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Excitatory amino acid receptor blockade within the caudal pressor area and rostral ventrolateral medulla alters cardiovascular responses to nucleus raphe obscurus stimulation in rats

Abstract

Pressor responses elicited by stimulation of the nucleus raphe obscurus (NRO) depend on the integrity of the rostral ventrolateral medulla (RVLM). Therefore, to test the participation of excitatory amino acid (EAA) receptors in the cardiovascular responses evoked by NRO stimulation (1 ms, 100 Hz, 40-70 µA, for 10 s), the EAA antagonist kynurenic acid (Kyn) was microinjected at different sites in the ventrolateral medullar surface (2.7 nmol/200 nl) of male Wistar rats (270-320 g, N = 39) and NRO stimulation was repeated. The effects of NRO stimulation were: hypertension (deltaMAP = +43 ± 1 mmHg, P<0.01), bradycardia (deltaHR = -30 ± 7 bpm, P<0.01) and apnea. Bilateral microinjection of Kyn into the RVLM, which did not change baseline parameters, almost abolished the bradycardia induced by NRO stimulation (deltaHR = -61 ± 3 before vs -2 ± 3 bpm after Kyn, P<0.01, N = 7). Unilateral microinjection of Kyn into the CVLM did not change baseline parameters or reduce the pressor response to NRO stimulation (deltaMAP = +46 ± 5 before vs +48 ± 5 mmHg after Kyn, N = 6). Kyn bilaterally microinjected into the caudal pressor area reduced blood pressure and heart rate and almost abolished the pressor response to NRO stimulation (deltaMAP = +46 ± 4 mmHg before vs +4 ± 2 mmHg after Kyn, P<0.01, N = 7). These results indicate that EAA receptors on the medullary ventrolateral surface play a role in the modulation of the cardiovascular responses induced by NRO stimulation, and also suggest that the RVLM participates in the modulation of heart rate responses and that the caudal pressor area modulates the pressor response following NRO stimulation.

Raphe nuclei; Electrical stimulation; Ventrolateral medulla; Caudal pressor area; Excitatory amino acid receptors; Kynurenic acid; Blood pressure


Braz J Med Biol Res, October 2002, Volume 35(10) 1237-1245

Excitatory amino acid receptor blockade within the caudal pressor area and rostral ventrolateral medulla alters cardiovascular responses to nucleus raphe obscurus stimulation in rats

N.F. Silva2, J.G.P. Pires1, M.A. Dantas1 and H.A. Futuro Neto1

1Departamento de Ciências Fisiológicas, Centro Biomédico, Universidade Federal do Espírito Santo, Vitória, ES, Brasil

2Associação Educacional de Vitória (FAESA), Vitória, ES, Brasil

References

Correspondence and Footnotes Correspondence and Footnotes Correspondence and Footnotes

Abstract

Pressor responses elicited by stimulation of the nucleus raphe obscurus (NRO) depend on the integrity of the rostral ventrolateral medulla (RVLM). Therefore, to test the participation of excitatory amino acid (EAA) receptors in the cardiovascular responses evoked by NRO stimulation (1 ms, 100 Hz, 40-70 µA, for 10 s), the EAA antagonist kynurenic acid (Kyn) was microinjected at different sites in the ventrolateral medullar surface (2.7 nmol/200 nl) of male Wistar rats (270-320 g, N = 39) and NRO stimulation was repeated. The effects of NRO stimulation were: hypertension (DMAP = +43 ± 1 mmHg, P<0.01), bradycardia (DHR = -30 ± 7 bpm, P<0.01) and apnea. Bilateral microinjection of Kyn into the RVLM, which did not change baseline parameters, almost abolished the bradycardia induced by NRO stimulation (DHR = -61 ± 3 before vs -2 ± 3 bpm after Kyn, P<0.01, N = 7). Unilateral microinjection of Kyn into the CVLM did not change baseline parameters or reduce the pressor response to NRO stimulation (DMAP = +46 ± 5 before vs +48 ± 5 mmHg after Kyn, N = 6). Kyn bilaterally microinjected into the caudal pressor area reduced blood pressure and heart rate and almost abolished the pressor response to NRO stimulation (DMAP = +46 ± 4 mmHg before vs +4 ± 2 mmHg after Kyn, P<0.01, N = 7). These results indicate that EAA receptors on the medullary ventrolateral surface play a role in the modulation of the cardiovascular responses induced by NRO stimulation, and also suggest that the RVLM participates in the modulation of heart rate responses and that the caudal pressor area modulates the pressor response following NRO stimulation.

