Interleukin‐18, IL‐18 binding protein and IL‐18 receptor expression in asthma: a hypothesis showing IL‐18 promotes epithelial cell differentiation

Davinder Kaur; Latifa Chachi; Edith Gomez; Nicolas Sylvius; Christopher E Brightling

doi:10.1002/cti2.1301

Clinical & Translational Immunology (Jan 2021)

Interleukin‐18, IL‐18 binding protein and IL‐18 receptor expression in asthma: a hypothesis showing IL‐18 promotes epithelial cell differentiation

Davinder Kaur,
Latifa Chachi,
Edith Gomez,
Nicolas Sylvius,
Christopher E Brightling

Affiliations

Davinder Kaur: Department of Respiratory Sciences Institute for Lung Health NIHR Biomedical Research Centre University of Leicester LeicesterLE1 7RHUK
Latifa Chachi: Department of Respiratory Sciences Institute for Lung Health NIHR Biomedical Research Centre University of Leicester LeicesterLE1 7RHUK
Edith Gomez: Department of Respiratory Sciences Institute for Lung Health NIHR Biomedical Research Centre University of Leicester LeicesterLE1 7RHUK
Nicolas Sylvius: Genomic Core Facility Department of Genetics University of Leicester Adrian Building, University Road, G23 LeicesterLE1 7RHUK
Christopher E Brightling: Department of Respiratory Sciences Institute for Lung Health NIHR Biomedical Research Centre University of Leicester LeicesterLE1 7RHUK

DOI: https://doi.org/10.1002/cti2.1301
Journal volume & issue: Vol. 10, no. 6
pp. n/a – n/a

Abstract

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Abstract Objective In asthma, genome‐wide association studies have shown that interleukin‐18 (IL‐18) receptor 1 gene (IL‐18R1) and sputum IL‐18 are increased during exacerbations. However, the role of the IL‐18 axis in bronchial epithelial function is unclear. To investigate IL‐18, IL‐18 binding protein (BP) and IL‐18R expression in bronchial biopsies and sputum samples from patients with asthma, and to determine its functional role using in vitro bronchial epithelial cells. Methods The expression of IL‐18, IL‐18BP and IL‐18Rα was examined in subjects with asthma and healthy controls in bronchial biopsies by immunohistochemistry and IL‐18 and IL‐18BP release in sputum. In epithelial cells, the mRNA and protein expression of IL‐18, IL‐18BP, IL‐18Rα and IL‐18Rβ was assessed by qPCR, flow cytometry, Western blotting and immunofluorescence respectively. IL‐18 function in epithelial cells was examined by intracellular calcium, wound repair, synthetic activation and epithelial differentiation changes. Results In biopsies from subjects with asthma, the IL‐18 expression was not different in the lamina propria compared with controls but was decreased in the epithelium. In contrast, the IL‐18BP was decreased in the lamina propria in asthma and was absent in the bronchial epithelium. IL‐18 was released in sputum with IL‐18BP elevated in patients with asthma. The IL‐18Rα expression was not different between health and disease. In vitro, IL‐18‐stimulated bronchial epithelial cells increased intracellular calcium, wound repair, metabolic activity, morphological changes and epithelial cellular differentiation. Conclusion In asthma, the dynamic interaction between IL‐18, its cognate receptor and natural inhibitor is complex, with differences between airway compartments. Upregulation of IL‐18 can promote epithelial activation and cellular differentiation.

Published in Clinical & Translational Immunology

ISSN: 2050-0068 (Online)
Publisher: Wiley
Country of publisher: Australia
LCC subjects: Medicine: Internal medicine: Specialties of internal medicine: Immunologic diseases. Allergy
Website: https://onlinelibrary.wiley.com/journal/20500068

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