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人核因子CBF/NF-Y对grp78/BiP启动子近端CCAAT调控元件的钙敏感转录激活作用。

Calcium-sensitive transcriptional activation of the proximal CCAAT regulatory element of the grp78/BiP promoter by the human nuclear factor CBF/NF-Y.

作者信息

Roy B, Li W W, Lee A S

机构信息

Department of Biochemistry and Molecular Biology and the Norris Comprehensive Cancer Center, University of Southern California School of Medicine, Los Angeles, California 90033-0800, USA.

出版信息

J Biol Chem. 1996 Nov 15;271(46):28995-9002. doi: 10.1074/jbc.271.46.28995.

DOI:10.1074/jbc.271.46.28995
PMID:8910550
Abstract

Transcription of the gene encoding GRP78/BiP, a calcium-binding molecular chaperone localized in the endoplasmic reticulum, is induced in mammalian cells through gradual depletion of the intracellular calcium stores. The multimeric CCAAT binding factor, CBF/NF-Y, binds to the most proximal CCAAT regulatory element (C1) of the grp78 promoter required for both basal level expression and stress response. Using an in vitro transcription system, we show through factor competition and immunodepletion that the grp78 C1-mediated enhancement of transcription requires primarily CBF. Correlating with the previous observation that CBF binding to the 78C1 site is enhanced by EGTA and EDTA, these divalent cation chelators specifically stimulate 78C1-directed transcription. In contrast, increasing amounts of calcium ions are inhibitory. These results provide evidence that CBF is functionally important in transactivating the grp78 C1 transcriptional activity, and suggest a possible mechanism by which grp78 transcription is stimulated by calcium depletion. We further discovered that in addition to binding CBF, both the 78C1 element and the CBF binding site of the alpha2(I) collagen promoter interact weakly with the multifunctional transcription factor YY1. Our studies show that the binding sites for CBF and YY1 are distinct for the two promoter sites, suggesting that YY1 and other interacting factors could exert differential effects on individual promoters bearing the same CBF site.

摘要

编码GRP78/BiP(一种定位于内质网的钙结合分子伴侣)的基因转录,在哺乳动物细胞中通过细胞内钙储备的逐渐耗尽而被诱导。多聚体CCAAT结合因子CBF/NF-Y,与grp78启动子最靠近近端的CCAAT调控元件(C1)结合,该元件对于基础水平表达和应激反应都是必需的。使用体外转录系统,我们通过因子竞争和免疫去除实验表明,grp78 C1介导的转录增强主要需要CBF。与之前观察到的EGTA和EDTA增强CBF与78C1位点的结合相一致,这些二价阳离子螯合剂特异性地刺激78C1指导的转录。相反,钙离子浓度增加则具有抑制作用。这些结果证明CBF在激活grp78 C1转录活性方面具有重要功能,并提示了一种可能的机制,即钙耗竭如何刺激grp78转录。我们进一步发现,除了结合CBF外,α2(I)胶原启动子的78C1元件和CBF结合位点都与多功能转录因子YY1存在弱相互作用。我们的研究表明,CBF和YY1在两个启动子位点的结合位点是不同的,这表明YY1和其他相互作用因子可能对带有相同CBF位点的单个启动子产生不同的影响。

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