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Endoglucanase 2 (Eng2), a shared immunodominant antigen in dimorphic fungi that elicits immunity during infection
Uju J. Okaa, Cleison Ledesma Taira, Lucas dos Santos Dias, Hannah Dobson, Gregory C. Kujoth, Althea Campuzano, E. Jane Homan, George R. Thompson, Chiung-Yu Hung, George S. Deepe Jr, Marcel Wüthrich, Bruce S. Klein
Uju J. Okaa, Cleison Ledesma Taira, Lucas dos Santos Dias, Hannah Dobson, Gregory C. Kujoth, Althea Campuzano, E. Jane Homan, George R. Thompson, Chiung-Yu Hung, George S. Deepe Jr, Marcel Wüthrich, Bruce S. Klein
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Research Article Immunology Infectious disease

Endoglucanase 2 (Eng2), a shared immunodominant antigen in dimorphic fungi that elicits immunity during infection

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Abstract

We describe here a shared surface and cell wall protein, endoglucanase 2 (Eng2), expressed on the etiological agents that cause the endemic systemic mycoses of North America — Blastomyces, Coccidioides, and Histoplasma. We demonstrate that, despite sequence variation of the protein across these related fungi, exposure to Eng2 vaccinated and protected inbred and humanized HLA-DR4 strains of mice against lethal experimental infections with these fungi by eliciting adaptive immunity mediated by CD4+ T cells. We also show that CD4+ T cell precursors against Eng2 were detectable in naive individuals and that patients who had recovered from these infections evinced a memory and recall CD4+ T cell response to Eng2 and its immunodominant epitopes that we have mapped. We created and cataloged new tools and information, such as immunodominant peptide epitopes of Eng2 from each fungus recognized by inbred mice and humans, and we engineered peptide–MHC II tetramers to track T cells in inbred and HLA-DR4–humanized mice. These tools and tetramers will be useful for those who study these infections in mice and humans. Last, because most patients demonstrated immune memory and recall responses against Eng2, our work offers tools for the diagnosis of this collection of infectious diseases across North America.

Authors

Uju J. Okaa, Cleison Ledesma Taira, Lucas dos Santos Dias, Hannah Dobson, Gregory C. Kujoth, Althea Campuzano, E. Jane Homan, George R. Thompson, Chiung-Yu Hung, George S. Deepe Jr, Marcel Wüthrich, Bruce S. Klein

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Figure 5

Vaccine protection conferred by immunodominant peptide versus the full-length protein homolog in WT C57BL/6 mice.

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Vaccine protection conferred by immunodominant peptide versus the full-l...
Mice were vaccinated with Cp-Eng2, Hc-Eng2, and Bl-Eng2 or an equimolar amount of immunodominant peptides from each homolog as described in Methods. Three weeks after the last boost, mice were challenged with a lethal dose of each organism. (A–C) Lung CD4+ T cells were analyzed for the frequency and number of tetramer+ cytokine-producing T cells at day 6 (C. posadasii), day 5 (H. capsulatum), and day 4 (B. dermatitidis) after infection (n = 5 mice/group). Data are represented as the mean ± SD and were analyzed using 1-way ANOVA with post hoc Dunnett’s test. (D) Lung CFU were analyzed 2 weeks after infection when mice in the control group was moribund (n = 10 mice/group). CFU are expressed as log10 and plotted using box-and-whisker plots with error bars showing minimum and maximum values. *P < 0.05 versus all other groups; &P < 0.05 versus protein-vaccinated mice. Data were analyzed using 1-way ANOVA with post hoc analysis by Dunnett’s test.

Copyright © 2025 American Society for Clinical Investigation
ISSN: 0021-9738 (print), 1558-8238 (online)

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