Key words: Raphe nuclei, Electrical stimulation, Ventrolateral medulla, Caudal pressor area, Excitatory amino acid receptors, Kynurenic acid, Blood pressure

Introduction

The participation of the nucleus raphe obscurus (NRO) in cardiovascular regulation using electrical stimulation has been demonstrated in various species. For instance, NRO stimulation in cats predominantly causes a fall in blood pressure (BP) (1,2), while in rabbits both depressor and pressor effects are observed (3). On the other hand, in hamsters (4) and guinea pigs (5) pressor responses to NRO stimulation are predominant. In anesthetized rats, electrical or chemical stimulation of the NRO and other raphe nuclei frequently causes increases in arterial BP (3,6) with wide heart rate (HR) variability. Dreteler et al. (7) demonstrated a rise in BP as a result of 5-HT1A receptor agonist microinjection into the NRO, and proposed that the related bradycardia was a baroreflex-mediated response. In contrast, Coleman and Dampney (8) observed sympathoinhibition and hypotension evoked by microinjection of L-glutamate into sites within the NRO in anesthetized rabbits.

Anatomical studies of rats have indicated that caudal raphe neurons project either directly to the intermediolateral (IML) cell column (9-11) or by sending axons to sites in the ventrolateral medulla (VLM) (12-14). Therefore, there is no conclusive evidence concerning NRO projections or their precise role in cardiovascular regulation. Campos Jr. et al. (15) showed that the pressor effects caused by stimulating the NRO require an intact rostral ventrolateral medulla (RVLM), an important area in the VLM involved in autonomic control (16), which directly projects to the IML (9). Preliminary results from our laboratory (17) failed to demonstrate direct functional connections between NRO and RVLM. We therefore hypothesized that the NRO might not have monosynaptic connections to the RVLM, and that the responses to NRO stimulation may be mediated by indirect projections to the RVLM.

At least two other areas in the VLM that are involved in autonomic control can influence RVLM activity: the caudal ventrolateral medulla (CVLM) (18,19), a sympathoinhibitory area with projections to the RVLM (20), and the caudal pressor area (CPA) (21), originally described as a hypertensive area in deeply anesthetized or decerebrate animals (22-24). The functional connections between the CPA and the RVLM (23,25) possibly occur via CVLM glutamatergic neurons (26).

The various cardiovascular and respiratory responses evoked by NRO stimulation have been credited to activation of serotonergic neurons (7). However, other neurotransmitters are present in NRO neurons, including excitatory amino acids (EAA; mainly L-glutamate). Since the blockade of 5-HT1-3 receptors in the VLM did not block the cardiovascular responses evoked by NRO stimulation (17), the present study was designed to test the possible role of EAA-mediated NRO projections to the RVLM, CVLM and CPA in these responses.

Material and Methods

Male Wistar rats weighing 270-320 g were anesthetized with urethane (1.2 g/kg, after induction with ether) injected into the left femoral vein cannulated with a polyethylene catheter (PE50). Supplementary doses of anesthetic were administered whenever necessary, as indicated by the paw pinch reflex and/or by unstable cardiovascular recordings. Arterial BP was recorded through a heparinized (40 U/ml) saline-filled catheter (PE50) inserted into the left femoral artery and connected to a pressure transducer (Statham P23 Db, Valley View, OH, USA). Pulsatile BP, mean arterial BP (MAP) and HR were recorded with a Gould RS 3400 polygraph. A tracheotomy was performed in all animals and respiration was recorded with a pneumotachograph (Fleish 0000) and a low-pressure transducer (Valadine) connected to the polygraph. Whenever necessary the rats were artificially ventilated (Harvard Rodent Ventilator, South Natick, MA, USA). All cardiovascular and respiratory activity data were digitalized (Biopac MP 100) and stored on a PC hard disk for later processing. Rectal temperature was maintained between 36-37ºC with a homeothermic blanket (Harvard).

