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Circulating CASK is associated with recurrent focal segmental glomerulosclerosis after transplantation.

PloS one (2019-07-30)
Severine Beaudreuil, Xiaomeng Zhang, Florence Herr, Francis Harper, Jean Jacques Candelier, Ye Fan, Hilal Yeter, Caroline Dudreuilh, Lola Lecru, Aime Vazquez, Bernard Charpentier, Hans K Lorenzo, Antoine Durrbach
RÉSUMÉ

Focal and Segmental GlomeruloSclerosis (FSGS) can cause nephrotic syndrome with a risk of progression to end-stage renal disease. The idiopathic form has a high rate of recurrence after transplantation, suggesting the presence of a systemic circulating factor that causes glomerular permeability and can be removed by plasmapheresis or protein-A immunoadsorption. To identify this circulating factor, the eluate proteins bound on therapeutic immunoadsorption with protein-A columns were analyzed by comparative electrophoresis and mass spectrometry. A soluble form of calcium/calmodulin-dependent serine protein kinase (CASK) was identified. CASK was immunoprecipitated only in the sera of patients with recurrent FSGS after transplantation and not in control patients. Recombinant-CASK (rCASK) induced the reorganization of the actin cytoskeleton in immortalized podocytes, a redistribution of synaptopodin, ZO-1,vinculin and ENA. rCASK also induced alterations in the permeability of a monolayer of podocytes and increased the motility of pdodocytes in vitro. The extracellular domain of CD98, a transmembrane receptor expressed on renal epithelial cells, has been found to co-immunoprecipitated with rCASK. The invalidation of CD98 with siRNA avoided the structural changes of rCask treated cells suggesting its involvement in physiopathology of the disease. In mice, recombinant CASK induced proteinuria and foot process effacement in podocytes. Our results suggest that CASK can induce the recurrence of FSGS after renal transplantation.

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Sigma-Aldrich
Anti-Vinculin antibody, Mouse monoclonal, clone VIN-11-5, purified from hybridoma cell culture