Intramuscular but not nebulized administration of a mRNA vaccine against Rhodococcus equi stimulated humoral immune responses in neonatal foals

Author:

Legere Rebecca M.1,Poveda Cristina23,Ott Jeannine A.4,Bray Jocelyne M.1,Villafone Emma G.1,Silveira Bibiana Petri da1,Kahn Susanne K.1,Martin Cameron L.5,Mancino Chiara67,Taraballi Francesca67,Criscitiello Michael F.4,Berghman Luc45,Bordin Angela I.1,Pollet Jeroen23,Cohen Noah D.1

Affiliation:

1. Equine Infectious Disease Laboratory, Department of Large Animal Clinical Sciences, School of Veterinary Medicine & Biomedical Sciences, Texas A&M University, College Station, TX

2. Department of Pediatrics, Division of Tropical Medicine, Baylor College of Medicine, Houston, TX

3. Texas Children’s Hospital Center for Vaccine Development, Houston, TX

4. Comparative Immunogenetics Laboratory, Department of Veterinary Pathobiology, School of Veterinary Medicine & Biomedical Sciences, Texas A&M University, College Station, TX

5. Department of Poultry Science, College of Agriculture & Life Sciences, Texas A&M University, College Station, TX

6. Center for Musculoskeletal Regeneration, Houston Methodist Research Institute, Houston, TX

7. Orthopedics and Sports Medicine, Houston Methodist Hospital, Houston, TX

Abstract

Abstract OBJECTIVE Design and evaluate immune responses of neonatal foals to a mRNA vaccine expressing the virulence-associated protein A (VapA) of Rhodococcus equi. ANIMALS Cultured primary equine respiratory tract cells; Serum, bronchoalveolar lavage fluid (BALF), and peripheral blood mononuclear cells (PBMCs) from 30 healthy Quarter Horse foals. METHODS VapA expression was evaluated by western immunoblot in cultured equine bronchial cells transfected with 4 mRNA constructs encoding VapA. The mRNA construct with greatest expression was used to immunize foals at ages 2 and 21 days in 5 groups: (1) 300 μg nebulized mRNA (n = 6); (2) 600 μg nebulized mRNA (n = 4); (3) 300 μg mRNA administered intramuscularly (IM) (n = 5); (4) 300 μg VapA IM (positive controls; n = 6); or (5) nebulized water (negative controls; n = 6). Serum, BALF, and PBMCs were collected at ages 3, 22, and 35 days and tested for relative anti-VapA IgG1, IgG4/7, and IgA activities using ELISA and cell-mediated immunity by ELISpot. RESULTS As formulated, nebulized mRNA was not immunogenic. However, a significant increase in anti-VapA IgG4/7 activity (P < .05) was noted exclusively in foals immunized IM with VapA mRNA by age 35 days. The proportion of foals with anti-VapA IgG1 activity > 30% of positive control differed significantly (P = .0441) between negative controls (50%; 3/6), IM mRNA foals (100%; 5/5), and IM VapA (100%; 6/6) groups. Natural exposure to virulent R equi was immunogenic in some negative control foals. CLINICAL RELEVANCE Further evaluation of the immunogenicity and efficacy of IM mRNA encoding VapA in foals is warranted.

Publisher

American Veterinary Medical Association (AVMA)

Subject

General Veterinary,General Medicine

Reference53 articles.

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3. Monitoring foals by thoracic ultrasonography, bacterial culture, and PCR: Diagnostic of Rhodococcus equi subclinical pneumonia in South of Brazil;Huber L,2018

4. Associations between physical examination, laboratory, and radiographic findings and outcome and subsequent racing performance of foals with Rhodococcus equi infection: 115 cases (1984-1992);Ainsworth DM,1998

5. Application of Sartwell’s model (lognormal distribution of incubation periods) to age at onset and age at death of foals with Rhodococcus equi pneumonia as evidence of perinatal infection;Horowitz ML,2001

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