trans-Caryophyllene, a Natural Sesquiterpene, Causes Tracheal Smooth Muscle Relaxation through Blockade of Voltage-Dependent Ca2+ Channels
by
Leidiane Pinho-da-Silva
1,2,†,
Paula Virgínia Mendes-Maia
1,2,†,
Taylena Maria Do Nascimento Garcia Teófilo
1,
Roseli Barbosa
1,
Vania Marilande Ceccatto
1,
Andrelina Noronha Coelho-de-Souza
1,
Jader Santos Cruz
3,* and 
José Henrique Leal-Cardoso
1,* 1
Laboratório de Eletrofisiologia, Instituto Superior de Ciências Biomédicas, Universidade Estadual do Ceará, Av. Paranjana #1700, Fortaleza 60740-000, Ceará, Brazil
2
Programa de Pos-Graduação em Fisiologia e Farmacologia, Universidade Federal de Minas Gerais, Avenida Antonio Carlos #6627, ICB-UFMG, Belo Horizonte 31270-010, Minas Gerais, Brazil
3
Departamento de Bioquímica e Imunologia, Universidade Federal de Minas Gerais, Avenida Antonio Carlos #6627, ICB-UFMG, Belo Horizonte 31270-010, Minas Gerais, Brazil
*
Authors to whom correspondence should be addressed.
†
These authors contributed equally to this work.
Molecules 2012, 17(10), 11965-11977; https://doi.org/10.3390/molecules171011965
Submission received: 10 July 2012
/
Revised: 19 September 2012
/
Accepted: 5 October 2012
/
Published: 11 October 2012
(This article belongs to the Section Natural Products Chemistry)
Abstract
:trans-Caryophyllene is a major component in the essential oils of various species of medicinal plants used in popular medicine in Brazil. It belongs to the chemical class of the sesquiterpenes and has been the subject of a number of studies. Here, we evaluated the effects of this compound in airway smooth muscle. The biological activities of trans-caryophyllene were examined in isolated bath organs to investigate the effect in basal tonus. Electromechanical and pharmacomechanical couplings were evaluated through the responses to K+ depolarization and exposure to acetylcholine (ACh), respectively. Isolated cells of rat tracheal smooth muscle were used to investigate trans-caryophyllene effects on voltage-dependent Ca2+ channels by using the whole-cell voltage-clamp configuration of the patch-clamp technique. trans-Caryophyllene showed more efficiency in the blockade of electromechanical excitation-contraction coupling while it has only minor inhibitory effect on pharmacomechanical coupling. Epithelium removal does not modify tracheal smooth muscle response elicited by trans-caryophyllene in the pharmacomechanical coupling. Under Ca2+-free conditions, pre-exposure to trans-caryophyllene did not reduce the contraction induced by ACh in isolated rat tracheal smooth muscle, regardless of the presence of intact epithelium. In the whole-cell configuration, trans-caryophyllene (3 mM), inhibited the inward Ba2+ current (IBa) to approximately 50% of control levels. Altogether, our results demonstrate that trans-caryophyllene has anti-spasmodic activity on rat tracheal smooth muscle which could be explained, at least in part, by the voltage-dependent Ca2+ channels blockade.
1. Introduction
The terpenes, found in essential oils of different plants, are micro-constituents most commonly used as flavor additives in food, toiletries, and perfumes [1]. Recent studies from different groups around the World have shown that terpenes and terpenoids exert a plethora of pharmacological effects [2]. trans-Caryophyllene is an important constituent of the essential oil of several species of plants. It is the major chemical constituent (20.6%) of the essential oil of Pterodon polygalaeflorus (EOPp). EOPp blocks the electromechanical excitation-contraction coupling without affecting the pharmacomechanical coupling [3]. The blocking effect caused by EOPp was suggested to result from inhibition of dihidropyridine-sensitive Ca2+ channels, but there were no evidence to support that suggestion [3].
trans-Caryophyllene has been reported to possess many pharmacological effects. For example, it displays antimicrobial [4] and analgesic activity [5]. It activates the endocannabinoid system [6]. trans-Caryophyllene also has a well-documented anti-inflammatory activity [7,8]. Additionally, trans-caryophyllene is effective on intestinal smooth muscle, blocking the electromechanical and pharmacomechanical excitation-contraction coupling [9]. Those activities allow it to be considered as a potential anti-spasmodic agent in tracheal smooth muscle.
