Background
The airway smooth muscle is implicated in the pathological process of chronic airway diseases, such as asthma and chronic obstructive pulmonary disease [
1]. These diseases exhibit common features like increased parasympathetic activity and acetylcholine release [
2], or airway remodeling [
3]. Airway remodeling comprises changes in the composition, quantity and organization of airway wall components as consequence of chronic injury and repair of the airway epithelial–mesenchymal trophic unit [
1,
4]. The increased thickness of the smooth muscle layer could enhance shortening, leading to increased airway narrowing and airflow obstruction [
1].
ASMC cultures are a mixed population of cells exhibiting variability between contractile and synthetic-proliferative phenotypes [
5]. The distinction between ASMC phenotypes is based on the different expression of proteins implicated in the contraction mechanism, proliferation ability and protein synthesis. Synthetic-proliferative ASMCs appear to proliferate, while the features of contractile ASMCs are similar to those of the cells normally present in intact airway tissue [
4]. Different stimuli drive the transition between the different ASMC phenotypes. Although the mechanism involved is not yet well understood, evidence supports the hypothesis that the p42/p44 MAPK pathway is involved in the shift of ASMCs toward a less contractile phenotype [
6‐
9]. On the other hand, serum deprivation increases the percentage of cells that exhibit the “contractile phenotype” in ASMC culture [
10]. The shift of ASMCs from synthetic-proliferative to contractile phenotypes is attended by a decrease in M
2 and a parallel increase in M
3 expression [
11].
ASMCs express abundant G
i coupled muscarinic M
2 and G
q coupled M
3 muscarinic receptors [
12,
13], stimulation of which leads to the activation of the MAPK and the PI3K signalling pathways [
14]. M
2 and/or M
3-receptor stimulation by muscarinic agonists could affect ASMC proliferation, but until now muscarinic receptor agonists have been reported to be mitogenic for ASMCs mainly in combination with growth factors [
11,
15], acting through M
3 muscarinic receptors [
11]. On the other hand, the effect of muscarinic agonists on ASMC phenotype and in consequence their ability to proliferate has not been thus far fully addressed. In the present study we investigate the effect of prolonged cell incubation with muscarinic agonists, acetylcholine or carbachol, on phenotype shifting and cell contractility of ASMC obtained from rabbit trachea. We also studied the mitogenic effect of muscarinic agonists on ASMC in relevance with their proliferative or contractile phenotype.
Methods
Animals
Adult rabbits were maintained in individual cages in a controlled environment and were provided with food and water before use for the study. Animals were treated in compliance with ethical and institutional guidelines. All protocols were approved by the Ethics Committee of the Department of Medicine, School of Health Sciences of University of Thessaly. Rabbits were euthanised by an overdose of intravenously administrated Pentothal (Abbott, Abbott Park, IL, USA).
ASMC isolation and culture
The isolation of ASMC from adult rabbit trachea was done as previously described [
16]. Briefly, tracheal smooth muscle was epithelium denuded, dissected from cartilage and washed in low Ca
2+ Krebs solution (139 mM NaCl, 5.4 mM KCl, 1.47 mM MgSO
4, 11 mM glucose, 1.47 mM KH
2PO
4, 2.8 mM Na
2HPO
4, 1.4 mM NaHCO
3, 0.2 mM CaCl
2). Tracheal smooth muscle was digested in 2 ml of low Ca
2+ Krebs solution containing 0.25% bovine serum albumin (BSA), 2 mg/ml collagenase I and 10 U/ml elastase IV, for 30 min at 37°C with vigorous shaking. Then it was washed in low Ca
2+ Krebs solution, centrifuged (1000 rpm for 10 min) and incubated for 45 min in low Ca
2+ Krebs solution containing 0.25% BSA, 1 mg/ml collagenase I and 20 U/ml elastase IV. Dispersed ASMCs were washed and centrifuged (1000 rpm for 10 min) twice in Dulbecco’s modified Eagle’s medium/Ham/F12 (DMEM/F12) containing 10% fetal bovine serum (FBS), 100 U/ml penicillin and 100 g/ml streptomycin. The isolated ASMC were placed in culture flasks and grown at 37°C in a humified incubator under 5% CO
2.
