Clonal analysis of SepSecS-specific B and T cells in autoimmune hepatitis
Michael Kramer, … , Benedetta Terziroli Beretta-Piccoli, Federica Sallusto
Michael Kramer, … , Benedetta Terziroli Beretta-Piccoli, Federica Sallusto
Published January 16, 2025
Citation Information: J Clin Invest. 2025;135(2):e183776. https://doi.org/10.1172/JCI183776.
View: Text | PDF
Research Article Autoimmunity Immunology

Clonal analysis of SepSecS-specific B and T cells in autoimmune hepatitis

Abstract

Autoimmune hepatitis (AIH) is a rare chronic inflammatory liver disease characterized by the presence of autoantibodies, including those targeting O-phosphoseryl-tRNA:selenocysteine-tRNA synthase (SepSecS), also known as soluble liver antigen (SLA). Anti-SepSecS antibodies have been associated with a more severe phenotype, suggesting a key role for the SepSecS autoantigen in AIH. To analyze the immune response to SepSecS in patients with AIH at the clonal level, we combined sensitive high-throughput screening assays with the isolation of monoclonal antibodies (mAbs) and T cell clones. The anti-SepSecS mAbs isolated were primarily IgG1, affinity-matured compared with their germline versions, and recognized at least 3 nonoverlapping epitopes. SepSecS-specific CD4+ T cell clones were found in patients with AIH who were anti-SLA-positive and anti-SLA-negative,and, to a lesser extent, in patients with non-AIH liver diseases and in healthy individuals. SepSecS-specific T cell clones from patients with AIH produced IFN-γ, IL-4, and IL-10, targeted multiple SepSecS epitopes, and, in one patient, were clonally expanded in both blood and liver biopsy. Finally, SepSecS-specific B cell clones, but not those of unrelated specificities, were able to present soluble SepSecS to specific T cells. Collectively, our study provides the first detailed analysis of B and T cell repertoires targeting SepSecS in patients with AIH, offering a rationale for improved targeted therapies.

Authors

Michael Kramer, Federico Mele, Sandra Jovic, Blanca Maria Fernandez, David Jarrossay, Jun Siong Low, Christiane Sokollik, Magdalena Filipowicz Sinnreich, Sylvie Ferrari-Lacraz, Giorgina Mieli-Vergani, Diego Vergani, Antonio Lanzavecchia, Antonino Cassotta, Benedetta Terziroli Beretta-Piccoli, Federica Sallusto

×

Figure 3

SepSecS-specific mAb recognize different epitopes and acquire high affinity through somatic mutations.

Options: View larger image (or click on image) Download as PowerPoint
SepSecS-specific mAb recognize different epitopes and acquire high affin...
(A) Competition-ELISA identifying 3 groups of recombinantly produced mAbs with different binding regions. ELISA-plates were coated for 24 hours at 4°C with 5 μg/mL SepSecS. First, mAbs were added in excess (20 μg/mL) to block mAb-specific epitopes completely. Biotinylated mAbs were added as second mAbs, and binding was assessed using streptavidin-HRP. The 12 recombinant mAbs were analyzed in 2 independent experiments of 7 (upper 3 plots) and 5 mAbs (lower 2 plots). MAb codes start with number of the patient with AIH from whom the mAb is derived. (B) EC50 values of SepSecS binding of recombinantly produced mAbs carrying different combinations of mutated (M) and germline (GL) heavy and light chain of the indicated mAbs as measured by flow cytometry assay. MAb codes start with number of the patient with AIH from whom the mAb is derived.