Not much information is currently available on the potential spasmolytic effects of trans-caryophyllene on tracheal smooth muscle. We demonstrate herein that trans-caryophyllene has anti-spasmodic effects on rat tracheal smooth muscle. In order to explain this result we hypothesized that trans-caryophyllene elicits tracheal smooth muscle relaxation by inhibiting voltage-dependent L-type Ca2+ channels.
2. Results and Discussion
2.1. Effects of trans-Caryophyllene on Basal Tone of Isolated Rat Trachea with or without Epithelium
trans-Caryophyllene activity on the basal tone of rat tracheal segments with or without epithelium differed. In rat tracheal segments with intact epithelium, trans-caryophyllene at the concentration range from 0.05 to 5.0 mM provoked a progressive and significant relaxation (Figure 1; p < 0.05; one way ANOVA; n = 6). Interestingly, when we used concentrations from 10 to 50 mM the tendency to provoke relaxation disappeared and the tonus returned to control levels. After epithelium removal, trans-caryophyllene had no significant effect on rat tracheal basal tone (Figure 1; n = 8).
2.2. Inhibitory Effects of trans-Caryophyllene on Contractions Induced by High-K+ in Isolated Rat Trachea with or without Epithelium
When non-cumulatively administered to the preparation, trans-caryophyllene (0.3 to 50 mM) concentration-dependently and significantly (p < 0.05, Two Way ANOVA) decreased the contractions induced by high K+ concentration (80 mM) (Figure 2Ai,Aii).
In the presence of intact epithelium trans-caryophyllene showed an IC50 value of 3.7 ± 0.4 mM (n = 5). When epithelium was removed the IC50 value was 8.4 ± 10.5 mM (n = 4). The results suggest that trans-caryophyllene induces relaxation in a concentration-dependent manner (Figure 2B). It seems that the effect is not dependent on the presence of intact epithelium.
2.3. Inhibitory Effects of trans-Caryophyllene on Contractions Induced by ACh in Isolated Rat Trachea with or without Epithelium
As trans-caryophyllene relaxed tracheal smooth muscle (with or without intact epithelium) contracted by 80 mM extracellular K+, the possible inhibitory effects of trans-caryophyllene on contractions induced by ACh was also investigated. It was found that in tracheal preparations with (Figure 3Ai, n = 6) or without (Figure 3Aii, n = 8) epithelium and pre-exposed for 5 min to a given trans-caryophyllene concentration (0.005 to 50 mM), there was inhibition of the contraction induced by sub-maximal concentration of ACh (10 μM) as compared to controls.
This inhibition, however, was only partial, reaching a peak at 30 mM trans-caryophyllene, at which concentration the sub-maximal ACh-induced contraction only declined to 64.43 ± 2.78 and 65.03% ± 2.15% of control in preparations with and without epithelium, respectively. The calculated relative IC50 values were 7.79 ± 1.47 mM and 8.55 ± 1.25 mM in preparations with and without epithelium, respectively (Figure 3B and 3C).
In segments with (five out of six) or without (six out of eight) epithelium, but previously challenged with ACh (10 µM), application of trans-caryophyllene at 10 mM or higher concentrations promoted a sustained contraction. In each of these cases time was allowed to achieve partial subsidizing of trans-caryophyllene-induced sustained contraction and for the subsequent contraction induced by ACh. The peak sustained tension was then measured. Peak contraction induced by 10 mM trans-caryophyllene in ACh-sensitized preparations reached 0.53 ± 0.06 and 0.31 ± 0.07 gF, with or without intact epithelium, respectively.
2.4. Effects of trans-Caryophyllene on Contractions Induced by ACh in Isolated Rat Trachea with or without Intact Epithelium in Ca2+-free Solution.
