Blockade of Delta Opioid Receptors in the Ventrolateral Periaqueductal Gray Region Inhibits the Fall in Arterial Pressure Evoked by Hemorrhage

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Vol. 297, Issue 2, 612-619, May 2001

Blockade of Delta Opioid Receptors in the Ventrolateral Periaqueductal Gray Region Inhibits the Fall in Arterial Pressure Evoked by Hemorrhage

Sinan Cavun, Garth E. Resch, Adam D. Evec, Michelle M. Rapacon-Baker and William R. Millington

Department of Basic and Pharmaceutical Sciences, Albany College of Pharmacy, Albany, New York (S.C., W.R.M.); and School of Biological Sciences (G.E.R.) and Medicine (A.D.E., M.M.R.-B.), University of Missouri, Kansas City, Missouri

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

Severe hemorrhage lowers arterial pressure by suppressing sympathetic activity. The central mechanism that initially triggersthe fall in arterial pressure evoked by hemorrhage is not wellunderstood, although opioid neurons are thought to play a role.This study tested the hypothesis that hemorrhagic hypotensionis mediated by delta opioid receptors in the ventrolateral periaqueductalgray (vlPAG), a region importantly involved in opioid analgesia.Depressor sites were first identified by microinjecting DL-homocysteicacid (20 nmol/0.1 µl) or $beta$ -endorphin (0.5 nmol/0.1 µl) into thevlPAG of halothane-anesthetized rats. Consistent with earlierreports, DL-homocysteic acid injection into the caudal vlPAG loweredarterial pressure and heart rate; $beta$ -endorphin evoked a comparabledepressor response, but did not affect heart rate. Naloxone orselective opioid receptor antagonists were subsequently injectedinto the vlPAG 5 min before hemorrhage (1.9 or 2.5 ml/100 g ofbody weight over 20 min) was initiated using the same stereotaxiccoordinates. Naloxone injection into the caudal vlPAG completelyprevented the fall in arterial pressure evoked by hemorrhage.The response was dose-dependent and evident with both fixed volumeand fixed pressure hemorrhage. The delta opioid receptor antagonistnaltrindole inhibited hemorrhagic hypotension significantly inboth conscious and anesthetized rats but mu and kappa receptorantagonists were ineffective. $beta$ -Endorphin_1-27, an endogenousopioid receptor antagonist, was also significantly inhibitory.Naltrindole was ineffective when injected into the dorsolateralperiaqueductal gray and did not influence cardiovascular functionin nonhemorrhaged animals. These data support the hypothesis thathemorrhagic hypotension is mediated by delta opioid receptorsin the vlPAG.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

In 1979, Faden and Holiday reported that intravenous injection of naloxone, an opioid receptor antagonist, inhibited the fallin arterial pressure caused by hemorrhage in conscious rats (Fadenand Holaday, 1979). Their data have since been reproduced in animalmodels of both hemorrhagic (Sandor et al., 1987; Schadt and Ludbrook,1991; Ludbrook and Ventura, 1994) and endotoxic (D'Amato and Holaday,1984) shock and have been shown to result from a central mechanism(Sandor et al., 1987; Schadt and Ludbrook, 1991; Owen et al.,1997) that involves delta, rather than mu or kappa, opioid receptors(D'Amato and Holaday, 1984; Ludbrook and Ventura, 1994). The findingthat opioid receptor blockade prevents hemorrhagic hypotensionwas initially controversial, however, because opioid receptorantagonists produce little or no change in cardiovascular functionin normotensive animals (Gordon, 1986; Morilak et al., 1990) andbecause delta opioid receptor agonists produce hypertension whenadministered centrally to conscious animals (May et al., 1989),not the hypotension predicted by the effects of delta receptorantagonists in hemorrhage. It thus appears that naloxone preventshemorrhagic hypotension through a central mechanism that is differentfrom the baroreceptor reflex that normally regulates cardiovascularhomeostasis.

This conclusion is consistent with extensive evidence that severe hemorrhage initially lowers arterial pressure through acentral mechanism that overrides the baroreceptor reflex (Schadtand Ludbrook, 1991). Although mild hemorrhage activates the baroreflex,which thus maintains arterial pressure within normal limits, severehemorrhage produces the opposite response; it abruptly inhibitssympathetic activity and thereby initiates the precipitous fallin arterial pressure that ultimately leads to hemorrhagic shock(Schadt and Ludbrook, 1991). The ability of delta receptor antagoniststo prevent the sympathoinhibition caused by hemorrhage means thatopioid peptide neurons play a pivotal role in the response. Butlittle is known about the anatomical pathway that initially triggersthe sympathoinhibitory phase of hemorrhage and neither the identitynor the location of the opioid neurons that mediate the responseisknown.

This study tested the hypothesis that naloxone inhibits hemorrhagic hypotension by blocking delta opioid receptors in theventrolateral column of the midbrain periaqueductal gray (vlPAG)region. The vlPAG is densely innervated by opioid peptide neurons(Khachaturian et al., 1985; Martin-Schild et al., 1999) and haslong been known to play an important role in the antinociceptioncaused by severe stress and injury (Lovick, 1993). More recentinvestigations indicate that antinociception is but one componentof a coordinated autonomic and behavioral repertoire that is generatedby the PAG. Activation of neurons in the vlPAG with excitatoryamino acids produces hypotension, bradycardia, and sympathoinhibitionaccompanied by behavioral quiescence, hyporeactivity, and opioid-dependentantinociception (Lovick, 1993; Bandler et al., 2000). Similarly,visceral and deep somatic pain and injury lower arterial pressureand heart rate, produce behavioral quiescence, and activate vlPAGneurons, as evidenced by expression of the immediate/early gene,c-fos (Clement et al., 1996). In marked contrast to the vlPAG,activation of the lateral and dorsolateral PAG (dlPAG) columnswith excitatory amino acids produces hypertension, tachycardia,and behavioral activation, and dlPAG neurons express c-fos inresponse to somatic, rather than visceral, pain (Lovick, 1993;Bandler et al., 2000). These findings are consistent with thehypothesis that hemorrhagic hypotension is mediated by the vlPAG,although not the dlPAG.

