HLA A*24:02–restricted T cell receptors cross-recognize bacterial and preproinsulin peptides in type 1 diabetes
Garry Dolton, … , Pierre J. Rizkallah, Andrew K. Sewell
Garry Dolton, … , Pierre J. Rizkallah, Andrew K. Sewell
Published September 17, 2024
Citation Information: J Clin Invest. 2024;134(18):e164535. https://doi.org/10.1172/JCI164535.
View: Text | PDF
Research Article Autoimmunity Immunology Article has an altmetric score of 127

HLA A*24:02–restricted T cell receptors cross-recognize bacterial and preproinsulin peptides in type 1 diabetes

Abstract

CD8+ T cells destroy insulin-producing pancreatic β cells in type 1 diabetes through HLA class I–restricted presentation of self-antigens. Combinatorial peptide library screening was used to produce a preferred peptide recognition landscape for a patient-derived T cell receptor (TCR) that recognized the preproinsulin-derived (PPI-derived) peptide sequence LWMRLLPLL in the context of disease risk allele HLA A*24:02. Data were used to generate a strong superagonist peptide, enabling production of an autoimmune HLA A*24:02–peptide–TCR structure by crystal seeding. TCR binding to the PPI epitope was strongly focused on peptide residues Arg4 and Leu5, with more flexibility at other positions, allowing the TCR to strongly engage many peptides derived from pathogenic bacteria. We confirmed an epitope from Klebsiella that was recognized by PPI-reactive T cells from 3 of 3 HLA A*24:02+ patients. Remarkably, the same epitope selected T cells from 7 of 8 HLA A*24+ healthy donors that cross-reacted with PPI, leading to recognition and killing of HLA A*24:02+ cells expressing PPI. These data provide a mechanism by which molecular mimicry between pathogen and self-antigens could have resulted in the breaking of self-tolerance to initiate disease.

Authors

Garry Dolton, Anna Bulek, Aaron Wall, Hannah Thomas, Jade R. Hopkins, Cristina Rius, Sarah A.E. Galloway, Thomas Whalley, Li Rong Tan, Théo Morin, Nader Omidvar, Anna Fuller, Katie Topley, Md Samiul Hasan, Shikha Jain, Nirupa D’Souza, Thomas Hodges-Hoyland, the TIRID Consortium, Owen B. Spiller, Deborah Kronenberg-Versteeg, Barbara Szomolay, Hugo A. van den Berg, Lucy C. Jones, Mark Peakman, David K. Cole, Pierre J. Rizkallah, Andrew K. Sewell

×

Figure 1

Sizing scan and positional scanning CPL screening of 4C6 T cells.

Options: View larger image (or click on image) Download as PowerPoint
Sizing scan and positional scanning CPL screening of 4C6 T cells. (A) Th...
(A) The 4C6 T cell clone was incubated overnight with sizing scan mixtures of defined amino acid length (x axis) using C1R-HLA A*24:02 as antigen-presenting cells. Assay supernatants used for MIP-1β ELISA. Data points shown for duplicate conditions. (B) Based on the results of the sizing scan, a 9-mer positional scanning CPL (PS-CPL) screen was performed, using 4C6 T cells and antigen-presenting cells and ELISA as in A. Key: Green bars indicate amino acid present in the natural PPI epitope; and magenta bars and arrows show amino acid present in the superagonist peptide (shared amino acid residues are underlined). Data points shown for duplicate conditions. A replicate assay gave similar results. (C) Motif logo plot summarizing the amino acid preference of 4C6 at each position of the PS-CPL.