犬细小病毒TaqMan MGB荧光定量PCR检测方法的建立及应用

中国畜牧兽医

犬细小病毒TaqMan MGB荧光定量PCR检测方法的建立及应用

刘毅¹^，2，吴志明²，闫若潜²，赵明军²，王东方²，赵雪丽²，刘梅芬²，程俊贞²^，3，薛晓^2，4，李宁^1，2

（1.河南科技大学动物科技学院，河南洛阳 471003；2.河南省动物疫病预防与控制中心，河南郑州 450008；3.许昌市动物疫病预防控制中心，河南许昌 461000；4.西南大学动物科技学院，重庆 404100)

修回日期:2014-02-25 出版日期:2014-06-20 发布日期:2014-07-24
通讯作者: 吴志明。E-mail: wuzhiming6@sina.com
作者简介:刘毅（1989—），男，河南人，硕士生，从事动物疫病综合防控技术研究。

Establishment and Application of TaqMan MGB Fluorescent-Quantitative PCR Assay for Detection of Canine Parvovirus

Revised:2014-02-25 Online:2014-06-20 Published:2014-07-24

摘要/Abstract

关键词:

犬细小病毒; TaqMan MGB探针; 荧光定量PCR; 建立; 应用

Abstract: In order to establish a TaqMan MGB fluorescent-quantitative PCR (FQ-PCR) assay for detecting canine parvovirus (CPV) specifically, sensitively and rapidly, a highly sensitive and specific TaqMan MGB FQ-PCR assay was developed using the specific primers and TaqMan MGB probe designed basing on the conservative sequences of VP2 gene of CPV in GenBank. The sensitivity, specificity and repetition assay of FQ-PCR assay were tested, and 46 clinic suspicious CPV infected samples were detected by the FQ-PCR assay in contrast to the routine PCR method. The results indicated that the FQ-PCR was successfully established. The developed FQ-PCR assay was able to detect as little as 1×10¹copies/μL of recombinant pGEX-T/CPV plasmid DNA, and the sensitivity of which was 100 times more than that of the routine PCR. The specificity assay exhibited that positive signals could be obtained from recombinant pGEM-T/CPV plasmid, but not from the genomic DNA or total cDNA of the other 5 kinds of pathogenic microorganism acting as the controls. The repetition tests were carried out by detection repeated 3 times for 3 different concentrations of recombinant pGEX-T/CPV plasmid, and the results indicated that the FQ-PCR was reproducible. Twenty-three positive results from 46 clinic suspicious CPV infected samples were obtained, which showed the better sensitivity than that of the routine PCR, with 19 positive samples from the same 46 suspected samples. The study suggested that the CPV FQ-PCR method was successfully established, and suitable for clinic rapid diagnosing of CPV and early detection of latent infection.

Key words:

canine parvovirus；TaqMan MGB probe；FQmso-bidi-font-family: 宋体" lang="EN-US">-PCR；establishment；application

刘毅，吴志明，闫若潜，赵明军，王东方，赵雪丽，刘梅芬，程俊贞，薛晓，李宁. 犬细小病毒TaqMan MGB荧光定量PCR检测方法的建立及应用[J]. 中国畜牧兽医.

LIU Yi, WU Zhi-ming, YAN Ruo-qian, ZHAO Ming-jun, WANG Dong-fang,ZHAO Xue-li, LIU Mei-fen, CHENG Jun-zhen, XUE Xiao, LI Ning. Establishment and Application of TaqMan MGB Fluorescent-Quantitative PCR Assay for Detection of Canine Parvovirus[J]. .

参考文献

1 卢亦愚，严菊英，冯燕，等. TaqMan-MGB荧光定量RT-PCR技术快速检测H5亚型禽流感病毒［J］. 中国病毒学，2006，21(5)：472～476.
2 刘忠华，黄韧，钟翎，等. 犬细小病毒的PCR诊断试剂盒的研制［J］. 中国实验动物学报，2002，10(3)：161～163.
3 闫若潜，安春霞，刘淑敏，等. 猪传染性胃肠炎与流行性腹泻病毒二重RT-PCR检测方法的建立及应用［J］. 中国畜牧兽医，2012，39(9)：38～42.
4 宋志军，宋长绪，杨增岐，等. 猪生殖与呼吸综合征病毒TaqMan荧光定量RT-PCR检测方法的建立［J］. 中国兽医科学，2006，36(2)：98～102.
5 张维谊，刘健，周锦萍，等. 犬细小病毒PCR检测方法的建立及其临床应用［J］. 中国畜牧兽医，2008，35(8)：96～97.
6 李河林，焦铁军，刘淑红，等. 犬细小病毒病研究进展［J］. 动物医学进展，2008，29(5)：73～77.
7 李英俊，史利军，李刚，等. 犬细小病毒荧光定量PCR检测方法的建立与评价［J］. 中国兽医学报，2010，30(12)：1594～1597.
8 夏咸柱，李六金，武德丽，等. 犬细小病毒性肠炎的诊断研究——犬细小病毒血凝和血凝抑制试验［J］. 中国人民解放军兽医大学学报，1983，3(2)：144～148.
9 熊炜，李健，邱璐，等. Real-time PCR和PCR方法快速检测犬细小病毒［J］. 中国兽医学报，2009，29(1)：36～40.
10 Binn L N, Marchwicki R H, Eckermann E H, et al. Viral antibody studies of laboratory dogs with diarrheal disease［J］. American Journal of Veterinary Research, 1981, 42(10): 1665.
11 Clegg S R, Coyne J, Parker S, et al. Molecular epidemiology and phylogeny reveal complex spatial dynamics in areas where canine parvovirus is endemic［J］. J Virol, 2011, 85(15): 7892～7899.
12 Gabriella E, Alessandra C, Costantina D, et al. Detection of infectious canine parvovirus type 2 by mRNA real-time RT-PCR［J］. Journal of Virological Methods, 2007, 146(1): 202～208.
13 Streck A F, Rüster D, Truyen U, et al. An updated TaqMan real-time PCR for canine and feline parvoviruses［J］. Journal of Virological Methods, 2013, 193(1): 6～8.
14 Waner T, Mazar S, Nachmias E, et al. Evaluation of a dot ELISA kit for measuring immunoglobulin M antibodies to canine parvovirus and distemper virus［J］. Veterinary Record, 2003, 152(19): 588～591.
15 Wang S J, Yang S T, Cheng C F, et al. Isolation and identification of canine parvovirus and sequence analysis of its VP2 gene［J］. Progress in Modern Biomedicine, 2009, 10: 26.
16 Xin X, Chang L Z, Cui C, et al. Isolation and identification of canine parvovirus［J］. Feed Review, 2012, 1:20.

