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首页> 外文期刊>Cellular and molecular life sciences: CMLS >An efficient method to enrich for knock-out and knock-in cellular clones using the CRISPR/Cas9 system
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An efficient method to enrich for knock-out and knock-in cellular clones using the CRISPR/Cas9 system

机译:使用CRISPR / CAS9系统丰富敲除和敲击蜂窝克隆的一种有效方法

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Clustered Regularly Interspaced Short Palin-dromic Repeats-associated protein 9 nuclease (CRISPR/Cas9) and Transcription Activator-Like Effector Nucleases (TALENs) are versatile tools for genome editing. Here we report a method to increase the frequency of Cas9-targeted cellular clones. Our method is based on a chimeric construct with a Blasticidin S Resistance gene (bsr) placed out-of-frame by a surrogate target sequence. End joining of the CRISPR/Cas9-induced double-strand break on the surrogate target can place the bsr in frame, thus providing temporary resistance to Blasticidin S: this is used to enrich for cells where Cas9 is active. By this approach, in a real experimental setting, we disrupted the Aicda gene in similar to 70% of clones from CH12F3 lymphoma cells (> 40% biallelically). With the same approach we knocked in a single nucleotide to reconstruct the frame of Aicda in these null cells, restoring the function in similar to 37% of the clones (less than 10% by the standard approach). Targeting of single nucleotide changes in other genes yielded analogous results. These results support our enrichment method as an efficient tool in genome editing.
机译:聚集定期间隙的短暂的牙龈摇粒型重复相关蛋白质9核酸酶(CRISPR / CAS9)和转录活化剂样效应核酸酶(TALENS)是基因组编辑的通用工具。在这里,我们报告了一种增加Cas9目标蜂窝克隆频率的方法。我们的方法基于嵌合体构建体,其具有替代靶序列置于框架外置于框架上的Blasticin S的抗性基因(BSR)。替换靶标的CRISPR / CAS9诱导的双链断裂的结束可以将BSR放置在框架中,从而为BlasticIdIN S提供暂时性的抗性:这用于富集Cas9活性的细胞。通过这种方法,在真实的实验环境中,我们中断了AICDA基因与CH12F3淋巴瘤细胞的70%克隆(20%双链)。具有相同的方法,我们敲入单个核苷酸中以重建在这些零细胞中的AICDA框架,恢复类似于克隆的克隆的功能(通过标准方法小于10%)。靶向其他基因的单核苷酸变化产生类似的结果。这些结果支持我们的浓缩方法作为基因组编辑的有效工具。

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