The rats were mounted on a stereotaxic apparatus (Stoelting, Wood Dale, IL, USA) and monopolar isolated cathodal stimulation (1 ms, 100 Hz, 40-70 µA, for 10 s) of the NRO (midline, 11.8 mm AP in relation to the bregma, 8 mm depth) was performed with stainless steel electrodes insulated throughout except at the tip (tip size 30-40 µm, resistance 15-30 kW), the anode being a clip attached to a neck muscle. The dorsal surface of the brainstem was exposed by retraction of the skin and muscles at the base of the skull, followed by the removal of the atlanto-occipital membrane and portions of the occipital bone. Kynurenic acid (Kyn; 2.7 nmol/200 nl) and artificial cerebrospinal fluid (CSF) containing 122 mM NaCl, 25.7 mM NaHCO3, 1 mM MgSO4, and 1 mM CaCl2, with pH adjusted to 7.2-7.4, were microinjected bilaterally into the RVLM (+3 mm AP in relation to the obex, 1.5 mm L), CVLM (+1 mm AP in relation to the obex, 1.5 mm L) or CPA (-1 mm AP in relation to the obex, 1.5 mm L). In a separate group of four animals, Kyn was microinjected unilaterally into the CVLM. Vertical positioning was obtained by slowly lowering both micropipettes placed inside the guide cannulae (which were 6-8 mm shorter than the micropipettes) until a slight displacement between them was observed (the displacement occurs when the tip of the micropipette touches the pia mater adjacent to the ventral medullar surface; the depth was 0.79 mm for the RVLM in relation to the dorsal surface of the cerebellum, 0.59 mm for the CVLM in relation to the dorsal surface of the cerebellum and 0.33 mm for the CPA in relation to the dorsal surface of the medulla. Therefore the microinjections were applied to the ventral layers of the nuclei).

At least three electrical stimulations of the NRO were performed at 3-min intervals and the means of the measured parameters were considered as controls. Kyn microinjection was performed ~1.5 min after the last control NRO stimulation and after a period of ~1.5 min a new series of three NRO stimulations was performed. A separate group of CSF-treated animals was used as time-matched controls.

At the end of each experiment the position of the stimulus or of the microinjection was determined by passing a DC current of 5-20 µA for 1 min (stainless steel electrode anode) or by microinjecting 200 nl 2% Evan's blue dye. The animals were then heparinized and transcardially perfused with 200 ml saline solution (0.9% NaCl) and a solution of 1% potassium ferrocyanide in 10% formaldehyde. The brain was removed and placed in formaldehyde for 7 days. Sites of microinjections or electrical NRO stimulation were identified and plotted on a schematic diagram.

Data are reported as means ± SEM. Paired or unpaired t-tests were used whenever appropriate for statistical comparisons of the means. Two-way ANOVA was used for comparisons between groups. In all cases, the level of significance was set at P£0.05.

Results

Effect of electrical stimulation of the NRO on arterial blood pressure, heart rate and respiration of anesthetized rats

In the 39 anesthetized rats studied, basal MAP and HR were 92 ± 1 mmHg and 384 ± 7 bpm, respectively. Electrical stimulation of a site within the NRO produced an increase of BP (MAP = 135 ± 2, DMAP = +43 ± 1 mmHg, P<0.01, N = 39; Figure 1). HR changes during NRO stimulation were variable, but bradycardia was observed in most animals (HR = 353 ± 9, DHR = -30 ± 7 bpm, P<0.01, N = 39; Figure 1). The stimulus frequently elicited apnea. These animals were divided into subgroups to test the effects of bilateral microinjections of CSF and Kyn within the RVLM, CVLM or CPA on the responses to NRO stimulation.

