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Next stop for the CRISPR revolution: RNA-guided epigenetic regulators

机译:CRISPR革命的下一站:RNA引导的表观遗传调控子

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摘要

Clustered regularly interspaced short palindromic repeats (CRISPRs) and CRISPR-associated (Cas) proteins offer a breakthrough platform for cheap, programmable, and effective sequence-specific DNA targeting. The CRISPR-Cas system is naturally equipped for targeted DNA cutting through its native nuclease activity. As such, groups researching a broad spectrum of biological organisms have quickly adopted the technology with groundbreaking applications to genomic sequence editing in over 20 different species. However, the biological code of life is not only encoded in genetics but also in epigenetics as well. While genetic sequence editing is a powerful ability, we must also be able to edit and regulate transcriptional and epigenetic code. Taking inspiration from work on earlier sequence-specific targeting technologies such as zinc fingers (ZFs) and transcription activator-like effectors (TALEs), researchers quickly expanded the CRISPR-Cas toolbox to include transcriptional activation, repression, and epigenetic modification. In this review, we highlight advances that extend the CRISPR-Cas toolkit for transcriptional and epigenetic regulation, as well as best practice guidelines for these tools, and a perspective on future applications.
机译:簇状规则间隔的短回文重复序列(CRISPR)和CRISPR相关(Cas)蛋白为廉价,可编程和有效的序列特异性DNA靶向提供了突破性平台。 CRISPR-Cas系统自然具备通过其天然核酸酶活性进行靶向DNA切割的能力。因此,研究广泛的生物体的研究小组已迅速将这项具有开创性应用的技术应用于20多个不同物种的基因组序列编辑中。但是,生命的生物学代码不仅在遗传学中被编码,在表观遗传学中也被编码。尽管基因序列编辑是一种强大的功能,但我们还必须能够编辑和调节转录和后生代码。研究人员从诸如锌指(ZF)和转录激活因子样效应物(TALE)等早期序列特异性靶向技术的研究中获得灵感,研究人员迅速扩展了CRISPR-Cas工具箱,使其包括转录激活,抑制和表观遗传修饰。在这篇综述中,我们重点介绍了将CRISPR-Cas工具箱扩展用于转录和表观遗传调控的进展,以及这些工具的最佳实践指南,以及对未来应用的展望。

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