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Rrd1 isomerizes RNA polymerase II in response to rapamycin

机译:Rrd1异构化对雷帕霉素的RNA聚合酶II

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Background In Saccharomyces cerevisiae, the immunosuppressant rapamycin engenders a profound modification in the transcriptional profile leading to growth arrest. Mutants devoid of Rrd1, a protein possessing in vitro peptidyl prolyl cis/trans isomerase activity, display striking resistance to the drug, although how Rrd1 activity is linked to the biological responses has not been elucidated. Results We now provide evidence that Rrd1 is associated with the chromatin and it interacts with RNA polymerase II. Circular dichroism revealed that Rrd1 mediates structural changes onto the C-terminal domain (CTD) of the large subunit of RNA polymerase II (Rpb1) in response to rapamycin, although this appears to be independent of the overall phosphorylation status of the CTD. In vitro experiments, showed that recombinant Rrd1 directly isomerizes purified GST-CTD and that it releases RNA polymerase II from the chromatin. Consistent with this, we demonstrated that Rrd1 is required to alter RNA polymerase II occupancy on rapamycin responsive genes. Conclusion We propose as a mechanism, that upon rapamycin exposure Rrd1 isomerizes Rpb1 to promote its dissociation from the chromatin in order to modulate transcription.
机译:背景技术在酿酒酵母中,雷帕霉素免疫抑制剂在转录谱上产生了深刻的改变,导致生长停滞。尽管尚未阐明Rrd1活性与生物学反应的关系,但缺少Rrd1的突变体对药物具有显着的抗药性,而Rrd1是具有体外肽基脯氨酰顺/反异构酶活性的蛋白质。结果我们现在提供证据表明Rrd1与染色质相关,并且与RNA聚合酶II相互作用。圆二色性显示Rrd1响应雷帕霉素介导RNA聚合酶II(Rpb1)的大亚基的C端结构域(CTD)的结构变化,尽管这似乎与CTD的整体磷酸化状态无关。体外实验表明,重组Rrd1直接异构化纯化的GST-CTD,并从染色质释放RNA聚合酶II。与此相符,我们证明了Rrd1是改变雷帕霉素反应基因上RNA聚合酶II占有率所必需的。结论我们提出了一种机制,即雷帕霉素暴露后Rrd1异构化Rpb1以促进其从染色质的解离,从而调节转录。

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