Figure 1.
Mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) before and after nucleus raphe obscurus (NRO) stimulation. B1, baseline before stimulation. Data are reported as means ± SEM for all 39 rats. *P<0.01 compared to B1 (Student
t-test).

[View larger version of this image (10 K GIF file)]

Effects of EAA receptor antagonism in the RVLM on the responses to NRO stimulation

A group of seven rats was used to study the effects of EEA receptor blockade in the RVLM with Kyn on the cardiovascular responses to NRO stimulation. Bilateral Kyn microinjection did not alter baseline arterial pressure, HR or respiration pattern. Also, pressor and respiratory responses to NRO stimulation were not modified by Kyn (Figure 2). The microinjection produced no significant changes in basal MAP (94 ± 3 to 89 ± 3 mmHg) or in the NRO stimulation pressor responses (135 ± 3 before Kyn and 131 ± 2 mmHg after Kyn, N = 7; Figure 3). On the other hand, although Kyn microinjection did not elicit variations in basal HR (control = 404 ± 9, after Kyn = 405 ± 11 bpm), it significantly reduced HR responses to NRO stimulation (DHR = -61 ± 3 and -2 ± 3 bpm, before and after Kyn, respectively, P<0.01, N = 7; Figure 3). Microinjection of vehicle (artificial CSF) into this area induced no significant changes in any of the parameters analyzed (MAP: 90 ± 3 to 91 ± 4 mmHg; NRO stimulation = 127 ± 3 before CSF and 129 ± 5 mmHg after CSF; HR: 378 ± 13 to 380 ± 15 bpm; NRO stimulation = 300 ± 17 before CSF and 303 ± 18 bpm after CSF; Figure 3).

Figure 2.

A, Tracings from one rat showing the cardiovascular and respiratory responses to nucleus raphe obscurus (NRO) stimulation (10 s at 100 Hz, 60 µA, and 1-ms pulse duration) before and after bilateral microinjection of kynurenic acid (Kyn, 2.7 nmol/200 nl) within the rostral ventrolateral medulla (RVLM). BP, pulsatile blood pressure; MAP, mean arterial BP; HR, heart rate; Resp, respiration. The triangles denote electrical stimulations, and the arrow indicates microinjection. B, The left representative section shows the location of the NRO stimulation site. The illustration on the right shows the injection site within the RVLM.

[View larger version of this image (14 K GIF file)]

Figure 3.
Effect on mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) of bilateral microinjections of cerebrospinal fluid (CSF, 200 nl) or kynurenic acid (Kyn, 2.7 nmol/200 nl) within the rostral ventrolateral medulla and effect of electrical nucleus raphe obscurus stimulation (NROS). B1, baseline values; B2, post-drug baseline values. Data are reported as means ± SEM for 7 rats. *P<0.01 compared to the preceding baseline value (Student
t-test).

[View larger version of this image (33 K GIF file)]

Effects of EAA receptor antagonism in the CVLM on the responses to NRO stimulation

In another group of animals (N = 7) in which Kyn was microinjected bilaterally within the CVLM, BP increased, HR was not significantly altered and respiration was completely blocked. HR responses were found to be variable; for instance, in Figure 4 one such tracing is shown, where an attenuation of HR was observed.

Statistical analysis of the pooled data (Figure 5)showed that Kyn injected bilaterally into the CVLM provoked an increase in MAP (89 ± 3 to 124 ± 4 mmHg, P<0.01, N = 7), and that the pressor response to NRO stimulation was slightly attenuated (DMAP = +48 ± 4 to +43 ± 3 mmHg after Kyn, P<0.05, N = 7).

Nonsignificant changes in cardiovascular and respiratory parameters to NRO stimulation were induced by CSF microinjections into the CVLM (baseline: MAP = 91 ± 4 to 92 ± 5 mmHg; NRO stimulation: DMAP = +41 ± 4 to +41 ± 5 mmHg; baseline: HR = 367 ± 31 to 369 ± 29 bpm; NRO stimulation: DHR = -19 ± 26 to -25 ± 23 bpm, before and after CSF, respectively, N = 6).