Study design
Isolated tracheal ASMCs were serum starved by incubation in Dulbecco’s modified Eagle’s medium/Ham/F12 (DMEM/F12) containing 100 U/ml penicillin and 100 g/ml streptomycin, as indicated, and treated with the muscarinic agonists, acetylcholine (ACh; 10-7 M-10-3 M), or carbachol (CCh; 10-9 M-10-5 M). The effect of the muscarinic agonists on the ASMC phenotype was studied using optical microscopy, as well as indirect immunofluorescence, and Western blot analysis with anti-smooth muscle α-actin mouse monoclonal antibody, anti-myosin (smooth) clone HSM-V mouse monoclonal antibody and anti-desmin rabbit polyclonal antibody. The density of muscarinic receptors on ASMCs was studied with [N-methyl-3H]scopolamine binding on isolated cell membranes and the effect of acetylcholine and/or carbachol on the contractile ability of individual ASMCs in culture was estimated by counting the cell area before and after muscarinic agonist treatment in the presence or absence of atropine.
Cell proliferation was estimated using the methyl-[3H]thymidine incorporation, the MTT-Cell Titer 96® AQueous One Solution Assay (Promega) and Trypan blue cell counting methods. In the MTT cell proliferation assay, the optical density (OD) of cells incubated in serum-free medium (24 h) was used as control (set at 100%). Results are presented as percentage of OD of the control cells, while the DNA synthesis is presented as cpm of radioactive material incorporated in ASMCs. The possible involvement of PI3K and MAPK signalling pathways was studied using the pathways inhibitors LY294002 and PD98059 respectively.
Cell culture treatment
ASMCs were trypsinised, counted and seeded into appropriate cell culture plates. They were allowed to adhere overnight, washed twice with phosphate buffered saline (1XPBS) and pre-incubated in FBS-free DMEM/F12 medium, containing 100U/ml penicillin and 100 μg/ml streptomycin. ASMCs were incubated in serum free medium for 1 or 7 days, and incubated in 10% FBS-containing medium or serum free medium in the presence or absence of increasing concentrations of the muscarinic agonists; acetylcholine (10-7 M-10-3 M) and carbachol (10-9 M-10-5 M) as indicated. Specifically, cells were incubated with ACh (10-7 M) or CCh (10-9 M) in morphology observation and thymidine incorporation experiments, with ACh (10-5 M) or CCh (3 × 10-7 M) in contractile phenotype marker protein expression, M3 muscarinic receptor expression and cell proliferation experiments and with ACh (10-3 M) or CCh (10-5 M) in responsiveness experiments. The culture medium was replaced every 3 days, during the incubation periods. For the study of the possible involvement of PI3K and/or MAPK signalling pathways, LY294002 (20 μΜ) and PD98059 (100 μΜ) inhibitors were added in cell culture medium 15 or 60 min prior to the addition of the muscarinic agonists, respectively.
Cell morphology
Cell morphology was observed with a reverse microscope Nikon Diaphot 300 (Nikon Inc., Melville, NY, USA).
Indirect immunofluorescence
Cells were plated onto glass slides, which were resided in culture plates and treated as indicated above. After the treatment, cells were fixed with PBS-3% formaldehyde and permeabilized with PBS-1% Triton X-100, blocked in PBS-0.1% Tween 20- 3% BSA and incubated with anti-smooth muscle α-actin mouse monoclonal antibody (1:1000, Sigma), anti-myosin (smooth) clone HSM-V mouse monoclonal antibody (1:1000, Sigma) and anti-desmin rabbit polyclonal antibody (1:1000, Sigma), followed by incubation with an anti-mouse IgG or anti-rabbit IgG antibodies conjugated with CY3. Finally, coverslips were mounted on Vectrashield solution containing DAPI for DNA staining and the percentage of the cells that expressed α-actin, SM-MHC (Smooth muscle-Myosin Heavy Chain) and desmin proteins was estimated.
