Development of a Homogeneous High-Throughput Screening Assay for Biological Inhibitors of Human Rhinovirus Infection

Author:

Newton Philip1,O’Shea Desmond2,Wells Edward3,Moakes Kerry3,Dunmore Rebecca1,Butler Robin J.1,Wilkinson Trevor1,Ward Alison3,Casson Nigel3,Strain Martin1,Vousden Katherine1,Lowe David C.1,Pattison Debbie V.1,Carruthers Alan M.1,Sleeman Matthew A.1,Vaughan Tristan J.1,Harrison Paula1

Affiliation:

1. MedImmune Ltd., Cambridge, UK

2. Formerly of MedImmune Ltd., Cambridge, UK

3. Formerly of AstraZeneca Ltd., Loughborough, UK

Abstract

Infection with human rhinovirus (HRV) is thought to result in acute respiratory exacerbations of chronic obstructive pulmonary disorder (COPD). Consequently, prevention of HRV infection may provide therapeutic benefit to these patients. As all major group HRV serotypes infect cells via an interaction between viral coat proteins and intercellular adhesion molecule–1 (ICAM-1), it is likely that inhibitors of this interaction would prevent or reduce infections. Our objective was to use phage display technology in conjunction with naive human antibody libraries to identify anti–ICAM-1 antibodies capable of functional blockade of HRV infection. Key to success was the development of a robust, functionally relevant high-throughput screen (HTS) compatible with the specific challenges of antibody screening. In this article, we describe the development of a novel homogeneous time-resolved fluorescence (HTRF) assay based on the inhibition of soluble ICAM-1 binding to live HRV16. We describe the implementation of the method in an antibody screening campaign and demonstrate the biological relevance of the assay by confirming the activity of resultant antibodies in a cell-based in vitro HRV infection assay.

Publisher

Elsevier BV

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