The IFN-γ receptor promotes immune dysregulation and disease in STING gain-of-function mice
W. Alexander Stinson, Cathrine A. Miner, Fang R. Zhao, Annena Jane Lundgren, Subhajit Poddar, Jonathan J. Miner
W. Alexander Stinson, Cathrine A. Miner, Fang R. Zhao, Annena Jane Lundgren, Subhajit Poddar, Jonathan J. Miner
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Research Article Inflammation

The IFN-γ receptor promotes immune dysregulation and disease in STING gain-of-function mice

Abstract

STING gain-of-function mutations cause STING-associated vasculopathy with onset in infancy (SAVI) in humans, a disease characterized by spontaneous lung inflammation and fibrosis. Mice with STING gain-of-function mutations (SAVI mice) develop αβ T cell–dependent lung disease and also lack lymph nodes. Although SAVI has been regarded as a type I interferonopathy, the relative contributions of the three interferon receptors are incompletely understood. Here, we show that STING gain of function led to upregulation of IFN-γ–induced chemokines in the lungs of SAVI mice and that deletion of the type II IFN receptor (IFNGR1), but not the type I IFN receptor (IFNAR1) or type III IFN receptor (IFNλR1), ameliorated lung disease and restored lymph node development in SAVI mice. Furthermore, deletion of IFNGR1, but not IFNAR1 or IFNλR1, corrected the ratio of effector to Tregs in SAVI mice and in mixed bone marrow chimeric mice. Finally, cultured SAVI mouse macrophages were hyperresponsive to IFN-γ, but not IFN-β, in terms of Cxcl9 upregulation and cell activation. These results demonstrate that IFNGR1 plays a major role in autoinflammation and immune dysregulation mediated by STING gain of function.

Authors

W. Alexander Stinson, Cathrine A. Miner, Fang R. Zhao, Annena Jane Lundgren, Subhajit Poddar, Jonathan J. Miner

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Figure 7

SAVI mouse T cells lacking the type II IFN receptor have a survival advantage in mixed bone marrow chimeric mice.

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SAVI mouse T cells lacking the type II IFN receptor have a survival adva...
(A) Diagram of the strategy used to generate Thy1.1 mixed bone marrow chimeric mice. (B) Representative FACS plot of the CD45.1/2 STING N153S (SAVI) and CD45.2 Ifngr1–/– SAVI mouse bone marrow cells, which were transferred at an approximately 1:1 ratio. (C) Representative FACS plots depicting donor (Thy1.1) cell chimerism within circulating CD3ε+ T cells and CD25+ FoxP3+ Tregs in the irradiated Thy1.1+ animals. (D) Percentages of circulating CD45.1/2 SAVI and CD45.2 Ifngr1–/– STING N153S CD3ε+, CD4+, CD8α+ T cells and CD25+FoxP3+ Tregs in irradiated Thy1.1+ animals. (E) Representative FACS plots depicting the distribution of late apoptotic donor CD3ε+ T cells (defined as annexin V+ LIVE/DEAD+) in the irradiated Thy1.1+ chimeric mice shown. Shown are CD45.1/2 SAVI (left) and CD45.2 Ifngr1–/– SAVI T cells (right). (F) Percentage of annexin V+ LIVE/DEAD+ CD45.1/2 SAVI and CD45.2 Ifngr1–/– SAVI CD3ε+, CD4+, and CD8α+ T cells. Data in C, E, and F represent the mean ± SEM of the indicated T cell populations isolated from the spleens of n = 12 Thy1.1+ chimeric mice from 2 independent experiments. Data were analyzed by Mann-Whitney test. ***P < 0.001, ****P < 0.0001.