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Hierarchical recruitment of ribosomal proteins and assembly factors remodels nucleolar pre-60S ribosomes

机译:核糖体蛋白和组装因子的分级募集重塑核仁60S前核糖体

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摘要

Ribosome biogenesis involves numerous preribosomal RNA (pre-rRNA) processing events to remove internal and external transcribed spacer sequences, ultimately yielding three mature rRNAs. Removal of the internal transcribed spacer 2 spacer RNA is the final step in large subunit pre-rRNA processing and begins with endonucleolytic cleavage at the C2 site of 27SB pre-rRNA. C2 cleavage requires the hierarchical recruitment of 11 ribosomal proteins and 14 ribosome assembly factors. However, the function of these proteins in C2 cleavage remained unclear. In this study, we have performed a detailed analysis of the effects of depleting proteins required for C2 cleavage and interpreted these results using cryo–electron microscopy structures of assembling 60S subunits. This work revealed that these proteins are required for remodeling of several neighborhoods, including two major functional centers of the 60S subunit, suggesting that these remodeling events form a checkpoint leading to C2 cleavage. Interestingly, when C2 cleavage is directly blocked by depleting or inactivating the C2 endonuclease, assembly progresses through all other subsequent steps.
机译:核糖体的生物发生涉及许多核糖体前RNA(pre-rRNA)处理事件,以去除内部和外部转录的间隔区序列,最终产生三个成熟的rRNA。内部转录间隔区2间隔区RNA的去除是大亚基pre-rRNA加工的最后一步,始于27SB pre-rRNA的C2位点的内切核酸酶切。 C2裂解需要11种核糖体蛋白和14种核糖体装配因子的分级募集。但是,这些蛋白在C2裂解中的功能仍不清楚。在这项研究中,我们对消耗C2裂解所需的蛋白质的效果进行了详细分析,并使用组装60S亚基的低温电子显微镜结构解释了这些结果。这项工作表明,这些蛋白质是几个邻域重塑所必需的,包括60S亚基的两个主要功能中心,表明这些重塑事件形成了导致C2裂解的检查点。有趣的是,当通过消耗或灭活C2核酸内切酶直接阻止C2裂解时,组装将继续进行所有其他后续步骤。

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