Characterization and functional analysis of the p42Ets-1 variant of the mouse Ets-1 transcription factor

被引:0
|
作者
Frédéric Lionneton
Etienne Lelièvre
David Baillat
Dominique Stehelin
Fabrice Soncin
机构
[1] Institut de Biologie de Lille,Center for Vascular Biology, Department of Physiology
[2] CNRS UMR 8526,undefined
[3] 1 rue Calmette,undefined
[4] University of Connecticut Health Center,undefined
来源
Oncogene | 2003年 / 22卷
关键词
Ets-1; endothelium; VE-cadherin; gene promoter;
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中图分类号
学科分类号
摘要
We have identified the mouse exon VII splice variant of the Ets-1 transcription factor. The variant is expressed in all cell lines which express ets-1, at lower levels, it is also expressed in the mouse embryo in vivo. The corresponding protein, p42Ets-1, is a transcription factor as it is able to bind to specific DNA sequences and to transactivate a bona fide ETS reporter vector. A comparison of optimal DNA-binding sites shows that p42Ets-1 binds to more various DNA sequences than p51Ets-1; p42Ets-1 recognizes the same optimal consensus sequence as p51Ets-1, but also many variations of it, mainly at base −1, which is located just prior to the GGAA/T core sequence. The binding differences were quantified by surface plasmon resonance analyses and the protein region responsible for the differences in DNA sequence recognition located in the Val280-Glu302 fragment, which is encoded by exon VII. The specific DNA-binding properties of each isoform translates into clear differences in activity, p42Ets-1 transactivates the natural VE-cadherin gene promoter through both ETS-binding site (EBS)2 and EBS4 whereas p51Ets-1 is mainly active on EBS4. Altogether, our data suggest that p42Ets-1 acts as a distinct transcription factor from p51Ets-1.
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页码:9156 / 9164
页数:8
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