Centaurium Erythraea Extracts Exert Vascular Effects through Endothelium- and Fibroblast-dependent Pathways

• Abstract
• Introduction
• Results
• Discussion
• Materials and Methods
• Plant material
• Extraction
• In vitro DPPH• antioxidant assay
• Animals
• Isolated MVB experiments
• NO determination
• Fibroblast culture and MTT cell viability assay
• HPLC-DAD analysis of phenolic compounds
• Chemicals and drugs
• Statistical analysis
• References

Abstract

Centaurium erythraea is a plant used in traditional medicine for several cardiovascular disorders, namely hypertension, but there is no scientific evidence able to provide a molecular basis for its claimed antihypertensive effects. After a preliminary screen of extracts obtained from sequential extraction of C. erythraea aerial parts, effects of the methanolic fraction (MFCE) on changes in perfusion pressure of isolated rat mesenteric vascular bed (MVB) and in rat cardiac fibroblasts proliferation were investigated, gathering information on the mechanisms involved in endothelium-dependent effects and their dependence on a pro-proliferative stimulus. The HPLC-DAD determination of the phenolics content of MFCE revealed the presence of 22 phenolic compounds. MFCE reduced (63.3 ± 3.9%; n = 4) perfusion pressure in MVB and almost completely abrogated the Ang II-induced increase in cardiac fibroblasts proliferation. Reduction of the perfusion pressure caused by MFCE was endothelium-dependent and occurred in parallel with an increase in NO release. These effects were inhibited by muscarinic receptor antagonists, by L-NAME (a NO synthase inhibitor), and by ODQ (a soluble guanylate cyclase inhibitor). Experiments revealed that effects required the involvement of K⁺ channels, being inhibited by tetraethylamonium (TEA; a Ca²⁺ activated K⁺ channels inhibitor) and by glibenclamide (an ATP-sensitive K⁺ channels inhibitor). In conclusion, extracts from C. erythraea, particularly the compounds present in the MFCE, induce endothelium-dependent vasodilation and prevent fibroblast proliferation induced by angiotensin II, which can account for the claimed antihypertensive effects of C. erythraea in traditional medicine.

Introduction

Centaurium erythraea Rafn. (C. erythraea), commonly known as “centaury,” is a shrub species, belonging to the Gentianaceae family. This native plant is widely distributed in the Mediterranean region, where it is one of the most widely used in traditional medicine. According to several ethnopharmacologic surveys, C. erythraea is used for the treatment of digestive, [1] renal, hepatic, respiratory, and rheumatic diseases [2]. It is also taken as an antidiabetic agent [3] and to treat cardiovascular diseases, namely hypertension [3], [4], [5], [6].

In vitro and in vivo studies support some of these traditional uses: extracts of C. erythraea were shown to possess antispasmodic [7], antioxidant [8], diuretic [9], gastroprotective [10], and antidiabetic properties [11]. Recently, it has also been shown that C. erythraea methanolic extract protects red blood cells from oxidative damage in diabetic rats [12].

In spite of the relevance of the use of extracts of C. erythraea in hypertension, the molecular mechanisms of its antihypertensive effects remain to be elucidated. Its clarification is crucial not only to understand the effectiveness of the consumption of these extracts but also to understand the risks associated with their use. The present study aimed at improving the knowledge about the mechanism of action of C. erythraea extracts in the vascular system, proceeding a line of investigation that demonstrated smooth muscle relaxant effects of the aqueous extract in the isolated rabbit jejunum [7]. Therefore, after a more general screening measuring the scavenging activity and vasorelaxation caused by different extracts obtained from the sequential extraction of C. erythraea aerial parts, the most active one (methanolic extract) was studied with more detail. Its composition was characterized and its effects on endothelium-dependent relaxation (a mechanism of short-term control of vascular function) and on fibroblast proliferation (a mechanism of medium- and long-term control of cardiac and vascular wall remodeling) were investigated.

Results

In order to identify which extract had a more pronounced scavenging activity, the hexane fraction (HFCE), the dichloromethane fraction (DFCE), the ethyl acetate fraction (EAFCE), the methanolic fraction (MFCE), and the aqueous fraction (AqFCE) from sequential extraction of C. erythraea aerial parts were tested using the DPPH · radical scavenging assay. Ascorbic acid (0.1 – 10 mg/mL) was used as positive control which presented an IC₅₀ value of 0.11 mg/mL (0.10 – 0.12 mg/mL; n = 4)

With the exception of HFCE, all extracts showed scavenging activity, which was concentration-dependent. Within the concentration range tested, MFCE was able to reach a maximum of scavenging activity identical to that caused by ascorbic acid ([Fig. 1]). MFCE was also shown to be the most potent: the IC₅₀ values of MFCE were (mg/mL): 0.67 (0.60 – 0.76) followed by EAFCE, DFCE, and AqFCE [1.39 (1.22 – 1.58), 2.25 (1.96 – 2.59), and 3.2 (2.58– 3.96)], respectively (n = 4).

An augmented production of oxygen free radicals can determine endothelium dysfunction and diminish its ability to induce relaxation of vascular smooth muscle cells [9]. To investigate whether the extracts that presented radical scavenging activity also influenced vascular reactivity, they were tested in doses ranging from 0.03 to 3.0 mg, on MVB preparations with preserved endothelium (confirmed by administration of a bolus of 5.5 nmol acetylcholine; see Methods), precontracted with phenylephrine (10 – 20 µM) to induce a plateau value of perfusion pressure of 80 – 100 mmHg. A reduction of perfusion pressure below this plateau value caused by the experimental treatments was assumed to reflect a vasorelaxation.

Only the DFCE failed to decrease perfusion pressure (PP; [Fig. 2 B]). In terms of the potency to reduce perfusion pressure, the MFCE caused the most pronounced effect (63.3 ± 3.9%; n = 4). The highest decrease in perfusion pressure caused by MFCE was followed by that caused by EAFCE (52.7 ± 2.6%; n = 4) and by the AqFCE (35.0 ± 4.0%; n = 4). [Fig. 2 A] show the typical trace of MFCE, the fraction that caused the most pronounced effect.

Since the methanolic extract (MFCE) caused the most potent vasorelaxation and radical scavenging activities, it was chosen to study, in more detail, the mechanisms involved. To investigate the endothelium-dependence of the vasorelaxation, experiments were performed in endothelium-denuded preparations (obtained by perfusing MVB with distilled water for 5 – 6 min). Removal of endothelium was confirmed by the lack of vasorelaxation caused by the bolus of 5.5 nmol acetylcholine, administered after reaching the plateau value of perfusion pressure induced by phenylephrine (see Methods). Integrity of smooth muscle was confirmed by evaluating the vasorelaxation induced by 10 nmol SNP, which was not different from that caused in endothelium preserved preparations (70.0 ± 3.2% vs. 76.0 ± 4.2%, respectively; n = 5). However, the vasorelaxation caused by all doses of MFCE was lost in endothelium-denuded preparations ([Fig. 3]).

In order to elucidate which endothelium derived factors are involved in the vasorelaxation induced by MFCE, experiments were conducted in the presence of 100 µM L-NAME, an arginine analog known to inhibit NO synthase, 1 µM ODQ, an inhibitor of soluble guanylate cyclase, or 10 µM indomethacin, a cyclooxygenase inhibitor. As shown in [Fig. 4], pretreatment with 100 µM L-NAME diminished the vasorelaxation caused by MFCE from 67.8 ± 3.0%; n = 8 (control conditions) to 29.5 ± 4.5%; n = 4 (p < 0.05). Pretreatment with 1 µM ODQ also diminished the maximal vasorelaxation of MFCE to 27.7 ± 0.8%; n = 4 (p < 0.05) whereas 10 µM indomethacin did not alter significantly MFCE induced vasorelaxation.

