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CRISPR-Cas12m 效应物的先天可编程 DNA 结合使碱基编辑得以高效进行。

Innate programmable DNA binding by CRISPR-Cas12m effectors enable efficient base editing.

机构信息

Institute of Biotechnology, Life Sciences Center, Vilnius University, Vilnius LT-10257, Lithuania.

Peter Debye Institute for Soft Matter Physics, University of Leipzig, Leipzig 04103, Germany.

出版信息

Nucleic Acids Res. 2024 Apr 12;52(6):3234-3248. doi: 10.1093/nar/gkae016.

Abstract

Cas9 and Cas12 nucleases of class 2 CRISPR-Cas systems provide immunity in prokaryotes through RNA-guided cleavage of foreign DNA. Here we characterize a set of compact CRISPR-Cas12m (subtype V-M) effector proteins and show that they provide protection against bacteriophages and plasmids through the targeted DNA binding rather than DNA cleavage. Biochemical assays suggest that Cas12m effectors can act as roadblocks inhibiting DNA transcription and/or replication, thereby triggering interference against invaders. Cryo-EM structure of Gordonia otitidis (Go) Cas12m ternary complex provided here reveals the structural mechanism of DNA binding ensuring interference. Harnessing GoCas12m innate ability to bind DNA target we fused it with adenine deaminase TadA-8e and showed an efficient A-to-G editing in Escherichia coli and human cells. Overall, this study expands our understanding of the functionally diverse Cas12 protein family, revealing DNA-binding dependent interference mechanism of Cas12m effectors that could be harnessed for engineering of compact base-editing tools.

摘要

CRISPR-Cas 系统 2 类的 Cas9 和 Cas12 核酸酶通过 RNA 引导的外源 DNA 切割为原核生物提供免疫。在这里,我们描述了一组紧凑型 CRISPR-Cas12m(亚型 V-M)效应蛋白,并表明它们通过靶向 DNA 结合而不是 DNA 切割来提供针对噬菌体和质粒的保护。生化分析表明,Cas12m 效应蛋白可以作为阻碍物抑制 DNA 转录和/或复制,从而引发针对入侵物的干扰。本文提供的 Gordonia otitidis (Go) Cas12m 三元复合物的冷冻电镜结构揭示了确保干扰的 DNA 结合的结构机制。利用 GoCas12m 结合 DNA 靶标的固有能力,我们将其与腺嘌呤脱氨酶 TadA-8e 融合,并在大肠杆菌和人类细胞中显示出有效的 A 到 G 编辑。总体而言,这项研究扩展了我们对功能多样的 Cas12 蛋白家族的理解,揭示了 Cas12m 效应蛋白依赖 DNA 结合的干扰机制,可用于工程紧凑型碱基编辑工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2e06/11013384/b2bde99c021a/gkae016figgra1.jpg

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