Role of the beta 3-Adrenoceptor in Urine Storage in the Rat: Comparison between the Selective beta 3-Adrenoceptor Agonist, CL316,243, and Various Smooth Muscle Relaxants

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Vol. 293, Issue 3, 939-945, June 2000

Role of the $beta$ ₃-Adrenoceptor in Urine Storage in the Rat: Comparison between the Selective $beta$ ₃-Adrenoceptor Agonist, CL316,243, and Various Smooth Muscle Relaxants¹

Hiroo Takeda, Yoshinobu Yamazaki, Masuo Akahane, Yasuhiko Igawa, Yukiyoshi Ajisawa and Osamu Nishizawa

Central Research Laboratory, Kissei Pharmaceutical Co., Ltd., Nagano (H.T., Y.Y., M.A., Y.A.); and Department of Urology, Shinshu University School of Medicine, Nagano, Japan (Y.I., O.N.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

The objective of this study was to compare the effects of a $beta$ ₃-adrenoceptor ( $beta$ ₃-AR) agonist on bladder function and cardiovascularparameters in rats with those of several drugs that act on smoothmuscle. CL316,243 ( $beta$ ₃-AR agonist), isoproterenol (nonselective $beta$ -AR agonist), procaterol ( $beta$ ₂-AR agonist), verapamil (Ca²⁺ antagonist), and papaverine (antispastic drug) each evoked aconcentration-dependent relaxation of the detrusor in vitro. Theyalso reduced bladder pressure in anesthetized rats, the $beta$ -AR agonistsapparently being more potent than the other drugs. Atropine (muscarinicantagonist) neither relaxed detrusor strips nor reduced bladderpressure. In anesthetized rats, CL316,243 and atropine each hadonly a slight influence on blood pressure and heart rate, butisoproterenol, procaterol, verapamil, and papaverine significantlyaffected cardiovascular function at the same dose range as thatrequired to reduce bladder pressure. In cystometry experiments,CL316,243 (10 µg/kg i.v.), verapamil (1 mg/kg i.v.), and papaverine(1 mg/kg i.v.) all significantly prolonged micturition intervaland increased bladder capacity, but did not change the residualurine volume after a micturition contraction. Procaterol (100µg/kg i.v.) prolonged the micturition interval and increased bothbladder capacity and residual urine volume (all significantly).Atropine (100 µg/kg i.v.) reduced micturition pressure and increasedresidual urine volume (both significantly). Because the humandetrusor, like the rat detrusor, relaxes on $beta$ ₃-AR stimulation,we conclude that this $beta$ ₃-AR agonist may have potential in pollakiuria(frequent urination) as a therapeutic agent without cardiovascularsideeffects.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Urinary bladder function is controlled by both the parasympathetic and sympathetic nervous systems, their activation mediatingbladder contraction and relaxation, respectively (Andersson, 1993).It is considered that pathophysiologic conditions such as pollakiuria,urgency, and incontinence arise from disturbances of this dualcontrol mechanism (Andersson, 1988). Consequently, drugs suchas muscarinic antagonists (Boman and von Garrelts, 1973; Blaivaset al., 1980), Ca²⁺ antagonists (Palmer et al., 1981), and antispastic drugs (Stanton,1973; Delaere et al., 1977) are considered useful for the treatmentof patients with pollakiuria caused by a hyperactive bladder.However, because they have little or no selectivity for the detrusor,such drugs often produce adverse systemiceffects.

In the bladder, the $beta$ -adrenoceptor ( $beta$ -AR) subtypes mediating sympathetic relaxation of the detrusor differ substantially fromspecies to species. For example, relaxation of the detrusor incats (Nergårdh et al., 1977) and guinea pigs (Li et al., 1992)is mediated mainly via $beta$ ₁-AR, whereas in rabbits (Anderson andMarks, 1984; Levin et al., 1988; Yamazaki et al., 1998) it issaid to be mediated entirely via $beta$ ₂-AR. Moreover, the rat detrusorrelaxes through not only $beta$ ₂-AR, but also $beta$ ₃-AR (Yamazaki et al.,1998) even though all three $beta$ -AR subtype mRNAs are expressed inthe detrusor in this species (Seguchi et al., 1998). We recentlyconfirmed that although all three $beta$ -AR subtype mRNAs are positivelyexpressed in the human detrusor, the major $beta$ -AR subtype responsiblefor its relaxation is neither the $beta$ ₁- nor the $beta$ ₂-AR, but the $beta$ ₃-AR(Igawa et al., 1997, 1998, 1999).