Quantification of nitrite formation, an oxidation product of the interaction of NO with the molecular oxygen and water, was used to further monitor NO synthesis. Very low levels of nitrite were detected in the perfusate obtained from MVB precontracted with phenylephrine in the absence of MFCE (1.38 ± 0.08 µM; n = 6). Under continuous infusion with 0.3 mg/mL of MFCE, an increase of about 5-fold in nitrite levels was detected in the perfusate of MVB precontracted with phenyelephrine, reaching 7.19 ± 0.13 µM (n = 6; p < 0.01, from phenylephrine alone). This increase in nitrate levels was reduced about 57% when MVB was perfused with MFCE in the presence of 100 µM L-NAME: 3.09 ± 0.23 µM (n = 6; p < 0.01, from MFCE alone).

Additional evidence for an increase in NO formation induced by MFCE was obtained in experiments carried out in breast cancer MCF-7 cells using DAF-FM DA (a highly sensitive and selective fluorescent NO probe). Representative images of cells submitted to the different treatments are shown in SI (Fig. 2S, panel A). MFCE caused a marked increase in DAF-FM DA fluorescence. This increase in fluorescence was dependent on the concentration of MFCE used (0.3 – 1.0 mg/mL) and was prevented when cells were incubated with 500 µM L-NAME, an inhibitor of nitric oxide synthase. The average values of a series of 4 independent experiments (total 24 measurements) are shown in SI (Fig 2S, panel B). This observation corroborates the hypothesis that MFCE induces nitric oxide production.

To investigate the involvement of K⁺channels in MVB vasorelaxation induced by MFCE, experiments were performed on preparations precontracted with 100 mM K⁺ (high K⁺). High K⁺ increased perfusion pressure to 94.0 ± 7.4 mmHg (n = 4), a value identical to that induced by phenylephrine (96.0 ± 4.2 mmHg; n = 4). However, relaxation caused by MFCE on MVB preparations was much lower on preparations precontracted with high K⁺ than on preparations precontracted with phenylephrine for all MFCE doses tested ([Fig. 5]). The highest dose of MFCE reduced perfusion pressure only 14.2 ± 1.9% (n = 4).

To identify the type of K⁺ channels involved on MFCE-induced vasorelaxation, TEA, BaCl₂, and glibenclamide, inhibitors of Ca²⁺ activated K⁺ channels, inwardly rectifying K⁺ channels, and ATP sensitive K⁺ channels inhibitor, respectively, were tested in endothelium-intact MVB preparations precontracted with phenylephrine.

As shown in [Fig. 6], 10 mM TEA and 1 µM glibenclamide, but not 100 mM BaCl₂, reduced the relaxation caused by MFCE. The maximal vasorelaxation induced by 3 mg MFCE was reduced by 10 mM TEA and 1 µM glibenclamide: from 66.9 ± 2.5% (n = 8) (solvent) to 14.5 ± 2.5% (n = 4) and to 38.6 ± 2.0% (n = 4), respectively (p < 0.05; see [Fig. 6]).

To examine the putative involvement of cholinergic mechanisms in the vasorelaxation caused by MFCE, the effect of the highest doses of MFCE was examined in the presence of atropine, a muscarinic receptor antagonist. As shown in [Fig. 7], 1 µM atropine prevented the reduction of perfusion pressure caused by 5.5 nmol acetylcholine. It also prevented reduction in perfusion pressure caused by 1 and 3 mg MFCE. Under the same experimental conditions, responses to 10 nmol SNP (as an exogenous donor of NO) were not altered.

The involvement of muscarinic receptors in the effects of MFCE was confirmed in experiments carried out in isolated ileum, a classical model to study muscarinic responses. Carbachol (7.5 nM to 25 µM) was used as a selective muscarinic-receptor agonist and caused concentration-dependent contractions that were blocked by the muscarinic receptor antagonists 1 µM atropine or 1 µM AQ-RA 741 (Supplementary material: Fig. 1S, panel A). Similar effects to 1 µM atropine or 1 µM AQ-RA 741 were obtained on the contractions caused by MFCE (0.015 – 1.0 mg/mL) (Supporting Information, Fig. 1S, panel B).

Considering the described contribution of fibroblast proliferation to cardiovascular diseases, the effect of MFCE was tested on primary cultures of rat cardiac fibroblasts. When tested alone, MFCE (0.01 – 1.0 mg/mL) failed to alter fibroblast proliferation (3 independent experiments, data not shown). However, when cardiac fibroblasts were treated with 0.1 µM angiotensin II, a known inducer of fibroblast proliferation, MFCE almost completely abrogated the Ang II-induced increase in cell proliferation ([Fig. 8]).

The analysis by HPLC-DAD allowed the identification of 22 phenolic compounds in MFCE, comprising quercetin, kaempferol, and isorhamnetin derivatives, most of them being acylated with hydroxycinnamic acids ([Fig. 9] and [Table 1]). The identification of these compounds was carried out by comparing chromatographic behavior with the results recently published by our group, using the same plant material, in which HPLC–DAD–ESI (IonTrap)/MSⁿ was used [10].

The quantification of MFCE compounds was carried out using external calibration curves resulting from 7 concentrations of the following standards: quercetin-3-O-rutinoside (y = 46 534 x; R² = 0.9996; limit of detection [LOD] = 6.10 × 10⁻⁴ mg/mL; limit of quantification [LOQ] = 1.85 × 10⁻⁴ mg/mL), kaempferol-3-O-rutinoside (y = 60 151 x; R² = 0.9994; LOD = 3.00 × 10⁻⁴ mg/mL; LOQ = 9.10 × 10⁻⁴ mg/mL) and isorhamnetin-3-O-rutinoside (y = 52 524 x; R² = 0.9995; LOD = 5.20 × 10⁻⁴ mg/mL; LOQ = 1.57 × 10⁻³ mg/mL). Under the chromatographic conditions described above, the calibration plots showed a good correlation. Concentrations ranging from 0.129 to 17.923 mg/g were found in this extract ([Table 1]). Phenolic compounds were mainly represented by kaempferol derivatives (47.5% of determined phenolic compounds), followed by quercetin heterosides (46.1%). The most abundant compounds in these 2 groups were kaempferol-3-O-(p-coumaroyl, rhamnosyl)rutinoside-7-O-rhamnoside (14) and quercetin-3-O-(rhamnosyl)rutinoside-7-O-(p-coumaroyl)rhamnoside (11), which represent 23.3% and 18.1% of the total phenolics content, respectively. Isorhamnetin-3-O-(p-coumaroyl, rhamnosyl)rutinoside-7-O-rhamnoside (15) was the only isorhamnetin derivative identified, accounting for 6.4% of the total phenolics content ([Table 1]).

