Author: Horndler, Lydia; Delgado, Pilar; Abia, David; Balabanov, Ivaylo; MartÃnezâ€Fleta, Pedro; Cornish, Georgina; Llamas, Miguel A; Serranoâ€Villar, Sergio; Sánchezâ€Madrid, Francisco; Fresno, Manuel; van Santen, Hisse M; Alarcón, Balbino
Title: Flow cytometry multiplexed method for the detection of neutralizing human antibodies to the native SARSâ€CoVâ€2 spike protein Cord-id: 4xinrp44 Document date: 2021_2_17
ID: 4xinrp44
Snippet: A correct identification of seropositive individuals for the severe acute respiratory syndrome coronavirusâ€2 (SARSâ€CoVâ€2) infection is of paramount relevance to assess the degree of protection of a human population to present and future outbreaks of the COVIDâ€19 pandemic. We describe here a sensitive and quantitative flow cytometry method using the cytometerâ€friendly nonâ€adherent Jurkat Tâ€cell line that stably expresses the fullâ€length native spike “S†protein of SARSâ€CoVâ€
Document: A correct identification of seropositive individuals for the severe acute respiratory syndrome coronavirusâ€2 (SARSâ€CoVâ€2) infection is of paramount relevance to assess the degree of protection of a human population to present and future outbreaks of the COVIDâ€19 pandemic. We describe here a sensitive and quantitative flow cytometry method using the cytometerâ€friendly nonâ€adherent Jurkat Tâ€cell line that stably expresses the fullâ€length native spike “S†protein of SARSâ€CoVâ€2 and a truncated form of the human EGFR that serves a normalizing role. S protein and huEGFRt coding sequences are separated by a T2A selfâ€cleaving sequence, allowing to accurately quantify the presence of antiâ€S immunoglobulins by calculating a score based on the ratio of fluorescence intensities obtained by doubleâ€staining with the test sera and antiâ€EGFR. The method allows to detect immune individuals regardless of the result of other serological tests or even repeated PCR monitoring. As examples of its use, we show that as much as 28% of the personnel working at the CBMSO in Madrid is already immune. Additionally, we show that antiâ€S antibodies with protective neutralizing activity are longâ€lasting and can be detected in sera 8 months after infection.
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