# A Host Cell Vector Model for Analyzing Viral Protective Antigens and Host Immunity

**Authors:** Sun-Min Ahn, Jin-Ha Song, Seung-Eun Son, Ho-Won Kim, Gun Kim, Seung-Min Hong, Kang-Seuk Choi, Hyuk-Joon Kwon

PMC · DOI: 10.3390/ijms26157492 · International Journal of Molecular Sciences · 2025-08-02

## TL;DR

Researchers developed a host-cell model to study avian influenza antigens and immune responses, identifying conserved viral epitopes for better vaccine design.

## Contribution

A novel MHC-matched host-cell system was developed to dissect antigen-specific immune responses and identify conserved CD8+ T cell epitopes in avian influenza.

## Key findings

- Live DF-1 cells expressing HA induced strong HI and VN antibody responses in chickens.
- NP-expressing DF-1 cells triggered stronger IFN-γ production than M1-expressing cells.
- Conserved HA and NP epitopes were identified, covering 97.6% and 98.5% of IAV subtypes, respectively.

## Abstract

Avian influenza A viruses (IAVs) pose a persistent threat to the poultry industry, causing substantial economic losses. Although traditional vaccines have helped reduce the disease burden, they typically rely on multivalent antigens, emphasize humoral immunity, and require intensive production. This study aimed to establish a genetically matched host–cell system to evaluate antigen-specific immune responses and identify conserved CD8+ T cell epitopes in avian influenza viruses. To this end, we developed an MHC class I genotype (B21)-matched host (Lohmann VALO SPF chicken) and cell vector (DF-1 cell line) model. DF-1 cells were engineered to express the hemagglutinin (HA) gene of clade 2.3.4.4b H5N1 either transiently or stably, and to stably express the matrix 1 (M1) and nucleoprotein (NP) genes of A/chicken/South Korea/SL20/2020 (H9N2, Y280-lineage). Following prime-boost immunization with HA-expressing DF-1 cells, only live cells induced strong hemagglutination inhibition (HI) and virus-neutralizing (VN) antibody titers in haplotype-matched chickens. Importantly, immunization with DF-1 cells transiently expressing NP induced stronger IFN-γ production than those expressing M1, demonstrating the platform’s potential for differentiating antigen-specific cellular responses. CD8+ T cell epitope mapping by mass spectrometry identified one distinct MHC class I-bound peptide from each of the HA-, M1-, and NP-expressing DF-1 cell lines. Notably, the identified HA epitope was conserved in 97.6% of H5-subtype IAVs, and the NP epitope in 98.5% of pan-subtype IAVs. These findings highlight the platform’s utility for antigen dissection and rational vaccine design. While limited by MHC compatibility, this approach enables identification of naturally presented epitopes and provides insight into conserved, functionally constrained viral targets.

## Linked entities

- **Genes:** ha (hair bristles) [NCBI Gene 251217], CHRM1 (cholinergic receptor muscarinic 1) [NCBI Gene 1128], PNP (purine nucleoside phosphorylase) [NCBI Gene 4860]
- **Diseases:** avian influenza (MONDO:0018695)

## Full-text entities

- **Genes:** MYH11 (myosin, heavy chain 11, smooth muscle) [NCBI Gene 396211], CD8A (CD8A molecule) [NCBI Gene 403158] {aka CD8, CD8-alpha}, INFG (interferon gamma) [NCBI Gene 396054] {aka IFNG}
- **Species:** H5N1 subtype (serotype) [taxon 102793], Gallus gallus (bantam, species) [taxon 9031], H9N2 subtype (serotype) [taxon 102796], Orthomyxoviridae (family) [taxon 11308]
- **Cell lines:** DF-1 — Gallus gallus (Chicken), Spontaneously immortalized cell line (CVCL_XF08)

## Full text

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## Figures

5 figures with captions in the complete paper: https://tomesphere.com/paper/PMC12347372/full.md

## References

35 references — full list in the complete paper: https://tomesphere.com/paper/PMC12347372/full.md

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Source: https://tomesphere.com/paper/PMC12347372