Background/Purpose:  Rheumatoid arthritis (RA) is the most frequent form of autoimmune arthritis with a prevalence of almost 1% worldwide. Anti-citrullinated protein antibodies (ACPA) are the most specific biomarker for rheumatoid arthritis (RA)(1). Although therapies designed to deplete B cells, which are the precursor to antibody-secreting cells, are effective in the treatment of RA(2), they only modestly affect ACPA and having no effect on antibodies to recall antigens in serum of treated patients(3). This suggests that autoreactive B cells may contribute to RA pathophysiology by additional mechanisms independent of terminal differentiation toward ACPA-producing plasma cells. Unfortunately, the lack of tools has prevented reliable identification of citrullinated protein (CP)-reactive B cells. Our objective was to develop a novel tool to characterize and model the function of (low-frequency) autoreactive B cells in RA.

Methods:  B-cell clones from either blood or synovial fluid of CCP2+ RA patients were immortalized by a technique previously described for obtaining clones for recall antigens(4). ELISA and FACS were used to identify CCP2-reactive clones and to further characterize surface marker and cytokine expression. BCR-signaling competence was tested by calcium flux, and antigen internalization was visualized on Amnis Imagestream. Global gene expression profiles were interrogated by RNA sequencing.

Results:  We have identified three unique B-cell clones from two RA patients that can secrete antibodies with specific binding to CCP2 yet show no reactivity to the control arginine variant. While clones generated through this method can secrete soluble antibody, they retain surface immunoglobulin expression, mobilize calcium in response to citrullinated protein antigen and can internalize their antigen. Finally, these clones have a unique surface profile of costimulatory molecules and can secrete both pro- and anti-inflammatory cytokines.

Conclusion:  We present here the application of a unique cloning method to establish autoreactive human B-cell clones in RA. We propose that this technique can also be used for other autoimmune diseases with described autoantigen reactivity and that these B cells can be in turn utilized for the identification of autoreactive T cells recognizing novel autoantigen epitopes.

References:

1. Vincent C, Nogueira L, Clavel C, Sebbag M, Serre G. Autoantibodies to citrullinated proteins: ACPA. Autoimmunity. 2005;38(1):17-24.

2. Edwards JC, Szczepanski L, Szechinski J, Filipowicz-Sosnowska A, Emery P, Close DR, et al. Efficacy of B-cell-targeted therapy with rituximab in patients with rheumatoid arthritis. N Engl J Med. 2004;350(25):2572-81.

3. Cambridge G, Leandro MJ, Edwards JC, Ehrenstein MR, Salden M, Bodman-Smith M, et al. Serologic changes following B lymphocyte depletion therapy for rheumatoid arthritis. Arthritis Rheum. 2003;48(8):2146-54.

4. Kwakkenbos MJ, Diehl SA, Yasuda E, Bakker AQ, van Geelen CM, Lukens MV, et al. Generation of stable monoclonal antibody-producing B cell receptor-positive human memory B cells by genetic programming. Nat Med. 2010;16(1):123-8.

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ACR Meeting Abstracts - https://acrabstracts.org/abstract/generation-and-characterization-of-anti-citrullinated-protein-antibody-producing-b-cell-clones/