The effects of trans-caryophyllene (10 mM) on ACh (60 μM)-induced contractions in preparations maintained in Ca2+-free solution [modified Tyrode’s solution from which Ca2+ was removed and EGTA (0.2 mM) was added] were investigated. In segments where epithelial layer was present trans-caryophyllene diminished the ACh-induced contraction (Figure 4B, p < 0.05). When contractions with (n = 8) or without (n = 8) intact epithelium were compared between themselves and with their respective controls no statistically significant difference (p > 0.05, One Way ANOVA) was observed (Figure 4 and Discussion). To avoid misinterpretations due to a possible decrease in ACh contractile response we decided to compare the effects of trans-caryophyllene with a second ACh application in Ca2+ free conditions (Figure 4, last two bar graphs). Figure 4B shows that trans-caryophyllene, under our experimental conditions, did not inhibit pharmacomechanical coupling.
2.5. Effects of trans-Caryophyllene on Isolated Tracheal Smooth Muscle Cells
Having established that the trans-caryophyllene effect was much more significant on the electromechanical coupling in isolated tracheal smooth muscle preparations, possibly by blocking Ca2+ influx, we next investigated whether 3 mM trans-caryophyllene [a concentration that blocks approximately 50% of K+(80 mM)-induced contraction] could block Ca2+ influx by inhibiting L-type Ca2+ channels in single rat tracheal smooth muscle cells. To provide direct evidence we performed whole-cell patch-clamp in myocytes to test the effects of trans-caryophyllene on L-type Ca2+ channels.
Figure 5A shows representative examples recorded at 10 mV test potential before (control condition, black trace) and after the application of trans-caryophyllene (gray trace). ICa,L (L-type calcium current) was reduced by approximately 50% of maximal current. To verify the time-course for inhibition provoked by trans-caryophyllene, ICa,L amplitudes were plotted as function of time (Figure 5B). These results were similar to all cells tested (n = 6) and pooled data are depicted in Figure 5C. The current-voltage relationships (I–V) were constructed by applying 100 ms step depolarizations from −70 to +60 mV in 10 mV increments. Figure 5D shows the average I-V in the absence (black symbols, n = 4) and presence of trans-caryophyllene (red symbols, 3 mM, n = 4).
2.6. Discussion
The current understanding of excitation-contraction coupling in smooth muscle cells indicates that the following two mechanisms may be involved: (1) Those dependent on changes in membrane potential (electromechanical coupling) and (2) those independent of the changes in membrane potential (pharmacomechanical coupling) [10]. Through these mechanisms intracellular Ca2+ ([Ca2+]i increases and triggers contractions. Thus, [Ca2+]i regulates smooth muscle contractions as a result of electro- and pharmacomechanical couplings. To clarify the mechanism of the trans-caryophyllene-induced relaxation of airway smooth muscle, we determined the effect of trans-caryophyllene on electromechanical and pharmacomechanical coupling. Our study shows for the first time a relaxant effect of trans-caryophyllene on airway basal tone in rat isolated trachea. This relaxation of basal tone is dependent of epithelial layer into the tracheal wall. In addition, pre-incubation of trans-caryophyllene caused a concentration-dependent decrease in high K+ depolarization-induced and ACh-induced contractions. Conversely, epithelium removal did not change the relaxation provoked by trans-caryophyllene. Overall, these findings corroborate our previous studies exploring the effects on trachealis muscle of an essential oil having trans-caryophyllene as its major constituent [3].
It is generally known that prostanoids synthesized by epithelial cyclo-oxygenases (COX) play a major role in the control of airway contractility since COX inhibitors diminish the airway basal tone [11,12,13,14,15,16,17]. trans-Caryophyllene decreased the basal tone in rat trachealis muscle only when epithelial layer was preserved. This observation could be explained by a direct inhibitory effect of trans-caryophyllene on the COX or by causing an imbalance between relaxant and constrictor prostanoids synthesized by epithelial COX. The absence of trans-caryophyllene-induced relaxant activity on preparations without intact epithelium is consistent with these assumptions. Further studies conducted with selective antagonists are needed to clarify this point.