In this study, we used rats to investigate the usefulness of a selective $beta$ ₃-AR agonist on aspects of bladder function closelyrelated to urine storage, and we compared its effects with thoseof other drugs expected to be useful clinically for the treatmentof such bladder dysfunctions as pollakiuria and urinaryincontinence.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Animals

This study was conducted according to guidelines approved by the Laboratory Animal Committee of Kissei Pharmaceutical Co.Ltd. Male and female Sprague-Dawley rats (SLC, Hamamatsu, Japan),weighing from 200 to 380 g at the beginning of the experiments,were used in this study. All rats were group-housed in cages forat least 1 week before the experiment, and they were fed laboratorychow and water ad libitum. The temperature of the room was 23± 1°C, and a 12-h light/dark cycle (lights on at 8:20 AM) wasused.

Isolated Preparations

Male rats, weighing from 250 to 380 g, were anesthetized with diethyl ether. They were then sacrificed, and the urinary bladderwas isolated and placed in Krebs solution of the following composition:118.1 mM NaCl, 4.7 mM KCl, 2.5 mM CaCl₂, 1.2 mM MgSO₄, 25.0 mMNaHCO₃, 1.2 mM KH₂PO₄, and 11.1 mM glucose (pH 7.4). The bladderwas opened longitudinally, and a detrusor strip approximately10 × 2 mm was taken and suspended in a 10-ml organ bath containingKrebs solution. This was maintained at 37°C and continuously gassedwith a mixture of 95% oxygen and 5% carbon dioxide. A restingtension of 0.5 g was applied to the preparation at the beginningof the experiment, and the tissue was equilibrated for at least60 min. The isometric tension generated by the tissue was measuredusing a force-displacement transducer (SB-1T; Nihon-Kohden, Tokyo,Japan) and recorded on a rectigraph (Rectigraph 8K; NEC San-ei,Tokyo, Japan). Concentration-response curves were obtained bycumulative addition of the appropriate drug to the bathing fluid.Each preparation was exposed to only one drug. All experimentswere conducted in the presence of 10⁶ M phentolamine, an $alpha$ -adrenoceptorantagonist.

In Vivo Experiments

Bladder Pressure in Anesthetized Rats. Male rats, weighing from 300 to 350 g, were anesthetized with urethane (1.5 g/kg s.c.). Through a midline abdominal incision,the pelvic viscera were exposed, and the ureter on each side wasligated and cut proximal to the ligature so as to allow urineto drain into cotton wads. After the urethra had been ligated,a polyethylene catheter (PE-50; Nihon Becton Dickinson, Tokyo,Japan) was inserted into the urinary bladder via the top of thebladder dome and connected through a three-way connector to apressure transducer (SPB-108; NEC San-ei) and a syringe filledwith warmed saline. The initial bladder pressure was adjustedto 6 cm H₂O by instillation of warmed saline (37°C) in 0.05-mlincrements. An arterial catheter was inserted into the left carotidartery (PE-90; Nihon Becton Dickinson) and connected to a pressuretransducer (SPB-108) for the measurement of blood pressure. Heartrate was measured via a tachometer (1321; NEC San-ei) connectedto the transducer amplifier (1829; NEC San-ei). Blood pressure,heart rate, and bladder pressure were recorded continuously ona rectigraph (Recti-Horiz-8K; NEC San-ei). Drug effects on bladderpressure, blood pressure, and heart rate were quantified by expressingeach postadministration value as a percentage of the value beforedrug administration. Each animal was either exposed to only onedose of each drug, or exposed to more than one dose of a givendrug with an interval of 60 min allowed between applications sothat each parameter could recover to its initial value. No animalwas exposed to more than one of the test drugs. A venous catheterwas inserted into the left femoral vein (PE-50; Nihon Becton Dickinson)for druginjection.

