Abstract
Background
Cigarette smoke (CS) is the main cause in the development of chronic obstructive pulmonary disease (COPD), the pathogenesis of which is related to an extended inflammatory response. In this study, we investigated the effect of low and high doses of gas phase cigarette smoke (GPS) on cultured lymphocyte progenitor cells, using techniques to assess cell viability and to elucidate whether cells die of apoptosis or necrosis upon exposure to different doses of GPS.
Methods
In our approach we utilised a newly-established system of exposure of cells to GPS that is highly controlled, accurately reproducible and simulates CS dosage and kinetics that take place in the smokers' lung. This system was used to study the mode of cell death upon exposure to GPS in conjunction with a range of techniques widely used for cell death studies such as Annexin V staining, activation of caspase -3, cytoplasmic release of cytochrome C, loss of mitochondrial membrane potential and DNA fragmentation.
Results
Low doses of GPS induced specific apoptotic indexes in CCRF-CEM cells. Specifically, cytochrome C release and cleaved caspase-3 were detected by immunofluorescence, upon treatment with 1-3 puffs GPS. At 4 h post-exposure, caspase-3 activation was observed in western blot analysis, showing a decreasing pattern as GPS doses increased. Concomitant with this behaviour, a dose-dependent change in Δψm depolarization was monitored by flow cytometry 2 h post-exposure, while at 4 h Δψm collapse was observed at the higher doses, indicative of a shift to a necrotic demise. A reduction in DNA fragmentation events produced by 5 puffs GPS as compared to those provoked by 3 puffs GPS, also pointed towards a necrotic response at the higher dose of GPS.
Conclusion
Collectively, our results support that at low doses gas phase cigarette smoke induces apoptosis in cultured T-lymphocytes, whereas at high doses GPS leads to necrotic death, by-passing the characteristic stage of caspase-3 activation and, thus, the apoptotic route.
Background
Tobacco smoke contains more than 4000 compounds [1,2] that have been shown to cause carcinogenesis and other serious lung diseases, such as chronic obstructive pulmonary disease (COPD) [3-6]. Cigarette smoke (CS) consists of the gaseous phase (GPS) and the particulate matter (tar) [7]. Although the carcinogenic properties of chemicals in tar are well known [8], more recent studies have emerged demonstrating major cytotoxic effects on pulmonary and immune cells attributed to the gaseous phase [7,9-11]. The effect of these compounds can be both direct on the most critical line of defence of the airway epithelium [7,12,13] and indirect evoking immune responses, which in turn have a deleterious effect on lung structure [13,14]. In the case of COPD, the progressive destruction of pulmonary tissue has been attributed to inflammation, oxidative stress and proteolysis, the underlying death mechanism of which is still a matter under debate. However, several studies have clearly shown that metabolically-activated or direct action genotoxic components and inhibitors of DNA repair in GPS may contribute to DNA damage and to smoking-related diseases of the upper aero-digestive tract [15].
In the past decade, a number of studies were carried out in order to characterise the mode of death of cells challenged with different doses of cigarette smoke [16-19]. Taking this into consideration, there has been increasingly intense interest in the effects of GPS. A common denominator in many of these in vitro studies has been an overwhelming system for CS administration. The practice of cigarette smoke extract or condensate (CSE or CSC) assumes the application of a large quantity of toxic substances on cell cultures, since the toxic load of a whole cigarette is withheld within a relatively small volume of diluents [20-22]. This locally creates a direct and appropriate critical mass of toxic substances, so that the defence mechanisms of the cells are promptly depleted. Such cumulative condition with large quantities of toxic/carcinogenic substances in the cell culture could occur only with exceptional difficulty during normal smoking.
