Cardiovascular Effects of Cholecystokinin-4 Are Mediated By the Cholecystokinin-B Receptor Subtype In the Conscious Guinea Pig and Dog

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Vol. 281, Issue 1, 180-187, 1997

Cardiovascular Effects of Cholecystokinin-4 Are Mediated By the Cholecystokinin-B Receptor Subtype In the Conscious Guinea Pig and Dog

Anthony A. Fossa, Michael J. Depasquale, Jean Morrone, Stevin H. Zorn, Dianne Bryce, John A. Lowe and Stafford McLean

Departments of General Pharmacology and Neurosciences, Pfizer Central Research, Groton, Connecticut

	Abstract

Top Abstract Introduction Methods Results Discussion References

Panicogenic effects in humans of the selective cholecystokinin (CCK_B) receptor agonist, cholecystokinin tetrapeptide (CCK₄),have been reported to correlate with increases in heart rate (HR)and mean arterial pressure (MAP). Previous investigators havedemonstrated that the nonselective CCK_A and CCK_B receptor agonist,sulfated cholecystokinin octapeptide, also produces increasesin HR and mean arterial pressure. The purpose of our study isto determine if the cardiovascular changes induced by CCK₄ aremediated by the CCK_A or CCK_B receptor subtype using selectiveCCK antagonists for both receptor subtypes. The rank order ofpotency of the CCK receptor antagonists affecting CCK₄-inducedHR and mean arterial pressure changes in the guinea pig correspondedto the rank order of potency for blockade of the CCK_B receptorbinding in rat cortex, phosphatidyl inositol turnover in AR 4-2Jrat pancreatoma cells and inhibition of pentagastrin-induced acidsecretion in the rat. The changes induced by CCK₄ on HR, but notmean arterial pressure, appear to be species dependent as reflectedby a decrease in the HR in the guinea pig and an increase in thedog. Nonetheless, the results from the antagonist studies indicatethat the cardiovascular responses to CCK₄ in both the guinea pigand dog are mediated by the CCK_B receptor subtype.

	Introduction

Top Abstract Introduction Methods Results Discussion References

CCK, a 33 amino acid peptide first isolated from porcine gut, is a member of a family of peptides that together with gastrinshare a common carboxyl-terminal pentapeptide amino acid sequence(Mutt and Jorpes, 1968). Both N-terminal extended forms of CCKhave been described as well as truncated forms such as CCK₈, pentagastrinand CCK₄ (Dockray et al., 1978; Larsson and Rehfeld, 1979; Reeveet al., 1990). These peptide fragments of CCK have been usefulin pharmacologically identifying two receptor types: CCK_A andCCK_B (Innis and Synder, 1980; Grider and Makhlouf, 1987; Hugheset al., 1990; Hill et al., 1987). CCK_A receptors, found primarilyin pancreatic acinar cells and in the gastrointestinal tract,have high affinity for sulfated CCK (i.e., CCK8S) and gastrinand a lower affinity for unsulfated CCK₈, pentagastrin and CCK₄.In contrast, the CCK_B receptors that predominate in brain havehigh affinity for pentagastrin and the tetrapeptide CCK₄ (Hugheset al., 1990). More recently, confirmation of receptor heterogeneityhas occurred with the development of selective, high affinitynonpeptide antagonists (Woodruff and Hughes, 1991) and the recentcloning of the CCK_A and CCK_B receptors (Wank et al., 1992a; Ulrichet al., 1993; Wank et al., 1992b; Pisegna et al., 1992; Lee etal., 1993).

The physiological functions described for the CCK_A receptor in the periphery are primarily related to pancreatic secretionof amylase and insulin, although in the gastrointestinal tractpepsinogen is secreted in addition to stimulation of longitudinalsmooth muscle (Woodruff and Hughes, 1991). In the central nervoussystem, CCK_A receptors have been identified in the substantianigra and striatum and appear to influence activity of the dopaminergicsystem (van Dijk et al., 1984; Hill et al., 1990). CCK_A receptorshave also been found in the dorsal raphe, area postrema, nucleustractus solitarius and interpeduncular nucleus (Woodruff and Hughes,1991).

Historically, elucidation of the physiological role of peripherally located CCK_B receptors has been limited. However, withthe development of such specific antagonists as CI-988 and L-365,260,the significance of this receptor is becoming more apparent. Severalinvestigators have reported that CCK_B receptors may mediate secretoryand contractile responses in the guinea pig (Lucaites et al.,1991, Grider and Makhlouf, 1990). Specific agonists that produceCCK_B-mediated peripheral effects include pentagastrin and CCK₄(Lucaites et al., 1991).