Bilateral Kyn microinjection into the CVLM induced an increase in basal BP and a statistically significant reduction of the pressor response to NRO stimulation. Therefore, a separate group of rats with unilateral Kyn microinjection was used to determine the influence of changes in basal BP on the reduction of NRO responses. After unilateral Kyn injection, which induced a smaller increase in basal BP and did not block respiration, no significant effects were observed on the pressor responses to NRO stimulation (DMAP = +46 ± 5 before Kyn and +48 ± 5 after Kyn, N = 6; data not shown). The use of this second group proved that the reduction in the pressor response was due to alteration in basal BP and not to a real blockade of the NRO response.

Figure 4.

A, Tracings from one rat showing the cardiovascular and respiratory responses to nucleus raphe obscurus (NRO) stimulation (10 s at 100 Hz, 60 µA, and 1-ms pulse duration) before and after bilateral microinjection of kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal ventrolateral medulla (CVLM). BP, pulsatile blood pressure; MAP, mean arterial BP; HR, heart rate; Resp, respiration. The triangles denote stimulations, and the arrow indicates microinjection. B, The left representative section shows the location of the NRO stimulation site. The illustration on the right shows the injection site within the CVLM.

[View larger version of this image (12 K GIF file)]

Figure 5.
Effect on mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) of bilateral microinjections of cerebrospinal fluid (CSF, 200 nl) or kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal ventrolateral medulla and effects of electrical nucleus raphe obscurus stimulation (NROS). B1, baseline values; B2, post-drug baseline values. Data are reported as means ± SEM for 7 rats.
+P<0.05 for B2 compared to B1 and *P<0.01 compared to preceding baseline value, B1 (ANOVA).

[View larger version of this image (30 K GIF file)]

Effects of EAA receptor antagonism in the CPA on the responses to NRO stimulation

The cardiovascular and respiratory changes after NRO stimulation mediated by bilateral Kyn microinjections within the CPA are shown in Figure 6. BP fell, HR was reduced and Kyn also induced respiratory arrest. Bilateral microinjections of Kyn within the CPA significantly reduced both basal MAP (before Kyn = 96 ± 2, after Kyn = 59 ± 4 mmHg, P<0.01, N = 7; Figure 7), and the pressor response to NRO stimulation (DMAP = +46 ± 4 mmHg before Kyn, +4 ± 2 mmHg after Kyn, P<0.01), while the vehicle (CSF) had no effect on either basal parameters (MAP before CSF = 93 ± 3, after CSF = 92 ± 2 mmHg, N = 6), or NRO stimulation (DMAP before CSF = +41 ± 4, after CSF = +40 ± 4 mmHg, N = 6).

Basal HR was significantly reduced by Kyn microinjection (control = 400 ± 7, after Kyn = 331 ± 14 bpm, P<0.01, N = 7; Figure 7) while CSF induced no obvious change in baseline HR (before Kyn = 367 ± 22, after Kyn = 366 ± 22 bpm, N = 6). The HR response to NRO stimulation was not significantly reduced after Kyn (DHR before Kyn = -10 ± 16, after Kyn = -1 ± 3 bpm, N = 7) or CSF (DHR before CSF = -20 ± 9, after CSF = -18 ± 8 bpm, N = 6).

Figure 6.

A, Tracings from one rat showing the cardiovascular and respiratory responses to nucleus raphe obscurus (NRO) stimulation (10 s at 100 Hz, 60 µA, and 1-ms pulse duration) before and after bilateral microinjection of kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal pressor area (CPA). BP, pulsatile blood pressure; MAP, mean arterial BP; HR, heart rate; Resp, respiration. The triangles denote stimulations, and the arrow indicates microinjection. B, The left representative section shows the location of the NRO stimulation site. The illustration on the right shows the injection site within the CPA.

