Involvement of Alpha-2 Adrenoceptors in the Effects of Moxonidine on Intestinal Motility and Fluid Transport

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Vol. 283, Issue 3, 1367-1374, 1997

Involvement of Alpha-2 Adrenoceptors in the Effects of Moxonidine on Intestinal Motility and Fluid Transport

Lu Liu and Ian M. Coupar

Department of Pharmaceutical Biology and Pharmacology, Victorian College of Pharmacy, Monash University, Parkville, Victoria, Australia

	Abstract

Abstract Introduction Methods Results Discussion References

The aims of this study were to examine how the imidazoline (I)₁/alpha-2 receptor agonist moxonidine and the putative endogenousimidazoline receptor agonist agmatine might affect intestinalmotility and fluid transport. The effects of moxonidine were comparedwith those of UK 14,304, a highly selective alpha-2 adrenoceptoragonist with very low affinity for I₁ receptors. Moxonidine andUK 14,304 inhibited the peristaltic reflex in the isolated ratileum. The inhibitory effects were antagonized by the selectivealpha-2 adrenoceptor antagonist yohimbine and the I₁/alpha-2 antagonistefaroxan and almost completely blocked by the irreversible alpha-2adrenoceptor antagonist EEDQ (N-ethoxycarbonyl-2-ethoxy-1,2-dihydroquinoline),whichhas a low affinity for imidazoline receptors. Yohimbine (3µM) and efaroxan (0.01 and 1 µM) caused parallel rightward shiftsto the concentration-response curves of moxonidine and UK 14,304,yielding pK_B values corresponding to those at alpha-2binding sites. Moxonidine induced dose-dependent proabsorptiveeffects in the jejunum and ileum and also reversed the secretoryphase of the vasoactive intestinal peptide-induced responses.The degree of antagonism by yohimbine and efaroxan was similaragainst moxonidine and UK 14,304 on the proabsorptive and antisecretoryeffects. We conclude that the effects of moxonidine in mediatinginhibition of intestinal motility and enhancing fluid transportare attributed predominantly to interaction with alpha-2 adrenoceptors.Agmatine had no effect on peristalsis but significantly decreasedthe rate of fluid absorption from the jejunum and ileum, an effectin contrast to moxonidine. A physiological role for agmatine inthe regulation of intestinal transport remains to be clarified.

	Introduction

Abstract Introduction Methods Results Discussion References

It is well accepted that I derivatives such as clonidine and idazoxan bind to alpha-2 adrenoceptors. In recent years, it hasbeen recognized that in addition, they interact with distinctnonadrenergic binding sites or I-preferring receptors. Radioligandbinding studies have demonstrated that I receptors exist in twomain subtypes: the clonidine-preferring receptor (I₁) and theidazoxan-preferring receptor (I₂) (for reviews, see Michel andInsel, 1989; Regunathan and Reis, 1996).

Recent studies have indicated that a number of drug effects previously attributed to activity at alpha-2 adrenoceptors mayin fact be mediated through activation of I receptors. In particular,there is strong evidence that the antihypertensive actions ofclonidine and related drugs, moxonidine and rilmenidine are primarilymediated by stimulation of central I₁ receptors in the rostralventrolateral medulla rather than by alpha-2 adrenoceptors (Bousquetet al., 1984; Ernsberger et al., 1990, 1992; Haxhiu et al., 1994;Head, 1995; Tibirica et al., 1991). There also is evidence thatactivation of I₁ receptors increases renal excretion of sodiumand water (Allan et al., 1993; Penner and Smyth, 1994; Smyth etal., 1992). In addition, moxonidine has been suggested to regulategastric secretion and protect against gastric mucosal injury throughactivation of I₁ receptors (Carlisle et al., 1995; Glavin andSmyth, 1995).

We demonstrated that alpha-2D adrenoceptors are involved in the control of intestinal motility and fluid transport in rats(Liu and Coupar, 1996, 1997). Whether I receptors are involvedin the regulation of these intestinal activities has not yet beendetermined. Therefore, moxonidine, which has been shown to displaya much greater selectivity and affinity for I₁ receptors overalpha-2 adrenoceptors (70-600 fold, Ernsberger et al., 1992, 1993),was used to investigate how it affects intestinal motility andfluid transport. UK 14,304, which is a selective alpha-2 adrenoceptoragonist (Cambridge, 1981) with low affinity for I₁ receptors (I₁/alpha-2affinity ratio <0.01, Bricca et al., 1993; Ernsberger et al.,1992), was used for comparison. The interactions with yohimbine,a selective alpha-2 adrenoceptor antagonist (Goldberg and Robertsson,1983) with very low affinity for I binding sites (I₁/alpha-2 affinityratio <0.01, Ernsberger et al., 1987, 1992; Hamilton et al., 1988,Senard et al., 1990), efaroxan, an I₁/alpha-2 receptor antagonistwith $approx$ 30-fold selectivity for I₁ receptors compared to alpha-2adrenoceptors (Ernsberger et al., 1992; Haxhiu et al., 1994),and EEDQ, an irreversible alpha-2 adrenoceptor antagonist withvery low affinity for I receptors (Pineda et al., 1993; Ruiz-Ortegaet al., 1995), were also studied.

