Cardiovascular changes induced by central hypertonic saline are accompanied by glutamate release in awake rats

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Cardiovascular changes induced by central hypertonic saline are accompanied by glutamate release in awake rats

Qing-Hua Jin¹, Yuto Ueda², Yuta Ishizuka², Takato Kunitake¹, and Hiroshi Kannan¹

¹ Department of Physiology and ² Department of Psychiatry, Miyazaki Medical College, Miyazaki 889 - 1692, Japan

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS AND MATERIALS
RESULTS
DISCUSSION
REFERENCES

To elucidate neurochemical mechanisms responsible for cardiovascular responses induced by central salt loading, we directlyperfused the paraventricular nucleus (PVN) of the hypothalamusregion with hypertonic saline (0.3 or 0.45 M) by using an in vivobrain microdialysis technique. We then measured the extracellularconcentrations of glutamate in the PVN region in conscious ratsalong with the blood pressure and heart rate. Blood pressure,heart rate, and glutamate levels were increased by perfusion of0.45 M saline; however, they did not change by perfusion of 0.3M saline. Next, we examined the possible involvement of glutamatein the cardiovascular responses induced by hypertonic saline.Dizocilpine, a noncompetitive antagonist of the N-methyl-D-aspartate(NMDA) receptor, attenuated the increases of blood pressure andheart rate, although 6-cyano-7-nitroquinoxaline-2,3-dione, anantagonist of the non-NMDA receptor, did not affect the bloodpressure and heart rate. Our results show that local perfusionof the hypothalamic PVN region with hypertonic saline elicitsa local release of glutamate, which may act via NMDA-type glutamatereceptors to produce cardiovascularresponses.

paraventricular nucleus; blood pressure; heart rate; microdialysis

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS AND MATERIALS RESULTS DISCUSSION REFERENCES

THE OSMOTIC HOMEOSTASIS and ionic balance of the body are mainly regulated by neural and humoral factors through the centralnervous system (CNS). Despite its clinical and physiological significance,however, little is known about the underlying cellular and molecularmechanisms by which the osmotic and ionic balances of the CNSare maintained in conscious and freely moving animals. Salt loadingis a potent stimulus for drinking, vasopressin (AVP) secretion,and increasing arterial blood pressure. Acute saline injectionseems to activate osmoreceptive structures, including those inthe subfornical organ and the anteroventral third ventricle (AV3Vregion) (17, 39), subsequently stimulating AVP secretion andneurons related to cardiovascular and behavioral responses inthe hypothalamus and brain stem (50). In addition, a numberof studies have pointed to the importance of the hypothalamicparaventricular nucleus (PVN) in the regulation of body fluidhomeostasis and in the central control of cardiovascular function(36, 46). The PVN is involved in the control of not only theneurohypophysial system but also the adenohypophysial system andautonomic nervous outflow (21). Several authors, employing electrophysiologicalmethods, have shown that, in addition to the supraoptic nucleus(SON), the PVN is a region where neurons sensitive to changesin osmolality and/or NaCl concentration are located (9, 13,26, 31, 40). Recent research has also shown that systemicadministration of hypertonic saline activates cells in the PVNand SON (16, 28, 41). Moreover, an increased c-Fos expressionin the PVN after dehydration and salt loading further confirmedthe role of this area in the regulation of body fluid balance(12, 39). Thus the PVN appears to be an important regulatoryregion of the hypothalamus that plays a critical role in the modulationof cardiovascular, neuroendocrine, and behavioral responses duringosmoticchallenges.

It has been reported that direct stimulation of the PVN and SON with a high-NaCl perfusion medium via microdialysis probesresulted in increased AVP and oxytocin release both locally intoextracellular fluid and into systemic circulation (14, 15,25, 29, 38). Similar releases of angiotensin (43), aminoacids, and dopamine (18) after local perfusion of hypertonicsaline have also been reported, and the findings have been interpretedas evidence for the roles of these substances in the central osmoticand ionic balance. However, the roles of endogenous neurochemicalsin the PVN responsible for cardiovascular responses induced bysalt loading remain to be elucidated. Glutamate (Glu) has beenrecognized as an important neurotransmitter/neuromodulator inthe CNS, mediating most of the excitatory synaptic transmission.An injection of Glu into the PVN raised blood pressure and heartrate (HR) accompanied with increases in plasma catecholamines(30). These findings raise the possibility that Glu may be involvedin the responses induced by central hypertonic salinestimulation.