[View larger version of this image (12 K GIF file)]

Figure 7.
Effect on mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) of bilateral microinjections of cerebrospinal fluid (CSF, 200 nl) or kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal pressor area, and effects of electrical nucleus raphe obscurus stimulation (NROS). B1, baseline values; B2, post-drug baseline values. Data are reported as means ± SEM for 6 rats.
+P<0.01 comparing B2 with B1 and *P<0.01 compared to preceding baseline values (ANOVA).

[View larger version of this image (49 K GIF file)]

Discussion

Electrical stimulation has become a useful tool to study the participation of the NRO in autonomic control in various species (2,3) by permitting a larger sampling rate in each experiment. The weakness of this technique is that it excites not only cell bodies but also fibers passing through the region. In contrast, neurochemical stimulation preferentially stimulates cell bodies. To avoid this problem the stimulation parameters were chosen so as to minimize current spread and activation of fibers of passage. These same stimulation parameters were previously used in the rat and other species in which they were paired with neurochemical stimulation, with the two different techniques yielding similar results (3-5). The present experimental protocol requires a large number of NRO stimulations separated by a short time interval so as to capture the full result of EAA receptor blockade in the different areas of the ventral medulla. These requirements make it difficult to use neurochemical stimulation of the NRO since tachyphylaxis will limit the number of successive doses of EAA that can be administered and will also force the experimenter to markedly increase the time interval between doses. In view of these limitations, we decided to use electrical stimulation in our experimental protocol.

As stated before, the present study was designed to evaluate the role of EAA receptors of the VLM in the cardiovascular responses to electrical NRO stimulation in the rat. Previous results have suggested that functional integrity of the RVLM is essential to obtain pressor responses evoked by electrical NRO stimulation (15) and that the NRO does not project directly to the IML (12,13). A particularly dense anatomical projection from the NRO to RVLM has been demonstrated (14,27). The cited authors suggest that these projections are mainly serotonergic but do not provide evidence for their function.

EAA receptors within the RVLM do not participate in the pressor responses to NRO stimulation since bilateral microinjections of Kyn (an antagonist of ionotropic EAA receptors) into the RVLM did not block the effects of NRO stimulation activity, although they blocked the HR responses to NRO stimulation, demonstrating that these receptors were probably involved in cardiac regulation following NRO stimulation. It was not clear if HR responses were due to direct NRO cell stimulation or to a secondary reflex response evoked by the baroreflex or the chemoreflex. Dreteler et al. (7) observed mild bradycardia in response to electrical NRO stimulation, which was often associated with the baroreflex. On the other hand, Amano et al. (28) and Koshiya et al. (29) demonstrated that bilateral microinjection of Kyn into the RVLM blocked the sympathetic chemoreflex response but left the sympathetic baroreflex response intact. Also, glutamate microinjection into the NRO resulted in a decrease in BP and HR in rabbits (8). Therefore it is possible that NRO neurons can inhibit cardiac sympathetic activity directly or indirectly within the RVLM without affecting the pressor responses. This differential activation has been previously demonstrated when the NRO is stimulated (30). Nevertheless, the changes in HR observed could also be due to activation of the nucleus ambiguus and or the peri-ambiguus region by NRO stimulation.

Another possibility tested was that the effects of electrical NRO stimulation were mediated by EAA receptors within the CVLM or CPA. The results showed that, despite the CVLM-mediated sympathoinhibitory activity on the RVLM (20), the EAA receptors were not involved in the NRO responses. However, they indicated that the pressor response induced by NRO stimulation in anesthetized rats is mediated by ionotropic EAA receptors in the CPA. Preliminary studies from our laboratory have demonstrated anatomical projections of the NRO to the CPA (31), suggesting that EAA receptors in the CPA play a role in the expression of the pressor response to electrical NRO stimulation. These results agree with other studies showing that the CPA is involved in cardiovascular control in anesthetized rats (22,24,26). However, the precise nature of this participation is not clear. One such possibility was proposed by Natarajan and Morrison (26), who demonstrated a pathway from CPA to RVLM involving sympathoexcitatory neurons in the vicinity of the CVLM. The present study suggests the existence of a pathway from CPA to RVLM mediating the pressor response elicited by NRO activation, but the precise nature of these projections has not been fully identified.