We tested this hypothesis, in an earlier study, by determining whether inhibition of neuronal activity in the vlPAG with lidocainewould prevent the fall in arterial pressure evoked by hemorrhage.Microinjection of lidocaine into the caudal vlPAG delayed theonset and reduced the degree of hypotension produced by hemorrhage(Cavun and Millington, 2000). Hemorrhagic hypotension was alsoattenuated by cobalt chloride which, unlike lidocaine, does notinhibit axonal conductance and thus demonstrates that synaptictransmission within the vlPAG is necessary for hemorrhage to lowerarterial pressure. Neither lidocaine nor cobalt chloride influencedcardiovascular function in normotensive animals. These data supportthe concept that the vlPAG is a component of a descending anatomicalpathway that is activated by hemorrhage but does not participatein the tonic regulation of cardiovascularhomeostasis.

Here, we report that bilateral injection of naloxone into the caudal vlPAG essentially abolished the fall in arterial pressureevoked by hemorrhage. Naltrindole, a selective delta opioid receptorantagonist, was also effective, but mu and kappa receptor antagonistswere inactive. These data provide additional evidence that thevlPAG is a critical component of a descending pathway that initiateshemorrhagic hypotension and show that delta opioid receptors inthe vlPAG play an important role in theresponse.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Animals and Surgery. Male Sprague-Dawley rats (250-300 g; Sasco, Inc., Omaha, NE, or Taconic Farms, Germantown, NY) were housed under a 12-h light/darkcycle with free access to food and water. Rats were anesthetizedwith halothane (1.5-4% in 100% O₂), and the right carotid arterywas cannulated with PE-50 tubing filled with heparinized saline(100 U/ml). The cannula was exteriorized at the nape of the neckand sealed until use. At the beginning of each experiment, thecannula was attached to a volumetric pressure transducer and arterialpressure and heart rate were recorded at 1-min intervals usinga MicroMed BPA-200 blood pressure analyzer (Micro-Med, Louisville,KY). Body temperature was not monitored or controlled. Experimentswith conscious animals were conducted 4 to 6 h after rats recoveredfrom anesthesia. The animal protocols were conducted in accordancewith the National Institutes of Health Guide for the Care andUse of Laboratory Animals.

DL-Homocysteic Acid (DLH) and $beta$ -Endorphin Injections. Depressor sites were identified by injecting DLH, $beta$ -endorphin, or saline (pH 7.3) unilaterally into the vlPAG. Halothane-anesthetizedrats were positioned in a stereotaxic apparatus, and a 32-gaugestainless steel cannula was lowered vertically through a smallcraniotomy 0.8 mm lateral and 8.3 mm posterior to bregma to adepth of 6.2 mm below the skull surface according to the atlasof Paxinos and Watson (1998). DLH (20 nmol/0.1 µl of saline; SigmaChemical Co., St. Louis, MO) was injected over a 1-min period,and arterial pressure and heart rate were recorded for 15 min.If no change in arterial pressure occurred, the injection cannulawas lowered 0.2 mm and the injection was repeated; up to threeDLH injections were made in the same animal. Criteria includeda greater than 5% change in, and restoration to, baseline arterialpressure. When a depressor site was identified, $beta$ -endorphin (0.5nmol/0.1 µl of saline; Peninsula Laboratories, Belmont, CA) wasinjected into the samesite.

Opioid Receptor Antagonist Injections and Hemorrhage. Rats were anesthetized with halothane and two 26-gauge guide cannulae were implanted bilaterally in the caudal or rostralvlPAG or the caudal dlPAG at a 27^o rostro-caudal angle. The tips of the guide cannulae were positioned0.8 mm lateral and 8.3 mm posterior to bregma and 6.2 mm belowthe skull surface for caudal vlPAG injections, 0.8 mm lateraland 7.3 mm posterior to bregma and 6.2 mm below the skull surfacefor rostral vlPAG injections, and 0.8 mm lateral and 8.3 mm posteriorto bregma and 4.6 mm below the skull surface for caudal dlPAGinjections (Paxinos and Watson, 1998). After obtaining stablebaseline arterial pressure and heart rate measurements, naloxoneHCl (1, 3, 10, or 100 nmol), naltrindole HCl (0.2, 2, or 20 nmol),D-Phe-Cys-Tyr-D-Trp-Orn-Thr-Pen-Thr amide (CTOP; 1 or 10 nmol),nor-binaltorphimine dihydrochloride (nor-BNI; 1 or 6 nmol) (allfrom Sigma Chemical Co., St. Louis, MO), or saline was injectedbilaterally (one-half the dose in each cannula) in a volume of0.5 µl of 0.9% saline (pH 7.3) delivered at a constant rate overa 1-min period. The injection volume was monitored by observingthe movement of an air bubble placed in the tubing. Five minuteslater, hemorrhage was initiated by withdrawing blood (1.9 ml or2.5 ml/100 g of body weight) through the carotid cannula overa 20-min period. At the end of each experiment, the injectionsite was marked with 0.1 µl of India Ink for DLH and $beta$ -endorphininjections or 0.5 µl of India Ink for opioid receptor antagonistexperiments. The brain was removed, immersed in 10% paraformaldehyde,imbedded with paraffin, sectioned (50 µm) with a sliding microtome,and stained witheosin.

