Beryllium-specific CD4+ T cells induced by chemokine neoantigens perpetuate inflammation
Michael T. Falta, … , Clemencia Pinilla, Andrew P. Fontenot
Michael T. Falta, … , Clemencia Pinilla, Andrew P. Fontenot
Published February 25, 2021
Citation Information: J Clin Invest. 2021;131(9):e144864. https://doi.org/10.1172/JCI144864.
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Research Article Pulmonology

Beryllium-specific CD4+ T cells induced by chemokine neoantigens perpetuate inflammation

Abstract

Discovering dominant epitopes for T cells, particularly CD4+ T cells, in human immune-mediated diseases remains a significant challenge. Here, we used bronchoalveolar lavage (BAL) cells from HLA-DP2–expressing patients with chronic beryllium disease (CBD), a debilitating granulomatous lung disorder characterized by accumulations of beryllium-specific (Be-specific) CD4+ T cells in the lung. We discovered lung-resident CD4+ T cells that expressed a disease-specific public CDR3β T cell receptor motif and were specific to Be-modified self-peptides derived from C-C motif ligand 4 (CCL4) and CCL3. HLA-DP2–CCL/Be tetramer staining confirmed that these chemokine-derived peptides represented major antigenic targets in CBD. Furthermore, Be induced CCL3 and CCL4 secretion in the lungs of mice and humans. In a murine model of CBD, the addition of LPS to Be oxide exposure enhanced CCL4 and CCL3 secretion in the lung and significantly increased the number and percentage of CD4+ T cells specific for the HLA-DP2–CCL/Be epitope. Thus, we demonstrate a direct link between Be-induced innate production of chemokines and the development of a robust adaptive immune response to those same chemokines presented as Be-modified self-peptides, creating a cycle of innate and adaptive immune activation.

Authors

Michael T. Falta, Jeremy C. Crawford, Alex N. Tinega, Laurie G. Landry, Frances Crawford, Douglas G. Mack, Allison K. Martin, Shaikh M. Atif, Li Li, Radleigh G. Santos, Maki Nakayama, John W. Kappler, Lisa A. Maier, Paul G. Thomas, Clemencia Pinilla, Andrew P. Fontenot

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Figure 5

An LKGGG CDR3β TCR crossreactive to CCL4 and PLXNA4 peptides.

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An LKGGG CDR3β TCR crossreactive to CCL4 and PLXNA4 peptides. (A) Set of...
(A) Set of CCL4 and PLXNA4 WT (red) and variant peptides that differed at the p4 and p6 positions. Colors highlight D5E8 and amino acids that vary at p4 and p6. (B) IL-2 production by hybridomas 8845-c1 (top) and AV22 (bottom) in response to CCL4 and PLXNA4 WT and variant peptides presented by HLA-DP2–transfected fibroblasts at 300 ng/mL in the presence of BeSO4. Data were normalized to WT peptides (CCL4 for 8845-c1; PLXNA4 for AV22) and are representative of 2 experiments done in duplicate.