2.1. Drugs and Solutions

The drugs used in this study were Cremophor EL, dimethyl sulphoxide (DMSO), L-phenylephrine chloride (Phe), acetylcholine chloride (Ach), glibenclamide, tetraethylammonium, 4-aminopyridine, and barium chloride (SIGMA). All compounds were dissolved in distilled water, except glibenclamide that was dissolved in DMSO. The composition of Tyrode’s solution used was as follows (mM): NaCl, 158.3; KCl, 4.0; CaCl₂, 2.0; MgCl₂, 1.05; NaH₂PO₄, 0.42; NaHCO₃, 10.0, and glucose, 5.6. K⁺-depolarizing solutions (KCl 20 and 80 mM) were prepared by replacing 20 or 80 mM KCl in Tyrode’s solution with equimolar NaCl, respectively.

2.2. Plant Material

Valeriana prionophylla Standl., Valerianaceae, were collected from cultivations in Tierra Blanca, Concepción Tutuapa, San Marcos (15° 14.808′N, 91° 55.430′W), Guatemala, a vegetative zone that resides in a very humid and low mountainous forest. Three-year-old rhizomes and roots were dug up, washed, and shade-dried. Botanical samples were determined by Mario Veliz at Herbarium BIGU, School of Biology, USAC, and a voucher sample deposited (no. 49183).

2.3. Preparation of Ethanol Extract

Dry material was ground, wetted with 50% ethanol, and placed in a stainless steel percolator. 50% ethanol was added to obtain a tincture, which was concentrated in a rotavapor. Fresh ethanol was added for five consecutive days, and the extract was concentrated. The final drying was performed in a vacuum dryer with silica gel, as described by Holzmann et al. [3]. The average yield of the extractable solids was 28.52%. For in vitro experiments, extracts of the roots and leaves from the Valeriana prionophylla Standl. species (VPR and VPF, resp.) were dissolved in a mixture of distilled water/Cremophor and diluted to the desired concentrations with distilled water just before use; the final concentration of Cremophor in the bath never exceeded 0.01%.

2.4. Animals

Male Wistar rats (250–300 g) were used for all experiments. Animals were housed under controlled temperature ( $21\pm 1$ °C), exposed to a 12 h light-dark cycle with free access to food (Purina, Brazil) and tap water. The study was carried out in accordance with the Guide for the Care and Use of Laboratory Animals as adopted by the US National Institutes of Health.

2.5. Tissue Preparation

Rats were euthanized, and superior mesenteric artery was removed, cleaned from connective tissue and fat as described by Silva and colleagues [10]. Whenever appropriate, the endothelium was removed by gently rubbing the intimal surface of the vessels. Rings (1-2 mm) were suspended in organ baths containing 10 mL of Tyrode’s solution, gassed with a mixture of 95% O₂ and 5% CO₂, maintained at 37°C and at pH 7.4. Isometric tension was recorded under a resting tension of 0.75 g. The solution was changed every 15 min during a stabilization period of 1 hr to prevent the accumulation of metabolites [11]. The isometric contractile force was recorded by a force transducer (MLT020, ADInstruments, Australia) coupled to an amplifier-recorder (ML870/P com LabChart versão 7.0, ADInstruments, Australia) and to a computer equipped with a data acquisition software. The presence of functional endothelium was assessed by the ability of Ach (10 μM) to induce more than 90% relaxation of pre-contracted vessels with Phe (10 μM) and the absence, less than 10% of relaxation induced by Ach.

2.6. Effects of VPF and VPR in Phenylephrine-Induced Contractions

In this experiment, sustained Phe-induced contractions were obtained in isolated rat superior mesenteric artery rings with or without endothelium. In the tonic phase of the second contraction induced by Phe (1 μM), increasing cumulative concentrations of VPF and VPR (0.01; 0.03; 0.1; 0.3; 1; 3; 10; 30; 100; and 300 μg/mL) were separately and continually added to the bath until a maximum response for the added extract was observed, as indicated by a plateau response (approximately 4–6 min).

2.7. Investigation of Nitric Oxide and COX-Derived Products Participation in the Vasorelaxation Mediated by VPR

To investigate the involvement of NO and prostanoids, endothelium-intact rings were incubated for 30 min with L-NAME (10⁻⁴ M) or indomethacin (10⁻⁵ M) (endothelial nitric oxide synthase (eNOS) or cyclooxygenase inhibitors, resp.) before the second application of Phe (1 μM), and the vasorelaxation induced by VPR (300 μg/mL) was investigated before and after the addition of the inhibitors.

