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酵母RAP1同源物的DNA结合与端粒长度调控

DNA binding and telomere length regulation of yeast RAP1 homologues.

作者信息

Wahlin Johan, Rosén Monika, Cohn Marita

机构信息

Department of Cell and Organism Biology, Lund University, Sölvegatan 35, S-22362 Lund, Sweden.

出版信息

J Mol Biol. 2003 Sep 26;332(4):821-33. doi: 10.1016/s0022-2836(03)00850-7.

Abstract

The repressor activator protein 1 (RAP1) has many important functions in Saccharomyces cerevisiae. At the chromosome ends, it is a negative regulator of telomere length. Here, we show that Saccharomyces castellii/Saccharomyces dairensis telomeric sequences inserted into a S.cerevisiae telomere are counted as part of the telomere, consistent with the presence of high-affinity Rap1p binding sites within these sequences. We show that S.castellii Rap1p (scasRap1p) can regulate telomere length in a S.cerevisiae strain, albeit less stringently. Cloning of the S.dairensis RAP1 homologue (sdaiRAP1) revealed that it encodes the largest RAP1 protein identified to date. Despite its large size, binding analyses of the recombinant sdaiRap1p revealed that the protein binds with the same spacing and with similar affinity to yeast telomeric sequences, as the scer- and scasRAP1 proteins. According to the Rap1p counting model for telomere length regulation, a low density of Rap1p binding sites in a telomere would result in a longer telomere in S.cerevisiae. We have compared the lengths of two individual S.dairensis telomeres and find that their lengths are not regulated to give the same number of high-affinity binding sites. This may be due to other factors than Rap1p having influence on the telomere length regulation.

摘要

阻遏激活蛋白1(RAP1)在酿酒酵母中具有许多重要功能。在染色体末端,它是端粒长度的负调节因子。在此,我们表明,插入酿酒酵母端粒中的卡氏酵母/戴尔酵母端粒序列被视为端粒的一部分,这与这些序列中存在高亲和力的Rap1p结合位点一致。我们发现卡氏酵母Rap1p(scasRap1p)能够在酿酒酵母菌株中调节端粒长度,尽管调控程度较低。戴尔酵母RAP1同源物(sdaiRAP1)的克隆显示,它编码了迄今为止鉴定出的最大的RAP1蛋白。尽管其体积较大,但重组sdaiRap1p的结合分析表明,该蛋白与酵母端粒序列的结合间距相同,亲和力也与酿酒酵母和卡氏酵母的RAP1蛋白相似。根据端粒长度调控的Rap1p计数模型,端粒中Rap1p结合位点的低密度会导致酿酒酵母中的端粒更长。我们比较了两个单独的戴尔酵母端粒的长度,发现它们的长度并未被调控为具有相同数量的高亲和力结合位点。这可能是由于除Rap1p之外的其他因素对端粒长度调控产生了影响。

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