Antioxidant Protective Effects of the Resveratrol on the Cardiac and Vascular Tissues from Renal Hypertensive Rats


Background: Accumulating reactive oxygen species (ROS) is involved in cellular signaling and function disturbances due to the oxidative stress, which contributes to several diseases. The consequences of ROS activity represent an im-portant mechanism on the pathogenesis of vascular diseases, such as hypertension. Increased blood pressure observed in renal hypertension of the 2 kidneys-1 clip (2K-1C) model involves increased ROS levels in the cardiovascular system. Resveratrol, a polyphenolic compound primarily found in red wine, has many biological and pharmacological proper-ties. Considering the antioxidant properties of resveratrol, the present study was aimed to investigate the effects of the chronic treatment with resveratrol on cardiovascular system from renal hypertensive rats. Results: 2K-1C hypertension presented increased blood pressure, which was reduced at the end of the fifth week of resveratrol treatment. The cardiac hypertrophy index and the basal levels of ROS in rat aortic rings were also reduced by resveratrol treatment. Conclusions: The present findings clearly show the protective effects from resveratrol on the blood pressure, the car-diac growth and the vascular ROS generation in renal hypertension.

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J. Oliveira, C. Antonietto, A. Scalabrini, T. Marinho, L. Pernomian, J. Corrêa and C. Restini, "Antioxidant Protective Effects of the Resveratrol on the Cardiac and Vascular Tissues from Renal Hypertensive Rats," Open Journal of Medicinal Chemistry, Vol. 2 No. 3, 2012, pp. 61-71. doi: 10.4236/ojmc.2012.23008.

1. Introduction

Hypertension is a well-studied risk factor for several car diovascular diseases. It has been established that hypetension is associated with cardiovascular damages such as endothelial dysfunction, microvascular impairments [1] and cardiovascular remodeling [2,3]. The pathological processes underlying hypertension have been extensively studied by applying some animal models [4], such as the 2-kidneys-1Clip (2K-1C) renovascular hypertension. In this model, designed by Goldblatt and cols in 1934 [5], a partial stenosis in the left renal artery is caused by placing a silver clip on the arterial side close to the aorta. This stenosis elicits a sustained increase in blood pressure mainly due to the increased plasma renin activity and subsequent increased circulating angiotensin-II (Ang II) [6]. Furthermore, an overproduction of superoxide anion () has been observed in some vessels from 2K-1C hypertensive an imals [7-9]. In 2K-1C pigs, the increased plasma renin activity and high blood pressure (BP) have been correlated to increased systemic oxidative stress [10-13]. Indeed, hypertensive patients with renovascular disease have shown a markedly in creased lipid peroxidation, which is partly related to the activation of the Renin-Angiotensin System (RAS) [8]. One of the most relevant damages caused by oxidative stress underlying hypertension and correlated diseases is the impairment of endothelium-dependent vasorelaxation mechanisms [9,10], which is generally related to the reduced endothelial nitric oxide (NO) generation or bioavailability [14-16]. In turn, the reduced NO bioavailability has been attributed to the oxidative inactivation of NO by the excessive generation of in the vascular wall

[17]. Besides the vessels, ROS generation also affects the heart. It is well-known that hydrogen peroxide (H2O2) impairs cardiac contraction and evokes cardiac hypertrophy [18]. Indeed, substantial evidence has pointed to oxidative stress as a major pathway in the cardiac remodeling and the transition of compensated cardiac hypertrophy during heart failure [19-23]. The consumption of flavonoid-rich food is associated to the reduced risk of many acute diseases. This protective effect is, at least in part, due to the antioxidant properties from flavonoids [24]. Part of the cardiovascular protective effects of red wine has been attributed to resveratrol, a polyphenolic compound present in the red grape skin [25]. The study of the biological properties from resveratrol began in the 80 s, but it became more extensive in the 90 s due to the French Paradox [26,27]. According to Renaud and Lorgeril [26], in most countries, high intake of saturated fat is positively related to high mortality from coronary heart disease (CHD). However, the situation in France is paradoxical in that there is high intake of saturated fat but low mortality from coronary heart disease. This paradox may be attributable in part to high wine consumption. Resveratrol acts as an active antioxidant by donating hydrogen protons to free radicals and by inhibiting lipid peroxidation and oxidizing enzymes [28]. Also, resveratrol stimulates the acute release of NO from endothelial cells, which improves NO-mediated vasorelaxation mechanisms [29]. Since oxidative stress impairs the cardiovascular function in 2K-1C renovascular hypertension, the hypothesis from the present study is that the chronic treatment of 2K-1C hypertensive rats with resveratrol would reduce the cardiovascular damages through the antioxidant properties of the polyphenol. Thereby, our aim was to evaluate the antioxidant effects of the chronic treatment with resveratrol on the structural and functional damages in 2K-1C rat aorta and heart.

