The druggable transcription factor Fli-1 regulates T cell immunity and tolerance in graft-versus-host disease
Steven D. Schutt, … , Yaacov Ben-David, Xue-Zhong Yu
Steven D. Schutt, … , Yaacov Ben-David, Xue-Zhong Yu
Published September 8, 2022
Citation Information: J Clin Invest. 2022;132(21):e143950. https://doi.org/10.1172/JCI143950.
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Research Article Immunology

The druggable transcription factor Fli-1 regulates T cell immunity and tolerance in graft-versus-host disease

Abstract

Graft-versus-host disease (GVHD), manifesting as either acute (aGVHD) or chronic (cGVHD), presents significant life-threatening complications following allogeneic hematopoietic cell transplantation. Here, we investigated Friend virus leukemia integration 1 (Fli-1) in GVHD pathogenesis and validated Fli-1 as a therapeutic target. Using genetic approaches, we found that Fli-1 dynamically regulated different T cell subsets in allogeneic responses and pathogenicity in the development of aGVHD and cGVHD. Compared with homozygous Fli1-deficient or WT T cells, heterozygous Fli1-deficient T cells induced the mildest GVHD, as evidenced by the lowest Th1 and Th17 cell differentiation. Single-cell RNA-Seq analysis revealed that Fli-1 differentially regulated CD4+ and CD8+ T cell responses. Fli-1 promoted the transcription of Th1/Th17 pathways and T cell receptor–inducible (TCR-inducible) transcription factors in CD4+ T cells, while suppressing activation- and function-related gene pathways in CD8+ T cells. Importantly, a low dose of camptothecin, topotecan, or etoposide acted as a potent Fli-1 inhibitor and significantly attenuated GVHD severity, while preserving the graft-versus-leukemia (GVL) effect. This observation was extended to a xenograft model, in which GVHD was induced by human T cells. In conclusion, we provide evidence that Fli-1 plays a crucial role in alloreactive CD4+ T cell activation and differentiation and that targeting Fli-1 may be an attractive strategy for treating GVHD without compromising the GVL effect.

Authors

Steven D. Schutt, Yongxia Wu, Arjun Kharel, David Bastian, Hee-Jin Choi, Mohammed Hanief Sofi, Corey Mealer, Brianyell McDaniel Mims, Hung Nguyen, Chen Liu, Kris Helke, Weiguo Cui, Xian Zhang, Yaacov Ben-David, Xue-Zhong Yu

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Figure 3

Fli-1 regulates T cell pathogenicity in aGVHD.

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Fli-1 regulates T cell pathogenicity in aGVHD. Purified T cells from spl...
Purified T cells from spleens and LNs of Fli1WT/WT, Fli1fl/WT, and Fli1fl/fl mice were CFSE labeled and infused into lethally irradiated BALB/c mice at 2 × 106 cells per mouse. Day-4 representative flow cytometry plots and cumulative frequencies of proliferated (CFSElo) donor+CD4+ cells producing IFN-γ (A) (Fli1WT, n = 6; Fli1fl/WT, n = 6; Fli1fl/fl, n = 6). Lethally irradiated BALB/c mice were transplanted with 5 × 106 TCD-BM from CD45.1 B6 donors supplemented or not with 0.5 × 106 purified total T cells from spleens and LNs of Fli1WT/WT, Fli1fl/WT, and Fli1fl/fl donors. aGVHD representative survival rates (B) and representative aGVHD clinical scores (C) (BM only, n = 7; Fli1WT, n = 17; Fli1fl/WT, n = 15; Fli1fl/fl, n = 15). On day 14 after BMT, the indicated tissues sections were H&E stained for pathologic scoring (D). mLNs were analyzed for donor T cell populations producing IFN-γ, IL-17A, or GM-CSF. Representative flow cytometry plots display IFN-γ–producing T cells in mLNs (E), and cumulative pathology scores are shown (F) (Fli1WT, n = 15; Fli1fl/WT, n = 12; Fli1fl/f,l n = 9). Frequencies of each indicated donor T cell population in mLNs (G) (Fli1WT, n = 5; Fli1fl/WT, n = 3; Fli1fl/fl, n = 2). Data in AF represent 2–3 independent experiments. Data in G were collected from 1 set of mice belonging to 3 independent experiments. Significance was determined using mixed-model tests for clinical scores, a log-rank test for survival data, and 1-way ANOVA for all other data. *P < 0.05 and ***P < 0.001.