Der p 1 facilitates transepithelial allergen delivery by disruption of tight junctions
Hong Wan, … , Mark B. Cannell, Clive Robinson
Hong Wan, … , Mark B. Cannell, Clive Robinson
Published July 1, 1999
Citation Information: J Clin Invest. 1999;104(1):123-133. https://doi.org/10.1172/JCI5844.
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Article

Der p 1 facilitates transepithelial allergen delivery by disruption of tight junctions

Abstract

House dust mite (HDM) allergens are important factors in the increasing prevalence of asthma. The lung epithelium forms a barrier that allergens must cross before they can cause sensitization. However, the mechanisms involved are unknown. Here we show that the cysteine proteinase allergen Der p 1 from fecal pellets of the HDM Dermatophagoides pteronyssinus causes disruption of intercellular tight junctions (TJs), which are the principal components of the epithelial paracellular permeability barrier. In confluent airway epithelial cells, Der p 1 led to cleavage of the TJ adhesion protein occludin. Cleavage was attenuated by antipain, but not by inhibitors of serine, aspartic, or matrix metalloproteinases. Putative Der p 1 cleavage sites were found in peptides from an extracellular domain of occludin and in the TJ adhesion protein claudin-1. TJ breakdown nonspecifically increased epithelial permeability, allowing Der p 1 to cross the epithelial barrier. Thus, transepithelial movement of Der p 1 to dendritic antigen-presenting cells via the paracellular pathway may be promoted by the allergen’s own proteolytic activity. These results suggest that opening of TJs by environmental proteinases may be the initial step in the development of asthma to a variety of allergens.

Authors

Hong Wan, Helen L. Winton, Christian Soeller, Euan R. Tovey, Dieter C. Gruenert, Philip J. Thompson, Geoffrey A. Stewart, Graham W. Taylor, David R. Garrod, Mark B. Cannell, Clive Robinson

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Figure 5

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Effects of purified Der p 1 on intercellular junctions of 16HBE14o– cell...
Effects of purified Der p 1 on intercellular junctions of 16HBE14o cells. (a) Sample through-focus images (3.2-μm thick) of occludin and desmoplakin staining in control and after exposure of the apical surface to Der p 1 for the periods indicated. The effects are similar to that seen in Figure 2a. (b) Isosurface-rendered images of the 3-dimensional distribution of occludin (Occl; green) and desmoplakin (Dp; red) for a part of the image in a. The left panel shows a typical untreated cell, whereas the 2 panels on the right show the heterogeneity of response after 2.5 hours. (c) Graphical analysis of occludin concentration and the number of breaks in continuity of the occludin ring per cell. Bars show mean and + SE of 8 cells (*P < 0.05). The method of measurement was the same as for Figure 2c. (d) Quantification of desmoplakin staining.