Various studies present conflicting evidence as to whether cells exposed to tobacco smoke die of apoptosis or due to necrosis, or both [16-20,22]. Given that the approach of CSE or CSC administration relates to overdosing cultured cells with CS constituents, then it is not surprising that many of these studies support the idea of necrotic death. Our approach is unique as we employed a method [11,23] for highly controlled and accurately reproducible cell exposure to gas phase CS that closely resembles the dosage and gas kinetics of CS in the smokers' lung, in conjunction with standard techniques to evaluate and quantify the mode of cellular death. In our study, we utilised a well-established lymphoblast cell line to examine CS toxicity in vitro. The lymphocyte cell system has previously been used in cell death research and is now considered a model system for similar studies [24-26]. In our experiments, the use of the CCRF-CEM cell line served an additional purpose: T cells are widely recruited in the sites of lung inflammation attributed to CS [27]; however, their precise function and involvement in lung tissue destruction remain to be elucidated. It is therefore of paramount importance to study the fate of T cells in response to various doses of tobacco smoke in vitro. Our results clearly demonstrate that the effects of CS administration are both dose- and time-dependent and that apoptosis is an active process triggered by tobacco smoke constituents at low toxicity. Necrosis, on the other hand, is a predominant phenomenon in cultures exposed to high toxicity GPS.
Methods
Cell culture
The human T-lymphoblastoid cell line CCRF-CEM (ATCC cat. No. CCL-119) was maintained in RPMI 1640 medium (Biochrom, Berlin, Germany) supplemented with 10% fetal bovine serum (FBS), L-glutamine (2 mM) and penicillin/streptomycin (100 U/ml). Cultures were grown in suspension in a 37°C/5% CO2 humidified incubator. Prior to experiments, cells were counted on a Neubauer Haemocytometer and cell viability was assessed with 0.5% Trypan Blue staining. For experimental purposes, cells were transferred to 6-well or 96-well tissue culture plates (Greiner Bio-One, Austria) at a density of 1 × 106 cells/ml, unless otherwise stated.
Cell exposure to Gas Phase Smoke (GPS)
Kentucky 1R3F research-reference filter cigarettes (The Tobacco Research Institute, University of Kentucky, Lexington, KY) were used throughout this study. Prior to use, cigarettes were conditioned for at least 48 h (up to 6 days), in a controlled environment chamber (Environ-Cab, Lab-Line Instruments Inc., IL, USA) at 22 ± 0.5°C temperature and 60 ± 1% humidity. Smoke was generated with a mechanical smoking machine (SM410, Cerulean, UK) according to ISO rules (2 seconds puff duration, 35 ml puff, bell shape puff profile, 1 minute puff cycle). In order to remove the particulate matter and obtain gas phase smoke (GPS), the cigarette smoke was passed through Cambridge filters rated to withhold 99.9% of all particles > 0.01 μm in diameter.
The second puff of a single 1R3F cigarette was used to generate each puff of GPS. The GPS was pumped directly into a gas-tight volumetric exposure chamber containing the cells in the lid-less multi-well format plates. Following GPS exposure, the cells were returned to the 37°C/5% CO2 incubator for the specified incubation time.
Cytotoxicity Assay
Cytotoxicity was assessed using the LDH assay (Roche Applied Science, Indianapolis, IN, USA), according to the manufacturer's instructions. Briefly, 2 × 104 cells per well were seeded in four flat-bottomed 96-well plates. The cells were treated with the required GPS dose (1, 3 or 5 puffs), whereas a plate was left untreated (control). Five replicates were included for each sample.
All cells were washed in 1% FBS medium and were finally resuspended in 1% FBS medium for assaying purposes. In the control plate, one row of cells was resuspended in 1% Triton buffer (1% Triton-X-100 in 1% FBS medium) and was incubated at 37°C for the maximum time allowed (24 hours) to assay for the maximum amount of LDH released from the cells (high control). Control cells that were assayed for LDH immediately after seeding provided the low control to determine basal levels of LDH release in the cell population. LDH was also assayed for in the 1% FBS medium to correct for LDH background in serum. Experimental samples were assayed at 1, 4 and 24 hours post-exposure to GPS. Like control cells, the treated samples were washed and resuspended in 1% FBS medium prior to assaying.
