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Snapshots of the RNA editing machine in trypanosomes captured at different assembly stages in vivo

机译:在体内不同组装阶段捕获的锥虫中RNA编辑器的快照

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摘要

Mitochondrial pre-messenger RNAs in kinetoplastid protozoa are substrates of uridylate-specific RNA editing. RNA editing converts non-functional pre-mRNAs into translatable molecules and can generate protein diversity by alternative editing. Although several editing complexes have been described, their structure and relationship is unknown. Here, we report the isolation of functionally active RNA editing complexes by a multistep purification procedure. We show that the endogenous isolates contain two subpopulations of ∼20S and ∼35–40S and present the three-dimensional structures of both complexes by electron microscopy. The ∼35–40S complexes consist of a platform density packed against a semispherical element. The ∼20S complexes are composed of two subdomains connected by an interface. The two particles are structurally related, and we show that RNA binding is a main determinant for the interconversion of the two complexes. The ∼20S editosomes contain an RNA-binding site, which binds gRNA, pre-mRNA and gRNA/pre-mRNA hybrid molecules with nanomolar affinity. Variability analysis indicates that subsets of complexes lack or possess additional domains, suggesting binding sites for components. Together, a picture of the RNA editing machinery is provided.
机译:动素体原生动物中的线粒体前信使RNA是尿嘧啶特异性RNA编辑的底物。 RNA编辑将非功能性前mRNA转换为可翻译分子,并可以通过其他编辑产生蛋白质多样性。尽管已经描述了几种编辑复合体,但是它们的结构和关系是未知的。在这里,我们报告通过多步纯化程序分离功能活跃的RNA编辑复合体。我们表明,内源分离株包含〜20S和〜35-40S的两个亚群,并通过电子显微镜显示了两种复合物的三维结构。约35-40S的复合物由堆积在半球形元素上的平台密度组成。 〜20S复合体由通过接口连接的两个子域组成。这两个粒子在结构上是相关的,并且我们表明RNA结合是两个复合物相互转化的主要决定因素。约20S的修饰小体包含一个RNA结合位点,该结合位点以纳摩尔的亲和力结合gRNA,pre-mRNA和gRNA / pre-mRNA杂种分子。变异性分析表明,复合物的子集缺少或拥有其他域,这提示组分的结合位点。一起提供了RNA编辑机制的图片。

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