Irgm1 coordinately regulates autoimmunity and host defense at select mucosal surfaces
Kathleen M. Azzam, … , Gregory A. Taylor, Michael B. Fessler
Kathleen M. Azzam, … , Gregory A. Taylor, Michael B. Fessler
Published August 17, 2017
Citation Information: JCI Insight. 2017;2(16):e91914. https://doi.org/10.1172/jci.insight.91914.
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Research Article Pulmonology

Irgm1 coordinately regulates autoimmunity and host defense at select mucosal surfaces

Abstract

The pathogenesis of primary Sjogren’s syndrome (SS), an autoimmune disease that targets the mucosa of exocrine tissues, is poorly understood. Although several mouse models have been developed that display features of SS, most of these are within the larger context of a lupus-like presentation. Immunity-related GTPase family M protein 1 (Irgm1) is an interferon-inducible cytoplasmic GTPase that is reported to regulate autophagy and mitochondrial homeostasis. Here, we report that naive Irgm1–/– mice display lymphocytic infiltration of multiple mucosal tissues including the lung in a manner reminiscent of SS, together with IgA class–predominant autoantibodies including anti-Ro and anti-La. This phenotype persists in the germ-free state, but is abolished by deletion of Irgm3. Irgm1–/– mice have increased local production in the lung of TECP15-idiotype IgA, a natural antibody with dual reactivity against host and pneumococcal phosphorylcholine. Associated with this, Irgm1–/– mice display enhanced opsonization and clearance of Streptococcus pneumoniae from the lung and increased survival from pneumococcal pneumonia. Taken together, our results identify Irgm1 as a master regulator of mucosal immunity that dually modulates evolutionarily conserved self- and other-directed immune responses at the interface of host with environment.

Authors

Kathleen M. Azzam, Jennifer H. Madenspacher, Derek W. Cain, Lihua Lai, Kymberly M. Gowdy, Prashant Rai, Kyathanahalli Janardhan, Natasha Clayton, Willie Cunningham, Heather Jensen, Preeyam S. Patel, John F. Kearney, Gregory A. Taylor, Michael B. Fessler

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Figure 1

Peribronchovascular lymphocytic infiltrates in the Irgm1–/– lung.

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Peribronchovascular lymphocytic infiltrates in the Irgm1–/– lung. (A) He...
(A) Hematoxylin and eosin–stained lungs from naive Irgm1–/– mice and littermate controls. Original magnification, ×1.1. (B) Peribronchovascular cellular infiltrates in Irgm1–/– lungs were evaluated by immunohistochemical (IHC) staining for CD3 (T cells) and Pax5 (B cells). Original magnification, ×20. (C) Irgm1–/– lung lesions were IHC stained for the targets shown. Original magnification, ×20. (D) B cells (CD45+CD19+CD3), and CD4+ and CD8+ T cells (CD45+CD19CD3+) were quantified by flow cytometry in lung digests from naive Irgm1–/– mice and controls (n = 4/genotype). (E) B1a (CD19+CD5+CD11b+IgMhi), B1b (CD19+CD5CD11b+IgMhi), and B2 (CD19+CD5CD11bIgMlo) cells were quantified by flow cytometry in lung digests from naive Irgm1–/–mice and controls (n = 4–6/genotype). Histology and IHC data are representative of at least 4–5 mice/genotype. Graphed data are the mean ± SEM and are representative of at least 3 independent experiments. *P < 0.05, ***P < 0.001 by unpaired 2-tailed Student’s t test.