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CRISPR-Cas 级联复合物形成 R 环的能量景观。

The energy landscape for R-loop formation by the CRISPR-Cas Cascade complex.

机构信息

Peter Debye Institute for Soft Matter Physics, Universität Leipzig, Leipzig, Germany.

Institute of Biotechnology, Life Sciences Center, Vilnius University, Vilnius, Lithuania.

出版信息

Nat Struct Mol Biol. 2023 Jul;30(7):1040-1047. doi: 10.1038/s41594-023-01019-2. Epub 2023 Jul 6.

Abstract

Clustered regularly interspaced short palindromic repeats (CRISPR) sequences and CRISPR-associated (Cas) genes comprise CIRSPR-Cas effector complexes, which have revolutionized gene editing with their ability to target specific genomic loci using CRISPR RNA (crRNA) complementarity. Recognition of double-stranded DNA targets proceeds via DNA unwinding and base pairing between crRNA and the DNA target strand, forming an R-loop structure. Full R-loop extension is a prerequisite for subsequent DNA cleavage. However, the recognition of unintended sequences with multiple mismatches has limited therapeutic applications and is still poorly understood on a mechanistic level. Here we set up ultrafast DNA unwinding experiments on the basis of plasmonic DNA origami nanorotors to study R-loop formation by the Cascade effector complex in real time, close to base-pair resolution. We resolve a weak global downhill bias of the forming R-loop, followed by a steep uphill bias for the final base pairs. We also show that the energy landscape is modulated by base flips and mismatches. These findings suggest that Cascade-mediated R-loop formation occurs on short timescales in submillisecond single base-pair steps, but on longer timescales in six base-pair intermediate steps, in agreement with the structural periodicity of the crRNA-DNA hybrid.

摘要

成簇规律间隔短回文重复序列(CRISPR)序列和 CRISPR 相关(Cas)基因组成 CRISPR-Cas 效应复合物,其使用 CRISPR RNA(crRNA)互补性靶向特定基因组位点的能力彻底改变了基因编辑。双链 DNA 靶标的识别通过 DNA 解旋和 crRNA 与 DNA 靶链之间的碱基配对进行,形成 R 环结构。完全 R 环延伸是随后 DNA 切割的前提。然而,对具有多个错配的非预期序列的识别限制了治疗应用,并且在机制水平上仍了解甚少。在这里,我们基于等离子体 DNA 折纸纳米转子建立了超快 DNA 解旋实验,以实时、接近碱基分辨率研究 Cascade 效应复合物形成的 R 环。我们解析了形成 R 环的弱全局下坡偏置,随后是最终碱基对的陡峭上坡偏置。我们还表明,能量景观受碱基翻转和错配的调节。这些发现表明,Cascade 介导的 R 环形成以亚毫秒单碱基对步骤的短时间尺度发生,但在六碱基对中间步骤以更长时间尺度发生,与 crRNA-DNA 杂交的结构周期性一致。

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