直接分析 RNA 聚合酶 II Rpb1 C 端域上的磷酸化位点

Hyunsuk Suh, Scott B Ficarro, Un-Beom Kang, Yujin Chun, Jarrod A Marto, Stephen Buratowski
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引用次数: 0

摘要

在转录的不同阶段,聚合酶亚基 Rpb1 的 C 端结构域(CTD)上不断变化的磷酸化模式介导了 RNA 聚合酶 II 与各种 mRNA 处理和染色质修饰酶之间的动态相互作用。CTD重复七聚体序列(YSPTSPS)内的磷酸化主要通过抗体来确定,但这些抗体不能区分不同的重复序列,也不能进行比较定量。我们使用一种经质谱修饰的 CTD(msCTD)表明,Ser5-P 和 Ser2-P 出现在整个 CTD 长度上,而且比其他磷酸化位点丰富得多。从几种 CTD 激酶或磷酸酶突变的细胞中提取的 msCTD 显示了预期的磷酸化变化。此外,与封顶酶相关的 msCTD 富含 Ser5-P,而与转录终止因子 Rtt103 结合的 msCTD 则具有较高水平的 Ser2-P。这些结果表明,"CTD代码 "相对稀疏而简单。
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Direct Analysis of Phosphorylation Sites on the Rpb1 C-Terminal Domain of RNA Polymerase II.

Dynamic interactions between RNA polymerase II and various mRNA-processing and chromatin-modifying enzymes are mediated by the changing phosphorylation pattern on the C-terminal domain (CTD) of polymerase subunit Rpb1 during different stages of transcription. Phosphorylations within the repetitive heptamer sequence (YSPTSPS) of CTD have primarily been defined using antibodies, but these do not distinguish different repeats or allow comparative quantitation. Using a CTD modified for mass spectrometry (msCTD), we show that Ser5-P and Ser2-P occur throughout the length of CTD and are far more abundant than other phosphorylation sites. msCTD extracted from cells mutated in several CTD kinases or phosphatases showed the expected changes in phosphorylation. Furthermore, msCTD associated with capping enzyme was enriched for Ser5-P while that bound to the transcription termination factor Rtt103 had higher levels of Ser2-P. These results suggest a relatively sparse and simple "CTD code."

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来源期刊
Journal of Medical and Dental Sciences
Journal of Medical and Dental Sciences Dentistry-Dentistry (all)
CiteScore
0.30
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0.00%
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期刊介绍: "Journal of Medical and Dental Sciences" publishes the results of research conducted at Tokyo Medical and Dental University. The journal made its first appearance in 1954. We issue four numbers by the year.
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