In some cases, anesthesia, well known for its profound effect on cardiovascular and autonomic function, reverses the responses(21, 32). Microdialysis is a useful method for pharmacologicalassessment and manipulation of the microenvironment in the brainof conscious and freely moving animals, in which changes in osmolalityor NaCl concentration, extracellular amino acids, and relatedmediator levels can be manipulated and measured (2). Therefore,in the present study, we have used a microdialysis technique toinvestigate the release of Glu in response to local stimulationwith hypertonic saline and to monitor cardiovascular responsesin conscious and freely moving rats. In addition, to test whetherthe observed Glu release is involved in the cardiovascular responses,N-methyl-D-aspartate (NMDA) and non-NMDA receptor antagonistswere coadministered with hypertonic saline stimulation, and thecardiovascular responses that were induced by hypertonic salinewereexamined.

	METHODS AND MATERIALS

TOP ABSTRACT INTRODUCTION METHODS AND MATERIALS RESULTS DISCUSSION REFERENCES

Animals and surgical procedures. Male Wistar rats, weighing 350-450 g at the start of the experiments, were used in our study. The experiments were performedin accordance with the National Institutes of Health Guide forthe Care and Use of Laboratory Animals [DHEW Publication No. (NIH)85-23, Revised 1985, Bethesda, MD] and were approved by the Committeeon Animal Care of Miyazaki Medical College. The rats were anesthetizedwith pentobarbital sodium (50 mg/kg ip) 5 days before the experiments.An arterial catheter (SP-31 polyethylene tubing heat-coupled toSP-50) was inserted into the surgically exposed abdominal aortafor measurement of arterial blood pressure (BP) and HR and tunneledunder the skin to exit at the nape of the neck. A guide cannula(0.50-mm ID, 0.70-mm OD) for the placement of a microdialysisprobe was stereotaxically implanted 2.0 mm above the PVN accordingto the atlas of Paxinos and Watson (42) and sealed with a dummycannula after implantation. The stereotaxic coordinates were 1.7mm posterior to the bregma, 0.3 mm lateral to the midline, and6.7 mm ventral to the dural surface. To determine whether thedirect effects of hypertonic saline (HTS) were specific to thePVN, the guide cannula was implanted into the outside of the PVNregion (1 mm rostral to the PVN, n = 2; 1 mm lateral to the PVN,n = 3) as an anatomic control group. A head plate for the fixationof the arterial catheter and a guide cannula were fitted to theskull by dentalcement.

Experimental procedure. On the day before the experiment, the animals were anesthetized with isoflurane (2.5-3.0% in 100% oxygen), and the dummy cannulaswere replaced with microdialysis probes. To reach the PVN region,the tip of the probe covered with a 2.0-mm length of hollow fibers(200-µm OD, cellulose acetate membrane, cut-off 4.8 × 10⁴ mol wt; Terumo, Japan) was set to extend 2 mm beyond the guideshaft, and a similar operation was performed in the anatomic controlgroup. So that they would get used to the environment in whichthe experiment would later be performed, the animals were placedin cylindrical metabolic cages (28-cm diameter × 28-cm height)that were controlled by computers. This system can protect thearterial catheter and tubes connected to the probe from the twistinduced by the movement of rats, allowing for long-term recordingwithout twisting. On the day of the experiments, the collectionof dialysates for the Glu and cardiovascular measurements werecarried out while the animals were permitted to move about freelyin their cages. The microdialysis probe was perfused with modifiedRinger solution (147 mM NaCl, 4 mM KCl, 2.3 mM CaCl₂; pH 6.5)at a constant rate of 1 µl/min using a microinfusion pump. Theperfusate from the PVN region was collected manually in an Eppendorftube every 20 min. After a 2-h stabilization period, two consecutivedialysate samples were collected to measure the baseline Glu levels.All samples of collected dialysates were kept at $-$ 80°C for lateranalysis. The arterial catheter was connected to a pressure transducer(P23 ID, Gould, Singapore) to monitor BP, while the HR was countedby BP wave. The BP and HR were monitored simultaneously and recordedon a thermal pen-writing recorder (RJG-4122, Nihon Kohden, Japan)and on an FM magnetic tape recorder (RM-7000, Sony, Tokyo, Japan).The mean arterial pressure (MAP) was obtained by electronic averagingof the pulsatile arterial pressuresignal.