CCK_B receptors are the predominant CCK-receptor subtype in the brain. Infusion of pentagastrin into the lateral ventriclesof sheep has been shown to produce behaviors equated to fear (Della-Feraand Baile, 1979). Hughes et al. (1990) showed that the specificreceptor antagonist, CI-988, reduced anxiety in the mouse black-whitetest and in the marmoset-human threat test. In humans with a historyof panic disorder, i.v. administered CCK₄ produces spontaneouspanic-like symptoms that are indistinguishable from endogenouspanic attacks. These symptoms have been characterized by increasesin anxiety and physiological signs such as increased heart rateand blood pressure (Bradwejn et al., 1992). Other investigatorshave reported that the nonselective CCK_A and CCK_B receptor agonist,CCK_8S, also produces increases or decreases in HR (dose dependent)and increases in mean arterial pressure of rats that are blockedby the CCK_A selective antagonist, devazepide (Guarini et al.,1988; Janssen et al., 1991; Gaw et al., 1995). The purpose ofthis study is to determine which CCK receptor subtype mediatesthe cardiovascular responses observed by Bradwejn et al. (1992)after administration of CCK₄.

	Methods

Top Abstract Introduction Methods Results Discussion References

Compounds

Cholecystokinin 4 (structure H-Trp-Met-Asp-Phe-NH2) was from Bachem Feinchemikalien AG, Germany. The CCK antagonists, CP-212,454(N-(1-t-butyl) 2-[3-(3-chlorophenylureido)-2-oxo-5-phenyl-8-methyl-2,3,4,5-tetrahydro-1H-(1)benzazepin-1-yl]ethanoic acid amide), CP-310,713 (N-(1-t-Butyl) 2-[3-(3-carboxyphenylureido)-2-oxo-5-cyclohexyl-8-methyl-2,3,4,5-tetrahydro-1H-(1)benzazepin-1-yl]ethanoic acid amide), L-365,260, devazepide and CI-988 were synthesizedby Pfizer Inc. (Groton, CT).

Receptor Binding

For CCK_B receptor binding assays guinea pig cortex was homogenized with a Teflon homogenizer in 20 vol of 50 mM Tris HCl (pH7.4) containing 5 mM MnCl₂ at 4°C and centrifuged at 100,000 ×g for 30 min. The supernatant was discarded and the pellet resuspendedand spun again. The pellet was diluted to a concentration of 10mg/ml (original wet weight) with assay buffer (10 mM HEPES, 5mM MgCl₂, 1 mM EGTA, 130 mM NaCl and 0.2 mg/ml bacitracin, pH6.5) before use. The incubation reaction was initiated by theaddition of 50 µl of tissue to 96-well plates containing 150 µlof assay buffer with 1% DMSO final concentration, 50 pM finalconcentration of ¹²⁵I-BH-CCK_8S (Du Pont NEN, Boston, MA) and the appropriate concentrationof drug or vehicle. Nonspecific binding was estimated using 1µM CCK_8S. The reaction was terminated by spinning the plates usinga H1000B rotor at 3000 rpm for 5 min at 4°C. The pellet was washedwith 200 µl of 50 mM Tris HCl and respun. The supernatant wasagain discarded, the pellet resuspended and the tissue harvestedonto Betaplate filters (Wallac Oy, Turku, Finland) soaked in 0.2%polyethylenimine for 2 hr using a Skatron cell harvester (SkatronInstruments, Inc., Sterling, VA). The filtermats were dried andcounted on a Betaplate counter (Wallac Inc., Gaithersburg, MD)for 45 sec per sample.