Discussion

C. erythraea is used in traditional medicine to treat cardiovascular diseases, namely hypertension [3], [4], [5], [6]. To the best of our knowledge, this is the first study that aimed to investigate the effects of C. erythraea extracts on the cardiovascular system. The purpose is to gather scientific evidence to better understand the real efficacy and safety of their use in traditional medicine. The main focus of the present study was to evaluate the capacity of extracts (i) to reduce oxidative stress, by measuring its radical scavenging activity; (ii) to potentiate endothelium dependent control of vascular resistance, by measuring endothelium dependent relaxation and (iii) to interfere with cardiovascular remodeling, by investigating their capacity to modulate fibroblast proliferation.

Several in vitro and epidemiological studies suggested an important role of herbal medicine extracts rich in polyphenols to preserve vascular health and to prevent cardiovascular diseases [13]. The oxidative stress results from a cellular imbalance between the effect of pro and antioxidants, in favor of the first, being considered as a factor that contributes to the atherogenic process [14]. Previous studies have shown that extracts from C. erythraea present antioxidant effects [15] using DPPH^•, 2,2-azinobis (3-ethyl-benzothiazoline-6-sulphonic acid ammonium salt; ABTS), and/or FRAP method. In addition to in vitro data, it was showed that C. erythraea also prevents oxidative stress on experimentally diabetic rats [12]. The results from the present study provide additional information about the nature of antioxidant effect of C. erythraea extracts, showing that scavenging activity was absent to moderate for the extracts with low and average polarity but important with polar methanolic extract (MFCE). The scavenging effect displayed by C. erythraea extracts could be a promising therapeutic agent to treat oxidative stress induced by pathological conditions.

To explore the vasoreactivity of bioactive extracts identified in the DPPH^• assay, endothelium-intact MVBs were precontracted with phenylephrine, a α₁-adrenoceptor agonist. In the presence of this contracting agent, MFCE, EAFCE, and AqFCE induced dose-dependent relaxation. Interestingly, MFCE-induced vasorelaxation was more potent than that induced by EAFCE and AqFCE. Considering this difference between MFCE and other extracts, and in order to diminish the number of animals used, only the MFCE mechanism for inducement of vasorelaxant activity was studied in more detail.

The use of antioxidant therapy has been considered a valid approach to improve vascular function in case of coronary artery disease, stroke, peripheral vascular disease, hypertension, and heart failure [16], [17]. Multiple mechanisms may be involved and mediate an improvement of the endothelium-dependent vasodilation [14] and an involvement of endothelium-dependent mechanisms on the reduction of perfusion pressure caused by MFCE extract is one of the major findings of the present study.

Endothelial control of vascular tone is achieved via synthesis and/or release of a wide range of biochemical mediators, namely EDRFs and endothelium-derived contracting factors [18]. Endothelium-dependent vasodilation is believed to be achieved by 3 main EDRFs: NO, EDHF, and prostacyclin [18], [19]. The present results support the involvement of NO and a probable contribution of EDHF in the vasorelaxation caused by the C. erythraea extract.

NO is a gaseous mediator that, in endothelial cells, is produced by a Ca²⁺-dependent constitutive isoform of NO synthase. Responses of vascular smooth muscle to NO are mainly mediated by the heme-containing soluble guanylate cyclase, causing an increase in cGMP levels, activation of protein kinase G, and reduction in intracellular free Ca²⁺ levels, leading to dilation of blood vessels [19]. The present study showed that MFCE may stimulate NO formation and the vasorelaxation be caused by activation of the NO-cGMP pathway, as it was inhibited by L-NAME, an inhibitor of NO synthase, and by ODQ, an inhibitor of guanylate cyclase. Taken together these results reveal a capacity of extracts of C. erythraea to induce NO release.

Mechanisms other than NO release may be involved in the endothelium-dependent vasodilation caused by C. erythraea extracts. The evidence presented in our study points to the involvement of EDHF. Release EDHF depends on activation of K⁺channels [19] and the results of the present study points to a K⁺ dependence of vascular relaxation caused by MFCE: relaxation was prevented when the equilibrium potential of K⁺ (high K⁺ conditions) is close to the membrane potential, by reducing the electrochemical gradient for K⁺ efflux and thus preventing relaxation mediated by opening of K⁺ channels [20]. Furthermore, relaxation seems to be mediated, at least in part, by increasing K⁺ efflux through K_ATP and K_Ca channels, according to the inhibition of this effect caused by glibenclamide (a K_ATP channel inhibitor) and tetraethylammonium (a K_Ca channel inhibitor).

The vasorelaxation caused by C. erythraea may involve activation of muscarinic receptors, which is one of the first and best known mechanisms to induce release of EDRFs [21]. The present study confirms that MFCE presents a cholinomimetic effect, and the induced vasorelaxation is secondary to activation of endothelial muscarinic receptors since it was blocked by different muscarinic receptor antagonists. The mechanisms that may be, directly or indirectly, involved in the vasodilation caused by MFCE are depicted in [Fig. 10].

In addition to the well-known effect of the endothelium in the genesis of cardiovascular diseases, a role of fibroblasts is also established [22]. In hypertension, vascular changes are the result of tissue remodeling in which adventitious fibroblasts increase production of collagen, and increase wall thickness and vasoconstriction [23], [24]. These changes are also directly implicated in ventricular fibrosis [25]. Angiotensin II is a messenger that has been implicated in inducing proliferation of fibroblasts [26], and blockade of this pro-proliferative effect is assumed to be one of the mechanisms that can explain the cardiovascular therapeutic effects of angiotensin converting enzyme inhibitors [23], [26] and of antagonists of AT₁ receptors [27]. In the present study, the MFCE extract inhibited fibroblast proliferation induced by angiotensin II, mimicking what would be expected from blockade of angiotensin II effects. Such observation suggests that, in addition to influencing endothelial function by preserving the endothelium vasodilatory function, C. erythraea contains compounds that may inhibit wall remodeling of the cardiovascular system, thus constituting an additional target to prevent or to treat hypertension.

Extracts have, in general, a complex composition. The qualitative profile of MFCE is identical to the one reported by Kachmar et al. [28] although quantitative differences were noticed, MFCE being richer than the aqueous extract of C. erythraea aerial parts ([Table 1]). From the 22 flavonoid derivatives identified in MFCE, most of them were acylated with hydroxycinammic acids (3, 4, 6–22) ([Table 1]). Quercetin, kaempferol, and isorhamnetin derivatives were also identified by comparing their UV spectra and chromatographic behavior with the results recently published by Kachmar and colleagues [10] for the aqueous extract of the same plant material using the same chromatographic conditions. With such high number of compounds present in the extract and having in mind that biological effects observed may be caused the additive or synergic effects, the attempt to identify which compounds are contributing for the observed biological effects is unfeasible. Evidence from the literature may point to relevant contributions of some compounds detected. For example, quercetin and isorhamnetin were reported to reduce oxidative stress and to improve NO bioavailability, leading to the attenuation of endothelial dysfunction [29], [30], [31], [32], [33], and kaempferol is known to have a relaxation effect on agonist-induced vascular contraction regardless of endothelial function [34], [35]. In addition, hydroxycinnamic acids, such as p-coumaric and caffeic acids, are known to exhibit vasorelaxant and antioxidant effects [36], [37].

In conclusion, C. erythraea extracts may alter vascular function by inducing endothelium-dependent vasodilation and preventing cardiac fibroblast proliferation. Since both effects have an impact on short and long-term vascular resistance and vessel wall remodeling, these may contribute to the claimed antihypertensive effects of C. erythraea in traditional medicine.

