Evaluating the serological status of COVID-19 patients using an indirect immunofluorescent assay, France

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Edouard, S. | Colson, P. | Melenotte, C. | Di Pinto, F. | Thomas, L. | La Scola, B. | Million, M. | Tissot-Dupont, H. | Gautret, P. | Stein, A. | Brouqui, P. | Parola, Philippe | Lagier, J. -C. | Raoult, D. | Drancourt, Michel

Edité par CCSD ; Springer Verlag -

International audience. An indirect in-house immunofluorescent assay was developed in order to assess the serological status of COVID-19 patients in Marseille, France. Performance of IFA was compared to a commercial ELISA IgG kit. We tested 888 RT-qPCR-confirmed COVID-19 patients (1302 serum samples) and 350 controls including 200 sera collected before the pandemic, 64 sera known to be associated with nonspecific serological interference, 36 sera from non-coronavirus pneumonia and 50 sera from patient with other common coronavirus to elicit false-positive serology. Incorporating an inactivated clinical SARS-CoV-2 isolate as the antigen, the specificity of the assay was measured as 100% for IgA titre >= 1:200, 98.6% for IgM titre >= 1:200 and 96.3% for IgG titre >= 1:100 after testing a series of negative controls. IFA presented substantial agreement (86%) with ELISA EUROIMMUN SARS-CoV-2 IgG kit (Cohen's Kappa = 0.61). The presence of antibodies was then measured at 3% before a 5-day evolution up to 47% after more than 15 days of evolution. We observed that the rates of seropositivity as well as the titre of specific antibodies were both significantly higher in patients with a poor clinical outcome than in patients with a favourable evolution. These data, which have to be integrated into the ongoing understanding of the immunological phase of the infection, suggest that detection anti-SARS-CoV-2 antibodies is useful as a marker associated with COVID-19 severity. The IFA assay reported here is useful for monitoring SARS-CoV-2 exposure at the individual and population levels.

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