Effect of ambient air quality on exacerbation of COPD in patients and its potential mechanism.

Background: Chronic obstructive pulmonary disease (COPD) is a disease of continuous progress and environmental factors may affect the progress. COPD patients' activity tolerance and quality of life are associated with air quality. COPD exacerbation from the perspective of geographical air quality has not been reported.
Objectives: To explore environmental effect of two different geographical places on COPD exacerbation and the effect of cigarette smoke extract and carbon particles on bronchial epithelial cell viability.
Methods: Total 139 COPD patients, who lived in Beijing during summer and temporarily migrated to Sanya city in winter, have been enrolled. Respiratory symptoms and lung function data were collected when they were living in Beijing or Sanya, respectively. Effect of cigarette smoke extract plus ultrafine carbon particles on airway epithelial cells were studied. Measurements and main results: Air pollution as measured by air quality index (AQI) in Beijing summer (113.1±14.2) was significantly worse than that in Sanya winter (49.4±8.9, p<0.001). The COPD Assessment Test (CAT) score was significantly higher in Beijing (26.4±7.1) than that in Sanya (20.0±8.0, p=0.019). Modified Medical Research Council dyspnea scale was also significantly higher in Beijing (2.9±0.9) than that in Sanya (1.9±0.8, p<0.001). FEV1 was significantly improved when the patients were in Sanya (48.88±24.78%) compared to that in Beijing (41.79±20.06%, p<0.01). Compared with Beijing and Sanya, the relative risk (RR) of hospitalization and acute exacerbation were 1.64 and 3.36, respectively. In vitro study demonstrated that apoptosis of BEAS2B cells in response to cigarette smoke extract plus ultrafine carbon particles (25.50±2.10%) was significantly higher than that of control culture (2.30±1.05%, p<0.01).
Conclusion: These findings suggested that ambient air pollution cause COPD exacerbation, and that air pollutants particle matters induce apoptosis of airway epithelial cells.

Introduction

With rapid industrialization and economic growth over the last decade, air pollution has become a serious issue in China. Especially, Beijing has been one of the several cities with deteriorating air quality. It this regard, in the last decade, Beijing experienced multiple prolonged periods of severe smog with extremely high ambient PM2.5 (Particles having a diameter of less than or equal to 2.5 μm) concentration.1 In contrast, Sanya city, a city in Hainan Island, China, has been a city with top quality air in China. Therefore, Sanya city becomes a preferred place to live for senior Chinese citizens and patients with respiratory diseases during the winter season.

The adverse health effects of air pollution have been reported in many epidemiological studies.2–4 Approximately, 3.1 million deaths were associated with ambient particulate matter pollution worldwide in 2010.5 Toxicological studies indicated that air pollution, especially, the exposure of particle matters with diameter 2.5 µm or less (PM2.5) can cause lung inflammation and suppression of pulmonary immune function.6 Studies have also demonstrated the association of air pollution and respiratory disease1,7 or exacerbation of COPD and asthma.8,9 However, to our knowledge, no study has reported on the association of ambient air pollution and COPD exacerbation in the patients who lived in a city with heavy air pollution and temporarily migrated to another city with top quality air in China. The current study was, therefore, designed to explore the association of ambient air quality and COPD exacerbation by investigating respiratory symptoms and lung functions in COPD patients who lived in Beijing during summer and temporarily migrated to Sanya during winter season, a subtropical city, in Hainan Island, China. Furthermore, potential mechanism of air pollutants effect on COPD exacerbation was investigated by exposing an airway epithelial cell line BEAS2B cells to cigarette smoke and ultrafine carbon particles.

Materials and methods

Environmental data collection from Sanya and Beijing

Daily data of ambient air quality of Beijing and Sanya were obtained from the following website: http://www.pm25.in/beijing and http://www.pm25.in/sanya. Daily temperature and humidity in Beijing and Sanya were obtained from the following website: http://www.cma.gov.cn.