It has been suggested that agmatine (decarboxylated arginine) is an endogenous neurotransmitter at alpha-2 adrenoceptors andI receptors (Li et al., 1994; Gonzalez et al., 1996). Like clonidine,it binds to alpha-2 adrenoceptors of all subclasses (Bylund, 1995)and I receptors of both subclasses (Li et al., 1994; Piletz etal., 1995). Agmatine and its biosynthetic enzyme, arginine decarboxylase,have been identified in a number of mammalian tissues, includingbrain, stomach, intestine and aorta (Li et al., 1994; Raasch etal., 1995). However, possible functions of agmatine mediated byalpha-2 adrenoceptors and I receptors are not yet clearly apparent.We have, therefore, attempted to examine whether agmatine modulatesrat intestinal activities in the in vivo and in vitro models describedin this study.

	Methods

Abstract Introduction Methods Results Discussion References

Peristalsis

The method used in this study has been described in detail by Coupar (1995). Briefly, hooded Wistar male rats (250-350 g)were stunned by a blow to the head and killed by exsanguination.Segments of ileum (15 cm proximal to the caecum) were excisedand tied at the aboral end onto a glass J tube. Each tissue wasplaced in a 30 ml jacketed organ bath containing Krebs-Henseleitsolution of the following composition (in mM): NaCl, 118; KCl,4.7; NaHCO₃, 25; KH₂PO₄, 1.2; CaCl₂, 2.5; MgSO₄, 1.2;and D-(+)-glucose,11, maintained at 37°C and continuously gassed with 95% oxygen/5%carbon dioxide. Segments were tied off at the oral end to givelengths of between 7 and 9 cm, and the cotton thread was connectedto an isotonic transducer (Ugo Basil, Varese, Italy) to monitorlength changes of the longitudinal smooth muscle under a restingtension of 1 g. The free end of the J tube was connected by flexibletubing to a 5-ml float chamber half-filled with Krebs-Henseleitsolution.

The float was connected to a second isotonic transducer to record volume changes related to circular muscle contraction. Boththe reservoir and transducer (volume meter) were attached to awormscrew stand, enabling them to be raised gradually above thefluid level of the organ bath to increase intraluminal pressurein the ileum and initiate peristaltic contractions. The frequencyand intensities of the longitudinal and circular muscle contractionswere recorded on a Grass model 79D polygraph.

After a 45-min equilibration period, the intraluminal pressure was increased gradually at $approx$ 3 mm/sec until it initiated a peristalticwave. This was recorded as a contraction of the longitudinal muscle(preparatory phase) closely followed by expulsion of fluid (circularmuscle contraction). The pressure resulting in a peristaltic contractionwas maintained for two periods of 15 min separated by a rest periodof 10 min at zero pressure. In each period, three to four controlperistaltic contractions were recorded before the agonists, moxonidine,rilmenidine or UK 14,304, were added cumulatively to the bathfluid until obvious decreases in the rate of peristaltic contractionsoccurred. The antagonists, yohimbine or efaroxan, added 10 minbefore the control contractions were present in the bathing fluidfor $approx$ 15 min before addition of agonist. Some tissues were pretreatedwith the irreversible alpha-2 adrenergic antagonist EEDQ at aconcentration of 3 µM for 20 min, followed by a 20-min washoutperiod before application of agonists. In some experiments, agmatinewas tested either as an agonist or as an antagonist against UK14,304 in the presence of the DAO inhibitor aminoguanidine 1 µM.

Intestinal Fluid Transport

Surgical and analytical procedures. The method follows that described in detail by Coupar (1985). In brief, hooded Wistar male rats (220-300 g weight) were deprivedof food over night but had free access to water. Rats were anesthetizedwith pentobarbital sodium (60 mg/kg s.c., supplemented when necessary)and placed on an electrically heated pad at $approx$ 35°C. The tracheawas cannulated and a second cannula was introduced into the leftjugular vein for administration of the agonist and/or antagonist,or in the case of controls, saline or vehicle at volumes of 0.1ml/100 g. Another cannula was introduced into the left commoncarotid artery for constant infusions of saline as control, agmatineor VIP (.8 µg/min) in saline into the aortic arch at a rate of40 µl/min by means of a microinjection pump (CMA/microdialysis,Stockholm, Sweden). MAP was recorded to monitor the conditionof the animals from a side-arm off the carotid cannula by meansof a Gould pressure transducer (Statham, Costa Mesa, CA) connectedto a Neotrace (Neomedix Systems, Sydney, Australia) recorder.

