| Literature DB >> 34251356 |
Ester Lopez1, Ebene R Haycroft1, Amy Adair2, Francesca L Mordant1, Matthew T O'Neill2, Phillip Pymm2, Samuel J Redmond1, Wen Shi Lee1, Nicholas A Gherardin1, Adam K Wheatley1, Jennifer A Juno1, Kevin John Selva1, Samantha K Davis1, Samantha L Grimley1, Leigh Harty1, Damian Fj Purcell1, Kanta Subbarao3, Dale I Godfrey1, Stephen J Kent1, Wai-Hong Tham2, Amy W Chung1.
Abstract
The SARS-CoV-2 Receptor Binding Domain (RBD) is both the principal target of neutralizing antibodies, and one of the most rapidly evolving domains, which can result in the emergence of immune escape mutations limiting the effectiveness of vaccines and antibody therapeutics. To facilitate surveillance, we developed a rapid, high-throughput, multiplex assay able to assess the inhibitory response of antibodies to 24 RBD natural variants simultaneously. We demonstrate how this assay can be implemented as a rapid surrogate assay for functional cell-based serological methods to measure the SARS-CoV-2 neutralising capacity of antibodies at the ACE2-RBD interface. We describe the enhanced affinity of RBD variants N439K, S477N, Q493L, S494P and N501Y to the ACE2 receptor, and demonstrate the ability of this assay to bridge a major gap for SARS-CoV-2 research; informing selection of complementary monoclonal antibody candidates and the rapid identification of immune escape to emerging RBD variants following vaccination or natural infection.Entities:
Keywords: COVID-19; Immunoglobulins
Year: 2021 PMID: 34251356 DOI: 10.1172/jci.insight.150012
Source DB: PubMed Journal: JCI Insight ISSN: 2379-3708