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逆转录酶-Cas1融合蛋白用于cDNA合成以及将RNA位点特异性整合到DNA基因组中的机制。

Mechanisms used for cDNA synthesis and site-specific integration of RNA into DNA genomes by a reverse transcriptase-Cas1 fusion protein.

作者信息

Mohr Georg, Yao Jun, Park Seung Kuk, Markham Laura M, Lambowitz Alan M

机构信息

Departments of Molecular Biosciences and Oncology University of Texas at Austin Austin TX, 78712.

出版信息

bioRxiv. 2023 Sep 3:2023.09.01.555893. doi: 10.1101/2023.09.01.555893.

Abstract

Reverse transcriptase-Cas1 (RT-Cas1) fusion proteins found in some CRISPR systems enable spacer acquisition from both RNA and DNA, but the mechanism of RNA spacer acquisition has remained unclear. Here, we found RT-Cas1/Cas2 adds short 3'-DNA (dN) tails to RNA protospacers enabling their direct integration into CRISPR arrays as 3'-dN-RNA/cDNA duplexes or 3'-dN-RNAs at rates comparable to similarly configured DNAs. Reverse transcription of RNA protospacers occurs by multiple mechanisms, including recently described initiation, protein priming with any dNTP, and use of short exogenous or synthesized DNA oligomer primers, enabling synthesis of cDNAs from diverse RNAs without fixed sequence requirements. The integration of 3'-dN-RNAs or single-stranded (ss) DNAs is favored over duplexes at higher protospacer concentrations, potentially relevant to spacer acquisition from abundant pathogen RNAs or ssDNA fragments generated by phage-defense nucleases. Our findings reveal novel mechanisms for site-specifically integrating RNA into DNA genomes with potential biotechnological applications.

摘要

在一些CRISPR系统中发现的逆转录酶-Cas1(RT-Cas1)融合蛋白能够从RNA和DNA中获取间隔序列,但RNA间隔序列获取的机制仍不清楚。在这里,我们发现RT-Cas1/Cas2会给RNA原间隔序列添加短的3'-DNA(dN)尾巴,使其能够以与类似配置的DNA相当的速率直接整合到CRISPR阵列中,形成3'-dN-RNA/cDNA双链体或3'-dN-RNA。RNA原间隔序列的逆转录通过多种机制发生,包括最近描述的起始、用任何dNTP进行蛋白质引发以及使用短的外源或合成DNA寡聚体引物,从而能够从各种RNA合成cDNA,而无需固定的序列要求。在较高的原间隔序列浓度下,3'-dN-RNA或单链(ss)DNA的整合比双链体更受青睐,这可能与从丰富的病原体RNA或由噬菌体防御核酸酶产生的ssDNA片段中获取间隔序列有关。我们的发现揭示了将RNA位点特异性整合到DNA基因组中的新机制,具有潜在的生物技术应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9fda/10491204/5d029d027d8c/nihpp-2023.09.01.555893v1-f0001.jpg

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