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上游刺激因子亚型的免疫化学特性及反式作用特性

Immunochemical characterization and transacting properties of upstream stimulatory factor isoforms.

作者信息

Viollet B, Lefrançois-Martinez A M, Henrion A, Kahn A, Raymondjean M, Martinez A

机构信息

Institut Cochin de Génétique Moléculaire, U129 INSERM, Université René Descartes, Paris, France.

出版信息

J Biol Chem. 1996 Jan 19;271(3):1405-15. doi: 10.1074/jbc.271.3.1405.

Abstract

The ubiquitous upstream stimulatory factor (USF) transcription factors encoded by two distinct genes (USF1 and USF2) exist under the form of various dimers able to bind E-boxes. We report the molecular cloning and functional characterization of USF2 isoforms, corresponding to a 44-kDa subunit, USF2a, and a new 38-kDa subunit, USF2b, generated by differential splicing. Using specific anti-USF antibodies, we define the different binding complexes in various nuclear extracts. In vivo, the USF1/USF2a heterodimer represents over 66% of the USF binding activity whereas the USF1 and USF2a homodimers represent less than 10%, which strongly suggests an in vivo preferential association in heterodimers. In particular, an USF1/USF2b heterodimer accounted for almost 15% of the USF species in some cells. The preferential heterodimerization of USF subunits was reproduced ex vivo, while the in vitro association of cotranslated subunits, or recombinant USF proteins, appeared to be random. In transiently transfected HeLa or hepatoma cells, USF2a and USF1 homodimers transactivated a minimal promoter with similar efficiency, whereas USF2b, which lacks an internal 67-amino acid domain, was a poor transactivator. Additionally, USF2b was an efficient as USF1 and USF2a homodimers in transactivating the liver-specific pyruvate kinase gene promoter.

摘要

由两个不同基因(USF1和USF2)编码的普遍存在的上游刺激因子(USF)转录因子以能够结合E盒的各种二聚体形式存在。我们报告了USF2亚型的分子克隆和功能表征,这些亚型对应于一个44 kDa的亚基USF2a和一个通过可变剪接产生的新的38 kDa亚基USF2b。使用特异性抗USF抗体,我们在各种核提取物中定义了不同的结合复合物。在体内,USF1/USF2a异二聚体占USF结合活性的66%以上,而USF1和USF2a同二聚体占比不到10%,这强烈表明在体内异二聚体中存在优先关联。特别是,在某些细胞中,USF1/USF2b异二聚体占USF种类的近15%。USF亚基的优先异二聚化在体外得以重现,而共翻译亚基或重组USF蛋白的体外关联似乎是随机的。在瞬时转染的HeLa细胞或肝癌细胞中,USF2a和USF1同二聚体以相似的效率激活一个最小启动子,而缺少一个内部67个氨基酸结构域(67-amino acid domain)的USF2b是一个较差的转录激活因子。此外,在激活肝脏特异性丙酮酸激酶基因启动子方面,USF2b与USF1和USF2a同二聚体一样有效。

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