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Target RNA capture and cleavage by the Cmr type III-B CRISPR–cas effector complex

机译:通过Cmr III-B型CRISPR–cas效应复合物捕获和切割靶RNA

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The effector complex of the Cmr/type III-B CRISPR (clustered regularly interspaced short palindromic repeat)–Cas (CRISPR-associated) system cleaves RNAs recognized by the CRISPR RNA (crRNA) of the complex and includes six protein subunits of unknown functions. Using reconstituted Pyrococcus furiosus Cmr complexes, we found that each of the six Cmr proteins plays a critical role in either crRNA interaction or target RNA capture. Cmr2, Cmr3, Cmr4, and Cmr5 are all required for formation of a crRNA-containing complex detected by native gel electrophoresis, and the conserved 5′ repeat sequence tag and 5′-OH group of the crRNA are essential for the interaction. Interestingly, capture of the complementary target RNA additionally requires both Cmr1 and Cmr6. In detailed functional studies, we determined that P. furiosus Cmr complexes cleave target RNAs at 6-nucleotide (nt) intervals in the region of complementarity, beginning 5 nt downstream from the crRNA tag and continuing to within ~14 nt of the 3′ end of the crRNA. Our findings indicate that Cmr3 recognizes the signature crRNA tag sequence (and depends on protein–protein interactions with Cmr2, Cmr4, and Cmr5), each Cmr4 subunit mediates a target RNA cleavage, and Cmr1 and Cmr6 mediate an essential interaction between the 3′ region of the crRNA and the target RNA.
机译:Cmr / III-B CRISPR(成簇的规则间隔的短回文重复序列)–Cas(CRISPR相关)系统的效应复合物切割复合物的CRISPR RNA(crRNA)识别的RNA,并包含功能未知的六个蛋白亚基。使用重构的激烈热球菌Cmr复合物,我们发现六个Cmr蛋白中的每一个在crRNA相互作用或靶RNA捕获中都起着关键作用。 Cmr2,Cmr3,Cmr4和Cmr5都是通过天然凝胶电泳检测到的含有crRNA的复合物的形成所必需的,crRNA的保守5'重复序列标签和5'-OH基对于相互作用至关重要。有趣的是,互补靶RNA的捕获还需要Cmr1和Cmr6。在详细的功能研究中,我们确定了P. furiosus Cmr复合物在互补区域以6个核苷酸(nt)的间隔切割靶RNA,从crRNA标签的下游5 nt开始,一直延伸到3'末端的〜14 nt之内。 crRNA。我们的发现表明,Cmr3识别特征性crRNA标签序列(并取决于与Cmr2,Cmr4和Cmr5的蛋白质​​-蛋白质相互作用),每个Cmr4亚基介导目标RNA切割,而Cmr1和Cmr6介导3'区域之间的基本相互作用。 crRNA和目标RNA的序列。

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