The Glu levels were measured by using high-performance liquid chromatography with electrochemical detection (HPLC-ECD). Beforeapplying the HPLC-ECD method, an o-phthalaldehyde (OPA) solution(40 mM) was made by adding 13.5 mg of OPA and 10 µl of 2-mercaptoethanolto 2.5 ml of 0.1 M K₂CO₃ buffer (pH 9.5) with 10% ethanol. Thesolution was then stored at $-$ 4°C and diluted in 0.1 M K₂CO₃ toyield a 4 mM OPA solution just before detection. The dialysate(18 µl) was mixed with 5 µl of the 4 mM OPA solution and allowedto react for 3 min at 25°C incubation. After completing the reaction,20 µl of the reaction mixture was applied to HPLC with an EicompakMA-5 ODS column (4.6-mm ID × 150 mm; Eicom, Tokyo, Japan). Detectionwas accomplished with an ECD (Eicom) with +700 mV Ag/AgCl electrodes.The elution buffer for the Glu was 0.1 M phosphate buffer, 30%methanol, and 0.5 mM EDTA (pH 6.5).

At the end of each experiment, the rats were killed with an overdose injection of pentobarbital sodium, and their brains werefixed in 10% neutral-buffered formalin. The implantation siteof the dialysis probe was verified histologically in 40-µm coronalsections after cresyl violetstaining.

Reagents. HTS with two different tonicities, 0.3 and 0.45 M (the osmolalities were 591 and 900 mosmol/kgH₂O, respectively), was usedin this experiment to observe the responses. The PVN region wasperfused with the HTS through the microdialysis probe at a constantrate of 1 µl/min for 20 min. Physiological saline (0.15 M NaCl)was used in this experiment as a control. In addition, 0.6 M mannitol(Nacalai Tesque, Kyoto, Japan) dissolved in the physiologicalsaline (the osmolality is 904 mosmol/kgH₂O) was perfused in thePVN via the microdialysis probe for 20 min, and 1 mM NMDA (NacalaiTesque) dissolved in the modified Ringer solution was perfusedfor 10min.

Dizocilpine (MK-801; Sigma), an NMDA-receptor antagonist, was dissolved in the modified Ringer solution (1 mM), and 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX; Sigma), a non-NMDA-receptor antagonist, was dissolved ina 0.1 N NaOH solution (1 mM). The drugs were then stored at 4°C.To measure the effect of these drugs on the responses inducedby HTS stimulation, both drugs were diluted with 0.45 M NaCl to100 µM, and the mixtures were administered via the microdialysisprobe. The same vehicles used to dilute the drugs were given atthe same concentration in the 0.45 M saline, and this solutionserved in this experiment as the vehiclecontrol.

Statistical analysis. All data are expressed as means ± SE, and statistical analysis was performed using ANOVA followed by Fisher's protected leastsignificant difference test. To provide a temporal descriptionof the cardiovascular responses, the area under the curve (AUC)was also calculated (1). A comparison of the maximal changesin BP and HR and in AUC between the PVN group and the anatomiccontrol group was carried out by a paired Student's t-test. Aprobability level of P < 0.05 was considered statisticallysignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS AND MATERIALS RESULTS DISCUSSION REFERENCES

In the present study, the baseline levels are the average of baseline values before stimulation in each parameter. The baselinelevels for MAP, HR, and Glu are shown in Table 1, with no significantdifferences between the groups. (See Fig. 2, top, for the exactpositioning of the probe.)

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Table 1. Baseline levels of MAP, HR, and Glu concentration in the PVN

Figure 1 shows the effect on MAP and HR of direct infusion of HTS into the PVN region for 20 min through a dialysis probe.The local perfusion of 0.45 M saline elicited significant increasesin MAP and HR from the baseline levels of 96.7 ± 3.6 mmHg and285.3 ± 3.5 beats/min to the maximums of 114.4 ± 2.4 mmHg and394.0 ± 10.7 beats/min, respectively. The MAP and HR began toincrease 12 min after starting the perfusion and returned to thebasal levels ~15 min after the perfusion was stopped. However,the 0.3 M saline did not cause significant increases in MAP andHR, although the maximums reached 99.8 ± 3.7 mmHg and 336.5 ±18.1 beats/min, respectively (baseline levels in this group were93.6 ± 1.9 mmHg and 297.6 ± 9.7 beats/min, respectively).

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Fig. 1. Effects of direct infusion of hypertonic saline (HTS) into the paraventricular nucleus (PVN) through microdialysis probes on mean arterial pressure (MAP; A) and heart rate (HR; B). In Figs. 1, 3, and 5-7, MAP and HR are shown by changed amounts from baseline levels, and horizontal bars show period of perfusion. Data are means ± SE. * P < 0.05 compared with 0.15 M NaCl group; + P < 0.05 compared with 0.3 M NaCl group.

