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Development of in vitro and in vivo rabies virus neutralization assays based on a high-titer pseudovirus system

机译:基于高滴定瘤系统的体外和体内狂犬病病毒中和测定的发展

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Pseudoviruses are useful virological tools because of their safety and versatility; however the low titer of these viruses substantially limits their wider applications. We developed a highly efficient pseudovirus production system capable of yielding 100 times more rabies pseudovirus than the traditional method. Employing the high-titer pseudoviruses, we have developed robust in vitro and in vivo neutralization assays for the evaluation of rabies vaccine, which traditionally relies on live-virus based assays. Compared with current rapid fluorescent focus inhibition test (RFFIT), our in vitro pseudovirus-based neutralization assay (PBNA) is much less labor-intensive while demonstrating better reproducibility. Moreover, the in vivo PBNA assay was also found to be superior to the live virus based assay. Following intravenous administration, the pseudovirus effectively infected the mice, with dynamic viral distributions being sequentially observed in spleen, liver and brain. Furthermore, data from in vivo PBNA showed great agreement with those generated from the live virus model but with the experimental time significantly reduced from 2 weeks to 3 days. Taken together, the effective pseudovirus production system facilitated the development of novel PBNA assays which could replace live virus-based traditional assays due to its safety, rapidity, reproducibility and high throughput capacity.
机译:假冒病毒是有用的病毒学工具,因为他们的安全性和多功能性;然而,这些病毒的低滴度基本上限制了其更广泛的应用。我们开发了一种高效的伪病毒生产系统,能够产生比传统方法更高的狂犬病症多病毒。采用高滴度伪病毒,我们在体外和体内中和测定中进行了稳健,用于评估狂犬病疫苗,其传统上依赖于基于病毒的测定。与目前的快速荧光聚焦抑制试验相比(RFFIT)相比,我们的体外伪病毒的中和中和测定(PBNA)的劳动密集较小,同时展示了更好的再现性。此外,还发现体内PBNA测定的基于活病毒的测定。在静脉内给药后,伪病毒有效地感染了小鼠,在脾脏,肝癌和脑中依次观察到动态病毒分布。此外,来自Vivo PBNA的数据与从活病毒模型产生的人表现出很大的一致,但实验时间从2周到3天显着降低。在一起,有效的假瘤生产系统促进了新的PBNA测定的开发,这可能是由于其安全性,快速,可重复性和高吞吐量的能力取代了基于病毒的传统测定。

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