https://www.ahs.ac.cn/images/0513-353X/images/top-banner1.jpg|#|苹果
https://www.ahs.ac.cn/images/0513-353X/images/top-banner2.jpg|#|甘蓝
https://www.ahs.ac.cn/images/0513-353X/images/top-banner3.jpg|#|菊花
https://www.ahs.ac.cn/images/0513-353X/images/top-banner4.jpg|#|灵芝
https://www.ahs.ac.cn/images/0513-353X/images/top-banner5.jpg|#|桃
https://www.ahs.ac.cn/images/0513-353X/images/top-banner6.jpg|#|黄瓜
https://www.ahs.ac.cn/images/0513-353X/images/top-banner7.jpg|#|蝴蝶兰
https://www.ahs.ac.cn/images/0513-353X/images/top-banner8.jpg|#|樱桃
https://www.ahs.ac.cn/images/0513-353X/images/top-banner9.jpg|#|观赏荷花
https://www.ahs.ac.cn/images/0513-353X/images/top-banner10.jpg|#|菊花
https://www.ahs.ac.cn/images/0513-353X/images/top-banner11.jpg|#|月季
https://www.ahs.ac.cn/images/0513-353X/images/top-banner12.jpg|#|菊花

园艺学报 ›› 2009, Vol. 36 ›› Issue (10): 1411-1416.

• 果树 • 上一篇    下一篇

苹果属小金海棠MxIrt1基因特异性片段的原核表达及多克隆抗体的制备

孙春玉1,2;王忆1;孔瑾1;许雪锋1;李天忠1;韩振海1*   

  1. (1中国农业大学园艺植物研究所, 北京100193; 2 吉林农业大学生命科学学院, 长春130118)
  • 收稿日期:2009-03-02 修回日期:2009-08-29 出版日期:2009-10-25 发布日期:2009-10-25
  • 通讯作者: 韩振海

Prokaryotic Expression of MxIrt1 Genes Segment and the Prepara tion of ItsPolyclonal Antibody

SUN Chun-yu1,2;WANG Yi1;KONG Jin1;XU Xue-feng1;L I Tian-zhong1;HAN Zhen-hai1*   

  1. (1 Institute of Horticultural Plants, China AgriculturalUniversity, Beijing 100193, China; 2College of Life Sciences, Jilin Agricultural University,Changchun130118, China)
  • Received:2009-03-02 Revised:2009-08-29 Online:2009-10-25 Published:2009-10-25
  • Contact: HAN Zhen-hai

PDF

1007

摘要: MxIrt1是从苹果属植物小金海棠中克隆出的二价阳离子转运膜蛋白基因。为进一步研究该基
因的功能, 利用MxIrt1基因位于第3和第4跨膜区之间的162 bp片段, 构建了原核表达载体pGEX-MxIrt1,经原核表达、亲和层析、获得GST2MxIRT1融合蛋白, 以融合蛋白为抗原, 制备多克隆抗体, ELISA方法检测抗体效价阳性, 蛋白质印迹检测植物体内总蛋白, 获得与预期大小一致的特异性条带。上述结果表明,表达的目的蛋白可用于免疫组织化学、蛋白质印迹检测。

关键词: 苹果属, 小金海棠, MxIrt1基因, 特异片段, 原核表达, 多克隆抗体

Abstract: MxIrt1 is a iron transport p rotein gene from M alus xiaojinensis. To study the functional characteristic of MxIrt1, the recombinant plasmid pGEX-MxIrt1 was constructed with 162 bp segments between 3 rd and 4 th TMR (Transmembrane region) , following the expression in E.coli with high efficiency, purification using Glutathione Sepharose 4B, the recombinant GST-MxIRT1 protein was obtained. ELISA assay detected the reactivity of the polycolonal antibody andWestern blot shows that specific band was corresponding to the expectation. The recombinant GST-MxIRT1 protein can also be used for immunohistochemistry.

Key words: Malus, Malus xiaojinensis, MxIrt1, specific segment, prokaryotic expression, polyclonal antibody

中图分类号: 

访问总数: 当日访问总数: 当前在线人数:

版权所有 © 2012 《园艺学报》编辑部 京ICP备10030308号-2 国际联网备案号 11010802023439

编辑部地址: 北京市海淀区中关村南大街12号中国农业科学院蔬菜花卉研究所 邮编: 100081

电话: 010-82109523 E-Mail: yuanyixuebao@126.com

技术支持:北京玛格泰克科技发展有限公司