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Effect of terminal nonhomologies on homologous recombination in Xenopus laevis oocytes.

机译:末端非同源性对非洲爪蟾卵母细胞同源重组的影响。

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Homologous recombination of linear DNA molecules in Xenopus laevis oocytes is very efficient. The predictions of molecular models for this recombination process were tested with substrates with terminal nonhomologies (nonhomologous sequences). It was found that nonhomologies on one or both ends of an otherwise efficient substrate substantially reduced the yield of recombination products. In the case of a single nonhomology, inhibition was observed for all lengths of nonhomology, from 60 to 1,690 bp, being most dramatic for the longer blocks. Examination of time courses of recombination showed that the blocks were largely kinetic; that is, substrates with short nonhomologies eventually yielded substantial levels of completed products. Intermediates that accumulated after the injection of end-blocked substrates were characterized by two-dimensional gel electrophoresis and hybridization with strand-specific oligonucleotide probes. These blocked intermediates were shown to have base-paired junctions, but resolution was prevented by the failure to remove the 3'-ending strand of the original nonhomology. Continuing exonuclease action created a single-strand gap adjacent to the position of the persistent nonhomology. In contrast, the strand that included the unblocked side of the junction could be sealed. These results are consistent with a nonconservative, resection-annealing mechanism of homologous recombination in the oocytes and suggest the absence of any activity that can efficiently remove 3' tails.
机译:非洲爪蟾卵母细胞中线性DNA分子的同源重组是非常有效的。使用具有末端非同源性(非同源序列)的底物测试了此重组过程的分子模型的预测。已经发现,在其他方面有效的底物的一个或两个末端上的非同源性大大降低了重组产物的产率。在单一非同源性的情况下,在从60到1,690 bp的所有长度的非同源性中均观察到抑制,对于更长的嵌段而言,抑制作用最为明显。检查重组的时间过程表明,这些嵌段主要是动力学的。也就是说,具有短非同质性的基板最终会产生大量的成品。注射末端封闭的底物后积累的中间体通过二维凝胶电泳和与链特异性寡核苷酸探针的杂交来表征。这些封闭的中间体显示具有碱基配对的连接,但是由于未能去除原始非同源性的3'端链而阻止了拆分。连续的核酸外切酶作用在持久非同源性的位置附近产生了单链缺口。相反,可以密封包括连接处未阻塞侧的线束。这些结果与卵母细胞中同源重组的非保守的切除退火机制相一致,表明没有任何可以有效去除3'尾巴的活性。

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