Following incubation, the supernatants of all samples were collected and spun to rid of cell remnants. The cleared supernatants were mixed 1:1 with the dye/catalyst mix, as per the manufacturer's protocol. The amount of LDH was measured using a TECAN spectrofluorimeter at 430 nm, using a 620 nm reference filter. Percent (%) cytotoxicity was calculated using the average of the 5 replicates and the formula provided by the manufacturer.
Annexin V-Propidium Iodide assay
To determine the percentage of apoptotic cells and differentiate these from necrotic populations, an Annexin V-fluorescein isothiocyanate (FITC)/Propidium Iodide (PI) detection kit (556547, BD Biosciences, UK) was used.
CCRF-CEM cells were exposed to 1, 3 or 5 puffs of GPS and were subsequently incubated for 2 hours. At the end of the incubation period, cells were collected, washed in cold PBS and stained with Annexin V FITC/PI, according to the manufacturer's instructions. Untreated cells were also stained, in order to determine the spontaneous apoptotic index of the cellular population. A 2 μM staurosporine (S4400, Sigma-Aldrich) (STS)-treated cell population, which was also harvested at 2 hours, was included as a positive control for apoptosis. Vehicle control was also included.
The cell suspensions were immediately analyzed using a FACSCalibur flow cytometer (BD Biosciences, UK), equipped with a 488 nm argon laser and the appropriate filter sets. Green fluorescence for FITC was collected using a 530/30 bandpass filter and red fluorescence for PI using a 585/42 bandpass filter. For each sample, ten thousands events were acquired and statistically analysed using CellQuest software version 7.5.3 (BD Biosciences, UK).
FACS analysis of mitochondrial membrane potential
For analysis of the mitochondrial inner membrane potential (Δψm) in whole cells, the membrane-permeable lipophilic cationic fluorochrome JC-1 was utilised (Mitoscreen kit, BD Biosciences, UK). In live cells, JC-1 exhibits potential-dependent accumulation in mitochondria forming J-aggregates. These aggregates can be detected within the red fluorescence spectrum (~590 nm), in contrast to the green fluorescence (~529 nm) emitted by JC-1 monomers. An increase in green fluorescence indicates depolarization of the mitochondrial membrane potential.
Briefly, CCRF-CEM cells, treated with GPS or STS as previously described, were collected by centrifugation (400 g). The cells were resuspended at 1 × 106/ml in pre-warmed JC-1 working buffer containing 2 μM JC-1 and incubated for 15 min in a 37°C/5% CO2 incubator. Subsequently, the cells were washed in assay buffer and directly analyzed in a FACSCalibur flow cytometer using the appropriate filter settings. Red and green populations were gated for quantification analysis using CellQuest software. Ten thousands events were acquired for each sample.
Western Blot Analysis
Whole cell lysates were prepared in RIPA buffer (50 mM Tris-HCl pH 8, 150 mM NaCl, 1 mM EDTA, 1 mM DTT, 0.5% NP-40) on ice, including a mix of protease inhibitors (P8340, Sigma-Aldrich). For cytoplasmic extracts, the lysates were centrifuged at 12,000 g for 15 min, at 4°C. Protein concentration was measured using the Bradford assay (B6916, Sigma-Aldrich) and approximately 40 μg from each sample were boiled in Laemmli buffer (50 mM Tris-HCL pH 6.8, 2% SDS, 1,25% β-MSH, 5% glycerol, 0.0125% bromophenol blue). Proteins were analysed on 11% SDS-PAGE followed by transfer onto nitrocellulose membrane. Active caspase-3 was detected using a commercially available antiserum (1:100; AB3623, Chemicon Millipore-MA, USA) and labelled with a HRP-conjugated secondary antibody (AV132P, Chemicon Millipore). For loading control, a monoclonal anti-a tubulin antiserum (MCA78G, ABD Serotec) was used (1:500) to identify cellular tubulin, together with an anti-rat HRP-conjugate (A9037, Sigma-Aldrich). The blots were developed using Amersham ECL Kit (GE Healthcare, UK).