[1]	邢玉娟, 赵尉丹, 朱浩, 秦俊杰, 侯晓礁, 王秀敏. 蛋鸡脂肪肝综合征模型的建立[J]. 《中国畜牧兽医》, 2018, 45(5): 1401-1407.
[2]	刘梅芬, 王淑娟, 闫若潜, 王东方, 曹伟伟, 赵雪丽, 李勤楠, 李宁. 猪瘟病毒巢式RT-PCR检测方法的建立与应用[J]. 《中国畜牧兽医》, 2016, 43(9): 2285-2290.
[3]	程振涛, 岳筠, 张华, 周碧君, 文明, 王开功, 欧德渊, 覃岚, 徐春志. 牛结核分枝杆菌实时荧光定量PCR检测方法的建立及应用[J]. , 2015, 42(8): 1979-1985.
[4]	王隆柏，张志刚，苏永裕，车勇良，吴学敏,周伦江. 5种猪病多重PCR检测方法的建立[J]. 中国畜牧兽医, 2014, 41(2): 21-25.
[5]	苗海明, 顾悦, 杨金丽, 高爱武, 黄亚娟, 王海荣. 蒙古绵羊肌内脂肪沉积相关基因实时荧光定量PCR检测方法的建立[J]. , 2013, 40(9): 37-41.
[6]	傅宏庆, 卢炜, 刘静, 贾红. 大鼠局灶性脑缺血后适应动物模型的建立与评估[J]. 中国畜牧兽医, 2013, 40(8): 72-78.
[7]	安春霞, 闫若潜, 吴志明, 赵明军, 赵雪丽, 王东方, 刘淑敏. 高致病性与低致病性猪繁殖与呼吸综合征病毒二重RT-PCR检测方法的建立及应用[J]. , 2013, (5): 66-70.
[8]	闫若潜, 安春霞, 刘淑敏, 赵雪丽, 郭小玲, 赵明军, 吴志明. 猪传染性胃肠炎与流行性腹泻病毒二重RT-PCR 检测方法的建立及应用[J]. 中国畜牧兽医, 2012, 39(9): 38-42.
[9]	王娟萍, 姚敬明, 赵喜有, 吴忻, 孟帆, 刘文俊, 樊振华, 米瑞娟. 猪细小病毒、猪伪狂犬病病毒和猪圆环病毒2型多重PCR检测方法的建立与应用[J]. 中国畜牧兽医, 2012, 39(8): 48-52.
[10]	邢佑尚, 汪琳, 张灿, 赵胤泽, 栢亚铎, 吴亚琼, 李玉欣. 禽流感免疫噬菌体抗体库构建及ELISA检测方法的建立[J]. , 2012, 39(6): 17-21.
[11]	罗金;刘光远;谢俊仁;田占成;党根生. 马泰勒虫病PCR检测方法的建立和应用[J]. , 2012, 39(2): 28-30.
[12]	曹军平;陆桂平;徐向明;顾敏;徐全刚;刘武杰;彭大新;刘秀梵. 荧光定量RT-PCR检测H5亚型禽流感病毒方法的建立与验证[J]. , 2011, 38(11): 169-174.
[13]	郑秀红;邢莹;贾立军;薛书江;甄立家;张守发. 猪附红细胞体巢式PCR诊断方法的建立及初步应用[J]. , 2011, 38(1): 194-197.
[14]	闫若潜;吴志明;张志凌;盛敏;王英华;拜廷阳. 猪链球菌1、7、9型多重PCR诊断方法的建立及初步应用[J]. , 2009, 36(7): 154-157.
[15]	蒋培红;李亚锋;初汉平;葛中东;冯善祥;孟冬梅;许化乾. 羊场疫病综合防疫体系的建立[J]. , 2008, 1(9): 127-130.