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Cracking pre-40S ribosomal subunit structure by systematic analyses of RNA–protein cross-linking

机译:通过RNA-蛋白质交联的系统分析来破解前40S核糖体亚基的结构

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摘要

Understanding of eukaryotic ribosome synthesis has been slowed by a lack of structural data for the pre-ribosomal particles. We report rRNA-binding sites for six late-acting 40S ribosome synthesis factors, three of which cluster around the 3′ end of the 18S rRNA in model 3D structures. Enp1 and Ltv1 were previously implicated in ‘beak' structure formation during 40S maturation—and their binding sites indicate direct functions. The kinase Rio2, putative GTPase Tsr1 and dimethylase Dim1 bind sequences involved in tRNA interactions and mRNA decoding, indicating that their presence is incompatible with translation. The Dim1- and Tsr1-binding sites overlap with those of homologous Escherichia coli proteins, revealing conservation in assembly pathways. The primary binding sites for the 18S 3′-endonuclease Nob1 are distinct from its cleavage site and were unaltered by mutation of the catalytic PIN domain. Structure probing indicated that at steady state the cleavage site is likely unbound by Nob1 and flexible in the pre-rRNA. Nob1 binds before pre-rRNA cleavage, and we conclude that structural reorganization is needed to bring together the catalytic PIN domain and its target.
机译:由于缺乏核糖体前颗粒的结构数据,对真核生物核糖体合成的了解已减慢。我们报告了六个后期作用的40S核糖体合成因子的rRNA结合位点,其中三个在模型3D结构中围绕18S rRNA的3'末端簇集。 Enp1和Ltv1以前与40S成熟期间的“喙”结构形成有关,它们的结合位点表明其直接功能。激酶Rio2,推定的GTPase Tsr1和二甲基酶Dim1结合了参与tRNA相互作用和mRNA解码的序列,表明它们的存在与翻译不兼容。 Dim1和Tsr1结合位点与同源大肠杆菌蛋白重叠,揭示了组装途径中的保守性。 18S 3'-核酸内切酶Nob1的主要结合位点不同于其切割位点,并且不受催化PIN结构域突变的影响。结构探测表明,在稳定状态下,切割位点可能不受Nob1结合并且在pre-rRNA中具有柔性。 Nob1结合前rRNA切割之前,我们得出结论,需要结构重组以将催化PIN域及其靶标整合在一起。

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