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山东大学学报(医学版)

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碳青霉烯酶OXA72在毕赤酵母中的表达和纯化

韩进1,吴大玮1,冯进波2,耿治英3,杨蕾1,李巧荣1
  

  1. (1. 山东大学齐鲁医院加强医疗科,济南 250012;2. 教育部和卫生部心血管重构与功能研究重点实验室,济南 250012;3.东营市人民医院呼吸科,山东 东营 257091)
  • 收稿日期:1900-01-01 修回日期:1900-01-01 出版日期:2009-01-16 发布日期:2009-01-16
  • 通讯作者: 吴大玮

Expression and purification of carbapenemase OXA72 in pichia pastoris

HAN Jin1, WU Dawei1, FENG Jinbo2, GENG Zhiying3, YANG Lei1, LI Qiaorong1
  

  1. (1. Department of Intensive Care Unit, Qilu Hospital of Shandong University, Jinan 250012, China;2. Key Laboratory of Cardiovascular Remodeling and Function Research, Chinese Ministry of Education and Chinese Ministry of
    Public Health, Jinan 250012, China;3. Dongying People′s Hospital, Dongying 257091, Shandong, China)
  • Received:1900-01-01 Revised:1900-01-01 Online:2009-01-16 Published:2009-01-16
  • Contact: WU Dawei

摘要: 目的对我国临床分离的第一株鲍曼不动杆菌产生的碳青霉烯酶OXA72在毕赤酵母表达系统中进行重组表达及分离纯化。方法提取临床分离的鲍曼不动杆菌菌株40的基因组DNA,PCR扩增oxa72全基因;将oxa72基因双酶切回收后与毕赤酵母表达载体连接,重组质粒分别以PCR、酶切及测序鉴定;电转化法将线性化的重组表达DNA转导入GS115感受态细胞,在Zeocin平板上筛选阳性转化子,并通过PCR和Western进行验证;对阳性克隆进行头孢硝噻吩实验,检测表达OXA72的活性。用镍柱分离纯化OXA72。结果以该株鲍曼不动杆菌的基因组DNA为模板,用目的引物进行PCR可获得843?bp的特异扩增条带;DNA测序证明核苷酸序列与Genbank公布的oxa72基因序列100%一致;电转化后经Zeocin平板筛选得到一株阳性克隆,SDSPAGE表明重组蛋白的相对分子量在34~43?kDa之间,Westem blot分析显示,重组蛋白能特异地与抗HisTag抗体结合。头孢硝噻吩试验为阳性。纯化得到纯度为95%的重组蛋白,纯化回收率达40%。结论成功构建了OXA72的表达载体,在毕赤酵母中成功地表达并分离纯化了具有酶活性的OXA72。

关键词: 碳青霉烯酶OXA, 巴斯德毕赤酵母, 表达, 纯化

Abstract: To amplify and identify the chromosomal DNA of Acinetobacter Baumanii which is the first isolate producing carbapenemase OXA72 in our country and to express and purify OXA72 in Pichia pastoris. MethodsThis study amplified the oxa72 gene by PCR using the extracted genomic DNA of the isolate 40 which was obtained from the clinic as a template. After the amplified gene was cloned into vector pGAPZalphaA, linearized recombinant plasmid oxa72pGAPZalphaA was transformed to Pichia pastoris GS115 by electroporation. Then the positive transformants were screened by colony PCR, western blot analysis and Nitrocefin test. Then we purified OXA72 with a nickel column. ResultsThe DNA sequence amplified by PCR from isolate 40 was identical with blaOXA72 (GenBank accession numbers AY739646). One positive transformant had a positive Nitrocefin test. SDSPAGE showed that the relative molecular weight of the recombined protein was 34?kDa43kDa. Western blotting showed the combined protein could specifically bind to the Histag antibody. The recombinant protein was obtained by purification with 95% final purity and 40% recovery rate. ConclusionWe successfully expressed and purified the carbapenemase OXA72 in Pichia pastoris.

Key words: Carbapenemase OXA72, Pichia pastoris, Expression, Purification

中图分类号: 

  • R503
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