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Harnessing CRISPR/Cas systems for programmable transcriptional and post transcriptional regulation

机译:利用CRISPR / CAS系统进行可编程转录和后转录调节

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摘要

Genome editing has enabled broad advances and novel approaches in studies of gene function and structure; now, emerging methods aim to precisely engineer post-transcriptional processes. Developing precise, efficient molecular tools to alter the transcriptome holds great promise for biotechnology and synthetic biology applications. Different approaches have been employed for targeted degradation of RNA species in eukaryotes, but they lack programmability and versatility, thereby limiting their utility for diverse applications. The CRISPR/Cas9 system has been harnessed for genome editing in many eukaryotic species and, using a catalytically inactive Cas9 variant, the CFUSPR/dCas9 system has been repurposed for transcriptional regulation. Recent studies have used other CRISPR/Cas systems for targeted RNA degradation and RNA-based manipulations. For example, Cas13a, a Type VI-A endonuclease, has been identified as an RNA-guided RNA ribonuclease and used for manipulation of RNA. Here, we discuss different modalities for targeted RNA interference with an emphasis on the potential applications of CRISPR/Cas systems as programmable transcriptional regulators for broad uses, including functional biology, biotechnology, and synthetic biology applications.
机译:基因组编辑能够实现基因功能和结构研究的广泛进步和新方法;现在,新兴的方法旨在精确地工程转录后流程。开发精确,有效的分子工具来改变转录体对生物技术和合成生物学应用具有很大的承担。已经采用不同的方法来用于真核生物中的RNA物种的靶向降解,但它们缺乏可编程性和多功能性,从而限制了它们进行各种应用的效用。 CRISPR / CAS9系统已经利用了许多真核生物种类的基因组编辑,并且使用催化活性CAS9变体,CFUSPR / DCAS9系统已被重新探测进行转录调控。最近的研究使用了其他CRAP / CAS系统,用于靶向RNA降解和基于RNA的操纵。例如,Cas13a,vi-a内切核酸酶,已被鉴定为RNA引导的RNA核糖核酸酶,并用于操纵RNA。在这里,我们讨论针对性RNA干扰的不同方式,强调CRISPR / CAS系统作为广泛用途的可编程转录调节器的潜在应用,包括功能生物学,生物技术和合成生物学应用。

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