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首页> 外文期刊>Japanese Journal of Cancer Research >Enhancer-promoter activity of human papillomavirus type 16 long control regions isolated from cell lines SiHa and CaSki and cervical cancer biopsies.
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Enhancer-promoter activity of human papillomavirus type 16 long control regions isolated from cell lines SiHa and CaSki and cervical cancer biopsies.

机译:从细胞系SiHa和CaSki以及宫颈癌活检组织中分离出的人类乳头瘤病毒16型长控制区的增强子-启动子活性。

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Expression of human papillomavirus 16 (HPV-16) oncogenes is markedly higher in cervical cancer cells than in precancerous cells, and the elevated expression is believed to be required for the malignant phenotypes. We compared cancer cell lines CaSki (with 200 to 400 copies of HPV-16 DNA per cell) and SiHa (with one to two copies of HPV-16 DNA per cell) for the E7 expression in cells and the enhancer-promoter activity of the isolated viral long control region (LCR). Although these parameters per cell were 10-fold higher in CaSki than in SiHa, the levels of the E7 mRNA and protein per HPV DNA copy were 10- to 20-fold higher in SiHa than in CaSki. Characterization of the isolated LCRs showed that, whereas the LCR from CaSki resembled the prototype in structure and activity, the LCR from SiHa, with a deletion of 38 base pairs, enhanced transcription from P97 as assayed by using a plasmid capable of expressing luciferase. The upregulation appeared to be due to removal of one of the silencer YY1-binding sites. Furthermore, we isolated and characterized LCRs from 51 cervical cancer patients' biopsies. Among them, one with a deletion including YY1-binding sites and the other with a substitution in a YY1-motif were found to enhance the transcription. These findings suggest that mutation affecting YY1-motifs in the LCR is one of the mechanisms enhancing the viral oncogene expression in the course of progression of cancer cells.
机译:在宫颈癌细胞中,人乳头瘤病毒16(HPV-16)癌基因的表达明显高于癌前细胞,并且据认为,对于恶性表型,表达的升高是必需的。我们比较了癌细胞系CaSki(每个细胞具有200至400个HPV-16 DNA的拷贝)和SiHa(每个细胞具有1至2个拷贝的HPV-16 DNA)在细胞中E7的表达和增强子的启动子活性。分离的病毒长控制区(LCR)。尽管在CaSki中每个细胞的这些参数比在SiHa中高10倍,但是在SiHa中,每个HPV DNA拷贝的E7 mRNA和蛋白质水平比在CaSki中高10到20倍。分离的LCR的表征显示,尽管来自CaSki的LCR在结构和活性上类似于原型,但通过使用能够表达荧光素酶的质粒进行分析,来自SiHa的LCR(缺失38个碱基对)增强了P97的转录。上调似乎是由于去除了沉默子YY1结合位点之一。此外,我们从51例宫颈癌患者的活检物中分离并鉴定了LCR。在它们之中,发现一个具有包括YY1结合位点的缺失的序列,另一个具有在YY1-基序中被取代的序列的序列可以增强转录。这些发现表明,影响LCR中YY1-基序的突变是在癌细胞进展过程中增强病毒癌基因表达的机制之一。

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