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直接重复序列结合蜕皮激素受体/超气门蛋白受体,并介导黑腹果蝇中的蜕皮甾体反应。

Direct repeats bind the EcR/USP receptor and mediate ecdysteroid responses in Drosophila melanogaster.

作者信息

Antoniewski C, Mugat B, Delbac F, Lepesant J A

机构信息

Institut Jacques Monod, CNRS et Université Paris, France.

出版信息

Mol Cell Biol. 1996 Jun;16(6):2977-86. doi: 10.1128/MCB.16.6.2977.

DOI:10.1128/MCB.16.6.2977
PMID:8649409
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC231292/
Abstract

The steroid hormone 20-hydroxyecdysone plays a key role in the induction and modulation of morphogenetic events throughout Drosophila development. Previous studies have shown that a heterodimeric nuclear receptor composed of the EcR and USP proteins mediates the action of the hormone at the transcriptional through binding to palindromic ecdysteroid mediates the action of the hormone at the transcriptional level through binding to palindromic ecdysteroid response elements (EcREs) such as those present in the promoter of the hsp27 gene or the fat body-specific enhancer of the Fbp1 gene. We show that in addition to palindromic EcREs, the EcR/USP heterodimer can bind in vitro with various affinities to direct repetitions of the motif AGGTCA separated by 1 to 5 nucleotides (DR1 to DR5), which are known to be target sites for vertebrate nuclear receptors. At variance with the receptors, EcR/USP was also found to bind to a DR0 direct repeat with no intervening nucleotide. In cell transformation assays, direct repeats DR0 to DR5 alone can render the minimum viral tk or Drosophila Fbp1 promoter responsive to 20-hydroxyecdysone, as does the palindromic hsp27 EcRE. In a transgenic assay, however, neither the palindromic hsp27 element nor direct repeat DR3 alone can make the Fbp1 minimal promoter responsive to premetamorphic ecdysteroid peaks. In contrast, DR0 and DR3 elements, when substituted for the natural palindromic EcRE in the context of the Fbp1 enhancer, can drive a strong fat body-specific ecdysteroid response in transgenic animals. These results demonstrate that directly repeated EcR/USP binding sites are as effective as palindromic EcREs in vivo. They also provide evidence that additional flanking regulatory sequences are crucially required to potentiate the hormonal response mediated by both types of elements and specify its spatial and temporal pattern.

摘要

类固醇激素20-羟基蜕皮酮在果蝇整个发育过程中形态发生事件的诱导和调节中起着关键作用。先前的研究表明,由EcR和USP蛋白组成的异二聚体核受体通过与回文蜕皮激素反应元件(EcREs)结合,在转录水平介导激素的作用,如热休克蛋白27(hsp27)基因启动子或Fbp1基因脂肪体特异性增强子中存在的那些元件。我们发现,除了回文EcREs外,EcR/USP异二聚体在体外还能以不同亲和力与由1至5个核苷酸隔开的基序AGGTCA的直接重复序列(DR1至DR5)结合,这些序列已知是脊椎动物核受体的靶位点。与这些受体不同的是,还发现EcR/USP能与没有间隔核苷酸的DR0直接重复序列结合。在细胞转化试验中,单独的直接重复序列DR0至DR5能使最小的病毒胸苷激酶(tk)或果蝇Fbp1启动子对20-羟基蜕皮酮产生反应,回文hsp27 EcRE也是如此。然而,在转基因试验中,单独的回文hsp27元件或直接重复序列DR3都不能使Fbp1最小启动子对变态前蜕皮激素峰值产生反应。相反,当在Fbp1增强子的背景下用DR0和DR3元件替代天然回文EcRE时,能在转基因动物中驱动强烈的脂肪体特异性蜕皮激素反应。这些结果表明,直接重复的EcR/USP结合位点在体内与回文EcREs一样有效。它们还提供了证据,表明额外的侧翼调控序列对于增强由这两种元件介导的激素反应并确定其时空模式至关重要。

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