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A Versatile Two-Step CRISPR- and RMCE-Based Strategy for Efficient Genome Engineering in Drosophila

机译:基于两步法的基于CRIspR和RmCE的策略,用于果蝇中的高效基因组工程

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摘要

The development of clustered, regularly interspaced, short palindromic repeats (CRISPR)/CRISPR-associated (Cas) technologies promises a quantum leap in genome engineering of model organisms. However, CRISPR-mediated gene targeting reports in Drosophila melanogaster are still restricted to a few genes, use variable experimental conditions, and vary in efficiency, questioning the universal applicability of the method. Here, we developed an efficient two-step strategy to flexibly engineer the fly genome by combining CRISPR with recombinase-mediated cassette exchange (RMCE). In the first step, two sgRNAs, whose activity had been tested in cell culture, were co-injected together with a donor plasmid into transgenic Act5C-Cas9, Ligase4 mutant embryos and the homologous integration events were identified by eye fluorescence. In the second step, the eye marker was replaced with DNA sequences of choice using RMCE enabling flexible gene modification. We applied this strategy to engineer four different locations in the genome, including a gene on the fourth chromosome, at comparably high efficiencies. Our data suggest that any fly laboratory can engineer their favorite gene for a broad range of applications within approximately 3 months.
机译:簇状,规则间隔,短回文重复(CRISPR)/ CRISPR相关(Cas)技术的发展有望为模型生物的基因组工程带来巨大的飞跃。然而,果蝇中的CRISPR介导的基因靶向报道仍然仅限于少数基因,使用可变的实验条件,并且效率不同,这对该方法的普遍适用性提出了质疑。在这里,我们开发了一种有效的两步策略,通过将CRISPR与重组酶介导的盒式交换(RMCE)结合起来灵活地设计果蝇基因组。第一步,将已在细胞培养中测试其活性的两个sgRNA与供体质粒一起共注射到转基因Act5C-Cas9,Ligase4突变体胚胎中,并通过眼睛荧光鉴定同源整合事件。第二步,使用RMCE使眼标记物替换为选择的DNA序列,从而实现灵活的基因修饰。我们采用了这种策略,以相对较高的效率设计了基因组中的四个不同位置,包括第四条染色体上的一个基因。我们的数据表明,任何苍蝇实验室都可以在大约3个月内对自己喜欢的基因进行广泛的应用工程改造。

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