Materials and Methods

Plant material

C. erythraea was collected at north Morocco (Taounate) between May and June 2017 and stored at room temperature in a dry place prior to use. The plant was identified (Amina Bari, Department of Biology, FSDM, University Sidi Mohamed Ben Abdellah, Fez, Maroc) and registered with the specimen number MA-FSTF 14, at the Faculty of Science and Technique (Fez, Morocco). Aerial parts (leaves and flowers) were dried protected from light.

Extraction

Dried aerial parts were ground into a fine powder. Fifty grams of this powder was sequentially extracted with 300 mL of hexane, dichloromethane, ethyl acetate, methanol, and water, using a Soxhlet extractor. The sequential extraction yields were 2.5%, 2.9%, 3.7%, 24.4%, and 3.1% for HFCE, DFCE, ethyl acetate (EAFCE), methanol (MFCE), and water extracts (AqFCE), respectively. These fractions were dried and stored at 4 °C, protected from light. Dry extracts were prepared in order to assure that no trace of organic solvents was detected in the highest concentration of extract used.

In vitro DPPH^• antioxidant assay

The DPPH^• (2,2-diphenyl-1-picryl hydrazyl radical) scavenging assay was carried out as described previously [38]. Briefly, 100 µL of each dissolved extract, in concentrations of 0.1, 0.2, 0.5, 1.0, 2.0, 5.0, or 10 mg/mL, were added to 400 µL of 0.5 mM DPPH^•. Thereafter, 1.5 mL of methanol was added and, after a 30 min incubation, absorbances were read at 517 nm. The IC₅₀ values (dose required to reduce DPPH^• absorbance by 50%) were calculated using nonlinear regression analysis. Ascorbic acid was used as reference antioxidant (positive control). The radical scavenging activity of extracts was estimated by calculating the absorbances ratios in the presence and in the absence of extracts and expressed as percentage of the maximal effect of ascorbic acid.

Animals

Male and female Wistar rats (250 – 350 g; Charles River) were used for all experiments. The animals were housed in appropriate facilities of the Institute of Biomedical Sciences of University of Porto or the Faculty of Sciences and Techniques, University Sidi Mohamed Ben Abdellah, at ambient temperature of 25 ± 2 °C. Animals had free access to food and tap water ad libitum. The present study was performed according to the guidelines of the European Communities Council Directive (86/609/EEC) and has received the Ethics Committee authorization with the reference number N^o 255/2018/ORBEA (ORBEA: Organismo Regulador do Bem-Estar Animal; the local organism that regulates experimental animal welfare), March 8, 2019.

Isolated MVB experiments

The MVB was removed from Wistar rats (male or female; 300 – 400 g) as previously described [39]. Rats were anesthetized with sodium pentobarbital (50 mg/kg, i. p.). After opening the abdominal cavity, the superior mesenteric artery was rapidly cannulated with a heparinized hypodermic needle at its origin from the abdominal aorta and immediately flushed with warm Krebs-Henseleit solution (KHS). The whole MVB was separated from the intestine by cutting close to the intestinal border and placed into a Petri dish. Once the MVB was isolated, KHS, at 37 °C, was pumped into the MVB using a peristaltic pump (Pharmacia Biotech) at a continuous constant flow of 2 mL/min. The MVB perfusion pressure was continuously measured using a pressure transducer (Capto SP844) and recorded on a universal oscillograph (50 – 8622, Harvard Apparatus Limited). The KHS had the following composition (mM): NaCl 118, NaHCO₃ 25, KCl 4.7, MgSO₄ 1.2, CaCl₂ 2.5, KH₂PO₄ 1.2, and glucose 11.0; it was continuously oxygenated (95% O₂, 5% CO₂; final pH 7.4).

After 60 min equilibration, the preparation was constricted by infusion of phenylephrine (10 – 20 µM), via a sidearm of the inflow of the perfusate, using a pump syringe (M365, Orion). The concentration of phenylephrine reached in the KHS was adjusted in every experiment in order to induce a stable perfusion pressure of 80 – 100 mmHg, as previously described [40]. An increase in perfusion pressure was interpreted as a vasoconstriction and expressed as the absolute increase in pressure (mmHg) above the baseline and a decrease in perfusion pressure of precontracted tissue preparations interpreted as a vasodilation. Drug-induced relaxation is expressed as a percentage of the decrease in perfusion pressure, assuming 100% relaxation a return to precontraction values.

In some experiments, endothelium was removed from the MVB, using the following protocol: following a return to resting conditions after the initial control responses had been obtained, distilled water was included in the perfusion stream for 5 – 6 min to remove the endothelium from the MVB, followed by a stabilization period of 30 – 40 min, as previously described [41], [42]. The presence of functional endothelium was confirmed by the ability of a bolus of acetylcholine (5.5 nmol) to induce more than 60% relaxation of vessels precontracted with phenylephrine. The absence of a relaxation response to acetylcholine was taken as evidence that MVBs were functionally denuded from endothelium. After a preliminary screen of each fraction, only the methanolic fraction of C. erythraea (MFCE) was studied in more detail. For the dose-response curve to MFCE (0.03, 0.1, 0.3, 1.0, and 3.0 mg), extract was administered by bolus injection of 10 µL to 100 µL into the perfusion stream close to the superior mesenteric artery canula, and its effects were measured in vessels precontracted with phenylephrine, with and without endothelium. In the experiments designed to investigate the molecular mechanisms of the vasodilation, drugs were added 20 min prior to phenylephrine, as indicated.

NO determination

The presence of NO in the MVB perfusate was determined by measuring the amount of nitrites. Nitrite determination was performed in MVB perfused with KHS containing phenylephrine, in the absence or in the presence MFCE (0.3 mg/mL), alone and in the presence of 100 µM L-NAME. In order to obtain detectable nitrite levels, samples of perfusate (6 mL) were collected at a flow rate of 2 mL/min. Nitrites were quantified using the Griess reagent (1% sulfanilamide, 0.1% napthylethylenediamine, 2.5% ortophosphoric acid) [43]. Briefly, Griess reagent (6 mL) was mixed with an equal volume of perfusate (6 mL), and optical density was determined at 550 nm, after a 10-min incubation period. For the quantification of the nitrites present in the perfusate, a calibration curve was constructed using known concentrations (1 – 50 µM) of sodium nitrite.

Fibroblast culture and MTT cell viability assay

Cells obtained from primary cultures of rat cardiac fibroblasts were kindly provided by Professor Paulo Correia-de-Sá (Laboratory of Pharmacology, ICBAS, University of Porto) and prepared accordingly [44], being cultured in DMEM (Sigma), supplemented with 15% (v/v) inactivated FBS (Sigma) and 1% (v/v) penicillin-streptomycin/amphotericin B solution. Cells were seeded in 96-well plates, at a density 3 × 10⁴ cells/mL, in a final volume 100 µL of DMEM supplemented with 15% FBS and 1% penicillin-streptomycin/amphotericin B. Cells were incubated for 96 h, at 5% CO₂ at 37 °C, in the absence or in the presence of MFCE (0.3 and 1 mg/mL), with or without angiotensin II (0.1 µM).

Cell viability was measured by a colorimetric assay with MTT, as described previously [45]. In brief, at the end of the incubation period, medium was removed and 100 µL of a MTT solution in PBS (0.5 mg/mL) was added to each well, and kept in the same incubation conditions (at 37 °C and 5% CO2) for 4 h, protected from the light. Thereafter, supernatants were aspired and 100 µL DMSO added to each well to dissolve the formazan crystals that resulted from MTT reduction. The quantity of formazan produced (an indicator of the number of viable cells) is measured by changes in absorbance at 570 nm, using a 96 well microplate reader (Sinergy HT, Biotek Instrumensts Inc).