Cystometry in Anesthetized Rats. Female rats, weighing from 200 to 230 g, were anesthetized with urethane (1.0 g/kg s.c.). Through a midline abdominal incision,the ureter on each side was ligated and cut proximal to the ligature.A polyethylene catheter (PE-50) was inserted into the urinarybladder and connected through a three-way connector to: 1) a pressuretransducer (SPB-108) for measurement of bladder pressure, and2) a syringe infusion pump (KD Scientific model 100; MuromachiKikai, Tokyo, Japan) for continuous infusion of saline into thebladder. Micturition volumes were measured by means of a fluidcollector connected to a force displacement transducer (Type 45196A;NEC San-ei). During cystometry, warmed saline was infused at arate of 3.6 ml/h. Bladder pressure and micturition volumes wererecorded continuously on a rectigraph (Recti-Horiz-8K). The followingcystometric parameters were obtained: micturition interval, micturitionpressure (maximum bladder pressure during micturition), micturitionvolume (volume of urine expelled), residual volume (residual volumeat the previous micturition plus volume of saline infused up tothe time of micturition minus micturition volume), and bladdercapacity (micturition volume plus residual volume). Two reproduciblemicturition cycles were recorded before drug administration andused to provide a baseline value to be compared with the firsttwo micturition cycles just after drug administration. Relativevalues for the various cystometric parameters were calculatedas follows: (mean value from two micturition cycles just afterdrug administration)/(mean value from two micturition cycles justbefore drug administration). Each animal was exposed to only onedose of one drug. A venous catheter was inserted into the leftfemoral vein for druginjection.

Analysis of Data

The results are expressed as mean ± S.E. Statistical analysis was performed using a one-way ANOVA followed by Dunnett's multiple-comparisonmethod. A probability level less than .05 was accepted as significant.The JMP Statistics and Graphics Guide (version 3.1; SAS InstituteInc., Cary, NC) was used as the resource text for the statisticalanalysis.

Drugs

The following drugs were used: atropine sulfate monohydrate (Wako Pure Chemical, Osaka, Japan), ( $-$ )-isoproterenol (+)-bitartrate,procaterol hydrochloride, (±)-verapamil hydrochloride, papaverinehydrochloride, urethane (Sigma Chemical Co, St. Louis, MO), andphentolamine mesylate (Ciba-Geigy, Basel, Switzerland). CL316,243[(R,R)-5-[2-[[2-(3-chlorophenyl)-2-hydroxyethyl]amino]propyl]-1,3-benzodioxole-2,2-dicarboxylate]was synthesized in our laboratories (Kissei, Hotaka, Japan). Thedrugs were dissolved in distilled water for the in vitro study,but in saline for the in vivo study. The solutions were preparedon the day of the experiment and kept in dark vessels to minimizelight-induceddegradation.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Isolated Preparations

The $beta$ -AR agonists isoproterenol, procaterol, and CL316,243 all caused concentration-dependent relaxation of the detrusor (Fig.1). The EC₅₀ values were (9.84 ± 2.29) × 10⁹ M for isoproterenol, (1.62 ± 0.76) × 10⁸ M for procaterol, and (7.08 ± 1.56) × 10⁹ M for CL316,243. Verapamil and papaverine relaxed the detrusoronly at the high end of their concentration range, the EC₅₀ valuesbeing (5.29 ± 1.25) × 10⁶ and (2.00 ± 0.28) × 10⁵ M, respectively. The intrinsic activities of these agents (relativeto that of isoproterenol, 1.0) were calculated to be 1.02 forprocaterol, 0.96 for CL316,243, 0.94 for verapamil, and 1.08 forpapaverine. Atropine had only a weak relaxing effect on the detrusor.As the relative intrinsic activity of atropine was 0.11 even atconcentrations of 10⁵ M or more, we could not calculate an EC₅₀ value for this drug.

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Fig. 1. Concentration-response curves for effects of test drugs on basal tone of rat detrusor. Each point is the mean ± S.E. of five to six experiments. $open circle$ , isoproterenol; $black-triangle$ , CL316,243; $black-square$ , procaterol;

, atropine;

, verapamil; $triangle$ , papaverine.

