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Generation of Recombinant Rabies Virus CVS-11 Expressing eGFP Applied to the Rapid Virus Neutralization Test

机译:表达eGFP的重组狂犬病病毒CVS-11的产生用于快速中和病毒测试

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The determination of levels of rabies virus-neutralizing antibody (VNA) provides the foundation for the quantitative evaluation of immunity effects. The traditional fluorescent antibody virus neutralization test (FAVN) using a challenge virus standard (CVS)-11 strain as a detection antigen and staining infected cells with a fluorescein isothiocyanate (FITC)-labeled monoclonal antibody, is expensive and high-quality reagents are often difficult to obtain in developing countries. Indeed, it is essential to establish a rapid, economical, and specific rabies virus neutralization test (VNT). Here, we describe a recombinant virus rCVS-11-eGFP strain that stably expresses enhanced green fluorescent protein (eGFP) based on a reverse genetic system of the CVS-11 strain. Compared to the rCVS-11 strain, the rCVS-11-eGFP strain showed a similar growth property with passaging stability in vitro and pathogenicity in vivo. The rCVS-11-eGFP strain was utilized as a detection antigen to determine the levels of rabies VNAs in 23 human and 29 canine sera; this technique was termed the FAVN-eGFP method. The good reproducibility of FAVN-eGFP was tested with partial serum samples. Neutralization titers obtained from FAVN and FAVN-eGFP were not significantly different. The FAVN-eGFP method allows rapid economical, specific, and high-throughput assessment for the titration of rabies VNAs.
机译:狂犬病毒中和抗体(VNA)水平的确定为定量评估免疫效果提供了基础。使用挑战病毒标准(CVS)-11菌株作为检测抗原并用异硫氰酸荧光素(FITC)标记的单克隆抗体对感染的细胞进行染色的传统荧光抗体病毒中和测试(FAVN)昂贵且通常使用高质量的试剂在发展中国家很难获得。确实,建立快速,经济且特定的狂犬病毒中和测试(VNT)非常重要。在这里,我们描述了一种重组病毒rCVS-11-eGFP菌株,该菌株基于CVS-11菌株的反向遗传系统稳定表达增强的绿色荧光蛋白(eGFP)。与rCVS-11菌株相比,rCVS-11-eGFP菌株显示出相似的生长特性,具有体外传代稳定性和体内致病性。 rCVS-11-eGFP菌株被用作检测抗原,以确定23个人和29犬血清中狂犬病VNA的水平;这项技术被称为FAVN-eGFP方法。用部分血清样品测试了FAVN-eGFP的良好再现性。从FAVN和FAVN-eGFP获得的中和效价没有显着差异。 FAVN-eGFP方法可用于滴定狂犬病VNA的快速经济,特异性和高通量评估。

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