Increased dimeric IgA‐producing B cells in tonsils in IgA nephropathy determined by in situ hybridization for J chain mRNA

SUMMARY The origin of mesangial IgA deposits in IgA nephropathy (IgAN) remains obscure. A significant proportion of deposited immunoglobulin is dimeric (J chain‐positive). Previous studies of J chain expression within lymphoid tissue in IgAN have utilized antibodies which other investigators have found to be non‐specific. To address this problem, we have developed an in situ hybridization (ISH) method for the detection of J chain mRNA within IgA plasma cells. Tonsils from 12 patients with IgAN and 12 controls were studied using (i) non‐isotopic ISH for J chain mRNA, and (ii) combined immunofluorescence (IF) and fluorescent ISH. J chain mRNA‐positive cells were identified in germinal centres, and within the subepithelial and interfollicular zones. A greater number of J chain mRNA‐positive cells were found in the germinal centres of patients (mean 57.7±4.6 cells/10 5 μm 2 ) compared with controls (mean 36.9±3.5 cells/10 5 μm 2 ) ( P < 0.001). Combined IF and fluorescent ISH showed a greater proportion of J chain mRNA‐positive interfollicular IgA cells in patient tonsils (3.2±3.4%) compared with controls (21±2.3%; P < 0.02). These results indicate a shift towards dimeric IgA production in the tonsils in IgAN. In addition, the finding of excess numbers of J chain‐positive IgA‐negative cells within germinal centres suggests that an abnormality may be present at the B cell differentiation stage before IgA switching. These results further highlight immune abnormalities within the tonsil as a central feature of abnormal polymeric IgA biology in this common form of glomerulonephritis.