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首页> 外文期刊>Eukaryotic cell >Normal Telomere Length Maintenance in Saccharomyces cerevisiae Requires Nuclear Import of the Ever Shorter Telomeres 1 (Est1) Protein via the Importin Alpha Pathway
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Normal Telomere Length Maintenance in Saccharomyces cerevisiae Requires Nuclear Import of the Ever Shorter Telomeres 1 (Est1) Protein via the Importin Alpha Pathway

机译:酿酒酵母中的正常端粒长度维持需要通过Importin Alpha途径核导入越来越短的端粒1(Est1)蛋白。

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The Est1 (ever shorter telomeres 1) protein is an essential component of yeast telomerase, a ribonucleoprotein complex that restores the repetitive sequences at chromosome ends (telomeres) that would otherwise be lost during DNA replication. Previous work has shown that the telomerase RNA component (TLC1) transits through the cytoplasm during telomerase biogenesis, but mechanisms of protein import have not been addressed. Here we identify three nuclear localization sequences (NLSs) in Est1p. Mutation of the most N-terminal NLS in the context of full-length Est1p reduces Est1p nuclear localization and causes telomere shortening—phenotypes that are rescued by fusion with the NLS from the simian virus 40 (SV40) large-T antigen. In contrast to that of the TLC1 RNA, Est1p nuclear import is facilitated by Srp1p, the yeast homolog of importin α. The reduction in telomere length observed at the semipermissive temperature in a srp1 mutant strain is rescued by increased Est1p expression, consistent with a defect in Est1p nuclear import. These studies suggest that at least two nuclear import pathways are required to achieve normal telomere length homeostasis in yeast.
机译:Est1(端粒越短越好)蛋白是酵母端粒酶的必不可少的成分,端粒酶是一种核糖核蛋白复合物,可恢复染色体末端的重复序列(端粒),否则在DNA复制过程中会丢失。先前的研究表明,端粒酶生物发生过程中端粒酶RNA组分( TLC1 )穿过细胞质,但蛋白质的导入机制尚未得到解决。在这里,我们确定Est1p中的三个核定位序列(NLSs)。在全长Est1p的情况下,最N末端NLS的突变会降低Est1p的核定位,并导致端粒缩短-通过与猿猴病毒40(SV40)大T抗原的NLS融合而挽救的表型。与 TLC1 RNA相比,Est1p的核导入由导入蛋白α的酵母同源物Srp1p促进。通过增加Est1p表达来挽救在 srp1 突变菌株中半容许温度下端粒长度的减少,这与Est1p核输入的缺陷相一致。这些研究表明,至少需要两个核输入途径才能在酵母中实现正常的端粒长度稳态。

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