A recirculation technique was used to measure the net fluid transport rates of the jejunum and ileum. Twenty- to 30-cm lengthsof the proximal jejunum (beginning distal from the ligament ofTrietz) and distal ileum (ending 2 cm from the ileocecal junction)were isolated, cannulated at each end and rinsed free of luminaldebris. Each loop was continuously perfused with 8 ml of an isosmoticsolution containing (in mM): NaCl 148, KCl 5, glucose 5.5 andphenol red 0.05, as a nonabsorbable water marker. The solutionswere contained in reservoirs maintained at 37°C and recirculatedthrough each lumen by gas lift with moistened CO₂ (5%) in O₂ fora period of 20 min. The pressure in the loops was 10 cm of H₂Oand the flow rates were $approx$ 60 ml/min.

The fluid from each loop was recovered at the end of the 20-min perfusion period, centrifuged and then diluted (2:25) withNaHCO₃/Na₂CO₃ buffer (pH 10.5). Peak absorbances were measuredat 560 nm as well as 520 and 600 nm to correct for nonspecificinterferences as described by Miller and Schedl (1972)

. The resultswere expressed as the amount absorbed (+) or secreted ( $-$ ) in µl/gwet weight tissue during the 20-min perfusion.

Systemic drug administration. In studies to determine the effect of drug treatments on basal absorption and VIP-induced secretion, the administration sequencecommenced with the i.v. injection of moxonidine, UK 14,304, vehicleor saline as the control. At 5 min later, the i.a. infusion ofsaline (for the basal absorption series of experiments) or VIP(for the secretion series) was commenced with associated measurementof MAP. The loops of jejunum and ileum were washed before intestinalperfusion was started at 10 min. At 30 min, the loops were removedand the perfusion fluid was collected for analysis. The segmentswere weighed after the removal of fluid content. The testing ofthe antagonists followed a similar protocol to above, except thatthe antagonists were injected i.v. 5 min before injecting moxonidine,UK 14,304 or saline. In some experiments, agmatine was infusedi.a. at rates of 0.1, 0.3 and 1 µmol/min and continued for thelength of the 20 min luminal perfusion which commenced 5 min later.Agmatine was administered by i.a. infusion to reduce the influenceof metabolism by endogenous enzymes because it has been reportedthat agmatine is a substrate for DAO.

Drugs

Agmatine sulfate, efaroxan hydrochloride and UK 14,304 [5-bromo-6-(2-imidazolin-2-yl-amino)-quinoxaline] were obtained fromResearch Biochemicals (Natick, MA); moxonidine hydrochloride fromBeiersdorf-Lilly (Hamburg, Germany); rilmenidine dihydrogenphosphatefrom Servier Laboratories (Hawthorn, Victoria, Australia); andbonyl-2-ethoxy-1,2-dihydroquinoline) from ICN Biochemicals (Aurora,OH).

EEDQ was dissolved in ethanol and then diluted in saline so that the final concentration of ethanol in the bath was <0.05%.UK 14,304 was dissolved in DMSO and further diluted with saline.Preliminary control experiments established that the bath concentrationof DMSO did not affect tissue responses. Also, the dilution ofDMSO (8%) did not influence basal values of absorption or VIP-inducedsecretion (Liu and Coupar, 1997; Hancock and Coupar 1997). Allother drugs were dissolved in 0.9% saline.

Statistical Analysis

Results are presented as arithmetic mean ± S.E.M. The peristaltic inhibitory effect of the agonists was expressed as a percentageof the contraction rate present before addition of the agonists.Semilogarithmic linear regression analysis (Tallarida and Murray,1987) was used to determine the potencies of the agonists, whichare expressed as IC₅₀ values defined as the concentration causinga 50% inhibition in the rate of peristalsis. The negative logarithmof receptor dissociation constants of yohimbine and efaroxan (pK_B)were calculated using the equation: pK_B = $-$ log [B] +log (DR $-$ 1) (Furchgott, 1972), where [B] is the one point molarconcentration of antagonist and DR (dose ratio) is the ratio ofthe agonist IC₅₀ in the presence of antagonist, divided by theIC₅₀ in the absence of antagonist. Student's unpaired t test wasused to compare individual means for differences, and one-wayanalysis of variance followed by Dunnett's t test was used tocompare treatment means with a common control and Bonferroni'stest for multiple comparisons (Prism, GraphPAD Software, San Diego,USA). The criterion for statistical significance was set at P< .05.

