Tregs from human blood differentiate into nonlymphoid tissue–resident effector cells upon TNFR2 costimulation
Mark Mensink, Lotte J. Verleng, Ellen Schrama, George M.C. Janssen, Rayman T.N. Tjokrodirijo, Peter A. van Veelen, Qinyue Jiang, M. Fernanda Pascutti, Marie-Louise van der Hoorn, Michael Eikmans, Sander de Kivit, Jannie Borst
Mark Mensink, Lotte J. Verleng, Ellen Schrama, George M.C. Janssen, Rayman T.N. Tjokrodirijo, Peter A. van Veelen, Qinyue Jiang, M. Fernanda Pascutti, Marie-Louise van der Hoorn, Michael Eikmans, Sander de Kivit, Jannie Borst
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Research Article Immunology

Tregs from human blood differentiate into nonlymphoid tissue–resident effector cells upon TNFR2 costimulation

Abstract

Tregs can facilitate transplant tolerance and attenuate autoimmune and inflammatory diseases. Therefore, it is clinically relevant to stimulate Treg expansion and function in vivo and to create therapeutic Treg products in vitro. We report that TNF receptor 2 (TNFR2) is a unique costimulus for naive, thymus-derived Tregs (tTregs) from human blood that promotes their differentiation into nonlymphoid tissue–resident (NLT-resident) effector Tregs, without Th-like polarization. In contrast, CD28 costimulation maintains a lymphoid tissue–resident (LT-resident) Treg phenotype. We base this conclusion on transcriptome and proteome analysis of TNFR2- and CD28-costimulated CD4+ tTregs and conventional T cells (Tconvs), followed by bioinformatic comparison with published transcriptomic Treg signatures from NLT and LT in health and disease, including autoimmunity and cancer. These analyses illuminate that TNFR2 costimulation promoted tTreg capacity for survival, migration, immunosuppression, and tissue regeneration. Functional studies confirmed improved migratory ability of TNFR2-costimulated tTregs. Flow cytometry validated the presence of the TNFR2-driven tTreg signature in effector/memory Tregs from the human placenta, as opposed to blood. Thus, TNFR2 can be exploited as a driver of NLT-resident tTreg differentiation for adoptive cell therapy or antibody-based immunomodulation in human disease.

Authors

Mark Mensink, Lotte J. Verleng, Ellen Schrama, George M.C. Janssen, Rayman T.N. Tjokrodirijo, Peter A. van Veelen, Qinyue Jiang, M. Fernanda Pascutti, Marie-Louise van der Hoorn, Michael Eikmans, Sander de Kivit, Jannie Borst

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Figure 1

CD28 and TNFR2 costimulation differentially affect naive Tconvs and Tregs.

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CD28 and TNFR2 costimulation differentially affect naive Tconvs and Treg...
Naive Tconvs and Tregs were purified from human peripheral blood and stimulated as indicated in Supplemental Figure 1. (A) Cell division assessed by CellTrace Violet (CTV) dilution in naive Tconvs and Tregs stimulated as indicated for 4 days (representative of n = 3). (B) Expansion of CD28- or TNFR2-costimulated Tconvs and Tregs, calculated by the ratio of live cell number on day 7 versus start of culture. Color legend as in A. Statistical analysis by 2-way ANOVA with Bonferroni’s post hoc test (n = 9). (C) Purity assessment of Treg cultures on day 7 by FOXP3 and Helios/IKZF2 expression, with representative plots (left) and FOXP3Helios cell frequencies (right). Statistical analysis by paired 2-tailed Student’s t test (n = 15). (D) Flow cytometric analysis of FOXP3 (n = 18), Helios/IKZF2 (n = 18), and Eos/IKZF4 (n = 7) in tTregs on day 7. Representative plots and quantified protein expression by mean fluorescence intensity (MFI) are shown. Color legend as in A. Statistical analysis by paired 2-tailed Student’s t test. (AD) Data are presented as mean ± SEM. Size (n) represents individual donors, analyzed in independent experiments. ***P < 0.001, ****P < 0.0001. (E) PCA of transcriptomics data from Tconvs and tTregs analyzed on day 7 (n = 5). (F) Volcano plots of transcriptomics data comparing CD28- or TNFR2-costimulated tTregs and Tconvs. Selected differentially expressed genes (FDR < 0.05) characteristic of Tconvs or Tregs are annotated. (G) GSEA evaluating the expression of signature genes of human Treg or Tconvs according to Ferraro et al. (27) in our transcriptomics data sets of CD28- or TNFR2-costimulated tTreg and Tconvs. Normalized enrichment scores (NES) are shown (FDR < 0.05).