首页> 外文期刊>Proceedings of the National Academy of Sciences of the United States of America >Chromosomal site-specific double-strand breaks are efficiently targeted for repair by oligonucleotides in yeast
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Chromosomal site-specific double-strand breaks are efficiently targeted for repair by oligonucleotides in yeast

机译:染色体位点特异性双链断裂被酵母中的寡核苷酸有效地靶向修复

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The repair of chromosomal double-strand breaks (DSBs) can be accomplished through homologous recombination in most organisms. We report here that exogenous oligonucleotides can efficiently target for repair a single DSB induced in a chromosome of yeast. The efficiency of recombinational targeting leading to a desired DNA change can be as high as 20% of cells. The DSB was generated either by a regulatable I-Scel endonuclease just before transformation or appeared spontaneously at the site of a long inverted repeat composed of human A/u sequences. The approach used features of our previously described delitto perfetto system for selecting transformants with integrative recombinant oligonucleotides. The DSB repair mediated by pairs of complementary integrative recombinant oligonucleotides was efficient for targeting to homologous sequences that were close to or distant from the DSB and in the presence of a competing homologous chromosome in diploid cells. We also demonstrate that a DSB can strongly stimulate recombination with single-stranded DNA, without strand bias. These findings expand current models of DSB repair. In addition, we establish a high-throughput system for rapid genome-wide modification with oligonucleotides.
机译:染色体双链断裂(DSB)的修复可通过大多数生物体中的同源重组来完成。我们在这里报告说,外源寡核苷酸可以有效地修复在酵母染色体中诱导的单个DSB。重组靶向导致所需DNA改变的效率可高达20%的细胞。 DSB是在转化前通过可调节的I-Scel核酸内切酶生成的,或自发出现在由人A / u序列组成的长反向重复序列的位点。该方法使用了我们先前描述的delitto perfetto系统的功能来选择带有整合重组寡核苷酸的转化子。由互补的整合重组寡核苷酸对介导的DSB修复可有效靶向接近或远离DSB的同源序列,并且在二倍体细胞中存在竞争性同源染色体。我们还证明了DSB可以强烈刺激与单链DNA的重组,而不会产生链偏向。这些发现扩展了DSB修复的当前模型。此外,我们建立了一个高通量系统,可利用寡核苷酸快速进行全基因组修饰。

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