Confocal microscopy
Control cells or cells exposed to 1, 3 or 5 puffs GPS and harvested at 1, 4 or 24 hours post-exposure were fixed in 4% paraformaldehyde/PBS, pH 6.9. The cells were permeabilised with 0.1% Triton-X-100 and non-specific sites were blocked with 1% BSA in PBS. As CCRF CEM were grown in suspension, prior to staining, cells were attached onto microscope slides using Shandon Cytospin Cytocentrifuge (Thermo Scientific, MA, USA).
Active caspase-3 staining was performed using a commercial antiserum (1:150; 9661; Cell Signaling, USA) and anti-rabbit FITC antibody (1:80; F0382, Sigma-Aldrich). Cytochrome C was identified using a monoclonal antibody (1:150; 13561; Santa Cruz Biotechnology) and anti-mouse Alexa 488 conjugate (1:100; A11029; Molecular Probes). Where necessary, nuclear counterstaining with 1 μg/ml propidium iodide (PI) was included. Apoptosis was induced using 2 μM staurosporine (positive control). Secondary antibody negative controls were also included.
The samples were visualised using a Nikon C1 Digital Eclipse Confocal Microscope system, equipped with a 488 nm Argon and a 543 Helium Neon laser through an oil immersion ×60/1.4 objective.
Detection of DNA fragmentation by flow cytometry
DNA fragmentation was assessed in smoke-treated cells and compared to healthy cells, as well as staurosporine-treated apoptotic cells using the Apo-BrdU Kit (556405, BD Biosciences, UK).
Approximately 2 × 106 cells were collected and briefly fixed in 1% paraformaldehyde/PBS, pH 6.9, followed by overnight fixation in 70% ethanol at -20°C. TdT-catalysed end-labelling of fragmented DNA with bromolated deoxyuridine triphosphates (Br-dUTP) was carried out at 37°C. End-labelled DNA was probed with anti-BrdU monoclonal antiserum provided in the kit. All cells were counterstained with a 5 μg/ml PI/200 μg/ml RNAse A solution.
All samples were analysed using a FACSCalibur cytometer and the appropriate green/red filter settings. Ten thousand events from each sample were analysed.
Statistical analysis
All data presentations (graphs etc.) and corresponding statistical analysis was performed using SigmaPlot and SigmaStat software packages (SPSS Inc.). All data in graphs are expressed as mean values ± SD. For one way ANOVA analysis a P < 0.05 was considered significant.
Results
The results described are representative of three or more independent experiments.
Cytotoxicity measurements
The cytotoxicity of gas phase cigarette smoke (GPS) on cultured lymphocytes was assessed using a kit to measure lactate dehydrogenase (LDH) release from compromised cell membranes (Figure 1). The amount of LDH released from cells exposed to the different doses of GPS (1, 3 or 5 puffs) at 1, 4 or 24 hours post-exposure was directly compared to the amount of enzyme from untreated cells (low control-basal levels of LDH in the cell culture) and cells treated for the lengthiest part of the experiment (24 hours) with 1% Triton-X buffer (1% Triton-X in 1% FBS medium) (high control-maximum LDH release). The mean of measurements for the spontaneous LDH activity in the culture media due to the presence of serum was subtracted from all experimental values.
The measurements taken at 1 hour post-exposure were not significantly different (p ≥ 0.47) among all three GPS doses. The average percentage of cytotoxicity at that exposure time was about 5.8% (± 0.8%). At 4 hours post-exposure, the percentages were markedly different, demonstrating a dose- and time-dependent increase in cytotoxicity. Exposure to 1 puff GPS resulted in cytotoxic death of approximately 7.15 ± 2.42% of the cells. The percentages were more than three-fold (22.76 ± 4.65%) and quadra-fold (32.92 ± 14.77%) higher for cells treated with 3 and 5 puffs GPS, respectively. It has to be noted, that the high standard deviation of the 5-puff data at 4 hours exposure did not allow for a statistically significant differentiation between the 3 and 5 puffs cytotoxicities, as determined by one-way ANOVA analysis (p < 0.22) although both 3 and 5 puff data were significantly different than the data for 1 puff (p < 0.05). At 24 hours post-exposure, LDH release from cells revealed the same cytotoxicity pattern. Cells treated with 1 puff GPS reached 42.46 ± 7.07% cytotoxicity, which was significantly lower than the percentages recorded for the cells treated with either 3 or 5 puffs (90.89 ± 5.98% and 93.49 ± 6.75%, respectively). As with 4 hours post exposure, at 24 hours the percentages of cytotoxicity of the cells treated with the higher doses (3 and 5 puffs) were not significantly different (p < 0.62).
