A stromal platform for robust expansion of functional IL-10–producing B cells for immune regulation
Ryo Kawakami, Keisuke Imabayashi, Akemi Baba, Yuichi Saito, Kazuhiko Kawata, Yutaro Yada, Airi Shibata, Rinka Ito, Ryo Kurasawa, Ryota Higuchi, Sungyeon Park, Hiroaki Niiro, Shinya Tanaka, Yoshihiro Baba
Ryo Kawakami, Keisuke Imabayashi, Akemi Baba, Yuichi Saito, Kazuhiko Kawata, Yutaro Yada, Airi Shibata, Rinka Ito, Ryo Kurasawa, Ryota Higuchi, Sungyeon Park, Hiroaki Niiro, Shinya Tanaka, Yoshihiro Baba
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Research Article Immunology

A stromal platform for robust expansion of functional IL-10–producing B cells for immune regulation

Abstract

IL-10–producing B cells exert immunosuppressive effects, yet their low abundance and poor in vitro viability have limited their therapeutic application. Here, we developed a stromal coculture system using MS5 cells engineered to express human CD40L, BAFF, and IFN-β1 (MS5-3F, for “3 factors”), which enables robust induction and greater than 1000-fold expansion of human IL-10–producing B cells. The expanded cells showed phenotypic and transcriptional profiles characteristic of unswitched (IgM+) plasmablasts and potently suppressed CD4+ T cell proliferation in an IL-10–dependent manner. MS5-3F–expanded B cells also increased the frequency of regulatory T cells in vitro, an effect that was not abrogated by IL-10/IL-10R blockade, suggesting contributions from additional mechanisms. IL-10 production originated predominantly from naive B cells, rather than memory B cells. Furthermore, B cells from patients with systemic lupus erythematosus, despite impaired IL-10 production under conventional conditions, were efficiently differentiated into IL-10–producing B cells using this system. The expanded cells showed minimal IgG-secreting output. Our platform offers a scalable strategy for generating human regulatory B cells, laying the foundation for B cell–based immunotherapies.

Authors

Ryo Kawakami, Keisuke Imabayashi, Akemi Baba, Yuichi Saito, Kazuhiko Kawata, Yutaro Yada, Airi Shibata, Rinka Ito, Ryo Kurasawa, Ryota Higuchi, Sungyeon Park, Hiroaki Niiro, Shinya Tanaka, Yoshihiro Baba

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Figure 2

MS5-3F coculture induces IgM+ plasmablast differentiation from human B cells.

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MS5-3F coculture induces IgM+ plasmablast differentiation from human B c...
(A and B) Temporal changes in activation markers of B cells cocultured with MS5-3F. (A) Representative flow cytometry plots. (B) Frequencies and absolute cell numbers of indicated subsets among CD19+ cells. (C) Representative histograms and summarized MFI of surface markers and transcriptional factors expressed on CD27hi and CD27lo B cells on days 0 and 12 of MS5-3F coculture. See also Supplemental Figure 3. (D) Morphological analysis of primary B cells (day 0) and MS5-3F–induced B cell subsets, stained with May-Grünwald-Giemsa. CD27hi and CD27lo B cells were sorted on day 12 of coculture. Original magnification, ×400. Scale bars: 20 μm. (E) Representative flow cytometry plots of IgM, IgD, and IgG on B cells on day 12 of MS5-3F coculture. (F) Quantification of IgM and IgG antibody production by cocultured B cells. Culture supernatants were harvested every 4 days and analyzed by ELISA. Data from 3 independent experiments were combined (B and C: n = 3 or 9; F: n = 9). Data are presented as mean ± SEM. P values are from 1-way ANOVA with Tukey’s post hoc test (C). **P ≤ 0.01; ***P ≤ 0.001; ****P ≤ 0.0001. NS, not significant.