Statistical Analyses. Data were analyzed by analysis of variance followed by Dunnett's multiple comparisons test or two-tailed Student's t test.The criteria for statistical significance was P < 0.05.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Microinjection of DLH or $beta$ -Endorphin into the vlPAG Lowers Arterial Pressure. The hypothesis that microinjection of delta opioid receptor antagonists into the vlPAG will inhibit hemorrhagic hypotensionis based on the assumption that hemorrhage stimulates opioid peptiderelease from vlPAG neurons. This hypothesis is supported by evidencethat vlPAG administration of a delta receptor selective agonistlowers arterial pressure, whereas mu receptor agonists generatea pressor response and kappa agonists produce little or no consistenteffect (Keay et al., 1997). The $beta$ -endorphin- and enkephalin-relatedpeptides that serve as endogenous ligands for delta opioid receptorsalso display relatively high affinity for mu receptors, however(Paterson et al., 1983), which raises the possibility that $beta$ -endorphin-and enkephalin-related peptides could produce little or no neteffect on arterial pressure in the vlPAG. We therefore testedwhether $beta$ -endorphin affects arterial pressure or heart rate whenmicroinjected into DLH-responsive depressor sites in the caudalvlPAG.

DLH (20 nmol/0.1 µl) injection produced a small but significant reduction in mean arterial pressure ( $-$ 9.5 ± 1.6 mm Hg; range= $-$ 5.4 to $-$ 25.6 mm Hg) and heart rate [ $-$ 20 ± 6.9 beats per minute(bpm); range = +9 to $-$ 58 bpm] (Table 1) in 41% of sites tested,consistent with previous reports (Carrive and Bandler, 1991

; Keayet al., 1997

). The maximum fall in arterial pressure occurred2.2 ± 0.2 min following DLH injection. The duration of the responsewas 6.0 ± 0.6 min.

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TABLE 1
Effects of vlPAG DLH or $beta$ -endorphin injection on arterial pressure and heart rate
DLH (20 nmol), $beta$ -endorphin (0.5 nmol), or saline (0.1 µl) was injected unilaterally into the caudal vlPAG. Data represent the maximal change in mean arterial pressure or heart rate (mean ± S.E.), and the numbers in parentheses indicate the number of animals in each group.

$beta$ -Endorphin (0.5 nmol/0.1 µl) injection into DLH-responsive vlPAG sites evoked a depressor response comparable in magnitudeto that following DLH (Table 1) in 58% of sites tested. The maximalfall in arterial pressure ( $-$ 10.6 ± 1.9 mm Hg; range $-$ 5.9 to $-$ 17.3mm Hg) was slower to develop (4.6 ± 0.9 min) and longer in duration(11.6 ± 2.6 min) than following DLH. Analysis of variance revealeda significant effect of DLH and $beta$ -endorphin treatment on arterialpressure [F(2,28) = 19.87, P < 0.01] and heart rate [F(2,28) =6.90, P < 0.01]; post hoc analysis showed that $beta$ -endorphin didnot change heart rate significantly (Table 1). Intra-arterialnaloxone (1 mg/kg) injection prevented the hypotension evokedby $beta$ -endorphin (+4.0 ± 1.7 mm Hg), but not DLH ( $-$ 16.7 ± 3.4 mmHg). $beta$ -Endorphin thus produced naloxone- reversible hypotension,but not bradycardia, in the caudal vlPAG.

Naloxone Prevents Hemorrhagic Hypotension in the vlPAG. Subsequently, we tested, in a separate group of animals, whether naloxone injection at the same vlPAG coordinates would preventthe fall in arterial pressure evoked by hemorrhage. During fixedvolume hemorrhage (1.9 ml/100 g of body weight), arterial pressurewas sustained at baseline levels initially, but it began to fallafter 10 min and reached $-$ 37.8 ± 1.7 mm Hg below initial baselinemeasurements by the end of the 20-min hemorrhage period (Fig.1). Heart rate was not affected by hemorrhage and did not differsignificantly from baseline values (340 ± 17 bpm) at the end ofthe 20-min hemorrhage period (328 ± 44 bpm).

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Fig. 1. Naloxone inhibits hemorrhagic hypotension. Naloxone (10 nmol; 5 nmol/cannula) or saline (0.5 µl/cannula) was injected bilaterally into the caudal vlPAG of halothane-anesthetized rats and, after a 5-min delay, blood (1.9 ml/100 g of body weight over 20 min) was withdrawn through an arterial cannula. Numbers in parentheses indicate the number of animals in each group. Baseline mean arterial pressure values at the $-$ 25 min time point were: saline control = 86.7 ± 1.7 mm Hg; naloxone = 87.0 ± 2.6 mm Hg. MAP, mean arterial pressure. *P < 0.05, **P < 0.01 differs from saline-treated controls.

