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RNA structure analysis of human spliceosomes reveals a compact 3D arrangement of snRNAs at the catalytic core

机译:人类剪接体的RNA结构分析显示snRNA在催化核心的紧凑3D排列

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摘要

Although U snRNAs play essential roles in splicing, little is known about the 3D arrangement of U2, U6, and U5 snRNAs and the pre-mRNA in active spliceosomes. To elucidate their relative spatial organization and dynamic rearrangement, we examined the RNA structure of affinity-purified, human spliceosomes before and after catalytic step 1 by chemical RNA structure probing. We found a stable 3-way junction of the U2/U6 snRNA duplex in active spliceosomes that persists minimally through step 1. Moreover, the formation of alternating, mutually exclusive, U2 snRNA conformations, as observed in yeast, was not detected in different assembly stages of human spliceosomal complexes (that is, B, Bact, or C complexes). Psoralen crosslinking revealed an interaction during/after step 1 between internal loop 1 of the U5 snRNA, and intron nucleotides immediately downstream of the branchpoint. Using the experimentally derived structural constraints, we generated a model of the RNA network of the step 1 spliceosome, based on the crystal structure of a group II intron through homology modelling. The model is topologically consistent with current genetic, biochemical, and structural data.
机译:尽管U snRNA在剪接中起着至关重要的作用,但对于活性剪接体中U2,U6和U5 snRNA的3D排列以及pre-mRNA知之甚少。为了阐明它们的相对空间组织和动态重排,我们通过化学RNA结构探测在催化步骤1之前和之后检查了亲和纯化的人类剪接体的RNA结构。我们在活动剪接体中发现了一个稳定的U2 / U6 snRNA双链体的三向连接,该连接在第1步中最少存在。此外,在酵母中观察到的交替,互斥的U2 snRNA构象的形成未在不同组装中检测到。剪接体复合体(即B,B act 或C复合体)的各个阶段。补骨脂素交联揭示了在步骤1期间/之后,U5 snRNA的内部环1与紧邻分支点下游的内含子核苷酸之间存在相互作用。使用实验得出的结构约束,我们通过同源建模,基于II组内含子的晶体结构,生成了第1步剪接体RNA网络的模型。该模型在拓扑上与当前的遗传,生化和结构数据一致。

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