HPLC-DAD analysis of phenolic compounds

The dried residue of MFCE was re-dissolved in methanol and filtered through a 0.45 µm size pore membrane (Millipore). Thereafter, 20 µL of re-dissolved extract was analyzed in a HPLC-DAD unit (Gilson), using a Kinetex column (5 µm, C18, 100 A, 150 × 4.6 mm; Phenomenex), following the conditions described before [10]. The mobile phase consisted of 2 phases: water-formic acid (1%) (Phase A) and acetonitrile (Phase B), starting with 15% B and using a gradient to obtain 20% B at 15 min, 25% B at 25 min, 30% B at 35 min, and 60% B at 45 min, at a flow rate of 0.5 mL/min. Detection was achieved with a Gilson diode array detector. Spectral data from all peaks were collected in the range of 200 – 400 nm and chromatograms were recorded at 330 nm. The data were processed on a Clarity Software system. Peak purity was checked by the software contrast facilities. Phenolic compounds quantification was achieved by interpolation with external standard calibration curves. Since standards of all identified compounds are not commercially available, quercetin derivatives were quantified as quercetin-3-O-rutinoside, isorhamnetin derivatives as isorhamnetin-3-O-rutinoside, and kaempferol derivatives as kaempferol-3-O-rutinoside. The LOD and the LOQ were calculated from the residual standard deviation of the linear regression (SD), following the equations: LOD = 3.3 × SD and LOQ = 10 × SD.

Chemicals and drugs

All solutions were prepared daily and kept on ice until used. Carbachol, acetylcholine chloride, L-NAME, phenylephrine, TEA, barium chloride (BaCl₂), angiotensin II, and atropine were dissolved in distilled water. Indomethacin was dissolved in 150 mM NaHCO₃. Glibenclamide, AQ-RA 741, and ODQ were dissolved in dimethyl sulfoxide (DMSO). The final concentration of DMSO used in the present study did not exceed 0.05%, which was proven to have no effect per se on the basal tonus of the preparations or on the effects of the drugs tested.

DMEM, FBS, and L-glutamine were purchased from Merck-Millipore (BioTecnómica). Quercetin-3-O-rutinoside, kaempferol-3-O-rutinoside and isorhamnetin-3-O-rutinoside were from Extrasynthèse. All other drugs and solvents were purchased from Sigma-Aldrich. All reagents used in this study were of the highest available analytic grade (purity ≥ 98%).

Statistical analysis

Statistical analysis and nonlinear regression analysis were carried out using GraphPad Prism 6.00 software. Results are presented as mean ± standard error of the mean (SEM) of, at least, 4 independent experiments expressed as a percentage of the respective control. IC₅₀ values were calculated using nonlinear regression analysis and presented as geometric means and 95% confidence intervals. Comparisons between groups were performed by analysis of variance test for repeated measurements (2-way analysis of variance [ANOVA]), followed by the multiple comparison Bonferroniʼs t-test. Comparisons between 2 means were performed by Studentʼs t-test. Differences were considered statistically significant at p < 0.05.

Conflict of Interest

The authors declare that they have no conflict of interest.

