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大肠杆菌中G→T突变的稳定期诱导

Stationary phase-induction of G-->T mutations in Escherichia coli.

作者信息

Shu Joline, Schellhorn Herb E, Murphy Terence M

机构信息

Section of Plant Biology, University of California, One Shields Avenue, Davis, CA 95616, USA.

出版信息

Mutat Res. 2006 Apr 11;596(1-2):106-12. doi: 10.1016/j.mrfmmm.2005.12.015. Epub 2006 Feb 21.

Abstract

A series of Escherichia coli mutants, constructed originally by Cupples and Miller [C.G. Cupples, J.H. Miller, A set of lacZ mutations in Escherichia coli that allow rapid detection of each of the six base substitutions, Proc. Natl. Acad. Sci. U.S.A. 86 (1989) 5345-5349], provides a unique system for quantifying base-change mutations, and the repair processes that limit their establishment, in bacteria under selective and non-selective conditions. We focussed on one strain in which a T-->G replacement inactivates the lacZ gene. Reversions of this strain can occur through oxidation of G, leading to G-->T transversions. We show that spontaneous reversions occurred both in lactose (selective) and glucose (non-selective) medium. The number of revertants per viable cell was much greater in medium containing lactose or both sugars than glucose alone. In glucose medium, the rate of reversion was highest below 0.6% glucose and strongly inhibited at and above that level. Evidence that reversions occurred through G-->T transversions in both lactose and glucose media came from two observations: by sequence analysis of a series of revertants and by comparing the reversion rates in strains possessing and lacking the mutM gene (encoding formamidopyrimidine DNA glycosylase, FPG). However, the rate of reversion was stimulated by reducing O2 to 1% and inhibited or delayed by increasing O2 to 90%. In mutM- cells grown on glucose medium, the proportion of revertants increased over a 5-day period. In contrast, in mutM+ cells, revertants appeared primarily during the first 2-3 days after plating; few new revertants appeared in the following days. These data imply that base excision repair initiated by FPG was less effective in the first 2 days and more effective later in stationary phase.

摘要

一系列最初由卡普尔斯和米勒构建的大肠杆菌突变体[C.G. 卡普尔斯、J.H. 米勒,一组大肠杆菌中的lacZ突变,可快速检测六种碱基替换中的每一种,《美国国家科学院院刊》86 (1989) 5345 - 5349],提供了一个独特的系统,用于在选择性和非选择性条件下,对细菌中的碱基变化突变以及限制其产生的修复过程进行定量分析。我们聚焦于其中一个菌株,该菌株中一个T→G的替换使lacZ基因失活。这个菌株的回复突变可以通过G的氧化发生,导致G→T的颠换。我们表明,自发回复突变在乳糖(选择性)和葡萄糖(非选择性)培养基中均会发生。在含有乳糖或两种糖的培养基中,每个活细胞的回复子数量比单独使用葡萄糖时多得多。在葡萄糖培养基中,回复突变率在葡萄糖浓度低于0.6%时最高,在该浓度及以上时受到强烈抑制。在乳糖和葡萄糖培养基中回复突变是通过G→T颠换发生的证据来自两个观察结果:对一系列回复子的序列分析,以及比较具有和缺乏mutM基因(编码甲酰胺嘧啶DNA糖基化酶,FPG)的菌株中的回复突变率。然而,将氧气浓度降至1%会刺激回复突变率,而将氧气浓度提高到90%会抑制或延迟回复突变。在葡萄糖培养基上生长的mutM-细胞中,回复子的比例在5天内增加。相比之下,在mutM+细胞中,回复子主要在接种后的头2 - 3天出现;在随后的几天里几乎没有新的回复子出现。这些数据表明,由FPG启动的碱基切除修复在最初2天效果较差,而在稳定期后期效果更好。

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