首页> 美国卫生研究院文献>Nucleic Acids Research >Identification of a mammalian RNA polymerase I holoenzyme containing components of the DNA repair/replication system.
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Identification of a mammalian RNA polymerase I holoenzyme containing components of the DNA repair/replication system.

机译:鉴定包含DNA修复/复制系统组件的哺乳动物RNA聚合酶I全酶。

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摘要

Traditional models for transcription initiation by RNA polymerase I include a stepwise assembly of basic transcription factors/regulatory proteins on the core promoter to form a preinitiation complex. In contrast, we have identified a preassembled RNA polymerase I (RPI) complex that contains all the factors necessary and sufficient to initiate transcription from the rDNA promoter in vitro. The purified RPI holoenzyme contains the RPI homolog of TFIID, SL-1 and the rDNA transcription terminator factor (TTF-1), but lacks UBF, an activator of rDNA transcription. Certain components of the DNA repair/replication system, including Ku70/80, DNA topoisomerase I and PCNA, are also associated with the RPI complex. We have found that the holo-enzyme supported specific transcription and that specific transcription was stimulated by the RPI transcription activator UBF. These results support the hypothesis that a fraction of the RPI exists as a preassembled, transcriptionally competent complex that is readily recruited to the rDNA promoter, i.e. as a holoenzyme, and provide important new insights into the mechanisms governing initiation by RPI.
机译:RNA聚合酶I转录起始的传统模型包括在核心启动子上逐步组装基本转录因子/调节蛋白以形成预起始复合物。相比之下,我们已经确定了一个预组装的RNA聚合酶I(RPI)复合物,其中包含所有必要的和足够的因子,可以在体外启动rDNA启动子的转录。纯化的RPI全酶含有TFIID,SL-1和rDNA转录终止因子(TTF-1)的RPI同源物,但缺少UDNA(rDNA转录的激活剂)。 DNA修复/复制系统的某些组件,包括Ku70 / 80,DNA拓扑异构酶I和PCNA,也与RPI复合物相关。我们发现,全酶支持特异性转录,并且该特异性转录受RPI转录激活因子UBF的刺激。这些结果支持以下假设:RPI的一部分以预先组装的转录感受态复合物的形式存在,该复合物很容易被募集到rDNA启动子,即全酶,并为控制RPI引发的机制提供了重要的新见解。

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