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修复功能正常和修复功能缺陷的仓鼠细胞中的链特异性突变谱。

Strand-specific mutation spectra in repair-proficient and repair-deficient hamster cells.

作者信息

Menichini P, Vrieling H, van Zeeland A A

机构信息

MGC Department of Radiation Genetics and Chemical Mutagenesis, State University of Leiden, The Netherlands.

出版信息

Mutat Res. 1991 Nov;251(1):143-55. doi: 10.1016/0027-5107(91)90224-c.

DOI:10.1016/0027-5107(91)90224-c
PMID:1944372
Abstract

The mutation spectrum induced by UV light has been determined at the hprt locus for both cultured normal (AA8) and UV-sensitive (UV-5) Chinese hamster ovary cells to investigate the effect of DNA repair on the nature of induced mutations. DNA base-pair changes of 23 hprt mutants of AA8 and of 28 hprt mutants of UV-5 were determined by sequence analysis of in vitro amplified hprt cDNA. Almost all mutants in AA8 carried single-base substitutions, transitions and transversions accounting for 38% and 62% of the base changes, respectively. In contrast, in repair-deficient cells (UV-5) tandem and nontandem double mutations represented a considerable portion of the mutations observed (30%), whereas the vast majority of base-pair substitutions were GC greater than AT transitions (87%). Moreover, 5 splice mutants and 2 frameshift mutations were found in the UV-5 collection. In almost all mutants analyzed base changes were located at dipyrimidine sites where UV photoproducts could have been formed. In AA8 the photolesions causing mutations were predominantly located in the nontranscribed strand whereas a strong bias for mutation induction towards photolesions in the transcribed strand was found in UV-5. We hypothesize that preferential removal of lesions from the transcribed strand of the hprt gene accounts for the observed DNA strand specificity of mutations in repair-proficient cells. Furthermore, differences in the degree of misincorporation opposite a lesion for lagging and leading strand DNA synthesis may dictate the pattern of UV-induced mutations in the absence of DNA repair.

摘要

为了研究DNA修复对诱导突变性质的影响,已在培养的正常(AA8)和紫外线敏感(UV-5)中国仓鼠卵巢细胞的hprt基因座处确定了紫外线诱导的突变谱。通过对体外扩增的hprt cDNA进行序列分析,确定了AA8的23个hprt突变体和UV-5的28个hprt突变体的DNA碱基对变化。AA8中的几乎所有突变体都携带单碱基取代,转换和颠换分别占碱基变化的38%和62%。相比之下,在修复缺陷细胞(UV-5)中,串联和非串联双突变占观察到的突变的相当一部分(30%),而绝大多数碱基对取代是GC大于AT转换(87%)。此外,在UV-5集合中发现了5个剪接突变体和2个移码突变。在几乎所有分析的突变体中,碱基变化位于可能形成紫外线光产物的二嘧啶位点。在AA8中,导致突变的光损伤主要位于非转录链中,而在UV-5中发现转录链中光损伤的突变诱导存在强烈偏向。我们假设从hprt基因的转录链中优先去除损伤是修复 proficient细胞中观察到的突变的DNA链特异性的原因。此外,滞后链和前导链DNA合成中与损伤相对的错配掺入程度的差异可能决定了在没有DNA修复的情况下紫外线诱导的突变模式。

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