在真核细胞中设计转录相关的 Cas9 靶向技术

IF 14.7 1区 综合性期刊 Q1 MULTIDISCIPLINARY SCIENCES
Gregory W. Goldberg, Manjunatha Kogenaru, Sarah Keegan, Max A. B. Haase, Larisa Kagermazova, Mauricio A. Arias, Kenenna Onyebeke, Samantha Adams, Daniel K. Beyer, David Fenyö, Marcus B. Noyes, Jef D. Boeke
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引用次数: 0

摘要

DNA 靶向第 2 类 CRISPR-Cas 效应核酸酶(包括研究得很清楚的 Cas9 蛋白)进化出了原间隔相邻基序(PAM)和引导 RNA 相互作用,这些作用按顺序许可它们在原间隔靶位点的结合和裂解活动。这两种相互作用都是核酸序列特异性的,但具有组成性功能;因此,它们提供了对 DNA 靶向活动的内在空间控制,但自然缺乏时间控制。在这里,我们展示了工程化的 Cas9 融合蛋白,它能与原空间定点附近的新生 RNA 结合,从而促进该原空间定点的转录和 DNA 靶向之间的时空耦合:转录相关Cas9靶向(TraCT)。在真核酵母或人类细胞中,当次优的 PAM 相互作用限制了基础活性,并且一个或多个新生 RNA 底物仍与活跃转录的靶 DNA 顺式连接时,就会启用工程化的 TraCT。我们利用酵母进一步证明,这种现象可用于选择性编辑不同基因位点上两个相同靶点中的一个,或者用于选择性编辑转录不同的二倍体等位基因位点。我们的工作表明,可以在不改变 Cas9 核心结构域和引导 RNA 成分或其表达水平的情况下,对 Cas9 在特定 DNA 位点的靶向活性进行时间控制。更广泛地说,它确立了共转录 RNA 结合作为一种顺式作用机制,可以有条件地刺激真核细胞中的 CRISPR-Cas DNA 靶向。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Engineered transcription-associated Cas9 targeting in eukaryotic cells

Engineered transcription-associated Cas9 targeting in eukaryotic cells

DNA targeting Class 2 CRISPR-Cas effector nucleases, including the well-studied Cas9 proteins, evolved protospacer-adjacent motif (PAM) and guide RNA interactions that sequentially license their binding and cleavage activities at protospacer target sites. Both interactions are nucleic acid sequence specific but function constitutively; thus, they provide intrinsic spatial control over DNA targeting activities but naturally lack temporal control. Here we show that engineered Cas9 fusion proteins which bind to nascent RNAs near a protospacer can facilitate spatiotemporal coupling between transcription and DNA targeting at that protospacer: Transcription-associated Cas9 Targeting (TraCT). Engineered TraCT is enabled in eukaryotic yeast or human cells when suboptimal PAM interactions limit basal activity and when one or more nascent RNA substrates are still tethered to the actively transcribed target DNA in cis. Using yeast, we further show that this phenomenon can be applied for selective editing at one of two identical targets in distinct gene loci, or, in diploid allelic loci that are differentially transcribed. Our work demonstrates that temporal control over Cas9’s targeting activity at specific DNA sites may be engineered without modifying Cas9’s core domains and guide RNA components or their expression levels. More broadly, it establishes co-transcriptional RNA binding as a cis-acting mechanism that can conditionally stimulate CRISPR-Cas DNA targeting in eukaryotic cells.

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来源期刊
Nature Communications
Nature Communications Biological Science Disciplines-
CiteScore
24.90
自引率
2.40%
发文量
6928
审稿时长
3.7 months
期刊介绍: Nature Communications, an open-access journal, publishes high-quality research spanning all areas of the natural sciences. Papers featured in the journal showcase significant advances relevant to specialists in each respective field. With a 2-year impact factor of 16.6 (2022) and a median time of 8 days from submission to the first editorial decision, Nature Communications is committed to rapid dissemination of research findings. As a multidisciplinary journal, it welcomes contributions from biological, health, physical, chemical, Earth, social, mathematical, applied, and engineering sciences, aiming to highlight important breakthroughs within each domain.
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