Different Munc18 proteins mediate baseline and stimulated airway mucin secretion
Ana M. Jaramillo, … , Michael J. Tuvim, Burton F. Dickey
Ana M. Jaramillo, … , Michael J. Tuvim, Burton F. Dickey
Published February 5, 2019
Citation Information: JCI Insight. 2019;4(6):e124815. https://doi.org/10.1172/jci.insight.124815.
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Research Article Cell biology Pulmonology

Different Munc18 proteins mediate baseline and stimulated airway mucin secretion

Abstract

Airway mucin secretion is necessary for ciliary clearance of inhaled particles and pathogens but can be detrimental in pathologies such as asthma and cystic fibrosis. Exocytosis in mammals requires a Munc18 scaffolding protein, and airway secretory cells express all 3 Munc18 isoforms. Using conditional airway epithelial cell–deletant mice, we found that Munc18a has the major role in baseline mucin secretion, Munc18b has the major role in stimulated mucin secretion, and Munc18c does not function in mucin secretion. In an allergic asthma model, Munc18b deletion reduced airway mucus occlusion and airflow resistance. In a cystic fibrosis model, Munc18b deletion reduced airway mucus occlusion and emphysema. Munc18b deficiency in the airway epithelium did not result in any abnormalities of lung structure, particle clearance, inflammation, or bacterial infection. Our results show that regulated secretion in a polarized epithelial cell may involve more than one exocytic machine at the apical plasma membrane and that the protective roles of mucin secretion can be preserved while therapeutically targeting its pathologic roles.

Authors

Ana M. Jaramillo, Lucia Piccotti, Walter V. Velasco, Anna Sofia Huerta Delgado, Zoulikha Azzegagh, Felicity Chung, Usman Nazeer, Junaid Farooq, Josh Brenner, Jan Parker-Thornburg, Brenton L. Scott, Christopher M. Evans, Roberto Adachi, Alan R. Burns, Silvia M. Kreda, Michael J. Tuvim, Burton F. Dickey

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Figure 5

Airway mucus occlusion and airway hyperreactivity of Munc18b–conditional deletant mice in an allergic asthma model.

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Airway mucus occlusion and airway hyperreactivity of Munc18b–conditional...
(A) Representative cross-sections of airways fixed with methacarn to preserve mucus volume and stained with PAFS. Mice were treated with IL-13 to induce mucin production and then stimulated with aerosolized 150 mM methacholine (Mch) to stimulate mucin secretion and smooth muscle contraction. Scale bar: 50 μm. (B) Cross-sectional area of lumenal mucus in the right caudal lobe measured at 1,000-μm intervals (n = 5–9 mice per group, representative experiment, >100 airways per group quantified). 18bΔ/Δ versus 18bF/F, P = 0.0002; Muc5ac–/– versus 18bF/F, P = 0.0378, Student’s 2-tailed t test. (C) Total respiratory system resistance (Rrs) at increasing doses of nebulized Mch in mice treated with or without IL-13 (n = 6–14 per group, 3 independent experiments combined). Line represents mean; error bar, SEM. (D) Fold-change in Rrs at the highest dose of nebulized Mch (30 mg/ml) from C. Each genotype is normalized to its own baseline measured with nebulized saline. 18bΔ/Δ versus 18bF/F, P = 0.0018; Muc5ac–/– versus 18bF/F, P = 0.0044, Student’s 2-tailed t test. *P < 0.05 versus floxed littermate. Bar, mean; error bar, SEM.