Patient enrollment

Patients who were at the GOLD (2014) II~IV of chronic obstructive pulmonary disease (COPD) were selected to be potential subjects for the current study. After obtaining consent forms, a total of 139 COPD patients, who lived in Beijing from April through September (late spring to early fall) and temporary lived in Sanya from October through March (late fall to early spring) every year for the last 3 years or longer, were finally enrolled into the current study. Among the 139 patients with COPD, the proportion of moderate, severe and extremely severe COPD patients was 21% (29), 39% (54) and 40% (56), respectively. The patients’ treatment used was constantly same in both places. The study protocol was approved by the Ethic Committee of The General Hospital of People’s Liberation Army, China (#S2014-099).

Inclusion criteria: patients with <80% predicted FEV1, and <70% of FEV1/FVC, at stable phase of COPD, and willing to sign the consent form.

Exclusion criteria: patients at exacerbation of COPD, or with comorbidity of asthma, tuberculosis, diffuse pan-bronchiolitis; patients who could not perform 6 mins walking test; patients with multi-organ dysfunction.

Patients who were enrolled into this study regularly visited The Hainan Branch of The PLA General Hospital or Sanya People’s Hospital for free lung function examination.

This study was conducted in accordance with the Declaration of Helsinki. We have no deidentified participant data to share.

Clinical evaluation and pulmonary function test

Patients’ symptoms and breathless severity were acquired by filling the publically available “COPD Assessment Test (CAT)” scorecard and “Modified Medical Research Council (MMRC)” dyspnea scale card. An exacerbation of COPD was defined as an acute event characterized by a worsening of the patient’s respiratory symptoms (baseline dyspnea, cough and/or sputum production) that was beyond normal day-to-day variations and leads to a change in medication.

Pulmonary function test (PFT) was performed by certified PFT technician using Master Screen PFT (Jaeger, Germany).

In vitro effect of cigarette smoke extract and carbon particles on bronchial epithelial cells

Cell culture: BEAS2B cells were purchased from ATCC, https://www.atcc.org/search#q=beas-2b&sort=relevancy. Cells were cultured with LHC-9 medium supplemented with 1% fetal calf serum (FCS), penicillin/streptomycin and fungizon (Life Technology, Shanghai, China).

Cigarette smoke extract (CSE) preparation: CSE was prepared with a modification of the method of Carp and Janoff.10 Briefly, one 100-mm research grade cigarette without filter (University of Kentucky, USA) was combusted through 15 mL distilled water a Variable Speed Pump (Fisher Scientific, Pittsburgh, USA). The resulting suspension was filtered through a 0.22-µm pore filter (Lida Manufacturing Corp., Kenosha, WI, USA). This solution was considered to be 100% CSE and diluted with LHC-9 medium as desired.

Cell treatment: Cells were treated with either 10% CSE or 5 µg/mL ultra fine carbon particles (UFCP), or both in the LHC-9 medium. Cells cultured in LHC-9-medium-only were served as control.

TUNEL assay: TUNEL assay was performed using the fluorescence-labeled TUNEL assay kit (Roche Molecular Biochemicals, USA). Briefly, BEAS2B cells were cultured in collagen-coated 8-chamber slides till confluence. Cells were fixed with formalin and permeabilized with 0.1% Tritone X-100 (in 0.1% sodium citrate) for 2 mins on ice and rinsed with PBS. The cells were then reacted with the TUNEL mixture at 37°C for 60 mins. After washing, cells were counter stained with 1 µg/mL DAPI for 5 mins. The fluorescence incorporation into nucleotide was detected and photographed under fluorescence microscopy. TUNEL positive cells vs total cell number was counted.

