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Regulation of mutY and Nature of Mutator Mutations in Escherichia coli Populations under Nutrient Limitation

机译:营养限制条件下大肠埃希菌群体中mutY和突变体突变性质的调控

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摘要

Previous analysis of aerobic, glucose-limited continuous cultures of Escherichia coli revealed that G:C-to-T:A (G:C→T:A) transversions were the most commonly occurring type of spontaneous mutation. One possible explanation for the preponderance of these mutations was that nutrient limitation repressed MutY-dependent DNA repair, resulting in increased proportions of G:C→T:A transversions. The regulation of the mutY-dependent DNA repair system was therefore studied with a transcriptional mutY-lacZ fusion recombined into the chromosome. Expression from the mutY promoter was fourfold higher under aerobic conditions than under anaerobic conditions. But mutY expression was higher in glucose- or ammonia-limited chemostats than in nutrient-excess batch culture, so mutY was not downregulated by nutrient limitation. An alternative explanation for the frequency of G:C→T:A transversions was the common appearance of mutY mutator mutations in the chemostat populations. Of 11 chemostat populations screened in detail, six contained mutators, and the mutator mutation in four cultures was located in the region of mutY at 66 min on the chromosome. The spectrum of mutations and rate of mutation in these isolates were fully consistent with a mutY-deficiency in each strain. Based on PCR analysis of the region within and around mutY, isolates from three individual populations contained deletions extending at least 2 kb upstream of mutY and more than 5 kb downstream. In the fourth population, the deletion was even longer, extending at least 5 kb upstream and 5 kb downstream of mutY. The isolation of mutY mutator strains from four independent populations with extensive chromosomal rearrangements suggests that mutY inactivation by deletion is a means of increasing mutation rates under nutrient limitation and explains the observed frequency of G:C→T:A mutations in glucose-limited chemostats.
机译:先前对有氧,葡萄糖受限的连续培养物的分析表明,G:C到T:A(G:C→T:A)的转化是最常见的自发突变类型。这些突变占优势的一种可能解释是营养限制限制了MutY依赖性DNA修复,导致G:C→T:A转化的比例增加。因此,通过将重组的mutY-lacZ融合重组到染色体中来研究mutY依赖的DNA修复系统的调控。在有氧条件下,mutY启动子的表达要比无氧条件下高四倍。但是在葡萄糖或氨限制的化学恒温器中,mutY的表达高于营养过量的分批培养,因此mutY不会因营养限制而下调。 G:C→T:A转化频率的另一种解释是在恒化种群中常见的mutY突变突变。在详细筛选的11个化学恒温器种群中,六个包含突变体,四种培养物中的突变体突变位于染色体上66分钟处的mutY区域。这些分离株的突变谱和突变率与每种菌株的mutY缺陷完全一致。基于对mutY内和周围区域的PCR分析,来自三个个体群体的分离株包含在mutY上游至少2 kb和下游5 kb以上延伸的缺失。在第四个种群中,缺失甚至更长,在mutY上游至少延伸5 kb,在下游延伸5 kb。从具有广泛染色体重排的四个独立种群中分离mutY突变株表明,通过缺失进行mutY灭活是在营养限制下增加突变率的一种手段,并解释了在葡萄糖受限的恒化器中观察到的G:C→T:A突变的频率。

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