发现由 RAGATH-18 衍生 RNA 引导的 DNA 内切酶及其结构机制

IF 28.1 1区 生物学 Q1 CELL BIOLOGY
Kuan Ren, Fengxia Zhou, Fan Zhang, Mingyu Yin, Yuwei Zhu, Shouyu Wang, Yan Chen, Tengjin Huang, Zixuan Wu, Jiale He, Anqi Zhang, Changyou Guo, Zhiwei Huang
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引用次数: 0

摘要

CRISPR-Cas系统和IS200/IS605转座子相关TnpBs已被用于基因组编辑技术的开发。通过生物信息学分析和生化实验,我们在此提出了一个新的 RNA 引导 DNA 内切酶家族。我们的生物信息学分析初步确定了保守的 RAGATH-18 衍生 RNA(reRNA)及其上游平均长度为 390 个氨基酸的 IS607 TnpB 的稳定共存。IS607 TnpBs 通过与 reRNAs 相互作用形成可编程的 DNases。我们发现 IS607 TnpB 系统在细菌和人类细胞中具有强大的 dsDNA 干扰活性。对真菌 IS607 TnpB 系统(ISFba1 TnpB)的进一步鉴定发现,它的 dsDNA 裂解活性对人类细胞中引导序列和目标序列之间的单个错配非常敏感。我们的研究结果表明,reRNA 引导序列中 20 nt 的长度可使 ISFba1 TnpB 获得最高的 DNA 切割活性。ISFba1 TnpB效应蛋白与其同源的含RAGATH-18基序的reRNA和dsDNA靶标结合的冷冻电镜结构揭示了ISFba1 TnpB识别reRNA、reRNA引导的dsDNA靶标以及ISFba1 TnpB系统对引导序列和靶标DNA之间碱基错配的敏感性的机制。总之,这项研究发现了 IS607 TnpB 家族紧凑而特异的 RNA 引导 DN 酶,它们在基因编辑方面具有巨大的应用潜力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Discovery and structural mechanism of DNA endonucleases guided by RAGATH-18-derived RNAs

Discovery and structural mechanism of DNA endonucleases guided by RAGATH-18-derived RNAs
CRISPR-Cas systems and IS200/IS605 transposon-associated TnpBs have been utilized for the development of genome editing technologies. Using bioinformatics analysis and biochemical experiments, here we present a new family of RNA-guided DNA endonucleases. Our bioinformatics analysis initially identifies the stable co-occurrence of conserved RAGATH-18-derived RNAs (reRNAs) and their upstream IS607 TnpBs with an average length of 390 amino acids. IS607 TnpBs form programmable DNases through interaction with reRNAs. We discover the robust dsDNA interference activity of IS607 TnpB systems in bacteria and human cells. Further characterization of the Firmicutes bacteria IS607 TnpB system (ISFba1 TnpB) reveals that its dsDNA cleavage activity is remarkably sensitive to single mismatches between the guide and target sequences in human cells. Our findings demonstrate that a length of 20 nt in the guide sequence of reRNA achieves the highest DNA cleavage activity for ISFba1 TnpB. A cryo-EM structure of the ISFba1 TnpB effector protein bound by its cognate RAGATH-18 motif-containing reRNA and a dsDNA target reveals the mechanisms underlying reRNA recognition by ISFba1 TnpB, reRNA-guided dsDNA targeting, and the sensitivity of the ISFba1 TnpB system to base mismatches between the guide and target DNA. Collectively, this study identifies the IS607 TnpB family of compact and specific RNA-guided DNases with great potential for application in gene editing.
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来源期刊
Cell Research
Cell Research 生物-细胞生物学
CiteScore
53.90
自引率
0.70%
发文量
2420
审稿时长
2.3 months
期刊介绍: Cell Research (CR) is an international journal published by Springer Nature in partnership with the Center for Excellence in Molecular Cell Science, Chinese Academy of Sciences (CAS). It focuses on publishing original research articles and reviews in various areas of life sciences, particularly those related to molecular and cell biology. The journal covers a broad range of topics including cell growth, differentiation, and apoptosis; signal transduction; stem cell biology and development; chromatin, epigenetics, and transcription; RNA biology; structural and molecular biology; cancer biology and metabolism; immunity and molecular pathogenesis; molecular and cellular neuroscience; plant molecular and cell biology; and omics, system biology, and synthetic biology. CR is recognized as China's best international journal in life sciences and is part of Springer Nature's prestigious family of Molecular Cell Biology journals.
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