Antigen processing and presentation in human muscle: cathepsin S is critical for MHC class II expression and upregulated in inflammatory myopathies

Publication

Antigen processing and presentation in human muscle: cathepsin S is critical for MHC class II expression and upregulated in inflammatory myopathies

Journal Paper/Review - May 1, 2003

Wiendl Heinz, Tolosa Eva, Melms Arthur, Lochmüller Hanns, Overkleeft Herman S, Weber Ekkehard, Morgalla Matthias, Wienhold Wolfgang, Erfurth Stella, Krause Sabine, Mitsdörffer Meike, Lautwein Alfred, Driessen Christoph

Units

Medizinische Onkologie und Hämatologie

PubMed

12742663

Citation

Wiendl H, Tolosa E, Melms A, Lochmüller H, Overkleeft H, Weber E, Morgalla M, Wienhold W, Erfurth S, Krause S, Mitsdörffer M, Lautwein A, Driessen C. Antigen processing and presentation in human muscle: cathepsin S is critical for MHC class II expression and upregulated in inflammatory myopathies. Journal of neuroimmunology 2003; 138:132-43.

Type

Journal Paper/Review (English)

Journal

Journal of neuroimmunology 2003; 138

Publication Date

May 1, 2003

Issn Print

0165-5728

Pages

132-43

Brief description/objective

The immunological properties of muscle cells are of critical importance for both the pathogenesis of inflammatory muscle disorders as well as for understanding and controlling novel therapeutic strategies. Muscle cells can present antigens to both CD4 and CD8 cells. However, the cellular biochemistry of antigen processing and presentation by muscle cells is not clear. Cathepsins play a central role in the generation of antigenic peptide and control transport and maturation of MHC class II molecules. To further elucidate the molecular basis for the MHC class II-mediated antigen presentation by muscle cells, we here analyzed cultured human myoblasts and biopsies from inflammatory myopathies with respect to the expression and function of the constituents of the MHC class II antigen presentation machinery. We identified cathepsin S (CatS) as the dominant endocytic protease that is specifically upregulated under inflammatory conditions to significant mRNA levels, synchronously with HLA-DR, -DM and the class II invariant chain (Ii), both in muscle biopsies from affected individuals with inflammatory myopathies and in human myoblasts cultured in the presence of IFN-gamma. This led to translation of the mature CatS polypeptide that was enzymatically active in human myoblasts under inflammatory conditions. By contrast, expression of CatL and CatB was unaffected by IFN-gamma at both the expression and activity levels. CatS activity is required for efficient surface display of MHC class II in this cell type: functional inhibition of CatS using a CatS-selective inhibitor reduced the levels of surface class II alphabeta:peptide complexes on stimulated myoblasts by almost 50%. Surprisingly, and in contrast to B cells and dendritic cells, this was not due to inefficient processing of Ii in the absence of CatS, which was unaffected by the elimination of CatS activity. We therefore conclude that CatS is involved in the regulation of class II expression in human myoblasts independently from Ii processing.