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CRISPR Display: A modular method for locus-specific targeting of long noncoding RNAs and synthetic RNA devices in vivo

机译:CRISPR展示:一种用于体内长非编码RNA和合成RNA装置的基因座特异性靶向的模块化方法

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摘要

Noncoding RNAs (ncRNAs) comprise an important class of regulatory molecules that mediate a vast array of biological processes. This broad functional capacity has also facilitated the design of artificial ncRNAs with novel functions. To further investigate and harness these capabilities, we developed CRISPR-Display (“CRISP-Disp”), a targeted localization method that uses Sp. Cas9 to deploy large RNA cargos to DNA loci. We demonstrate that exogenous RNA domains can be functionally appended onto the CRISPR scaffold at multiple insertion points, allowing the construction of Cas9 complexes with protein-binding cassettes, artificial aptamers, pools of random sequences, and RNAs up to 4.8 kilobases in length, including natural lncRNAs. Unlike most existing CRISPR methods, CRISP-Disp allows simultaneous multiplexing of distinct functions at multiple targets, limited only by the number of available functional RNA motifs. We anticipate that this technology will provide a powerful method with which to ectopically localize functional RNAs and ribonucleoprotein (RNP) complexes at specified genomic loci.
机译:非编码RNA(ncRNA)包含一类重要的调节分子,可介导大量生物过程。这种广泛的功能能力也促进了具有新颖功能的人工ncRNA的设计。为了进一步研究和利用这些功能,我们开发了CRISPR-Display(“ CRISP-Disp”),这是一种使用Sp的靶向定位方法。 Cas9将大型RNA货物部署到DNA基因座。我们证明了外源RNA结构域可以在多个插入点功能上附加到CRISPR支架上,从而允许构建具有蛋白质结合盒,人工适体,随机序列库和最长4.8千碱基(包括天然)的RNA的Cas9复合物。 lncRNA。与大多数现有的CRISPR方法不同,CRISP-Disp允许在多个靶标上同时复用不同功能,而仅受限于可用功能性RNA基序的数量。我们预计,这项技术将提供一种功能强大的方法,可将功能性RNA和核糖核蛋白(RNP)复合体异位定位在指定的基因组位点。

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