Membrane depolarization by high extracellular K+ concentrations induces contraction of airway smooth muscle that is easily relaxed by Ca2+ channel antagonists [18] and largely abolished in a Ca2+ free medium [18] indicating that high K+-elicited contraction is triggered by Ca2+ influx through activation of voltage-operated Ca2+ channels. We showed that pre-incubation of trans-caryophyllene caused a concentration-dependent decrease in high K+ elicited contractions suggesting that a blockade of voltage-operated Ca2+ channels could be involved. We would argue that trans-caryophyllene may have exerted its effect by directly acting on airway smooth muscle cells. This idea is rather likely because mechanical removal of the epithelium did not alter the effect of trans-caryophyllene. Therefore, the inhibition of airway smooth muscle contraction elicited by high K+ may not requires epithelium-derived relaxing factors.
In the current study, the application of ACh on rat tracheal strips increased tension. This response is a composite of two phases, a rapid raise (which is assumed to be dependent on Ca2+ influx and Ca2+ release from internal stores) followed by a sustained component (produced mainly by the influx of extracellular Ca2+) [19]. In the presence of extracellular Ca2+, pre-incubation of trans-caryophyllene promoted only a minor inhibition (about 20% at concentrations above 10 mM) of ACh-induced contractions in preparations, with or without intact epithelium. We examined trans-caryophyllene effects on Ca2+ release elicited by exposure to ACh in the absence of extracellular Ca2+. It is worth noting that ACh causes Ca2+ release by pharmacomechanical coupling mediated by inositol 1,4,5-trisphosphate [16,20]. In the absence of extracellular Ca2+, trans-caryophyllene was not found to have any inhibiting effect on contractions induced by ACh. These results indicate that trans-caryophyllene do not affect Ca2+ release from intracellular stores.
The lack of effect on ACh-induced contractions is consistent with the hypothesis of trans-caryophyllene activity being largely restricted to voltage-dependent Ca2+ channels, since only a minor part of ACh-induced contraction is due to depolarization and Ca2+ influx through these channels [13]. In order to evaluate this hypothesis we used the patch-clamp technique in dissociated cells of the trachealis muscle to make a direct measurement of trans-caryophyllene effect on voltage-dependent Ca2+ currents. Ba2+ was used because this ion permeates the voltage-dependent Ca2+ channels but not the receptor-operated Ca2+ channels and it blocks K+ channels [14,15]. These experiments (Figure 5) showed that trans-caryophyllene, in a concentration in which it decreases high K+-induced contractions, also blocked the voltage-dependent Ca2+ current.
This profile presented by trans-caryophyllene, which shows a predominant activity on voltage-dependent Ca2+ channels, has not been found in other biological preparations. For example, we did find evidences for a relative selectivity of trans-caryophyllene activity on voltage-dependent Ca2+ channels in ileum [9]. trans-Caryophyllene is a major component in many essential oils from plants that are reported to be used to treat inflammation and asthma [21]. Our study is important because it shows, by the first time, the antispasmodic effect elicited by trans-caryophyllene in the airway smooth muscle due to voltage-dependent Ca2+ channels blockage.
Recently, clinicians have been seeking additional options other than the currently available conventional treatments to improve the condition of patients with asthma and to spare systemic corticosteroid administration. Therefore, new drugs such as calcium channel inhibitors have been developed to treat asthma-related symptoms [22]. We think that our study could raise the possibility of trans-caryophyllene be used as a lead compound for this purpose, especially because it has very low toxicity.
3. Experimental
3.1. Animals
Wistar male rats (Rattus novergicus), weighing 250–350 g were used. Animals were bred and housed in the animal facility of State University of Ceará under a controlled environment (23–25 °C). Experiments performed were in accordance with the Conselho Nacional de Controle de Experimentação Animal (CONCEA) and US guidelines (NIH publication #85-23, revised in 1996) and received previous approval by local ethical committee on use of animals for experimentation (Comitê de Ética para o Uso de Animais em Pesquisa CEUA/UECE – Protocol # 06379067-0).
