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由I型人类T细胞白血病病毒的癌蛋白Tax反式激活的gp34基因启动子调控的分子机制。

Molecular mechanisms of promoter regulation of the gp34 gene that is trans-activated by an oncoprotein Tax of human T cell leukemia virus type I.

作者信息

Ohtani K, Tsujimoto A, Tsukahara T, Numata N, Miura S, Sugamura K, Nakamura M

机构信息

Human Gene Sciences Center, Japan.

出版信息

J Biol Chem. 1998 Jun 5;273(23):14119-29. doi: 10.1074/jbc.273.23.14119.

DOI:10.1074/jbc.273.23.14119
PMID:9603911
Abstract

We investigated the molecular mechanism of transcriptional activation of the gp34 gene by the Tax oncoprotein of human T cell leukemia virus type I (HTLV-I). gp34 is a type II transmembrane molecule belonging to the tumor necrosis factor family and is constitutively expressed on HTLV-I-producing cells but not normal resting T cells. The transcriptional regulatory region of the gp34 gene was activated by HTLV-I Tax in the human T cell line Jurkat, in which endogenous gp34 is induced by Tax. Sequence analysis demonstrated that two NF-kappaB-like elements (1 and 2) were present in the regulatory region. Both NF-kappaB-like elements were able to bind to NF-kappaB or its related factor(s) in a Tax-dependent manner. Chloramphenicol acetyltransferase assays indicated that NF-kappaB-like element 1 was Tax-responsive, although the activity was lower than that the native promoter. NF-kappaB-like element 2 elevated promoter activity when combined with NF-kappaB-like element 1, indicating cooperative function of the elements for maximum promoter function. Unlike typical NF-kappaB elements, the NF-kappaB-like elements in gp34 were not activated by treatment of Jurkat cells with phorbol ester despite induction of the NF-kappaB-like binding activity. Chloramphenicol acetyltransferase reporter assays using the region upstream of the NF-kappaB-like elements identified an upstream region that reduced transcription from cognate and noncognate core promoters in a Tax-independent manner. Our results imply complex regulation of expression of the gp34 gene and suggest implication of gp34 in proliferation of HTLV-I infected T cells.

摘要

我们研究了I型人类T细胞白血病病毒(HTLV-I)的Tax癌蛋白对gp34基因转录激活的分子机制。gp34是一种属于肿瘤坏死因子家族的II型跨膜分子,在产生HTLV-I的细胞中组成性表达,但在正常静息T细胞中不表达。gp34基因的转录调控区域在人T细胞系Jurkat中被HTLV-I Tax激活,在该细胞系中内源性gp34由Tax诱导产生。序列分析表明,调控区域存在两个类NF-κB元件(元件1和元件2)。两个类NF-κB元件都能够以Tax依赖的方式与NF-κB或其相关因子结合。氯霉素乙酰转移酶分析表明,类NF-κB元件1对Tax有反应,尽管其活性低于天然启动子。当类NF-κB元件2与类NF-κB元件1结合时,启动子活性升高,表明这些元件具有协同功能以实现最大启动子功能。与典型的NF-κB元件不同,尽管类NF-κB结合活性被诱导,但用佛波酯处理Jurkat细胞并不能激活gp34中的类NF-κB元件。使用类NF-κB元件上游区域的氯霉素乙酰转移酶报告基因分析确定了一个上游区域,该区域以Tax非依赖的方式降低了同源和非同源核心启动子的转录。我们的结果暗示了gp34基因表达的复杂调控,并提示gp34在HTLV-I感染的T细胞增殖中的作用。

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