HMGB1 enhances epithelial permeability via p63/TGF-β signaling in lung and terminal bronchial epithelial cells

High mobility group box 1 (HMGB1) is involved in the induction of airway inflammation and injury in patients with chronic obstructive pulmonary disease (COPD) and idiopathic pulmonary fibrosis (IPF). HMGB1 increased by transforming growth factor-β1 (TGF-β1), impairs airway epithelial barrier functio...

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Published in:Tissue barriers 2020-10, Vol.8 (4), p.1805997
Main Authors: Kodera, Yuki, Kohno, Takayuki, Konno, Takumi, Arai, Wataru, Tsujiwaki, Mitsuhiro, Shindo, Yuma, Chiba, Hirofumi, Miyakawa, Maki, Tanaka, Hiroki, Sakuma, Yuji, Watanabe, Atsushi, Takahashi, Hiroki, Kojima, Takashi
Format: Article
Language:English
Subjects:
2.5D Matrigel cultures
Bronchioles - metabolism
Epithelial Cells - metabolism
epithelial permeability
Epithelium - metabolism
EW-7197
HMGB1
HMGB1 Protein - metabolism
Humans
Membrane Proteins - metabolism
normal human lung epithelial cells
Research Paper
Signal Transduction
TGF-Β
tight junctions
TNFα-antibody
Transforming Growth Factor beta1 - metabolism
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Summary:High mobility group box 1 (HMGB1) is involved in the induction of airway inflammation and injury in patients with chronic obstructive pulmonary disease (COPD) and idiopathic pulmonary fibrosis (IPF). HMGB1 increased by transforming growth factor-β1 (TGF-β1), impairs airway epithelial barrier function in the lung. In the present study, to investigate how HMGB1 affects the barrier of normal human lung epithelial (HLE) cells, monolayer cells (2D culture) and bronchial-like spheroid cells (2.5 D Matrigel culture), which have lumen formation, were pretreated with TGF-β type I receptor kinase inhibitor EW-7197 before treatment with HMGB1. In 2D culture, treatment with HMGB1 decreased expression of angulin-1/LSR, TRIC and CLDN-1, −4, −7 and increased that of CLDN-2. Pretreatment with EW-7197 prevented the changes of all tight junction molecules induced by HMGB1. In 2.5D Matrigel culture, treatment with HMGB1 induced permeability of FITC-dextran (FD-4) into the lumen, whereas pretreatment with EW-7197 prevented the hyperpermeability of FD-4 into the lumen caused by HMGB1. In 2.5D Matrigel culture, knockdown of transcription factor p63 prevented the hyperpermeability induced by HMGB1 as well as pretreatment with EW-7197. In the 2D culture of HLE cells with HMGB1, knockdown of p63 increased the level of angulin-1/LSR and CLDN-4, while pretreatment with EW-7197 enhanced the increase of CLDN-4 induced by knockdown of p63. Immunohistochemical analysis of IPF, CLDN-2, HMGB1 and p63 revealed that their levels were higher in the regenerative epithelium of the terminal bronchial region than in normal epithelium. HMGB1 induces epithelial permeability of HLE cells via p63/TGF-β signaling in normal lung and IPF.
ISSN:2168-8370
2168-8362
2168-8370
DOI:10.1080/21688370.2020.1805997