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糖皮质激素和c-Jun的显性负性突变体对干扰素-γ启动子的负转录调控

Negative transcriptional regulation of the interferon-gamma promoter by glucocorticoids and dominant negative mutants of c-Jun.

作者信息

Cippitelli M, Sica A, Viggiano V, Ye J, Ghosh P, Birrer M J, Young H A

机构信息

Biological Carcinogenesis and Development Program, Program Resources Inc./DynCorp, Frederick, Maryland, USA.

出版信息

J Biol Chem. 1995 May 26;270(21):12548-56. doi: 10.1074/jbc.270.21.12548.

DOI:10.1074/jbc.270.21.12548
PMID:7759501
Abstract

Interferon-gamma (IFN-gamma) is an immunoregulatory cytokine expressed in large granular lymphocytes and T cells. However, the molecular mechanisms underlying IFN-gamma gene transcription have not been fully defined. Here, we analyze the mechanisms responsible for the inhibition of IFN-gamma promoter activity by the glucocorticoid hormone dexamethasone. Cotransfection assays performed in Jurkat T cells demonstrated that the activity of the initial 108 base pairs of the IFN-gamma promoter was down-regulated in the presence of dexamethasone. Furthermore, utilizing electrophoretic mobility shift analysis, we identified activator protein 1 AP-1-cAMP response element binding protein-activating transcription factor (CREB-ATF) binding elements situated in positions of the IFN-gamma promoter previously identified as essential for promoter activity. Moreover, dominant negative mutants of the c-Jun proto-oncogene were able to mimic the same down-regulatory effect exerted by dexamethasone, and mutations that abolished the binding of the AP-1 CREB-ATF factors were able to block the glucocorticoid effect. These results suggest a model involving the inhibition of IFN-gamma AP-1 CREB-ATF DNA binding complexes as one of the mechanisms involved in the negative regulatory action of glucocorticoids on IFN-gamma gene expression and support the relevance of AP-1 CREB-ATF binding factors during the transcriptional activation of the IFN-gamma promoter in T cells.

摘要

干扰素-γ(IFN-γ)是一种在大颗粒淋巴细胞和T细胞中表达的免疫调节细胞因子。然而,IFN-γ基因转录的分子机制尚未完全明确。在此,我们分析了糖皮质激素地塞米松抑制IFN-γ启动子活性的机制。在Jurkat T细胞中进行的共转染实验表明,在地塞米松存在的情况下,IFN-γ启动子最初的108个碱基对的活性被下调。此外,利用电泳迁移率变动分析,我们确定了位于IFN-γ启动子中先前被确定为启动子活性所必需位置的激活蛋白1(AP-1)-环磷酸腺苷反应反应元件元件结合蛋白-激活转录因子(CREB-ATF)结合元件。此外,c-Jun原癌基因的显性负性突变体能够模拟地塞米松所发挥的相同下调作用,而消除AP-1 CREB-ATF因子结合的突变能够阻断糖皮质激素的作用。这些结果提示了一个模型,即抑制IFN-γ AP-1 CREB-ATF DNA结合复合物是糖皮质激素对IFN-γ基因表达负调控作用所涉及的机制之一,并支持了AP-1 CREB-ATF结合因子在T细胞中IFN-γ启动子转录激活过程中的相关性。

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