Por favor, use este identificador para citar o enlazar este ítem: http://hdl.handle.net/20.500.12666/451
Título : A multiplex antigen microarray for simultaneous IgG and IgM detection against SARS-CoV-2 reveals higher seroprevalence than reported
Autor : Ruano Gallego, D.
García Villadangos, M.
Moreno Paz, M.
Gómez Elvira, J.
Postigo, M.
Simón Sacristan, M.
Reyburn, H. T.
Carolis, C.
Rodrigo, N.
Codeseira, Y. B.
Rueda, P.
Zúñiga, Sonia
Enjuanes, L.
Parro García, V.
Fecha de publicación : 30-abr-2021
Editorial : Society for Applied Microbiology
DOI: 10.1111/1751-7915.13801
Versión del Editor: https://sfamjournals.onlinelibrary.wiley.com/doi/10.1111/1751-7915.13801
Citación : Microbial Biotechnology 14(3): 1228-1236(2021)
Resumen : The surge of SARS-CoV-2 has challenged health systems worldwide and efficient tests to detect viral particles, as well as antibodies generated against them, are needed. Specificity, sensitivity, promptness or scalability are the main parameters to estimate the final performance, but rarely all of them match in a single test. We have developed SCOVAM, a protein microarray with several viral antigens (spike, nucleocapsid, main protease Nsp5) as capturing probes in a fluorescence immunoassay for COVID-19 serological testing. SCOVAM depicts IgG and IgM antibody responses against each of these proteins of 22 individuals in a single microscope slide. It detects specific IgM (0.094 μg ml-1) and IgG (~0.017 μg ml-1) and is scalable and cost-effective. We validated SCOVAM by comparing with a widely used chemiluminescent commercial serological test (n = 742). SCOVAM showed twice the sensitivity and allowed following seroconversion in a single assay. By analysing the prevalence 4 months later in a subset of 76 positive sera, we still detected 93.42% of positives, almost doubling the detection of the commercial assay. The higher sensitivity of SCOVAM is especially relevant to screen sera for convalescent plasma-based treatments, high-throughput antibody response monitoring after vaccination or evaluation of vaccine efficiency.
URI : http://hdl.handle.net/20.500.12666/451
E-ISSN : 1751-7915
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