Development and Validation of a Gamma Interferon ELISPOT Assay for Quantitation of Cellular Immune Responses to Varicella-Zoster Virus

Jeffrey G. Smith, Xu Liu, R. Kaufhold, J. Clair, M. Caulfield
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引用次数: 169

Abstract

ABSTRACT Cell-mediated immunity appears to be critical for the prevention and control of varicella-zoster virus (VZV) infection and complications arising from zoster. Current assays of VZV-specific cell-mediated immunity are cumbersome or lack sensitivity. We have developed a gamma interferon ELISPOT assay that provides a direct measure of the number of T cells secreting a cytokine following stimulation with antigen. This assay is extremely sensitive and specific, with the ability to detect gamma interferon spot-forming cells (SFC) in the range of 10 to 1,000 SFC per million peripheral blood mononuclear cells (PBMCs). This assay has been validated by demonstrating the following: (i) the response detected is mediated almost entirely by CD4+ T cells, (ii) ELISPOT responses from fresh-frozen PBMCs are equivalent to those from freshly isolated cells, (iii) frozen PBMCs can be shipped on dry ice for up to 48 h without loss of activity, (iv) frozen PBMC samples can be stored in liquid nitrogen over long periods (>22 months) without any significant change in response, and (v) the numbers of ELISPOTs counted using a computer-based imaging system are equivalent to those counted by humans but have lower variability. The ability to use frozen cells is facilitated by the use of a recombinant nuclease (Benzonase) that can prevent cell clumping when samples are thawed. Frozen PBMC samples can be cycled through multiple changes in storage between liquid nitrogen and dry ice without any change in response being detected. This facilitates collection of samples at one site and testing performed at a remote location. This VZV ELISPOT assay provides a new versatile tool for monitoring cellular immune responses either during a herpes zoster disease outbreak or following vaccination.
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用于水痘-带状疱疹病毒细胞免疫应答定量的γ干扰素ELISPOT测定方法的建立和验证
细胞介导的免疫似乎对预防和控制水痘-带状疱疹病毒(VZV)感染和带状疱疹引起的并发症至关重要。目前的vzv特异性细胞介导免疫测定方法繁琐或缺乏敏感性。我们开发了一种γ干扰素ELISPOT检测方法,可直接测量抗原刺激后分泌细胞因子的T细胞数量。这种检测方法非常敏感和特异,能够检测到γ干扰素斑点形成细胞(SFC),范围为每百万外周血单个核细胞(PBMCs) 10至1,000 SFC。该分析已通过演示以下内容得到验证:(i)检测到的反应几乎完全由CD4+ T细胞介导,(ii)新鲜冷冻的PBMC的ELISPOT反应与新鲜分离的细胞相当,(iii)冷冻的PBMC可以在干冰上运输长达48小时而不失去活性,(iv)冷冻的PBMC样品可以在液氮中长期储存(>22个月)而没有任何明显的反应变化。(v)使用计算机成像系统计数的elispot数量与人类计数的数量相当,但变异性较低。使用重组核酸酶(苯并酶)可以在样品解冻时防止细胞结块,从而促进了使用冷冻细胞的能力。冷冻的PBMC样品可以在液氮和干冰之间多次循环储存,而不会检测到任何响应变化。这有利于在一个地点收集样品,并在远程地点进行测试。这种VZV ELISPOT检测提供了一种新的多功能工具,用于在带状疱疹疾病爆发期间或接种疫苗后监测细胞免疫反应。
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