In Vivo Studies

Effects on Bladder Pressure and Cardiovascular Variables in Anesthetized Rats. Figure 2 shows representative recordings of bladder pressure, blood pressure, and heart rate in rats given isoproterenol orCL316,243 by i.v. administration. The mean values for bladderpressure, blood pressure, and heart rate before drug administrationwere 6.00 ± 0.26 cm H₂O, 103 ± 2 mm Hg, and 414 ± 7 beats/min,respectively. Tables 1, 2, and 3 show the maximum responseduring the observation for 30 min after the drug administration.Injection of vehicle (saline, 1 ml/kg i.v.) had no effect on theseparameters. Isoproterenol (10 µg/kg i.v.) significantly reducedboth bladder pressure and blood pressure, and significantly increasedheart rate. CL316,243 (100 µg/kg i.v.) also reduced bladder pressuresignificantly, but the changes in blood pressure and heart ratewere minimal. Table 1 summarizes the effects of the test drugson bladder pressure. The data for each parameter are expressedas a percentage of the preadministration value. All three $beta$ -ARagonists produced a dose-dependent reduction in bladder pressure.CL316,243 had the longest duration of action among these drugs,bladder pressure did not return to preadministration value at120 min after CL316,243 (100 µg/kg) administration. At their highestdose, isoproterenol, procaterol, and CL316,243 significantly reducedbladder pressure to 77.7, 72.8, and 65.8%, respectively, of theresting pressure. Procaterol (100 µg/kg) plus CL316,243 (100 µg/kg)reduced bladder pressure to 63.6% of the resting pressure (datanot shown). Isoproterenol lowered blood pressure to 69.2% of theresting value (10 µg/kg) and increased heart rate to 122.6% (at1 µg/kg) (Tables 2 and 3). Procaterol produced a decrease inblood pressure to 72.3% (at 100 µg/kg i.v.) and a slight increasein heart rate to 106% (at 100 µg/kg). CL316,243 had only weakeffects on blood pressure and heart rate; the values obtainedwere 87.9 and 100.1%, respectively, of the basal values (at 100µg/kg). Blood pressure and heart rate 120 min after CL316,243(100 µg/kg) administration were 86.9 ± 3.4 and 105.8 ± 3.3%, respectively,of their basal values. Atropine reduced neither bladder pressurenor heart rate. Verapamil and papaverine produced similar effectsto each other on bladder pressure, blood pressure, and heart ratein anesthetized rats. Bladder pressure was reduced slightly byboth verapamil (1 mg/kg i.v.) and papaverine (10 mg/kg i.v.),to 91.4 and 84.5% of the resting pressure, respectively. Bothdrugs induced a greater percent decrease in blood pressure thanin bladder pressure. The heart rate was slightly decreased bythese two drugs.

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Fig. 2. Changes in bladder pressure, blood pressure, and heart rate in anesthetized rats. A, representative recordings from in vivo experiments in anesthetized rats showing changes in bladder pressure, blood pressure, and heart rate after isoproterenol or CL316,243 (both by i.v. administration). B, time course of bladder pressure, blood pressure, and heart rate in anesthetized rats after i.v. saline (1 ml/kg, ×), isoproterenol (10 µg/kg, $open circle$ ), CL316,243 (10 µg/kg,

), procaterol (10 µg/kg,

), atropine (1 mg/kg, $black-square$ ), verapamil (1 mg/kg, $triangle$ ), and papaverine (10 mg/kg, $black-triangle$ ) administration. Results are expressed as a percentage of the value before drug administration, and are given as the mean ± S.E. of five to eight animals.

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TABLE 1
Effects of isoproterenol, CL316,243, procaterol, atropine, verapamil, and papaverine on bladder pressure in urethane-anesthetized rats
Results are expressed as a percentage of the value before drug administration, and are given as the mean ± S.E. of data from seven to eight animals. The values show the maximum response during the observation for 30 min after the drug administration.

