Development and Validation of an Enzyme-Linked Immunosorbent Assay-Based Protocol for Evaluation of Respiratory Syncytial Virus Vaccines

Author:

Nham Eliel12,Jang A-Yeung12ORCID,Ji Hyun Jung3,Ahn Ki Bum3,Bae Joon-Yong24,Park Man-Seong24,Yoon Jin Gu12,Seong Hye12,Noh Ji Yun12,Cheong Hee Jin12,Kim Woo Joo12ORCID,Seo Ho Seong3ORCID,Song Joon Young12ORCID

Affiliation:

1. Division of Infectious Diseases, Department of Internal Medicine, Korea University College of Medicine, Seoul 02841, Republic of Korea

2. Vaccine Innovation Center-KU Medicine (VIC-K), Seoul 02841, Republic of Korea

3. Korea Atomic Energy Research Institute, Jeongeup 56212, Republic of Korea

4. Department of Microbiology, Korea University College of Medicine, Seoul 02841, Republic of Korea

Abstract

Recently, respiratory syncytial virus (RSV) vaccines based on the prefusion F (pre-F) antigen were approved in the United States. We aimed to develop an enzyme-linked immunosorbent assay (ELISA)-based protocol for the practical and large-scale evaluation of RSV vaccines. Two modified pre-F proteins (DS-Cav1 and SC-TM) were produced by genetic recombination and replication using an adenoviral vector. The protocol was established by optimizing the concentrations of the coating antigen (pre-F proteins), secondary antibodies, and blocking buffer. To validate the protocol, we examined its accuracy, precision, and specificity using serum samples from 150 participants across various age groups and the standard serum provided by the National Institute of Health. In the linear correlation analysis, coating concentrations of 5 and 2.5 μg/mL of DS-Cav1 and SC-TM showed high coefficients of determination (r > 0.90), respectively. Concentrations of secondary antibodies (alkaline phosphatase-conjugated anti-human immunoglobulin G, diluted 1:2000) and blocking reagents (5% skim milk/PBS-T) were optimized to minimize non-specific reactions. High accuracy was observed for DS-Cav1 (r = 0.90) and SC-TM (r = 0.86). Further, both antigens showed high precision (coefficient of variation < 15%). Inhibition ELISA revealed cross-reactivity of antibodies against DS-Cav1 and SC-TM, but not with the attachment (G) protein.

Funder

Ministry of Food and Drug Safety

Publisher

MDPI AG

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