Development of a high-throughput SARS-CoV-2 antibody testing pathway using dried blood spot specimens

Author:

Moat Stuart J12ORCID,Zelek Wioleta M3,Carne Emily4,Ponsford Mark J45ORCID,Bramhall Kathryn4,Jones Sara6,El-Shanawany Tariq4,Wise Matt P7,Thomas Annette6,George Chloe8,Fegan Christopher9,Steven Rachael4,Webb Russell4,Weeks Ian10,Morgan B Paul3,Jolles Stephen4

Affiliation:

1. Wales Newborn Screening Laboratory, Department of Medical Biochemistry, Immunology and Toxicology, University Hospital of Wales, Cardiff, Wales, UK

2. School of Medicine, Cardiff University, Cardiff, Wales, UK

3. Systems Immunity University Research Institute and Dementia Research Institute, Cardiff University, Cardiff, UK

4. Immunodeficiency Centre for Wales, University Hospital of Wales, Cardiff, UK

5. Division of Infection, Inflammation and Immunity, School of Medicine, Cardiff University, Cardiff, UK

6. Weqas, Cardiff and Vale University Health Board, Cardiff, UK

7. Adult Critical Care, University Hospital of Wales, Cardiff, UK

8. Welsh Blood Service, Ely Valley Road, Talbot Green, Pontyclun, UK

9. Department of Haematology, University Hospital of Wales, Cardiff, Wales, UK

10. College of Biomedical and Life Sciences, Cardiff University, Cardiff, UK

Abstract

Background Serological assays for Severe Acute Respiratory Syndrome Coronavirus 2 (SARS-CoV-2) have roles in seroepidemiology, convalescent plasma-testing, antibody durability and vaccine studies. Currently, SARS-CoV-2 serology is performed using serum/plasma collected by venepuncture. Dried blood spot (DBS) testing offers significant advantages as it is minimally invasive, avoids venepuncture with specimens being mailed to the laboratory. Methods A pathway utilizing a newborn screening laboratory infrastructure was developed using an enzyme-linked immunosorbent assay to detect IgG antibodies against the receptor-binding domain of the SARS-CoV-2 spike protein in DBS specimens. Paired plasma and DBS specimens from SARS-CoV-2 antibody-positive and -negative subjects and polymerase chain reaction positive subjects were tested. DBS specimen stability, effect of blood volume and punch location were also evaluated. Results DBS specimens from antibody-negative ( n = 85) and -positive ( n = 35) subjects and polymerase chain reaction positive subjects ( n = 11) had a mean (SD; range) optical density (OD) of 0.14 (0.046; 0.03–0.27), 0.98 (0.41; 0.31–1.64) and 1.12 (0.37; 0.49–1.54), respectively. An action value OD >0.28 correctly assigned all cases. The weighted Deming regression for comparison of the DBS and the plasma assay yielded: y = 0.004041 + 1.005 x, r = 0.991, Sy/ x 0.171, n = 82. Extraction efficiency of antibodies from DBS specimens was >99%. DBS specimens were stable for at least 28 days at ambient room temperature and humidity. Conclusions SARS-CoV-2 IgG receptor-binding domain antibodies can be reliably detected in DBS specimens. DBS serological testing offers lower costs than either point of care or serum/plasma assays that require patient travel, phlebotomy and hospital/clinic resources; the development of a DBS assay may be particularly important for resource poor settings.

Publisher

SAGE Publications

Subject

Clinical Biochemistry,General Medicine

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