Establishment and characterization of noro-VLP measurement by digital ELISA

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-10-09 DOI:10.1039/D4AY01012D
Takema Hasegawa, Yuriko Adachi, Kazumi Saikusa and Megumi Kato
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Abstract

Highly sensitive viral analytical techniques are essential tools for preventing the spread of infections. In this study, we established a digital enzyme-linked immunosorbent assay (ELISA) system to quantify norovirus proteins with high sensitivity. We used norovirus-like particles (noro-VLPs) as a surrogate for norovirus and constructed two digital ELISA systems using two different antibody pairs. The quantitative performance of the noro-VLP measurement using each digital ELISA system was evaluated. Both assay systems exhibited high sensitivity, good linearity, and high stability. The first system exhibited a limit of detection (LOD) of 87 pg mL−1 and correlation coefficient (R2) of 0.9984. Analysis of samples containing 5 ng per mL noro-VLP confirmed inter-assay variation of 5.5%, and intra-assay variation of 5.2%. The second system exhibited an LOD of 19 pg mL−1 and R2 of 0.9984. Analysis of samples containing 5 ng per mL noro-VLP confirmed inter-assay variation of 4.5%, and intra-assay variation of 2.5%. Comparison of the two systems using the same calibrant for unpurified and fractionated noro-VLPs revealed that the quantitative values for unpurified noro-VLPs were the same, whereas those for fractionated noro-VLPs were dramatically different. Our findings indicate that the reactivity to various components in the noro-VLP solution was altered depending on the different antibodies. Furthermore, our study highlights the importance of using appropriate calibrants, which contain the same ratio of components as the noro-VLP analyte, to afford accurate measurements.

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利用数字酶联免疫吸附技术建立和鉴定诺-VLP 测量方法。
高灵敏度的病毒分析技术是预防感染传播的重要工具。在这项研究中,我们建立了一个数字酶联免疫吸附测定(ELISA)系统,以高灵敏度量化诺如病毒蛋白。我们使用诺如病毒样颗粒(诺如病毒样颗粒)作为诺如病毒的替代物,并使用两种不同的抗体对构建了两种数字酶联免疫吸附测定系统。我们评估了每种数字 ELISA 系统对诺如病毒样颗粒(noro-VLP)的定量检测性能。两种检测系统都表现出了高灵敏度、良好的线性和高稳定性。第一个系统的检测限(LOD)为 87 pg mL-1,相关系数(R2)为 0.9984。对每毫升含有 5 毫微克 noro-VLP 的样品进行分析后证实,测定间的差异为 5.5%,测定内的差异为 5.2%。第二个系统的检测限为 19 pg mL-1,R2 为 0.9984。对每毫升含有 5 毫微克 noro-VLP 的样品进行分析,结果表明测定间差异为 4.5%,测定内差异为 2.5%。使用相同的校准物对未净化和分馏的去甲-VLP 进行比较后发现,未净化去甲-VLP 的定量值相同,而分馏去甲-VLP 的定量值则大不相同。我们的研究结果表明,不同抗体对去甲斑蝥素-VLP溶液中各种成分的反应性会发生改变。此外,我们的研究还强调了使用适当校准物的重要性,校准物中含有与去甲-VLP 分析物相同比例的成分,这样才能进行准确的测量。
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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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