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邻苯二酚2,3-双加氧酶基因克隆、定位和高效表达 被引量:13

CLONING,LOCATION AND OVEREXPRESSION OF CATECHOL 2,3-DIOXYGENASE GENE
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摘要 采用特异性引物 ,以菲、芘降解菌株ZL5的代谢性质粒为模板 ,扩增出邻苯二酚 2 ,3-双加氧酶 (C2 3O)基因 .将该基因和表达载体pET - 30a(+)连接 ,转化E .coliJM10 9(DE3) ,获得了高效表达的转化子 .SDS -PAGE结果表明 ,转化子的C2 3O蛋白不仅在细胞内存在 ,而且能被分泌到胞外 ,薄层扫描显示 ,转化子细胞内和细胞外表达蛋白总量占细胞总蛋白的 4 2 % .酶活分析表明 ,分布在转化子细胞内、外的表达蛋白都具有较高的C2 3O比活力 .Southern杂交将菌株ZL5的C2 3O基因定位在内生质粒的不同酶切片段上 .图 5表 1参 Catechol 2,3-dioxygenase(C23O) gene was amplified with the specific primer and the template from plasmid in the strain ZL5 degrading phenanthrene and pyrene. The cloned gene was connected with pET-30a(+) vector carring T7 promotor and transformed to E.coli JM109(DE3), and the overexpressing recombinants were obtained. SDS-PAGE showed that the expressed protein was also secreted to the supernant. The total C23O protein outside and inside the recombinant cells was about 42% of the total cell proteins according to the thin layer scanning. The C23O specific activity was high both in and out of the recombinant cells. Southern blotting showed that the C23O gene was located on different fragments of the resident plasmid digested by different restriction enzymes. Fig 5, Tab 1, Ref 12
作者 张杰 刘永生 冯家勋 柏学亮 张忠泽
机构地区 中国科学院沈阳应用生态研究所 广西大学分子遗传研究所
出处 《应用与环境生物学报》 CAS CSCD 2003年第5期542-545,共4页 Chinese Journal of Applied and Environmental Biology
基金 中国科学院知识创新工程资助项目 (KZCX 2 - 4 0 1 )~~
关键词 邻苯二酚2 3—双加氧酶 基因克隆 高效表达 多环芳烃 杂交定位 PAHs Sphingomonas sp. catechol 2,3-dioxygenase (C23O) location by southern blotting
分类号 Q78 [生物学—分子生物学] Q55 [生物学—生物化学]
  • 相关文献

参考文献12

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二级参考文献16

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应用与环境生物学报
2003年 第5期

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