Emerging Microbes and Infections (Jan 2020)

Validation and clinical evaluation of a SARS-CoV-2 surrogate virus neutralisation test (sVNT)

  • Benjamin Meyer,
  • Johan Reimerink,
  • Giulia Torriani,
  • Fion Brouwer,
  • Gert-Jan Godeke,
  • Sabine Yerly,
  • Marieke Hoogerwerf,
  • Nicolas Vuilleumier,
  • Laurent Kaiser,
  • Isabella Eckerle,
  • Chantal Reusken

DOI
https://doi.org/10.1080/22221751.2020.1835448
Journal volume & issue
Vol. 9, no. 1
pp. 2394 – 2403

Abstract

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ABSTRACTTo understand SARS-CoV-2 immunity after natural infection or vaccination, functional assays such as virus neutralising assays are needed. So far, assays to detect SARS-CoV-2 neutralising antibodies rely on cell-culture based infection assays either using wild type SARS-CoV-2 or pseudotyped viruses. Such assays are labour-intensive, require appropriate biosafety facilities and are difficult to standardize. Recently, a new surrogate virus neutralisation test (sVNT) was described that uses the principle of an ELISA to measure the neutralisation capacity of anti-SARS-CoV-2 antibodies directed against the receptor binding domain. Here, we performed an independent evaluation of the robustness, specificity and sensitivity on an extensive panel of sera from 269 PCR-confirmed COVID-19 cases and 259 unmatched samples collected before 2020 and compared it to cell-based neutralisation assays. We found a high specificity of 99.2 (95%CI: 96.9–99.9) and overall sensitivity of 80.3 (95%CI: 74.9–84.8) for the sVNT. Clinical sensitivity increased between early (14 dpos/dpd) from 75.0 (64.7–83.2) to 83.1 (76.5–88.1). Also, higher severity was associated with an increase in clinical sensitivity. Upon comparison with cell-based neutralisation assays we determined an analytical sensitivity of 74.3 (56.4–86.9) and 98.2 (89.4–99.9) for titres ≥10 to <40 and ≥40 to <160, respectively. Only samples with a titre ≥160 were always positive in the sVNT. In conclusion, the sVNT can be used as an additional assay to determine the immune status of COVID-19 infected of vaccinated individuals but its value needs to be assessed for each specific context.

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