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重组和RAD52在转化到酵母中的染色体DNA突变中的作用。

The role of recombination and RAD52 in mutation of chromosomal DNA transformed into yeast.

作者信息

Larionov V, Graves J, Kouprina N, Resnick M A

机构信息

Laboratory of Molecular Genetics, National Institute of Environmental Health Sciences, Research Triangle Park, NC 27709.

出版信息

Nucleic Acids Res. 1994 Oct 11;22(20):4234-41. doi: 10.1093/nar/22.20.4234.

Abstract

While transformation is a prominent tool for genetic analysis and genome manipulation in many organisms, transforming DNA has often been found to be unstable relative to established molecules. We determined the potential for transformation-associated mutations in a 360 kb yeast chromosome III composed primarily of unique DNA. Wild-type and rad52 Saccharomyces cerevisiae strains were transformed with either a homologous chromosome III or a diverged chromosome III from S. carlsbergensis. The host strain chromosome III had a conditional centromere allowing it to be lost on galactose medium so that recessive mutations in the transformed chromosome could be identified. Following transformation of a RAD+ strain with the homologous chromosome, there were frequent changes in the incoming chromosome, including large deletions and mutations that do not lead to detectable changes in chromosome size. Based on results with the diverged chromosome, interchromosomal recombinational interactions were the source of many of the changes. Even though rad52 exhibits elevated mitotic mutation rates, the percentage of transformed diverged chromosomes incapable of substituting for the resident chromosome was not increased in rad52 compared to the wild-type strain, indicating that the mutator phenotype does not extend to transforming chromosomal DNA. Based on these results and our previous observation that the incidence of large mutations is reduced during the cloning of mammalian DNA into a rad52 as compared to a RAD+ strain, a rad52 host is well-suited for cloning DNA segments in which gene function must be maintained.

摘要

虽然转化是许多生物体中进行遗传分析和基因组操作的重要工具,但相对于已有的分子,转化DNA往往被发现是不稳定的。我们确定了在一条主要由独特DNA组成的360 kb酵母III号染色体中与转化相关的突变可能性。用来自卡尔酵母的同源III号染色体或分歧的III号染色体转化野生型和rad52酿酒酵母菌株。宿主菌株的III号染色体有一个条件性着丝粒,使其在半乳糖培养基上丢失,从而可以鉴定转化染色体中的隐性突变。用同源染色体转化RAD+菌株后,导入的染色体频繁发生变化,包括大的缺失和不会导致染色体大小有可检测变化的突变。根据分歧染色体的结果,染色体间的重组相互作用是许多变化的来源。尽管rad52表现出较高的有丝分裂突变率,但与野生型菌株相比,rad52中不能替代常驻染色体的转化分歧染色体的百分比并未增加,这表明突变体表型并不延伸到转化染色体DNA。基于这些结果以及我们之前的观察,即与RAD+菌株相比,将哺乳动物DNA克隆到rad52中时大突变的发生率降低,rad52宿主非常适合克隆必须维持基因功能的DNA片段。

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