PM2.5 downregulates miR-194-3p and accelerates apoptosis in cigarette-inflamed bronchial epithelium by targeting death-associated protein kinase 1

Tianyu Zhou; Yijue Zhong; Yan Hu; Chao Sun; Yunxia Wang; Guangfa Wang

doi:10.2147/COPD.S168629

PM_2.5 downregulates miR-194-3p and accelerates apoptosis in cigarette-inflamed bronchial epithelium by targeting death-associated protein kinase 1

Int J Chron Obstruct Pulmon Dis. 2018 Aug 1:13:2339-2349. doi: 10.2147/COPD.S168629. eCollection 2018.

Authors

Tianyu Zhou¹, Yijue Zhong¹, Yan Hu¹, Chao Sun¹, Yunxia Wang¹, Guangfa Wang¹

Affiliation

¹ Department of Respiratory and Critical Care Medicine, Peking University First Hospital, Beijing, 100034, China, wangguangfa@hotmail.com.

Abstract

Background: Persistent exposure to cigarette smoke or biomass fuels induces oxidative stress and apoptosis in bronchial epithelium, which is one of the most important pathogenic mechanisms of chronic obstructive pulmonary disease (COPD). Fine particulate matter (PM_2.5) is an aggravating risk factor of COPD exacerbation. Animal evidence showed PM_2.5accelerated lung inflammation and oxidative stress in COPD mice, but the mechanism is still not clear. Recently, we found that miR-194-3p is a novel biomarker of both COPD and PM_2.5 exposure, and miR-194 family has been reported to be involved in cell proliferation and apoptosis. Thus, we propose a hypothesis: PM_2.5 can accelerate apoptotic response of airway epithelial cells in COPD and miR-194 is a potential involved regulator.

Materials and methods: Human bronchial epithelial cells (HBEpiCs) were treated with normal media, cigarette smoke solution (CSS) and PM_2.5-CSS for 24 h. miR-194-3p mimics, inhibitors and scrambled controls were non-transfected or pre-transfected into HBEpiCs for 48 h. MircroRNAs and mRNA expression were quantified by qRT-PCR. Protein expression was analyzed by western blotting. Caspase activities, mitochondrial membrane potential and TUNEL-positive cells were detected to analyze apoptosis. Bioinformatics and luciferase analysis were used to identify the predicted binding site of miR-194-3p and potential targets.

Results: In our study, we found that PM_2.5 significantly aggravated apoptosis in cigarette-inflamed HBEpiCs. miR-194-3p was dramatically downregulated in PM_2.5-CSS-treated HBEpiCs. Bioinformatics and luciferase experiments reported that death-associated protein kinase 1 (DAPK1), regulating caspase 3 activities in apoptosis, was directly targeted by miR-194-3p. Inhibition of miR-194-3p increased DAPK1 expression and apoptosis in normal HBEpiCs. Importantly, overexpression of miR-194-3p suppressed apoptosis in PM_2.5-CSS HBEpiCs.

Conclusion: These results suggested that miR-194-3p was a protective regulator involved in apoptosis pathway and a potential therapeutic target for treatment of bronchial epithelial injury aggravation induced by PM_2.5.

Keywords: COPD; PM2.5; apoptosis; bronchial epithelial cells; fine particulate matter; miR-194-3p.

MeSH terms

Apoptosis*
Bronchi / cytology
Caspase 3 / metabolism
Disease Progression
Down-Regulation
Epithelial Cells / metabolism*
Humans
Membrane Proteins / metabolism*
MicroRNAs / antagonists & inhibitors
MicroRNAs / metabolism*
Oxidative Stress
Particulate Matter / toxicity*
Pulmonary Disease, Chronic Obstructive / etiology
Smoke / adverse effects*
Smoking / adverse effects*

Substances

DAPL1 protein, human
MIRN194 microRNA, human
Membrane Proteins
MicroRNAs
Particulate Matter
Smoke
Caspase 3