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首页> 外文期刊>RNA >A conserved Lsm-interaction motif in Prp24 required for efficient U4/U6 di-snRNP formation.
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A conserved Lsm-interaction motif in Prp24 required for efficient U4/U6 di-snRNP formation.

机译:有效U4 / U6 di-snRNP形成所需的Prp24中保守的Lsm相互作用基序。

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摘要

The assembly of the U4 and U6 snRNPs into the U4/U6 di-snRNP is necessary for pre-mRNA splicing, and in Saccharomyces cerevisiae requires the splicing factor Prp24. We have identified a family of Prp24 homologs that includes the human protein SART3/p110nrb, which had been identified previously as a surface antigen in several cancers. Sequence conservation among the Prp24 homologs reveals the existence of a fourth previously unidentified RNA recognition motif (RRM) in Prp24, which we demonstrate is necessary for growth of budding yeast at 37 degrees C. The family is also characterized by a highly conserved 12-amino-acid motif at the extreme C terminus. Deletion of this motif in Prp24 causes a cold-sensitive growth phenotype and a decrease in base-paired U4/U6 levels in vivo. The mutant protein also has a reduced association with U6 snRNA in extract, and is unable to interact with the U6 Lsm proteins by two-hybrid assay. In vitro annealing assays demonstrate that deletion of the motif causes a defect in U4/U6 formation by reducing binding of Prp24 to its substrate. We conclude that the conserved C-terminal motif of Prp24 interacts with the Lsm proteins to promote U4/U6 formation.
机译:U4和U6 snRNPs组装到U4 / U6 di-snRNP中对于进行mRNA前剪接是必需的,在酿酒酵母中,需要剪接因子Prp24。我们已经鉴定出一个包括人类蛋白SART3 / p110nrb的Prp24同源物家族,该蛋白先前已被鉴定为几种癌症中的表面抗原。 Prp24同源物之间的序列保守性揭示了Prp24中存在第四个先前未鉴定的RNA识别基序(RRM),我们证明了这对于37℃下萌芽酵母的生长是必需的。该家族还具有高度保守的12-氨基极端C末端的酸性基序。 Prp24中此基序的删除会导致感冒敏感的生长表型和体内的碱基配对U4 / U6水平降低。突变蛋白在提取物中与U6 snRNA的结合也减少,并且无法通过双杂交法与U6 Lsm蛋白相互作用。体外退火试验表明,基序的缺失通过减少Prp24与其底物的结合而导致U4 / U6形成缺陷。我们得出结论,Prp24的保守C端基序与Lsm蛋白相互作用,以促进U4 / U6的形成。

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