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Development and validation of IMMUNO-COV™: a high-throughput clinical assay for detecting antibodies that neutralize SARS-CoV-2

Rianna Vandergaast, Timothy Carey, Samantha Reiter, Patrycja Lech, Clement Gnanadurai, Mulu Tesfay, Jason Buehler, Lukkana Suksanpaisan, Shruthi Naik, Bethany Brunton, Jordan Recker, Michelle Haselton, Christopher Ziegler, Anne Roesler, John R. Mills, Elitza Theel, Scott C. Weaver, Grace Rafael, Matthew M. Roforth, Calvin Jerde, Sheryl Tran, Rosa Maria Diaz, Alice Bexon, Alina Baum, Christos A. Kyratsous, Kah Whye Peng, Stephen J. Russell
doi: https://doi.org/10.1101/2020.05.26.117549
Rianna Vandergaast
1Imanis Life Sciences, Rochester, MN 55901
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  • For correspondence: sjrussell@vyriad.com Vandergaast.rianna@imanislife.com
Timothy Carey
1Imanis Life Sciences, Rochester, MN 55901
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Samantha Reiter
1Imanis Life Sciences, Rochester, MN 55901
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Patrycja Lech
1Imanis Life Sciences, Rochester, MN 55901
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Clement Gnanadurai
1Imanis Life Sciences, Rochester, MN 55901
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Mulu Tesfay
1Imanis Life Sciences, Rochester, MN 55901
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Jason Buehler
1Imanis Life Sciences, Rochester, MN 55901
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Lukkana Suksanpaisan
1Imanis Life Sciences, Rochester, MN 55901
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Shruthi Naik
2Vyriad, Inc., Rochester, MN 55901
3Mayo Clinic Department of Molecular Medicine, Rochester, MN 55905
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Bethany Brunton
2Vyriad, Inc., Rochester, MN 55901
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Jordan Recker
2Vyriad, Inc., Rochester, MN 55901
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Michelle Haselton
1Imanis Life Sciences, Rochester, MN 55901
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Christopher Ziegler
1Imanis Life Sciences, Rochester, MN 55901
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Anne Roesler
1Imanis Life Sciences, Rochester, MN 55901
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John R. Mills
4Mayo Clinic Department of Laboratory Medicine and Pathology, Rochester, MN 55905
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Elitza Theel
4Mayo Clinic Department of Laboratory Medicine and Pathology, Rochester, MN 55905
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Scott C. Weaver
5World Reference Center for Emerging Viruses and Arboviruses, Institute for Human Infections and Immunity, University of Texas Medical Branch, Galveston, TX 77555
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Grace Rafael
5World Reference Center for Emerging Viruses and Arboviruses, Institute for Human Infections and Immunity, University of Texas Medical Branch, Galveston, TX 77555
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Matthew M. Roforth
6Mayo Clinic Advanced Diagnostic Laboratory, Rochester, MN 55905
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Calvin Jerde
6Mayo Clinic Advanced Diagnostic Laboratory, Rochester, MN 55905
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Sheryl Tran
2Vyriad, Inc., Rochester, MN 55901
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Rosa Maria Diaz
2Vyriad, Inc., Rochester, MN 55901
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Alice Bexon
2Vyriad, Inc., Rochester, MN 55901
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Alina Baum
7Regeneron Pharmaceuticals Inc., Tarrytown, NY 10591
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Christos A. Kyratsous
7Regeneron Pharmaceuticals Inc., Tarrytown, NY 10591
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Kah Whye Peng
1Imanis Life Sciences, Rochester, MN 55901
2Vyriad, Inc., Rochester, MN 55901
3Mayo Clinic Department of Molecular Medicine, Rochester, MN 55905
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Stephen J. Russell
1Imanis Life Sciences, Rochester, MN 55901
2Vyriad, Inc., Rochester, MN 55901
3Mayo Clinic Department of Molecular Medicine, Rochester, MN 55905
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  • For correspondence: sjrussell@vyriad.com Vandergaast.rianna@imanislife.com
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Abstract

