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首页> 外文期刊>Journal of Virological Methods >Estimation of the number of infectious measles viruses in live virus vaccines using quantitative real-time PCR.
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Estimation of the number of infectious measles viruses in live virus vaccines using quantitative real-time PCR.

机译:使用定量实时PCR估算活病毒疫苗中的麻疹传染性病毒数量。

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The potency of live attenuated virus vaccines is determined by counting or titrating viable viruses in cell cultures. These classical potency tests have the drawback that they are time consuming and laborious and show a high laboratory-to-laboratory variation. In the present study we describe the development and validation of a fast method to measure the potency of measles in trivalent measles, mumps and rubella (MMR) vaccines using quantitative real-time PCR (qPCR). Vero cells were infected with serial dilutions of a trivalent vaccine or a trivalent reference with known potency. Virus was allowed to replicate and subsequently replicated virus was quantitated by qPCR using the LightCycler technology. The virus titer in vaccine samples was estimated against reference preparations using parallel line analysis. In comparison to the plaque assay, the qPCR infectivity assay was faster and less laborious, while accuracy and intermediate precision were similar.
机译:减毒活疫苗的效力通过计数或滴定细胞培养物中的活病毒来确定。这些经典的效能测试具有耗时且费力的缺点,并且显示出实验室之间差异很大。在本研究中,我们描述了使用定量实时PCR(qPCR)测量三价麻疹,腮腺炎和风疹(MMR)疫苗中麻疹效价的快速方法的开发和验证。 Vero细胞用已知效力的三价疫苗或三价参考品的系列稀释液感染。允许病毒复制,然后使用LightCycler技术通过qPCR对随后复制的病毒进行定量。使用平行线分析,相对于参考制剂估计疫苗样品中的病毒滴度。与噬菌斑测定相比,qPCR感染性测定更快,更省力,而准确性和中等精度相似。

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