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介导人嗜T淋巴细胞病毒I型(HTLV-I)反式激活蛋白Tax对白细胞介素-2受体α κB增强子效应的转录激活因子包括原癌基因c-rel的产物。

The transcriptionally active factors mediating the effect of the HTLV-I Tax transactivator on the IL-2R alpha kappa B enhancer include the product of the c-rel proto-oncogene.

作者信息

Crenon I, Béraud C, Simard P, Montagne J, Veschambre P, Jalinot P

机构信息

Laboratoire de Biologie Moléculaire et Cellulaire, Ecole Normale Supérieure de Lyon, France.

出版信息

Oncogene. 1993 Apr;8(4):867-75.

PMID:8455941
Abstract

The transactivator HTLV-I Tax activates the promoter of the gene coding for the interleukin 2 alpha-chain receptor (IL-2R alpha) via a kappa B site that can bind several protein species of the rel family. Tax1 strongly activates the enhancer activity of this motif, in both epithelial HeLa and lymphoid Jurkat cells. This activation was not observed in undifferentiated embryocarcinoma F9 cells. Overexpression of the p50, p65 and Rel proteins in these cells showed that significant activation of the IL-2R alpha kappa B site was observed only with Rel and Rel plus p65. Moreover, whereas both Tax and phorbol 12-myristate 13-acetate (PMA) are able to efficiently induce the binding of NF-kappa B to the IL-2R alpha kappa B site, PMA is functionally inactive. Using the DNA affinity precipitation assay, we observed that Tax1 is able to efficiently induce the binding of Rel, whereas PMA is not. This established a clear difference between both stimuli, indicating that Rel is the functionally active factor. We conclude from these results that the functional activity of members of the rel family is regulated by their interaction with DNA and that Rel can be a potent transcriptional activator on specific kappa B sites.

摘要

反式激活因子HTLV-I Tax通过一个可结合rel家族多种蛋白质的κB位点激活编码白细胞介素2α链受体(IL-2Rα)的基因启动子。Tax1在上皮性HeLa细胞和淋巴样Jurkat细胞中均能强烈激活该基序的增强子活性。在未分化的胚胎癌细胞F9中未观察到这种激活。在这些细胞中过表达p50、p65和Rel蛋白表明,仅Rel以及Rel与p65共同作用时,才能观察到IL-2Rα κB位点的显著激活。此外,虽然Tax和佛波酯12-肉豆蔻酸酯13-乙酸酯(PMA)均能有效诱导NF-κB与IL-2Rα κB位点结合,但PMA在功能上无活性。使用DNA亲和沉淀试验,我们观察到Tax1能够有效诱导Rel结合,而PMA则不能。这明确显示了两种刺激之间的差异,表明Rel是功能活性因子。我们从这些结果得出结论,rel家族成员的功能活性受其与DNA相互作用的调节,并且Rel在特定的κB位点上可能是一种有效的转录激活因子。

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