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作 者:徐晓霞[1] 夏青娟[1] 徐艳玲[1] 岳立广[1] 惠琦[1] 褚东林 曹玉婷[1] 刘令九[1]
机构地区:[1]长春生物制品研究所有限责任公司,吉林长春130062
出 处:《微生物学免疫学进展》2014年第4期7-10,共4页Progress In Microbiology and Immunology
摘 要:目的建立一种细胞培养与实时荧光RT-PCR相结合的快速检测甲肝病毒滴度的方法。方法根据甲肝病毒(HAV)L-A-1株5'端基因组序列,设计了2条基因特异性引物及一条探针,建立实时荧光RT-PCR法,结合细胞培养检测甲肝病毒滴度,并与ELISA检测法进行比较。结果实验中建立的方法能特异检测甲肝病毒,细胞培养8d检测病毒滴度为lg107.0CCID50/mL。同一样本重复检测3次,批内样本Ct值的变异系数最大为0.89%,批间样本Ct值变异系数最大为1.66%。建立的细胞培养结合实时荧光RT-PCR法(细胞培养8 d)与细胞培养ELISA法(细胞培养28 d)检测甲肝病毒滴度结果差异无统计学意义(P>0.05)。结论该方法具有快速、灵敏、特异等优点,应用于疫苗常规检测有良好前景。Objective To establish a method for the rapid detection of hepatitis A virus by cell culture combined with Taq- Man-based Real-time RT-PCR. Methods The specific primers and probe were designed in the 5 '-NCR of HAV ( L-A- 1). Cell culture combined with TaqMan-based real-time RT-PCR was used in determination of HAV, and compared with detec- tion by ELISA. Results The developed method is able to detect hepatitis A virus after HAV infected 2BS cells. The titer of HAV reaches lgl07~CCIDs0/mLas the HAV infected 2BS cells at 8th day, The coefficients of variation (CV) of intra-and inter-assay are calculated and they were less than 0.89% and 1.66% respectively, when the detection of a sample is re- peated for three times. Cell culture combined with TaqMan-based real-time RT-PCR is used in determination of hepatitis A vaccine, and compared with detection by ELISA, which has no statistical significance( P〉0.05 ). Conclusion Determination of hepatitis A vaccine by cell culture combined with TaqMan-based real-time RT-PCR is sensitive, specific and rapid. It could be applied in detection of HAV in the vaccine production process.
关 键 词:甲型肝炎病毒 细胞培养 实时荧光RT-PCR ELISA
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