FcγRIIB is a T cell checkpoint in antitumor immunity
Clara R. Farley, Anna B. Morris, Marvi Tariq, Kelsey B. Bennion, Sayalee Potdar, Ragini Kudchadkar, Michael C. Lowe, Mandy L. Ford
Clara R. Farley, Anna B. Morris, Marvi Tariq, Kelsey B. Bennion, Sayalee Potdar, Ragini Kudchadkar, Michael C. Lowe, Mandy L. Ford
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Research Article Immunology Oncology

FcγRIIB is a T cell checkpoint in antitumor immunity

Abstract

In the setting of cancer, T cells upregulate coinhibitory molecules that attenuate TCR signaling and lead to the loss of proliferative capacity and effector function. Checkpoint inhibitors currently in clinical use have dramatically improved mortality from melanoma yet are not effective in all patients, suggesting that additional pathways may contribute to suppression of tumor-specific CD8+ T cell responses in melanoma. Here, we show that FcγRIIB, an inhibitory Fc receptor previously thought to be exclusively expressed on B cells and innate immune cells, is upregulated on tumor-infiltrating effector CD8+ T cells in an experimental melanoma model and expressed on CD8+ T cells in patients with melanoma. Genetic deficiency of Fcgr2b resulted in enhanced tumor-infiltrating CD8+ T cell responses and significantly reduced tumor burden. Adoptive transfer experiments of Fcgr2b–/– tumor antigen-specific T cells into FcγRIIB-sufficient hosts resulted in an increased frequency of tumor-infiltrating CD8+ T cells with greater effector function. Finally, FcγRIIB was expressed on CD8+ memory T cells isolated from patients with melanoma. These data illuminate a cell-intrinsic role for the FcγRIIB checkpoint in suppressing tumor-infiltrating CD8+ T cells.

Authors

Clara R. Farley, Anna B. Morris, Marvi Tariq, Kelsey B. Bennion, Sayalee Potdar, Ragini Kudchadkar, Michael C. Lowe, Mandy L. Ford

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Figure 2

FcγRIIB is associated with 2B4 and PD-1 expression on CD44hiCD8+ T cells in the spleen and dLN in mice with melanoma.

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FcγRIIB is associated with 2B4 and PD-1 expression on CD44hiCD8+ T cells...
106 B16-OVA melanoma cells were subcutaneously injected into the right flank of C57BL/6 mice on day 0. Spleen and dLN were harvested on day 14. (A) Using conventional fluorescence-based flow cytometry, bulk CD3+CD8+ T cells (B and C) and CD44hiCD8+ CD3+ T cells (D and E) were gated and exported as FCS files for viSNE analysis. (B) viSNE maps showing the intensity of FcγRIIB, CD44, and CD62L expression on CD8+ T cells in the spleen. (C) viSNE maps showing intensity of FcγRIIB, CD44, and CD62L expression on CD8+ T cells in the dLN. (D) viSNE maps showing intensity of expression of FcγRIIB, 2B4, and PD-1 on CD44hiCD8+ T cells in the spleen. (E) viSNE maps showing intensity of expression of FcγRIIB, 2B4, and PD-1 on CD44hiCD8+ T cells in the dLN. (F) Summary data of the frequency of CD62Lhi, 2B4+, and PD1+FcγRIIB+ and FcγRIIB CD44hiCD8+ T cells in the spleen. (G) Summary data of the frequency of CD62Lhi, 2B4+, and PD1+FcγRIIB+ and FcγRIIB CD44hiCD8+ T cells in the dLN. Data shown are representative of 2 independent experiments; n = 5 mice/group/experiment. Mann-Whitney U test, *P < 0.05, **P < 0.005. dLN, draining lymph node.