Immunoblotting: After exposure to desired reagents, BEAS2B cells were lysed with lysing buffer (Thermo Fisher China, Shanghai, China). After brief sonication, the cell lysate was centrifuged at 12,000 g for 10 mins at 4°C. Protein concentrations in the supernatant were determined by a protein-binding assay (Thermo Fisher China, Shanghai, China). After heating at 95°C for 5 mins and rapid cooling on ice, 10 µg of total protein was mixed with 2 x sample loading buffer and loaded into each well of Mini-protein 3 Cell System (Bio-Rad, Life Science, Beijing, China). After electrophoresis, the proteins were transferred to PVDF membrane with the semi-dry electrophoretic transfer system (Bio-Rad, Life Science, Beijing, China). The membrane was blocked with 5% nonfat milk in PBS-tween at room temperature for 1 hr and then exposed to primary antibodies at 4°C overnight. Target proteins were subsequently detected using horseradish peroxidase-conjugated 2nd antibody and with an enhanced chemiluminescence detection system.

ELISA: Quantification of the cytokines (IL-1ß, IL-6, IL-8, TNF-α and TGF-ß1) and matrix metalloproteinases (MMP-1 and MMP-9) were performed using ELISA Duoset and following the manufacturer's instruction (R&D Systems China, Shanghai, China).

Statistical analysis

Each experiment was repeated at least three times. All quantitative data were expressed as mean ± SD. Comparison of paired data was performed using the Student t-test, whereas multi-group data were analyzed by ANOVA followed by Tukey correction using PRISM 6 software. P<0.05 was considered significant.

Results

Total of 139 COPD patients were enrolled into the current study. Of them, 48 were male and 91 were female, with average age of 71.39±10.07 years old. These patients lived in Beijing for most of their life and temporarily migrated to Sanya City, Hainan Island, during the winter season at least for 3 consecutive years. As shown in Figure 1, during winter season in Sanya city, temperature was above 20°C with average of 23.1±4.2°C, which was similar to that of summer weather in Beijing (24.3±6.7, p=0.674, Figure 1A). Humidity, however, was higher in Sanya winter (90.6±4.9%) than that in Beijing summer (58.0±10.0%, p=0.001, Figure 1B). In contrast, air pollution as measured by air quality index (AQI) in Beijing summer (113.1±14.2) was significantly worse than that in Sanya winter (49.4±8.9, p<0.001, Figure 1C).

Figure 1

Comparison of temperature, humidity and ambient air quality between Beijing and Sanya. Monthly average temperature, humidity and air quality data were obtained from the Meteorological Department of Beijing City and Sanya City. (A) Monthly average of temperature. (B) Monthly average of humidity. (C) Monthly average of air quality in Beijing and Sanya.

Patients visited Sanya Hospital, Affiliated to The General Hospital of PLA when they were living in Sanya during the winter season, and visited The General Hospital of PLA in Beijing when they returned to Beijing during the summer season. As shown in Figure 2, the comparison of COPD Assessment Test (CAT) score for the same patients in two different cities indicated that CAT score was significantly higher in Beijing (26.4±7.1) than that in Sanya (20.0±8.0, p=0.019, Figure 2B). Similarly, Modified Medical Research Council (MMRC) dyspnea scale was also significantly higher in Beijing (2.9±0.9) compared to that in Sanya (1.9±0.8, p<0.001, Figure 3).

Figure 2

Comparison of COPD Assessment Test (CAT) score in patients when they were in Beijing or Sanya. (A) CAT score of common symptoms. (B) Average CAT score of the patients in Beijing or Sanya.

Figure 3

Comparison of Modified Medical Research Council (MMRC) dyspnea scale.

Of the 139 COPD patients, 89 patients completed pulmonary function test (PFT) in both places. It was found that forced expiratory volume in 1 second (FEV1) for same patients was significantly improved when the patients were in Sanya (48.88±24.78%) compared to that in Beijing (41.79±20.06%, p<0.01, Figure 4A). Similarly, other PFT parameters including forced vital capacity (FVC), maximum expiratory flow (MEF) and 50% vital capacity maximal expiratory flow (MEF50) or 25% vital capacity maximal expiratory flow (MEF25) were also significantly improved when the patients were in Sanya in comparison to that in Beijing (Figure 4B–E). Consistent with the findings of lung function status, COPD acute exacerbation rate and hospitalization rate were significantly higher in the patients when they were living in Beijing (188.49% acute exacerbation rate and 51.80% hospitalization rate) compared to that of living in Sanya (56.12% and 31.65%, respectively, Table 1). When the patients returned to Beijing from Sanya, the relative risk of the hospital admission was 1.64; and the relative risk of acute exacerbation was 3.36 (Table 1).

