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对病毒粒子的生物物理特性进行具体分析,以更精确地定义病毒稳定性。

Biophysical virus particle specific characterization to sharpen the definition of virus stability.

机构信息

Bioprocess R&D Department, Sanofi Pasteur, Marcy l'Étoile, France.

Analytical R&D Department, Sanofi Pasteur, Marcy l'Étoile, France.

出版信息

Eur J Pharm Biopharm. 2018 Nov;132:62-69. doi: 10.1016/j.ejpb.2018.08.006. Epub 2018 Aug 14.

DOI:10.1016/j.ejpb.2018.08.006
PMID:30118752
Abstract

Vaccine thermostability is key to successful global immunization programs as it may have a significant impact on the continuous cold-chain maintenance logistics, as well as affect vaccine potency. Modern biological and biophysical techniques were combined to in-depth characterize the thermostability of a formulated rabies virus (RABV) in terms of antigenic and genomic titer, virus particle count and aggregation state. Tunable resistive pulse sensing (TRPS) and nanoparticle tracking analysis (NTA) were used to count virus particles while simultaneously determining their size distribution. RABV antigenicity was assessed by NTA using a monoclonal antibody that recognize a rabies glycoprotein (G protein) conformational epitope, enabling to specifically count antigenic rabies viruses. Agreement between antigenicity results from NTA and conventional method, as ELISA, was demonstrated. Additionally, NTA and ELISA showed mirrored loss of RABV antigenicity during forced degradation studies performed between 5 °C and 45 °C temperature exposure for one month. Concomitant with decreased antigenicity, emergence of RABV particle populations larger than those expected for rabies family viruses was observed, suggesting RABV aggregation induced by thermal stress. Finally, using a kinetic-based modeling approach to explore forced degradation antigenicity data (NTA, ELISA), a two-step model accurately describing antigenicity loss was identified. This model predicted a RABV shelf-life of more than 3 years at 5 °C; significant loss of antigenicity was predicted for samples maintained several months at ambient temperature. This thorough characterization of RABV forced degradation study originally provided a time-temperature mapping of RABV stability.

摘要

疫苗热稳定性对于成功的全球免疫计划至关重要,因为它可能对冷链的持续维护物流产生重大影响,并影响疫苗效力。现代生物和生物物理技术被结合用于深入研究狂犬病病毒(RABV)在抗原和基因组滴度、病毒粒子计数和聚集状态方面的热稳定性。可调电阻脉冲感测(TRPS)和纳米颗粒跟踪分析(NTA)用于计数病毒颗粒,同时确定它们的尺寸分布。使用单克隆抗体通过 NTA 评估 RABV 抗原性,该抗体识别狂犬病糖蛋白(G 蛋白)构象表位,能够特异性计数抗原性狂犬病病毒。NTA 和 ELISA 之间的抗原性结果的一致性得到了证明。此外,NTA 和 ELISA 显示在 5°C 和 45°C 温度暴露下进行一个月的强制降解研究中,RABV 抗原性呈镜像下降。与抗原性下降同时发生的是,观察到 RABV 粒子群体大于预期的狂犬病病毒家族病毒的出现,表明热应激诱导的 RABV 聚集。最后,使用基于动力学的建模方法探索强制降解抗原性数据(NTA、ELISA),确定了一个准确描述抗原性丧失的两步模型。该模型预测 RABV 在 5°C 下的保质期超过 3 年;在环境温度下保存几个月的样品预测会有明显的抗原性丧失。这项对 RABV 强制降解的深入研究最初提供了 RABV 稳定性的时间-温度映射。

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