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TABLE 2
Effects of isoproterenol, CL316,243, procaterol, atropine, verapamil, and papaverine on blood pressure in urethane-anesthetized rats
Results are expressed as a percentage of the value before drug administration, and are given as the mean ± S.E. of data from seven to eight animals. The values show the maximum response during the observation for 30 min after the drug administration.

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TABLE 3
Effects of isoproterenol, CL316,243, procaterol, atropine, verapamil, and papaverine on heart rate in urethane-anesthetized rats
Results are expressed as a percentage of the value before drug administration, and are given as the mean ± S.E. of data from seven to eight animals. The values show the maximum response during the observation for 30 min after the drug administration.

Cystometry in Anesthetized Rats. Figure 3 shows representative recordings of cystometrograms taken from anesthetized rats. The mean values for the variouscystometric parameters before drug administration (n = 133 inall animals tested) were as follows: micturition interval, 6.34± 0.20 min; micturition pressure, 30.86 ± 0.54 cm H₂O; micturitionvolume, 0.36 ± 0.01 ml; residual urine volume, 0.40 ± 0.02 ml;bladder capacity, 0.75 ± 0.02 ml. Table 4 shows relative valuesfor these cystometric parameters after drug administration. Injectionof vehicle (saline, 1 ml/kg i.v.) had no effect on the cystometricparameters. Procaterol (1 to 100 µg/kg i.v.) increased bladdercapacity, prolonged micturition interval, and increased residualurine volume in a dose-dependent manner. Relative values for bladdercapacity, micturition interval, and residual urine volume were1.39 ± 0.09, 1.30 ± 0.08, and 1.70 ± 0.30, respectively, afterthe administration of procaterol at 100 µg/kg. CL316,243 (10 and100 µg/kg i.v.) significantly increased bladder capacity, andprolonged micturition interval by 1.3-fold or more, effects comparablein size to those produced by procaterol. With CL316,243 at thesedoses, micturition pressure was reduced by about 10%, but residualurine volume was not increased significantly. Combined administrationof procaterol (100 µg/kg) with CL316,243 (100 µg/kg) increasedboth bladder capacity and residual volume, and prolonged micturitioninterval (all significantly). Atropine (10 µg/kg to 1 mg/kg i.v.)reduced micturition pressure and increased residual volume toin a dose-dependent manner; residual volume was 2 times the controlvalue at 1 mg/kg. Verapamil (1 mg/kg i.v.) and papaverine (1 and10 mg/kg i.v.) each increased bladder capacity and prolonged micturitioninterval (both significantly), but of these two drugs, only papaverine(10 mg/kg i.v.) produced a significant increase in residual volume.

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Fig. 3. Representative recordings from cystometric investigations in urethane-anesthetized rats. At the arrow, saline (A), CL316,243 (B), procaterol (C), atropine (D), verapamil (E), or papaverine (F) was administered i.v. Asterisk (*) indicates adjustment to baseline position.

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TABLE 4
Effects of CL316,243, procaterol, atropine, verapamil, and papaverine on cystometric parameters in urethane-anesthetized rats
Relative values for the various cystometric parameters were calculated as follows: (mean value from two micturition cycles just after drug administration)/(mean value from two micturition cycles just before drug administration). Results are expressed as mean ± S.E. of data from seven to eight animals.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Although it is accepted that the sympathetic nervous system plays an important role in the control of micturition in a varietyof species, including humans, its role in human bladder functionhas been the subject of much debate, partly because of the paucityof adrenergic innervation of the human detrusor. Recently, attentionhas focused on the $beta$ ₃-AR after the publication of evidence ofits existence in the detrusor and of its importance in the relaxationof the human detrusor during adrenergic stimulation (Igawa etal., 1997, 1998, 1999). It has been reported that $beta$ ₃-AR also playan important role in the relaxation of the detrusor in rats inassociation with $beta$ ₂-AR (Yamazaki et al., 1998).

In this study, we attempted to gain some insight into the potential usefulness of a $beta$ ₃-AR agonist as a therapeutic agent forpollakiuria by comparing its effects in rats with those of severalsmooth muscle relaxants including a $beta$ ₂-AR agonist, a muscarinicantagonist, a Ca²⁺ antagonist, and an antispasticagent.