• References

• 1 Merzouki A, Ed-derfoufi F, Molero Mesa J. Contribution to the knowledge of Rifian traditional medicine. II: folk medicine in Ksar Lakbir district (NW Morocco). Fitoterapia 2000; 71: 278-307
  CrossrefPubMedGoogle Scholar
• 2 Bouyahya A, Abrini J, Et-Touys A, Bakri Y, Dakka N. Indigenous knowledge of the use of medicinal plants in the north-west of Morocco and their biological activities. Eur J Integr Med 2017; 13: 9-25
  CrossrefPubMedGoogle Scholar
• 3 Bnouham M, Mekhfi H, Legssyer A, Ziyyat A. Medicinal plants used in the treatment of diabetes in Morocco. Int J Diabetes Metab 2002; 10: 33-50
  PubMedGoogle Scholar
• 4 Bellakhdar J, Claisse R, Fleurentin J, Younos C. Repertory of standard herbal drugs in the Moroccan pharmacopoea. J Ethnopharmacol 1991; 35: 123-143
  CrossrefPubMedGoogle Scholar
• 5 Uncini Manganelli RE, Chericoni S, Baragatti B. Ethnopharmacobotany in Tuscany: plants used as antihypertensives. Fitoterapia 2000; 71: S95-S100
  CrossrefPubMedGoogle Scholar
• 6 Calvo MI, Cavero RY. Medicinal plants used for cardiovascular diseases in Navarra and their validation from official sources. J Ethnopharmacol 2014; 157: 268-273
  CrossrefPubMedGoogle Scholar
• 7 Chda A, Kabbaoui M, Chokri A, Abida K, Tazi A, Bencheikh R. Spasmolytic action of Centaurium erythraea on rabbit jejunum is through calcium channel blockade and NO release. European J Med Plants 2016; 11: 1-13
  PubMedGoogle Scholar
• 8 Valentão P, Fernandes E, Carvalho F, Andrade PB, Seabra RM, Bastos ML. Antioxidant activity of Centaurium erythraea infusion evidenced by its superoxide radical scavenging and xanthine oxidase inhibitory activity. J Agric Food Chem 2001; 49: 3476-3479
  CrossrefPubMedGoogle Scholar
• 9 Haloui M, Louedec L, Michel JB, Lyoussi B. Experimental diuretic effects of Rosmarinus officinalis and Centaurium erythraea . J Ethnopharmacol 2000; 71: 465-472
  CrossrefPubMedGoogle Scholar
• 10 Tuluce Y, Ozkol H, Koyuncu I, Ine H. Gastroprotective effect of small centaury (Centaurium erythraea L) on aspirin-induced gastric damage in rats. Toxicol Ind Health 2011; 27: 760-768
  CrossrefPubMedGoogle Scholar
• 11 Sefi M, Fetoui H, Lachkar N, Tahraoui A, Lyoussi B, Boudawara T, Zeghal N. Centaurium erythrea (Gentianaceae) leaf extract alleviates streptozotocin-induced oxidative stress and β-cell damage in rat pancreas. J Ethnopharmacol 2011; 135: 243-250
  CrossrefPubMedGoogle Scholar
• 12 Đorđević M, Mihailović M, Arambašić Jovanović J, Grdović N, Uskoković A, Tolić A, Sinadinović M, Rajić J, Mišić D, Šiler B, Poznanović G, Vidaković M, Dinić S. Centaurium erythraea methanol extract protects red blood cells from oxidative damage in streptozotocin-induced diabetic rats. J Ethnopharmacol 2017; 202: 172-183
  CrossrefPubMedGoogle Scholar
• 13 Varadharaj S, Kelly OJ, Khayat RN, Kumar PS, Webb AJ, Miller MR. Role of dietary antioxidants in the preservation of vascular function and the modulation of health and disease. Front Cardiovasc Med 2017; 4: 1-11
  PubMedGoogle Scholar
• 14 Brocq ML, Leslie SJ, Milliken P, Megson IL. Endothelial dysfunction: from molecular mechanisms to measurement, clinical implications and therapeutic opportunities. Antioxid Redox Signal 2008; 10: 1631-1674
  CrossrefPubMedGoogle Scholar
• 15 Božunović J, Živković S, Gašić U, Glamočlija J, Ćirić A, Matekalo D, Šiler B, Soković M, Tešić Ž, Mišić D. In vitro and in vivo transformations of Centaurium erythraea secoiridoid glucosides alternate their antioxidant and antimicrobial capacity. Ind Crops Prod 2018; 111: 705-721
  CrossrefPubMedGoogle Scholar
• 16 Ghiadoni L, Taddei S, Virdis A. Hypertension and endothelial dysfunction: therapeutic approach. Curr Vasc Pharmacol 2011; 10: 43-60
  PubMedGoogle Scholar
• 17 Goszcz K, Deakin SJ, Duthie GG, Stewart D, Leslie SJ, Megson IL. Antioxidants in cardiovascular therapy: panacea or false hope?. Front Cardiovasc Med 2015; 2: 1-22
  PubMedGoogle Scholar
• 18 Vanhoutte PM, Shimokawa H, Feletou M, Tang EHC. Endothelial dysfunction and vascular disease – a 30th anniversary update. Acta Physiol (Oxf) 2017; 219: 22-96
  CrossrefPubMedGoogle Scholar
• 19 Mombouli JV, Vanhoutte PM. Endothelium-derived hyperpolarizing factor(s): updating the unknown. Trends Pharmacol Sci 1997; 18: 252-256
  PubMedGoogle Scholar
• 20 Nelson MT, Quayle JM. Physiological roles and properties of potassium channels in arterial smooth muscle. Am J Physiol 1995; 4: C799-C822
  PubMedGoogle Scholar
• 21 Furchgott RF. The role of endothelium in the responses of vascular smooth muscle to drugs. Annu Rev Pharmacol Toxicol 1984; 24: 175-197
  CrossrefPubMedGoogle Scholar
• 22 McAnulty RJ. Fibroblasts and myofibroblasts: their source, function and role in disease. Int J Biochem Cell Biol 2007; 39: 666-671
  CrossrefPubMedGoogle Scholar
• 23 Brecher P. Angiotensin II and cardiac fibrosis. Trends Cardiovasc Med 1996; 6: 193-198
  CrossrefPubMedGoogle Scholar
• 24 Kim S, Iwao H. Molecular and cellular mechanisms of angiotensin II-mediated cardiovascular and renal diseases. Pharmacol Rev 2000; 52: 11-34
  PubMedGoogle Scholar
• 25 Porter KE, Turner NA. Cardiac fibroblasts: at the heart of myocardial remodeling. Pharmacol Ther 2009; 123: 255-278
  CrossrefPubMedGoogle Scholar
• 26 van Eickels M, Vetter H, Grohe C. Angiotensin-converting enzyme (ACE) inhibition attenuates insulin-like growth factor-I (IGF-I) induced cardiac fibroblast proliferation. Br J Pharmacol 2000; 131: 1592-1596
  CrossrefPubMedGoogle Scholar
• 27 Sadoshima J, Izumo S. Molecular characterization of angiotensin II-induced hypertrophy of cardiac myocytes and hyperplasia of cardiac fibroblasts. Critical role of the AT1 receptor subtype. Circ Res 1993; 73: 413-423
  CrossrefPubMedGoogle Scholar
• 28 Kachmar MR, Oliveira AP, Valentão P, Gil-Izquierdo A, Domínguez-Perles R, Ouahbi A, Badaoui KE, Andrade PB, Ferreres F. HPLC-DAD-ESI/MSn phenolic profile and in vitro biological potential of Centaurium erythraea Rafn aqueous extract. Food Chem 2019; 278: 424-433
  CrossrefPubMedGoogle Scholar
• 29 Sanchez M, Lodi F, Vera R, Villar IC, Cogolludo A, Jimenez R, Moreno L, Romero M, Tamargo J, Perez-Vizcaino F, Duarte J. Quercetin and isorhamnetin prevent endothelial dysfunction, superoxide production, and overexpression of p47phox induced by angiotensin II in rat aorta. J Nutr 2007; 137: 910-915
  CrossrefPubMedGoogle Scholar
• 30 Penso J, Cordeiro K, da Cunha CR, da Silva Castro PF, Martins DR, Lião LM, Rocha ML, de Oliveira V. Vasorelaxant activity of 7-β-O-glycosides biosynthesized from flavonoids. Eur J Pharmacol 2014; 733: 75-80
  CrossrefPubMedGoogle Scholar
• 31 Hügel HM, Jackson N, May B, Zhang AL, Xue CC. Polyphenol protection and treatment of hypertension. Phytomedicine 2016; 23: 220-231
  CrossrefPubMedGoogle Scholar
• 32 Peluso MR. Flavonoids attenuate cardiovascular disease, inhibit phosphodiesterase, and modulate lipid homeostasis in adipose tissue and liver. Exp Biol Med 2006; 231: 1287-1299
  CrossrefPubMedGoogle Scholar
• 33 Gasparotto Junior A, Dos Reis Piornedo R, Assreuy J, Da Silva-Santos JE. Nitric oxide and Kir6.1 potassium channel mediate isoquercitrin-induced endothelium-dependent and independent vasodilation in the mesenteric arterial bed of rats. Eur J Pharmacol 2016; 788: 328-334
  CrossrefPubMedGoogle Scholar
• 34 Mahobiya A, Singh TU, Rungsung S, Kumar T, Chandrasekaran G, Parida S, Kumar D. Kaempferol-induces vasorelaxation via endothelium-independent pathways in rat isolated pulmonary artery. Pharmacol Rep 2018; 70: 863-874
  CrossrefPubMedGoogle Scholar
• 35 Xiao H, Lu X, Chen X, Sun Z. Protective effects of kaempferol against endothelial damage by an improvement in nitric oxide production and a decrease in asymmetric dimethylarginine level. Eur J Pharmacol 2009; 616: 213-222
  CrossrefPubMedGoogle Scholar
• 36 Teixeira J, Gaspar A, Garrido EM, Garrido J, Borges F. Hydroxycinnamic acid antioxidants: an electrochemical overview. Biomed Res Int 2013; 2013: 251754 doi:10.1155/2013/251754
  PubMedGoogle Scholar
• 37 Mudnic I, Modun D, Rastija V, Vukovic J, Brizic I, Katalinic V, Kozina B, Medic-Saric M, Boban M. Antioxidative and vasodilatory effects of phenolic acids in wine. Food Chem 2010; 119: 1205-1210
  CrossrefPubMedGoogle Scholar
• 38 Brand-Williams W, Cuvelier ME, Berset C. Use of a free radical method to evaluate antioxidant activity. Lebensm Wiss Technol 1995; 28: 25-30
  CrossrefPubMedGoogle Scholar
• 39 Mcgregor DD. The effect of sympathetic nerve stimulation of vasoconstrictor responses in perfused mesenteric blood vessels of the rat. J Physiol 1965; 177: 21-30
  CrossrefPubMedGoogle Scholar
• 40 Bencheikh R, Féray JC, Alaoui A, Crozatier B. Thromboxane A2 in vasomotor effects of phenylephrine, acetylcholine, and bradykinin in rat mesenteric bed. J Cardiovasc Pharmacol 2002; 40: 255-264
  CrossrefPubMedGoogle Scholar
• 41 Adeagbo ASO, Tabrizchi R, Triggle CR. The effects of perfusion rate and NG-nitro-L-arginine methyl ester on cirazoline- and KCl-induced responses in the perfused mesenteric arterial bed of rats. Br J Pharmacol 1994; 111: 13-20
  CrossrefPubMedGoogle Scholar
• 42 Chda A, El Kabbaoui M, Baba BF, Mahfoud A, El Abida K, Bousfiha A, Al Houari G, Abdelali T, Kerbal A, Ben Cheikh R. Endothelium-independent vasorelaxant effect of synthestized 2-hydroxymethylchromone on rat mesenteric arterial bed. Curr Bioact Compd 2018; 14: 289-298
  CrossrefPubMedGoogle Scholar
• 43 Green L, Wagner D, Glogowski J, Skipper P, Wishnok JS, Tannenbaum S. Analysis of nitrate, nitrite, and [¹⁵N]nitrate in biological fluids. Anal Biochem 1982; 126: 131-138
  CrossrefPubMedGoogle Scholar
• 44 Certal M, Vinhas A, Pinheiro AR, Ferreirinha F, Barros-Barbosa AR, Silva I, Costa MA, Correia-de-Sá P. Calcium signaling and the novel antiproliferative effect of the UTP-sensitive P2Y11 receptor in rat cardiac myofibroblasts. Cell Calcium 2015; 58: 518-533
  CrossrefPubMedGoogle Scholar
• 45 Denizot F, Lang R. Rapid colorimetric assay for cell growth and survival. Modifications to the tetrazolium dye procedure giving improved sensitivity and reliability. J Immunol Methods 1986; 89: 271-277
  CrossrefPubMedGoogle Scholar

