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黑腹果蝇Fbp1基因的蜕皮激素反应增强子是EcR/USP核受体的直接靶点。

The ecdysone response enhancer of the Fbp1 gene of Drosophila melanogaster is a direct target for the EcR/USP nuclear receptor.

作者信息

Antoniewski C, Laval M, Dahan A, Lepesant J A

机构信息

Institut Jacques Monod, Centre National de la Recherche Scientifique, Paris, France.

出版信息

Mol Cell Biol. 1994 Jul;14(7):4465-74. doi: 10.1128/mcb.14.7.4465-4474.1994.

DOI:10.1128/mcb.14.7.4465-4474.1994
PMID:8007953
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC358818/
Abstract

The transcription of the Drosophila melanogaster Fbp1 gene is induced by the steroid hormone 20-hydroxyecdysone and restricted to the late-third-instar fat body tissue. In a previous study we showed that the -68 to -138 region relative to the transcription start site acts as an ecdysone-dependent third-instar fat body-specific enhancer in a transgenic assay. Here we report that seven nucleoprotein complexes are formed in vitro on this enhancer when a nuclear extract from late-third-instar fat body is used in a gel shift assay. Accurate mapping of the binding sites of the complexes revealed a remarkably symmetrical organization. Using specific antibodies, one of the complexes was identified as a heterodimer consisting of the ecdysone receptor (EcR) and Ultraspiracle (USP) proteins. The binding site of the heterodimer as defined by mutagenesis and methylation interference experiments bears strong sequence similarity to the canonical hsp27 ecdysone response element, including an imperfect palindromic structure. The two elements diverge at three positions in both half-sites, indicating that the structure of an active EcR/USP binding site allows considerable sequence variations. In vivo footprinting experiments using ligation-mediated PCR and wild-type or ecdysteroid-deficient larvae show that occupancy of the Fbp1 EcR/USP binding site and adjacent region is dependent on a high concentration of ecdysteroids. These results provide strong evidence for a direct role of the EcR/USP heterodimer in driving gene expression in response to changes of the ecdysteroid titer during Drosophila larval development.

摘要

果蝇Fbp1基因的转录由类固醇激素20-羟基蜕皮激素诱导,并局限于三龄后期的脂肪体组织。在之前的一项研究中,我们发现在转基因实验中,相对于转录起始位点的-68至-138区域作为一个依赖蜕皮激素的三龄脂肪体特异性增强子。在此我们报告,当使用来自三龄后期脂肪体的核提取物进行凝胶迁移实验时,在该增强子上体外形成了七种核蛋白复合物。对这些复合物结合位点的精确映射揭示了一种显著的对称组织。使用特异性抗体,其中一种复合物被鉴定为是由蜕皮激素受体(EcR)和超气门蛋白(USP)组成的异二聚体。通过诱变和甲基化干扰实验确定的该异二聚体的结合位点与典型的hsp27蜕皮激素反应元件具有很强的序列相似性,包括一个不完全的回文结构。这两个元件在两个半位点的三个位置上有所不同,表明活性EcR/USP结合位点的结构允许相当大的序列变异。使用连接介导的PCR以及野生型或蜕皮类固醇缺陷型幼虫进行的体内足迹实验表明,Fbp1 EcR/USP结合位点及相邻区域的占据取决于高浓度的蜕皮类固醇。这些结果为EcR/USP异二聚体在果蝇幼虫发育过程中响应蜕皮类固醇滴度变化驱动基因表达方面的直接作用提供了有力证据。

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