Activation of autoreactive lymphocytes in the lung by radioresistant cells expressing a STING gain-of-function mutation
Kevin MingJie Gao, Kristy Chiang, Sharon Subramanian, Xihui Yin, Paul J. Utz, Kerstin Nündel, Kate A. Fitzgerald, Ann Marshak-Rothstein
Kevin MingJie Gao, Kristy Chiang, Sharon Subramanian, Xihui Yin, Paul J. Utz, Kerstin Nündel, Kate A. Fitzgerald, Ann Marshak-Rothstein
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Research Article Inflammation

Activation of autoreactive lymphocytes in the lung by radioresistant cells expressing a STING gain-of-function mutation

Abstract

Gain-of-function mutations in the dsDNA sensing adaptor STING lead to a severe autoinflammatory syndrome known as STING-associated vasculopathy with onset in infancy (SAVI). Patients with SAVI develop interstitial lung disease (ILD) and produce autoantibodies that are commonly associated with systemic autoimmune diseases. Mice expressing the most common SAVI mutation, STING V154M (VM), similarly develop ILD but exhibit severe T and B cell lymphopenia and low serum Ig titers, and they lack autoantibodies. Importantly, lethally irradiated VM hosts reconstituted with WT stem cells (WT→VM) still develop ILD. In this study, we find that WT→VM chimeras had restored B cell function, produced autoantibodies, and thereby recapitulated the loss of tolerance seen in patients with SAVI. Lymphocytes derived from both WT and BCR or TCR transgenic (Tg) donors accumulated in the extravascular lung tissue of WT+Tg→VM mixed chimeras, but lymphocyte activation and germinal center formation required WT cells with a diverse repertoire. Furthermore, when T cells isolated from the WT→VM chimeras were adoptively transferred to naive Rag1-deficient secondary hosts, they trafficked to the lung and recruited neutrophils. Overall, these findings indicated that VM expression by radioresistant cells promoted the activation of autoreactive B cells and T cells that then differentiated into potentially pathogenic effector subsets.

Authors

Kevin MingJie Gao, Kristy Chiang, Sharon Subramanian, Xihui Yin, Paul J. Utz, Kerstin Nündel, Kate A. Fitzgerald, Ann Marshak-Rothstein

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Figure 1

B cell intrinsic VM expression impairs antibody production, proliferation, and survival.

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B cell intrinsic VM expression impairs antibody production, proliferatio...
(A) Serum titers of IgM, IgG1 and IgG2c in age- and sex-matched WT (n = 7) and VM (n = 7–14) mice at 3–4 months of age, or from WT→WT (n = 10–11) and WT→VM (n = 13–15) chimeric mice at 8 weeks after reconstitution. (BG) Splenic B220+ B cells from biologic replicates of WT (n = 6) versus VM (n = 6) B cells and WT→WT (n = 4) and WT→VM (n = 4) B cells labeled with violet proliferative dye (VPD) were stimulated for 72 hours with BLyS alone (NS) or anti≠IgM F(ab’)2 antibody and BLyS (+αIgM), and they were then stained with TOPRO to assess cell death. Cell division is shown by representative VPD histograms (B) and division index (C and D). Cell death is shown by representative TOPRO histograms (E) and percentage of TOPRO live cells (F and G). Nonparametric Mann-Whitney U tests were used for pair-wise comparisons to determine statistical significance (*P < 0.05, **P < 0.01, ***P < 0.001).