Development and utility of a SARS-CoV-2 pseudovirus assay for compound screening and antibody neutralization assays
Aaron A. Manu,
Irene A. Owusu,
Fatima O. Oyawoye,
Sylvester Languon,
Ibrahim Anna Barikisu,
Sylvia Tawiah-Eshun,
Osbourne Quaye,
Kwaku Jacob Donkor,
Lily Paemka,
Gloria A. Amegatcher,
Prince M.D. Denyoh,
Daniel Oduro-Mensah,
Gordon A. Awandare,
Peter K. Quashie
Affiliations
Aaron A. Manu
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Biochemistry, Cell, and Molecular Biology, School of Biological Sciences, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Irene A. Owusu
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Fatima O. Oyawoye
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Biochemistry, Cell, and Molecular Biology, School of Biological Sciences, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Sylvester Languon
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Cellular and Molecular Biomedical Sciences Program, University of Vermont, Burlington, VT, USA
Ibrahim Anna Barikisu
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Sylvia Tawiah-Eshun
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Osbourne Quaye
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Biochemistry, Cell, and Molecular Biology, School of Biological Sciences, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Kwaku Jacob Donkor
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Biochemistry, Cell, and Molecular Biology, School of Biological Sciences, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Lily Paemka
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Biochemistry, Cell, and Molecular Biology, School of Biological Sciences, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Gloria A. Amegatcher
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Medical Laboratory Sciences, School of Biomedical and Allied Health Sciences, Korle bu, University of Ghana, Legon, Accra, Ghana
Prince M.D. Denyoh
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Daniel Oduro-Mensah
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Biochemistry, Cell, and Molecular Biology, School of Biological Sciences, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Gordon A. Awandare
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; Department of Biochemistry, Cell, and Molecular Biology, School of Biological Sciences, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana
Peter K. Quashie
West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana; The Francis Crick Institute, 1 Midland Rd, London, NW1 1AT, United Kingdom; Corresponding author. West African Centre for Cell Biology of Infectious Pathogens, College of Basic and Applied Sciences, University of Ghana, Legon-Accra, Ghana.
Background: The highly infectious nature of SARS-CoV-2 necessitates using bio-containment facilities to study viral pathogenesis and identify potent antivirals. However, the lack of high-level bio-containment laboratories across the world has limited research efforts into SARS-CoV-2 pathogenesis and the discovery of drug candidates. Previous research has reported that non-replicating SARS-CoV-2 Spike-pseudotyped viral particles are effective tools to screen for and identify entry inhibitors and neutralizing antibodies. Methods: To generate SARS-CoV-2 pseudovirus, a lentiviral packaging plasmid p8.91, a luciferase expression plasmid pCSFLW, and SARS-CoV-2 Spike expression plasmids (Wild-type (D614G) or Delta strain) were co-transfected into HEK293 cells to produce a luciferase-expressing non-replicating pseudovirus which expresses SARS-CoV-2 spike protein on the surface. For relative quantitation, HEK293 cells expressing ACE2 (ACE2-HEK293) were infected with the pseudovirus, after which luciferase activity in the cells was measured as a relative luminescence unit. The ACE2-HEK293/Pseudovirus infection system was used to assess the antiviral effects of some compounds and plasma from COVID-19 patients to demonstrate the utility of this assay for drug discovery and neutralizing antibody screening. Results: We successfully produced lentiviral-based SARS-CoV2 pseudoviruses and ACE2-expressing HEK293 cells. The system was used to screen compounds for SARS-CoV-2 entry inhibitors and identified two compounds with potent activity against SARS-CoV-2 pseudovirus entry into cells. The assay was also employed to screen patient plasma for neutralizing antibodies against SARS-CoV-2, as a precursor to live virus screening, using successful hits. Significance: This assay is scalable and can perform medium-to high-throughput screening of antiviral compounds with neither severe biohazard risks nor the need for higher-level containment facilities. Now fully deployed in our resource-limited laboratory, this system can be applied to other highly infectious viruses by swapping out the envelope proteins in the plasmids used in pseudovirus production.