For CCK_A receptor binding the pancreas was dissected from a male Hartley guinea pig and placed in saline. Fatty tissue andblood vessels were dissected away and the tissue placed in 20vol of buffer (50 mM Tris HCl, pH 7.4, 0.35 mg/ml bacitracin and0.5 mg/ml soybean trypsin inhibitor) at 4°C and minced using scissors.The tissue was homogenized (Polytron, setting no. 9 for two 15-secbursts), strained through gauze and centrifuged at 100,000 × gfor 15 min at 4°C. The supernatant was discarded and the pelletresuspended in 20 vol of buffer and recentrifuged. The final pelletwas diluted to a concentration of 1.25 mg/ml (original wet weight)in buffer and kept on ice until used. The incubation reactionwas initiated by the addition of 100 µl of tissue to 96-well platescontaining 150 µl of incubation buffer (50 mM Tris HCl, pH 7.4,and at final concentration 5 mM MgCl₂, 5 mM dithiothreitol and1% DMSO) with 60 pM final concentration of ¹²⁵I-BH-CCK_8S, and drug or vehicle. Nonspecific binding was estimatedusing 1 µM L-364,718. After a 30-min incubation the reaction wasterminated by rapid filtration using a Skatron cell harvesteronto GF/B filters that were soaked for 2 hr in 50 mM Tris HCl,0.1 mg/ml bovine serum albumin. The filtermats were dried andcounted on a Betaplate counter for 45 sec per sample.

Phosphatidylinositol Turnover

AR 4-2J rat pancreatoma cells obtained from Dr. J. Putney (NIEHS, Research Triangle Park, NC) were grown in DMEM supplementedwith L-glutamine and 10% fetal bovine serum (FBS). AR 4-2J cellswere prelabeled with 10 µCi/ml [³H]-myo-inositol overnight. The cells were incubated with agonistsfor 45 min in the presence of LiCl 10 mM and the reaction terminatedby adding CHCl3:MeOH (1:2). The cells were harvested with PBScontaining 3 mM EDTA, spun down and resuspended in PBS with 20mM HEPES and 3 mg/ml D-glucose at a concentration of 1 to 5 ×10⁶ cells/ml. Cells were exposed to antagonists 10 min before agonistexposure. [³H]-inositol phosphates were isolated by a batch technique usinga dowex AG1-X8 anion exchange resin. Corrected IC50s (K_i) werecalculated by K_i = IC50/1 + [pentagastrin]/[EC₅₀ pentagastrin],where [] = concentration.

Gastric Acid Secretion

Gastric acid secretion studies were conducted in rats using a modification of the pylorus ligation model described by Hakkinenet al. (1991). Fasted male Sprague-Dawley rats (125-250 g) wereanesthetized by inhalation with methoxyflurane (Metofane, Pitman-Moore,Inc., Chicago, IL) and the pylorus ligated. Compounds were administeredin a vehicle DMSO:emulphor:saline (5:15:80) by s.c. injection(4 ml/kg). Pentagastrin was administered in a 1:99 vehicle ofDMSO:saline (v:v). Rats were killed 2 hr after administrationof drugs and pentagastrin and the gastric fluid was diluted withwater and titrated to pH 7.0 with 0.1 N sodium hydroxide usinga Radiometer TTT85 Titrator and an ABU80 Autoburette (RadiometerAmerica, Inc., Westlake, OH). The amount of sodium hydroxide usedwas taken as a direct measure of the titratable acid (expressedin µEq) in the sample. The acid content was calculated per mlof gastric fluid and normalized to the time of the ligation andthe body weight of the rat.

In Vivo Cardiovascular Studies

Animals. All animal studies were conducted in accordance with protocols approved by the Pfizer Institutional Animal Care and Use Committee.Male Hartely guinea pigs were obtained from Charles River BreedingLaboratories (Wilmington, MA). Purpose-bred mongrel dogs wereobtained from Hazelton Labs (Kalamazoo, MI). Animals were housedon a 12-hr light cycle (0700-1900 hr) at 27 ± 5°C.

On the day before experimentation, guinea pigs (300-350 g) were anesthetized with xylazine (10 mg/kg s.c.; Mobay Corp., Shawnee,KS) and ketamine (80 mg/kg, i.m.; Parke-Davis, Morris Plains,NJ) and the right jugular vein and left carotid artery were isolatedand cannulated with polyethylene tubing (0.58 mm i.d. × 0.965mm o.d.). Both catheters were exteriorized at the interscapularregion and filled with a heparin-(500 U/ml) dextrose (50%) lockto ensure patency. Before surgery, the animals were dosed orally(1 ml) with the antibiotic combination trimethoprim: 8 mg/sulfamethoxazole:40 mg (Roche Laboratories, Nutley, NJ). The animals were allowedto recover overnight with food and water ad libitum.

