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羊痘病毒实时荧光定量TaqMan PCR检测方法的建立
引用本文:康文玉,徐自忠,花群义,杨云庆,周晓黎,董俊,尹尚莲,高洪. 羊痘病毒实时荧光定量TaqMan PCR检测方法的建立[J]. 中国兽医科学, 2006, 36(7): 529-533
作者姓名:康文玉  徐自忠  花群义  杨云庆  周晓黎  董俊  尹尚莲  高洪
作者单位:1. 云南农业大学,动物科学技术学院,云南,昆明,650201
2. 云南出入境检验检疫局,技术中心,云南,昆明,650228
基金项目:国家核工业地质局资助项目
摘    要:参照羊痘病毒(CaPV)P32的基因序列,设计合成了2套引物和1条探针,建立了实时荧光定量PCR技术,对细胞培养物、皮肤丘疹、痂皮等组织病料中的GPV进行了特异性检测和敏感性试验。结果显示,用300 nmol/L引物浓度和200 nmol/L探针浓度,获得的Cr值较小,而△Rn最大;可检测到相当于0.1 TCID50的病毒DNA;制作的标准曲线中各浓度范围内有极好的线性关系且线性范围宽,相关系数为0.999 5以上;组内和组间试验重复性的变异系数分别为2.3%和3.4%;与常规的PCR相比较,该方法具有快速、特异、敏感、可定量,可同时检测大量样品等优点。表明。荧光TaqMan PCR是一种检测CaPV的良好方法,可对组织病料中低含量的CaPV或持续带毒宿主进行准确检测。

关 键 词:羊痘病毒  荧光定量TaqMan PCR  检测
文章编号:1673-4696(2006)07-0529-05
修稿时间:2006-02-13

Development of a real-time fluorescent TaqMan-quantitative PCR assay for detection of capripoxvirus
KANG Wen-yu,XU Zi-zhong,HUA Qun-yi,YANG Yun-qing,ZHOU Xiao-li,DONG Jun,YIN Shang-lian,GAO Hong. Development of a real-time fluorescent TaqMan-quantitative PCR assay for detection of capripoxvirus[J]. Chinese Veterinary Science, 2006, 36(7): 529-533
Authors:KANG Wen-yu  XU Zi-zhong  HUA Qun-yi  YANG Yun-qing  ZHOU Xiao-li  DONG Jun  YIN Shang-lian  GAO Hong
Abstract:A real-time fluorescent TaqMan-quantitative PCR assay using 2 pairs of primers and a probe designed and synthesized according to the P32 gene of the virus genome was developed for the specific detection of capripox virus in epithelial suspensions and cell culture preparations. The real-time fluorescent PCR assay detected specifically CaPV virus in samples with greater sensitivity than the conventional PCR procedure. The fluorescent PCR assay was fast, and could quantitatively assess the virus amounts and could handle more samples and/or replicates of samples in a single assay than the conventional PCR procedure. The results showed that this assay is a valuable complementary tool to the routine diagnostic procedures for the detection of capripox virus infection.
Keywords:capripoxvirus  fluorescent TaqMan-quantitative PCR assay  detection
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