因,而Novs基因是非活跃形式。在比较nov基因侧翼的核苷酸序列与现有数据后,我们得出结论,该大肠杆菌K-12图区域中的基因顺序为att phi 80-未知功能-kch(钾通道蛋白)-nov的开放阅读框-opp。最后,还讨论了nov基因与编码心磷脂合酶的基因cls的可能同一性。

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