首页> 美国卫生研究院文献>Mediterranean Journal of Hematology and Infectious Diseases >Development of an Improved Epstein-Barr Virus (EBV) Neutralizing Antibody Assay to Facilitate Development of a Prophylactic gp350-Subunit EBV Vaccine
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Development of an Improved Epstein-Barr Virus (EBV) Neutralizing Antibody Assay to Facilitate Development of a Prophylactic gp350-Subunit EBV Vaccine

机译:改进的爱泼斯坦-巴尔病毒(EBV)中和抗体检测方法的开发以促进预防性gp350亚基EBV疫苗的开发

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摘要

No licensed vaccine is available for prevention of EBV-associated diseases, and robust, high-throughput bioanalytical assays are needed to evaluate immunogenicity of gp350 subunit-based candidate EBV vaccines. Here we have developed an improved EBV-GFP based neutralization assay for such a vaccine’s pre-clinical and clinical validation to measure EBV specific neutralizing antibodies in human donors. The supplementation of guinea pig complement of our previously published high-throughput EBV-GFP fluorescent focus (FFA)-based neutralization assay allowed the detection of complement-dependent neutralizing antibodies using a panel of heat-inactivated healthy human sera. Anti-gp350 antibody titers, which were evaluated using a previously optimized anti-gp350 IgG ELISA assay, were moderately correlated to the FFA-based neutralization titers. Overall, this improved high-throughput neutralization assay is capable of characterizing the serologic neutralizing antibody response to natural EBV infection, with applications in evaluating EBV antibody status in epidemiologic studies and immunogenicity of candidate gp350-subunit EBV vaccines in clinical studies.
机译:没有获得许可的疫苗可用于预防与EBV相关的疾病,并且需要强大,高通量的生物分析方法来评估基于gp350亚基的候选EBV疫苗的免疫原性。在这里,我们针对这种疫苗的临床前和临床验证开发了一种改进的基于EBV-GFP的中和测定法,以测量人类供体中的EBV特异性中和抗体。补充我们先前发表的基于高通量EBV-GFP荧光聚焦(FFA)的中和试验的豚鼠补体,可以使用一组热灭活的健康人血清检测补体依赖性中和抗体。使用先前优化的抗gp350 IgG ELISA分析评估的抗gp350抗体滴度与基于FFA的中和滴度适度相关。总体而言,这种改进的高通量中和测定法能够表征对天然EBV感染的血清中和抗体反应,并在流行病学研究中评估EBV抗体状态并在临床研究中评估候选gp350亚基EBV疫苗的免疫原性。

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