Naloxone (10 nmol/0.5 µl; 5 nmol/cannula) injection into the caudal vlPAG prevented the fall in arterial pressure evoked byhemorrhage completely (Fig. 1). Analysis of variance revealeda significant effect of naloxone treatment [F(1,11) = 11.58, P< 0.01], time [F(18,198) = 24.0, P < 0.001], and a significanttreatment-time interaction [F(18,198) = 10.0, P < 0.001] on meanarterial pressure (Fig. 1). The response was dose-related between1 and 100 nmol (0.5-50 nmol/cannula) [F(4,26) = 26.1, P < 0.001];the minimal dose necessary to inhibit hemorrhagic hypotensionsignificantly was 1 nmol (Fig. 2). Unilateral injection of 10nmol of naloxone in a smaller injection volume (0.1 µl) was ineffective(data not shown). Heart rate was not affected significantly byany naloxone dose during hemorrhage (data not shown). Naloxone(100 nmol) did not change arterial pressure or heart rate in nonhemorrhagedcontrol animals (data not shown). Bilateral naloxone administrationinto the vlPAG thus produces a dose-related inhibition of hemorrhage-inducedhypotension without affecting cardiovascular function in normotensiveanimals.

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Fig. 2. Dose-response effect of naloxone on mean arterial pressure following hemorrhage. The indicated dose of naloxone was injected bilaterally (one-half the dose per cannula) into the caudal vlPAG of halothane-anesthetized rats (n = 6-7 per group). After a 5-min delay, hemorrhage was initiated by withdrawing blood (1.9 ml/100 g of body weight) over a 20-min period. Data indicate the change in mean arterial pressure at the end of the 20-min hemorrhage period. *P < 0.05, **P < 0.01 differs from saline-treated controls.

Naloxone was also evaluated in fixed-pressure hemorrhage (Sandor et al., 1987

). Rats were pretreated with naloxone (10 nmol;5 nmol/cannula) and, 5 min later, sufficient blood was withdrawnto lower arterial pressure to approximately 50 mm Hg within 20min. In control animals, withdrawal of 1.8 ± 0.1 ml blood wasrequired to lower arterial pressure from 86.2 ± 1.8 to 52.9 ±1.4 mm Hg (n = 6). Following naloxone pretreatment, a significantlylarger blood volume was required (2.3 ± 0.1 ml; P < 0.01) to lowerarterial pressure to a comparable extent (from 86.6 ± 3.4 to 54.9± 0.5 mm Hg; n = 6). This shows that naloxone attenuates hemorrhagichypotension in both fixed volume and fixed pressure models ofcontrolledhemorrhage.

Hemorrhagic Hypotension is Inhibited by Delta, but Not Mu or Kappa, Opioid Receptor Antagonists. The finding that vlPAG naloxone administration inhibits hemorrhagic hypotension supports the hypothesis that hemorrhage activatesvlPAG opioid receptors but does not establish whether delta, mu,or kappa receptors mediate the response because naloxone is notreceptor selective. Previous studies have shown that intracerebroventricular(i.c.v.) administration of delta, but not mu or kappa, opioidreceptor antagonists inhibit hypovolemic (Ludbrook and Ventura,1994) and endotoxic (D'Amato and Holaday, 1984) hypotension. Receptorselectivity is thus a necessary criterion for establishing thatopioid receptors in the vlPAG mediate hemorrhagic hypotension.To establish this, we tested whether hemorrhagic hypotension isinhibited by naltrindole, a delta opioid receptor antagonist,CTOP, a mu receptor antagonist, or nor-BNI, a kappa receptorantagonist.

For these and subsequent experiments, hemorrhage was induced by withdrawing 2.5 ml/100 g of body weight, a somewhat largervolume than used for naloxone experiments (1.9 ml/100 g of bodyweight). The fall in arterial pressure induced by this hemorrhageprotocol was greater in magnitude and longer in duration (Fig.3) than the more transient hypotension produced by mild hemorrhage(Fig. 1). This, more severe hemorrhage protocol, also generateda significant reduction in heart rate [F(13,70) = 3.37, P < 0.001](Fig. 4) in halothane-anesthetized rats, in contrast to mild hemorrhage,which did not affect heart rate (data not shown).

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Fig. 3. Naltrindole injection into the vlPAG inhibits hemorrhagic hypotension. Naltrindole (0.2, 2, or 20 nmol) or saline (0.5 µl) was injected bilaterally (one-half the dose per cannula) into the vlPAG of halothane-anesthetized rats and, after a 5-min delay, blood (2.5 ml/100 g of body weight) was withdrawn through an arterial cannula over a 20-min period. Nonhemorrhage controls received naltrindole (20 nmol) bilaterally but blood was not withdrawn. Numbers in parentheses denote the number of animals in each group. Baseline mean arterial pressure values at the $-$ 25 min time point were: saline control = 113 ± 7 mm Hg; naltrindole 0.2 nmol = 104 ± 2 mm Hg; 2.0 nmol = 106 ± 7 mm Hg; 20 nmol = 100 ± 6 mm Hg; 20 nmol of naltrindole, nonhemorrhage control = 108 ± 4 mm Hg. *P < 0.05, **P < 0.01 differs from control.

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Fig. 4. Naltrindole injection into the vlPAG inhibits hemorrhage-induced bradycardia. Naltrindole (0.2, 2.0, or 20 nmol) or saline (0.5 µl) was injected bilaterally into the vlPAG of halothane-anesthetized rats 5 min before hemorrhage was initiated (2.5 ml/100 g of body weight over a 20-min period). Baseline heart rate values were: control = 359 ± 21 bpm; naltrindole 0.2 nmol = 326 ± 13 bpm; 2.0 nmol = 314 ± 20 bpm; 20 nmol = 333 ± 24 bpm; 20 nmol of naltrindole, nonhemorrhage = 354 ± 8 bpm. *P < 0.05, **P < 0.01 differs from controls.

