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维甲酸诱导的人γ-干扰素启动子的转录调控

Retinoic acid-induced transcriptional modulation of the human interferon-gamma promoter.

作者信息

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

机构信息

Intramural Research Support Program, Scientific Application International Corporation Frederick, Frederick, Maryland 21702-1201, USA.

出版信息

J Biol Chem. 1996 Oct 25;271(43):26783-93. doi: 10.1074/jbc.271.43.26783.

DOI:10.1074/jbc.271.43.26783
PMID:8900159
Abstract

Disregulation of vitamin A metabolism is able to generate different immunological effects, including altered response to infection, reduced IgG production, and differential regulation of cytokine gene expression (including interleukin-2 and -4 and interferon-gamma (IFN-gamma)). In particular, IFN-gamma gene expression is significantly affected by vitamin A and/or its derivatives (e.g. retinoic acid (RA)). Here, we analyze the effect of retinoic acid on IFN-gamma transcription. Transient transfection assays in the human T lymphoblastoid cell line Jurkat demonstrated that the activation of the IFN-gamma promoter was significantly down-regulated in the presence of RA. Surprisingly, two different AP-1/CREB-ATF-binding elements situated in the initial 108 base pairs of the IFN-gamma promoter and previously shown to be critical for transcriptional activity were unaffected by RA. Utilizing promoter deletions and electrophoretic mobility shift analysis, we identified a USF/EGR-1-binding element cooperating in the modulation of IFN-gamma promoter activity by RA. This element was found to be situated in a position of the IFN-gamma promoter close to a silencer element previously identified in our laboratory. These results suggest that direct modulation of IFN-gamma promoter activity is one of the possible mechanisms involved in the inhibitory effect of retinoids on IFN-gamma gene expression.

摘要

维生素A代谢失调能够产生不同的免疫效应,包括对感染的反应改变、IgG产生减少以及细胞因子基因表达的差异调节(包括白细胞介素-2和-4以及干扰素-γ(IFN-γ))。特别是,IFN-γ基因表达受到维生素A和/或其衍生物(如视黄酸(RA))的显著影响。在此,我们分析视黄酸对IFN-γ转录的影响。在人T淋巴母细胞系Jurkat中进行的瞬时转染实验表明,在RA存在的情况下,IFN-γ启动子的激活显著下调。令人惊讶的是,位于IFN-γ启动子最初108个碱基对中的两个不同的AP-1/CREB-ATF结合元件,先前已证明对转录活性至关重要,但不受RA影响。利用启动子缺失和电泳迁移率变动分析,我们鉴定出一个USF/EGR-1结合元件,它在RA对IFN-γ启动子活性的调节中起协同作用。发现该元件位于IFN-γ启动子中一个靠近我们实验室先前鉴定的沉默子元件的位置。这些结果表明,直接调节IFN-γ启动子活性是类视黄醇对IFN-γ基因表达抑制作用的可能机制之一。

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