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Alternative Chromatin Structures of the 35S rRNA Genes in Saccharomyces cerevisiae Provide a Molecular Basis for the Selective Recruitment of RNA Polymerases I and II▿

机译:酿酒酵母中35S rRNA基因的替代染色质结构为RNA聚合酶I和II的选择性招募提供了分子基础

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摘要

In all eukaryotes, a specialized enzyme, RNA polymerase I (Pol I), is dedicated to transcribe the 35S rRNA gene from a multicopy gene cluster, the ribosomal DNA (rDNA). In certain Saccharomyces cerevisiae mutants, 35S rRNA genes can be transcribed by RNA polymerase II (Pol II). In these mutants, rDNA silencing of Pol II transcription is impaired. It has been speculated that upstream activating factor (UAF), which binds to a specific DNA element within the Pol I promoter, plays a crucial role in forming chromatin structures responsible for polymerase specificity and silencing at the rDNA locus. We therefore performed an in-depth analysis of chromatin structure and composition in different mutant backgrounds. We demonstrate that chromatin architecture of the entire Pol I-transcribed region is substantially altered in the absence of UAF, allowing RNA polymerases II and III to access DNA elements flanking a Pol promoter-proximal Reb1 binding site. Furthermore, lack of UAF leads to the loss of Sir2 from rDNA, correlating with impaired Pol II silencing. This analysis of rDNA chromatin provides a molecular basis, explaining many phenotypes observed in previous genetic analyses.
机译:在所有真核生物中,一种专门的酶RNA聚合酶I(Pol I)致力于从多拷贝基因簇,核糖体DNA(rDNA)中转录35S rRNA基因。在某些酿酒酵母突变体中,35S rRNA基因可以被RNA聚合酶II(Pol II)转录。在这些突变体中,Pol II转录的rDNA沉默受损。已经推测,与Pol I启动子内的特定DNA元件结合的上游活化因子(UAF)在形成负责聚合酶特异性和在rDNA基因座处沉默的染色质结构中起着至关重要的作用。因此,我们对不同突变体背景下的染色质结构和组成进行了深入分析。我们证明了在没有UAF的情况下,整个Pol I转录区域的染色质结构发生了实质性变化,从而允许RNA聚合酶II和III访问位于Pol启动子附近Reb1结合位点两侧的DNA元件。此外,缺乏UAF会导致rDNA缺失Sir2,这与Pol II沉默受损有关。对rDNA染色质的这种分析提供了分子基础,解释了在先前的遗传分析中观察到的许多表型。

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