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猿猴病毒40晚期启动子的反式激活需要细胞转录因子TEF-1的结合位点。

trans activation of the simian virus 40 late promoter by large T antigen requires binding sites for the cellular transcription factor TEF-1.

作者信息

Casaz P, Sundseth R, Hansen U

机构信息

Laboratory of Eukaryotic Transcription, Dana Farber Cancer Institute, Boston, Massachusetts.

出版信息

J Virol. 1991 Dec;65(12):6535-43. doi: 10.1128/JVI.65.12.6535-6543.1991.

DOI:10.1128/JVI.65.12.6535-6543.1991
PMID:1658359
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC250705/
Abstract

Simian virus 40 (SV40) T antigen stimulates the level of transcription from several RNA polymerase II promoters, including the SV40 late promoter. The mechanism of trans activation appears to be indirect since binding of T antigen to specific DNA sequences is not required. However, specific promoter elements that respond to T antigen have not previously been defined. We identified DNA sequences from the SV40 late promoter whose ability to stimulate transcription is induced by the expression of T antigen. In particular, the Sph I + II motifs of the SV40 enhancer can confer T-antigen inducibility to the normally uninducible herpes simplex virus thymidine kinase gene promoter when multiple copies of the sequence are inserted 5' of the transcription initiation site and TATA sequence. Binding sites for the cellular transcription factor TEF-1 and octamer binding proteins are contained within the Sph I + II motifs, as well as at other positions in the SV40 promoter. To study the role of individual protein-binding sites in trans activation by T antigen, mutations were constructed in various TEF-1 and octamer protein-binding sites of the SV40 late promoter. These mutations did not significantly affect basal promoter activity. However, mutation of all three TEF-1 sites prevented detectable activation by T antigen. DNase I footprinting of the mutated promoters with purified proteins demonstrated that inducibility by T antigen correlated with binding affinity of TEF-1 for the DNA and not with binding affinity of an octamer binding protein.

摘要

猿猴病毒40(SV40)T抗原可刺激包括SV40晚期启动子在内的几种RNA聚合酶II启动子的转录水平。反式激活机制似乎是间接的,因为T抗原与特定DNA序列的结合并非必需。然而,此前尚未明确对T抗原产生反应的特定启动子元件。我们从SV40晚期启动子中鉴定出DNA序列,其刺激转录的能力可被T抗原的表达所诱导。特别是,当在转录起始位点和TATA序列的5'端插入多个该序列拷贝时,SV40增强子的Sph I + II基序可赋予通常不可诱导的单纯疱疹病毒胸苷激酶基因启动子T抗原诱导性。细胞转录因子TEF-1和八聚体结合蛋白的结合位点包含在Sph I + II基序内,以及SV40启动子的其他位置。为了研究各个蛋白质结合位点在T抗原反式激活中的作用,我们在SV40晚期启动子的各种TEF-1和八聚体蛋白质结合位点构建了突变体。这些突变并未显著影响基础启动子活性。然而,所有三个TEF-1位点的突变均阻止了T抗原的可检测激活。用纯化蛋白对突变启动子进行的DNase I足迹分析表明,T抗原的诱导性与TEF-1对DNA的结合亲和力相关,而与八聚体结合蛋白的结合亲和力无关。

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