结合基因靶向和重组酶介导的盒式交换对人ESCs中hprt位点的序贯遗传修饰。

Alexandra I Di Domenico, Ioannis Christodoulou, Steve C Pells, Jim McWhir, Alison J Thomson
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引用次数: 43

摘要

人类胚胎干细胞(hESCs)的遗传修饰将是使这些细胞在再生医学和hESCs生物学研究中充分利用的重要工具。在这里,我们报道了hESCs中一个内源性基因(hprt)的多个序列修饰。通过同源重组(homologous recombination, HR),首次在hprt基因中引入了一个带有异源特异性位点的选择性标记。在随后的步骤中,通过重组酶介导的卡带交换(RMCE)将可选择标记物与另一个卡带交换。我们发现100%的恢复克隆是在hprt位点使用启动子陷阱策略进行RMCE的结果。靶向hprt的H1细胞维持二倍体核型,并在RMCE前后表达hESC表面标记物。最后,我们报告了一种双重替代策略,使用两个顺序的基因靶向步骤,导致hprt突变的hESC系的靶向纠正。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Sequential genetic modification of the hprt locus in human ESCs combining gene targeting and recombinase-mediated cassette exchange.

Genetic modification of human embryonic stem cells (hESCs) will be an essential tool to allow full exploitation of these cells in regenerative medicine and in the study of hESC biology. Here we report multiple sequential modifications of an endogenous gene (hprt) in hESCs. A selectable marker flanked by heterospecific lox sites was first introduced by homologous recombination (HR) into the hprt gene. In a subsequent step, exchange of the selectable marker with another cassette was achieved by recombinase-mediated cassette exchange (RMCE). We show that 100% of the recovered clones were the result of RMCE using a promoter trap strategy at the hprt locus. hprt-targeted H1 cells maintained a diploid karyotype and expressed hESC surface markers before and after RMCE. Finally, we report a double replacement strategy using two sequential gene targeting steps resulting in the targeted correction of an hprt-mutated hESC line.

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