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Endothelial cells in the innate response to allergens and initiation of atopic asthma
Kewal Asosingh, … , Mark Aronica, Serpil Erzurum
Kewal Asosingh, … , Mark Aronica, Serpil Erzurum
Published June 18, 2018
Citation Information: J Clin Invest. 2018;128(7):3116-3128. https://doi.org/10.1172/JCI97720.
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Research Article Angiogenesis Pulmonology

Endothelial cells in the innate response to allergens and initiation of atopic asthma

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Abstract

Protease-activated receptor 2 (PAR-2), an airway epithelial pattern recognition receptor (PRR), participates in the genesis of house dust mite–induced (HDM-induced) asthma. Here, we hypothesized that lung endothelial cells and proangiogenic hematopoietic progenitor cells (PACs) that express high levels of PAR-2 contribute to the initiation of atopic asthma. HDM extract (HDME) protease allergens were found deep in the airway mucosa and breaching the endothelial barrier. Lung endothelial cells and PACs released the Th2-promoting cytokines IL-1α and GM-CSF in response to HDME, and the endothelium had PAC-derived VEGF-C–dependent blood vessel sprouting. Blockade of the angiogenic response by inhibition of VEGF-C signaling lessened the development of inflammation and airway remodeling in the HDM model. Reconstitution of the bone marrow in WT mice with PAR-2–deficient bone marrow also reduced airway inflammation and remodeling. Adoptive transfer of PACs that had been exposed to HDME induced angiogenesis and Th2 inflammation with remodeling similar to that induced by allergen challenge. Our findings identify that lung endothelium and PACs in the airway sense allergen and elicit an angiogenic response that is central to the innate nonimmune origins of Th2 inflammation.

Authors

Kewal Asosingh, Kelly Weiss, Kimberly Queisser, Nicholas Wanner, Mei Yin, Mark Aronica, Serpil Erzurum

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Figure 2

Expression of PAR-2 by lung endothelial cells and production of Th2-promoting cytokines.

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Expression of PAR-2 by lung endothelial cells and production of Th2-prom...
(A) Lungs were harvested from naive mice and digested into a single-cell suspension for flow cytometric analysis. Gating strategy for endothelial cells is shown. Endothelial cells were further subgrouped into lymphatic endothelial cells and blood vessel endothelial cells and analyzed for PAR-2 expression. Gray histograms represent samples stained for the full panel without PAR-2 primary antibody. (B and C) Lung endothelial cells isolated from naive mice were incubated with or without HDME for 5 days, and GM-CSF and IL-1α were analyzed in the supernatant. Mean ± SE values of 5 mice are shown. Two-tailed Student’s t test was used.

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