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Modeling and structure function analysis of the putative anchor site of yeast telomerase

机译:酵母端粒酶推定锚定位点的建模和结构功能分析

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Telomerase is a ribonucleoprotein reverse transcriptase responsible for extending one strand of the telomere terminal repeats. Unique among reverse transcriptases, telomerase is thought to possess a DNA-binding domain (known as anchor site) that allows the enzyme to add telomere repeats processively. Previous crosslinking and mutagenesis studies have mapped the anchor site to an N-terminal region of TERT, and the structure of this region of Tetrahymena TERT was recently determined at atomic resolutions. Here we use a combination of homology modeling, electrostatic calculation and site-specific mutagenesis analysis to identify a positively charged, functionally important surface patch on yeast TERT. This patch is lined by both conserved and non-conserved residues, which when mutated, caused loss of telomerase processivity in vitro and telomere shortening in vivo. In addition, we demonstrate that a point mutation in this domain of yeast TERT simultaneously enhanced the repeat addition processivity of telomerase and caused telomere elongation. Our data argue that telomerase anchor site has evolved species-specific residues to interact with species-specific telomere repeats. The data also reinforce the importance of telomerase processivity in regulating telomere length.
机译:端粒酶是核糖核蛋白逆转录酶,负责延长端粒末端重复序列的一条链。端粒酶在逆转录酶中是独一无二的,被认为具有DNA结合域(称为锚定位点),该结构域允许该酶逐步添加端粒重复序列。先前的交联和诱变研究已将锚定位点定位于TERT的N端区域,最近在原子分辨率下确定了四膜虫TERT区域的结构。在这里,我们将同源性建模,静电计算和特定位点诱变分析相结合,以鉴定酵母TERT上带正电,功能重要的表面补丁。该补丁由保守和非保守残基排列,当突​​变时,它们会导致体外的端粒酶合成能力丧失和体内的端粒缩短。另外,我们证明了在酵母TERT的该结构域中的点突变同时增强了端粒酶的重复添加持续性并引起了端粒延长。我们的数据认为端粒酶锚定位点已经进化出物种特异性残基,以与物种特异性端粒重复序列相互作用。数据还增强了端粒酶持续性在调节端粒长度中的重要性。

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