Pescini R, Kaszubska W, Whelan J, DeLamarter J F, Hooft van Huijsduijnen R
GLAXO Institute for Molecular Biology, Geneva, Switzerland.
J Biol Chem. 1994 Jan 14;269(2):1159-65.
We have isolated a cDNA encoding a variant of the transcription factor ATF-a (called ATF-a0) by screening a HeLa cDNA expression library with a regulatory element of the E-selectin promoter, NF-ELAM1/delta A. Relative to full-length ATF-a, the ATF-a0 cDNA contains a large in-frame deletion of 525 base pairs that removes the P/S/T-rich putative transactivation domain. Using reverse-transcription-polymerase chain reaction and Northern blot hybridization to characterize ATF-a0 expression, we found that putative mRNAs for ATF-a0 and ATF-a are present at varying ratios in different tissues. Full-length ATF-a is a transcriptional activator for the NF-ELAM1/delta A site of the E-selectin promoter. In contrast, we show ATF-a0 has no measurable transactivating function on this element. Moreover, we demonstrate that co-expressed ATP-a0 and ATF-a preferentially heterodimerize. In the heterodimer ATF-a0 is a dominant inhibitor that completely blocks the transactivating activity of ATF-a. Both forms of ATF-a bind the p50 subunit of NF-kappa B as shown by affinity chromatography. ATF-a0 appears to be a splice variant similar to the one found for ATF-2, its closest homologue in structure and function. Taken together, our results suggest that ATF-a0 is an important member of the ATF family with a negative regulatory role in transactivation.
我们通过用E-选择素启动子的调控元件NF-ELAM1/δA筛选HeLa cDNA表达文库,分离出了一个编码转录因子ATF-α变体(称为ATF-α0)的cDNA。相对于全长ATF-α,ATF-α0 cDNA包含一个525个碱基对的大框内缺失,该缺失去除了富含脯氨酸/丝氨酸/苏氨酸的假定反式激活结构域。我们使用逆转录-聚合酶链反应和Northern印迹杂交来表征ATF-α0的表达,发现在不同组织中,ATF-α0和ATF-α的假定mRNA以不同比例存在。全长ATF-α是E-选择素启动子的NF-ELAM1/δA位点的转录激活因子。相比之下,我们发现ATF-α0对该元件没有可测量的反式激活功能。此外,我们证明共表达的ATF-α0和ATF-α优先形成异源二聚体。在异源二聚体中,ATF-α0是一种显性抑制剂,它完全阻断了ATF-α的反式激活活性。亲和层析结果表明,两种形式的ATF-α都能与NF-κB的p50亚基结合。ATF-α0似乎是一种剪接变体,类似于在其结构和功能上最接近的同源物ATF-2中发现的变体。综上所述,我们的结果表明,ATF-α0是ATF家族的一个重要成员,在反式激活中起负调控作用。
