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Construction and selection of subtracted cDNA library of mouse hepatocarcinoma cell lines with different lymphatic metastasis potential

机译:小鼠具有不同淋巴转移潜能的肝癌细胞株减去cDNA文库的构建和选择

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摘要

AIM: In order to elucidate the molecular mechanism of lymphatic metastasis of hepatocarcinoma, we detected the difference of gene expression between mouse hepatocarcinoma cell lines Hca-F and Hca-P with different lymphatic metastasis potential.METHODS: cDNA of Hca-F cells was used as a tester and cDNA of Hca-P cells was used as a driver. cDNAs highly expressed in Hca-F cells were isolated by the suppression subtractive hybridization (SSH) method. The isolated cDNA was cloned into T/A cloning vector. The ligation products were transformed into DH5 α competent cells. Individual clones were randomly selected and used for PCR amplification. Vector DNA from positive clones was isolated for sequencing.RESULTS: There were 800 positive clones in amplified subtracted cDNA library. Random analysis of 160 clones with PCR showed that 95% of the clones contained 100-700 bp inserts. Analysis of 20 sequenced cDNA clones randomly picked from the SSH library revealed 4 known genes (mouse heat shock protein 84 ku, DNA helicase, ribosomal protein S13 ,ethanol induced 6 gene) and 3 expressed sequence tags (ESTs). Four cDNAs showed no homology and presumably represent novel genes.CONCLUSION: A subtracted cDNA library of differentially expressed genes in mouse heptocarcinoma cell lines with different lymphatic metastasis potential was successfully constructed with SSH and T/A cloning techniques. The library is efficient and lays a solid foundation for searching new lymphatic metastasis related genes. The expression of mouse heat shock protein gene, DNA helicase and other 4 novel gene may be different between mouse heptocarcinoma cell lines with different lymphatic metastasis potential.
机译:目的:为阐明肝癌淋巴转移的分子机制,我们检测了具有不同淋巴转移潜能的小鼠肝癌细胞系Hca-F和Hca-P之间的基因表达差异。方法:使用Hca-F细胞的cDNA作为测试者,Hca-P细胞的cDNA被用作驱动程序。通过抑制消减杂交(SSH)方法分离在Hca-F细胞中高表达的cDNA。分离的cDNA被克隆到T / A克隆载体中。将连接产物转化到DH5α感受态细胞中。随机选择单个克隆并用于PCR扩增。结果:从扩增出的cDNA文库中分离出800个阳性克隆。用PCR对160个克隆进行随机分析,结果表明95%的克隆包含100-700 bp插入片段。分析从SSH文库中随机挑选的20个测序的cDNA克隆,发现了4个已知基因(小鼠热休克蛋白84 ku,DNA解旋酶,核糖体蛋白S13,乙醇诱导的6个基因)和3个表达的序列标签(EST)。结论:利用SSH和T / A克隆技术成功构建了具有不同淋巴转移潜能的小鼠肝癌细胞系中差异表达基因的cDNA文库。该库是高效的,并为寻找新的淋巴转移相关基因奠定了坚实的基础。在具有不同淋巴转移潜能的小鼠肝癌细胞系中,小鼠热休克蛋白基因,DNA解旋酶等4种新基因的表达可能不同。

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