To investigate whether the increases in BP and HR in response to local administration of HTS were specific to the PVN, perfusionof 0.45 M saline into a region outside the PVN [~1 mm rostral(n = 2) or lateral (n = 3)] was performed (Fig. 2, middle andbottom). In this anatomic control group, BP and HR did not showsignificant increases after 0.45 M saline perfusion, althoughthe maximal changes reached 7.2 ± 2.7 mmHg and 39.2 ± 22.2 beats/min,respectively. The maximal changes in the HTS perfusion of thePVN region were 20.9 ± 2.6 mmHg and 115.9 ± 8.7 beats/min, respectively,which were strikingly larger than the anatomic control group.

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Fig. 2. Photomicrographs of a typical placement of the unilateral microdialysis probe in the PVN (top) and rostral (middle) and lateral to the PVN (bottom). Arrows indicate tip of the microdialysis probe. SCh, suprachiasmatic nucleus.

In addition, a 0.6 M mannitol solution dissolved in the 0.15 M saline was used to determine whether the cardiovascular responsesto direct HTS perfusion into the PVN region were caused by a changein ions, sodium chloride, or osmolality. The mannitol solution,its osmolality approximately equivalent to 0.45 M saline, causedlittle increase in BP and HR after the perfusion was stopped (Fig.3). The maximal changes were only 4.7 ± 2.5 mmHg and 42.1 ± 14.9beats/min, respectively. As shown in Fig. 3, the responses ofBP and HR to the mannitol were markedly less than they were toNaCl, and their durations were also shorter than they were inthe NaCl group.

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Fig. 3. Comparison between 0.45 M NaCl and 0.6 M mannitol groups in responses of MAP (A) and HR (B) induced by direct perfusion of the PVN. Data are means ± SE.* P < 0.05 compared with baseline levels; + P < 0.05 compared with 0.6 M mannitol group.

The effect of local stimulation of PVN with HTS on Glu levels in the PVN region is summarized in Fig. 4. The Glu levels inthe PVN region showed an immediate increase by the local administrationof 0.45 M saline, which reached to 249.8 ± 54.7% of the basallevel. The elevated Glu levels remained after the perfusion andalmost returned to the basal levels at 40 min after the perfusionwas stopped. The direct perfusion of 0.3 M saline increased theGlu levels to 118.4 ± 7.4% of the basal level, but there was nosignificant difference compared with the control group with 0.15M NaCl.

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Fig. 4. Effects on glutamate (Glu) level in the PVN by direct infusion of HTS into the PVN through microdialysis probes. Glu levels are expressed as percentages of baseline levels. Horizontal bar shows period of perfusion. Data are means ± SE. * P < 0.05 compared with 0.15 M NaCl group; + P < 0.05 compared with 0.3 M NaCl group.

Figure 5 shows the effects of MK-801 on the responses of MAP and HR that were induced by 0.45 M saline. Coadministration ofMK-801 (100 µM) with HTS significantly attenuated the increasedresponses of MAP and HR. The AUC in the MAP and HR was changedfrom 314.0 ± 70.7 mmHg · m and 1,791.6 ± 465.4 beats/min · m ofthe vehicle control group to 85.8 ± 21.1 mmHg · m and 533.3 ±206.6 beats/min · m (both P < 0.05), respectively. On the otherhand, the responses of MAP and HR, induced by direct perfusionof 0.45 M saline into the PVN, were not influenced by CNQX (100µM; Fig. 6). The AUC in the MAP and HR in the CNQX group was 209.9± 23.7 mmHg · m and 1,119.8 ± 149.9 beats/min · m, and in thevehicle group it was 295.0 ± 73.7 mmHg · m and 1,320.3 ± 396.2beats/min · m, respectively (both P > 0.05).

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Fig. 5. Effects of MK-801 (100 µM) on HTS-induced increases in MAP (A) and HR (B). Data are means ± SE. * P < 0.05 compared with baseline levels; + P < 0.05 compared with vehicle group.

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Fig. 6. Effects of 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX; 100 µM) on HTS-induced increases in MAP (A) and HR (B). Data are means ± SE. * P < 0.05 compared with baseline levels.