3.2. Drugs
Acetylcholine (ACh) was used at 10 and 60 μM to elicit contractions in 2.0 and in 0.0 mM calcium concentration, respectively. High extracellular K+ concentration (80 mM) was used to elicit contractions. The inhibitory effects of trans-caryophyllene were investigated by pre-incubating it in the tissue bath chamber. Bath final trans-caryophyllene concentrations were prepared by dilution of 245 mM trans-caryophyllene stock solution. This stock solution was prepared by diluting trans-caryophyllene directly in Tween 80 (dispersant agent) and afterwards in Tyrode’s solution [composition in mM: NaCl 136.0, KCl 5.0, MgCl2 0.98, CaCl2 2.0, NaH2PO4 0.36, NaHCO3 11.9 and glucose 5.5 (pH 7.4)]. The equivalent Tween 80 concentration had a very small effect on pre-contracted tracheal strips (<5%, data not shown).
Drugs [ACh, trans-caryophyllene, ethylene glycol-bis(aminoethylether)-N,N,N',N'-tetraacetic acid (EGTA), N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid (HEPES), tetraethylammonium chloride (TEA), adenosine 5'-triphosphate disodium (Na2-ATP), papain, bovine serum albumin (BSA), dithiothreithol (DTT), collagenase type II and hyaluronidase] were purchased from Sigma Chemical Company (St. Louis, MO, USA) and from Reagen (Colombo, Paraná, Brazil). All drugs and salts were of analytical grade.
3.3. Isolated Tissue Preparation
The animals were sacrificed by cervical dislocation. To study the tracheal muscle relaxation tracheal ring strips were then mounted in a 5 mL tissue bath containing modified Tyrode’s solution maintained at 37 °C. Under baseline tension of 1.0–1.15 gF the isolated tissues were allowed to equilibrate for 1–2 h before the addition of any substance. Experiments were performed on isolated tracheal smooth muscle preparations with or without intact epithelium. Isometric contractions were recorded through a force displacement transducer (Grass, FT-03, Quincy, MA, USA) coupled to an integrated organ bath system attached to a computer (WinDaq, version 1.65, DATAQ Instruments, Akron, OH, USA).
3.3.1. Effects of trans-Caryophyllene on Tracheal Basal Tone
In order to assess the effect of the trans-caryophyllene on tracheal basal tone, isolated tracheal rings with or without intact epithelium were exposed to increasing concentrations of trans-caryophyllene (0.0005–50 mM). The tracheal epithelium was mechanically removed by rubbing with a cotton bud and it was confirmed by measurement of contraction’s magnitude promoted by KCl 60 mM. Contractions above 1300 gF were considered without functional epithelium.
3.3.2. Effects of trans-Caryophyllene on the Contractions Induced by ACh and KCl in Isolated Trachea Maintained in Ca2+-Containing Medium
In this series of experiments, effects of non-cumulative increasing concentrations of trans-caryophyllene (0.005–50 mM) on the contractile responses to ACh (10 μM) and (0.3–50 mM) to K+ (80 mM) were studied in rat tracheal smooth muscle maintained in Ca2+-containing medium.
3.3.3. Effects of trans-Caryophyllene on ACh-Induced Contraction of Rat Isolated Trachea Maintained in Ca2+-Free Medium
Ca2+ availability from extracellular Ca2+ entry was indirectly evaluated by recording the contraction induced by ACh in Ca2+-free medium (containing 0.2 mM EGTA). After the equilibration period, ACh at 60 μM (a concentration able to promote contractions in Ca2+ free medium with amplitude large enough to allow good resolution) was added to the bath and produced a contraction that was established as control response. After washing preparation again with calcium free solution, trans-caryophyllene (10 mM) was added to the preparations. Afterwards, in the presence of trans-caryophyllene the preparation was challenged with ACh (60 μM). As there is a possibility of time-dependent decrease in the ACh elicited smooth muscle contraction we compared trans-caryophyllene effects with the response to a second application of ACh. In all experimental series external controls (tracheal ring strips exposed only to vehicle) were done.