Address for correspondence: H.A. Futuro Neto, Av. Marechal Campos, 1468, 29040-090 Vitória, ES, Brasil. Fax: +55-27-3335-7330. E-mail: futuront@npd.ufes.br

Research supported by CNPq and FINEP. Received August 7, 2001. Accepted June 24, 2002.

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  • Figure 1. Mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) before and after nucleus raphe obscurus (NRO) stimulation. B1, baseline before stimulation. Data are reported as means ± SEM for all 39 rats. *P<0.01 compared to B1 (Student t-test).
  • Figure 2. A, Tracings from one rat showing the cardiovascular and respiratory responses to nucleus raphe obscurus (NRO) stimulation (10 s at 100 Hz, 60 µA, and 1-ms pulse duration) before and after bilateral microinjection of kynurenic acid (Kyn, 2.7 nmol/200 nl) within the rostral ventrolateral medulla (RVLM). BP, pulsatile blood pressure; MAP, mean arterial BP; HR, heart rate; Resp, respiration. The triangles denote electrical stimulations, and the arrow indicates microinjection. B, The left representative section shows the location of the NRO stimulation site. The illustration on the right shows the injection site within the RVLM.
  • Figure 3. Effect on mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) of bilateral microinjections of cerebrospinal fluid (CSF, 200 nl) or kynurenic acid (Kyn, 2.7 nmol/200 nl) within the rostral ventrolateral medulla and effect of electrical nucleus raphe obscurus stimulation (NROS). B1, baseline values; B2, post-drug baseline values. Data are reported as means ± SEM for 7 rats. *P<0.01 compared to the preceding baseline value (Student t-test).
  • Figure 4. A, Tracings from one rat showing the cardiovascular and respiratory responses to nucleus raphe obscurus (NRO) stimulation (10 s at 100 Hz, 60 µA, and 1-ms pulse duration) before and after bilateral microinjection of kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal ventrolateral medulla (CVLM). BP, pulsatile blood pressure; MAP, mean arterial BP; HR, heart rate; Resp, respiration. The triangles denote stimulations, and the arrow indicates microinjection. B, The left representative section shows the location of the NRO stimulation site. The illustration on the right shows the injection site within the CVLM.
  • Figure 5. Effect on mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) of bilateral microinjections of cerebrospinal fluid (CSF, 200 nl) or kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal ventrolateral medulla and effects of electrical nucleus raphe obscurus stimulation (NROS). B1, baseline values; B2, post-drug baseline values. Data are reported as means ± SEM for 7 rats. +P<0.05 for B2 compared to B1 and *P<0.01 compared to preceding baseline value, B1 (ANOVA).
  • Figure 6. A, Tracings from one rat showing the cardiovascular and respiratory responses to nucleus raphe obscurus (NRO) stimulation (10 s at 100 Hz, 60 µA, and 1-ms pulse duration) before and after bilateral microinjection of kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal pressor area (CPA). BP, pulsatile blood pressure; MAP, mean arterial BP; HR, heart rate; Resp, respiration. The triangles denote stimulations, and the arrow indicates microinjection. B, The left representative section shows the location of the NRO stimulation site. The illustration on the right shows the injection site within the CPA.
  • Figure 7. Effect on mean arterial blood pressure (MAP; panel A) and heart rate (HR; panel B) of bilateral microinjections of cerebrospinal fluid (CSF, 200 nl) or kynurenic acid (Kyn, 2.7 nmol/200 nl) within the caudal pressor area, and effects of electrical nucleus raphe obscurus stimulation (NROS). B1, baseline values; B2, post-drug baseline values. Data are reported as means ± SEM for 6 rats. +P<0.01 comparing B2 with B1 and *P<0.01 compared to preceding baseline values (ANOVA).
  • Correspondence and Footnotes

  • Publication Dates

    • Publication in this collection
      13 Oct 2002
    • Date of issue
      Oct 2002

    History

    • Accepted
      24 June 2002
    • Received
      07 Aug 2001
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