Naltrindole microinjection (0.2, 2.0, or 20 nmol) into the vlPAG bilaterally (0.1, 1.0, or 10 nmol/cannula) inhibited thehypotension (Fig. 3) and bradycardia (Fig. 4) evoked by hemorrhagesignificantly. The higher naltrindole doses (2 and 20 nmol) notonly reduced the magnitude, but also delayed the onset and shortenedthe duration of hemorrhagic hypotension. Analysis of varianceconfirmed that the effects of naltrindole treatment [F(4,21) =96.6, P < 0.001], time [F(16,357) = 17.9, P < 0.001], and treatment-timeinteraction [F(64,357) = 3.1, P < 0.001] were significant. Naltrindolealso prevented the bradycardia induced by hemorrhage in anesthetizedrats [F(4,21) = 19.2, P < 0.001] (Fig. 4), although time and treatment-timeeffects were not significant. The highest naltrindole dose (20nmol) prevented hemorrhage-induced bradycardia completely, althoughit did not elevate heart rate significantly above baseline, prehemorrhagevalues (Fig. 4). Naltrindole administration had no effect on arterialpressure (Fig. 3) or heart rate (Fig. 4) in nonhemorrhaged animals.In contrast, vlPAG microinjection of CTOP (1 or 10 nmol), a muopioid receptor antagonist, or nor-BNI (1 or 6 nmol), a kappareceptor antagonist, had no effect whatsoever on the hypotension(Fig. 5) or bradycardia (data not shown) evoked by hemorrhage.Hemorrhagic hypotension is thus inhibited by microinjection ofdelta, but not mu or kappa, receptor antagonists into the vlPAG.

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Fig. 5. CTOP and nor-BNI fail to inhibit the fall in arterial pressure evoked by hemorrhage. The indicated dose of CTOP (top panel), nor-BNI (bottom panel) or saline (0.5 µl) was injected bilaterally (one-half the dose per cannula) into the vlPAG of halothane-anesthetized rats 5 min before hemorrhage (2.5 ml/100 g of body weight; 20 min). Baseline mean arterial pressure (MAP) values at the $-$ 25 min time point were: top $---$ 116.0 ± 6.6 mm Hg for the CTOP 1 nmol treated group, 107.8 ± 4.2 mm Hg for the CTOP 10 nmol treated group, and 108.5 ± 6.7 mm Hg for saline-treated controls: bottom $---$ 100.0 ± 2.9 mm Hg for the nor-BNI 1 nmol treated group, 102.9 ± 2.2 mm Hg for the nor-BNI 6 nmol treated group, and 108.5 ± 6.7 mm Hg for controls.

$beta$ -Endorphin_1-27 Administration into the vlPAG Inhibits Hemorrhagic Hypotension. We also tested whether hemorrhagic hypotension is inhibited by $beta$ -endorphin_1-27. $beta$ -Endorphin_1-27 is an endogenous $beta$ -endorphin-derived peptide that inhibits the antinociceptionproduced by $beta$ -endorphin administration into the PAG (Nicolas andLi, 1985; Tseng and Tang, 1990; Monroe et al., 1996). The receptormechanism responsible for the inhibitory effects of $beta$ -endorphin_1-27is controversial, however (Monroe et al., 1996). Receptor bindingexperiments indicate that $beta$ -endorphin_1-27 displays relativelyhigh affinity for both mu and delta opioid receptors (Nicolasand Li, 1985; Monroe et al., 1996), although some functional studiessuggest that $beta$ -endorphin_1-27 blocks a distinct, $beta$ -endorphin-specificepsilon receptor thought to mediate $beta$ -endorphin-elicited antinociceptionin the PAG (Tseng and Tang, 1990).

Microinjection of $beta$ -endorphin_1-27 (3 nmol) into the vlPAG 5 min before initiating hemorrhage (2.5 ml/100 g of body weight)inhibited the subsequent fall in arterial pressure significantly.Hemorrhage alone lowered arterial pressure by $-$ 70 ± 5 mm Hg (n= 5) by the end of the 20-min hemorrhage period in saline-treatedcontrols. $beta$ -Endorphin_1-27 pretreatment reduced the fallin arterial pressure significantly; mean arterial pressure fell $-$ 45 ± 2 mm Hg (n = 5) (P < 0.01) by the end of the hemorrhageperiod. $beta$ -Endorphin_1-27 also inhibited the response to mildhemorrhage (1.9 ml/100 g of body weight; control = $-$ 37.8 mm Hg(n = 7); $beta$ -endorphin_1-27 = $-$ 22.0 mm Hg (n = 5; P < 0.01). $beta$ -Endorphin_1-27 did not affect arterial pressure in nonhemorrhagedcontrol animals (2 ± 2 mm Hg; n =3).

Naltrindole Injection into the vlPAG Prevents Hemorrhagic Hypotension in Conscious Rats. Thus far, the data show that delta opioid receptor antagonists inhibit hemorrhagic hypotension in halothane-anesthetized rats,but anesthetics can influence the cardiovascular response to hypovolemiamarkedly (Schadt and Ludbrook, 1991; Owen et al., 1997). To determinewhether halothane anesthesia is a significant complicating factor,we tested whether naltrindole inhibits hemorrhagic hypotensionin conscious animals. We found that hemorrhage (2.5 ml/100 g ofbody weight over 20 min) produced essentially the same effecton arterial pressure in conscious rats (Fig. 6) as it did in halothane-anesthetizedanimals (Fig. 3). In both conscious and halothane-anesthetizedrats, arterial pressure was initially sustained at baseline values,began to fall within 10 min, reached approximately the same lowlevels by the end of the 20-min hemorrhage period (conscious rats= $-$ 63.4 ± 2.8 mm Hg; anesthetized rats = $-$ 66.3 ± 3.6 mm Hg), andthen increased spontaneously, although it did not achieve baselinevalues by the end of the experiment. The effect of hemorrhageon heart rate was different in conscious than in halothane-anesthetizedrats, however. Severe blood loss had no significant effect onheart rate in conscious rats (Fig. 6) but produced a sustainedbradycardia in halothane-anesthetized animals (Fig. 4).