Western blot analysis
Cells were lysed in 20 mM Tris-Cl pH 8.0, 150 mM NaCl, 1% Triton X-100, 1 mM dithiothreitol, and 100 mg/mL-1 phenylmethylsulphonyl fluoride. Total cell extracts were cleared by centrifugation (10000 g for 20 min at 4°C). 40 mg of protein were analysed in 10% sodium dodecyl sulphate–polyacrylamide electrophoresis gel and transferred to a nitrocellulose membrane. Western blot analysis was performed using anti- smooth muscle β-actin mouse monoclonal antibody (1:5000, Cell Signalling), anti-smooth muscle α-actin mouse monoclonal antibody (1:1000, Sigma), anti- myosin (smooth) clone HSM-V mouse monoclonal antibody (1:1000, Sigma) and anti-desmin rabbit polyclonal antibody (1:1000, Sigma). Membranes were then incubated with horseradish peroxidase conjugated anti-rabbit IgG (1:3000, Cell Signalling) or anti-mouse IgG (1:3000, Cell Signalling), and signals visualised by enhanced chemoluminescence (ECL).
[N-methyl-3H]scopolamine binding studies
The binding of [
N-methyl-
3H]scopolamine ([
3H]NMS) was done as previously described [
17]. Briefly, ASMCs were serum deprived for 24 h and then incubated for 3, 7 or 15 days with 10% FBS, ACh (10
-5 M) or CCh (3 × 10
-7 M). Control cells were incubated in serum free medium. Cells were lysed by scraping in buffer (25 mM Tris-HCl, 2.5 mM CaCl
2, 1 mM PMSF, 1 mM Pefabloc and 10 μg/ml aprotinin). Cell extracts were homogenized with 5 strokes in a Heidolph Silent Crusher S (Heidolph Instruments GmbH & Co. KG, Germany) and the homogenate was centrifuged at 10000 g for 5 min at 4°C. The supernatant was diluted up to 11 ml in assay buffer (10 mM HEPES, 100 mM NaCl, 10 mM MgCl
2) and centrifuged at 150000 g for 30 min at 4°C. The pellet was then resuspended in assay buffer and subjected to sonication for 5 sec. 30 μg of protein was added in the reaction, along with 5 nM of [
3H]NMS. Nonspecific binding was estimated by the presence of 100 μM atropine. After 80 min of incubation in order to allow radioligand binding only to M
3 receptors [
17], the samples were filtered through GF/B filters (Millipore) using a Millipore vacuum filtration system (EMD Millipore Corporation, Billerica, MA, USA). Before radiation counting in a Wallac β-counter, filters were dried overnight and incubated in Ultimate gold XR (Perkin Elmer) scintillation fluid for 1 h at RT.
Contractility studies
ASMCs were grown to confluence in culture plates and incubated 3-15 days in serum-free medium, or medium containing 10% FBS, acetylcholine (10-5 M), carbachol (3 × 10-7 M). The cells were washed twice with phosphate buffered saline (1xPBS), and then incubated for 5 min with trypsin-EDTA solution, in order to detach myocytes from the substrata. The detached cells were incubated with acetylcholine (10-3 M) or carbachol (10-5 M) for 5 min. Photographs were taken before and after cell treatment, in a phase-contrast microscopy Nikon Diaphot 300 (Nikon Inc., Melville, NY, USA) with Leica DFC480 Camera (Leica Microsystems, Wetzlar, Germany). The ratio of total cell area before and after treatment was measured using the Image J programme. To confirm that contractile shortening responses were the direct result of ACh or CCh stimulation, atropine (10-6 M) was added in control experiments before ACh or CCh exposure.
Cell proliferation studies
Proliferation of cultured ASMCs was estimated using (A) the methyl-[
3H]thymidine incorporation method,(B) the MTT-Cell Titer 96® AQueous One Solution Assay (Promega) method and (C) the Trypan blue method.
(A)
DNA synthesis in airway smooth muscle cells was estimated by measuring methyl-[3H]thymidine incorporation. Methyl-[3H]thymidine was added in the culture medium the last 18 h of incubation. The counts per minute (cpm) of the radioactive DNA were counted using a Wallac scintillation counter. Cells incubated in serum free medium were used as negative control in each experiment. The proliferating capability of cells was evaluated by positive controls, which were cells incubated in 10% FBS.
(B)
The number of airway smooth muscle cells was estimated using the Cell Titer 96® AQueous One Solution Assay (Promega) method as previously described [
18]. The absorbance of the MTT formazan reduction product was measured at 490 nm with a reference at 630 nm in an ELISA plate reader. The measured optical density (OD) is reminiscent of the cell number in the well, since there is a linear response between the measured OD and cell number (data not shown).