FACS analysis of Annexin V/PI-stained cells
To determine the mode of cell death upon GPS treatment, cells were stained with AnnexinV/PI and analysed by flow cytometry, 2 h post-exposure. As seen in Figure 2, the percentage of the Annexin V-stained populations (early apoptotic cells - lower right quadrants) in the control group and all groups of GPS-treated cells were not significantly different (one-way ANOVA, p < 0.43).
A clear dose-dependent increase of cells stained with both Annexin V and PI (late apoptotic cells - upper right quadrants) was observed (one-way ANOVA, p < 0.001). The percentage of double-stained cells treated with 1 puff was 11.37 ± 1.45% compared to 5.10 ± 0.41% for the untreated cells, representing an almost 2-fold increase. At higher toxicity conditions, there was a steady increase in the AnnexinV/PI-positive cell numbers, with the corresponding population reaching 17.62 ± 0.82% at 3 puffs and 26.66 ± 1.66% at 5 puffs. A similar pattern was observed in the PI-stained cell population (necrotic cells; upper left quadrants) as judged by one way ANOVA (p < 0.0001), with the exception of the 1 puff treated cells that showed no statistically significant differences compared to the control (untreated) cells group (p < 0.33).
Analysis of the mitochondrial membrane potential
The dissipation of the mitochondrial inner membrane potential (Δψm) is considered as an early sign of apoptosis, preceding phosphatidylserine exposure on the outer plasma membrane [28]. In necrotic cells, Δψm and mitochondrial integrity are irreversibly compromised. In order to typify the mode of GPS- induced cell death, we examined the status of the mitochondrial membrane potential, Δψm, from cells treated with different doses of GPS, using the marker JC-1.
The status of the mitochondrial membrane potential was examined initially at 2 hours post-exposure (Figure 3A-B). Following exposure to 1 puff GPS, the cell population with disrupted Δψm (green), was almost double (31.62 ± 1.74%) compared to control cells (16.64 ± 0.52%). At higher doses, green fluorescence increased remarkably, reaching 48.27 ± 3.18% for cells treated with 3 puffs and 75.90 ± 3.07% for cells exposed to 5 puffs. The results were more prominent at 4 h post exposure (Figure 3C), especially for cells treated with the higher doses. Δψm depolarization ascended to 81.90 ± 0.40% for the cell sample treated with 3 puffs and to 90.24 ± 1.33% for cells exposed to 5 puffs GPS. Cells exposed to 1 puff, at 4 hours post-exposure did not exhibit such a dramatic increase in the percentage of the population (42.06 ± 2.03%) with disrupted Δψm when compared to the equivalent at 2 hours post-exposure. One way ANOVA analysis among groups of data for untreated and GPS-treated samples showed high statistical significance (p < 0.001 or p < 0.0001) in all cases, both for 2 hours and 4 hours examined samples, accentuating the observed dose-dependent effect of GPS on the depolarization of the mitochondrial potential in treated cells.
Confocal microscopy of cytochrome C and active caspase-3
Confocal laser scanning microscopy was utilised to visualise two events that are characteristic in the classical apoptotic process: the cytoplasmic release of cytochrome C from compromised mitochondria and the downstream activation of caspase-3.
