Hepatocyte-derived FGL1 accelerates liver metastasis and tumor growth by inhibiting CD8+ T and NK cells
Fengjia Xi, … , Rui Sun, Yongyan Chen
Fengjia Xi, … , Rui Sun, Yongyan Chen
Published July 8, 2024
Citation Information: JCI Insight. 2024;9(13):e173215. https://doi.org/10.1172/jci.insight.173215.
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Research Article Hepatology Immunology

Hepatocyte-derived FGL1 accelerates liver metastasis and tumor growth by inhibiting CD8+ T and NK cells

Abstract

Fibrinogen-like protein 1 (FGL1) contributes to the proliferation and metabolism of hepatocytes; however, as a major ligand of the immune checkpoint, its role in the liver regional immune microenvironment is poorly understood. Hepatocytes specifically and highly expressed FGL1 under normal physiological conditions. Increases in hepatic CD8+ T and NK cell numbers and functions were found in Fgl1-deficient (Fgl1–/–) mice, but not in the spleen or lymph node, similar to findings in anti-FGL1 mAb–treated wild-type mice. Furthermore, Fgl1 deficiency or anti-FGL1 mAb blockade restrained liver metastasis and slowed the growth of orthotopic tumors, with significantly prolonged survival of tumor-bearing mice. Tumor-infiltrating hepatic CD8+ T and NK cells upregulated the expression of lymphocyte activation gene-3 (LAG-3) and exhibited stronger antitumor activities after anti-FGL1 treatment. The antitumor efficacy of FGL1 blockade depended on cytotoxic T lymphocytes and NK cells, demonstrated by using a cell-deficient mouse model and cell transfer in vivo. In vitro, FGL1 directly inhibited hepatic T and NK cells related to the receptor LAG-3. In conclusion, hepatocyte-derived FGL1 played critical immunoregulatory roles in the liver and contributed to liver metastasis and tumor growth by inhibiting CD8+ T and NK cell functions via the receptor LAG-3, providing a new strategy for liver cancer immunotherapy.

Authors

Fengjia Xi, Haoyu Sun, Hui Peng, Zhexiong Lian, Haiming Wei, Zhigang Tian, Rui Sun, Yongyan Chen

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Figure 2

Fgl1-deficient mice exhibit accumulation and activation of CD8+ T and NK cells in the liver.

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Fgl1-deficient mice exhibit accumulation and activation of CD8+ T and N...
(A) Generation and identification method of Fgl1-deficient mice. (B) Genotyping results for Fgl1+/+ and Fgl1–/– alleles in mice. (C) Western blot analysis of FGL1 protein in the livers of Fgl1+/+, Fgl1+/–, and Fgl1–/– mice. β-Tubulin was the internal control. MNCs from the livers, spleens, and lymph nodes (LN) of Fgl1+/+ and Fgl1–/– mice were isolated and analyzed by flow cytometry. (D) Absolute numbers of hepatic CD8+ T cells (left). The expression of CD69 on hepatic CD8+ T cells is shown in a representative dot plot (middle). Frequencies of CD69 on hepatic CD8+ T cells (right). (n = 8 for Fgl1+/+ mice; n = 7 for Fgl1–/– mice.) (E) Absolute numbers of hepatic NK cells (left). Percentages of the CD27CD11b+ NK cell subset in the liver are shown by a representative dot plot and were statistically analyzed (middle). Frequencies of NKG2D on hepatic NK cells. (n = 8 for Fgl1+/+ mice; n = 7 for Fgl1–/– mice.) (F) Absolute numbers of CD8+ T cells and frequencies of CD69 on CD8+ T cells in the spleen and LN of Fgl1+/+ and Fgl1–/– mice. Absolute numbers of NK cells, percentages of the CD27CD11b+ NK cell subset, and frequencies of NKG2D on NK cells in the spleen and LN of Fgl1+/+ and Fgl1–/– mice. Spleen (n = 4 for Fgl1+/+ mice; n = 3 for Fgl1–/– mice), LN (n = 5/group). Data are pooled from 2 independent experiments (D and E) and representative of at least 2 independent experiments (F). Comparisons were performed by using 2-tailed unpaired Student’s t test (DF). Data are presented as the mean ± SEM (DF). ***P < 0.001, *P < 0.05.