Designing a chimeric subunit vaccine for influenza virus, based on HA2, M2e and CTxB: a bioinformatics study

Davod Jafari; Sara Malih; Mohammad Mahmoudi Gomari; Marzieh Safari; Rasool Jafari; Mohammad Morad Farajollahi

doi:10.1186/s12860-020-00334-6

BMC Molecular and Cell Biology (Dec 2020)

Designing a chimeric subunit vaccine for influenza virus, based on HA2, M2e and CTxB: a bioinformatics study

Davod Jafari,
Sara Malih,
Mohammad Mahmoudi Gomari,
Marzieh Safari,
Rasool Jafari,
Mohammad Morad Farajollahi

Affiliations

Davod Jafari: Student Research Committee, Faculty of Allied Medicine, Iran University of Medical Sciences
Sara Malih: Department of Medical Biotechnology, Faculty of Medical Sciences, Tarbiat Modares University
Mohammad Mahmoudi Gomari: Department of Medical Biotechnology, Faculty of Allied Medicine, Iran University of Medical Sciences
Marzieh Safari: Department of Microbiology, Faculty of Medicine, Isfahan University of Medical Sciences
Rasool Jafari: Department of Medical Parasitology and Mycology, Faculty of Medicine, Urmia University of Medical Sciences
Mohammad Morad Farajollahi: Student Research Committee, Faculty of Allied Medicine, Iran University of Medical Sciences

DOI: https://doi.org/10.1186/s12860-020-00334-6
Journal volume & issue: Vol. 21, no. 1
pp. 1 – 13

Abstract

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Abstract Background Type A influenza viruses are contagious and even life-threatening if left untreated. So far, no broadly protective vaccine is available due to rapid antigenic changes and emergence of new subtypes of influenza virus. In this study, we exploited bioinformatics tools in order to design a subunit chimeric vaccine from the antigenic and highly conserved regions of HA and M2 proteins of H7N9 subtype of influenza virus. We used mucosal adjuvant candidates, including CTxB, STxB, ASP-1, and LTB to stimulate mucosal immunity and analyzed the combination of HA2, M2e, and the adjuvant. Furthermore, to improve the antigen function and to maintain their three-dimensional structure, 12 different linkers including six rigid linkers and six flexible linkers were used. The 3D structure model was generated using a combination of homology and ab initio modeling methods and the molecular dynamics of the model were analyzed, either. Results Analysis of different adjuvants showed that using CtxB as an adjuvant, results in higher overall vaccine stability and higher half-life among four adjuvant candidates. Fusion of antigens and the CTxB in the form of M2e-linker-CTxB-linker-HA2 has the most stability and half life compared to other combination forms. Furthermore, the KPKPKP rigid linker showed the best result for this candidate vaccine among 12 analyzed linkers. The changes in the vaccine 3D structure made by linker insertion found to be negligible, however, although small, the linker insertion between the antigens causes the structure to change slightly. Eventually, using predictive tools such as Ellipro, NetMHCpan I and II, CD4episcore, CTLpred, BepiPred and other epitope analyzing tools, we analyzed the conformational and linear epitopes of the vaccine. The solubility, proteasome cleavage sites, peptidase and potential chemical cutters, codon optimization, post translational modification were also carried out on the final vaccine. Conclusions It is concluded that M2e-Linker-CTxB-Linker-HA2 combination of chimeric vaccine retains its 3D structure and antigenicity when KPKPKP used as linker and CTxB used as adjuvant.

Published in BMC Molecular and Cell Biology

ISSN: 2661-8850 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Science: Biology (General): Cytology
Website: https://bmcmolcellbiol.biomedcentral.com/

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