2. Materials and Methods

2.1. Experimental Groups and Resveratrol Treatment

All procedures were performed in agreement with international ethical standards of animal experimentation and approved by the Ethics Committee of the University of Ribeirão Preto (protocol No.). Animals were maintained on a standard rat chow with a 12-hlight/dark cycle and free access to food and water. Renovascular hypertension was induced in male Wistar rats (180 g - 220 g) following the 2K-1C Goldblatt model [5]. Briefly, the rats were anaesthetized (0.2 mL of Ketamine chloride and 0.1 mL of Xylazine hydrochloride, ip), and a midline laparotomy was performed. Then, a silver clip (0.2 mm of internal diameter) was placed around the left renal artery. Sham-operated rats were only submitted to laparotomy, without the silver clip placing. Thus, these animals were named as the 2 kidneys (2K) group. One day after the surgery, the chronic treatment with resveratrol started, by gavage (20 mg/Kg, prepared in 0.05% Tween 80 suspension), which was performed three times a week, during six weeks. Juan et al. [30] had proved the safety and effectiveness of the oral treatment with resveratrol (20 mg/Kg) in rats. In this sense, we have defined this dose for the treatment.

2K or 2K-1C rats received the solution containing resveratrol + Tween 80 or water + Tween 80 by gavage. Thus, our study was composed by four experimental groups, as follows: 1) 2K rats treated with water + Tween 80 solution (2K control group); 2) 2K rats treated with resveratrol + Tween 80 suspension (2K Resv group); 3) 2K-1C rats treated with water + Tween 80 solution (2K-1C control group); and 4) 2K-1C rats treated with resveratrol + Tween 80 suspension (2K-1C Resv group).

2.2. Blood Pressure Measurements

Systolic blood pressure (SBP) was measured one day before the surgery (control). After the surgery SBP was weekly measured in non-anaesthetized animals by an indirect tail-cuff method [31]. Rats were considered hypertensive when SBP was higher than 160 mm Hg [31].

2.3. Rat Euthanasia

The experimental procedures described below were performed at the end of the sixth week of the treatment. The animals were euthanized by CO2 exposure followed by cervical dislocation (Office of Laboratory Animal Welfare, National Institutes of Health, US Department of Health and Human Services, 2002. Public Health Service Policy on Humane Care and Use of Laboratory AnimalsClarification Regarding Use of Carbon Dioxide for Euthanasia of Small Laboratory Animals. (

2.4. Cardiac Hypertrophy Index

Rat thoracic cavity was opened to expose the heart, which was quickly removed and washed in cold saline 0.9%. Excess of the saline was gently removed with filter paper and the heart was weighed. The cardiac hypertrophy index (CHI) was calculated from the heart weight and the animal body weight, which was obtained in the day of the experiment, as follows: CHI = heart wet weight (mg)/body weight (g) × 1000 [32].

2.5. Vascular Reactivity Studies

Rat thoracic aorta was isolated for the vascular reactivity studies. Aortic rings (3 mm in length) were placed in isolated organ bath chambers (5 ml) containing Krebs Physiological Salt solution (in mmol/L: NaCl 130.0; KCl 4.7; KH2PO4 1.2; CaCl2 1.6; MgSO4 1.2; NaHCO3 14.9; glicose 5.5) at 37˚C, continuously bubbled with 95% O2 and 5% CO2, at pH 7.4. Two stainless steel holders were placed through the lumen of the aortic rings. One of the holders was fixed to the tissue chamber and the other one was connected to a F-60 force-displacement transducer, in order to record the muscular tension on a polygraph (Power Lab, 415-ADInstruments). The aortic rings were submitted to a basal tension of 1.5 g, for a 60 min equilibration period before drug addition. The optimal basal tension (1.5 g) in aortic rings from 2K or 2K-1C rats, treated or not with resveratrol, was previously standardized by exposing the vessels to 90 mmol/L KCl under a set resting tensions (0.5 g - 2.5 g). The arterial functional viability was tested by phenylerpine (PHE, 0.1 μmol/L). The main vascular ROS source is the endothelium [33, 34]. Since the aim of this set of experiments was to investigate the direct effects of the treatment with resveratrol on the vascular tone, the endothelial layer from aortic rings was removed. Thus, in all vascular reactivity protocols, the endothelium was mechanically removed by gently rubbing. The absence of the endothelium was confirmed with no (0%) relaxation to acetylcholine (1 μmol/ L) after the pre-contraction with PHE (0.1 μmol/L).

