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Rrp5p, a trans-acting factor in yeast ribosome biogenesis, is an RNA-binding protein with a pronounced preference for U-rich sequences.

机译:Rrp5p是酵母核糖体生物发生中的反式作用因子,是一种RNA结合蛋白,对富含U的序列具有明显的偏好。

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Rrp5p is a trans-acting factor important for biogenesis of both the 40S and 60S subunit of the Saccharomyces cerevisiae ribosome. The protein contains 12 tandemly repeated S1 RNA binding motifs in its N-terminal region, suggesting the ability to interact directly with the pre-rRNA. In vitro binding studies, using immunopurified Rrp5p and in vitro transcribed, 32P-UTP-labeled RNA fragments, revealed that Rrp5p is a general RNA-binding protein with a strong preference for single-stranded sequences rich in uridines. Co-immunoprecipitation studies in yeast cells expressing ProtA-tagged Rrp5p showed that the protein is still associated with pre-ribosomal particles containing 27SA2 pre-rRNA but not with particles containing the 27SB precursor. Thus, Rrp5p appears to dissociate from the 66S pre-ribosome upon or immediately after further processing of 27SA2 pre-rRNA, suggesting the presence of (an) important binding site(s) within the 3'-terminal portion of ITS1. The location of these possible binding site(s) was further delimited using rrp2-1 mutant cells, which accumulate the 5'-extended 5.8S pre-rRNA species. The results indicate that association of Rrp5p with the pre-ribosome is abolished upon removal of a 30-nt region downstream from site A2, which contains two short, single-stranded U stretches. Sequence comparison shows that only the most 5' of these two U-rich stretches is conserved among yeast species whose ITS1 can functionally replace the S. cerevisiae spacer. The implications for the role of Rrp5p in yeast ribosome biogenesis are discussed.
机译:Rrp5p是对酿酒酵母核糖体的40S和60S亚基的生物发生很重要的反式作用因子。该蛋白在其N端区域包含12个串联重复的S1 RNA结合基序,表明可以直接与pre-rRNA相互作用。使用免疫纯化的Rrp5p和体外转录的32P-UTP标记的RNA片段进行的体外结合研究表明,Rrp5p是一种通用的RNA结合蛋白,对富含尿苷的单链序列具有强烈的偏好。在表达ProtA标签的Rrp5p的酵母细胞中进行的免疫共沉淀研究表明,该蛋白质仍与含有27SA2 pre-rRNA的核糖体前颗粒有关,但与含有27SB2前体的颗粒无关。因此,在进一步处理27SA2 pre-rRNA时或之后,Rrp5p似乎与66S前核糖体解离,表明ITS1的3'-末端部分存在一个或多个重要结合位点。这些可能的结合位点的位置使用rrp2-1突变细胞进一步定界,该细胞积累了5'延伸的5.8S pre-rRNA种类。结果表明,从位点A2下游的30 nt区域被去除后,Rrp5p与前核糖体的结合被取消,该区域包含两个短的单链U链。序列比较显示,在这两个富含U的区段中,最保守的5'在其ITS1可以功能上替代酿酒酵母间隔子的酵母物种中是保守的。讨论了Rrp5p在酵母核糖体生物发生中的作用。

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