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裂殖酵母中保守的Wat1/Pop3 WD重复蛋白通过微管完整性确保基因组稳定性,并且可能参与mRNA成熟。

Conserved Wat1/Pop3 WD-repeat protein of fission yeast secures genome stability through microtubule integrity and may be involved in mRNA maturation.

作者信息

Ochotorena I L, Hirata D, Kominami K, Potashkin J, Sahin F, Wentz-Hunter K, Gould K L, Sato K, Yoshida Y, Vardy L, Toda T

机构信息

Laboratory of Cell Regulation, Imperial Cancer Research Fund, London, UK.

出版信息

J Cell Sci. 2001 Aug;114(Pt 16):2911-20. doi: 10.1242/jcs.114.16.2911.

Abstract

Accurate chromosome segregation is dependent upon the integrity of mitotic spindles, which pull each pair of sister chromatids towards opposite poles. In this study, we have characterised fission yeast pop3-5235, a diploidising mutant that is impaired in genome stability. Pop3 is the same as Wat1, a conserved protein containing 7 WD repeats. Pop3/Wat1 has also been isolated from a two-hybrid screen as a binding partner to Prp2, the large subunit of the essential splicing factor U2AF. In wat1 mutants, the cellular amount of alpha-tubulin is decreased to very low levels, which results in compromised microtubules and spindles, consequently leading to unequal chromosome separation. Further analysis shows that, in spite of the binding between Wat1 and Prp2, Wat1 may not be involved directly in splicing reactions per se. Instead, we find that Wat1 is required for the maintenance of alpha-tubulin mRNA levels; moreover, transcript levels of genes other than the alpha-tubulin gene are also equally decreased in this mutant. Wild-type Wat1, but not the mutant protein, forms a large complex in the cell with several other proteins, suggesting that Wat1 functions as a structural linker in the complex. The results suggest that Wat1 plays a role in mRNA maturation as a coupling protein between splicing and synthesis and/or stabilisation.

摘要

准确的染色体分离依赖于有丝分裂纺锤体的完整性,纺锤体将每对姐妹染色单体拉向相反的两极。在本研究中,我们对裂殖酵母pop3-5235进行了表征,它是一种在基因组稳定性方面存在缺陷的二倍体化突变体。Pop3与Wat1相同,后者是一种含有7个WD重复序列的保守蛋白。Pop3/Wat1也已从双杂交筛选中分离出来,作为必需剪接因子U2AF的大亚基Prp2的结合伴侣。在wat1突变体中,α-微管蛋白的细胞含量降至极低水平,这导致微管和纺锤体受损,进而导致染色体分离不均。进一步分析表明,尽管Wat1与Prp2之间存在结合,但Wat1本身可能并不直接参与剪接反应。相反,我们发现Wat1是维持α-微管蛋白mRNA水平所必需的;此外,在该突变体中,除α-微管蛋白基因外的其他基因的转录水平也同样降低。野生型Wat1而非突变蛋白在细胞中与其他几种蛋白形成一个大的复合物,这表明Wat1在复合物中起结构连接物的作用。结果表明,Wat1作为剪接与合成和/或稳定之间的偶联蛋白,在mRNA成熟过程中发挥作用。

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