All of the $beta$ -AR agonists tested (isoproterenol, procaterol, and CL316,243) not only relaxed the detrusor in vitro, but alsoreduced bladder pressure in vivo in rats. The maximal reductionin bladder pressure induced in vivo did not differ among the threedrugs. The rank order of potency in vivo was isoproterenol (nonselective $beta$ -AR agonist) > procaterol ( $beta$ ₂-AR agonist, Yoshizaki et al., 1976)= CL316,243 ( $beta$ ₃-AR agonist, Bloom et al., 1992). Combination ofprocaterol with CL316,243 at the highest dose of each drug (100µg/kg) did not produce any additional reduction in bladder pressurebeyond the level achieved with CL316,243 alone. In terms of theircardiovascular effects, isoproterenol increased heart rate, whereasboth isoproterenol and procaterol lowered blood pressure significantlyas a result of their respective stimulating effects on $beta$ ₁- and $beta$ ₂-ARs (Lands et al., 1967a,b). In the rat heart, $beta$ ₃-AR mRNA isnot detectable in the atria or in the right ventricular myocardium,and there is a low level of $beta$ ₃-AR mRNA in the left ventricle,which contains major blood vessels (Evans et al., 1996). Furthermore,there has been no report of the existence of $beta$ ₃-AR mRNA in aortaor veins. In this study, CL316,243 produced only slight effectson heart rate and blood pressure, presumably because of its excellent $beta$ ₃-AR selectivity (Bloom et al., 1992; Dolan et al., 1994). Inthe cystometry test, CL316,243 increased bladder capacity, leadingto an apparent prolongation of micturition interval. Micturitionpressure was slightly but significantly reduced, and residualurine volume tended to increase only at higher doses of CL316,243.The major neuronal stimulus for physiological bladder contractionis an acetylcholine-induced stimulation of parasympatheticallyinnervated muscarinic receptors on the detrusor. Because isoproterenol(30 µM) does not affect the (+)-cis-dioxolane (muscarinic agonist)-inducedconcentration-dependent contraction of rat detrusor preparations(Hegde et al., 1997), a specific $beta$ -AR agonist, such as CL316,243,might be expected to lack a significant influence over the bladdercontraction induced by acetylcholine at the time of micturition.The results of this study demonstrate that in the rat, CL316,243,a $beta$ ₃-AR agonist, is the most selective at prolonging the micturitioninterval among the $beta$ -AR agonists we tested, and that it has theweakest cardiovascular side effects among these agents. Procaterol,a $beta$ ₂-AR agonist, prolonged micturition interval and significantlyincreased residual urine volume without reducing micturition pressure.Because procaterol has been found to increase the contractileforce induced in the rabbit external urethral sphincter by electricalfield stimulation (Morita et al., 1995), it seems likely thatthis agent produces an increase in residual urine volume as aconsequence of its stimulating effect on the external sphincter.The changes in cystometric parameters observed after the combinedadministration of CL316,243 with procaterol could be explainedas a result of a simple summation of their effects (Table 4).

Atropine, a nonselective muscarinic antagonist, relaxed the detrusor muscle hardly at all in vitro or in vivo. In the cystometryexperiment, atropine reduced micturition pressure and shortenedmicturition interval in a dose-dependent manner. Although atropinedelayed the first micturition occurring just after drug administration,it simultaneously lowered micturition pressure. As a consequence,residual urine volume was increased and the next micturition occurredsooner, without an increase in bladder capacity. Urinary bladdersmooth muscle is rich in muscarinic receptors, both M₂- and M₃-subtypesbeing present in the rat (Hegde et al., 1997), and their stimulationleads to contraction of the bladder. Our study suggests that atropinereduces micturition pressure by antagonizing micturition stimuliarriving through the pelvic nerve, leading to an augmented retentionof urine, but that when the bladder pressure is below thresholdpressure, the collecting phase for urine, this drug has no effecton bladderpressure.