Correspondence

• References

• 1 Merzouki A, Ed-derfoufi F, Molero Mesa J. Contribution to the knowledge of Rifian traditional medicine. II: folk medicine in Ksar Lakbir district (NW Morocco). Fitoterapia 2000; 71: 278-307
  CrossrefPubMedGoogle Scholar
• 2 Bouyahya A, Abrini J, Et-Touys A, Bakri Y, Dakka N. Indigenous knowledge of the use of medicinal plants in the north-west of Morocco and their biological activities. Eur J Integr Med 2017; 13: 9-25
  CrossrefPubMedGoogle Scholar
• 3 Bnouham M, Mekhfi H, Legssyer A, Ziyyat A. Medicinal plants used in the treatment of diabetes in Morocco. Int J Diabetes Metab 2002; 10: 33-50
  PubMedGoogle Scholar
• 4 Bellakhdar J, Claisse R, Fleurentin J, Younos C. Repertory of standard herbal drugs in the Moroccan pharmacopoea. J Ethnopharmacol 1991; 35: 123-143
  CrossrefPubMedGoogle Scholar
• 5 Uncini Manganelli RE, Chericoni S, Baragatti B. Ethnopharmacobotany in Tuscany: plants used as antihypertensives. Fitoterapia 2000; 71: S95-S100
  CrossrefPubMedGoogle Scholar
• 6 Calvo MI, Cavero RY. Medicinal plants used for cardiovascular diseases in Navarra and their validation from official sources. J Ethnopharmacol 2014; 157: 268-273
  CrossrefPubMedGoogle Scholar
• 7 Chda A, Kabbaoui M, Chokri A, Abida K, Tazi A, Bencheikh R. Spasmolytic action of Centaurium erythraea on rabbit jejunum is through calcium channel blockade and NO release. European J Med Plants 2016; 11: 1-13
  PubMedGoogle Scholar
• 8 Valentão P, Fernandes E, Carvalho F, Andrade PB, Seabra RM, Bastos ML. Antioxidant activity of Centaurium erythraea infusion evidenced by its superoxide radical scavenging and xanthine oxidase inhibitory activity. J Agric Food Chem 2001; 49: 3476-3479
  CrossrefPubMedGoogle Scholar
• 9 Haloui M, Louedec L, Michel JB, Lyoussi B. Experimental diuretic effects of Rosmarinus officinalis and Centaurium erythraea . J Ethnopharmacol 2000; 71: 465-472
  CrossrefPubMedGoogle Scholar
• 10 Tuluce Y, Ozkol H, Koyuncu I, Ine H. Gastroprotective effect of small centaury (Centaurium erythraea L) on aspirin-induced gastric damage in rats. Toxicol Ind Health 2011; 27: 760-768
  CrossrefPubMedGoogle Scholar
• 11 Sefi M, Fetoui H, Lachkar N, Tahraoui A, Lyoussi B, Boudawara T, Zeghal N. Centaurium erythrea (Gentianaceae) leaf extract alleviates streptozotocin-induced oxidative stress and β-cell damage in rat pancreas. J Ethnopharmacol 2011; 135: 243-250
  CrossrefPubMedGoogle Scholar
• 12 Đorđević M, Mihailović M, Arambašić Jovanović J, Grdović N, Uskoković A, Tolić A, Sinadinović M, Rajić J, Mišić D, Šiler B, Poznanović G, Vidaković M, Dinić S. Centaurium erythraea methanol extract protects red blood cells from oxidative damage in streptozotocin-induced diabetic rats. J Ethnopharmacol 2017; 202: 172-183
  CrossrefPubMedGoogle Scholar
• 13 Varadharaj S, Kelly OJ, Khayat RN, Kumar PS, Webb AJ, Miller MR. Role of dietary antioxidants in the preservation of vascular function and the modulation of health and disease. Front Cardiovasc Med 2017; 4: 1-11
  PubMedGoogle Scholar
• 14 Brocq ML, Leslie SJ, Milliken P, Megson IL. Endothelial dysfunction: from molecular mechanisms to measurement, clinical implications and therapeutic opportunities. Antioxid Redox Signal 2008; 10: 1631-1674
  CrossrefPubMedGoogle Scholar
• 15 Božunović J, Živković S, Gašić U, Glamočlija J, Ćirić A, Matekalo D, Šiler B, Soković M, Tešić Ž, Mišić D. In vitro and in vivo transformations of Centaurium erythraea secoiridoid glucosides alternate their antioxidant and antimicrobial capacity. Ind Crops Prod 2018; 111: 705-721
  CrossrefPubMedGoogle Scholar
• 16 Ghiadoni L, Taddei S, Virdis A. Hypertension and endothelial dysfunction: therapeutic approach. Curr Vasc Pharmacol 2011; 10: 43-60
  PubMedGoogle Scholar
• 17 Goszcz K, Deakin SJ, Duthie GG, Stewart D, Leslie SJ, Megson IL. Antioxidants in cardiovascular therapy: panacea or false hope?. Front Cardiovasc Med 2015; 2: 1-22
  PubMedGoogle Scholar
• 18 Vanhoutte PM, Shimokawa H, Feletou M, Tang EHC. Endothelial dysfunction and vascular disease – a 30th anniversary update. Acta Physiol (Oxf) 2017; 219: 22-96
  CrossrefPubMedGoogle Scholar
• 19 Mombouli JV, Vanhoutte PM. Endothelium-derived hyperpolarizing factor(s): updating the unknown. Trends Pharmacol Sci 1997; 18: 252-256
  PubMedGoogle Scholar
• 20 Nelson MT, Quayle JM. Physiological roles and properties of potassium channels in arterial smooth muscle. Am J Physiol 1995; 4: C799-C822
  PubMedGoogle Scholar
• 21 Furchgott RF. The role of endothelium in the responses of vascular smooth muscle to drugs. Annu Rev Pharmacol Toxicol 1984; 24: 175-197
  CrossrefPubMedGoogle Scholar
• 22 McAnulty RJ. Fibroblasts and myofibroblasts: their source, function and role in disease. Int J Biochem Cell Biol 2007; 39: 666-671
  CrossrefPubMedGoogle Scholar
• 23 Brecher P. Angiotensin II and cardiac fibrosis. Trends Cardiovasc Med 1996; 6: 193-198
  CrossrefPubMedGoogle Scholar
• 24 Kim S, Iwao H. Molecular and cellular mechanisms of angiotensin II-mediated cardiovascular and renal diseases. Pharmacol Rev 2000; 52: 11-34
  PubMedGoogle Scholar