2.6. Vascular ROS Measurement by Confocal Microscopy

Aortic rings (250 μm thick) were placed in a coverslip covered with poly-L-lysine solution, and loaded with the fluorescent dye for ROS, dihydroethidium (DHE, 50 μmol/L, 30 min, at 37˚C), which was prepared in Hanks solution (composition in mmol/L: CaCl2 1.6; MgSO4 1.0; NaCl 145.0; KCl 5.0; NaH2PO4 0.5; dextrose 10.0; HEPES 10.0), at pH 7.4. The excess of the dye was removed by washing with Hanks solution. After washing, the coverslips were placed on a chamber with Hanks buffer (pH 7.4). The ROS level was assessed by a confocal laser microscope (Leica TSC SP5). DHE was excited with the 488 nm line of an argon ion laser at 570 nm and the emitted fluorescence was measured at 650 nm. Time course software was used to capture images of the tissues at 1.314 second intervals (xyt) in the Live Data Mode acquisition. By applying the laser scanning confocal microscope (LSCM) computer software, the intracellular minimum or maximum fluorescence intensity values were measured. From these data, the initial fluorescence value at s was taken as the basal fluorescence (F0), and the final fluorescence intensity value (F) was registered after PHE addition (0.1 μmol/L), at.

The confocal fluorescence experiments were conducted in the “Live Data Mode”. Thus, the images were captured in function of the time, which required that the calibration was set up in a xyt way (but not in a xyz way). After the regions of interest (ROI: cells) were chosen, the fluorescence intensity values were captured. The fluorescence was considered from each selected ROI, in each layer (endothelium or smooth muscle) of each aortic ring. In our study, we selected a fixed number of five (05) ROI in each arterial layer from each rat aorta. This approach allowed us to compare the fluorescence intensity values between these two arterial layers. Afterwards, the average of the fluorescence in each selected cell in its respecttive layer was calculated for each animal (n). Following the ROI selection, the mean value was obtained from the fluorescence intensity values from these five regions. We obtained the median value by plotting the median values from all arteries within an experimental group. This value was posteriorly summed with the other animals’ values from the same group of treatment in order to reach the mean ± SEM. The ethidium (DHE) fluorescence is emitted by the cellular nuclei, in this sense each designed ROI was guided by this organelle.

2.7. Solutions and Drugs

Krebs PSS was prepared in deionised water at the day of the respective experiments. Salts were purchased from Synth (Diadema/SP-Brazil. Phenylephrine, (PHE) acetylcholine (ACh), HEPES (4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid), dihydroethidium (DHE), DMSO and Resveratrol were obtained from Sigma-Aldrich (St. Louis, MO, USA). Stock solution of PHE and ACh were prepared in deionized water (100 mmol/L) and kept on –20˚C. Stock solution DHE was prepared in DMSO (0.01mol/L), and kept on –20˚C. Resveratrol was dissolved in deionised water with 0.05% Tween 80 at the day of the treatment.

2.8. Data Analysis

Results were expressed as the mean ± SEM, and n indicates the number of animals. Statistical significance was evaluated by analysis of variance (one-way ANOVA) and post hoc test Newman Keuls by GraphPad Prismâ 5.0 Software (San Diego, CA-USA). Values of p < 0.05 were considered to be significant. The pharmacological parameters analyzed from concentration-effect curves to phenylephrine were represented by the pD2 (–logEC50: negative logarithm of the molar concentration of the drug required to promotes 50% of the maximal effect) and the Emax (maximal contraction) values. The EC50 values were calculated by means of linear regression analysis from complete concentration-effect curves in individual experiments.

3. Results

3.1. Systolic Blood Pressure

The values of the SBP are shown in the Figure 1 and represent data from the measurement at the end of the sixth week.

The treatment with resveratrol has significantly reduced the hypertensive level from the 2K-1C Resv group () when compared to the 2K-1C control group (). This reduction did not reach the values from 2K Resv group () or the values from 2K control group ().

3.2. Cardiac Hypertrophy Index (CHI)

The CHI in 2K-1C control group () was significantly higher compared to 2K control group (). The treatment with resverat-rol did not alter the cardiac hypertrophy index in 2K rats (2K Resv group:), but reduced it in 2K-1C rats (2K-1C Resv group:) to the 2K control group levels (Figure 2). CHI in 2K-1C Resv group was statistically similar to the value obtained in 2K control or 2K Resv groups.

