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Rap1蛋白与端粒结构调控酿酒酵母中的端粒位置效应。

RAP1 and telomere structure regulate telomere position effects in Saccharomyces cerevisiae.

作者信息

Kyrion G, Liu K, Liu C, Lustig A J

机构信息

Molecular Biology Program, Sloan-Kettering Institute, New York, New York.

出版信息

Genes Dev. 1993 Jul;7(7A):1146-59. doi: 10.1101/gad.7.7a.1146.

Abstract

To investigate the role of the yeast telomere-, silencing-, and UAS-binding protein RAP1 in telomere position effects, we have characterized two sets of mutant cells: (1) a set of rap1 alleles (termed the rap1t alleles) that produce truncated RAP1 proteins missing the carboxy-terminal 144-165 amino acids; and (2) null mutants of the RIF1 gene, encoding a protein capable of interaction with the carboxyl terminus of RAP1. The data presented here indicate that loss of the carboxyl terminus of RAP1 abolishes position effects at yeast telomeres and diminishes silencing at the HML locus. Elimination of position effects in these cells is associated with increased accessibility to the Escherichia coli dam methylase in vivo. Thus, the carboxy-terminal domain of RAP1 is required for telomere position effects. In contrast, rif1 deletion alleles increase the frequency of repressed cells. Using the rap1t alleles to generate wild-type cells differing only in telomere tract lengths, we also show that telomere position effects are highly sensitive to changes in the size (or structure) of the telomeric tract. Longer poly(G1-3T) tracts can increase the frequency of transcriptional repression at the telomere, suggesting that telomeric poly(G1-3T) tracts play an active role in the formation or stability of subtelomeric transcriptional states.

摘要

为了研究酵母端粒、沉默及UAS结合蛋白RAP1在端粒位置效应中的作用,我们鉴定了两组突变细胞:(1)一组rap1等位基因(称为rap1t等位基因),其产生缺失羧基末端144 - 165个氨基酸的截短型RAP1蛋白;(2)RIF1基因的缺失突变体,该基因编码一种能够与RAP1羧基末端相互作用的蛋白。本文给出的数据表明,RAP1羧基末端的缺失消除了酵母端粒处的位置效应,并减弱了HML位点的沉默作用。这些细胞中位置效应的消除与体内对大肠杆菌dam甲基化酶的可及性增加有关。因此,RAP1的羧基末端结构域是端粒位置效应所必需的。相反,rif1缺失等位基因增加了受抑制细胞的频率。利用rap1t等位基因产生仅端粒序列长度不同的野生型细胞,我们还表明端粒位置效应对端粒序列大小(或结构)的变化高度敏感。更长的聚(G1 - 3T)序列可增加端粒处转录抑制的频率,这表明端粒聚(G1 - 3T)序列在亚端粒转录状态的形成或稳定性中发挥积极作用。

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