• 25 Porter KE, Turner NA. Cardiac fibroblasts: at the heart of myocardial remodeling. Pharmacol Ther 2009; 123: 255-278
  CrossrefPubMedGoogle Scholar
• 26 van Eickels M, Vetter H, Grohe C. Angiotensin-converting enzyme (ACE) inhibition attenuates insulin-like growth factor-I (IGF-I) induced cardiac fibroblast proliferation. Br J Pharmacol 2000; 131: 1592-1596
  CrossrefPubMedGoogle Scholar
• 27 Sadoshima J, Izumo S. Molecular characterization of angiotensin II-induced hypertrophy of cardiac myocytes and hyperplasia of cardiac fibroblasts. Critical role of the AT1 receptor subtype. Circ Res 1993; 73: 413-423
  CrossrefPubMedGoogle Scholar
• 28 Kachmar MR, Oliveira AP, Valentão P, Gil-Izquierdo A, Domínguez-Perles R, Ouahbi A, Badaoui KE, Andrade PB, Ferreres F. HPLC-DAD-ESI/MSn phenolic profile and in vitro biological potential of Centaurium erythraea Rafn aqueous extract. Food Chem 2019; 278: 424-433
  CrossrefPubMedGoogle Scholar
• 29 Sanchez M, Lodi F, Vera R, Villar IC, Cogolludo A, Jimenez R, Moreno L, Romero M, Tamargo J, Perez-Vizcaino F, Duarte J. Quercetin and isorhamnetin prevent endothelial dysfunction, superoxide production, and overexpression of p47phox induced by angiotensin II in rat aorta. J Nutr 2007; 137: 910-915
  CrossrefPubMedGoogle Scholar
• 30 Penso J, Cordeiro K, da Cunha CR, da Silva Castro PF, Martins DR, Lião LM, Rocha ML, de Oliveira V. Vasorelaxant activity of 7-β-O-glycosides biosynthesized from flavonoids. Eur J Pharmacol 2014; 733: 75-80
  CrossrefPubMedGoogle Scholar
• 31 Hügel HM, Jackson N, May B, Zhang AL, Xue CC. Polyphenol protection and treatment of hypertension. Phytomedicine 2016; 23: 220-231
  CrossrefPubMedGoogle Scholar
• 32 Peluso MR. Flavonoids attenuate cardiovascular disease, inhibit phosphodiesterase, and modulate lipid homeostasis in adipose tissue and liver. Exp Biol Med 2006; 231: 1287-1299
  CrossrefPubMedGoogle Scholar
• 33 Gasparotto Junior A, Dos Reis Piornedo R, Assreuy J, Da Silva-Santos JE. Nitric oxide and Kir6.1 potassium channel mediate isoquercitrin-induced endothelium-dependent and independent vasodilation in the mesenteric arterial bed of rats. Eur J Pharmacol 2016; 788: 328-334
  CrossrefPubMedGoogle Scholar
• 34 Mahobiya A, Singh TU, Rungsung S, Kumar T, Chandrasekaran G, Parida S, Kumar D. Kaempferol-induces vasorelaxation via endothelium-independent pathways in rat isolated pulmonary artery. Pharmacol Rep 2018; 70: 863-874
  CrossrefPubMedGoogle Scholar
• 35 Xiao H, Lu X, Chen X, Sun Z. Protective effects of kaempferol against endothelial damage by an improvement in nitric oxide production and a decrease in asymmetric dimethylarginine level. Eur J Pharmacol 2009; 616: 213-222
  CrossrefPubMedGoogle Scholar
• 36 Teixeira J, Gaspar A, Garrido EM, Garrido J, Borges F. Hydroxycinnamic acid antioxidants: an electrochemical overview. Biomed Res Int 2013; 2013: 251754 doi:10.1155/2013/251754
  PubMedGoogle Scholar
• 37 Mudnic I, Modun D, Rastija V, Vukovic J, Brizic I, Katalinic V, Kozina B, Medic-Saric M, Boban M. Antioxidative and vasodilatory effects of phenolic acids in wine. Food Chem 2010; 119: 1205-1210
  CrossrefPubMedGoogle Scholar
• 38 Brand-Williams W, Cuvelier ME, Berset C. Use of a free radical method to evaluate antioxidant activity. Lebensm Wiss Technol 1995; 28: 25-30
  CrossrefPubMedGoogle Scholar
• 39 Mcgregor DD. The effect of sympathetic nerve stimulation of vasoconstrictor responses in perfused mesenteric blood vessels of the rat. J Physiol 1965; 177: 21-30
  CrossrefPubMedGoogle Scholar
• 40 Bencheikh R, Féray JC, Alaoui A, Crozatier B. Thromboxane A2 in vasomotor effects of phenylephrine, acetylcholine, and bradykinin in rat mesenteric bed. J Cardiovasc Pharmacol 2002; 40: 255-264
  CrossrefPubMedGoogle Scholar
• 41 Adeagbo ASO, Tabrizchi R, Triggle CR. The effects of perfusion rate and NG-nitro-L-arginine methyl ester on cirazoline- and KCl-induced responses in the perfused mesenteric arterial bed of rats. Br J Pharmacol 1994; 111: 13-20
  CrossrefPubMedGoogle Scholar
• 42 Chda A, El Kabbaoui M, Baba BF, Mahfoud A, El Abida K, Bousfiha A, Al Houari G, Abdelali T, Kerbal A, Ben Cheikh R. Endothelium-independent vasorelaxant effect of synthestized 2-hydroxymethylchromone on rat mesenteric arterial bed. Curr Bioact Compd 2018; 14: 289-298
  CrossrefPubMedGoogle Scholar
• 43 Green L, Wagner D, Glogowski J, Skipper P, Wishnok JS, Tannenbaum S. Analysis of nitrate, nitrite, and [¹⁵N]nitrate in biological fluids. Anal Biochem 1982; 126: 131-138
  CrossrefPubMedGoogle Scholar
• 44 Certal M, Vinhas A, Pinheiro AR, Ferreirinha F, Barros-Barbosa AR, Silva I, Costa MA, Correia-de-Sá P. Calcium signaling and the novel antiproliferative effect of the UTP-sensitive P2Y11 receptor in rat cardiac myofibroblasts. Cell Calcium 2015; 58: 518-533
  CrossrefPubMedGoogle Scholar
• 45 Denizot F, Lang R. Rapid colorimetric assay for cell growth and survival. Modifications to the tetrazolium dye procedure giving improved sensitivity and reliability. J Immunol Methods 1986; 89: 271-277
  CrossrefPubMedGoogle Scholar

• Supplementary Material