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植物研究 ›› 2016, Vol. 36 ›› Issue (3): 401-408.doi: 10.7525/j.issn.1673-5102.2016.03.013

• 研究报告 • 上一篇    下一篇

农杆菌介导rd29A启动子驱动otsB基因转化紫茉莉的研究

陆玉建1,2,3, 张韩杰3, 韩文瑜2, 沈志强1,4   

  1. 1. 山东省滨州畜牧兽医研究院/博士后科研工作站, 滨州 256600;
    2. 吉林大学博士后科研流动站, 长春 130062;
    3. 滨州学院生命科学系/山东省黄河三角洲野生植物资源开发利用工程技术研究中心, 滨州 256603;
    4. 山东省滨州畜牧兽医研究院, 滨州 256600
  • 收稿日期:2015-11-19 出版日期:2016-05-15 发布日期:2016-05-20
  • 通讯作者: 沈志强,E-mail:bzshenzq@163.com E-mail:bzshenzq@163.com
  • 作者简介:陆玉建(1979-),男,博士,讲师,主要从事细胞工程及分子生物学研究。
  • 基金资助:
    山东省自然科学基金(ZR2012CL14);滨州学院博士基金(2010Y08)

Transformation of Mirabilis jalapa L. with otsB Gene in E.coli Driven by rd29A Promoter from Arabidopsis thaliana

LU Yu-Jian1,2,3, ZHANG Han-Jie3, HAN Wen-Yu2, SHEN Zhi-Qiang1,4   

  1. 1. Postdoctoral Programme, Binzhou Animal Science & Veterinary Medicine Academy, Binzhou 256600;
    2. Postdoctoral Programme, Jilin University, Changchun 130062;
    3. Shandong Provincial Engineering and Technology Research Center for Wild Plant Resources Development and Application of Yellow River Delta, Department of Life Sciences, Binzhou University, Binzhou 256603;
    4. Binzhou Animal Science & Veterinary Medicine Academy, Binzhou 256600
  • Received:2015-11-19 Online:2016-05-15 Published:2016-05-20

摘要: 紫茉莉为紫茉莉科紫茉莉属多年生草本植物,具有较高观赏和药用价值,对重金属和石油污染有较强修复能力。然而目前为止,紫茉莉再生和遗传转化体系尚未建立。本研究以紫茉莉为材料,初步建立起较为稳定的再生体系。通过克隆拟南芥rd29A启动子和大肠杆菌otsB基因,构建了p2300-rd29Apro-otsB植物表达载体。利用根癌农杆菌介导法对紫茉莉进行遗传转化。结果表明,当农杆菌的OD600=0.5,侵染成熟胚或带芽茎段60min,共培养2d,紫茉莉的转化效率较高。通过对筛选出的转基因植株进行PCR检测,显示大肠杆菌otsB基因已成功整合到紫茉莉的基因组中,并可有效的进行转录。

关键词: 紫茉莉, rd29A启动子, otsB基因, 农杆菌, 遗传转化

Abstract: Mirabilis jalapa L. is a perennial herb of Nyctaginaceae. Not only is it a high-value ornamental flowering and greening plants, but also can be used as medicine. M.jalapa L. has good bioremediation function. M.jalapa L. was used as experimental material, and the perfect regeneration system was initially established. The rd29A promoter of Arabidopsis thaliana and otsB gene in E.coli were cloned by PCR respectively. Afterwards, the rd29A promoter and otsB gene were ligated into plasmid p2300-GFP, which would lead to the construction of p2300-rd29A pro-otsB expression vector. Then, the expression vector was introduced into the cells of M.jalapa L. by Agrobacterium-mediated method. The genetic transformation results showed that when the concentration of Agrobacterium was OD600=0.5, the time of infection of mature embryo or nodal stem segments was 60 min, and the co-culture time was 2 d, the transformation efficiency of M.jalapa L. was the highest. By PCR detection, otsB gene was successfully integrated into the genome of M.jalapa L., and the efficient transcription could be performed.

Key words: Mirabilis jalapa L., rd29A promoter, otsB gene, Agrobacterium, genetic transformation

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