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一种用于检测和定量人血清中抗黄热病毒抗体的微量中和试验的开发与验证。

The development and validation of a microneutralization assay for the detection and quantification of anti-yellow fever virus antibodies in human serum.

作者信息

Fries Katherine, Luo Ping, Baldwin Rebekah, Goldberg Raechel, Ordonez Ivan, Zheng Lingyi, Huleatt James, Devlin Louis

机构信息

Global Clinical Immunology, Sanofi, Swiftwater, Pennsylvania, USA.

Translational and Early Development Biostatistics, Sanofi, Orlando, Florida, USA.

出版信息

Microbiol Spectr. 2025 Apr;13(4):e0334824. doi: 10.1128/spectrum.03348-24. Epub 2025 Mar 4.

Abstract

UNLABELLED

The plaque reduction neutralization test (PRNT) has been used widely for the detection and quantitation of yellow fever (YF) virus-neutralizing antibodies in human serum; however, it is labor-intensive and challenging to adapt to high-throughput clinical testing needed for vaccine licensure. Here, we describe the development and validation of a new Vero cell-based YF microneutralization (MN) assay, with immunostaining readout, for the detection and quantification of YF virus-neutralizing antibodies in human serum. Comparison of neutralizing antibody titers measured with the YF MN assay versus the historical YF PRNT, based on a 50% reduction in plaque counts (PRNT), demonstrated 100% serostatus agreement at a titer of 10 (1/dil) in participants with a history of YF vaccination. For validation, intra-assay precision (repeatability), intermediate precision, dilutional accuracy, linearity, specificity, upper limit of quantitation (ULOQ), and lower limit of quantitation (LLOQ) were assessed. The YF MN assay demonstrated suitable intra-assay precision (repeatability) and intermediate precision of 36% and 54%, respectively, with an ULOQ of 10,240. At the lower end of detection, repeatability and intermediate precision were 38% and 41%, respectively, with a LLOQ of 10 (1/dil). Suitable dilutional accuracy, linearity, and specificity across orthoflaviviruses (dengue virus, Japanese encephalitis virus, and Zika virus) and serum matrices (hemolytic, lipemic, and icteric) were also demonstrated. Overall, these promising results led the Center for Biologics Evaluation and Research to confirm the suitability of the validated YF MN assay for the detection and quantification of YF virus-neutralizing antibodies.

IMPORTANCE

With increased globalization and shifting climate patterns, yellow fever (YF) is re-emerging as a global threat. At present, vaccination remains the most effective prevention strategy. This study describes the development and validation of a new YF microneutralization (MN) assay for the detection and quantification of YF virus-neutralizing antibodies in human serum that offers increased throughput compared with the current standard assay. Overall, the YF MN assay demonstrated acceptable intra-assay precision (repeatability), intermediate precision, dilutional accuracy, linearity, and specificity and is suitable for the detection of YF virus-neutralizing antibodies. Further, the Center for Biologics Evaluation and Research (CBER) supports the use of the YF MN assay in the licensure of candidate YF vaccines.

摘要

未标记

蚀斑减少中和试验(PRNT)已被广泛用于检测和定量人血清中的黄热病毒中和抗体;然而,该方法劳动强度大,且难以适应疫苗许可所需的高通量临床检测。在此,我们描述了一种基于Vero细胞的新型黄热病毒微中和(MN)试验的开发与验证,该试验采用免疫染色读数,用于检测和定量人血清中的黄热病毒中和抗体。基于蚀斑计数减少50%(PRNT),将黄热病毒MN试验测得的中和抗体滴度与历史黄热病毒PRNT进行比较,结果表明,有黄热疫苗接种史的参与者在滴度为10(1/稀释度)时血清状态一致性达100%。为进行验证,评估了试验内精密度(重复性)、中间精密度、稀释准确性、线性、特异性、定量上限(ULOQ)和定量下限(LLOQ)。黄热病毒MN试验的试验内精密度(重复性)和中间精密度分别为36%和54%,ULOQ为10240,表现良好。在检测下限,重复性和中间精密度分别为38%和41%,LLOQ为10(1/稀释度)。在跨黄病毒属(登革病毒、日本脑炎病毒和寨卡病毒)和血清基质(溶血、脂血和黄疸)方面也表现出合适的稀释准确性、线性和特异性。总体而言,这些令人鼓舞的结果促使生物制品评估与研究中心确认经验证的黄热病毒MN试验适用于检测和定量黄热病毒中和抗体。

重要性

随着全球化加剧和气候模式变化,黄热病(YF)重新成为全球威胁。目前,接种疫苗仍是最有效的预防策略。本研究描述了一种新型黄热病毒微中和(MN)试验的开发与验证,该试验用于检测和定量人血清中的黄热病毒中和抗体,与当前标准试验相比,通量更高。总体而言,黄热病毒MN试验的试验内精密度(重复性)、中间精密度、稀释准确性、线性和特异性均可接受,适用于检测黄热病毒中和抗体。此外,生物制品评估与研究中心(CBER)支持在候选黄热疫苗的许可过程中使用黄热病毒MN试验。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/075e/11960057/abc451f8a140/spectrum.03348-24.f001.jpg

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