3.4. Isolation of Single Tracheal Smooth Muscle Cells
A 15-cm segment of trachea was immediately removed and placed at room temperature in a low-Ca2+ physiological salt solution (PSS) in mM: 137 NaCl, 5.6 KCl, 0.44 NaH2PO4, 0.42 Na2HPO4, 4.17 NaHCO3, 3.55 MgCl2, 0.05 CaCl2, 10 HEPES and 5 glucose. The tracheal muscle was dissected away from the cartilage and minced with scalpel blades. Tracheal smooth muscle strips were divided and transferred to 3 mL of dissociation solution containing normal PSS (in mM): 137 NaCl, 5.6 KCl, 0.44 NaH2PO4, 0.42 Na2HPO4, 4.17 NaHCO3, 1 MgCl2, 2.6 CaCl2, 10 Hepes and 5 glucose, papain (0.9 mg/mL), BSA (1 mg/mL), and DTT (0.9 mg/mL). The strips were placed in a 37 °C water bath during 60 min and minced every seven-minute interval. After, tracheal smooth muscle strips were transferred to 3 mL of low-Ca2+ PSS supplemented with collagenase (1 mg/mL, type II), BSA (1 mg/mL) and hyaluronidase (0.9 mg/mL) for further digestion. The strips were placed in a 37 °C water bath during approximately 30 min and minced every seven-minute interval. All enzymes were obtained from Sigma Chemical Co. The solution was centrifuged at 1,500 revolutions/min for 1 min three times and washed twice with low-Ca2+ PSS. Afterwards, cells were resuspended in normal PSS and triturated with a pipette to release individual smooth muscle cells from the tissue. The solution containing the dissociated cells was poured onto glass coverslips, and the cells were allowed to adhere for 40–60 min at room temperature.
3.5. Membrane Current Recordings
The standard bath solution employed in the whole-cell voltage-clamp experiments contained the following composition (in mM): 130 NaCl, 20 BaCl2, 0.5 MgCl2, 10 HEPES and 5 glucose (pH 7.4 corrected with NaOH). Currents were compared in the presence and absence of trans-caryophyllene (3 mM). Pipettes were pulled from glass capillaries (Perfecta, São Paulo, SP, Brazil) with a micropipette puller (PP-830, Narishige, Tokyo, Japan). They had resistances of 2–4 MΩ (average 3.4 ± 0.3 MΩ) when filled with pipette solution (in mM: 130 CsCl, 10 TEA, 10 EGTA, 4 MgCl2, 10 Hepes and 4 Na2ATP). An Ag–AgCl wire was used as reference electrode.
An EPC-9 patch clamp amplifier (HEKA Instruments, Lambrecht/Pfalz, Germany) and pulse software were used to record whole-cell Ca2+ channel currents. Capacitive currents were compensated electronically and a P/4 protocol was used for linear leak and residual capacitance subtraction. Ca2+ currents were low-pass filtered at 3 kHz and sampled at 10 kHz. Patch clamp experiments were performed on 35-mm Petri dishes using an inverted microscope (Axiovert 20, Carl Zeiss, Göttingen, Germany). The bath was continuously perfused at 1–2 mL/min throughout the experiment. Solutions were gravity fed to the input ports of a solenoid valve mounted close to the bath, which was used to choose between one of two solutions.
Currents through high-voltage-activated (HVA) Ca2+ channels were evaluated using Ba2+ (I Ba) as the charge carrier. The currents were generated by 100 ms steps to 10 mV from a holding potential of −80 mV. To determine current–voltage relationships, cells were held at holding potential of −80 mV and subjected to step depolarizations of 100 ms from −70 to +60 mV in 10 mV increments every 10 s. Data were collected after the whole-cell configuration was obtained and current amplitude had stabilized, usually approximately 3 min after rupture of the cell membrane. Only cells with an input resistance >1 GΩ with no substantial rundown were analyzed.
3.6. Statistical Analysis
All values were presented as mean ± S.E.M., and statistical comparisons were made using the paired Student’s t test, one-way and two-way analysis of variance (ANOVA). p < 0.05 was considered to be significant.
