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人8号染色体通过微细胞介导转移至高转移性大鼠肝癌细胞系C5F中。

The microcell mediated transfer of human chromosome 8 into highly metastatic rat liver cancer cell line C5F.

作者信息

Liu Hu, Ye Sheng-Long, Yang Jiong, Tang Zhao-You, Liu Yin-Kun, Qin Lun-Xiu, Qiu Shuang-Jian, Sun Rui-Xia

机构信息

Liver Cancer Institute, Zhong Shan Hospital, Fudan University, Shanghai 200032, China.

出版信息

World J Gastroenterol. 2003 Mar;9(3):449-53. doi: 10.3748/wjg.v9.i3.449.

Abstract

AIM

Our previous research on the surgical samples of primary liver cancer with CGH showed that the loss of human chromosome 8p had correlation with the metastatic phenotype of liver cancer. In order to seek the functional evidence that there could be a metastatsis suppressor gene(s) for liver cancer on human chromosome 8, we tried to transfer normal human chromosome 8 into rat liver cancer cell line C5F, which had high metastatic potential to lung.

METHODS

Human chromosome 8 randomly marked with neo gene was introduced into C5F cell line by MMCT and positive microcell hybrids were screened by double selections of G418 and HAT. Single cell isolation cloning was applied to clone microcell hybrids. Finally, STS-PCR and WCP-FISH were used to confirm the introduction.

RESULTS

Microcell hybrids resistant to HAT and G418 were obtained and 15 clones were obtained by single-cell isolation cloning. STS-PCR and WCP-FISH proved that human chromosome 8 had been successfully introduced into rat liver cancer cell line C5F. STS-PCR detected a random loss in the chromosome introduced and WCP-FISH found a consistent recombination of the introduced human chromosome with the rat chromosome.

CONCLUSION

The successful introduction of human chromosome 8 into highly metastatic rat liver cancer cell line builds the basis for seeking functional evidence of a metastasis suppressor gene for liver cancer harboring on human chromosome 8 and its subsequent cloning.

摘要

目的

我们先前利用比较基因组杂交技术对原发性肝癌手术样本进行的研究表明,人类8号染色体短臂缺失与肝癌的转移表型相关。为了寻找人类8号染色体上可能存在肝癌转移抑制基因的功能证据,我们尝试将正常人类8号染色体导入对肺具有高转移潜能的大鼠肝癌细胞系C5F。

方法

通过微细胞介导的染色体转移(MMCT)将随机标记有新霉素基因的人类8号染色体导入C5F细胞系,并通过G418和次黄嘌呤氨基蝶呤胸腺嘧啶核苷(HAT)双重筛选来筛选阳性微细胞杂种。应用单细胞分离克隆技术克隆微细胞杂种。最后,采用序列标签位点聚合酶链反应(STS-PCR)和全染色体涂染荧光原位杂交(WCP-FISH)来证实导入情况。

结果

获得了对HAT和G418耐药的微细胞杂种,并通过单细胞分离克隆获得了15个克隆。STS-PCR和WCP-FISH证明人类8号染色体已成功导入大鼠肝癌细胞系C5F。STS-PCR检测到导入的染色体存在随机丢失,WCP-FISH发现导入的人类染色体与大鼠染色体发生了一致的重组。

结论

将人类8号染色体成功导入高转移潜能的大鼠肝癌细胞系,为寻找人类8号染色体上肝癌转移抑制基因的功能证据及其后续克隆奠定了基础。

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