Maintenance DNA methylation is required for induced Treg reparative function following viral pneumonia in mice
Anthony M. Joudi, Jonathan K. Gurkan, Qianli Liu, Elizabeth M. Steinert, Manuel A. Torres Acosta, Kathryn A. Helmin, Luisa Morales-Nebreda, Nurbek Mambetsariev, Carla Patricia Reyes Flores, Hiam Abdala-Valencia, Samuel E. Weinberg, Benjamin D. Singer
Anthony M. Joudi, Jonathan K. Gurkan, Qianli Liu, Elizabeth M. Steinert, Manuel A. Torres Acosta, Kathryn A. Helmin, Luisa Morales-Nebreda, Nurbek Mambetsariev, Carla Patricia Reyes Flores, Hiam Abdala-Valencia, Samuel E. Weinberg, Benjamin D. Singer
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Research Article Immunology Inflammation Pulmonology

Maintenance DNA methylation is required for induced Treg reparative function following viral pneumonia in mice

Abstract

FOXP3+ natural regulatory T cells (nTregs) promote resolution of inflammation and repair of epithelial damage following viral pneumonia–induced lung injury, thus representing a cellular therapy for patients with severe viral pneumonia and the acute respiratory distress syndrome. Whether in vitro–induced Tregs (iTregs), which can be rapidly generated in substantial numbers from conventional T cells, also promote lung recovery is unknown. nTregs require specific DNA methylation patterns maintained by the epigenetic regulator ubiquitin-like with PHD and RING finger domains 1 (UHRF1). Here, we tested whether iTregs promote recovery following viral pneumonia and whether iTregs require UHRF1 for their pro-recovery function. We found that adoptive transfer of iTregs to mice with influenza virus pneumonia promotes lung recovery and that loss of UHRF1-mediated maintenance DNA methylation in iTregs leads to reduced engraftment and a delayed repair response. Transcriptional and DNA methylation profiling of adoptively transferred UHRF1-deficient iTregs that had trafficked to influenza-injured lungs demonstrated transcriptional instability with gain of transcription factors that define effector T cell lineage. Strategies to promote the stability of iTregs could be leveraged to further augment their pro-recovery function during viral pneumonia and other causes of severe lung injury.

Authors

Anthony M. Joudi, Jonathan K. Gurkan, Qianli Liu, Elizabeth M. Steinert, Manuel A. Torres Acosta, Kathryn A. Helmin, Luisa Morales-Nebreda, Nurbek Mambetsariev, Carla Patricia Reyes Flores, Hiam Abdala-Valencia, Samuel E. Weinberg, Benjamin D. Singer

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Figure 4

UHRF1-deficient iTregs promote an insufficient tissue-protective response during peak lung injury.

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UHRF1-deficient iTregs promote an insufficient tissue-protective respons...
Foxp3GFP-DTR mice were treated with DTx every 48 hours beginning 2 days before inoculation with 6.5 PFU of influenza A/WSN/33 H1N1 virus and received retro-orbital adoptive transfer of 1 × 106 Uhrf1fl/fl or Uhrf1+/+ iTregs at 5 DPI. iTregs were treated with tamoxifen from day 0 to day 3 of culture and harvested for adoptive transfer on culture day 5. Recipient mice were euthanized 11 DPI, and lungs and spleen were analyzed by flow cytometry. Epithelial cell data are derived from the post-caval lobes. Transferred iTreg quantification is derived from the remaining lung lobes. (A) Total number of ATII cells (n = 15 per group). (B) Total number of Ki-67+ ATII cells (Uhrf1+/+ iTregs n = 13, Uhrf1fl/fl iTregs n = 14). (C) Total number of CD326CD31+ (endothelial) cells (Uhrf1+/+ iTregs n = 14, Uhrf1fl/fl iTregs n = 15). (D) Frequency of tdTomato+ cells in lung (n = 16 per group). (E) Total number of tdTomato+ cells in lung (n = 16 per group). (F) Frequency of Foxp3-GFPtdTomato+ (ex-FOXP3) cells in lung (Uhrf1+/+ n = 15, Uhrf1fl/fl n = 16). (G) Frequency of tdTomato+ cells in spleen (n = 8 per group). (H) Total number of tdTomato+ cells in spleen (n = 4 per group). (I) Frequency of Foxp3-GFPtdTomato+ cells in spleen (n = 8 per group). Data presented as mean and SD. *P < 0.05, **P < 0.005, according to Mann-Whitney U test. Data in AF generated from 2 independent experiments. Data in GI generated from 1 independent experiment.