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Flow cytometry multiplexed method for the detection of neutralizing human antibodies to the native SARS‐CoV‐2 spike protein

机译:流式细胞术多重方法用于检测对天然SARS-COV-2穗蛋白的中和人抗体

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摘要

A correct identification of seropositive individuals for the severe acute respiratory syndrome coronavirus‐2 (SARS‐CoV‐2) infection is of paramount relevance to assess the degree of protection of a human population to present and future outbreaks of the COVID‐19 pandemic. We describe here a sensitive and quantitative flow cytometry method using the cytometer‐friendly non‐adherent Jurkat T‐cell line that stably expresses the full‐length native spike “S” protein of SARS‐CoV‐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 self‐cleaving sequence, allowing to accurately quantify the presence of anti‐S immunoglobulins by calculating a score based on the ratio of fluorescence intensities obtained by double‐staining with the test sera and anti‐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 anti‐S antibodies with protective neutralizing activity are long‐lasting and can be detected in sera 8 months after infection.
机译:正确鉴定严重急性呼吸综合征Coronavirus-2(SARS-COV-2)感染的血清阳性个体是最重要的,以评估人口的保护程度,以评估人口的保护程度和未来的Covid-19流行病的爆发。这里我们在此描述了一种敏感和定量的流式细胞术方法,其使用细胞差计友好的非粘附jurkat t细胞稳定地表达SARS-COV-2的全长天然尖峰和人EGFR的截短形式这有助于标准化作用。 S蛋白质和HueGFRT编码序列通过T2A自切割序列分离,允许通过基于通过用试验血清双染量的荧光强度的比率计算得分来精确地量化抗S免疫球蛋白的存在。 EGFR。该方法允许检测免疫细胞,无论其他血清学检测还是甚至重复的PCR监测。作为其使用的例子,我们表明,在马德里的CBMSO工作中的28%的人员已经是免疫。此外,我们表明,具有保护性中和活性的防抗抗体是持久的,并且可以在感染后8个月在血清中检测到。

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