IL-27/Blimp-1 axis regulates the differentiation and function of Tim-3+ Tregs during early pregnancy
Si-Jia Zhao, Xiao-Hui Hu, Xin-Xiu Lin, Yu-Jing Zhang, Jing Wang, Huan Wang, Guang-Shun Gong, Gil Mor, Ai-Hua Liao
Si-Jia Zhao, Xiao-Hui Hu, Xin-Xiu Lin, Yu-Jing Zhang, Jing Wang, Huan Wang, Guang-Shun Gong, Gil Mor, Ai-Hua Liao
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Research Article Immunology Reproductive biology

IL-27/Blimp-1 axis regulates the differentiation and function of Tim-3+ Tregs during early pregnancy

Abstract

Decidual regulatory T cells (Tregs) are essential for successful pregnancy outcome. A subset of Tregs, T cell immunoglobulin and mucin domain-containing protein 3–positive regulatory T cells (TregsTim-3+), plays a central role in the acceptance of the fetus during early stages of normal pregnancy. The molecular mechanism regulating the differentiation and function of TregsTim-3+ is unknown. Here, we investigated the role of the transcription factor B lymphocyte-induced maturation protein 1 (Blimp-1) on decidual TregTim-3+ differentiation. We demonstrated that Blimp-1 enhanced the coexpression of negative costimulatory molecules (Tim-3, T cell immunoreceptor with Ig and ITIM domains, and programmed cell death protein 1) on Tregs and improved their immunosuppressive functions, including increased IL-10 secretion, suppression of effector T cell proliferation, and promotion of macrophage polarization toward the M2 phenotype. Furthermore, we showed that IL-27 regulated the expression of Tim-3 and Blimp-1 through the STAT1 signaling pathway and that transfer of TregsBlimp-1+ into an abortion-prone mouse model effectively reduced embryo absorption rate. We postulated that abnormalities in the IL-27/Blimp-1 axis might be associated with recurrent pregnancy loss (RPL). These findings provided insights for developing more efficient immunotherapies for women with RPL.

Authors

Si-Jia Zhao, Xiao-Hui Hu, Xin-Xiu Lin, Yu-Jing Zhang, Jing Wang, Huan Wang, Guang-Shun Gong, Gil Mor, Ai-Hua Liao

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Figure 5

Upregulation of Tim-3 expression on Tregs by IL-27/Blimp-1 axis.

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Upregulation of Tim-3 expression on Tregs by IL-27/Blimp-1 axis. (A) Sch...
(A) Schematic representation of in vitro culture strategy divided into 3 groups (n = 6): Treg alone (Treg group), Treg + IL-27 (IL-27 group) and Treg + Trophoblast supernatant (Tro-sup group). (B) Representative diagram for FCM and comparison of the proportions of Foxp3+CD4+ T cells, Tim-3+ Tregs, and Tim-3+Blimp-1+ Tregs after 5 days of culture in 3 groups. (C) Schematic diagram illustrating IL-27 downstream signaling pathways. (D) Detection of mRNA levels of IL-27 downstream signaling molecules, including MAPK, PI3K, STAT1, STAT3, and AKT. (E) Detection of the protein levels of IL-27 downstream signaling molecules by Western blotting (WB). (F) Detection of phosphorylated Stat1 and phosphorylated Stat3 levels by FCM. (G) ELISA measurement of IL-27 levels in plasma and decidua from NP, PW, and RPL groups. NP, normal pregnancy; PW, 1 to 2 years postpartum after a normal delivery; RPL, recurrent pregnancy loss. (H) Detection of Blimp-1 expression in decidua by qPCR, WB, and IHC staining in NP and RPL groups. The upper row shows the view under ×200 original magnification (scale bar: 200 μm), and the lower row shows the corresponding magnified view under ×400 original magnification (scale bar: 100 μm). Data are represented as the mean ± SEM via 1-way ANOVA test (B and G) and unpaired, 2-tailed Student’s t test (D and H). *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001.