3.3. Vascular Reactivity

The concentration-effect curves evoked by phenylephrine (PHE: 0.01 nmol/L - 10μ mol/L) in endothelium denude aortic rings were constructed. Contractions stimulated in preparations from 2K-1C control group (Emax: 100 ±

0.033%; pD2 = 7.6 ± 0.27, n = 5) were not statistically preparations from 2K-1C control group (Emax: 100 ±

Figure 1. Effect of the treatment with resveratrol on the Systolic Blood Pressure (SBP) of the hypertensive rats. SBP was measured by tail cuff method before and after six weeks of treatment with resveratrol (Resv 20 mg/Kg) or control (treatment with water + Tween 80). Values represents the measurement at the end of treatments and are expressed as mean ± SEM (n = 10 - 23). *Difference between the 2K-1C control vs. 2K control and 2K-1C Resv vs. 2K resv (p < 0.01). #Difference between 2K-1C Resv (treated with resveratrol) and 2K-1C control (non-treated). ANOVA, one way; Neuman-Keuls’ post-test.

different from that one evoked in 2K control rat aorta (Emax: 98.79 ± 0.74%; pD2 = 7.07 ± 0.15, n = 5). At the same way, the contraction evoked by phenylephrine in aorta from 2K Resv group (Emax: 99.25 ± 2.71%; pD2: 8.6 ± 0.27, n = 5) or 2K-1C Resv group (Emax: 97.32 ± 2.39%; pD2: 7.5 ± 0.057, n = 5) was not different from that one evoked in aorta from 2K control group (Figure 3).

3.4. Vascular ROS Measurement

Basal DHE fluorescence results are shown in the Figure

Figure 2. Effect of resveratrol treatment on cardiac hypertrophy index (heart wet weight (mg)/body weight (g)) of 2K and 2K-1C rats treated with resveratrol (resv 20 mg/Kg) or control (treatment with water + Tween 80) during six weeks. Y-axis is represented in the cardiac hypertrophy index for different groups of animals. Values are expressed as mean ± SEM (n = 7 - 11). *Indicates statistical difference between the control 2K-1C and the other groups. One way analysis of variance (ANOVA), Neuman-Keuls post test.

Figure 3. Effect of treatment with resveratrol on vascular reactivity to phenylephrine (PHE) in aortic rings isolated from 2K and 2K-1C. The contractile-response curves were obtained by adding increasing cumulative concentrations of PHE (0.01 nmol/L - 10 μmol/L) in isolated aortic rings without endothelium from 2K and 2K-1C treated with resveratrol (Resv 20 mg/Kg) or control (water + Tween 80) for six weeks. Values are expressed as mean ± SEM (n = 5).

4(a) and the DHE fluorescence results after stimulation with phenylephrine are shown in the Figure 4(b).

Comparing the respective arterial layers, the basal DHE fluorescence intensity emitted by the endothelial (35.70 ± 4.826, n = 4, p < 0.0001) or muscular (79.09 ± 8.468, n = 4, p < 0.001) layers of the aorta from 2K-1C control group was significantly higher than the basal DHE fluorescence intensity emitted by the endothelial (5.133 ± 1.535, n = 4, p < 0.0001) or the muscular (12.43 ± 1.896, n = 4, p < 0.001) layers of the aorta from 2K control group, respectively (Figure 4(a)). The treatment with resveratrol did not alter the basal DHE fluorescence both in the endothelial (4.13 ± 0.165, n = 4) or the muscular (15.307 ± 2.397, n = 4) layers of the aorta from 2K Resv group when compared to the 2K control group. On the other hand, the basal DHE fluorescence was signifycantly reduced after resveratrol treatment in the endothelial (7.097 ± 2.032, n = 4) or muscular (28.365 ± 8.680, n = 4) layers of the aorta from 2K-1C Resv group, when compared to the 2K-1C control group (Figure 4(a)).

The Figure 4(b) represents the DHE fluorescence after the stimulus with the alpha-1 agonist, phenylephrine. Phenylephrine did not alter the basal DHE fluorescence emitted by the endothelial (6.123 ± 1.406, n = 4) or muscular (14.953 ± 3.256, n = 4) layers of the aorta from 2K control group when compared to the endothelial

(4.300 ± 0.138, n = 4) or muscular layers (13.857 ± 9.074, n = 4) of the aorta from 2K Resv group, respectively.

Conversely, phenylephrine increased the basal DHE fluorescence emitted by the endothelial (68.635 ± 11.501, n = 4, p < 0.0001) or muscular (121.442 ± 9.074, n = 4, p < 0.0001) layers of the aorta from 2K-1C control group the respective arterial layer of the aorta from 2K control or Resv groups. Resveratrol treatment prevented the increase induced by phenylephrine in the basal DHE fluorescence emitted by the endothelial (7.160 ± 1.967, n = 4, p < 0.0001) or muscular (28.327 ± 8.585, n = 4, p < 0.0001) layers of the aorta from 2K-1C group (Figure 4(b)).

Figure 5 reports representative images from the ROS levels in aortic rings from 2K or 2K-1C control or Resv groups, detected by dihydroethidium (DHE) staining in confocal microscopy assays.

Conflicts of Interest

The authors declare no conflicts of interest.


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