Adult mongrel dogs (8-12 kg) were anesthetized with isoflurane (1-1.5%) and nitrous oxide (0.2 liter/min) and instrumentedwith a Data Sciences, Inc. (St. Paul, MN) pressure/ECG telemetrydevice (model TL10M2D70-PC), with the pressure catheter tip placedin the abdominal aorta via the femoral artery and the ECG leadstunneled s.c. to the upper right thorax and the lower left innerthigh for obtaining a Lead II electrocardiogram. The telemetrytransmitter body was secured s.c. on the dog's flank. The dogswere allowed to recover from surgery for at least 2 wk and trainedto lie quietly in a sling. Subjects were fasted for 12 hr beforeexperiments.

Cardiovascular measurements. Animals were studied in the conscious state. Guinea pigs were placed in Plexiglas restraining tubes. Carotid catheters wereconnected to a Statham P23ID pressure transducer (Ohmeda, Oxnard,CA) positioned at the level of the heart and interfaced with aGould (Gould Instrument Systems Inc., Valley View, OH) transduceramplifier (model 20-4615-50). The telemetered signals from dogswere transformed back to calibrated analog signals using a DataSciences UA10 Universal Adapter D/A converter. The pulsatile waveformswere displayed on an Astromed MT95000 polygraph (Astromed, WestWarwick, RI). Mean arterial pressure and heart rate were derivedfrom a beat-to-beat analysis of the pulsatile waveform using Po-Ne-Mahmodel MA-1 data acquisition and analysis software (Po-Ne-Mah,Inc., Simsbury, CT). Values were averaged over 60-sec intervalsduring base-line periods. To increase the sensitivity of the systemto acute changes in pressure and heart rate, measurements wereaveraged over 10-sec intervals after i.v. challenge with CCK₄.

Dose response to CCK₄. A dose of CCK₄ that gave a robust and reproducible increase in mean arterial pressure and decrease in heart rate after i.v.bolus administration was established. A dose response curve toCCK₄ was generated over a range of 1 to 160 µg/kg in guinea pigs(n = 4) and 1 to 20 µg/kg in mongrel dogs (n = 3). The peptidewas dissolved in 0.9% saline vehicle at a volume of 1 ml/kg i.v.in guinea pigs or 0.1 ml/kg i.v. for dogs. The dose concentrationswere delivered in a random fashion. At the end of the study, selecteddoses were repeated in the animals to evaluate whether there wasany tolerance or tachyphylaxis to the CCK₄ injection.

Experimental protocol. After obtaining stable base-line measurements of mean arterial pressure and heart rate, the animal was challenged with ani.v. bolus injection of the 0.9% saline vehicle and changes inpressure and heart rate recorded. Fifteen min later, the maximalcontrol cardiovascular response to an i.v. bolus injection CCK₄(20 µg/kg for guinea pigs; 10 µg/kg for dogs) was measured. Forguinea pig studies, the CCK receptor antagonist or vehicle (3ml/kg) was administered by a slow i.v. push. For dog experiments,the antagonist or vehicle (2% Tween 80 in water at 4 ml/kg) wasadministered orally. All antagonists were prepared in a 5:5:90(v:v:v) DMSO/emulphor/5% dextrose vehicle. CCK₄ challenges werethen repeated at 15, 45, 75, 105 and 135 min and the peak changesin mean arterial pressure and heart rate were recorded. The activityof a given CCK receptor antagonist was expressed as its abilityto attenuate the cardiovascular response to CCK₄ as compared tothe maximal control CCK₄ response recorded initially in a givenanimal.

Statistical analyses. All results are reported as the mean ± S.E.M. A one-way analysis of variance with an unpaired Student's t test was used forreceptor binding and gastric acid secretion studies. When examiningthe cardiovascular effects of CCK antagonists, a two-way analysisof variance with repeated measures using time and treatment asfactors was performed. If the variances were not homogenous, aStudent-Newman-Keuls method was used for pairwise multiple comparisons,otherwise a Bonferroni t test was performed. A value of P < .05was considered significant.

	Results

Top Abstract Introduction Methods Results Discussion References

Effect of agonists and antagonists on ¹²⁵I-BH-CCK_8S binding to CCK_B and CCK_A receptors. The binding of agonists and antagonists to CCK_B and CCK_A receptors was examined using ¹²⁵I-BH-CCK_8S binding to guinea pig cortex and pancreas, respectively.Of the antagonists tested, CP-310,713 had the highest affinityand selectivity for CCK_B receptors followed by CI-988, CP-212,454and L-365,260 (table 1). Devazepide was 500-fold selective forCCK_A receptors, binding with an IC₅₀ value of 0.23 ± 0.015 nM.

