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热链球菌 III-A 型 CRISPR-Cas 系统的可编程 RNA 降解。

Programmable RNA shredding by the type III-A CRISPR-Cas system of Streptococcus thermophilus.

机构信息

Department of Protein-DNA Interactions, Institute of Biotechnology, Vilnius University, Graiciuno 8, Vilnius 02241, Lithuania.

Department of Bioinformatics, Institute of Biotechnology, Vilnius University, Graiciuno 8, Vilnius 02241, Lithuania.

出版信息

Mol Cell. 2014 Nov 20;56(4):506-17. doi: 10.1016/j.molcel.2014.09.027. Epub 2014 Nov 6.

Abstract

Immunity against viruses and plasmids provided by CRISPR-Cas systems relies on a ribonucleoprotein effector complex that triggers the degradation of invasive nucleic acids (NA). Effector complexes of type I (Cascade) and II (Cas9-dual RNA) target foreign DNA. Intriguingly, the genetic evidence suggests that the type III-A Csm complex targets DNA, whereas biochemical data show that the type III-B Cmr complex cleaves RNA. Here we aimed to investigate NA specificity and mechanism of CRISPR interference for the Streptococcus thermophilus Csm (III-A) complex (StCsm). When expressed in Escherichia coli, two complexes of different stoichiometry copurified with 40 and 72 nt crRNA species, respectively. Both complexes targeted RNA and generated multiple cuts at 6 nt intervals. The Csm3 protein, present in multiple copies in both Csm complexes, acts as endoribonuclease. In the heterologous E. coli host, StCsm restricts MS2 RNA phage in a Csm3 nuclease-dependent manner. Thus, our results demonstrate that the type III-A StCsm complex guided by crRNA targets RNA and not DNA.

摘要

CRISPR-Cas 系统提供的针对病毒和质粒的免疫依赖于一种核糖核蛋白效应复合物,该复合物触发入侵核酸(NA)的降解。I 型(Cascade)和 II 型(Cas9-双链 RNA)的效应复合物靶向外源 DNA。有趣的是,遗传证据表明,III-A 型 Csm 复合物靶向 DNA,而生化数据表明,III-B 型 Cmr 复合物切割 RNA。在这里,我们旨在研究链球菌热球菌 Csm(III-A)复合物(StCsm)的 NA 特异性和 CRISPR 干扰机制。当在大肠杆菌中表达时,两种具有不同化学计量的复合物分别与 40 和 72 nt crRNA 物种共纯化。这两种复合物都靶向 RNA,并在 6 nt 间隔处产生多个切割。Csm3 蛋白在两种 Csm 复合物中以多个拷贝存在,作为内切核酸酶。在异源大肠杆菌宿主中,StCsm 以 Csm3 核酸酶依赖的方式限制 MS2 RNA 噬菌体。因此,我们的结果表明,由 crRNA 引导的 III-A 型 StCsm 复合物靶向 RNA 而不是 DNA。

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