Lee S H, Wang X, DeJong J
Department of Molecular and Cell Biology, The University of Texas at Dallas, 2601 North Floyd Road, Richardson, TX 75080, USA.
Nucleic Acids Res. 2000 May 15;28(10):2091-8. doi: 10.1093/nar/28.10.2091.
The phenobarbital-inducible rat cytochrome P450 (CYP) 2B1 and 2B2 proteins are encoded by homologous genes whose promoters contain a mammalian-apparent long terminal repeat retrotransposon (MaLR). An NF-kappaB-like site within the MaLR forms multiple protein-DNA complexes with rat liver and HeLa cell nuclear extracts. Using antibody supershift assays, we have identified these complexes as NF-kappaB and RPB-Jkappa/CBF1. Competition assays using a series of single site mutant oligonucleotides reveal that the recognition sites for these two factors overlap. We also show that the CYP2B1/2 NF-kappaB element, but not the Igkappa NF-kappaB element, can repress transcription in vitro when positioned upstream of the heterologous adenovirus major late core promoter. In addition, RBP-Jkappa over-expressed in COS-7 cells repressed expression in vivo from an SV40-luciferase reporter construct that contained the CYP2B1/2 NF-kappaB element. Finally, we observe similar levels of NF-kappaB and RBP-Jkappa binding activities in nuclear extracts prepared from control and phenobarbital-induced rat livers. The results suggest that RBP-Jkappa/CBF1 binds an atypical NF-kappaB site in the CYP2B1/2 promoters and may help to maintain a low level of expression in the absence of inducer.
苯巴比妥诱导的大鼠细胞色素P450(CYP)2B1和2B2蛋白由同源基因编码,其启动子含有一个哺乳动物明显的长末端重复逆转座子(MaLR)。MaLR内的一个类NF-κB位点与大鼠肝脏和HeLa细胞核提取物形成多种蛋白质-DNA复合物。使用抗体超迁移试验,我们已将这些复合物鉴定为NF-κB和RPB-Jκ/CBF1。使用一系列单一位点突变寡核苷酸的竞争试验表明,这两种因子的识别位点重叠。我们还表明,当位于异源腺病毒主要晚期核心启动子上游时,CYP2B1/2 NF-κB元件而非Igκ NF-κB元件可在体外抑制转录。此外,在COS-7细胞中过表达的RBP-Jκ可在体内抑制含有CYP2B1/2 NF-κB元件的SV40-荧光素酶报告构建体的表达。最后,我们在从对照和苯巴比妥诱导的大鼠肝脏制备的核提取物中观察到相似水平的NF-κB和RBP-Jκ结合活性。结果表明,RBP-Jκ/CBF1结合CYP2B1/2启动子中的一个非典型NF-κB位点,并可能有助于在没有诱导剂的情况下维持低水平的表达。