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TABLE 1
Receptor binding of CCK_A and CCK_B antagonists: results are means ± S.E.M. from three to seven determinations

CCK8S did not discriminate between CCK_B and CCK_A receptors with IC₅₀ values of 0.15 and 0.19 nM, respectively (table 1).Compared to CCK8S, CCK8US had an approximately 25-fold reductionin affinity for CCK_B receptors, but a 1000-fold loss in bindingaffinity to the CCK_A receptor. Pentagastrin displaced ¹²⁵I-BH-CCK8S to cortex and pancreas with IC₅₀ values of 1.3 and1600 nM, respectively. CCK₄ was selective for CCK_B receptors bindingwith an IC₅₀ value of 78 nM to the CCK_B receptor and lacking appreciableaffinity for CCK_A receptors with an IC₅₀ value of 5700 nM.

Effect of antagonists on pentagastrin-induced phosphatidylinositol turnover in rat AR 4-2J pancreatoma cells. Pentagastrin (PG) stimulated PI turnover in late passage AR 4-2J rat pancreatoma cells with an EC₅₀ of 0.3 nM. The specificCCK_B receptor antagonists, L-365,260, CI-988, CP-212,454 and CP-310,713all showed dose-dependent inhibition of the pentagastrin-induced(0.33 nM) PI turnover with K_i values of 4.1, 2.4, 0.65 and 0.23nM, respectively. In contrast, the selective CCK_A receptor antagonist,devazepide, had little effect on pentagastrin-induced PI turnoverwith a K_i value >300 nM (table 2).

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TABLE 2
Inhibition of pentagastrin-stimulated phosphatidylinositol hydrolysis in AR 4-2J cells

Effect of antagonists on pentagastrin-induced acid secretion in rats. The specific CCK_B receptor antagonists, L-365,260, CP-212,454 and CP-310,713 all showed dose-dependent inhibition of gastricacid secretion with s.c. ID₅₀ values of 1.5, 0.80 and 0.01 mg/kg,respectively. The CCK_B receptor antagonist, CI-988, blocked 60%of the pentagastrin-mediated effect with an ID₅₀ value of 0.08mg/kg, consistent with some reports indicating that it is a partialagonist at this receptor. The CCK_A receptor antagonist, devazepide,was the least potent with an ID₅₀ of 8.0 mg/kg when given s.c.(fig. 1).

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Fig. 1. Dose-response curves for the CCK_A receptor antagonist, devazepide ( $black-down-triangle$ ), and the CCK_B receptor antagonists L-365,260 ( $black-square$ ), CP-212,454( $bullet$ ) and CI-988 ( $black-triangle$ ), to antagonize pentagastrin-induced acid secretionin the pylorus ligated rat. Data are expressed as percentage ofcontrol maximum response to pentagastrin and each point representsthe mean of not less than 10 rats. The coefficient of variationfor each point ranged from 5 to 25%.

Effect of CCK₄ on heart rate and mean arterial pressure. The cardiovascular effects of CCK₄ on HR and MAP were examined in the conscious guinea pig and dog. Dose-response curves inguinea pigs with i.v. bolus doses of CCK₄ from 1 to 160 µg/kgwere generated for changes in HR and MAP. Decreases in HR andincreases in MAP were observed in a dose-dependent manner up to20 µg/kg of CCK₄. Doses of CCK₄ between 20 and 160 µg/kg producedonly small increases in the magnitude of both the HR and MAP responses.No tachyphylaxis was observed when CCK₄ was repeatedly administeredevery 30 min over a 135-min period (fig. 2). Because 20 µg/kgof CCK₄ produced the most consistent response, this dose was chosenfor all subsequent studies to compare receptor antagonists inthe guinea pig.

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Fig. 2. Effect of repeated doses of CCK₄ (20 µg/kg, i.v.) on blood pressure in the conscious guinea pig. CCK₄ was administered at30-min intervals for 135 min starting 15 min before administrationof the CCK₄ antagonist, CP-212,454 or vehicle.