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Fig. 6. The effect of vlPAG naltrindole administration on arterial pressure and heart rate following hemorrhage in conscious rats. Naltrindole (0.2, 2 or 20 nmol) or saline (0.5 µl) was injected bilaterally (one-half the dose per cannula) into the vlPAG of conscious rats 5 min before hemorrhage (2.5 ml blood/100 g of body weight over 20 min) was initiated. Mean arterial pressure (MAP; top panel) and heart rate (bottom panel) were recorded at 5-min intervals. Numbers in parentheses indicate the number of animals in each group. Baseline mean arterial pressure values at the $-$ 25 min time point were: saline = 125.0 ± 2.5 mm Hg; naltrindole 0.2 nmol = 123.3 ± 3.2 mm Hg, naltrindole 2.0 nmol = 125.6 ± 2.6 mm Hg; naltrindole 20 nmol = 130.1 ± 4.3 mm Hg; naltrindole-treated nonhemorrhage control = 111.2 ± 11.2 mm Hg; saline-treated nonhemorrhaged control = 130.5 ± 4.3 mm Hg. Baseline heart rate values were: control = 380 ± 10 bpm; naltrindole 0.2 nmol = 305 ± 20 bpm; naltrindole 2.0 nmol = 358 ± 19 bpm; naltrindole 20 nmol = 368 ± 17 bpm; and saline-treated nonhemorrhage control = 395 ± 17 bpm. *P < 0.05, **P < 0.01 differs from control.

Naltrindole injection (0.2, 2, or 20 nmol) bilaterally into the vlPAG of conscious rats inhibited the hypotension caused byhemorrhage significantly (Fig. 6). The response was dose-relatedand essentially the same as observed in halothane-anesthetizedrats. Statistical analysis confirmed that the effects of naltrindoletreatment [F(4, 25) = 170.8, P < 0.001], time [F(16,366) = 42.4,P < 0.001] and treatment-time interaction [F(64,366) = 3.1, P< 0.001] were significant. Naltrindole had no overall effect onheart rate, although the highest naltrindole dose (20 nmol) produceda mild tachycardia. Analysis of variance indicated that the effectof naltrindole treatment on heart rate was significant [F(4,13)= 10.4, P < 0.001], but time and treatment-time interactive effectswere not, and post hoc analysis did not reveal a significant treatmenteffect at any individual time point. These data indicate thatthe effects of naltrindole on arterial pressure during hemorrhageare not dependent on concurrentanesthesia.

Effects of Naltrindole in the Rostral vlPAG and Caudal dlPAG. Next, we tested whether opioid receptor antagonists inhibit hemorrhagic hypotension only in the caudal vlPAG or if they arealso effective in the rostral vlPAG. The vlPAG is viscerotopicallyorganized to the extent that rostral and caudal vlPAG regionsregulate different vascular beds (Carrive and Bandler, 1991),although activation of either vlPAG region with excitatory aminoacids lowers arterial pressure and heart rate (Carrive and Bandler,1991; Keay et al., 1997) (A. D. Evec and M. M. Rapacon-Baker,unpublished observations). Figure 7 shows that bilateral naltrindoleinjection (2 nmol; 1 nmol/cannula) into the rostral vlPAG inhibitedhemorrhagic hypotension significantly (P < 0.01) in consciousrats. The response was comparable in magnitude to caudal vlPAGnaltrindole injection. Heart rate was not affected significantlyby naltrindole in either the rostral (data not shown) or caudal(Fig. 6) vlPAG. Naltrindole thus inhibits hemorrhage-induced hypotensionin either the rostral or caudal vlPAG.

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Fig. 7. Naltrindole inhibits hemorrhagic hypotension in the caudal and rostral vlPAG, but not the dlPAG. Naltrindole (2 nmol) was injected bilaterally (1 nmol/cannula) into either the caudal vlPAG (left), rostral vlPAG (middle), or caudal dlPAG (right), and hemorrhage was induced 5 min later by withdrawing 2.5 ml/100 g of body weight blood over a 20-min period. Columns depict the change in mean arterial pressure (MAP) at the end of the 20-min hemorrhage period (n = 4-7). **P < 0.01 differs from controls.

In contrast to the vlPAG, excitatory amino acid injection into the lateral or dlPAG produces hypertension and tachycardia(Bandler et al., 2000

). This makes it unlikely that activationof delta opioid receptors in the dlPAG triggers the hypotensionthat results from hemorrhage. To test this assumption, we injectednaltrindole (2 nmol) bilaterally (1 nmol/cannula) into the caudaldlPAG 5 min before initiating hemorrhage. Dorsolateral PAG naltrindoleinjection had no effect on arterial pressure (Fig. 7) or heartrate (data not shown). Thus, delta opioid receptors in the vlPAG,but not the dlPAG, mediate hemorrhagic hypotension.

