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用于测量人偏肺病毒中和抗体的微量中和测定法。

Microneutralization assay for the measurement of neutralizing antibodies to human metapneumovirus.

机构信息

Department of Medicine, Rochester General Hospital, Rochester, NY 14621-3001, USA.

出版信息

J Clin Virol. 2009 Dec;46(4):314-7. doi: 10.1016/j.jcv.2009.09.020. Epub 2009 Oct 8.

Abstract

BACKGROUND

Human metapneumovirus (hMPV) is a newly discovered virus which causes respiratory illness in persons of all ages.

OBJECTIVE

A simple and rapid method to determine neutralizing antibody titers against hMPV is needed to facilitate the development of vaccines and therapeutics for hMPV. Therefore, we sought to adapt the methodology used for RSV microneutralization assay (MNA) to measure neutralizing antibody titers against hMPV.

STUDY DESIGN

Serial 2-fold dilutions of serum were made in 96 well microtiter plates and incubated with approximately 50pfu of hMPV A or B strain for 60min at room temperature. LLC-MK2 cells were added to the serum-virus mixtures and plates incubated at 35 degrees C in CO(2) for 5 days. Plates were fixed with acetone; air dried, blocked and then developed with monoclonal antibody to the hMPV N protein followed by horse radish peroxidase labeled antibody and substrate. Neutralization titer was defined as the titer of serum that reduced color development by 50% compared to the positive control wells.

RESULTS

Titers measured by MNA correlated well with those determined by standard plaque reduction assay (R=0.77). Neutralization titers determined by MNA demonstrated excellent inter-assay variability (coefficient of variance=7%). In addition, there was good correlation of antibody titers from 10 hMPV infected adults measured by MNA using either group A or group B hMPV (R=0.87).

CONCLUSION

MNA is a simple and reproducible method for the measurement of serum neutralizing antibody against hMPV.

摘要

背景

人偏肺病毒(hMPV)是一种新发现的病毒,可引起各年龄段人群的呼吸道疾病。

目的

需要一种简单、快速的方法来确定针对 hMPV 的中和抗体滴度,以促进 hMPV 疫苗和疗法的开发。因此,我们试图采用用于 RSV 微量中和测定(MNA)的方法来测量针对 hMPV 的中和抗体滴度。

研究设计

将血清进行连续 2 倍稀释,在 96 孔微量滴定板中进行孵育,室温下与约 50pfu 的 hMPV A 或 B 株孵育 60min。将 LLC-MK2 细胞加入血清-病毒混合物中,在 CO(2)中于 35°C 孵育 5 天。用丙酮固定平板;风干,封闭,然后用针对 hMPV N 蛋白的单克隆抗体开发,然后用辣根过氧化物酶标记的抗体和底物开发。中和滴度定义为与阳性对照孔相比,颜色发展减少 50%的血清滴度。

结果

MNA 测量的滴度与标准蚀斑减少测定法(R=0.77)测定的滴度密切相关。MNA 确定的中和滴度显示出极好的实验内变异性(变异系数=7%)。此外,使用 MNA 通过 MNA 测量的 10 名 hMPV 感染成人的抗体滴度之间也存在良好的相关性,无论是使用 A 组还是 B 组 hMPV(R=0.87)。

结论

MNA 是一种简单、可重复的方法,可用于测量针对 hMPV 的血清中和抗体。

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