2.8. Effect of VPR on Contraction Induced by Depolarization with High K⁺ Concentration

After the stabilization period, rings without endothelium were precontracted with high potassium concentration solution (KCl 80 mM), and, in the tonic phase, different concentrations of VPR (0.01–300 μg/mL) were added cumulatively to the organ bath, and relaxations were measured, as previously described.

2.9. Investigation of K⁺ Channel Participation in the Vasorelaxation Elicited by VPR

To investigate the involvement of K⁺ channels, in the first set of experiments, vasorelaxation with VPR was performed in vessels with denuded endothelium that were precontracted with Phe in Tyrode’s solution with elevated K⁺ (20 mM equimolar replacement of NaCl with KCl) to attenuate K⁺ efflux [10]. Additionally, in the second group of experiments, endothelium-denuded rings were incubated for 30 min with putative K⁺ channel blockers before the second application of Phe (1 μM), and the inhibition was calculated by comparing the response elicited by VPR, before and after the addition of the inhibitors. Preparations were exposed to tetraethylammonium (TEA, 3 mM), a nonselective K⁺ channel blocker; TEA (1 mM), a large-conductance calcium-activated K⁺ channel ( $\text{BK}{}_{\text{Ca}}$ ) selective blocker in this concentration; 4-aminopyridine (4-AP) (1 mM), a voltage-dependent K⁺ ( ${\text{K}}_v$ ) channel blocker; glibenclamide (Glib) (10 μM), an ATP-sensitive K⁺ (K_ATP) channel blocker; and barium chloride (BaCl₂) (30 μM), an inward rectifier K⁺ (K_ir) channel blocker.

2.10. Investigation of Effect of VPR on CaCl₂-Induced Contractions

To investigate the hypothesis that VPR act through the blockade of extracellular calcium influx in endothelium-denuded rings, cumulative concentrations of CaCl₂ (10⁻⁶–10⁻² M) were added in medium containing Ca²⁺-free depolarizing solution (KCl, 60 mM) in absence (control) or in presence of VPR (300 μg/mL).

2.11. Measurement of Mean Arterial Pressure and Heart Rate in Nonanesthetized Normotensive Rats

The day before the experimental session, a catheter (PE₅₀) filled with heparinized saline solution (1000 U/mL) was inserted into the left carotid artery under ketamine/xylazine anesthesia and exteriorized at the nape of the animal’s neck to permit blood pressure recording. An additional catheter was placed in the right femoral vein to allow intravenous drug administration. After 24 hours, arterial pressure was continuously monitored through the carotid catheter connected to a blood pressure transducer (World Precision Instruments) whose signal was amplified and digitally recorded by an analog-to-digital interface (AqDados, application for data acquisition, Lynx Tecnologia Eletrônica Ltda, version 7.0, São Paulo, Brazil) and recorded (1 kHz) on a microcomputer for later analysis. Mean arterial pressure (MAP) was calculated from systolic and diastolic pressure data, while heart rate (HR) was determined by the pulsation of arterial pressure using the AcqKnowledge software program, version 3.5.7, developed by Biopac Systems, Inc., California, USA.

2.12. Statistical Analysis

Data are presented as the mean ± SEM, and n represents a number of rings prepared from different rats. Concentration-response curves to VPR and VPF were based on the percent relaxation of the agonist-induced contraction. A 100% relaxation was assigned when the precontracted rings returned to the baseline values. The curves were fitted using a variable slope sigmoid fitting routine in GraphPad Prism5.0 (Graph Pad Software, Inc., La Jolla, CA, USA). EC₅₀ (concentration required to relax the induced tone by half, and maximum response (MR) values were calculated from the fitted sigmoidal curves. Statistical analyses were performed by comparing $E_{\max }$ and EC₅₀ values between groups from independent observations. Unpaired Student’s t-test or one-way ANOVAs were used to compare 2, 3, or more groups, respectively, with the addition of Bonferroni’s multiple comparisons post-est. Two-sided $P<0.05$ was considered statistically significant.

