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Assembly of ribosomes and spliceosomes: complex ribonucleoprotein machines

机译:核糖体和剪接体的组装:复杂的核糖核蛋白机器

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摘要

Ribosomes and spliceosomes are ribonucleoprotein nanomachines that catalyze translation of mRNA to synthesize proteins and splicing of introns from pre-mRNAs, respectively. Assembly of ribosomes involves more than 300 proteins and RNAs, and that of spliceosomes over 100 proteins and RNAs. Construction of these enormous ribonucleoprotein particles (RNPs) is a dynamic process, in which the nascent RNPs undergo numerous ordered rearrangements of RNA-RNA, RNA-protein, and protein-protein interactions. Here we outline similar principles that have emerged from studies of ribosome and spliceosome assembly. Constituents of both RNPs form subassembly complexes, which can simplify the task of assembly and segregate functions of assembly factors. Reorganization of RNP topology, and proofreading of proper assembly, are catalyzed by protein- or RNA-dependent ATPases or GTPases. Dynamics of intermolecular interactions may be facilitated or regulated by cycles of post-translational modifications. Despite this repertoire of tools, mistakes occur in RNP assembly or in processing of RNA substrates. Quality control mechanisms recognize and turnover misassembled RNPs and reject improper substrates.
机译:核糖体和剪接体是核糖核蛋白纳米机器,它们分别催化mRNA的翻译以合成蛋白质和剪接pre-mRNA的内含子。核糖体的组装涉及300多种蛋白质和RNA,剪接体的组装涉及100多种蛋白质和RNA。这些巨大的核糖核蛋白颗粒(RNP)的构建是一个动态过程,其中新生的RNP经历了RNA-RNA,RNA-蛋白质和蛋白质-蛋白质相互作用的许多有序重排。在这里,我们概述了从核糖体和剪接体组装研究中出现的相似原理。两个RNP的组成都形成子装配体,可以简化装配任务并分离装配因子的功能。 RNP拓扑结构的重组和正确装配的校对,是由蛋白质或RNA依赖的ATPase或GTPases催化的。分子间相互作用的动力学可以通过翻译后修饰的循环来促进或调节。尽管使用了这些工具,但在RNP组装或RNA底物处理中仍会出现错误。质量控制机制可以识别和转换组装不正确的RNP,并拒绝不适当的基材。

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