Stünkel W, Huang Z, Tan S H, O'Connor M J, Bernard H U
Institute of Molecular and Cell Biology, National University of Singapore, Singapore 117609, Republic of Singapore.
J Virol. 2000 Mar;74(6):2489-501. doi: 10.1128/jvi.74.6.2489-2501.2000.
Two nuclear matrix attachment regions (MARs) bracket a 550-bp segment of the long control region (LCR) containing the epithelial cell-specific enhancer and the E6 promoter of human papillomavirus type 16 (HPV-16). One of these MARs is located in the 5' third of the LCR (5'-LCR-MAR); the other lies within the E6 gene (E6-MAR). To study their function, we linked these MARs in various natural or artificial permutations to a chimeric gene consisting of the HPV-16 enhancer-promoter segment and a reporter gene. In transient transfections of HeLa cells, the presence of either of these two MARs strongly represses reporter gene expression. In contrast to this, but similar to the published behavior of cellular MARs, reporter gene expression is stimulated strongly by the E6-MAR and moderately by the 5'-LCR-MAR in stable transfectants of HeLa or C33A cells. To search for binding sites of soluble nuclear proteins which may be responsible for repression during transient transfections, we performed electrophoretic mobility shift assays (EMSAs) of overlapping oligonucleotides that represented all sequences of these two MARs. Both MARs contain multiple sites for two strongly binding proteins and weak binding sites for additional factors. The strongest complex, with at least five binding sites in each MAR, is generated by the CCAAT displacement factor (CDP)/Cut, as judged by biochemical purification, by EMSAs with competing oligonucleotides and with anti-CDP/Cut oligonucleotides, and by mutations. CDP/Cut, a repressor that is down-regulated during differentiation, apparently represses HPV-16 transcription in undifferentiated epithelials cells and in HeLa cells, which are rich in CDP/Cut. In analogy to poorly understood mechanisms acting on cellular MARs, activation after physical linkage to chromosomal DNA may result from competition between the nuclear matrix and CDP/Cut. Our observations show that cis-responsive elements that regulate the HPV-16 E6 promoter are tightly clustered over at least 1.3 kb and occur throughout the E6 gene. HPV-16 MARs are context dependent transcriptional enhancers, and activated expression of HPV-16 oncogenes dependent on chromosomal integration may positively select tumorigenic cells during the multistep etiology of cervical cancer.
两个核基质附着区(MARs)包围着一段550碱基对的长控制区(LCR)片段,该片段包含人乳头瘤病毒16型(HPV - 16)的上皮细胞特异性增强子和E6启动子。其中一个MAR位于LCR的5'端三分之一处(5'-LCR-MAR);另一个位于E6基因内(E6-MAR)。为了研究它们的功能,我们将这些MAR以各种天然或人工排列方式与一个由HPV - 16增强子 - 启动子片段和一个报告基因组成的嵌合基因相连。在HeLa细胞的瞬时转染中,这两个MAR中的任何一个的存在都会强烈抑制报告基因的表达。与此相反,但与已发表的细胞MAR的行为相似,在HeLa或C33A细胞的稳定转染中,报告基因的表达受到E6-MAR的强烈刺激,并受到5'-LCR-MAR的中度刺激。为了寻找可能在瞬时转染期间负责抑制作用的可溶性核蛋白的结合位点,我们对代表这两个MAR所有序列的重叠寡核苷酸进行了电泳迁移率变动分析(EMSA)。两个MAR都含有两个强结合蛋白的多个位点以及其他因子的弱结合位点。通过生化纯化、使用竞争性寡核苷酸和抗CDP/Cut寡核苷酸的EMSA以及突变判断,最强的复合物是由CCAAT置换因子(CDP)/Cut产生的,每个MAR中至少有五个结合位点。CDP/Cut是一种在分化过程中下调的阻遏物,显然在未分化的上皮细胞和富含CDP/Cut的HeLa细胞中抑制HPV - 16转录。与作用于细胞MAR的 poorly understood机制类似,与染色体DNA物理连接后的激活可能是由于核基质和CDP/Cut之间的竞争。我们的观察结果表明,调节HPV - 16 E6启动子的顺式反应元件紧密聚集在至少1.3 kb范围内,并贯穿E6基因。HPV - 16 MARs是上下文依赖的转录增强子,并且依赖于染色体整合的HPV - 16癌基因的激活表达可能在宫颈癌的多步骤病因学过程中对致瘤细胞进行正向选择。
