引用本文
  •    [点击复制]
  •    [点击复制]
【打印本页】 【下载PDF全文】 查看/发表评论下载PDF阅读器关闭

←前一篇|后一篇→

过刊浏览    高级检索

本文已被:浏览 2054次   下载 1330 本文二维码信息
码上扫一扫!
利用荧光定量PCR检测猪细小病毒在IBRS-2细胞增殖动态研究
马慧慧,谢红玲
0
(武汉中博生物股份有限公司)
摘要:
为了解猪细小病毒(PPV)在IBRS-2细胞中的增殖规律,建立了基于TaqMan实时荧光定量PCR技术的PPV检测方法,并应用该方法研究PPV在IBRS-2细胞中的增殖动态。结果显示,该方法特异性较好且灵敏度高,可检测低至1.4?100拷贝/μL的病毒量。检测显示PPV接种IBRS-2细胞后12h开始大量增殖,60~72h增殖最为迅速,到72h病毒含量达到最高峰,之后逐渐下降。结果表明所建立的荧光定量PCR检测方法可用于PPV的快速定量检测,对病毒增殖规律的研究为该病毒疫苗的生产提供了科学依据。
关键词:  猪细小病毒  IBRS-2细胞  荧光定量PCR  增殖动态
DOI:
投稿时间:2013-05-30修订日期:2013-07-25
基金项目:
Study on the proliferation dynamics of porcine parvovirus in IBRS-2 cells using Real-time PCR technology
(wuhan chopper biology co.,itd.)
Abstract:
To explore the proliferation dynamics of PPV in IBRS-2 cells,a TaqMan fluorescent quantitative real-time PCR technology was established. The results showed that this method is specific and sensitive for the detection of PPV. Experiment of sensitivity indicated that this method could detect 1.4?100copies/μL viral load at least. After inoculation of PPV, the IBRS-2 cells showed obvious CPE. Virus began to proliferate when the cells infected with PPV after 12 hours, and proliferated rapidly during 60 to 72 hours, viral load achieved the highest value in 72hours and then decreased gradually.This study results indicated that the TaqMan Real-time PCR technology could be used in the rapid quantitative detection of PPV. The proliferation dynamics also could provided a scientific basis for the vaccine production of PPV.
Key words:  porcine parvovirus  IBRS-2 cells  real-time fluorescent quantitative PCR  proliferation dynamics

用微信扫一扫

用微信扫一扫