[1]曹成,魏梅生,吴兴泉,等.菜豆荚斑驳病毒RT-PCR扩增产物胶体金层析检测方法的建立[J].大豆科学,2010,29(06):1024-1027.[doi:10.11861/j.issn.1000-9841.2010.06.1024]
 CAO Cheng,WEI Mei-sheng,WU Xing-quan,et al.Detection of Bean Pod Mottle Virus RT-PCR Amplicon by Dipstick Assay[J].Soybean Science,2010,29(06):1024-1027.[doi:10.11861/j.issn.1000-9841.2010.06.1024]
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菜豆荚斑驳病毒RT-PCR扩增产物胶体金层析检测方法的建立

《大豆科学》[ISSN:1000-9841/CN:23-1227/S] 卷: 第29卷 期数: 2010年06期 页码: 1024-1027 栏目: 出版日期: 2010-12-25
Title:
Detection of Bean Pod Mottle Virus RT-PCR Amplicon by Dipstick Assay
文章编号:
1000-9841(2010)06-1024-04
作者:
曹成1 魏梅生2吴兴泉1张永江2李桂芬2
1.河南工业大学 生物工程学院,河南 郑州 450001;
2. 中国检验检疫科学研究院 动植物检疫研究所,北京 100029
Author(s):
CAO Cheng1 WEI Mei-sheng2 WU Xing-quan1 ZHANG Yong-jiang2 LI Gui-fen2
1.College of Bioengineering, Henan University of Technology, Zhengzhou 450001,Henan;
2.Institute of Animal and Plant Quarantine, Chinese Academy of Inspection and Quarantine, Beijing 100029, China
关键词:
胶体金试纸条菜豆荚斑驳病毒RT-PCR核酸检测
Keywords:
Colloidal goldDipstickBPMVRT-PCR Nucleic acid detection
分类号:
S565.1
DOI:
10.11861/j.issn.1000-9841.2010.06.1024
文献标志码:
A
摘要:
菜豆荚斑驳病毒是我国进境植物检疫性有害生物,为了能在现场快速检测出该病毒,将PCR核酸扩增的高灵敏度和胶体金层析方法快速简便、直观的优点结合起来,建立了PCR扩增产物的胶体金层析检测方法。该方法是用生物素标记上一个引物,用荧光素(或地高辛)标记上另一个引物,通过PCR扩增产生双标记的扩增产物。将兔抗生物素多克隆抗体与20~30 nm大小的胶体金颗粒结合上并固定在释放垫上,同时在硝酸纤维素层析膜上点上抗荧光素(或地高辛)的单克隆抗体作为T检测点,点上羊抗兔多克隆抗体作为C质控点。这种RT-PCR扩增产物可在T点上被检测到,同时C点也要显色。用所建立方法在15 min内可检测出菜豆荚斑驳病毒的RT-PCR扩增产物,免去了溴化乙锭染色和电泳的过程。
Abstract:
Bean pod mottle virus (BPMV) is a quarantine pest for China. In order to detect the virus on site, we have developed a rapid method for detection of RT-PCR amplicon of the virus. The method is performed by labeling one prime with biotin the other primer with fluorescein (or digoxigenin). The dual-labeled amplicon can be generated from routine polymerase chain reaction. Rabbit polyclonal antibody against biotin is conjugated with 20~30 nm colloidal gold particles fixed in a conjugate pad.Monoclonal antibody against fluorescein (or digoxigenin) is spotted on nitrocellulose membrane as T dot. Goat anti-rabbit polyclonal antibody is spotted on nitrocellulose membrane as C dot. The RT-PCR amplicon is detected on the test dot(T dot), while the C dot serves as a control. Using this method we have detected the RT-PCR amplicon of bean pod mottle virus within 15 minutes without the staining of ethidium bromide and the running of agarose gel.

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相似文献/References:

[1]张晓雷,檀根甲,魏梅生,等.GICA-RT-PCR检测菜豆荚斑驳病毒的新方法[J].大豆科学,2008,27(06):1019.[doi:10.11861/j.issn.1000-9841.2008.06.1019]
 ZHANG Xiao-lei,TAN Gen-jia,WEI Mei-sheng,et al.A New Method for Detecting Bean Pod Mottle Virus by GICA-RT-PCR[J].Soybean Science,2008,27(06):1019.[doi:10.11861/j.issn.1000-9841.2008.06.1019]

备注/Memo

基金项目:国家质量监督检验检疫总局资助项目(2009IK322)。

第一作者简介:曹成(1986-),男,在读硕士,从事检疫性植物病毒检测研究。E-mail:lllaohucao@163.com。
通讯作者:魏梅生,研究员。 E-mail: wmsh02@yahoo.com.cn。

更新日期/Last Update: 2014-09-15