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Transcriptional repression by Tup1–Ssn6

机译:Tup1–Ssn6抑制转录

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摘要

The Tup1–Ssn6 complex from budding yeast is one of the best studied corepressors and has served as a model for the study of similar corepressor complexes in higher eukaryotes. Tup1–Ssn6 represses multiple subsets of genes when recruited to promoters by sequence-specific DNA binding repressors. Tup1–Ssn6 mediated repression involves interactions among the corepressor and hypoacetylated histones, histone deacetylases, and the RNA transcriptional machinery. Nucleosome positioning is also involved in repression of a subset of Tup1–Ssn6 regulated genes. These findings highlight the importance of chromatin modification states in Tup1–Ssn6 mediated repression. Here we review the multiple mechanisms involved in repression and discuss Tup1–Ssn6 homolog functions in higher organisms. We also present a model for how repression by Tup1–Ssn6 may be established.
机译:出芽酵母中的Tup1-Ssn6复合物是研究最深入的核心抑制剂之一,已成为研究高等真核生物中类似核心抑制剂复合物的模型。当通过序列特异性DNA结合阻遏物募集到启动子时,Tup1-Ssn6会抑制基因的多个子集。 Tup1–Ssn6介导的阻遏作用涉及到corepressor和低乙酰化组蛋白,组蛋白脱乙酰酶和RNA转录机制之间的相互作用。核小体的定位还参与了Tup1-Ssn6调控基因的一个亚型的抑制。这些发现突出了染色质修饰状态在Tup1–Ssn6介导的阻遏中的重要性。在这里,我们回顾了参与抑制的多种机制,并讨论了高等生物中的Tup1-Ssn6同源功能。我们还提出了一个模型,说明如何建立由Tup1–Ssn6抑制。

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