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Development of a novel vaccinia-neutralization assay based on reporter-gene expression.

机译:基于报告基因表达的新型疫苗中和测定方法的开发。

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In anticipation of large-scale smallpox vaccination, clinical trials of new vaccine candidates with improved safety profiles, and new vaccinia immune globulin (VIG) products, there is an immediate need to develop new assays to measure vaccinia-specific immune responses. The classical assay to measure vaccinia neutralization, the plaque-reduction neutralization test (PRNT), is slow, labor intensive, and difficult to validate and transfer. Here we describe the development of a novel vaccinia-neutralization assay based on the expression of a reporter gene, beta-galactosidase (beta-Gal). Using a previously constructed vaccinia-beta-Gal recombinant virus, vSC56, we developed a neutralization assay that is rapid, sensitive, and reproducible. The readout is automated. We show that the neutralizing titers, ID(50), for several VIG products measured by our assay were similar to those obtained by PRNTs. A new Food and Drug Administration VIG standard was established for distribution to other laboratories. The newassay will serve as an important tool both for preclinical and clinical trials of new smallpox vaccines and for evaluation of therapeutic agents to treat vaccine-associated adverse reactions.
机译:在期待大规模天花疫苗接种,具有改进的安全性的新型候选疫苗和新型牛痘免疫球蛋白(VIG)产品的临床试验中,迫切需要开发新的测定方法来测量牛痘特异性免疫反应。减少痘苗中和试验(PRNT)是经典的测定牛痘中和的方法,测定速度慢,劳动强度大,并且难以验证和转移。在这里,我们基于报告基因β-半乳糖苷酶(β-Gal)的表达描述了一种新型的牛痘中和测定方法的开发。使用以前构建的牛痘-β-Gal重组病毒vSC56,我们开发了一种快速,灵敏且可重现的中和测定方法。读数是自动的。我们显示,通过我们的测定测得的几种VIG产品的中和效价ID(50)与PRNTs相似。建立了新的食品药品监督管理局VIG标准,以分发给其他实验室。新方法将成为新天花疫苗的临床前和临床试验以及评估与疫苗相关的不良反应的治疗剂的重要工具。

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