(C)
Cell number was estimated by direct cell counting, using the Trypan blue method. Trypan blue dye was added to ASMCs detached and suspended in 1ΧPBS solution and live cells that did not absorb the dye were counted using a Neubauer slide.
Data analysis
In ASMCs contractility studies each point represents the mean value of 5 cells, while in [3H]NMS binding and cell proliferation experiments each point was performed in triplicate. In immunofluorescence experiments the percentage of cells expressing the contractile proteins was estimated by counting the cells that were fluorescent, as well as the total cell number as indicated by DAPI staining. Image analysis of the images obtained from the Western blotting and the contractility studies was conducted with the use of MacBiotronics Image J programme for Light Microscopy (National Institutes of Health, Bethesda, MD, USA) and results were expressed as intensity values or as percentage of the initial cell area, respectively.
All data are expressed as means ± SEM and N refers to the number of independent experiments. Differences between means were analysed by Unpaired t-test with statistically significant differences between groups being determined by Mann-Whitney test. A comparison was considered significant when P < 0.05. The statistical analysis was performed using Graph Prism.
Discussion
In airway smooth muscle, muscarinic agonists may activate signalling pathways such as the Rho kinase, PI3K or MAPK pathways [
2]. Since the MAPK pathway is involved in modulation of ASMCs toward a less contractile phenotype [
6,
7,
10], we hypothesized that muscarinic agonists could affect ASMC phenotype. Indeed, we found that rabbit tracheal ASMCs subjected to prolonged (30 days) incubation with ACh or CCh switched to a proliferative phenotype, i.e. cells appeared flat, similar to that observed in ASMCs cultured in the presence of 10% FBS. Accordingly, indirect immunofluoresence, as well as western blot analysis experiments demonstrated that this “induction” of a proliferative phenotype was accompanied by a significant decrease in the expression of the contractile phenotype markers α-actin, SM-MHC and desmin. To our knowledge, this is the first study reporting that muscarinic agonists induce the shift of ASMCs toward a proliferative phenotype. Our results are in agreement with a previous study by Gosens et al. [
20] who showed that prolonged treatment with the muscarinic agonist methacholine of bovine tracheal smooth muscle strips in organ-cultures diminished the expression of myosin and actin.
Furthermore, there are studies indicating that the switch of ASMC phenotype from proliferative to contractile caused by incubation in the absence of FBS is accompanied by an increase in M
3 expression [
11]. Accordingly, our results demonstrate that the ACh or CCh induced shift of the cell phenotype towards a proliferative one, was followed by a decrease of the M
3 receptors density, as shown by decreased [
3H]NMS binding in cells incubated with ACh or CCh for 7-15 days. Evidence suggests that agonists may induce phosphorylation and internalization of muscarinic receptors [
21]. In our study, the down regulation of M
3 receptors of ASMCs was accompanied by decreased responsiveness of isolated cells, incubated for 3-15 days with muscarinic agonists, to ACh or CCh, due probably also by the decrease of smooth muscle protein expression. These results are in agreement with results obtained from contractility studies demonstrated that long-term methacholine pretreatment of bovine tracheal smooth muscle strips decreased maximal contraction and sensitivity to methacholine [
20]. In vivo studies revealed increased cholinergic tone in asthma [
22] and clinical studies showed that the addition of anti-cholinergic drugs to the corticosteroid or long-acting β2-agonist treatment is beneficial for asthmatic patients [
23,
24]. On the other hand in vitro studies performed with bronchial smooth muscle from asthmatic patients showed that the altered airway responsiveness seen in asthmatic patients is not reflected in airway smooth muscle sensitivity in vitro and that the sensitivity to carbachol was significantly reduced in tissue from asthmatic patients [
25,
26].