In the dog, the response to CCK₄ was different from that of the guinea pig. Dose-response curves for both CCK₄-mediated changesin HR and MAP were examined by intravenous bolus doses from 1to 20 µg/kg. Increases in both HR and MAP were observed up to20 µg/kg of CCK₄. A dose of 10 µg/kg was chosen for subsequentstudies with CCK antagonists in the dog. As in the guinea pig,no tachyphylaxis to the HR or blood pressure responses was apparentwhen 10 µg/kg of CCK₄ was administered repeatedly over a 120-minperiod (see vehicle data in figs. 5 and 6).

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Fig. 5. Effect of the CCK_B antagonist on heart rate changes in the conscious dog. Top panel, Effect of 50 mg/kg of orally administeredCP-212,454 ( $black-square$ ) or 4 ml/kg vehicle ( $bullet$ ) on basal heart rate beforeCCK₄ challenges. Bottom panel, Percentage change in maximal heartrate response to CCK₄ after CP-212,454 ( $black-square$ ) or vehicle ( $square$ ). Eachpoint represents the mean of at least four dogs.

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Fig. 6. Effect of the CCK_B antagonist on mean arterial blood pressure changes in the conscious dog. Top panel, Effect of 50 mg/kgof orally administered CP-212,454 ( $black-square$ ) or 4 ml/kg vehicle ( $bullet$ ) onbasal mean arterial blood pressure before CCK₄ challenges. Bottompanel, Percentage change in maximal mean arterial pressure increaseto CCK₄ after CP-212,454 ( $black-square$ ) or vehicle ( $square$ ). Each point representsthe mean (±S.E.M.) of at least four dogs.

Dose-response effect of CCK_A and CCK_B receptor antagonists on HR and MAP. Dose-response curves for changes in HR and MAP with specific CCK_A and CCK_B receptor antagonists in guinea pigs are shown infigures 3 and 4, respectively.

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Fig. 3. Dose-response curves for the CCK_A receptor antagonist, devazepide ( $black-down-triangle$ ), and the CCK_B receptor antagonists L-365,260 ( $black-square$ ), CP-212,454( $bullet$ ), CI-988 ( $black-triangle$ ), CP-310,713 ( $black-lozenge$ ) to antagonize CCK₄-induced decreasesin HR in the guinea pig. Data are expressed as percentage of controlmaximum response to CCK₄ and each point represents the mean (±S.E.M.)of not less than four guinea pigs.

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Fig. 4. Dose-response curves for the CCK_A receptor antagonist, devazepide ( $black-down-triangle$ ), and the CCK_B receptor antagonists L-365,260 ( $black-square$ ), CP-212,454( $bullet$ ), CI-988 ( $black-triangle$ ), CP-310,713 ( $black-lozenge$ ) to antagonize CCK₄-induced increasesin MAP in the guinea pig. Data are expressed as percentage ofcontrol maximum response to CCK₄ and each point represents themean (±S.E.M.) of not less than four guinea pigs.

The specific CCK_B receptor antagonists, L-365,260, CI-988, CP-212,454 and CP-310,713 produced dose-dependent blockade of HRand MAP changes induced by CCK₄ in the guinea pig. The approximateID₅₀ in decreasing order of potency for inhibition of HR and MAPchanges induced by CCK₄ were 0.04 and 0.02; 0.08 and 0.03; 0.3and 0.5 µmol/kg for CP-310,713, CI-988 and CP-212,454, respectively.The CCK_A receptor antagonist, devazepide, at a single dose of10 µmol/kg (the highest soluble dose achievable) had no effecton the HR or MAP changes induced by CCK₄. The ID₅₀ for L-365,260and devazepide could not be determined because compound solubilityprecluded higher i.v. doses from being given.

Because no tachyphylaxis to CCK₄ was observed in dogs, this model was used to assess the duration of activity of orally actingCCK receptor antagonists. CP-212,454 showed no effect on base-lineHR or MAP after an oral dose of 50 mg/kg (figs. 5 and 6). Forty-fivemin after receiving CP-212,454, the dogs showed a 60 to 80% suppressionof CCK₄-induced increase in HR and MAP that lasted throughoutthe remainder of the 135-min observation period.

