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果蝇体节极性基因“engrailed”中两种不同类型的抑制结构域:一种与gro核心抑制因子相互作用,且对整合的靶基因具有优先活性。

Two distinct types of repression domain in engrailed: one interacts with the groucho corepressor and is preferentially active on integrated target genes.

作者信息

Tolkunova E N, Fujioka M, Kobayashi M, Deka D, Jaynes J B

机构信息

Department of Microbiology and Immunology, Kimmel Cancer Institute, Thomas Jefferson University, Philadelphia, Pennsylvania 19107, USA.

出版信息

Mol Cell Biol. 1998 May;18(5):2804-14. doi: 10.1128/MCB.18.5.2804.

Abstract

Active transcriptional repression has been characterized as a function of many regulatory factors. It facilitates combinatorial regulation of gene expression by allowing repressors to be dominant over activators under certain conditions. Here, we show that the Engrailed protein uses two distinct mechanisms to repress transcription. One activity is predominant under normal transient transfection assay conditions in cultured cells. A second activity is predominant in an in vivo active repression assay. The domain mediating the in vivo activity (eh1) is highly conserved throughout several classes of homeoproteins and interacts specifically with the Groucho corepressor. While eh1 shows only weak activity in transient transfections, much stronger activity is seen in culture when an integrated target gene is used. In this assay, the relative activities of different repression domains closely parallel those seen in vivo, with eh1 showing the predominant activity. Reducing the amounts of repressor and target gene in a transient transfection assay also increases the sensitivity of the assay to the Groucho interaction domain, albeit to a lesser extent. This suggests that it utilizes rate-limiting components that are relatively low in abundance. Since Groucho itself is abundant in these cells, the results suggest that a limiting component is recruited effectively by the repressor-corepressor complex only on integrated target genes.

摘要

主动转录抑制已被表征为许多调节因子的一种功能。它通过使阻遏物在某些条件下比激活剂占优势,促进基因表达的组合调控。在此,我们表明Engrailed蛋白利用两种不同机制抑制转录。一种活性在培养细胞的正常瞬时转染试验条件下占主导。第二种活性在体内活性抑制试验中占主导。介导体内活性的结构域(eh1)在几类同源异型蛋白中高度保守,并与Groucho共抑制因子特异性相互作用。虽然eh1在瞬时转染中仅表现出微弱活性,但当使用整合的靶基因时,在培养中可观察到更强的活性。在该试验中,不同抑制结构域的相对活性与体内观察到的活性密切平行,其中eh1表现出主要活性。在瞬时转染试验中减少阻遏物和靶基因的量也会增加该试验对Groucho相互作用结构域的敏感性,尽管程度较小。这表明它利用了丰度相对较低的限速成分。由于Groucho本身在这些细胞中含量丰富,结果表明只有在整合的靶基因上,阻遏物 - 共抑制因子复合物才能有效招募一种限制成分。

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