突变SOD1cDNA亚克隆入酵母穿梭表达质粒pGBKT7中 Subcloning Mutant SOD1cDNA into pGBKT7 of Yeast Expression Plasmid期刊界 All Journals 搜尽天下杂志传播学术成果专业期刊搜索期刊信息化学术搜索

突变SOD1cDNA亚克隆入酵母穿梭表达质粒pGBKT7中

引用本文：	陈桂生,史树贵,李露斯,陈康宁,袁顺宗,彭旭,吴军,罗高兴. 突变SOD1cDNA亚克隆入酵母穿梭表达质粒pGBKT7中[J]. 中国药业, 2008, 17(1): 3-4

作者姓名：	陈桂生史树贵李露斯陈康宁袁顺宗彭旭吴军罗高兴

作者单位：	1. 第三军医大学西南医院神经内科,重庆,400038 2. 第三军医大学西南医院烧伤研究所,重庆,400038

基金项目：	国家自然科学基金资助项目,项目编号:30300116

摘要：	目的将突变SOD1cDNA亚克隆入酵母穿梭表达质粒pGBKT7中。方法利用PCR方法从重组子pEGFP—N2-mSOD1中扩增突变的SOD1cDNA片断。以EcoRⅠ／salⅠ双酶切突变SOD1cDNA片断和酵母穿梭表达质粒pGBKT7，在T4DNA连接酶的作用下，连接突变SOD1cDNA片断和酵母穿梭表达质粒pGBKT7。转化感受态DH5α，筛选重组子，进行双酶切和测序鉴定。结果经酶切和测序鉴定，突变SOD1cDNA成功地亚克隆入酵母穿梭表达质粒pGBKT7中。结论亚克隆成功，可以对目的基因进行下一步研究。
关键词：	突变SOD1cDNA 亚克隆 pGBKT7
文章编号：	1006-4931(2008)01-0003-02
修稿时间：	2007-10-16
Subcloning Mutant SOD1cDNA into pGBKT7 of Yeast Expression Plasmid

Chen Guisheng,Shi Shugui,Li Lusi,Chen Kangning,Yuan Shunzong,Peng Xu,Wu Jun,Luo Gaoxing. Subcloning Mutant SOD1cDNA into pGBKT7 of Yeast Expression Plasmid[J]. China Pharmaceuticals, 2008, 17(1): 3-4

Authors:	Chen Guisheng Shi Shugui Li Lusi Chen Kangning Yuan Shunzong Peng Xu Wu Jun Luo Gaoxing

Affiliation:	Chen Guisheng, Shi Shugui, Li Lusi, Chen Kangning, Yuan Shunzong, Peng Xu2, Wu Jun, Luo Gaoxing (1. Department of Neurology, the Affiliated Southwest Hospital of Third Military Medical University, Chongqing, China 400038; 2. Research Institute of Burn, the Affiliated Southwest Hospital of Third Military Medical University, Chongqing, China 400038)

Abstract:	Objective To subelone mutant SODleDNA into pGBKT7 of yeast expression plasmid. Methods The SODleDNA fragment was gotten from pEGFP- N2- mSODleDNA by polymer ease reaction （PCR）. After digestion by Sal I and EeoR Ⅰ,mSOD1 fragment was subeoloned into pGBKT7 of yeast two hybird expression plasmid by action of T4 ligase. To transform competence DH5α, screening reeon by double enzyme cutting and sequencing. Results The mSOD1 fragment was subeoloned into pGBKT7 of yeast two hybird expression plasmid by identification of double enzyme cutting and sequenein. Conclusion To succeed subeloning is helpful to the next research of mutant SOD1.

Keywords:	mutant SOD1cDNA subclone pGBKT7
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