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控制大鼠谷氨酰胺合成酶转录的糖皮质激素反应元件的鉴定。

Identification of glucocorticoid-responsive elements that control transcription of rat glutamine synthetase.

作者信息

Chandrasekhar S, Souba W W, Abcouwer S F

机构信息

Surgical Oncology Research Laboratories, Massachusetts General Hospital, and Department of Surgery, Harvard Medical School, Boston, Massachusetts 02114-2696, USA.

出版信息

Am J Physiol. 1999 Feb;276(2):L319-31. doi: 10.1152/ajplung.1999.276.2.L319.

DOI:10.1152/ajplung.1999.276.2.L319
PMID:9950895
Abstract

Basal expression of glutamine synthetase (GS) is very low in rat lung and muscle and remarkably enhanced by glucocorticoid hormones during trauma and catabolic states. Although this response is believed to be transcriptionally regulated, the genetic elements responsible for tissue-specific glucocorticoid induction of GS expression have not been identified. A rat lung epithelial cell line (L2) and a glucocorticoid receptor-deficient human prostate cancer cell line (PC3), together with GS reporter gene constructs, were utilized in gene transfer experiments to identify two regions within the rat genomic clone gGS3 that imparted dexamethasone (Dex) responsiveness to both the homologous GS promoter and the heterologous herpes simplex virus thymidine kinase promoter in glucocorticoid receptor-dependent fashions. One region lies nearly 6 kb upstream of the GS transcription initiation site, and the other lies within the first intron of the GS gene. Dex responsiveness was localized to a 325-bp fragment of the intron region containing a canonical glucocorticoid response element and to a 225-bp fragment of the far-upstream region containing three separate glucocorticoid response element half-sites. The GS promoter exhibited relatively high basal activity that was repressed by inclusion of the far-upstream or the intron glucocorticoid-responsive region. Dex treatment negated this repression. A model is suggested in which the glucocorticoid-receptor unit causes derepression of lung and muscle GS transcription during trauma and catabolic states.

摘要

谷氨酰胺合成酶(GS)在大鼠肺和肌肉中的基础表达非常低,在创伤和分解代谢状态下,糖皮质激素可使其显著增强。尽管这种反应被认为是由转录调控的,但尚未确定负责糖皮质激素对GS表达进行组织特异性诱导的遗传元件。在基因转移实验中,使用了大鼠肺上皮细胞系(L2)和糖皮质激素受体缺陷的人前列腺癌细胞系(PC3)以及GS报告基因构建体,以确定大鼠基因组克隆gGS3中的两个区域,这两个区域以糖皮质激素受体依赖的方式赋予地塞米松(Dex)对同源GS启动子和异源单纯疱疹病毒胸苷激酶启动子的反应性。一个区域位于GS转录起始位点上游近6 kb处,另一个区域位于GS基因的第一个内含子内。Dex反应性定位于内含子区域的一个325 bp片段,该片段包含一个典型的糖皮质激素反应元件,以及位于上游远端区域的一个225 bp片段,该片段包含三个独立的糖皮质激素反应元件半位点。GS启动子表现出相对较高的基础活性,当包含上游远端或内含子糖皮质激素反应区域时,该活性受到抑制。Dex处理消除了这种抑制。提出了一个模型,其中糖皮质激素受体单位在创伤和分解代谢状态下导致肺和肌肉GS转录的去抑制。

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