Fgl2 regulates FcγRIIB+CD8+ T cell responses during infection
Anna B. Morris, … , Colleen S. Kraft, Mandy L. Ford
Anna B. Morris, … , Colleen S. Kraft, Mandy L. Ford
Published April 8, 2025
Citation Information: JCI Insight. 2025;10(7):e186259. https://doi.org/10.1172/jci.insight.186259.
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Research Article Immunology

Fgl2 regulates FcγRIIB+CD8+ T cell responses during infection

Abstract

While the inhibitory receptor FcγRIIB has been shown to be upregulated on activated CD8+ T cells in both mice and humans, its effect on T cell fate during infection has not been fully elucidated. We identified an increase in FcγRIIB-expressing CD8+ T cells in patients with COVID-19 relative to healthy controls as well as in mouse models of viral infection. Despite its well-known role as an Fc receptor, FcγRIIB also ligates the immunosuppressive cytokine Fgl2, resulting in CD8+ T cell apoptosis. Both chronic LCMV infection in mice and COVID-19 in humans resulted in a significant increase in plasma Fgl2. Transfer of CD8+ T cells into a Fgl2-replete, but not Fgl2-devoid, environment resulted in elimination of FcγRIIB+, but not FcγRIIB–, CD8+ T cells. Similarly, plasma Fgl2 was directly proportional to CD8+ T cell lymphopenia in patients with COVID-19. RNA-Seq analysis demonstrated that Fgl2 was produced by murine virus–specific CD8+ T cells, with an increase in Fgl2 in CD8+ T cells elicited during chronic versus acute viral infection. Fgl2 was also upregulated in CD8+ T cells from patients with COVID-19 versus healthy controls. In summary, CD8+ T cell production of Fgl2 during viral infection underpinned an FcγRIIB-mediated loss of CD8+ T cell immunity in both mice and humans.

Authors

Anna B. Morris, Max W. Adelman, Kelsey B. Bennion, Catherine D. Martinez, Kem-Maria McCook, Michael H. Woodworth, Charles R. Langelier, Nadine Rouphael, Christopher D. Scharer, Cheryl L. Maier, Colleen S. Kraft, Mandy L. Ford

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Figure 1

FcγRIIB is upregulated on CD8+ T cells isolated from patients with COVID.

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FcγRIIB is upregulated on CD8+ T cells isolated from patients with COVID...
Patients testing positive for SARS CoV-2 admitted as inpatients at Emory University Hospital from May to July 2020 (n = 31; Table 1) and normal healthy controls (n = 15) were consented for blood draw and CD8+ T cells were analyzed by flow cytometry. (A) Bulk CD8+ T cell frequencies were analyzed by Mann-Whitney U nonparametric test. (B) Frequencies of naive (CCR7+CD45RA+), TCM (CCR7+CD45RA), TEM (CCR7CD45RA), and TEMRA (CCR7CD45RA+) cells among CD8+ T cells are shown (analyzed by 2-way ANOVA). (C and D) Flow cytometry data were subjected to spanning-tree progression analysis for density-normalized events (SPADE) analysis. Shaded areas represent clusters of cells that were differentially represented in healthy individuals versus patients with COVID. Phenotypic characteristics of cells in those clusters are shown in D. Intensity of expression (MFI) is indicated by colorimetric scale. (EG) Flow cytometry data were analyzed via FlowJo. (E) Representative flow cytometry staining of FcγRIIB+ cells among CD8+ T cells. (F) Summary data of FcγRIIB+ cells among CD8+ cells (Mann-Whitney U nonparametric test). (G) Summary data of FcγRIIB+ cells among CD8+ Tem (Mann-Whitney U nonparametric test). Data are depicted as mean ± SEM. *P < 0.05, **P < 0.01, ***P < 0.001.