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Restriction enzymes increase efficiencies of illegitimate DNA integration but decrease homologous integration in mammalian cells

机译:限制性内切酶提高了非法DNA整合的效率,但降低了哺乳动物细胞中的同源整合

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摘要

Mammalian cells repair DNA double-strand breaks by illegitimate end-joining or by homologous recombination. We investigated the effects of restriction enzymes on illegitimate and homologous DNA integration in mammalian cells. A plasmid containing the neO~R expression cassette, which confers G418 resistance, was used to select for illegitimate integration events in CHO wild-type and xrcc5 mutant cells. Co-transfection with the restriction enzymes BamHI, BglII, EcoRI and KpnI increased the efficiency of linearized plasmid integration up to 5 fold in CHO cells. In contrast, the restriction enzymes did not increase the integration efficiency in xrcc5 mutant cells. Effects of restriction enzymes on illegitimate and homologous integration were also studied in mouse embryonic stem (ES) cells using a plasmid containing the neo~R gene flanked by exon 3 of Hprt. The enzymes BamHI, BglII and EcoRI increased the illegitimate integration efficiency of transforming DNA several-fold, similar to the results for CHO cells. However, all three enzymes decreased the absolute frequency of homologous integration ~2-fold, and the percentage of homologous integration decreased >10-fold. This suggests that random DNA breaks attract illegitimate recombination (IR) events that compete with homology search.
机译:哺乳动物细胞通过非法末端连接或同源重组来修复DNA双链断裂。我们调查了限制酶对哺乳动物细胞中非法和同源DNA整合的影响。含有赋予G418抗性的neO〜R表达盒的质粒被用于选择CHO野生型和xrcc5突变细胞中的非法整合事件。与限制酶BamHI,BglII,EcoRI和KpnI共转染将线性化质粒整合的效率提高到CHO细胞的5倍。相反,限制性内切酶并未增加xrcc5突变细胞中的整合效率。还使用含有Hprt外显子3侧翼的neo-R基因的质粒,在小鼠胚胎干(ES)细胞中研究了限制酶对非法和同源整合的影响。酶BamHI,BglII和EcoRI将转化DNA的非法整合效率提高了几倍,类似于CHO细胞的结果。但是,这三种酶均使同源整合的绝对频率降低了约2倍,并且同源整合的百分比降低了> 10倍。这表明随机DNA断裂会吸引与同源搜索竞争的非法重组(IR)事件。

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