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A Molecular Chipper technology for CRISPR sgRNA library generation and functional mapping of noncoding regions

机译:用于CRISPR sgRNA文库生成和非编码区功能定位的Molecular Chipper技术

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摘要

Clustered regularly-interspaced palindromic repeats (CRISPR)-based genetic screens using single-guide-RNA (sgRNA) libraries have proven powerful to identify genetic regulators. Applying CRISPR screens to interrogate functional elements in noncoding regions requires generating sgRNA libraries that are densely covering, and ideally inexpensive, easy to implement and flexible for customization. Here we present a Molecular Chipper technology for generating dense sgRNA libraries for genomic regions of interest, and a proof-of-principle screen that identifies novel cis-regulatory domains for miR-142 biogenesis. The Molecular Chipper approach utilizes a combination of random fragmentation and a type III restriction enzyme to derive a densely covering sgRNA library from input DNA. Applying this approach to 17 microRNAs and their flanking regions and with a reporter for miR-142 activity, we identify both the pre-miR-142 region and two previously unrecognized cis-domains important for miR-142 biogenesis, with the latter regulating miR-142 processing. This strategy will be useful for identifying functional noncoding elements in mammalian genomes.
机译:已证明使用单向导RNA(sgRNA)文库的基于规则间隔的回文重复序列(CRISPR)的遗传筛选可有效识别遗传调控因子。将CRISPR筛选应用于非编码区域中的功能元件需要生成sgRNA文库,该文库密集覆盖,并且理想情况下价格低廉,易于实现且可灵活定制。在这里,我们介绍了一种用于生成感兴趣的基因组区域的密集sgRNA文库的Molecular Chipper技术,以及一种原理证明屏幕,它可以识别miR-142生物发生的新型顺式调控域。 Molecular Chipper方法利用随机片段化和III型限制性内切酶的组合,从输入DNA中获得密集覆盖的sgRNA文库。将这种方法应用于17个microRNA及其侧翼区域,并带有miR-142活性的报告基因,我们可以识别出miR-142前区和两个先前无法识别的对miR-142生物发生重要的顺式结构域,而后者则调控miR-142。 142处理。该策略对于鉴定哺乳动物基因组中的功能性非编码元件将是有用的。

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