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Structural basis for dimer formation of the CRISPR-associated protein Csm2 of Thermotoga maritima

机译:滨海嗜热菌的CRISPR相关蛋白Csm2二聚体形成的结构基础

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The clusters of regularly interspaced short palindromic repeats (CRISPR) and the Cas (CRISPR-associated) proteins form an adaptive immune system in bacteria and archaea that evolved as an RNA-guided interference mechanism to target and degrade foreign genetic elements. In the so-called type IIIA CRISPR-Cas systems, Cas proteins from the Csm family form a complex of RNPs that are involved in surveillance and targeting tasks. In the present study, we report the crystal structure of Thermotoga maritima Csm2. This protein is considered to assemble into the helically shaped Csm RNP complex in a site opposite to the CRISPR RNA binding backbone. Csm2 was solved via cadmium single wavelength anomalous diffraction phasing at 2.4 angstrom resolution. The structure reveals that Csm2 is composed of a large 42 amino-acid long -helix flanked by three shorter -helices. The structure also shows that the protein is capable of forming dimers mainly via an extensive contact surface conferred by its long -helix. This interaction is further stabilized by the N-terminal helix, which is inserted into the C-terminal helical portion of the adjacent subunit. The dimerization of Csm2 was additionally confirmed by size exclusion chromatography of the pure recombinant protein followed by MS analysis of the eluted fractions. Because of its role in the assembly and functioning of the Csm CRISPR RNP complex, the crystal structure of Csm2 is of great importance for clarifying the mechanism of action of the subtype IIIA CRISPR-Cas system, as well as the similarities and diversities between the different CRISPR-Cas system.
机译:规则间隔的短回文重复序列(CRISPR)和Cas(CRISPR相关)蛋白簇在细菌和古细菌中形成了一种适应性免疫系统,其进化为RNA导向的干扰机制,可靶向和降解外源遗传元件。在所谓的IIIA型CRISPR-Cas系统中,Csm家族的Cas蛋白形成RNP的复合体,参与监视和靶向任务。在本研究中,我们报告了Thermotoga maritima Csm2的晶体结构。该蛋白被认为在与CRISPR RNA结合骨架相反的位点组装成螺旋形的Csm RNP复合物。通过镉单波长异常衍射定相为2.4埃,可解决Csm2的问题。结构表明,Csm2由一个大的42个氨基酸长螺旋组成,两侧是三个短螺旋。该结构还表明,该蛋白质能够主要通过其长螺旋赋予的广泛接触表面形成二聚体。这种相互作用通过插入相邻亚基的C末端螺旋部分的N末端螺旋进一步稳定。 Csm2的二聚化还通过纯重组蛋白的尺寸排阻色谱,然后对洗脱级分进行MS分析来确认。由于其在Csm CRISPR RNP复合体的组装和功能中的作用,Csm2的晶体结构对于阐明IIIA型CRISPR-Cas系统的作用机理以及不同之间的相似性和多样性非常重要。 CRISPR-Cas系统。

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