引用本文:吴 锟,谢玉波,王连振,肖 强.人胃癌组织定向cDNA文库的构建[J].中国临床新医学,2011,4(5):394-397.
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人胃癌组织定向cDNA文库的构建
吴 锟,谢玉波,王连振,肖 强
530021 南宁,广西医科大学第一附属医院胃肠腺体外科(吴 锟,王连振,肖 强),麻醉科(谢玉波)
摘要:
[摘要] 目的 快速构建成人胃癌组织cDNA文库。方法 从人胃癌组织分离总RNA,以含有Sfi IB酶切位点的oligo(dT)引物合成第1链cDNA,以含Sfi IA酶切位点的SMART寡核苷酸为引物经LD-PCR扩增双链cDNA,双链cDNA经Sfi I(IA & IB)酶切,以CHROMA SPIN+TE-1000柱分级分离cDNA,收集符合需要的cDNA片段并纯化,随后将之与λTripIEx2载体连接经体外包装成噬菌体cDNA文库。结果 经检测共获得2.73×106个重组子,重组率约为94%,插入片段大小平均为1.2 kb。结论 用SMART方法构建的胃癌组织cDNA文库质量较高,为以后筛选胃癌相关基因奠定了基础。
关键词:  cDNA文库  胃癌  定向克隆
DOI:10.3969/j.issn.1674-3806.2011.05.02
分类号:R 735.2
基金项目:国家自然科学基金资助项目(编号:81060201);广西科学研究与技术开发计划项目(编号:桂科攻10124001A-22);中国博士后科学基金特别资助项目(编号:201003342)
Construction of directional cDNA library from human gastric carcinoma tissues
WU Kun,XIE Yu-bo, WANG Lian-zhen, et al.
Department of Gastrointestinal Gland Surgery, the First Affiliated Hospital of Guangxi Medical University,Nanning 530021, China
Abstract:
[Abstract] Objective To quickly construct a directional cDNA library from human gastric carcinoma tissues.Methods The total RNA was separated from mixed human gastric carcinoma tissues, then the first strand cDNA was synthesized with oligo(dT)primer containing Sfi I-digested sites before the double-strand cDNA was amplified through LD-PCR (long-distance PCR) by SMART technology. The double-strand cDNA was digested by Sfi I(IA &IB)restriction enzyme before cDNA size fractionation, the double-strand cDNA fractionated was ligated into λTripIEx2 vector and packaged in vitro.Results The unamplified human gastric carcinoma tissues cDNA library consisted of 2.73×106 independent clones with recombinant clones was 94%. The average size of the recombinants insert 1.2 kb.Conclusion The quality of the constructed human gastric carcinoma tissues cDNA library is excellent and helpful to screen human gastric carcinoma specific antigen.
Key words:  cDNA library  Human gastric carcinoma  Directional cloning