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酵母羧基末端结构域激酶I对RNA聚合酶II羧基末端结构域的磷酸化起正向和负向调节作用。

Yeast carboxyl-terminal domain kinase I positively and negatively regulates RNA polymerase II carboxyl-terminal domain phosphorylation.

作者信息

Patturajan M, Conrad N K, Bregman D B, Corden J L

机构信息

Department of Molecular Biology and Genetics, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21205, USA.

出版信息

J Biol Chem. 1999 Sep 24;274(39):27823-8. doi: 10.1074/jbc.274.39.27823.

DOI:10.1074/jbc.274.39.27823
PMID:10488128
Abstract

Monoclonal antibodies that recognize specific carboxyl-terminal domain (CTD) phosphoepitopes were used to examine CTD phosphorylation in yeast cells lacking carboxyl-terminal domain kinase I (CTDK-I). We show that deletion of the kinase subunit CTK1 results in an increase in phosphorylation of serine in position 5 (Ser(5)) of the CTD repeat (Tyr(1)-Ser(2)-Pro(3)-Thr(4)-Ser(5)-Pro(6)-Ser(7)) during logarithmic growth. This result indicates that CTDK-I negatively regulates CTD Ser(5) phosphorylation. We also show that CTK1 deletion (ctk1Delta) eliminates the transient increase in CTD serine 2 (Ser(2)) phosphorylation observed during the diauxic shift. This result suggests that CTDK-I may play a direct role in phosphorylating CTD Ser(2) in response to nutrient depletion. Northern blot analysis was used to show that genes normally induced during the diauxic shift are not properly induced in a ctk1Delta strain. Glycogen synthase (GSY2) and cytosolic catalase (CTT1) mRNA levels increase about 10-fold in wild-type cells, but this increase is not observed in ctk1Delta cells suggesting that increased message levels may require Ser(2) phosphorylation. Heat shock also induces Ser(2) phosphorylation, but we show here that this change in CTD modification and an accompanying induction of heat shock gene expression is independent of CTDK-I. The observation that SSA3/SSA4 expression is increased in ctk1Delta cells grown at normal temperature suggests a possible role for CTDK-I in transcription repression. We discuss several possible positive and negative roles for CTDK-I in regulating CTD phosphorylation and gene expression.

摘要

利用识别特定羧基末端结构域(CTD)磷酸表位的单克隆抗体,检测缺乏羧基末端结构域激酶I(CTDK-I)的酵母细胞中的CTD磷酸化情况。我们发现,在对数生长期,激酶亚基CTK1的缺失会导致CTD重复序列(Tyr(1)-Ser(2)-Pro(3)-Thr(4)-Ser(5)-Pro(6)-Ser(7))第5位丝氨酸(Ser(5))的磷酸化增加。这一结果表明CTDK-I对CTD Ser(5)磷酸化起负调控作用。我们还发现,CTK1缺失(ctk1Δ)消除了在双相转变期间观察到的CTD丝氨酸2(Ser(2))磷酸化的短暂增加。这一结果表明,CTDK-I可能在响应营养物质耗尽时直接参与CTD Ser(2)的磷酸化。Northern印迹分析表明,在双相转变期间正常诱导的基因在ctk1Δ菌株中没有被正确诱导。糖原合酶(GSY2)和胞质过氧化氢酶(CTT1)的mRNA水平在野生型细胞中增加约10倍,但在ctk1Δ细胞中未观察到这种增加,这表明mRNA水平的增加可能需要Ser(2)磷酸化。热休克也会诱导Ser(2)磷酸化,但我们在此表明,CTD修饰的这种变化以及伴随的热休克基因表达的诱导与CTDK-I无关。在正常温度下生长的ctk1Δ细胞中SSA3/SSA4表达增加的观察结果表明CTDK-I在转录抑制中可能发挥作用。我们讨论了CTDK-I在调节CTD磷酸化和基因表达中的几种可能的正向和负向作用。

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