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Ribosomal proteins Rps0 and Rps21 of Saccharomyces cerevisiae have overlapping functions in the maturation of the 3' end of 18S rRNA

机译:酿酒酵母的核糖体蛋白Rps0和Rps21在18S rRNA 3'端的成熟中具有重叠功能

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摘要

The Rps0 proteins of Saccharomyces cerevisiae are components of the 40S ribosomal subunit required for maturation of the 3' end of 18S rRNA. Drosophila and human homologs of the Rps0 proteins physically interact with Rps21 proteins, and decreased expression of both proteins in Drosophila impairs control of cellular proliferation in hematopoietic organs during larval development. Here, we characterize the yeast RPS21A/B genes and show that strains where both genes are disrupted are not viable. Relative to the wild type, cells with disrupted RPS21A or RPS21B genes exhibit a reduction in growth rate, a decrease in free 40S subunits, an increase in the amount of free 60S subunits, and a decrease in polysome size. Ribosomal RNA processing studies reveal RPS21 and RPS0 mutants have virtually identical processing defects. The pattern of processing defects observed in RPS0 and RPS21 mutants is not a general characteristic of strains with suboptimal levels of small subunit ribosomal proteins, since disruption of the RPS18A or RPS18B genes results in related but distinct processing defects. Together, these data link the Rps0 and Rps21 proteins together functionally in promoting maturation of the 3' end of 18S rRNA and formation of active 40S ribosomal subunits.
机译:酿酒酵母的Rps0蛋白是18S rRNA 3'末端成熟所需的40S核糖体亚基的组成部分。果蝇和Rps0蛋白的人类同源物在物理上与Rps21蛋白相互作用,果蝇中这两种蛋白的表达降低会削弱幼虫发育过程中造血器官中细胞增殖的控制。在这里,我们表征了酵母RPS21A / B基因,并表明两个基因都被破坏的菌株是不可行的。相对于野生型,具有RPS21A或RPS21B基因被破坏的细胞表现出生长速率的降低,游离40S亚基的减少,游离60S亚基的数量的增加和多核糖体大小的减小。核糖体RNA加工研究表明,RPS21和RPS0突变体实际上具有相同的加工缺陷。在RPS0和RPS21突变体中观察到的加工缺陷模式不是具有亚最佳水平的小亚基核糖体蛋白的菌株的一般特征,因为RPS18A或RPS18B基因的破坏会导致相关但明显的加工缺陷。总之,这些数据将Rps0和Rps21蛋白在功能上联系在一起,以促进18S rRNA 3'端的成熟和活性40S核糖体亚基的形成。

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