3.1. Effects of VPR and VPF in Phenylephrine-Induced Contractions

In isolated rat superior mesenteric artery rings, VPR (0.01–300 μg/mL) decreased in a concentration-dependent manner following Phe-induced contraction (1 μM) (EC₅₀ values = 5.96 (3.8−9.2) μg/mL) (Figure 1(a)). In the absence of the vascular endothelium, the potency of VPR was significantly shifted (EC₅₀ values = 39.63 (27.2−57.6) μg/mL; $P<0.05$ ) (Figure 1(a), Table 1), whereas VPF (0.01–300 μg/mL) induced a vasorelaxant effect in the presence and absence of vascular endothelium (maximum response (MR) = $29.39\pm 9.4$ %, MR = $27.05\pm 6.2$ %, resp.; $n=4$ ) (Figure 1(b)); however, this response was reduced in comparison to that obtained by VPR (MR = $75.43\pm 4.08$ %, MR = $70.33\pm 4.58$ %, $P<0.05$ , resp.).

Table 1

Participation of K⁺ channels in the vasorelaxation induced by VPR in mesenteric artery rings precontracted with phenylephrine.

Values are expressed as mean ± SEM; unpaired Student’s $t$ -tests were used to examine the difference between denuded endothelium and intact endothelium; one-way ANOVAs with the addition of Bonferroni's multiple comparisons post hoc test were used to compare denuded endothelium (control) with different inhibitors groups. ^#No significance versus intact endothelium, * $P<0.05$ versus intact endothelium; ** $P<0.01$ versus denuded endothelium; ^## $P<0.01$ versus denuded endothelium; ^nsno significance versus denuded endothelium.

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3.2. Effect of VPR on Endothelium-Intact Rings in the Presence of L-NAME or Indomethacin

To investigate the involvement of NO and prostanoids, endothelium-intact rings were preincubated for 30 min with L-NAME (100 μM) or indomethacin (10 μM) before the second contraction with Phe (1 μM). Figure 2 shows that the vasorelaxant activity of VPR (300 μg/mL) was significantly reduced in the presence of these inhibitors.

3.3. Effects of VPR on Contraction Induced by High K⁺ Concentration

As illustrated in Figure 3, following contraction with KCl 80 mM, VPR-mediated relaxation of endothelium-removed rings was significantly reduced when compared to the contractile response induced by Phe (Table 1), as demonstrated by the displacement of the concentration-response curve to the right.

3.4. Effect of VPR on Arteries Treated with KCl 20 mM

To evaluate the involvement of K⁺ channels in the VPR-mediated vasorelaxant response, experiments were performed in endothelium-denuded rings incubated with KCl 20 mM and precontracted with Phe. As shown in Figure 4(a), the VPR-mediated vasorelaxation was reduced, with significant alterations in pharmacological efficacy when compared to the control (Table 1).

[figures omitted; refer to PDF]

3.5. Effect of VPR on Endothelium-Denuded Rings in the Presence of Different K⁺ Channel Inhibitors

Figure 4(a) shows that the vasorelaxant activity of VPR at the highest concentration was significantly rightward shifted in the presence of TEA (3 mM) (Table 1). However, in the presence of Glib (10 μM), 4-AP (1 mM), or BaCl₂ (30 μM), VPR-mediated relaxation in rings lacking the vascular endothelium and precontracted with Phe was not significantly reduced. In the presence of TEA (1 mM), the vasorelaxant response was significantly attenuated (Figures 4(b) and 4(c), Table 1).

3.6. Effect of VPR on CaCl₂-Induced Contractions

To investigate the hypothesis of the residual vasorelaxant effect induced by VPR being the same as in the presence of the K⁺ channels inhibitors, concentration-response curve was induced with CaCl₂ in Ca²⁺-free depolarizing solution. Figure 5 illustrates that VPR (300 μg/mL) was not able to inhibit CaCl₂-induced contractions, demonstrating that VPR extract probably does not inhibit extracellular calcium influx.

3.7. VPR Effect on MAP and HR in Nonanesthetized Rats

As Figure 6 shows, in nonanesthetized normotensive rats, intravenous bolus injections of VPR (1, 5, 10, and 20 mg/kg) induced hypotension (MAP = $-13.18\pm 1.6$ , $-18.54\pm 6.4$ , $-16.36\pm 5.6$ , and $-28.32\pm 3.4$  mmHg, resp.; $n=5$ ) (Figures 6(a) and 6(b)) associated with tachycardia (HR = $11.64\pm 5.5$ ; $50.24\pm 14.0$ ; $61.45\pm 8.0$ ; and $69.88\pm 8.4$  bpm, resp.; $n=5$ ) (Figure 6(c)).

[figures omitted; refer to PDF]