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Fig. 8. Schematic representation of coronal sections through the rostral ( $-$ 7.3 mm from bregma) and caudal ( $-$ 8.3 mm from bregma) PAG illustrating the drug and peptide injection sites. Aq = Sylvian aqueduct.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Naloxone and delta opioid receptor antagonists inhibit hemorrhagic hypotension through a central mechanism, presumably byinterrupting synaptic transmission by opioid peptide neurons inan anatomical pathway that inhibits sympathetic neuronal activity.In this study, we tested the hypothesis that the opioid receptorsthat initiate the fall in arterial pressure caused by hemorrhageare located in the vlPAG. We found that naloxone injection intothe caudal vlPAG essentially abolished hemorrhage-induced hypotension.Naloxone was effective at doses at least an order of magnitudelower than required to inhibit hemorrhagic hypotension followingi.c.v. injection (Owen et al., 1997), which makes it unlikelythat naloxone acts by diffusing from the vlPAG to a distant site.Hemorrhagic hypotension was also inhibited by naltrindole, butnot by CTOP or nor-BNI, which confirms that delta opioid receptorsmediate the response. Naltrindole did not affect arterial pressureor heart rate in normotensive animals, consistent with evidencethat opioid neurons are specifically activated by hemorrhage,but do not contribute substantially to the tonic regulation ofarterial pressure (Gordon, 1986). These findings support the conceptthat activation of delta opioid receptors in the vlPAG plays apivotal role in the response tohemorrhage.

Naltrindole is a relatively selective opioid receptor antagonist with an affinity for delta receptors at least 100-fold higherthan for mu and kappa receptors (Portoghese et al., 1988). Itis thus unlikely that naltrindole inhibits hemorrhagic hypotensionthrough a nonselective receptor mechanism. To further rule outthis possibility, we tested whether the mu and kappa receptorselective antagonists, CTOP (1 and 10 nmol) and nor-BNI (1 and6 nmol), inhibit the response to hemorrhage following vlPAG administrationat doses comparable with the naltrindole doses (0.2-20 nmol) wefound to be effective. Neither drug had any discernible effect.Their lack of efficacy was not attributable to dose inequivalencebecause the relative affinity of CTOP (K_d = 0.16 nM) (Hawkinset al., 1989) and nor-BNI (K_i = 0.06 nM) (Emmerson et al., 1994)for mu and kappa receptors is higher than the affinity of naltrindolefor delta receptors (K_i = 1.4 nM) (Emmerson et al., 1994). Itseems safe to conclude, therefore, that naltrindole inhibits hemorrhagichypotension by blocking delta opioid receptors in the vlPAG, andthat mu and kappa receptors do not participate in theresponse.

This conclusion is consistent with a report by Keay et al. that microinjecting the delta receptor agonist [D-Pen², D-Pen⁵]enkephalin (DPDPE) into the vlPAG lowers arterial pressure andheart rate (Keay et al., 1997). [D-Pen², D-Pen⁵]Enkephalin was effective in approximately 35% of tested siteslocated throughout the rostro-caudal extent of the vlPAG and extendinginto the lateral and dlPAG. The mu receptor agonist [D-Ala²,N-Me-Phe⁴,Gly⁵-ol]enkephalin (DAMGO) produced the opposite response, hypertensionand tachycardia, and the kappa receptor agonist, U69-593, generateda small but inconsistent depressor and bradycardic effect. Thepresent data extend these findings by demonstrating that vlPAGdelta receptors function endogenously in the regulation of arterialpressure duringhemorrhage.

The finding that delta receptors in the vlPAG influence cardiovascular function is somewhat unexpected because delta receptorbinding densities (Mansour et al., 1987) and mRNA levels (Kalyuzhnyand Wessendorf, 1998) are quite low in the vlPAG. Furthermore,both opioid- and stress-induced antinociception are mediated primarily,if not exclusively, by mu receptors in the vlPAG, not delta receptors(Yaksh, 1997). This conclusion is derived from microinjectionstudies showing that selective delta receptor agonists have noeffect at all on nociceptive response latencies following vlPAGadministration (Smith et al., 1988; Yaksh, 1997). Subsequent studiesdid show, however, that delta agonists inhibit neuropathic pain(Sohn et al., 2000) and potentiate DAMGO-induced antinociception(Rossi et al., 1994) following vlPAG administration, which suggeststhat vlPAG delta receptors may influence nociception under specificcircumstances. But despite conflicting evidence, it would appearthat endogenous opioids normally influence pain perception andcardiovascular function through different receptor mechanisms,mu and delta receptors, respectively, in the vlPAG.

The opioid peptide neurons that mediate hemorrhagic hypotension remain to be identified. The vlPAG contains relatively highamounts of immunoreactive $beta$ -endorphin and met-enkephalin (Khachaturianet al., 1985), both of which serve as endogenous agonists fordelta opioid receptors (Paterson et al., 1983), as well endomorphin-(Martin-Schild et al., 1999) and dynorphin- (Khachaturian et al.,1985) related peptides, which, in general, are selective for muand kappa receptors, respectively. Although there is evidencethat both $beta$ -endorphin- and met-enkephalin-releasing neurons modulatepain perception in the PAG (Yaksh, 1997), a report by Sandor etal. (1987) implicates $beta$ -endorphin-releasing neurons as exclusiveregulators of cardiovascular function during hemorrhage. Theyfound that i.c.v. injection of a $beta$ -endorphin antiserum inhibits,and $beta$ -endorphin potentiates, the hypotension produced by hemorrhage,whereas met-enkephalin antisera or peptide administration areineffective (Sandor et al., 1987).

