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TFIID的多个Taf亚基与Ino2激活域相互作用,并有助于酵母磷脂生物合成所需基因的表达。

Multiple Taf subunits of TFIID interact with Ino2 activation domains and contribute to expression of genes required for yeast phospholipid biosynthesis.

作者信息

Hintze Stefan, Engelhardt Maike, van Diepen Laura, Witt Eric, Schüller Hans-Joachim

机构信息

Institut für Genetik und Funktionelle Genomforschung, Ernst-Moritz-Arndt-Universität Greifswald, Jahnstrasse 15a, D-17487 Greifswald, Germany.

出版信息

Mol Microbiol. 2017 Dec;106(6):876-890. doi: 10.1111/mmi.13850. Epub 2017 Oct 17.

DOI:10.1111/mmi.13850
PMID:28994223
Abstract

Expression of phospholipid biosynthetic genes in yeast requires activator protein Ino2 which can bind to the UAS element inositol/choline-responsive element (ICRE) and trigger activation of target genes, using two separate transcriptional activation domains, TAD1 and TAD2. However, it is still unknown which cofactors mediate activation by TADs of Ino2. Here, we show that multiple subunits of basal transcription factor TFIID (TBP-associated factors Taf1, Taf4, Taf6, Taf10 and Taf12) are able to interact in vitro with activation domains of Ino2. Interaction was no longer observed with activation-defective variants of TAD1. We were able to identify two nonoverlapping regions in the N-terminus of Taf1 (aa 1-100 and aa 182-250) each of which could interact with TAD1 of Ino2 as well as with TAD4 of activator Adr1. Specific missense mutations within Taf1 domain aa 182-250 affecting basic and hydrophobic residues prevented interaction with wild-type TAD1 and caused reduced expression of INO1. Using chromatin immunoprecipitation we demonstrated Ino2-dependent recruitment of Taf1 and Taf6 to ICRE-containing promoters INO1 and CHO2. Transcriptional derepression of INO1 was no longer possible with temperature-sensitive taf1 and taf6 mutants cultivated under nonpermissive conditions. This result supports the hypothesis of Taf-dependent expression of structural genes activated by Ino2.

摘要

酵母中磷脂生物合成基因的表达需要激活蛋白Ino2,它可以结合肌醇/胆碱反应元件(ICRE)中的上游激活序列(UAS)元件,并利用两个独立的转录激活结构域TAD1和TAD2触发靶基因的激活。然而,仍不清楚哪些辅因子介导Ino2的TADs的激活作用。在这里,我们表明基础转录因子TFIID的多个亚基(TBP相关因子Taf1、Taf4、Taf6、Taf10和Taf12)能够在体外与Ino2的激活结构域相互作用。与TAD1的激活缺陷变体不再观察到相互作用。我们能够在Taf1的N端鉴定出两个不重叠的区域(氨基酸1-100和氨基酸182-250),每个区域都可以与Ino2的TAD1以及激活剂Adr1的TAD4相互作用。Taf1结构域氨基酸182-250内影响碱性和疏水残基的特定错义突变阻止了与野生型TAD1的相互作用,并导致INO1表达降低。使用染色质免疫沉淀,我们证明了Ino2依赖的Taf1和Taf6募集到含有ICRE的启动子INO1和CHO2。在非允许条件下培养的温度敏感型taf1和taf6突变体中,INO1的转录去抑制不再可能。这一结果支持了由Ino2激活的结构基因依赖Taf表达的假说。

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