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酵母RME1基因编码一种假定的锌指蛋白,该蛋白直接受a1 - α2抑制。

The yeast RME1 gene encodes a putative zinc finger protein that is directly repressed by a1-alpha 2.

作者信息

Covitz P A, Herskowitz I, Mitchell A P

机构信息

Institute of Cancer Research, Columbia University, New York, New York 10032.

出版信息

Genes Dev. 1991 Nov;5(11):1982-9. doi: 10.1101/gad.5.11.1982.

Abstract

In the yeast Saccharomyces cerevisiae, a/alpha cells can enter meiosis whereas a and alpha cells cannot. The a/alpha cell type is determined by presence of a repressor, a1-alpha 2. Previous studies indicate that a/alpha cells lack an inhibitor of meiosis, the RME1 gene product, and that a and alpha cells express RME1. We report here the sequence of RME1 and functional analysis of its regulatory and coding regions. The 5'-region of RME1 includes a sequence resembling a1-alpha 2 repression sites. Deletion of this site at RME1 relieves repression by a1-alpha 2, and insertion of the site into a heterologous regulatory region (CYC1) confers weak repression in a/alpha cells. These observations indicate that RME1 is directly repressed by a1-alpha 2. The RME1 product has three regions that resemble C2H2 zinc fingers, which are characteristic of a class of nucleic-acid-binding proteins. Substitution of serine for cysteine in each of the putative fingers abolishes RME1 function; serine substitutions in the second and third putative fingers do not affect RME1 stability. These findings indicate that at least two putative zinc fingers are critical for RME1 structure or activity. Therefore RME1, which is formally a negative regulator of the meiotic gene IME1, may act directly as a repressor.

摘要

在酿酒酵母中,a/α细胞可以进入减数分裂,而a细胞和α细胞则不能。a/α细胞类型由一种阻遏物a1-α2的存在决定。先前的研究表明,a/α细胞缺乏减数分裂抑制剂RME1基因产物,而a细胞和α细胞表达RME1。我们在此报告RME1的序列及其调控区和编码区的功能分析。RME1的5'区域包含一个类似于a1-α2阻遏位点的序列。在RME1处删除该位点可解除a1-α2的阻遏作用,而将该位点插入异源调控区(CYC1)可在a/α细胞中产生弱阻遏作用。这些观察结果表明RME1直接受到a1-α2的阻遏。RME1产物有三个类似于C2H2锌指的区域,这是一类核酸结合蛋白的特征。在每个假定的锌指中将半胱氨酸替换为丝氨酸会消除RME1的功能;在第二个和第三个假定的锌指中进行丝氨酸替换不会影响RME1的稳定性。这些发现表明至少两个假定的锌指对RME1的结构或活性至关重要。因此,RME1虽然正式上是减数分裂基因IME1的负调控因子,但可能直接作为阻遏物起作用。

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