Figure 4

Comparison of pulmonary function test. Patients’ pulmonary function was tested when they were in Beijing or Sanya. (A) FVE1 or FEV1/FVC. (B) FVC. (C) MEF75. (D) MEF50. (E) MEF25. Abbreviations: MEF, maximum expiratory flow; L, liter.

Table 1

Relative risk (RR) of hospitalization and acute exacerbation

	Beijing(N=139)	Sanya(N=139)
Hospitalization times (%)	72 (51.80)	44 (31.65)
Acute exacerbation times (%)	262 (188.49)	78 (56.12)

Notes: RR of hospitalization =51.80/31.65=1.64. RR of acute exacerbation =188.49/56.12=3.36.

In order to explore potential mechanisms of air pollutants on COPD exacerbation, in vitro cell culture model was utilized to investigate the effect of particle matters and cigarette smoke on bronchial epithelial cells. As shown in Figure 5, either 10% cigarette smoke extract (CSE) or 5 µg/mL UFCP induced apoptosis in BEASE2 cells as evidenced by positive TUNEL staining (Figure 5A), which was statistically significant (Figure 5B, 10.42±1.42% of CSE alone, and 15.42±1.21% of UFCP alone versus 2.30±1.05% of control, p<0.05). CSE plus UFCP further resulted in higher rate of positive TUNEL staining (Figure 5B, 25.50±2.10%, p<0.01 compared to control). Consistent with the findings of TUNEL staining, 10% CSE and 5 µg/mL UFCP significantly stimulated caspase-3 expression, but did not affect caspase-9 level (Figure 6A–C). Furthermore, CSE and UFCP significantly inhibited Bcl-2 protein expression (Figure 6A and D).

Figure 5

Effect of CSE and UFCP on BEAS2B cell viability. BEAS2B cells were exposed to 10% cigarette smoke extract (CSE) and/or ultrafine carbon particles (UFCP) for 24 hrs. TUNEL assay was performed as described in the methods. (A) Representative image of TUNEL staining. Green: TUNEL positive staining; Blue: nuclei. (B) Quantitative graph of TUNEL positivity. Horizontal axis: treatment of the cells; vertical axis: TUNEL positivity in 5 high power field. *p<0.05.

Figure 6

Immunoblotting of caspase-3, caspase-9 and Bcl-2. BEAS2B cells were exposed to 10% cigarette smoke extract (CSE) and/or ultrafine carbon particle (UFCP) for 24 hrs. Cells were harvested with cell lysis buffer and subjected for immunoblotting as described in the methods. (A) Representative image of the immunoblotting. (B) Semi-quantification of caspase-3. *p<0.05 compared to control. (C) Semi-quantification of caspase-9. (D) Semi-quantification of Bcl-2. *p<0.05.

