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首页> 外文期刊>Nucleic Acids Research >Functional domains of the 50S subunit mature late in the assembly process
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Functional domains of the 50S subunit mature late in the assembly process

机译:50S亚基的功能域在组装过程中成熟

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摘要

Despite the identification of many factors that facilitate ribosome assembly, the molecular mechanisms by which they drive ribosome biogenesis are poorly understood. Here, we analyze the late stages of assembly of the 50S subunit using Bacillus subtilis cells depleted of RbgA, a highly conserved GTPase. We found that RbgA-depleted cells accumulate late assembly intermediates bearing sub-stoichiometric quantities of ribosomal proteins L16, L27, L28, L33a, L35 and L36. Using a novel pulse labeling/quantitative mass spectrometry technique, we show that this particle is physiologically relevant and is capable of maturing into a complete 50S particle. Cryo-electron microscopy and chemical probing revealed that the central protuberance, the GTPase associating region and tRNA-binding sites in this intermediate are unstructured. These findings demonstrate that key functional sites of the 50S subunit remain unstructured until late stages of maturation, preventing the incomplete subunit from prematurely engaging in translation. Finally, structural and biochemical analysis of a ribosome particle depleted of L16 indicate that L16 binding is necessary for the stimulation of RbgA GTPase activity and, in turn, release of this co-factor, and for conversion of the intermediate to a complete 50S subunit.
机译:尽管已鉴定出许多促进核糖体组装的因素,但人们对它们驱动核糖体生物发生的分子机制了解甚少。在这里,我们使用枯草芽孢杆菌细胞耗尽RbgA(一种高度保守的GTP酶)来分析50S亚基装配的后期阶段。我们发现,耗尽RbgA的细胞积聚具有亚化学计量量的核糖体蛋白L16,L27,L28,L33a,L35和L36的后期组装中间体。使用一种新颖的脉冲标记/定量质谱技术,我们表明该粒子具有生理相关性,并且能够成熟为一个完整的50S粒子。低温电子显微镜和化学探测表明,该中间体的中央突起,GTPase结合区和tRNA结合位点是无结构的。这些发现表明,50S亚基的关键功能位点保持未结构化直至成熟后期,从而防止了不完全的亚基过早地参与翻译。最后,对耗尽了L16的核糖体颗粒的结构和生化分析表明,L16结合对于刺激RbgA GTPase活性,进而释放该辅因子以及将中间体转化为完整的50S亚基是必需的。

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