4. Conclusions
In conclusion, we have clearly demonstrated that trans-caryophyllene has anti-spasmodic activity on trachealis muscle. We also demonstrated by means of direct electrophysiological measurements (using the patch-clamp method) that trans-caryophyllene-induced blockade of Ca2+ influx through voltage-dependent Ca2+ channels. The provided information that will certainly enrich the pharmacological profile of trans-caryophyllene, a substance that thus appears as a candidate worthy of more investigations envisaging its pharmacotherapeutic use.
Acknowledgments
The authors would like to thank CNPq, CAPES, FAPEMIG and FUNCAP for the financial support.
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Figure 1.
Effects of cumulatively increasing concentrations (0.0005–50 mM) of trans-caryophyllene on basal tonus of isolated rat tracheal preparations with (closed triangles; n = 6) or without (closed circles; n = 8) intact epithelium. Ordinate represents the force variation of basal tone (positive deflections means contraction and negative deflections means relaxation). EPT (+) and EPT (−) are preparations without and with epithelium removal, respectively. Symbols indicate means ± S.E.M.
Figure 1.
Effects of cumulatively increasing concentrations (0.0005–50 mM) of trans-caryophyllene on basal tonus of isolated rat tracheal preparations with (closed triangles; n = 6) or without (closed circles; n = 8) intact epithelium. Ordinate represents the force variation of basal tone (positive deflections means contraction and negative deflections means relaxation). EPT (+) and EPT (−) are preparations without and with epithelium removal, respectively. Symbols indicate means ± S.E.M.
Figure 2.
Representative experimental traces showing the relaxant effects of non-cumulatively increasing concentrations of trans-caryophyllene (0.3–50 mM) with (EPT(+), Ai; n = 5) and without (EPT(−), Aii; n = 4) intact epithelium on the high K+-induced contraction (K 80) of rat isolated tracheal smooth muscle. (B) Concentration-response curves of trans-caryophyllene-induced relaxation. Closed triangles represent segments with intact epithelium and open circles without intact epithelium. Symbols are means ± S.E.M.
Figure 2.
Representative experimental traces showing the relaxant effects of non-cumulatively increasing concentrations of trans-caryophyllene (0.3–50 mM) with (EPT(+), Ai; n = 5) and without (EPT(−), Aii; n = 4) intact epithelium on the high K+-induced contraction (K 80) of rat isolated tracheal smooth muscle. (B) Concentration-response curves of trans-caryophyllene-induced relaxation. Closed triangles represent segments with intact epithelium and open circles without intact epithelium. Symbols are means ± S.E.M.
Figure 3.
Representative experimental tracings showing the inhibitory effects of non-cumulative increasing concentrations (0.005–50 mM) of trans-caryophyllene on the ACh-induced contractions in rat isolated trachea with (EPT(+), Ai; n = 6) and without (EPT(−), Aii; n = 8) intact epithelium. Inverted triangles indicate drug application. (B) Concentration-response curves of the relaxant actions of trans-caryophyllene. Closed triangles represent segments with intact epithelium and closed circles without intact epithelium. Symbols are means ± S.E.M. (C) Average values for relative IC50.
Figure 3.
Representative experimental tracings showing the inhibitory effects of non-cumulative increasing concentrations (0.005–50 mM) of trans-caryophyllene on the ACh-induced contractions in rat isolated trachea with (EPT(+), Ai; n = 6) and without (EPT(−), Aii; n = 8) intact epithelium. Inverted triangles indicate drug application. (B) Concentration-response curves of the relaxant actions of trans-caryophyllene. Closed triangles represent segments with intact epithelium and closed circles without intact epithelium. Symbols are means ± S.E.M. (C) Average values for relative IC50.
Figure 4.
Effect of trans-caryophyllene on contractions induced by ACh on preparations maintained in Ca2+-free solution. (A) Examples of experimental traces obtained from segments where the epithelium is present (EPT(+), Ai) or absent (EPT(−), Aii). Open circles indicate ACh application at 60 µM. (B) Bar graphs showing average of contraction force. Black bars represent mean ± S.E.M. (n = 8) for segments containing intact epithelium. Open bars represent mean ± S.E.M. (n = 8) for segments without intact epithelium.
Figure 4.
