Establishment and characterization of noro-VLP measurement by digital ELISA

28 May 2024, Version 1
This content is a preprint and has not undergone peer review at the time of posting.

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, correlation coefficient (R2) of 0.9984, inter-assay variation of 5.5 %, and intra-assay variation of 5.2 %. The second system exhibited an LOD of 19 pg/mL, R2 of 0.9984, 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.

Keywords

Noro-VLP
Digital ELISA
Quantitative performance

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