We here describe the development and validation of IMMUNO-COV™, a high-throughput clinical test to quantitatively measure SARS-CoV-2-neutralizing antibodies, the specific subset of anti-SARS-CoV-2 antibodies that block viral infection. The test measures the capacity of serum or purified antibodies to neutralize a recombinant Vesicular Stomatitis Virus (VSV) encoding the SARS-CoV-2 spike glycoprotein. This recombinant virus (VSV-SARS-CoV-2-S-Δ19CT) induces fusion in Vero cell monolayers, which is detected as luciferase signal using a dual split protein (DSP) reporter system. VSV-SARS-CoV-2-S-Δ19CT infection was blocked by monoclonal α-SARS-CoV-2-spike antibodies and by plasma or serum from SARS-CoV-2 convalescing individuals. The assay exhibited 100% specificity in validation tests, and across all tests zero false positives were detected. In blinded analyses of 230 serum samples, only two unexpected results were observed based on available clinical data. We observed a perfect correlation between results from our assay and 80 samples that were also assayed using a commercially available ELISA. To quantify the magnitude of the anti-viral response, we generated a calibration curve by adding stepped concentrations of α-SARS-CoV-2-spike monoclonal antibody to pooled SARS-CoV-2 seronegative serum. Using the calibration curve and a single optimal 1:100 serum test dilution, we reliably measured neutralizing antibody levels in each test sample. Virus neutralization units (VNUs) calculated from the assay correlated closely (p < 0.0001) with PRNTEC50 values determined by plaque reduction neutralization test against a clinical isolate of SARS-CoV-2. Taken together, these results demonstrate that the IMMUNO-COV™ assay accurately quantitates SARS-CoV-2 neutralizing antibodies in human sera and therefore is a potentially valuable addition to the currently available serological tests. The assay can provide vital information for comparing immune responses to the various SARS-CoV-2 vaccines that are currently in development, or for evaluating donor eligibility in convalescent plasma therapy studies.

Competing Interest Statement

Vyriad, Imanis Life Sciences, Regeneron, and Mayo Clinic are collaborating in the commercial development of this assay. Most coauthors of this manuscript are employees of at least one of the above organizations as noted in the author affiliations. SJR and KWP are co-founding scientists, officers, and stockholders both in Vyriad and Imanis Life Sciences; both are employees of Mayo Clinic.

Footnotes

  • Conflicts of Interest Vyriad, Imanis Life Sciences, Regeneron, and Mayo Clinic are collaborating in the commercial development of this assay. Most coauthors of this manuscript are employees of at least one of the above organizations as noted in the author affiliations. SJR and KWP are co-founding scientists, officers, and stockholders both in Vyriad and Imanis Life Sciences; both are employees of Mayo Clinic.

Copyright 
The copyright holder for this preprint is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity. All rights reserved. No reuse allowed without permission.
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Posted May 27, 2020.
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Development and validation of IMMUNO-COV™: a high-throughput clinical assay for detecting antibodies that neutralize SARS-CoV-2
Rianna Vandergaast, Timothy Carey, Samantha Reiter, Patrycja Lech, Clement Gnanadurai, Mulu Tesfay, Jason Buehler, Lukkana Suksanpaisan, Shruthi Naik, Bethany Brunton, Jordan Recker, Michelle Haselton, Christopher Ziegler, Anne Roesler, John R. Mills, Elitza Theel, Scott C. Weaver, Grace Rafael, Matthew M. Roforth, Calvin Jerde, Sheryl Tran, Rosa Maria Diaz, Alice Bexon, Alina Baum, Christos A. Kyratsous, Kah Whye Peng, Stephen J. Russell
bioRxiv 2020.05.26.117549; doi: https://doi.org/10.1101/2020.05.26.117549
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Development and validation of IMMUNO-COV™: a high-throughput clinical assay for detecting antibodies that neutralize SARS-CoV-2
Rianna Vandergaast, Timothy Carey, Samantha Reiter, Patrycja Lech, Clement Gnanadurai, Mulu Tesfay, Jason Buehler, Lukkana Suksanpaisan, Shruthi Naik, Bethany Brunton, Jordan Recker, Michelle Haselton, Christopher Ziegler, Anne Roesler, John R. Mills, Elitza Theel, Scott C. Weaver, Grace Rafael, Matthew M. Roforth, Calvin Jerde, Sheryl Tran, Rosa Maria Diaz, Alice Bexon, Alina Baum, Christos A. Kyratsous, Kah Whye Peng, Stephen J. Russell
bioRxiv 2020.05.26.117549; doi: https://doi.org/10.1101/2020.05.26.117549

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