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在c-myc的内源性靶基因处对不同E盒结合蛋白的区分。

Discrimination between different E-box-binding proteins at an endogenous target gene of c-myc.

作者信息

Desbarats L, Gaubatz S, Eilers M

机构信息

Zentrum für Molekulare Biologie der Universität Heidelberg, Germany.

出版信息

Genes Dev. 1996 Feb 15;10(4):447-60. doi: 10.1101/gad.10.4.447.

DOI:10.1101/gad.10.4.447
PMID:8600028
Abstract

c-myc plans a key role in regulating mammalian cell proliferation and apoptosis. The gene codes for a transcription factor, Myc, that belongs to the helix-loop-helix/leucine zipper (HLH/LZ) family of proteins. Myc heterodimerizes with a partner protein termed Max; the heterodimeric complex binds to CAC(G/A)TG (E-box) sequences and activates transcription from these sites. However, several other HLH/LZ proteins, including USF and TFE-3, bind to and trans-activate from the same element, yet have no documented effect on cell proliferation or apoptosis. Therefore, it is likely that mechanisms exist that discriminate between these proteins for activation of natural target genes of Myc. We now show that trans-activation from the E-box in the rat prothymosin-alpha intron enhancer is indeed specific for Myc, and identify both the distance from the start site of transcription and a second E-box element adjacent to that recognized by Myc as critical determinants of specificity. Surprisingly, transcription activation domains required for Myc to activate from this distal enhancer position differ from previously mapped domains and closely correlate with those domains essential for transformation. As observed in transformation assays, Myc and Max strongly synergize in activation from a distal enhancer position. Our data suggest that trans-activation from the prothymosin intron enhancer is a faithful reflection of the transforming properties of the Myc protein.

摘要

c-myc在调节哺乳动物细胞增殖和凋亡中起关键作用。该基因编码一种转录因子Myc,它属于螺旋-环-螺旋/亮氨酸拉链(HLH/LZ)蛋白家族。Myc与一种称为Max的伴侣蛋白形成异二聚体;这种异二聚体复合物与CAC(G/A)TG(E-box)序列结合并激活这些位点的转录。然而,包括USF和TFE-3在内的其他几种HLH/LZ蛋白也能与同一元件结合并进行反式激活,但对细胞增殖或凋亡没有记录在案的影响。因此,很可能存在一些机制来区分这些蛋白,以激活Myc的天然靶基因。我们现在表明,大鼠前胸腺素α内含子增强子中E-box的反式激活确实对Myc具有特异性,并确定了与转录起始位点的距离以及与Myc识别的元件相邻的第二个E-box元件是特异性的关键决定因素。令人惊讶的是,Myc从这个远端增强子位置激活所需的转录激活结构域与先前定位的结构域不同,并且与转化所必需的那些结构域密切相关。正如在转化试验中观察到的那样,Myc和Max在从远端增强子位置的激活中强烈协同作用。我们的数据表明,前胸腺素内含子增强子的反式激活忠实地反映了Myc蛋白的转化特性。

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