Cells treated with 1, 3 or 5 puffs were harvested and fixed in 4% paraformaldehyde/PBS, pH 6.9 at 1, 4 or 24 hours post-exposure. Staining of untreated cells for cytochrome C (Figure 4B) showed bright fluorescence, which was localised in a distinct pattern in the perinuclear area. Cells treated with 1 puff, exhibited diffuse cytoplasmic staining for cytochrome C from 4 hours post-exposure (data not shown). Cells treated with 3 puffs GPS showed a widespread cytoplasmic staining pattern, resembling that observed in the staurosporine control, which increased in a time-dependent manner (Figure 4C-D). At 5 puffs GPS, cytoplasmic staining appeared as early as 1 hour post-exposure, and by 24 hours almost every cell was shrunk and exhibited a diffuse, yet fading pattern of fluorescence (data not shown).
Cells treated with 1 or 3 puffs GPS and stained for active caspase-3 exhibited a gradual increase in the occurrence of FITC-positive cells over time during the acute phase (1 and 4 hours post-exposure) (Figure 5, selected data shown). At 4 hours post-exposure (Figure 5, panels 5J-5L), the detected fluorescence was similar to the stauroporine control (panels 5D-5F) with some blebbing apparent. By 24 hours, the cells looked markedly shrunk and staining was non-specific (panels J-L). Moreover, 5 puff GPS treatment resulted in extremely limited signal at 4 hours and non-specific signal at 24 hours (Panels 5M)-5O).
Immunoblot analysis of active caspase-3
Caspase-3 activation was detected in Western blots probed with a specific polyclonal antibody that recognized the 17 kDa cleaved form of caspase-3 (Figure 6). CCRF-CEM cells were treated with 1, 2, 3 or 5 puffs of GPS and samples were harvested 30 min, 1, 2, 4 and 24 hours post-exposure. In apoptosis-positive control cells, apoptosis and caspase-3 activation were induced for 2 hours with 2 μM staurosporine.
In immunoblots, optimal signal for active caspase-3 was detected 4 hours post-exposure in the samples exposed to 1, 2 and 3 puffs, whereas in samples treated with 5 puffs, caspase-3 cleavage was undetected at all time-points examined (data not shown). At 4 hours post-exposure (Figure 5 panels J-L), caspase-3 activation was most prominent in the sample treated with 1 puff (Figure 6). Detection of the cleaved caspase-3 gradually decreased in the rest of the samples, as the number of puffs increased. Active caspase-3 was absent from the sample exposed to 5 puffs. Equal loading was verified by probing the samples analysed with an anti-α-tubulin antiserum.
DNA fragmentation analysis by flow cytometry
DNA fragmentation of cells treated with GPS was assessed quantitatively using DNA end-labelling (TUNEL) and flow cytometry (Figure 7). Cell populations exposed to 1, 3 or 5 puffs of GPS were treated with BrdU and DNA nicks were identified with an anti-BrdU monoclonal antiserum.
The untreated cells (Figure 7A) demonstrated basal levels (2.20 ± 0.48%) of DNA fragmentation (BrdU/PI-positive cells; upper right quadrant), with the majority of the population (97.09 ± 0.25%) located at the upper left quadrant (propidium iodide staining). The positive control was indicative of the DNA fragmentation occurring upon a two-hour induction of apoptosis with 2 μM staurosporine (Figure 7B). When treated with 1 puff GPS, there was almost a three-fold increase in the cell population with fragmented DNA (6.95 ± 0.65%) (Figure 7C), when compared to the negative control (one-way ANOVA, p < 0.0011). The cells treated with 3 puffs showed a maximum population stained for BrdU incorporation (81.77 ± 3.11%) (Figure 7D). At 5 puffs (Figure 7E), the BrdU/PI-positive population revealed a statistically significant decrease (70.78 ± 3.99%, p < 0.037) when compared to cells exposed to 3 puffs.
