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Mcm1调控酿酒酵母交配型转换中由重组增强子控制的供体偏好。

Mcm1 regulates donor preference controlled by the recombination enhancer in Saccharomyces mating-type switching.

作者信息

Wu C, Weiss K, Yang C, Harris M A, Tye B K, Newlon C S, Simpson R T, Haber J E

机构信息

Rosenstiel Center and Department of Biology, Brandeis University, Waltham, Massachusetts 02254-9110 USA.

出版信息

Genes Dev. 1998 Jun 1;12(11):1726-37. doi: 10.1101/gad.12.11.1726.

Abstract

Switching of Saccharomyces mating type by replacement of sequences at the MAT locus involves a choice between two donors, HML and HMR. MATalpha cells inhibit recombination along the entire left arm of chromosome III, including HML, whereas MATa cells activate this same region. MATa-dependent activation of HML depends on a small, cis-acting DNA sequence designated the recombination enhancer (RE), located 17 kb centromere-proximal to HML. A comparison of RE sequences interchangeable between Saccharomyces cerevisiae and Saccharomyces carlsbergensis defines a minimum RE of 244 bp. RE activity is repressed in MATalpha cells by binding of the Matalpha2-Mcm1 corepressor to a site within the RE. Mutation of the two Matalpha2 binding sites removes most, but not all, of this repression, and RE chromatin structure in MATalpha cells becomes indistinguishable from that seen in MATa. Surprisingly, a 2-bp mutation in the Mcm1 binding site completely abolishes RE activity in MATa cells; moreover, RE chromatin structure in the MATa mutant becomes very similar to that seen in MATalpha cells with a normal RE, displaying highly ordered nucleosomes despite the absence of Matalpha2. Further, a mutation that alters the ability of Mcm1 to act with Matalpha2 in repressing a-specific genes also alters donor preference in either mating type. Thus, Mcm1 is critically responsible for the activation as well as the Matalpha2-Mcm1-mediated repression of RE activity.

摘要

通过替换MAT基因座处的序列来转换酿酒酵母的交配型涉及在两个供体HML和HMR之间进行选择。MATα细胞抑制沿染色体III整个左臂的重组,包括HML,而MATa细胞激活相同区域。MATa依赖性的HML激活取决于一个小的顺式作用DNA序列,即重组增强子(RE),它位于HML着丝粒近端17 kb处。酿酒酵母和卡尔斯伯酵母之间可互换的RE序列比较确定了最小的244 bp的RE。在MATα细胞中,RE活性通过Matalpha2-Mcm1共抑制因子与RE内的一个位点结合而受到抑制。两个Matalpha2结合位点的突变消除了大部分但不是全部的这种抑制作用,并且MATα细胞中的RE染色质结构变得与MATa细胞中的无法区分。令人惊讶的是,Mcm1结合位点中的一个2 bp突变完全消除了MATa细胞中的RE活性;此外,MATa突变体中的RE染色质结构变得与具有正常RE的MATα细胞中的非常相似,尽管没有Matalpha2,但仍显示出高度有序的核小体。此外,一个改变Mcm1与Matalpha2一起抑制a特异性基因能力的突变也改变了任一交配型中的供体偏好。因此,Mcm1对于RE活性的激活以及Matalpha2-Mcm1介导的抑制至关重要。

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