Construction of a metastasis-associated gene subtracted cDNA library of human colorectal carcinoma by suppression subtraction hybridization 被引量：4

Construction of a metastasis-associated gene subtracted cDNA library of human colorectal carcinoma by suppression subtraction hybridization

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摘要 AIM: To construct a differentially-expressed gene subtracted cDNA library from two colorectal carcinoma (CRC) cell lines with different metastatic phenotypes by suppression subtractive hybridization.METHODS: Two cell lines of human CRC from the same patient were used. SW620 cell line showing highly metastatic potential was regarded as tester in the forward subtractive hybridization, while SW480 cell line with lowly metastatic potential was treated as tester in the reverse hybridization. Suppression subtractive hybridization (SSH) was employed to obtain cDNA fragments of differentially expressed genes for the metastasis of CRC. These fragments were ligated with T vectors, screened through the blue-white screening system to establish cDNA library.RESULTS: After the blue-white screening, 235 white clones were picked out from the positive-going hybridization and 232 from the reverse. PCR results showed that 200-700 bp inserts were seen in 98% and 91% clones from the forward and reverse hybridizations, respectively.CONCLUSIONS: A subtractive cDNA library of differentially expressed genes specific for metastasis of CRC can be constructed with SSH and T/A cloning techniques. AIM:To construct a differentially-expressed gene subtracted cDNA library from two colorectal carcinoma (CRC) cell lines with different metastatic phenotypes by suppression subtractive hybridization. METHODS:Two cell lines of human CRC from the same patient were used.SW620 cell line showing highly metastatic potential was regarded as tester in the forward subtractive hybridization,while SW480 cell line with lowly metastatic potential was treated as tester in the reverse hybridization.Suppression subtractive hybridization (SSH) was employed to obtain cDNA fragments of differentially expressed genes for the metastasis of CRC.These fragments were ligated with T vectors,screened through the blue- white screening system to establish cDNA library. RESULTS:After the blue-white screening,235 white clones were picked out from the positive-going hybridization and 232 from the reverse.PCR results showed that 200-700 bp inserts were seen in 98% and 91% clones from the forward and reverse hybridizations,respectively. CONCLUSIONS:A subtractive cDNA library of differentially expressed genes specific for metastasis of CRC can be constructed with SSH and T/A cloning techniques.

作者 LiLiang Yan-QingDing XinLi Guang-ZhiYang JunXiao Li-ChunLu Jin-HuaZhang

机构地区 DepartmentofPathology DepartmentofTropicMedicine

出处《World Journal of Gastroenterology》 SCIE CAS CSCD 2004年第9期1301-1305,共5页 世界胃肠病学杂志（英文版）

基金 Supported by the Military Medical Foundation of China,No.01MA128

关键词结直肠癌肿瘤转移相关基因消减cDNA文库消减杂交法聚合酶链反应

分类号 R735.3 [医药卫生—肿瘤]

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World Journal of Gastroenterology

2004年第9期

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