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酿酒酵母在交配型转换过程中的供体偏好取决于染色体结构和组织。

Saccharomyces cerevisiae donor preference during mating-type switching is dependent on chromosome architecture and organization.

作者信息

Coïc Eric, Richard Guy-Franck, Haber James E

机构信息

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

出版信息

Genetics. 2006 Jul;173(3):1197-206. doi: 10.1534/genetics.106.055392. Epub 2006 Apr 19.

Abstract

Saccharomyces mating-type (MAT) switching occurs by gene conversion using one of two donors, HMLalpha and HMRa, located near the ends of the same chromosome. MATa cells preferentially choose HMLalpha, a decision that depends on the recombination enhancer (RE) that controls recombination along the left arm of chromosome III (III-L). When RE is inactive, the two chromosome arms constitute separate domains inaccessible to each other; thus HMRa, located on the same arm as MAT, becomes the default donor. Activation of RE increases HMLalpha usage, even when RE is moved 50 kb closer to the centromere. If MAT is inserted into the same domain as HML, RE plays little or no role in activating HML, thus ruling out any role for RE in remodeling the silent chromatin of HML in regulating donor preference. When the donors MAT and RE are moved to chromosome V, RE increases HML usage, but the inaccessibility of HML without RE apparently depends on other chromosome III-specific sequences. Similar conclusions were reached when RE was placed adjacent to leu2 or arg4 sequences engaged in spontaneous recombination. We propose that RE's targets are anchor sites that tether chromosome III-L in MATalpha cells thus reducing its mobility in the nucleus.

摘要

酿酒酵母交配型(MAT)转换通过基因转换发生,使用位于同一条染色体末端附近的两个供体之一,即HMLα和HMRa。MATa细胞优先选择HMLα,这一决定取决于重组增强子(RE),它控制着沿着第三条染色体左臂(III-L)的重组。当RE失活时,两条染色体臂构成彼此无法进入的独立结构域;因此,位于与MAT同一条臂上的HMRa成为默认供体。RE的激活增加了HMLα的使用频率,即使RE被移至距离着丝粒更近50 kb的位置。如果MAT被插入到与HML相同的结构域中,RE在激活HML方面几乎不发挥作用或根本不起作用,因此排除了RE在调节供体偏好时重塑HML沉默染色质方面的任何作用。当供体MAT和RE被转移到第五条染色体上时,RE增加了HML的使用频率,但没有RE时HML的不可接近性显然取决于第三条染色体上的其他特定序列。当RE与参与自发重组的leu2或arg4序列相邻放置时,也得出了类似的结论。我们提出,RE的靶点是在MATα细胞中束缚III-L染色体的锚定位点,从而降低其在细胞核中的移动性。

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