Discussion
In smokers' lungs, circulating lymphocytes are exposed to cigarette smoke through the wall of the capillary vessels on the surface of alveoli. T cells are one of the major groups of immune cells activated and recruited at the sites of lung lesions caused by CS inhalation [3,27,29]. In our study, we focused on the immediate effects of the gaseous phase of CS (GPS) on T lymphocytes, a cell group of the immune system, which has received little emphasis in the past. The objective was to determine the mode of lymphocyte cell death upon exposure to the gaseous phase of cigarette smoke (GPS) in vitro. For this purpose, we utilised a well-established T lymphoblast cell line to examine the effects of GPS.
Our results demonstrated that the mode of cell death was dose-dependent. We examined early and late events in the apoptotic pathway using cells exposed to low (1-2 puffs) and higher (3 or 5 puffs) doses of the gaseous phase. Experiments pertaining to the cytoplasmic release of cytochrome C and the subsequent activation of caspase-3, collectively pointed towards the activation of the caspase-3 dependent apoptotic pathway in a dose-dependent, as well as time-dependent manner. Furthermore, our results from the quantitative evaluation of the mitochondrial inner membrane potential and the late event of DNA fragmentation further supported a dose- and time-dependent change in the mode of cell death, albeit both DNA fragmentation [30] and mitochondrial inner membrane depolarization can occur both in apoptotic and necrotic cells [18].
Annexin V detection of phosphatidylserines on the outer plasma membrane indicated a dose-dependent increase in cell death, although it did not provide a solid basis for discrimination between apoptotic and necrotic death. The presence of Annexin V-positive cells at the higher doses of GPS cannot rule out a caspase-independent death. The apoptosis-specific markers cytochrome C and active caspase 3 prevailed at the low dose (1 puff) and partly at some of the higher doses (3 puffs) up to 4 hours post-exposure. Therefore, our findings are in agreement with previous work that supported a caspase 3-dependent apoptotic death [31,32]. In our system, we observed a dose-dependent decrease in caspase-3 activation, as GPS-doses increased. A switch from apoptosis to necrosis was evident in samples examined at a later time-point (24 h), mainly in cells treated with 3 puffs. The use of the higher dose (5 puffs) resulted mainly in necrotic death, as caspase-3 activation was undetectable. This was further supported by examination of the mitochondrial membrane potential (Δψm) of cell treated with low or high doses of GPS. At low toxicity, Δψm was disturbed enough so that caspase-dependent apoptosis would follow. When exposed to high toxicity, the majority of the cell populations exhibited great loss of Δψm, thus becoming deprived of mitochondrial ATP production, which is required for an apoptotic response together with cytosolic ATP [33]. Similarly, the results from DNA fragmentation point towards a dose-dependent transition from apoptosis to necrosis. This was most evident in the cell populations examined following exposure to 3 or 5 puffs. Although the cells exposed to the 3 puffs showed a maximum of BrdU/PI-positives, at 5 puffs the equivalent population was a lot less. Perhaps, the toxic shock that lead to the depletion of intracellular ATP resulted in the inhibition of endonucleases, which require ATP to be active [30]. Yet, necrosis following caspase-independent apoptosis cannot be ruled out.
Earlier studies supported that treatment with cigarette smoke condensate or extract (CSC or CSE) resulted in apoptosis in a range of cell lines, such as A549 alveolar epithelial cells [34,35], HFL-1 lung fibroblasts [22], human aortic endothelial cells [31], human umbilical vein endothelial cells [32] and alveolar macrophages [36]. Some cases showed a dose-dependent increase of activated caspase-3 [31,32]. There has also been evidence for caspase-independent apoptosis in CSE-treated cells, as shown with the use of caspase inhibitors [34,36].
Other groups concluded that necrosis was the only outcome following CSE treatment of A549, Jurkat and human umbilical vein cells [37], or human primary and BEAS-2B cells [18,20]. Finally, other research supported that CSE induced both apoptosis and necrosis in a dose-dependent manner in A549 [34], HFL-1 [38], U937 human premonocytic [39] and BEAS-2B cells [40].