In addition to apoptosis induction, cigarette smoke and particle matters stimulated IL-1ß production by the BEAS2B cells (34.1±2.5 pg/mL of CSE and 30.7±2.2 pg/mL of UFCP versus 16.6±3.0 pg/mL of control, p<0.05, Figure 7A). Furthermore, CSE plus ultrafine carbon black particle could further stimulate IL-1ß production (55.9±4.0 pg/mL, p<0.01 compared to CSE or UFCP alone, Figure 7A). While neither CSE nor UFCP alone had significant effect on IL-6 (102.1±9.7 pg/mL of CSE and 120.3±13.0 pg/mL of UFCP versus 80.1±9.1 pg/mL of control, p>0.05, Figure 7B) or IL-8 (220.4±78.3 pg/mL of CSE and 314.9±24.2 pg/mL of UFCP versus 152.7±13.3 pg/mL of control, p>0.05, Figure 7C) production, CSE plus UFCP significantly stimulated IL-6 (176.4±7.2 pg/mL, p<0.05, Figure 7B) or IL-8 production (363.3±66.9 pg/mL, Figure 7C). In contrast, total TGF-ß1 production was significantly inhibited in the presence of CSE (902.0±68.0 pg/mL) or UFCP (934.4±3.9 pg/mL versus 1296.0±61.0 pg/mL of control, p<0.05, Figure 7D), and the suppression was further augmented in the presence of CSE plus UFCP (436.7±13.9 pg/mL, p<0.01, Figure 7D). In addition, neither CSE nor UFCP had significant effect on TNF-α, MMP-1 or MMP-9 production by the cells (data not shown).

Figure 7

Effect of CSE and UFCP on production of inflammatory cytokines and growth factors. BEAS2B cells were treated with 10% cigarette smoke extract (CSE) and/or ultrafine carbon particle (UFCP) for 24 hrs. Medium was harvested and used for quantification of cytokines and growth factors as described in the methods. (A) IL-1ß; (B) IL-6; (C) IL-8; (D) TGF-ß1. Vertical axis: concentration of cytokines or growth factor (pg/mL); horizontal axis: treatment of the cells. *p<0.05; **p<0.01.

Discussion

The current study longitudinally compared COPD patients’ symptoms and lung functions when they were living in two different cities, where ambient air quality and relative humidity were significantly different. We found that COPD patients’ symptoms were reduced, lung function was improved and exacerbation rate and hospitalization rate were significantly decreased when the patients temporarily migrated to Sanya city, a city with best air quality and higher relative humidity in China, compared with that in Beijing, the Capital city with heavy air pollution and relatively dry city. We further demonstrated that BEAS2B cells underwent significant apoptosis in response to UFCP and CSE, and that Bcl-2 was significantly decreased while caspase-3 was significantly increased in response to UFCP and CSE. CSE and/or UFCP also stimulated synthesis of inflammatory cytokines (IL-1ß, IL-6 and IL-8), but significantly inhibited TGF-ß1 synthesis by the BEAS2B cells. These findings suggested that ambient air quality be associated with COPD exacerbation, and that PM2.5 and cigarette smoke cause airway cellular injury through inducing airway epithelial cell apoptosis as well as stimulating airway inflammation.

During the last decade, Beijing has experienced heavy air pollution, especially in winter and early spring, because of the coal burning and wind-blown dust from the surrounding industrial cities as well as the vehicle exhaust from exponential growing number of automobiles.11 In this regard, it has been reported that the peak hourly concentration of ambient PM2.5 in Beijing was up to 800 μg/m3, and the average ambient PM2.5 concentration in 2013 reached 89.5 μg/m3.1 The deteriorating air quality and its harmful effect to the public health have been extensively attracted not only scientists, but also patients, especially patients with respiratory diseases such as COPD and asthma. In contrast to Beijing, air quality in Sanya, a city located in the South of Hainan Island, has been kept in high quality in China in the last decade. Consequently, senior residents and patients with COPD or asthma from Beijing temporarily migrated to Sanya city during the winter and early spring and back to Beijing during summer and early fall months.

In the current study, therefore, symptoms and lung function of the COPD patients from Beijing were compared with that of the same patients when they temporarily migrated to Sanya. We found that Sanya city air quality and relative humidity from October through March was significantly better and higher compared with that of Beijing from April through September. Consistent with air quality and relatively high humidity, COPD symptoms were significantly relieved when the patients, who lived in Beijing for their whole life, temporarily migrated to Sanya during the winter season as evidenced by improved CAT score and MMRC dyspnea scale suggesting COPD patients’ exacerbation be associated with ambient air quality and relative humidity.

