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| nm23-H1基因转染前后人大细胞肺癌细胞株抑制消减cDNA文库的构建 | |
| 引用本文: | 叶苏娟,冯志华,朱文,蔡春季,李璐,孙丽亚,万海粟,马力,周清华. nm23-H1基因转染前后人大细胞肺癌细胞株抑制消减cDNA文库的构建[J]. 中国肺癌杂志, 2008, 11(4) |
| 作者姓名: | 叶苏娟 冯志华 朱文 蔡春季 李璐 孙丽亚 万海粟 马力 周清华 |
| 作者单位: | 1. 四川大学华西医院生物治疗国家重点实验室,成都,610041 2. 四川大学华西医院肿瘤中心,成都,610041 3. 天津医科大学总医院天津市肺癌研究所,天津市肺癌转移与肿瘤微环境重点实验室,天津,300052 |
| 基金项目: | 国家自然科学基金,国家自然科学基金 |
| 摘 要: | 背景与目的 已有的研究表明,nm23-H1基因是一个重要的肺癌转移抑制基因,为了筛选与该基因表达相关的差异表达基因.本研究拟构建nm23-H1基因转染前后人大细胞肺癌细胞株(L9981和L9981-nm23-H1)差异表达基因的抑制消减cDNA文库,为进一步筛选、克隆与nm23-H1转移相关的基因奠定基础.方法利用抑制消减杂交(suppressive subtractive hybridization,SSH)技术构建nm23-H1基因转染前后人大细胞肺癌细胞株(L9981和L9981-nm23-H1)间差异表达基因的正向和反向消减cDNA文库,经蓝白菌落筛选克隆,并PCR反应鉴定.结果 成功构建了该两株细胞株差异表达基因的正向和反向消减cDNA文库.经蓝白菌落筛选,正向消减文库总共获得约300个白斑克隆,反向消减文库总共获得约400个白斑克隆,从正反向消减文库中各挑选96个克隆进行PCR扩增检测是否有插入片段,结果显示在挑选的正向文库中有84个克隆有插入片段,反向文库中有83个克隆有插入片段.其片段大小范围为(300-750)bp.结论 抑制消减杂交是克隆差异表达基因的有效方法,我们应用SSH法和T/A克隆技术成功建立了nm23-H1基因转染前后人大细胞肺癌细胞株(L9981和L9981-nm23-H1)差异表达基因的抑制消减cDNA文库.nm23-H1基因在肺癌细胞中的表达可能影响某些转移相关基因的差异表达. |
| 关 键 词: | 肺肿瘤 nm23-H1基因 抑制消减杂交 cDNA文库 转移相关基因 |
Construction of the suppression subtractive cDNA libraries of human large cell lung cancer line L9981 before and after transfection with nm23-H1 gene |
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| YE Sujuan,FENG Zhihua,ZHU Wen,Cai Chunji,Li Lu,SUN Liya,WAN Haisu,Ma Li,ZHOU Qinghua. Construction of the suppression subtractive cDNA libraries of human large cell lung cancer line L9981 before and after transfection with nm23-H1 gene[J]. Chinese journal of lung cancer, 2008, 11(4) | |
| Authors: | YE Sujuan FENG Zhihua ZHU Wen Cai Chunji Li Lu SUN Liya WAN Haisu Ma Li ZHOU Qinghua |
| Abstract: | Background and objective It has been proven that nm23-H1 gene is an important metastatic- suppressed gene of lung cancer. In order to screen the differential expression genes related to nm23-H1, we constructed the suppression subtractive cDNA libraries of human large cell lung cancer line L9981 transfected and untransfected with nm23-H1 gene by suppression subtractive hybridization (SSH) in this study, which lay a solid foundation for further screening and cloning metastatic-related genes of nm23-H1. Methods The forward and reverse suppression subtractive cDNA libraries were constructed in the human large cell lung cancer line L9981 before and after transfection with nm23-H1 gene (L9981 and L9981-nm23-H1) by SSH method. The positive clones were preliminarily screened by blue- white colony, and precisely identified by PCR. Results The suppression subtractive cDNA libraries were successfully constructed in the human large cell lung cancer line L9981 transfected and untransfected with nm23-H1 gene (L9981- nm23-H1 and L9981). After the blue-white screening, about three hundred positive clones in the forward subtracted library and four hundred positive clones in the reverse subtracted library were obtained. Ramdom analysis of 96 clones in each library with colony PCR methods showed that 84 clones in the forward subtracted library and 83 clones in the reverse subtracted library contained (300-750) bp inserts. Conclusion SSH is proved to be an efficient tool for differential expression gene cloning. The forward and reverse suppression subtractive cDNA libraries of human large cell lung cancer line L9981 transfected and untransfected with nm23-H1 gene (L9981-nm23-H1 and L9981) are successfully constructed by SSH and T/A cloning technology. The expression of nm23-H1 gene in the human large cell lung cancer cell lines may affect the differential expression of some metastatic-related genes. |
| Keywords: | Lung neoplasms nm23-H1 gene Suppression subtractive hybridization cDNA library Metastatic-related gene |
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