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Structural basis of Type IV CRISPR RNA biogenesis by a Cas6 endoribonuclease

机译:Cas6内衣核酸酶IV型克隆RNA生物生物发生的结构基础

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Prokaryotic CRISPR-Cas adaptive immune systems rely on small non-coding RNAs derived from CRISPR loci to recognize and destroy complementary nucleic acids. However, the mechanism of Type IV CRISPR RNA (crRNA) biogenesis is poorly understood. To dissect the mechanism of Type IV CRISPR RNA biogenesis, we determined the x-ray crystal structure of the putative Type IV CRISPR associated endoribonuclease Cas6 from Mahella australiensis (Ma Cas6-IV) and characterized its enzymatic activity with RNA cleavage assays. We show that Ma Cas6-IV specifically cleaves Type IV crRNA repeats at the 3MODIFIER LETTER PRIME side of a predicted stem loop, with a metal-independent, single-turnover mechanism that relies on a histidine and a tyrosine located within the putative endonuclease active site. Structure and sequence alignments with Cas6 orthologs reveal that although Ma Cas6-IV shares little sequence homology with other Cas6 proteins, all share common structural features that bind distinct crRNA repeat sequences. This analysis of Type IV crRNA biogenesis provides a structural and biochemical framework for understanding the similarities and differences of crRNA biogenesis across multi-subunit Class 1 CRISPR immune systems.
机译:原核Crispr-CAS自适应免疫系统依赖于衍生自Crisp锁的小非编码RNA识别和破坏互补核酸。然而,IV型CRISPRRNA(CRRNA)生物发生的机制很差。为了对IV型CRISPRRNA生物发生的机制来描述,我们确定了来自Mahella Asserraliensis(MA Cas6-IV)的推定型IV克隆相关的内衣核酸酶Cas6的X射线晶体结构,并具有RNA切割测定的酶活性。我们表明MA Cas6-IV特别切割IV型CRRNA在预测的阀杆环的3型字母主要侧重复,具有依赖于组氨酸和位于推定内切核酸酶活性位点内的组氨酸和酪氨酸的金属无关的单周转机制。 Cas6 Orthologs的结构和序列对准表明,尽管MA Cas6-IV与其他Cas6蛋白份数较少,但所有这些都共用结合不同CRRNA重复序列的常见结构特征。该分析IV型CRRNA生物发生器提供了一种结构和生化框架,用于了解CRRNA生物发生在多亚基1级CRISPR免疫系统中的相似性和差异。

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