Finally, effects of direct perfusion of NMDA into the PVN region on BP and HR were examined. BP and HR increased strikinglyby perfusion of 1 mM NMDA. The maximal changes reached ~25.0 ±3.6 mmHg and 132.4 ± 11.8 beats/min, respectively, and the increasesremained at high levels for 15 min after the NMDA perfusion wasstopped (Fig. 7).

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Fig. 7. Effect on MAP (A) and HR (B) of direct infusion of N-methyl-D-aspartate (NMDA) into the PVN through a dialysis probe. Data are means ± SE. * P < 0.05 compared with vehicle group.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS AND MATERIALS RESULTS DISCUSSION REFERENCES

This study demonstrates that dialysis with hypertonic saline in the PVN region results in increased BP and HR accompaniedwith an increase in the Glu level in the dialysates obtained fromthe PVN. These changes are related to the tonicity of the hypertonicsaline. Any consideration of the effects of hypertonic salinesolution requires recognition of whether either osmotic or ion-specificfactors are involved. In the PVN, some neurons show excitationand others show inhibition in response to hypertonic saline andother osmotic stimuli in vitro and in vivo (11, 13, 36,40, 52). On the other hand, in vivo local microdialysis of1 M hypertonic saline elicited oxytocin release in the PVN, whereasdialysis with equimolar mannitol did not (14). Present workshowed that equiosmotic mannitol perfusion in the PVN showed amuch lesser cardiovascular effect than the hypertonic saline solutionin conscious rats (Fig. 3). Therefore, the results observed inthe present studies with hypertonic saline solution might be muchmore dependent on an ion effect, i.e., Na⁺ or Cl, than on an osmotic effect. In this regard, Eriksson and colleagues(10) found in the goat that antidiuretic and thirst responsescould be induced by intracerebroventricular (icv) infusion ofhypertonic NaCl but not by solutions of equivalent osmolaritymade from sucrose in water. They proposed that a periventricularsodium-sensitive receptor system, located in the vicinity of thethird ventricle, was responsible for the regulation of antidiuresis,thirst, and renal Na excretion. However, McKinley and colleagues(33) revealed that icv infusion of hypertonic sucrose in sheepcan elicit thirst and antidiuresis if the solution contains sufficientamounts of NaCl to prevent the osmotic dilution of cerebrospinalfluid (CSF) Na. These results provided support for the involvementof osmoreceptors. Whether sodium and/or an osmoreceptor is involvedin the cardiovascular responses that are induced by salt loadingremains to be elucidated. Because cardiovascular responses inducedby local perfusion of hypertonic saline in the PVN region weremore prominent than those induced by mannitol in the present study,activation of NaCl receptors rather than osmoreceptors might beinvolved in the cardiovascular responses induced by hypertonicsaline.

Considerable evidence exists that extracellular concentrations of putative amino acid neurotransmitters are also affectedby osmotic and/or NaCl changes in the microenvironment (4,47, 49). It is known from immunocytochemical and physiologicalstudies that glutamatergic synaptic terminals innervate neuronsin the PVN and control their activity (7, 8, 34, 48).In addition, the injection of Glu into the PVN evoked the increasesof MAP, HR, and plasma catecholamines (30), and the unilateralinfusion of the PVN region with Glu produced a great increaseof plasma oxytocin level (15).

Therefore, we asked whether the release of Glu on local stimulation with hypertonic saline solutions is involved in the cardiovascularresponses. If so, blockade of glutamatergic synaptic transmissionwith antagonists could modify the cardiovascular responses. Wefound an increase in extracellular Glu concentration after localperfusion of hypertonic saline. Furthermore, the NMDA-receptorblocker MK-801, but not the non-NMDA-receptor antagonist CNQX,attenuated cardiovascular responses after local perfusion of thePVN with hypertonic saline, and local injection of NMDA into thePVN region evoked increases in BP and HR. Glu excites parvocellularneurons in the PVN (8), some of which project directly to thepreganglionic sympathetic neurons in the intermediolateral cellcolumn of the spinal cord (44, 46). Electrical and chemicalstimulation of the PVN increases BP and renal sympathetic nerveactivity in conscious rats (21). Therefore, released Glu inthe PVN might be involved in the cardiovascular responses inducedby hypertonicsaline.

Hypertonic saline stimulation of the PVN and SON was reported to increase AVP and oxytocin in the nuclei, with a maximum duringpoststimulation (14, 25, 28, 37, 38). In contrast tothese studies on hypothalamic oxytocin and AVP release, we observedthat the stimulated release of Glu in the PVN was quantitativelyrelated to the increase in tonicity, which increased immediatelyduring the hypertonic saline stimulation and returned graduallyto baseline when the stimulus was withdrawn. These findings suggestthat a mechanism different from the one operating for AVP andoxytocin release is responsible for Glu release in the PVN regionunder hypertonic salineloading.

