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鉴定 E2F1 作为调节 tapasin 表达的重要转录因子。

Identification of E2F1 as an important transcription factor for the regulation of tapasin expression.

机构信息

Institute of Medical Immunology, Martin Luther University Halle-Wittenberg, 06112 Halle, Saale, Germany.

出版信息

J Biol Chem. 2010 Oct 1;285(40):30419-26. doi: 10.1074/jbc.M109.094284. Epub 2010 Jul 27.

Abstract

HER-2/neu overexpression in tumor cells caused abnormalities of MHC class I surface expression due to impaired expression of components of the antigen-processing machinery (APM) including the low molecular weight proteins, the transporter associated with antigen processing (TAP), and the chaperone tapasin, whereas the expression of MHC class I heavy chain as well as β(2)-microglobulin was only marginally affected. This oncogene-mediated deficient APM component expression could be reverted by interferon-γ treatment, suggesting a deregulation rather than structural alterations as underlying molecular mechanisms. To determine the level of regulation, the transcriptional activity of APM components was analyzed in HER-2/neu(-) and HER-2/neu(+) cells. All major APM components were transcriptionally down-regulated in HER-2/neu(+) when compared with HER-2/neu(-) cells, which was accompanied by a reduced binding of RNA polymerase II to the APM promoters. Site-directed mutagenesis of the p300- and E2F-binding sites in the APM promoters did not reconstitute the oncogene-mediated decreased transcription rate with the exception of tapasin, which was restored in HER-2/neu(+) cells to levels of wild type tapasin promoter activity in HER-2/neu(-) fibroblasts. The E2F-directed control of tapasin expression was further confirmed by chromatin immunoprecipitation analyses showing that E2F1 and p300 bind to the tapasin and APM promoters in both cell lines. Moreover, siRNA-mediated silencing of E2F1 was associated with an increased tapasin expression, whereas transient overexpression of E2F1 launch a reduced tapasin transcription, suggesting that E2F1 is an essential transcription factor for tapasin.

摘要

肿瘤细胞中 HER-2/neu 的过表达导致 MHC Ⅰ类表面表达异常,这是由于抗原加工机制(APM)成分的表达受损,包括低分子量蛋白、抗原加工相关转运体(TAP)和伴侣蛋白 tapasin,而 MHC Ⅰ类重链和 β(2)-微球蛋白的表达仅受到轻微影响。这种致癌基因介导的 APM 成分表达缺陷可以通过干扰素-γ治疗逆转,这表明潜在的分子机制是调节异常而不是结构改变。为了确定调节水平,分析了 HER-2/neu(-)和 HER-2/neu(+)细胞中 APM 成分的转录活性。与 HER-2/neu(-)细胞相比,HER-2/neu(+)细胞中所有主要的 APM 成分的转录均受到下调,这伴随着 RNA 聚合酶 II 与 APM 启动子的结合减少。APM 启动子中 p300 和 E2F 结合位点的定点突变并没有重建致癌基因介导的转录率降低,除了 tapasin,HER-2/neu(+)细胞中的 tapasin 恢复到 HER-2/neu(-)成纤维细胞中野生型 tapasin 启动子活性的水平。染色质免疫沉淀分析进一步证实了 E2F 对 tapasin 表达的定向控制,结果表明 E2F1 和 p300 结合到两种细胞系中的 tapasin 和 APM 启动子上。此外,siRNA 介导的 E2F1 沉默与 tapasin 表达增加相关,而瞬时过表达 E2F1 则导致 tapasin 转录减少,表明 E2F1 是 tapasin 的必需转录因子。

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