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Autoregulated expression of the yeast INO2 and INO4 helix-loop-helix activator genes effects cooperative regulation on their target genes.

机译:酵母INO2和INO4螺旋-环-螺旋激活基因的自动调节表达对其目标基因产生协同调节作用。

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摘要

In the yeast Saccharomyces cerevisiae, the phospholipid biosynthetic genes are highly regulated at the transcriptional level in response to the phospholipid precursors inositol and choline. In the absence of inositol and choline (derepressing), the products of the INO2 and INO4 genes form a heteromeric complex which binds to a 10-bp element, upstream activation sequence INO (UASINO), in the promoters of the phospholipid biosynthetic genes to activate their transcription. In the presence of inositol and choline (repressing), the product of the OPI1 gene represses transcription dictated by the UASINO element. Curiously, we identified a UASINO-like element in the promoters of both the INO2 and INO4 genes. The presence of the UASINO element in these two promoters suggested that the mechanism for the inositol-choline response would involved regulating expression of the two activator genes. Using a cat reporter gene, we find that INO2-cat expression was regulated 12-fold in response to inositol and choline but that INO4-cat was constitutively expressed. We further observed that INO2-cat was not expressed in either an ino2 or an ino4 mutant strain and was constitutively overexpressed in an opi1 mutant strain. Expression of the INO4-cat gene was affected only by mutation in the INO4 gene itself. Therefore, INO2-cat transcription is regulated by the products of both the INO2 and INO4 genes whereas INO4 must interact with another protein to activate its own transcription. Our data show that derepression of phospholipid biosynthetic gene expression involves two mechanisms: increasing the levels of the INO2 and INO4 gene products and inactivating the OPI1-mediated repression mechanism. We propose a model suggesting that this dual mechanism of regulation accounts for the observed cooperative stimulation of IN01 and CH01 gene expression (phospholipids biosynthetic genes).
机译:在酵母酿酒酵母中,响应于磷脂前体肌醇和胆碱,磷脂生物合成基因在转录水平上受到高度调节。在不存在肌醇和胆碱的情况下(抑制),INO2和INO4基因的产物形成一个杂合复合物,该复合物与10 bp的上游激活序列INO(UASINO)结合,在磷脂生物合成基因的启动子中激活他们的转录。在肌醇和胆碱的存在下(阻抑),OPI1基因的产物会抑制UASINO元件决定的转录。奇怪的是,我们在INO2和INO4基因的启动子中发现了类似UASINO的元件。这两个启动子中UASINO元件的存在表明,肌醇-胆碱应答的机制涉及调节两个激活基因的表达。使用猫报道基因,我们发现响应肌醇和胆碱,INO2-cat的表达被调节了12倍,但是INO4-cat却是组成型表达的。我们进一步观察到,INO2-cat在ino2或ino4突变株中均未表达,并且在opi1突变株中组成性过表达。 INO4-cat基因的表达仅受INO4基因本身突变的影响。因此,INO2-cat转录受INO2和INO4基因产物的调节,而INO4必须与另一种蛋白质相互作用才能激活其自身的转录。我们的数据表明,磷脂生物合成基因表达的抑制受到两种机制的影响:增加INO2和INO4基因产物的水平以及使OPI1介导的抑制机制失活。我们提出一个模型,表明这种双重调控机制解释了观察到的IN01和CH01基因表达(磷脂生物合成基因)的协同刺激。

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  • 作者

    Ashburner, B P; Lopes, J M;

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  • 年度 1995
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  • 原文格式 PDF
  • 正文语种 en
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