	Discussion

Top Abstract Introduction Methods Results Discussion References

Our study demonstrates that the cardiovascular responses to CCK₄ in the guinea pig and dog are mediated by the CCK_B receptorsubtype. Three established models, in vitro receptor binding,inhibition of pentagastrin stimulated phosphatidylinositol hydrolysisin AR 4-2J cells and in vivo inhibition of pentagastrin-inducedacid secretion, were used to rank order the affinity of antagonistsfor the CCK_B receptor. The rank order of potency of antagonistsin blocking CCK₄-induced HR and MAP changes in the guinea pigcorresponded closely to the rank order of their affinity and/oractivity in all three models. The qualitative changes inducedby CCK₄ on HR, but not MAP, appear to be species dependent. CCK₄decreased the HR in the guinea pig although in the dog an increasewas observed. However, in the rat, administration of CCK_8S hasbeen reported to increase HR at low doses but at higher dosesthere is a transient decrease followed by an increase in HR (Janssenet al., 1991). MAP is consistently increased by CCK in studiesperformed in our laboratory using guinea pigs and dogs and byother investigators using rats (Gaw et al., 1995).

The anxiolytic activity of CCK receptor antagonists has been shown to be mediated through the CCK_B-receptor subtype (Harroand Vasar, 1991; Singh et al., 1991). Bradwejn et al. (1992) hasshown that the anxiogenic effects of increasing i.v. doses ofCCK₄ in patients with panic disorders showed a strong relationshipto the increases in HR and diastolic blood pressure experiencedin the same patients. The central or peripheral origin of thecardiovascular activity of CCK in animals is uncertain. No definitivestudy demonstrating the partitioning of CCK into the brain forcentral activity after i.v. administrations has been reported.However, high immunoreactive concentrations of the endogenouspeptide have been found in regions of the brain associated withcardiovascular control such as the nucleus tractus solitarius(NTS) and area postrema (AP) (Newton and Maley, 1985; Howes etal., 1989). These regions can also be indirectly affected by stimulationof CCK at peripheral vagal afferent fibers leading into this areaof the brain (Koyama et al., 1990). This hypothesis is supportedby experiments where i.v. injection of CCK has been shown to stimulategene expression of Fos-like protein, an indicator of neural stimuli,not only in the nucleus tractus solitarius and area postrema,but also in the ventrolateral medulla that receives projectionsfrom the nucleus tractus solitarius (Luckman, 1992).

Although the cardiovascular activity of different CCK peptides has been known for some time, the association to a particularreceptor is just beginning to be addressed. In 1991, Mei and Handescribed that intrathecal CCK₈ can antagonize the hypotensioninduced by µ and $kappa$ opioid agonists. The antagonist activity wasmediated by the CCK_B receptor subtype (Mei and Han, 1993), asevidenced by the 20- to 40-fold greater potency of the CCK_B receptorantagonist, L-365,260, over the CCK_A receptor antagonist, devazepide,to block the effect of CCK₈. More recently, Gaw et al. (1995)concluded that the cardiovascular effects of CCK_8S could be attributedto CCK_A-mediated activity. This conclusion was supported by datathat showed bolus i.v. doses of CCK_8S in the pithed rat producedincreases in the MAP and decreases HR. These effects curiouslywere only partially attenuated with devazepide but not at allwith L-365,260 or CI-988. However, in the same report when CCK₄was used, similar increases in MAP were produced and were unaffectedby treatment with devazepide, L-365,260 or phentolamine. BecauseCCK_8S has almost equal affinity to both the CCK_A and CCK_B receptors(see table 1), the unaccounted for activity observed after devazepidewith CCK_8S may be due to the remaining CCK_B activity. Gaw et al.(1995) also concluded that because neither devazepide nor L-365,260blocked the increase in MAP induced by CCK₄, these effects werenot mediated by either CCK_A or CCK_B receptors. Our data suggestthat even though L-365,260 has affinity for CCK_B in vitro, itis a relatively weak antagonist for CCK_B-mediated activity inall three of our functional assays. In the binding assay, therank order for potency at displacing ¹²⁵I-BH-CCK_8S binding for the CCK_B receptor was CP-310,713 > CI-988> CP-212,454 > L-365,260 > devazepide. The order of potency wasclosely followed for inhibiting pentagastrin-stimulated PI hydrolysisin rat pancreatoma cells and inhibition of pentagastrin-inducedacid secretion in the rat model that also followed the observedactivity in the guinea pig cardiovascular system.

