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大鼠肝脏c-erb Aβ1甲状腺激素受体在酵母(酿酒酵母)中是一种组成型激活剂:结构域D、E和F在非激素依赖性转录中的重要作用。

Rat liver c-erb A beta 1 thyroid hormone receptor is a constitutive activator in yeast (Saccharomyces cerevisiae): essential role of domains D,E and F in hormone-independent transcription.

作者信息

Ohashi H, Yang Y F, Walfish P G

机构信息

Thyroid Research Laboratory, Samuel Lunenfeld Research Institute, Mount Sinai Hospital, University of Toronto, Ontario, Canada.

出版信息

Biochem Biophys Res Commun. 1991 Aug 15;178(3):1167-75. doi: 10.1016/0006-291x(91)91015-5.

Abstract

To assess thyroid hormone receptor (TR)-mediated activation of transcription in yeast in the presence or absence of thyroid hormone (T3), we developed a co-expression system using a TR-beta 1 expression vector and a reporter plasmid containing a 16 base pair palindromic thyroid hormone response element (TRE) upstream from a proximal CYC1 promoter that was fused to the beta-galactosidase lac Z gene of Escherichia coli. Although TR-beta 1 functions as a repressor in most mammalian systems, using our system we observed a unique thyroid hormone-independent transcriptional response indicating that wild TR-beta 1 acted as a constitutive activator in yeast; the addition of 1 microM T3 induced a moderate but significant (p less than 0.01) 25-40% further increase in transcriptional activity. Using a series of rat TR-beta 1 mutant constructs, we found that deletion of domain D and portions of E completely eliminated transcriptional activity, whereas truncations of domain F and E permitted a partial (20-40%) response compared to wild TR-beta 1 in the presence or absence of T3. These observations indicate that TR-beta 1 functions as an activator in yeast and that domains D,E and F play important interactive roles in its hormone-independent gene activation with the D domain likely being the most essential. Furthermore, our results suggest that the different transcriptional property of TR-beta 1 in yeast compared to mammalian cells i.e. activator vs repressor function, is likely determined by transcriptional factor differences which are dependent upon cellular origin.

摘要

为了评估在存在或不存在甲状腺激素(T3)的情况下,甲状腺激素受体(TR)介导的酵母转录激活作用,我们开发了一种共表达系统,该系统使用TR-β1表达载体和一个报告质粒,该报告质粒在近端CYC1启动子上游含有一个16碱基对的回文甲状腺激素反应元件(TRE),该启动子与大肠杆菌的β-半乳糖苷酶lac Z基因融合。尽管TR-β1在大多数哺乳动物系统中起阻遏作用,但使用我们的系统,我们观察到了一种独特的甲状腺激素非依赖性转录反应,这表明野生型TR-β1在酵母中作为组成型激活剂起作用;添加1μM T3可诱导转录活性适度但显著(p小于0.01)进一步增加25 - 40%。使用一系列大鼠TR-β1突变体构建体,我们发现缺失结构域D和部分结构域E完全消除了转录活性,而截短结构域F和E在存在或不存在T3的情况下与野生型TR-β1相比允许部分(20 - 40%)反应。这些观察结果表明,TR-β1在酵母中作为激活剂起作用,并且结构域D、E和F在其激素非依赖性基因激活中发挥重要的相互作用,其中D结构域可能是最关键的。此外,我们的结果表明,与哺乳动物细胞相比,TR-β1在酵母中的不同转录特性,即激活剂与阻遏剂功能,可能由取决于细胞来源的转录因子差异决定。

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