Consistent with our findings, previous studies have reported that PM2.5 level was significantly associated with respiratory morbidity in Beijing.12,13 It has also reported that every 10 μg/m3 increase in PM2.5 concentration was associated with an increase of 1.46% (95% CI: 0.13–2.79%) emergency room visit for acute exacerbation of COPD. In clinical practice, worsening of the respiratory symptoms, especially dyspnea and sputum, is the best definition of COPD exacerbations.14 In the current study, therefore, we collected records of respiratory symptoms and lung function tests in Sanya and in Beijing for the same patients and found that ambient air pollution (including particle matters) were associated with increased occurrence of respiratory symptoms in the COPD patients when they were living in Beijing, suggesting that ambient air pollution may induce adverse symptoms in COPD.

COPD patients often have emergency hospital admissions due to the exacerbation, which significantly affect patient’s quality of life and even could increase COPD patients’ mortality. COPD exacerbation may be associated with many risk factors. In this content, the effect of environmental exposure on COPD exacerbations has been previously reported.15,16 However, to our knowledge, longitudinal study on the association of air pollution and COPD exacerbation in same COPD patients living in different geographic locations with significantly different air quality has not been reported. Here, we report that COPD exacerbation rate and hospitalization rate were significantly reduced when the COPD patients were temporarily living in Sanya, a city with better air quality, compared with that when the patients were living in Beijing. In addition, we also noticed that dry air in Beijing might also contribute to the exacerbation of COPD in that relative humidity was year-around high in Sanya, where patients had significantly lower rate of COPD exacerbation.

The mechanisms that air pollution leads to pulmonary illnesses are so far poorly understood. Studies have shown that inflammatory mediators and reaction oxidative species (ROS) may be involved in mediating air-pollution-induced respiratory diseases.17,18 Consistently, we found that cigarette smoke extract and/or ultrafine carbon particles significantly stimulated release of pro-inflammatory cytokines, including IL-1ß, IL-6 and IL-8, by the airway epithelial cells. In contrast, TGF-ß1 production was significantly inhibited by cigarette smoke and/or ultrafine carbon particles, suggesting particular matters not only induce airway inflammation, but also may suppress airway tissue repair through inhibiting synthesis of growth factors.

Previous studies have also shown that both cigarette smoke extract and ultrafine carbon black caused airway epithelial cells and lung fibroblasts DNA damage and apoptosis.19,20 Therefore, the current study further investigated potential adverse effect of cigarette smoke plus ultrafine carbon particles on human airway epithelial cell viability. Consistent with previous report,19,20 we found that either cigarette smoke or ultrafine carbon particle could induce BEAS2B cell apoptosis. We further demonstrated that cigarette smoke plus ultrafine carbon particle dramatically increased the number of apoptosis compared to that of either reagent alone, suggesting cigarette smoke plus air pollution will further cause airway cellular damage.

There were limitations in the current study. First, number of the patients enrolled into this study was limited. Second, components of the air pollutants that contribute to the exacerbation of COPD were not identified. Third, PM2.5 or PM10 isolated from air pollutant was not available and thus, ultrafine carbon particle was used to investigate PM2.5 effect. Finally, signal transduction pathways that mediate cigarette smoke and ultrafine carbon particle-induce epithelial cell apoptosis was not identified in this study. Therefore, further studies remain to be conducted.

Taken together, the current study explored the effect of air quality in two different geographic cities on the same COPD patients’ symptoms, lung function and COPD exacerbation. We found that COPD symptoms were relieved, lung function was improved and COPD exacerbation was reduced when the COPD patients temporarily migrated from Beijing, the Capital city of China with deteriorating air quality, to Sanya city, a city with top quality ambient air in China. We proposed that ambient air quality and relative humidity are associated with the COPD exacerbation. Mechanisms of air pollutant-induced COPD exacerbation might be due to its effect on airway epithelial cell apoptosis and inflammatory injury.