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人类Gli2癌基因新亚型的克隆及其增强人类1型T细胞白血病病毒基因组tax依赖性转录的活性。

Cloning of novel isoforms of the human Gli2 oncogene and their activities to enhance tax-dependent transcription of the human T-cell leukemia virus type 1 genome.

作者信息

Tanimura A, Dan S, Yoshida M

机构信息

Department of Cellular and Molecular Biology, Institute of Medical Science, University of Tokyo, Japan.

出版信息

J Virol. 1998 May;72(5):3958-64. doi: 10.1128/JVI.72.5.3958-3964.1998.

DOI:10.1128/JVI.72.5.3958-3964.1998
PMID:9557682
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC109622/
Abstract

The expression of human T-cell leukemia virus type 1 (HTLV-1) is activated by interaction of a viral transactivator protein, Tax, and cellular transcription factor, CREB (cyclic AMP response element binding protein), which bind to a 21-bp enhancer in the long terminal repeats (LTR). THP (Tax-helping protein) was previously determined to enhance the transactivation by Tax protein. Here we report novel forms of the human homolog of a member of the Gli oncogene family, Gli2 (also termed Gli2/THP), an extended form of a zinc finger protein, THP, which was described previously. Four possible isoforms (hGli2 alpha, beta, gamma, and delta) are formed by combinations of two independent alternative splicings, and all the isoforms could bind to a DNA motif, TRE2S, in the LTR. The longer isoforms, alpha and beta, were abundantly expressed in various cell lines including HTLV-1-infected T-cell lines. Fusion proteins of the hGli2 isoforms with the DNA-binding domain of Gal4 activated transcription when the reporter contained a Gal4-binding site and one copy of the 21-bp sequence, to which CREB binds. This activation was observed only in the presence of Tax. The 21-bp sequence in the reporter was also essential for the activation. These results suggest that simultaneous binding of hGli2 and CREB to the respective sites in the reporter seems to be critical for Tax protein to activate transcription. Consequently, it is probable that the LTR can be regulated by two independent signals through hGli2 and CREB, since the LTR contains the 21-bp and TRE2S sequences in the vicinity.

摘要

人类嗜T细胞病毒1型(HTLV-1)的表达是由一种病毒反式激活蛋白Tax与细胞转录因子CREB(环磷酸腺苷反应元件结合蛋白)相互作用所激活的,二者结合于长末端重复序列(LTR)中的一个21碱基对增强子。THP(Tax辅助蛋白)先前被确定可增强Tax蛋白的反式激活作用。在此我们报告了Gli癌基因家族成员之一的人类同源物Gli2的新形式(也称为Gli2/THP),即先前描述的一种锌指蛋白THP的延伸形式。通过两种独立的可变剪接组合形成了四种可能的异构体(hGli2α、β、γ和δ),并且所有异构体都能与LTR中的一个DNA基序TRE2S结合。较长的异构体α和β在包括HTLV-1感染的T细胞系在内的各种细胞系中大量表达。当报告基因含有一个Gal4结合位点和一个CREB结合的21碱基对序列的拷贝时,hGli2异构体与Gal4的DNA结合结构域的融合蛋白可激活转录。仅在有Tax存在时才观察到这种激活作用。报告基因中的21碱基对序列对激活也至关重要。这些结果表明,hGli2和CREB同时结合到报告基因中的各自位点似乎对Tax蛋白激活转录至关重要。因此,由于LTR在附近含有21碱基对和TRE2S序列,LTR很可能可通过hGli2和CREB这两个独立信号进行调控。

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Cloning of novel isoforms of the human Gli2 oncogene and their activities to enhance tax-dependent transcription of the human T-cell leukemia virus type 1 genome.人类Gli2癌基因新亚型的克隆及其增强人类1型T细胞白血病病毒基因组tax依赖性转录的活性。
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