Virus-like particles displaying the mature C-terminal domain of filamentous hemagglutinin are immunogenic and protective against Bordetella pertussis respiratory infection in mice

Author:

Pyles Gage M.12ORCID,Huckaby Annalisa B.12,Gutierrez Maria de la Paz12,Witt William T.12,Mateu-Borrás Margalida12,Dublin Spencer R.12,Rocuskie-Marker Carleena12,Sesti Bethany N.12,Peasak Kerrington12,Bitzer Graham J.12,Rader Nathaniel12,Weaver Kelly L.12,Boehm Dylan T.12,Fitzgerald Nicholas12,Chapman Joshua12,Ulicny Samuel12,Damron F. Heath12ORCID,Barbier Mariette12ORCID

Affiliation:

1. Department of Microbiology, Immunology and Cell Biology, West Virginia University , Morgantown, West Virginia, USA

2. Vaccine Development Center, West Virginia University Health Sciences Center , Morgantown, West Virginia, USA

Abstract

ABSTRACT Bordetella pertussis, the bacterium responsible for whooping cough, remains a significant public health challenge despite the existing licensed pertussis vaccines. Current acellular pertussis vaccines, though having favorable reactogenicity and efficacy profiles, involve complex and costly production processes. In addition, acellular vaccines have functional challenges such as short-lasting duration of immunity and limited antigen coverage. Filamentous hemagglutinin (FHA) is an adhesin of B. pertussis that is included in all multivalent pertussis vaccine formulations. Antibodies to FHA have been shown to prevent bacterial attachment to respiratory epithelial cells, and T cell responses to FHA facilitate cell-mediated immunity. In this study, FHA’s mature C-terminal domain (MCD) was evaluated as a novel vaccine antigen. MCD was conjugated to virus-like particles via SpyTag-SpyCatcher technology. Prime-boost vaccine studies were performed in mice to characterize immunogenicity and protection against the intranasal B. pertussis challenge. MCD-SpyVLP was more immunogenic than SpyTag-MCD antigen alone, and in Tohama I strain challenge studies, improved protection against challenge was observed in the lungs at day 3 and in the trachea and nasal wash at day 7 post-challenge. Furthermore, a B. pertussis strain encoding genetically inactivated pertussis toxin was used to evaluate MCD-SpyVLP vaccine immunity. Mice vaccinated with MCD-SpyVLP had significantly lower respiratory bacterial burden at both days 3 and 7 post-challenge compared to mock-vaccinated animals. Overall, these data support the use of SpyTag-SpyCatcher VLPs as a platform for use in vaccine development against B. pertussis and other pathogens.

Funder

HHS | National Institutes of Health

West Virginia Higher Education Policy Commission

Publisher

American Society for Microbiology

Reference56 articles.

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