Identification of potential antigenic peptides of Brucella through proteome and peptidome

Meijuan Pei; Ao Dong; Xueping Ma; Shulei Li; Yan Guo; Menglan Li; Zhenghui Wang; Hengliang Wang; Li Zhu; Chao Pan; Yufei Wang

doi:10.1002/vms3.1048

Identification of potential antigenic peptides of Brucella through proteome and peptidome

Vet Med Sci. 2023 Jan;9(1):523-534. doi: 10.1002/vms3.1048. Epub 2022 Dec 30.

Authors

Meijuan Pei^{1

2}, Ao Dong², Xueping Ma³, Shulei Li^{1

2}, Yan Guo², Menglan Li³, Zhenghui Wang³, Hengliang Wang², Li Zhu², Chao Pan², Yufei Wang^{1

3}

Affiliations

¹ Department of Clinical Laboratory, The Third Medical Centre of Chinese PLA General Hospital, The Training Site for Postgraduate of Jinzhou Medical University, Beijing, China.
² State Key Laboratory of Pathogen and Biosecurity, Beijing Institute of Biotechnology, Beijing, China.
³ Department of Clinical Laboratory, The Third Medical Centre of Chinese PLA General Hospital, Beijing, China.

Abstract

Background: Brucellosis, caused by Brucella spp., is a major zoonotic public health threat. Although several Brucella vaccines have been demonstrated for use in animals, Brucella spp. can cause human infection and to date, there are no human-use vaccines licensed by any agency. Recently, methods in vaccine informatics have made major breakthroughs in peptide-based epitopes, opening up a new avenue of vaccine development.

Objectives: The purpose of this article was to identify potential antigenic peptides in Brucella by proteome and peptidome analyses.

Methods: Mouse infection models were first established by injection with Brucella and spleen protein profiles were then analysed. Subsequently, the major histocompatibility complex class I or II (major histocompatibility complex [MHC]-I/II)-binding peptides in blood samples were collected by immunoprecipitation and peptides derived from Brucella proteins were identified through liquid chromatography-mass spectrometry (LC-MS/MS). These peptides were then evaluated in a variety of ways, such as in terms of conservation in Brucella and synchronicity in predicted peptides (similarity and coverage), which allowed us to more effectively measure their antigenic potential.

Results: The expression of the inflammatory cytokines IL1B and IFN-γ was significantly altered in the spleen of infected mice and some Brucella proteins, such as Muri, AcpP and GroES, were also detected. Meanwhile, in blood, 35 peptides were identified and most showed high conservation, highlighting their potential as antigen epitopes for vaccine development. In particular, we identified four proteins containing both MHC-I- and MHC-II-binding peptides including AtpA, AtpD, DnaK and BAbS19_II02030. They were also compared with the predicted peptides to estimate their reliability.

Conclusions: The peptides we screened could bind to MHC molecules. After being stimulated with antigen T epitopes, Memory T cells can stimulate T cell activation and promote immune responses. Our results indicated that the peptides we identified may be good candidate targets for the design of subunit vaccines and these results pave the way for the study of safer vaccines against Brucella.

Keywords: Brucella abortus; MHC; mass spectrometry; proteomics.

MeSH terms

Animals
Brucella*
Chromatography, Liquid / veterinary
Epitopes
Mice
Peptides
Proteome
Reproducibility of Results
Tandem Mass Spectrometry / veterinary

Substances

Proteome
Epitopes
Peptides

Abstract

MeSH terms

Substances

Grants and funding