The contribution of CCK to endogenous tone of the cardiovascular system appears to be neglible under normal circumstances.Figures 7 and 8 show that when 1.0 µM/kg of CP-212,454 is givenas a bolus i.v. dose that concentrations are sufficient to antagonizethe transient increases in HR and MAP for at least 135 min yetno changes were observed in the basal values at each time periodbefore CCK₄ challenges. At the highest dose of CP-212,454, therewas a significant decrease in basal HR with no concomitant dropin MAP. The decrease in HR was not blocked by a 0.1 mg/kg i.v.atropine pretreatment (data not shown) indicating that the effectwas not vagally mediated. Two other possibilities are a directnegative chronotropic effect on the heart or a decrease in sympathetictone. In the experimental rat model of hemorrhagic shock, Guariniet al. (1988) has shown that the CCK_8S quickly produces a sustainedelevation in blood pressure and pulse amplitude that is significantlyantagonized by sympatholytics such as prazosin, reserpine andyohimbine. Interestingly, in this study devazepide, given i.v.at 0.01 to 0.05 mg/kg (0.025-0.123 µmol/kg) but not intracerebroventricularly(0.002 mg/kg or 0.005 µmol/kg), completely antagonized the responseof CCK_8S. Although these and other data by Gaw et al. (1995) indicatea sympathetic component for the effect of CCK_8S but not CCK₄,the issue of whether the activity is of central or peripheralorigin still remains unclear because a specific CCK_B receptorantagonist has not been examined centrally.

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Fig. 7. Effect of the CCK_B antagonist on HR changes in the conscious guinea pig. Top panel, Effect of 0.1 µM/kg ( $black-down-triangle$ ), 1.0 µM/kg ( $black-triangle$ ),10 µM/kg ( $black-square$ ) or 3 ml/kg vehicle ( $open circle$ ) of CP-212,454 (i.v.) on HRchanges induced by CCK₄ (20 µg/kg, i.v.) challenges. Bottom panel,Percentage change in maximal heart rate decrease to CCK₄ after0.1 µM/kg (

), 1.0 µM/kg ( $||$ ), 10 µM/kg (

) or 3 ml/kg vehicle( $square$ ) of CP-212,454 (i.v.). Each point represents the mean (±S.E.M.)of at least five guinea pigs.

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Fig. 8. Effect of the CCK_B antagonist on mean arterial blood pressure changes in the conscious guinea pig. Top panel, Effect of 0.1µM/kg ( $black-down-triangle$ ), 1.0 µM/kg ( $black-triangle$ ), 10 µM/kg ( $black-square$ ) or 3 ml/kg vehicle ( $open circle$ )of CP-212,454 (i.v.) on mean arterial pressure changes inducedby CCK₄ (20 µg/kg, i.v.) challenges. Bottom panel, Percentagechange in maximal mean arterial pressure increase to CCK₄ after0.1 µM/kg (

), 1.0 µM/kg ( $||$ ), 10 µM/kg (

) or 3 ml/kg vehicle( $square$ ) of CP-212,454 (i.v.). Each point represents the mean (±S.E.M.)of at least five guinea pigs.

Our data from the dog and the guinea pig suggest that CCK₄-induced cardiovascular changes are mediated by the CCK_B receptorssubtype. This is consistent with reports that a CCK_B receptorantagonist can block the cardiovascular responses in man elicitedby CCK₄ or pentagastrin (Bradwejn et al., 1992). One explanationfor the conflicting observations in the literature would be thatthe CCK_A receptors may reside on peripheral afferent fibers (Luckman,1992) that when stimulated by CCK_8S modulate sympathetic outflowfrom the brain resulting in increases in HR and blood pressurethat are blocked with prazosin or devazepide (Guarini et al.,1988). A separate population of peripheral CCK_B may be more directlyinvolved in modulating cardiovascular responses not influencedby the sympathetic system (Gaw et al., 1995). Therefore theseeffects were previously indistinguishable with the nonspecificagonist, CCK_8S, but can be separated using the selective, peripheralCCK_B agonist, CCK₄.

	Acknowledgments

The authors thank Ms. Laura Ringer and Roxanne Winslow for their invaluable technical assistance with these studies.

	Footnotes

Accepted for publication December 10, 1996.

Received for publication June 11, 1996.

Send reprint requests to: Dr. Anthony A. Fossa, Department of General Pharmacology, Pfizer Central Research, Groton, CT 06340.

	Abbreviations

CCK, cholecystokinin; CCK₄, cholecystokinin tetrapeptide; CCK₈, cholecystokinin octapeptide; CCK_8S, sulfated cholecystokinin octapeptide; CCK_8US, unsulfated cholecystokinin octapeptide; PI, phosphatidylinositol; HR, heart rate; MAP, mean arterial pressure.

	References

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