Even though a more proliferative phenotype was induced by muscarinic agonists, this phenotype is not necessarily associated to increased proliferative capacity, since each phenotype has different expression of proteins, as well as receptors that affect the activation of signalling pathways that are involved in the proliferation process. We studied the proliferative effect of muscarinic agonists ACh and CCh on ASMCs that were serum starved for 24 h or 7 days. According to our results and previous studies [
5], 24 h serum starved cells express mainly the proliferative ASMC phenotype while 7 days serum starved cells express an increased percentage of ASMCs with contractile phenotype. We found that ACh and CCh increased [
3H]thymidine incorporation in rabbit tracheal ASMCs, serum starved for 24 h before muscarinic agonists addition (Figure
7), but did not affect cell number (data not shown). On the other hand when cells grew in serum free medium for 7 days prior to the addition of ACh and CCh, both muscarinic agonists significantly increased cell number (Figures
8 and
9). This effect was transient since no further increase was observed after 24 h (2-15 days incubation with muscarinic agonists). These results suggest that the mitogenic effect of muscarinic agonists depends on the ASMC phenotype. Although, in airways, muscarinic agonists have a proliferative effect on fibroblasts [
27,
28] until now available data demonstrate that stimulation of muscarinic receptors is not sufficient to induce ASMC proliferation, but the synergetic muscarinic receptor stimulation with growth factors may cause an induction of mitogenesis [
29]. However, our results demonstrate that the mitogenic effect of muscarinic agonists may depend on ASMC phenotype, since it seems reasonable that the decrease of M
3 receptor expression in cells cultured in the presence of FBS, ACh or CCh is responsible for the weak mitogenic effect of muscarinic agonists.
It has been reported that the stimulation of muscarinic receptors in ASMCs activates the PI3K or MAPK pathways [
3]. However, the PI3K pathway inhibitor LY294002 reduced [
3H]thymidine incorporation induced by ACh, while MAPK pathway inhibitor PD98059 reduced [
3H]thymidine incorporation induced by CCh. These results suggest that whereas the stimulation of muscarinic receptors may cause the [
3H]thymidine incorporation in rabbit tracheal ASMCs via either PI3K or MAPK pathways, these pathways are activated differentially by ACh and CCh. Both ACh and CCh are agonists of all muscarinic and also nicotinic receptors. Although the main difference between ACh and CCh is their resistance to the cholinesterase activity, some data suggest that acetylcholine and carbachol interact with different muscarinic receptors [
30,
31]. However both LY294002 and PD98059 abolished the effect of ACh and CCh on ASMC number suggesting that although ACh and CCh may activate PI3K or MAPK pathways differently, the activation of both pathways is required for ASMC proliferation.
Conclusions
In conclusion, muscarinic receptor stimulation may shift ASMC phenotype to “proliferative”, reduce ASMC responsiveness and have a transient mitogenic effect, via MAPK and PI3K pathway signalling, depending on the ASMC phenotype. These results may have clinical significance given that in chronic inflammatory airway diseases increased acetylcholine release is observed in a periodical pattern, for example during asthma attacks [
2]. Therefore, the presence of acetylcholine in the airway can lead to alteration in the ASMC phenotype that makes them more prone to be affected by growth or inflammatory factors present in the airway in such diseases, and lead to increased proliferation rate. Both the phenotype shift and the increased proliferation can lead to the ASMC hypertrophy and hyperplasia, which are characteristics of airway remodeling. Furthermore, there are studies that propose that muscarinic agonists have an immediate effect on airway tone, since they can increase the contractility of isolated ovine tracheal strips [
2,
32‐
34]. This acute effect of muscarinic agonists on airways, accompanied by changes in ASMC phenotype and induction of cell proliferation under prolonged incubation, indicates the significance of muscarinic agonists in the physiology and pathophysiology of airway function.
Competing interests
The authors declare that this manuscript has been financed by Boehringer Ingelheim Pharma GmbH & Co, KG, Biberach an der Riss, Germany. Specifically, Boehringer Ingelheim Pharma GmbH & Co has funded the experimental procedure, paid the salary of the researcher and is financing the article-processing charge. The authors do not hold any stocks or shares in an organization that may in any way gain or lose financially from the publication of this manuscript, either now or in the future. The authors are not currently applying for any patents relating to the content of the manuscript, or have not received reimbursements, fees, funding, or salary from an organization that holds or has applied for patents relating to the content of the manuscript. The authors have no other financial or non-financial (political, personal, religious, academic, ideological, intellectual, commercial or any other) competing interests.
Authors’ contributions
RS has been involved in acquisition, analysis of data and interpretation. EP has been involved in data analysis and interpretation and participated in the design of the study. AV has been involved in data acquisition, analysis and interpretation IM has been involved in data acquisition and analysis. PAM conceived of the study and participated in its design. KG conceived of the study and participated in its design. AH has designed and coordinated the study and participated in data analysis and interpretation. All authors have read, commented on and approved of the manuscript.