Nevertheless, the prospect that either $beta$ -endorphin or met-enkephalin lowers arterial pressure in the vlPAG seems paradoxicalbecause these peptides display a high affinity for both mu anddelta receptors (Paterson et al., 1983), which produce oppositeeffects on cardiovascular function in the vlPAG (Keay et al.,1997). But we found that $beta$ -endorphin generated a depressor responsein the vlPAG equivalent in magnitude to, although longer in durationthan, that produced by DLH. The reason for $beta$ -endorphin's unexpectedefficacy is not readily apparent, although it may be due to differencesin the cellular location of mu and delta receptors in the vlPAG(Kalyuzhny and Wessendorf, 1998). Alternatively, $beta$ -endorphin maylower arterial pressure through a receptor mechanism that doesnot involve mu or delta receptors, as shown previously for $beta$ -endorphin-inducedantinociception (Tseng and Tang, 1990; Monroe et al., 1996). Thefinding that $beta$ -endorphin_1-27 inhibits hemorrhagic hypotensionmay provide support for this contention. Tseng and Tang (1990)reported that $beta$ -endorphin_1-27 selectively inhibits the antinociceptionproduced by $beta$ -endorphin, but not morphine, in the PAG, suggestingthat it blocks a $beta$ -endorphin-specific receptor; contradictoryevidence has also been reported, however (Monroe et al., 1996).In either case, the present data support the hypothesis that endogenousopioid peptides contribute to the fall in arterial pressure causedby hemorrhage, despite their lack of selectivity for deltareceptors.

Anatomically, the vlPAG is strategically situated to mediate the effects of hemorrhage. Ventrolateral PAG neurons denselyinnervate the midline raphe nuclei, raphe obscurus, and pallidus(Cameron et al., 1995; Henderson et al., 1998). Activation ofneurons in the midline raphe nuclei and adjacent regions of thecaudal midline medulla lowers arterial pressure and heart rateand inhibits sympathetic neuronal activity (Coleman and Dampney,1995; Henderson et al., 1998). The midline raphe influence cardiovascularfunction both directly, by innervating preganglionic sympatheticneurons in the intermediolateral cell column, and indirectly,through axonal projections to the rostral ventrolateral medulla(RVLM) pressor and caudal ventrolateral medulla (CVLM) depressorregions (Romagnano et al., 1991; Lovick, 1993). Recently, Hendersonet al. (2000) showed that inactivation of the caudal midline medullawith either lidocaine or cobalt chloride inhibits hemorrhage-evokedhypotension, but does not affect cardiovascular function in normotensiverats. These data provide evidence that the caudal midline medulladepressor region is a second component of the descending pathwaythat initiates hemorrhagic hypotension. Ventrolateral PAG neuronsalso innervate the rostral ventrolateral medulla and the caudalventrolateral medulla directly (Cameron et al., 1995; Chen andAston-Jones, 1996; Henderson et al., 1998; Keay et al., 2000),which raises the possibility that multiple descending pathwaysmay be influenced by hemorrhage. The caudal midline medulla isthus an important component of a descending pathway that conveysthe effects of vlPAG activation to preganglionic sympathetic neurons,although other cardioregulatory brainstem regions may also beinvolved.

Opioid receptor antagonists may act at multiple locations in this descending pathway. Ang et al. (1999) reported recentlythat intrathecal injection of naloxone or a delta opioid receptorantagonist inhibits hemorrhagic hypotension without affectingresting arterial pressure or heart rate. The conclusion that deltaopioid receptors in the spinal cord mediate the effects of hemorrhage(Ang et al., 1999) is supported by evidence that enkephalinergicneurons in the midline raphe nuclei innervate preganglionic sympatheticneurons in the spinal cord (Romagnano et al., 1991). Microinjectionof a delta opioid receptor antagonist into the caudal midlinemedulla depressor region also attenuates the effects of hemorrhage(Henderson et al., 1999). These findings support the hypothesisthat hemorrhage stimulates opioid peptide release at multiplesites in a descending cardioregulatory pathway that includes thevlPAG, caudal midline medulla, and intermediolateral cell column.In this way, the descending cardioregulatory pathway that precipitateshemorrhagic hypotension is similar to the descending pain controlpathway that inhibits pain perception during periods of extremestress (Yaksh, 1997). Opioid receptors are situated strategicallyin the vlPAG, midline raphe nuclei, and spinal cord in both thecardioregulatory and pain control pathway and microinjection ofopioid receptor agonists and/or antagonists influence both nociceptionand cardiovascular function in each of these three regions. Thesimilar location of opioid neurons and receptors in the two descendingpathways may, in part, explain the simultaneous hypotension andantinociception generated by severe pain, serious injury, andhemorrhagicshock.

	Footnotes

Accepted for publication January 9, 2001.

Received for publication October 30, 2000.

This research was supported by a grant from the Office of Naval Research (N00014-98-1-0249).

Send reprint requests to: Dr. William R. Millington, Department of Basic and Pharmaceutical Sciences, Albany College of Pharmacy, 106 New Scotland Ave., Albany, NY 12208-3492. E-mail: millingw{at}acp.edu

	Abbreviations

vlPAG, ventrolateral periaqueductal gray; PAG, periaqueductal gray; dlPAG, dorsolateral periaqueductal gray; DLH, DL-homocysteic acid; CTOP, D-Phe-Cys-Tyr-D-Trp-Orn-Thr-Pen-Thr amide; nor-BNI, nor-binaltorphimine; bpm, beats per minute; DAMGO, [D-Ala², N-Me-Phe⁴, Gly⁵-ol]enkephalin.

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