Kisseljova N P, Zueva E S, Pevzner V S, Grachev A N, Kisseljov F L
Institute of Carcinogenesis, Cancer Research Center, Kashirskoye shosse 24, Moscow 115478, Russia.
Int J Oncol. 1998 Jan;12(1):203-9.
We have explored a possible role of an activated N-ras oncogene in aberrant methylation of CpG clusters in DNAs of transformed cells. Using three lines of hamster cells transformed by Rous sarcoma virus (RSV) and the method of detection of CpG islands as clustered sites for methylation-sensitive restriction enzymes we have demonstrated that in each cell line the transcribed RSV proviruses are integrated in the vicinity of sequence containing the cluster of unmethylated CpG dinucleotides. Two out of three examined CpG clusters had hypermethylation patterns in N-ras-neo- but not in neo-transfected variants of the cell lines. De novo methylation of CpG dinucleotides correlated with transcriptional inactivation of adjacent RSV proviruses that was related neither to the lack of transcriptional factors binding RSV long terminal repeat (LTR) nor to the transcriptional incompetence of the LTR, as measured by reporter gene assays with the LTR cloned from DNA of these cells. These data suggest that activation of N-ras signal transduction pathway in transformed cells may be relevant to long-term inactivation of selective genes by hypermethylation of their CpG islands.
我们探讨了激活的N-ras癌基因在转化细胞DNA中CpG簇异常甲基化过程中可能发挥的作用。利用劳氏肉瘤病毒(RSV)转化的三株仓鼠细胞系,并采用将CpG岛作为甲基化敏感限制酶的聚类位点的检测方法,我们证明在每个细胞系中,转录的RSV前病毒整合在含有未甲基化CpG二核苷酸簇的序列附近。在检测的三个CpG簇中,有两个在细胞系的N-ras-neo转染变体中呈现高甲基化模式,而在neo转染变体中则没有。CpG二核苷酸的从头甲基化与相邻RSV前病毒的转录失活相关,这既与缺乏结合RSV长末端重复序列(LTR)的转录因子无关,也与LTR的转录无能无关,这是通过用从这些细胞DNA中克隆的LTR进行报告基因检测来衡量的。这些数据表明,转化细胞中N-ras信号转导途径的激活可能与通过其CpG岛的高甲基化导致选择性基因的长期失活有关。
