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肺炎支原体P1蛋白羧基端基因片段在大肠杆菌中克隆的研究
引用本文:王桂珍,李保强,董占双,刘忠顺. 肺炎支原体P1蛋白羧基端基因片段在大肠杆菌中克隆的研究[J]. 微生物学杂志, 2001, 21(2): 13-14
作者姓名:王桂珍  李保强  董占双  刘忠顺
作者单位:1. 中国医科大学病原生物教研室,
2. 中国人民解放军 202医院,
基金项目:辽宁省自然科学基金资助项目(519068)
摘    要:在大肠杆菌中克隆肺炎支原体P1蛋白羧基端基因片段,为P1蛋白基因片段的扩增、表达及探讨羧基端基因片段功能打基础.采用PCR扩增方法获取P1结构基因.扩增产物用SalI和EcoRI酶切消化,回收1kb大小的DNA片段并与pUC19DNA连接,转入大肠杆菌JM109菌株.用X-gal平板及质粒图谱分析方法筛选重组克隆株,再用限制性核酸内切酶酶切图谱分析鉴定.经PCR扩增MPDNA获得1条5.0kbDNA片段.重组质粒限制性内切酶指纹图谱显示出2条带,1条为pUC19载体DNA带,另1条是1kb的插入片段.实验获得肺炎支原体P1蛋白结构基因及含P1蛋白羧基端DNA片段的重组克隆株.

关 键 词:肺炎支原体  P1蛋白  基因克隆
文章编号:1005-7021(2001)02-0013-02
修稿时间:2000-12-25

CLONING OF P1 PROTEIN C END GENE FRAGMENT OF Mycoplasma pneumonia INTO E.coli
Wang Guizhen et al.. CLONING OF P1 PROTEIN C END GENE FRAGMENT OF Mycoplasma pneumonia INTO E.coli[J]. Journal of Microbiology, 2001, 21(2): 13-14
Authors:Wang Guizhen et al.
Affiliation:Dept. Phathogenic Biol.Coll. Basic Med. Sci. China Med. Univ. Shenyang 110001
Abstract:Cloning of P1 protein C end gene fragment of M. pneumonia into E. coli laid a foundation of its amplification, expression, and probe into its function. The P1 structure gene was amplified by PCR method. The 1kb DNA fragments were recovered and linked with pUC19 vector DNA, then transformed into E. coli JM109. The recombinant clones was screened by X-gal plate and plasmid map analysis, and identified by restricted enzyme mapping analysis. A 5.0kb DNA fragment was obtained by MP DNA amplified with PCR. The fingerprint of endonuclease mapping of the recombinant plasmid showed two bands, one was pUC19 DNA band, and the other was 1kb insert fragment.
Keywords:Mycoplasma pneumonia   P1 protein   gene cloning.
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