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RNA stem structure governs coupling of dicing and gene silencing in RNA interference.RNA 茎结构控制 RNA 干扰中的切割和基因沉默的偶联。
Proc Natl Acad Sci U S A. 2017 Nov 28;114(48):E10349-E10358. doi: 10.1073/pnas.1710298114. Epub 2017 Nov 13.
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Prokaryotic Argonaute proteins: novel genome-editing tools?原核 Argonaute 蛋白:新型基因组编辑工具?
Nat Rev Microbiol. 2018 Jan;16(1):5-11. doi: 10.1038/nrmicro.2017.73. Epub 2017 Jul 24.
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DNA recognition by an RNA-guided bacterial Argonaute.由RNA引导的细菌Argonaute蛋白对DNA的识别
PLoS One. 2017 May 17;12(5):e0177097. doi: 10.1371/journal.pone.0177097. eCollection 2017.
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Structural and mechanistic insights into an archaeal DNA-guided Argonaute protein.古菌 DNA 指导的 Argonaute 蛋白的结构和机制见解。
Nat Microbiol. 2017 Mar 20;2:17035. doi: 10.1038/nmicrobiol.2017.35.
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Guide-independent DNA cleavage by archaeal Argonaute from Methanocaldococcus jannaschii.古菌 Argonaute 对 Methanocaldococcus jannaschii 的无向导 RNA 切割。
Nat Microbiol. 2017 Mar 20;2:17034. doi: 10.1038/nmicrobiol.2017.34.
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Mol Cell. 2017 Mar 16;65(6):985-998.e6. doi: 10.1016/j.molcel.2017.01.033. Epub 2017 Mar 2.
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TRBP ensures efficient Dicer processing of precursor microRNA in RNA-crowded environments.TRBP 确保了在 RNA 拥挤环境中前体 microRNA 的高效 Dicer 加工。
Nat Commun. 2016 Dec 9;7:13694. doi: 10.1038/ncomms13694.
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Mechanistic Insights into Archaeal and Human Argonaute Substrate Binding and Cleavage Properties.古菌和人类AGO蛋白底物结合与切割特性的机制研究
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QM/MM free energy simulations: recent progress and challenges.量子力学/分子力学自由能模拟:近期进展与挑战
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两个对称的精氨酸残基在 Argonaute 引导链介导的 DNA 靶标切割中发挥不同的作用。

Two symmetric arginine residues play distinct roles in Argonaute DNA guide strand-mediated DNA target cleavage.

机构信息

Department of Chemistry, Center of Systems Biology and Human Health, State Key Laboratory of Molecular Neuroscience, Hong Kong Branch of Chinese National Engineering Research Center for Tissue Restoration & Reconstruction, The Hong Kong University of Science and Technology, 190, Clear Water Bay, Kowloon, Hong Kong.

Key Laboratory of RNA Biology, Chinese Academy of Sciences Center for Excellence in Biomacromolecules, Institute of Biophysics, Chinese Academy of Sciences, 100101 Beijing, China.

出版信息

Proc Natl Acad Sci U S A. 2019 Jan 15;116(3):845-853. doi: 10.1073/pnas.1817041116. Epub 2018 Dec 27.

DOI:10.1073/pnas.1817041116
PMID:30591565
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6338865/
Abstract

Bacterium Argonaute (Ago; Ago) is a prokaryotic Ago (pAgo) that acts as the host defense against the uptake and propagation of foreign DNA by catalyzing the DNA cleavage reaction. The Ago active site consists of a plugged-in glutamate finger with two arginine residues (R545 and R486) located symmetrically around it. An interesting challenge is to understand how they can collaboratively facilitate enzymatic catalysis. In Ago, a eukaryotic Ago, the evolutionarily symmetrical residues are arginine and histidine, both of which function to stabilize the plugged-in catalytic tetrad conformation. Surprisingly, our simulation results indicated that, in Ago, only R545 is involved in the cleavage reaction by serving as a critical structural anchor to stabilize the catalytic tetrad Asp-Glu-Asp-Asp that is completed by the insertion of the glutamate finger, whereas R486 is not involved in target cleavage. The Ago-mediated target DNA cleavage occurs in a substrate-assisted mechanism, in which the pro-Rp (Rp, a tetrahedral phosphorus center with "R-type" chirality) oxygen of scissile phosphate acts as a general base to activate the nucleophilic water. Our unexpected theoretical findings on distinct roles played by R545 and R486 in Ago catalysis have been validated by single-point site-mutagenesis experiments, wherein the target cleavage is abolished for all mutants of R545. In sharp contrast, the cleavage activity is maintained for all mutants of R486. Our work provides mechanistic insights on the catalytic specificity of Ago proteins and could facilitate the design of new gene-editing tools in the long term.

摘要

细菌 Argonaute(Ago;Ago)是一种原核 Ago(pAgo),通过催化 DNA 切割反应,充当宿主防御以阻止外来 DNA 的摄取和传播。Ago 的活性位点由一个插入的谷氨酸手指组成,手指周围有两个精氨酸残基(R545 和 R486)对称排列。一个有趣的挑战是理解它们如何协同促进酶催化。在真核 Ago 中,进化上对称的残基是精氨酸和组氨酸,两者都有助于稳定插入的催化四联体构象。令人惊讶的是,我们的模拟结果表明,在 Ago 中,只有 R545 通过充当稳定催化四联体 Asp-Glu-Asp-Asp 的关键结构锚点参与切割反应,该四联体由谷氨酸手指的插入完成,而 R486 不参与靶切割。Ago 介导的靶 DNA 切割发生在底物辅助机制中,其中切割磷酸酯的 pro-Rp(Rp,四面体磷中心,具有“R 型”手性)氧作为广义碱激活亲核水。我们关于 R545 和 R486 在 Ago 催化中发挥不同作用的意外理论发现已通过单点定点诱变实验得到验证,其中所有 R545 突变体的靶切割均被废除。相比之下,所有 R486 突变体的切割活性都得以维持。我们的工作为 Ago 蛋白的催化特异性提供了机制见解,并可能从长远来看促进新型基因编辑工具的设计。