ACR Meeting Abstracts

ACR Meeting Abstracts

Abstract Number: 2732

Massive Ex Vivo Expansion of Functionally Stable Behcet’s Patient-Derived Regulatory T Cell Clones

Johannes Nowatzky1, Olivier Manches1, Yusuf Yazici2 and Juan Lafaille1, 1New York University School of Medicine, New York, NY, 2Department of Medicine, Division of Rheumatology, New York University School of Medicine, New York, NY

Meeting: 2014 ACR/ARHP Annual Meeting

Keywords: ,

Session Information

Title: T cell Biology in Lupus, Vasculitis, Myositis and Other Autoimmunity

Session Type: Abstract Submissions (ACR)

Background/Purpose: Adoptive transfer of regulatory T cells (Treg) is a promising strategy for the treatment of human autoimmune diseases. Most currently tested approaches focus on the polyclonal expansion of human thymus-derived Treg (tTreg), and are limited by potentially harmful and efficacy-limiting co-expansion of effector T cells (Teff). We hypothesized that the ex vivo isolation and massive expansion of CD4+/CD25high/CD127low/FoxP3+/HeliostTreg clones results in maximal purity of the generated cellular product, preserving its suppressor function stability over several re-expansion cycles while yielding cell numbers sufficient for preclinical and clinical testing.

Methods: To validate our approach for a human rheumatic disease in which antigen-specific T effector responses have been implicated in target organ damage (uveitis), we chose to identify and expand Behcet’s disease patient-derived tTreg clones. CD4+/CD25high/CD127low T cells were isolated by magnetic bead separation, subsequently cloned in a limiting dilution approach and massively expanded in at least four re-expansion cycles. Suppression was tested in suppression assays of CD3/CD28-stimulated effector T cells at repeated expansion cycles over at least 8 weeks. Clonality was demonstrated by Vβ staining.

Results: Cloning efficiency was 2-5/100 seeded cells. Treg clones were homogeneously CD4+/CD25high/FoxP3+/Heliosand stained positive for one unique TCR Vβ chain. Clones maintained around 80% suppression at 1:4 Treg:Teff ratios over as long as 11 weeks in culture and at least 4 re-expansion cycles. Proliferation was in the 108 to 109-fold range at day 50. When compared to tTreg clones generated from healthy human donors there were no significant differences in suppressive capacity, suppressor function stability, or phenotype.

Conclusion: Our results suggest that tTreg are not intrinsically dysfunctional in Behcet’s disease, and they deliver proof of principle that the massive monoclonal expansion of antigen-specific human Treg clones from patients with a rheumatic disease is possible and yields a functionally stable, ultra-pure cellular product for pre-clinical and clinical testing.

Disclosure:

J. Nowatzky,
None;

O. Manches,
None;

Y. Yazici,
None;

J. Lafaille,
None.

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