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Investigating the role of the Est3 protein in yeast telomere replication.

机译:研究Est3蛋白在酵母端粒复制中的作用。

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摘要

The Est3 subunit of yeast telomerase, which adopts a predicted OB-fold, is essential for telomere replication. To assess the possible contributions that Est3 might make to enzyme catalysis, we compared telomerase activity from wild type and est3-Delta strains of Saccharomyces castellii, which revealed that loss of the Est3 subunit results in a 2- to 3-fold decline in nucleotide addition. This effect was not primer-specific, based on assessment of a panel of primers that spanned the template of the S. castellii telomerase RNA. Furthermore, using nuclear magnetic resonance chemical shift perturbation, no chemical shift change was observed at any site in the protein upon addition of single-stranded DNA, arguing against a role for Est3 in recognition of telomeric substrates by telomerase. Addition of exogenous Est3 protein, including mutant Est3 proteins that are severely impaired for telomere replication in vivo, fully restored activity in est3-Delta telomerase reactions. Thus, Est3 performs an in vivo regulatory function in telomere replication, which is distinct from any potential contribution that Est3 might make to telomerase activity.
机译:酵母端粒酶的Est3亚基采用预测的OB倍数,对于端粒复制至关重要。为了评估Est3可能对酶催化做出的贡献,我们比较了野生型和酿酒酵母cast3-的est3-Delta菌株的端粒酶活性,这表明Est3亚基的丢失导致核苷酸添加量下降了2到3倍。 。根据对跨越卡氏链球菌端粒酶RNA模板的一组引物的评估,该效应不是引物特异性的。此外,使用核磁共振化学位移扰动,在添加单链DNA后在蛋白质的任何位点均未观察到化学位移变化,这与Est3端粒酶识别端粒底物的作用相反。外源Est3蛋白的添加,包括在体内端粒复制受到严重损害的突变Est3蛋白,可完全恢复est3-Delta端粒酶反应的活性。因此,Est3在端粒复制中执行体内调节功能,这与Est3可能对端粒酶活性做出的任何潜在贡献不同。

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