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GSP1 and GSP2, genetic suppressors of the prp20-1 mutant in Saccharomyces cerevisiae: GTP-binding proteins involved in the maintenance of nuclear organization.

机译:GSP1和GSP2,啤酒酵母中prp20-1突变体的遗传抑制剂:GTP结合蛋白,参与维持核组织。

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摘要

The temperature-sensitive mutation prp20-1 of Saccharomyces cerevisiae exhibits a pleiotropic phenotype associated with a general failure to maintain a proper organization of the nucleus. Its mammalian homolog, RCC1, is not only reported to be involved in the negative control of chromosome condensation but is also believed to assist in the coupling of DNA replication to the entry into mitosis. Recent studies on Xenopus RCC1 have strongly suggested a further role for this protein in the formation or maintenance of the DNA replication machinery. To elucidate the nature of the various components required for this PRP20 control pathway in S. cerevisiae, we undertook a search for multicopy suppressors of a prp20 thermosensitive mutant. Two genes, GSP1 and GSP2, were identified that encode almost identical polypeptides of 219 and 220 amino acids. Sequence analyses of these proteins show them to contain the ras consensus domains involved in GTP binding and metabolism. The levels of the GSP1 transcript are about 10-fold those of GSP2. As for S. cerevisiae RAS2, GSP2 expression exhibits carbon source dependency, while GSP1 expression does not. GSP1 is an essential gene, and GSP2 is not required for cell viability. We show that GSP1p is nuclear, that it can bind GTP in an in vitro assay, and finally, that a mutation in GSP1p which activates small ras-like proteins by increasing the stability of the GTP-bound form causes a dominant lethal phenotype. We believe that these two gene products may serve in regulating the activities of the multicomponent PRP20 complex.
机译:酿酒酵母的温度敏感突变prp20-1表现出多效性表型,与维持细胞核正确组织的普遍失败有关。据报道,它的哺乳动物同源物RCC1不仅参与染色体浓缩的负调控,而且还被认为有助于DNA复制与有丝分裂的结合。对非洲爪蟾RCC1的最新研究强烈暗示了这种蛋白质在DNA复制机制的形成或维持中的进一步作用。为了阐明酿酒酵母中该PRP20控制途径所需的各种组分的性质,我们进行了寻找prp20热敏突变体的多拷贝抑制剂的研究。鉴定出两个基因GSP1和GSP2,它们编码几乎相同的219和220个氨基酸的多肽。这些蛋白质的序列分析表明它们含有参与GTP结合和代谢的ras共有结构域。 GSP1转录本的水平约为GSP2的10倍。至于酿酒酵母RAS2,GSP2表达表现出碳源依赖性,而GSP1表达则没有。 GSP1是必不可少的基因,而GSP2对于细胞生存力不是必需的。我们表明GSP1p是核的,它可以在体外测定中结合GTP,最后,通过增加GTP结合形式的稳定性来激活小ras样蛋白的GSP1p中的突变会导致显性致死表型。我们认为这两个基因产物可能在调节多组分PRP20复合物的活性中起作用。

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