The mechanism that triggers the hypertonic saline-induced release of amino acids is not known. One plausible explanation isthat the amino acids are released as neurotransmitters in responseto direct NaCl and/or osmotic stimulation of the neurons of theirorigin (18). In this regard, Glu, $gamma$ -aminobutyric acid, and glycinecan be released from nerve terminals through their carrier byexchanging with extracellular amino acids sharing the same transportsystem (22, 27). Therefore, it is unclear which of the releasedsubstances may trigger a possible secondary amino acid substance.Another possible explanation could involve pH changes due to activationof the plasmalemmal sodium/hydrogen exchanger (20) or sodium/calciumexchange mechanisms, causing the release of intracellular calciumfrom internal stores such as mitochondria (6), resulting infacilitation of exocytosis. It has been known for many years thatincreases in the frequency of spontaneous miniature end-platepotentials at a neuromuscular junction occur after exposure tohigh osmotic pressure (35). Despite continued investigation,an explanation for this mechanism remains to be revealed (19,23). However, the question arises whether the measured extracellularconcentrations of Glu within the PVN originated from neuronalor glial release. Both glial cells and neurons contain Glu, andthe release could have come from either cellular compartment.The possible release of Glu from glia rather than, or in additionto, that from neuronal axon terminals raises the possibility ofthe reversal of normal glial Glu uptake by transporters due todisturbance of the ionic concentration of the extracellular milieu.A recent study by Landgraf and colleagues (18) demonstratedthat the changes in extracellular amino acid concentration withinthe PVN are calcium dependent for some amino acids but not forothers. Thus it can be presumed that local perfusion with hypertonicsaline solution evokes an increase in Glu release in the PVN throughmultiplepathways.

Excitatory amino acid (EAA) receptors have been implicated in cardiovascular and body fluid regulation at the brain stem andhypothalamus levels (24, 45, 50). These ionotropic EAA receptorsare classified as NMDA and non-NMDA ( $alpha$ -amino-3-hydroxy-5-methyl4-isoxazolepropionic acid and kainate) (5). The noncompetitive NMDA-receptorantagonist MK-801 could significantly suppress the increases inBP and HR induced by local application of hypertonic saline. Thissuggests that Glu transmission through an NMDA receptor in thePVN is involved in the neural mechanism whereby hypertonic salinestimuli provoke cardiovascular activation. The non-NMDA-receptorantagonist CNQX had no effect on cardiovascular responses, suggestingthat the effects observed were specific for an NMDA subtype ofthe Glu receptor. Other findings also point to NMDA being involvedin the central regulation of body fluid balance (50, 51),such as, for example, icv administration of NMDA-stimulated dipsogenicresponses in pigeons (3).

Perspectives

The phenomenon of hypertonic saline-induced release of amino acids such as Glu appears to be constant throughout many areasof the CNS (18), although the sensitivity to hypertonic salinesolution might be different on the basis of areas examined. However,cardiovascular responses induced by injection of hypertonic salinethrough microdialysis probes were presumed to be site specific.This assumption can be supported by the following. Cardiovascularresponses were not induced or greatly attenuated after hypertonicNaCl perfusion into areas 1.0 mm rostral to or 1.0 mm lateralto the PVN, suggesting a localized site of action. However, usingmicrodialysis probes to administer or collect substances, we cannotbe certain 1) from what volume of tissue the substances releasedare collected, 2) into what volume of tissue or extracellularspace the substances administered can diffuse, and 3) what theeffective concentrations of drugs administered will be at anypoint in this sphere of influence. Therefore, we have to be guardedabout claiming very localized effects or claiming that concentrationsarephysiological.

	ACKNOWLEDGEMENTS

The hollow fibers were a gift from Terumo (Tokyo, Japan). This research was supported in part by Grants-in-Aid for ScientificResearch 10557009 and 11470019 (to H. Kannan) from the Japan Ministryof Education, Science, Sports, andCulture.

	FOOTNOTES

Address for reprint requests and other correspondence: H. Kannan, Dept. of Physiology, Miyazaki Medical College, 5200 Kihara,Kiyotake, Miyazaki 889-1692, Japan (E-mail: kannan{at}post.miyazaki-med.ac.jp).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 28 December 2000; accepted in final form 20 June 2001.

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