Most of the times, the application of CSC or CSE on cultured cells assumes the concentration of the toxic components of one full-flavoured cigarette in a small volume of saline buffer or growth medium. The practice of CSC or CSE results in an overwhelming toxic shock to a small number of cultured cells. The lung epithelium cells are interconnected in a vast area structure, which almost uniformly accepts the toxic chemicals per CS inhalation [7,41]. These chemicals are in turn diluted in the existing air volume in the airways so that the resulting toxicity is not instantly detrimental for the epithelium, or the tissues surrounding it. Instead, chronic smoking results in the well-documented loss of the lung internal structures [27], which is due to the accumulation of toxic insults, increased epithelial cell death and a decline in immune cell function.
Exposure of cells to CS by means of CSC or CSE does not provide a reliable simulation system of normal smoking. In human lungs, the inhaled tobacco smoke is extensively diluted (approximately 15 times) due to the huge volume of air inhaled (500 c.c.) after each puff [41]. This dilution of the CS prevents the acute accumulation of a toxic critical mass and the ensuing cell damage, which more than likely happens when either CSC or CSE is used to challenge cultured cells. Furthermore, using either of these methods, it is very difficult to determine the quantity and the quality of the supplied dose and its toxicity. To our knowledge, there has never been in the literature a systematic and quantitative analysis of the tobacco components present in such a preparation. Therefore, it is plausible that only the water-soluble components of CS and a small part of the particulate matter contribute to the toxicity of these preparations. According to our method, the toxic substances in the gaseous phase of CS that are supplied to cells are diluted in a measured air volume within the volumetric chamber so that their contact with the cells simulates normal smoking conditions. In addition, each dose of the GPS supplied has previously been tested for its toxic component load using a well-established method [23].
Previous research mainly focused on the effect of CS on airway epithelium cells, since they are the first cell lineage directly exposed to the toxic effects of tobacco smoke [22,34,35]. Smoking, however, triggers inflammation of the airways, which is brought about by a cascade of events attributed to both innate and acquired immune reactions [27,29]. It is therefore of interest to study the immediate effect of CS on immune cells, as they have the ability to both initiate and perpetuate inflammatory responses in the diseased lung. To date, there are several accounts in the literature that report impaired responsiveness of immune cells -mainly T cells- in murine models that have been attributed to mainstream tobacco smoke [42,43]. It is possible that further research into the impact of CS on immune cells will open up new routes for COPD diagnosis and improve our understanding on the inflammatory versus immunosuppressant cascades, which will allow the design of more effective treatments for the related diseases.
Conclusion
In conclusion, from our work it is evident that: 1) exposure of cells to low toxicity GPS leads to apoptosis, while high toxicity GPS results in necrotic cell death; 2) supply of GPS should be carried out in an appropriately designed volumetric space, where CS is diluted at approximately the same proportion as in the smoker's airways, and 3) with each supply of CS to cell cultures, prior measurement of the toxic components of CS is necessary, using a well-established and reproducible method.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
AS, ALP and NDS were involved in the conception and experimental design of this study. NDS carried out the western blot analysis and FACS analysis for Annexin V/PI staining and JC-1 monitoring of Δψm depolarization. ALP performed the LDH cytotoxicity assay, the immunofluorescence experiments and the DNA fragmentation analysis. ADV and LHM were responsible for the confocal microscopy images. GB was involved in the flow cytometry analysis. DGH realized the gas chromatography analyses for the obtained GPS samples. All authors read and approved the final manuscript.
Contributor Information
Nadia D Sdralia, Email: sdralia@ibeb.gr.
Alexandra L Patmanidi, Email: alexpatmanidi@ibeb.gr.
Athanassios D Velentzas, Email: tveletz@biol.uoa.gr.
Loukas H Margaritis, Email: lmargar@biol.uoa.gr.
George E Baltatzis, Email: gbaltatzis@ibeb.gr.
Dimitris G Hatzinikolaou, Email: xatzdim@biol.uoa.gr.
Anastasia Stavridou, Email: nstavr@ibeb.gr.
Acknowledgements
We are grateful to Prof. John C. Stavrides for his important suggestions and critical reading of the manuscript.
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