Bolwig G M, Bruder J T, Hearing P
Department of Microbiology, Health Sciences Center, State University of New York, Stony Brook 11794.
Nucleic Acids Res. 1992 Dec 25;20(24):6555-64. doi: 10.1093/nar/20.24.6555.
The human transcription factor EF-1A binds to the purine-rich E1A core enhancer sequence in the adenovirus E1A and E4 and polyomavirus enhancer regions. The consensus binding site for EF-1A resembles that of members of the ets domain protein family. EF-1A activation of transcription requires a dimeric binding site. Analysis of binding sites containing point mutations revealed that EF-1A binding is determined by the core nucleotides of the binding site, while transcriptional activation is determined both by the core and some peripheral nucleotides that do not affect binding. We have purified EF-1A and analyzed its two constituent subunits, EF-1A alpha and EF-1A beta. EF-1A alpha (MW approximately 60kD) makes the primary DNA contacts. EF-1A beta (MW approximately 50 kD) forms a heteromultimeric complex with EF-1A alpha both in solution and on a dimeric binding site. Binding of both EF-1A subunits is necessary, but not sufficient, for transcriptional activation. We present immunochemical and functional evidence that EF-1A alpha is related to the murine ets-related protein GABP alpha and that EF-1A beta is related to the murine protein GABP beta.
人类转录因子EF-1A可与腺病毒E1A和E4以及多瘤病毒增强子区域中富含嘌呤的E1A核心增强子序列结合。EF-1A的共有结合位点类似于ets结构域蛋白家族成员的结合位点。EF-1A的转录激活需要一个二聚体结合位点。对含有点突变的结合位点进行分析表明,EF-1A的结合由结合位点的核心核苷酸决定,而转录激活则由核心核苷酸以及一些不影响结合的外围核苷酸共同决定。我们已经纯化了EF-1A,并分析了其两个组成亚基,即EF-1Aα和EF-1Aβ。EF-1Aα(分子量约60kD)与DNA进行主要接触。EF-1Aβ(分子量约50kD)在溶液中和二聚体结合位点上均与EF-1Aα形成异源多聚体复合物。两个EF-1A亚基的结合对于转录激活是必要的,但并不充分。我们提供了免疫化学和功能证据,证明EF-1Aα与小鼠ets相关蛋白GABPα相关,而EF-1Aβ与小鼠蛋白GABPβ相关。
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