It is well known that Ca²⁺ is essential for producing contractile activity in smooth muscle. Verapamil, a Ca²⁺ antagonist, also relaxed the detrusor in a concentration-dependentmanner in vitro, and reduced bladder pressure in vivo, in rats.In the cystometry experiment, verapamil increased bladder capacityand prolonged micturition interval at a dose that reduced bladderpressure (1 mg/kg i.v.), but it did not affect micturition pressureat this dose. It has been reported that verapamil attenuated theintensity of both spontaneous and carbachol-induced contractionsof the rat detrusor (Maggi et al., 1982). In addition, there isanother report showing that verapamil (1 mg/kg i.v.) increasedbladder capacity without reducing micturition pressure in anesthetizeddogs (Kaneko et al., 1989). Our data are mostly in accord withthese reports. However, the effect of verapamil was not selectivefor bladder function; indeed, it produced significant decreasesin both blood pressure and heart rate. In actual fact, a significantdecrease in blood pressure was induced by verapamil at doses lowerthan those producing an apparent reduction in bladder pressurein anesthetizedrats.

In this experiment, papaverine relaxed the detrusor in vitro in a concentration-dependent manner and reduced bladder pressurein vivo, just as verapamil did. In the cystometry experiment,papaverine increased bladder capacity and prolonged the micturitioninterval in a dose-dependent manner. Neither micturition pressurenor micturition volume changed after an i.v. injection of papaverineat 10 mg/kg. However, residual urine volume was increased significantlyat this dose. Moreover, its cardiovascular side effects were extremelysevere compared with those of verapamil. Indeed, at a dose of10 mg/kg (which was effective at reducing bladder pressure inour anesthetized rats), papaverine produced a significant decreasein blood pressure (to 56% of basal blood pressure), leading tothe death of the rat in some cases. Papaverine, an antispasticdrug, is known to be a nonspecific phosphodiesterase inhibitor(Kukovetz and Pöch, 1970); it produces a nonselective relaxationof smooth muscle. In terms of its influence on bladder functionin rats, papaverine proved to be a less selective drug. In fact,although papaverine increased residual urine volume, it does nothave a contraction-repressing action as muscarinic antagonistsdo, and its systemic side effects were so severe as to lead tothe death of some of therats.

In conclusion, this study has clearly shown that the effects of $beta$ -AR agonists in reducing bladder pressure in rats are morepronounced than those of a muscarinic antagonist, a Ca²⁺ antagonist, and an antispastic drug. Although the $beta$ ₃-AR agonistand the Ca²⁺ antagonist we tested were each effective in increasing bladdercapacity and in prolonging the micturition interval without increasingresidual urine volume, the $beta$ ₃-AR agonist had much weaker cardiovascularside effects. In humans, as in the rat, $beta$ ₃-AR mRNA has been detectedin the bladder (Igawa et al., 1999), and only a low level of $beta$ ₃-ARmRNA is present in the human heart (Krief et al., 1993; Berkowitzet al., 1995) and probably in blood vessels. Consequently, $beta$ ₃-ARagonists would be expected to have fewer and weaker cardiovascularside effects than those produced by $beta$ -AR agonists acting on $beta$ ₁-and/or $beta$ ₂-AR. Our data strongly support this idea. Because thehuman detrusor relaxes mainly through $beta$ ₃-AR stimulation, we suggestthat the $beta$ ₃-AR agonist may have a potential role in pollakiuriaas a useful therapeutic drug without cardiovascular sideeffects.

	Footnotes

Accepted for publication February 14, 2000.

Received for publication December 13, 1999.

¹ Part of this investigation was presented at the 1st International Consultation on Incontinence (Takeda H. et al., June 28,1998) and at the XIIIth International Congress of Pharmacology(Takeda H. et al., July 26,1998).

Send reprint requests to: Hiroo Takeda, Central Research Laboratory, Kissei Pharmaceutical Co. Ltd., 4365-1, Hotaka, Nagano-Pref., 399-8304, Japan. E-mail: hiroo_takeda{at}pharm.kissei.co.jp

	Abbreviations

$beta$ -AR, $beta$ -adrenoceptor; CL316,243, (R,R)-5-[2-[[2-(3-chlorophenyl)-2-hydroxyethylamino]propyl]-1,3-benzodioxole-2,2-dicarboxylate.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

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