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Fos相关抗原(Fra-1)、junB和junD通过与近端和远端AP1位点结合来激活人内披蛋白启动子转录,从而介导佛波酯对启动子活性的影响。

Fos-related antigen (Fra-1), junB, and junD activate human involucrin promoter transcription by binding to proximal and distal AP1 sites to mediate phorbol ester effects on promoter activity.

作者信息

Welter J F, Crish J F, Agarwal C, Eckert R L

机构信息

Department of Physiology and Biophysics, Case Western Reserve University School of Medicine, Cleveland, Ohio 44106-4970, USA.

出版信息

J Biol Chem. 1995 May 26;270(21):12614-22. doi: 10.1074/jbc.270.21.12614.

DOI:10.1074/jbc.270.21.12614
PMID:7759510
Abstract

Human involucrin (hINV) is a cornified envelope precursor that is specifically expressed in the suprabasal epidermal layers. We previously demonstrated that 2500 base pairs of the hINV gene upstream regulatory region confers differentiation appropriate regulation in transgenic mice. An analysis of the hINV gene sequence upstream of the transcription start site reveals five potential AP1 binding sites (AP1-1 to 5). Using reporter gene constructs in human keratinocytes, we show that the most distal (AP1-5) and most proximal (AP1-1) AP1 sites are essential for high level transcriptional activity. Simultaneous mutation of these sites reduces transcription by 80%. Gel supershift experiments indicate the interaction of these sites with Fra-1, junB, and junD. Involucrin mRNA levels increase 10-fold and promoter activity 5-11-fold when differentiation is induced by phorbol ester. Functional studies implicate AP1-1 and AP1-5 in mediating the phorbol ester-dependent increase in promoter activity. No involucrin promoter activity or involucrin mRNA was detected in 3T3 fibroblasts. We conclude that (i) two AP1 sites in the hINV promoter are important elements required for keratinocyte-specific expression, (ii) these AP1-1 sites mediate the phorbol ester-dependent increase in promoter activity, and (iii) Fra-1, junB, and junD may be important regulators of hINV expression in epidermis.

摘要

人内披蛋白(hINV)是一种角质化包膜前体,在表皮基底层以上各层中特异性表达。我们之前证明,hINV基因上游调控区的2500个碱基对在转基因小鼠中赋予了与分化相适应的调控。对转录起始位点上游的hINV基因序列分析揭示了五个潜在的AP1结合位点(AP1 - 1至5)。利用人类角质形成细胞中的报告基因构建体,我们发现最远端(AP1 - 5)和最近端(AP1 - 1)的AP1位点对于高水平转录活性至关重要。同时突变这些位点会使转录降低80%。凝胶超迁移实验表明这些位点与Fra - 1、junB和junD相互作用。当佛波酯诱导分化时,内披蛋白mRNA水平增加10倍,启动子活性增加5 - 11倍。功能研究表明AP1 - 1和AP1 - 5介导了佛波酯依赖性的启动子活性增加。在3T3成纤维细胞中未检测到内披蛋白启动子活性或内披蛋白mRNA。我们得出结论:(i)hINV启动子中的两个AP1位点是角质形成细胞特异性表达所需的重要元件;(ii)这些AP1 - 1位点介导了佛波酯依赖性的启动子活性增加;(iii)Fra - 1、junB和junD可能是表皮中hINV表达的重要调节因子。

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Fos-related antigen (Fra-1), junB, and junD activate human involucrin promoter transcription by binding to proximal and distal AP1 sites to mediate phorbol ester effects on promoter activity.Fos相关抗原(Fra-1)、junB和junD通过与近端和远端AP1位点结合来激活人内披蛋白启动子转录,从而介导佛波酯对启动子活性的影响。
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