Effect of trans-caryophyllene on contractions induced by ACh on preparations maintained in Ca2+-free solution. (A) Examples of experimental traces obtained from segments where the epithelium is present (EPT(+), Ai) or absent (EPT(−), Aii). Open circles indicate ACh application at 60 µM. (B) Bar graphs showing average of contraction force. Black bars represent mean ± S.E.M. (n = 8) for segments containing intact epithelium. Open bars represent mean ± S.E.M. (n = 8) for segments without intact epithelium.
Figure 5.
trans-Caryophyllene inhibited IBa in tracheal smooth muscle cells. (A) Effect of trans-caryophyllene (3 mM) on the IBa evoked by a depolarizing test pulse to 10 mV from a holding potential of −70 mV. The dotted line denotes zero current. (B) Time-course of IBa blockade caused by trans-caryophyllene. Data were normalized to maximum peak current. (C) Average IBa at control (black bar) and after addition of 3 mM trans-caryophyllene (gray bar). Bars represent means ± S.E.M, * p < 0.05. (D) Current-voltage relationships of IBa in the presence (closed inverted triangles) and absence (closed circles) of trans-caryophyllene. Error bars represent S.E.M.
Figure 5.
trans-Caryophyllene inhibited IBa in tracheal smooth muscle cells. (A) Effect of trans-caryophyllene (3 mM) on the IBa evoked by a depolarizing test pulse to 10 mV from a holding potential of −70 mV. The dotted line denotes zero current. (B) Time-course of IBa blockade caused by trans-caryophyllene. Data were normalized to maximum peak current. (C) Average IBa at control (black bar) and after addition of 3 mM trans-caryophyllene (gray bar). Bars represent means ± S.E.M, * p < 0.05. (D) Current-voltage relationships of IBa in the presence (closed inverted triangles) and absence (closed circles) of trans-caryophyllene. Error bars represent S.E.M.
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Pinho-da-Silva, L.; Mendes-Maia, P.V.; Teófilo, T.M.D.N.G.; Barbosa, R.; Ceccatto, V.M.; Coelho-de-Souza, A.N.; Santos Cruz, J.; Leal-Cardoso, J.H. trans-Caryophyllene, a Natural Sesquiterpene, Causes Tracheal Smooth Muscle Relaxation through Blockade of Voltage-Dependent Ca2+ Channels. Molecules 2012, 17, 11965-11977. https://doi.org/10.3390/molecules171011965
AMA Style
Pinho-da-Silva L, Mendes-Maia PV, Teófilo TMDNG, Barbosa R, Ceccatto VM, Coelho-de-Souza AN, Santos Cruz J, Leal-Cardoso JH. trans-Caryophyllene, a Natural Sesquiterpene, Causes Tracheal Smooth Muscle Relaxation through Blockade of Voltage-Dependent Ca2+ Channels. Molecules. 2012; 17(10):11965-11977. https://doi.org/10.3390/molecules171011965
Chicago/Turabian StylePinho-da-Silva, Leidiane, Paula Virgínia Mendes-Maia, Taylena Maria Do Nascimento Garcia Teófilo, Roseli Barbosa, Vania Marilande Ceccatto, Andrelina Noronha Coelho-de-Souza, Jader Santos Cruz, and José Henrique Leal-Cardoso. 2012. "trans-Caryophyllene, a Natural Sesquiterpene, Causes Tracheal Smooth Muscle Relaxation through Blockade of Voltage-Dependent Ca2+ Channels" Molecules 17, no. 10: 11965-11977. https://doi.org/10.3390/molecules171011965
APA StylePinho-da-Silva, L., Mendes-Maia, P. V., Teófilo, T. M. D. N. G., Barbosa, R., Ceccatto, V. M., Coelho-de-Souza, A. N., Santos Cruz, J., & Leal-Cardoso, J. H. (2012). trans-Caryophyllene, a Natural Sesquiterpene, Causes Tracheal Smooth Muscle Relaxation through Blockade of Voltage-Dependent Ca2+ Channels. Molecules, 17(10), 11965-11977. https://doi.org/10.3390/molecules171011965