	Results

Abstract Introduction Methods Results Discussion References

Peristalsis

In control preparations of rat ileum, a mean pressure of 4.9 ± 0.2 cm H₂O (n = 11) was required to initiate rhythmic contractionsof the longitudinal muscle and associated volume expulsions. Thefrequency of peristalsis remained the same over 15 min at 0.66± 0.05 peristaltic waves/min (n = 11).

Inhibitory effect of agonists on peristalsis. The alpha-2 adrenoceptor agonist UK 14,304 (1-10 nM) and I₁/alpha-2 receptor agonists moxonidine (10-100 nM) and rilmenidine(50-300 nM) all induced concentration-dependent decreases in therate of peristalsis with the after order of potency: UK 14,304> moxonidine > rilmenidine. IC₅₀ values were (95% CI in parentheses):UK 14,304, 4.1 nM (2.3-7.3, n = 5); moxonidine, 35.0 nM (19.6-62.2,n = 5) and rilmenidine, 145.0 nM (91.9-228.8, n = 5). At concentrations $approx$ 10 times higher than the IC₅₀ values, each agonist completelyblocked the peristaltic reflex, but the inhibitory effects, however,were reversible on wash out.

Influence of yohimbine and efaroxan on the inhibitory effect of agonists. The addition of yohimbine (3 µM, 10- min incubation) or efaroxan (0.01 or 1 µM, 10-min incubation) to the bathing fluid didnot influence the frequency of peristaltic contractions comparedto the control rate. The influence of yohimbine and efaroxan onthe inhibitory effects of moxonidine and UK 14304 is shown infigure 1. Yohimbine (3 µM) and efaroxan (0.01 and 1 µM) causedparallel rightward shifts to the concentration-response curvesof moxonidine and UK 14,304. The apparent pK_B valuesfor yohimbine against moxonidine, rilmenidine or UK 14,304 andfor efaroxan against moxonidine or UK 14,304 were summarized intable 1.

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Fig. 1. Effects of moxonidine (A) and UK 14,304 (B) at inhibiting the peristaltic reflex of the rat ileum. The peristaltic inhibitionby the agonists was expressed as a percentage of the contractionrate present before addition of the agonists. Tissues were pretreatedwithout antagonist ( $open circle$ ) or with yohimbine 3 µM ( $bullet$ ), efaroxan 0.01µM ( $black-triangle$ ), efaroxan 1 µM ( $black-down-triangle$ ) and EEDQ 3 µM ( $black-square$ ). Mean values withS.E.M. are shown from 4 to 5 rats.

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TABLE 1
pK_B values of the alpha-2 adrenoceptor antagonist yohimbine and I₁/alpha-2 receptor antagonist efaroxan against agonists

Influence of EEDQ on the inhibitory effect of moxonidine and UK 14,304. Pretreatment of rat ileum preparations with the irreversible alpha-2 adrenoceptor antagonist EEDQ (3 µM) did not influencethe frequency of peristaltic contractions compared to the control.EEDQ, however, almost entirely prevented the inhibitory activitiesof moxonidine and UK 14,304. The maximal inhibitions were <20%at the high concentrations up to 30 µM for moxonidine and 10 µMfor UK 14,304 (fig. 1).

The effect of the putative endogenous I receptor agonist agmatine. Agmatine (0.01-100 µM) did not significantly affect the rate of peristalsis. Pretreatment of tissues with the DAO inhibitoraminoguanidine (1 µM, 20 min) did not reveal any effect of agmatineon peristalsis. The frequencies of peristalsis in the presenceof 100 µM agmatine were 0.55 ± 0.03 (n = 4) and 0.57 ± 0.05 (n= 5) waves/min, respectively, without and with aminoguanidine.

Also, the potency of UK 14,304 for the inhibition of peristalsis (IC₅₀ = 4.1 nM), was not affected by the presence of 100µM agmatine and 1 µM aminoguanidine, IC₅₀ = 3.9 nM (95% CI, 2.4-6.4nM, n = 5, P > .05).

Fluid Transport

Absorption. Basal net fluid transport was an absorptive state. The values from the jejunum and ileum of rats infused i.a. and injectedi.v. with saline as a control were 192 ± 24 (n = 16) and 362 ±22 (n = 16) µl/g wet weight in 20 min, respectively.

Dose-dependent effect of moxonidine. Intravenous injection of moxonidine resulted in a dose-dependent increase in the rate of net fluid absorption from both jejunumand ileum (fig. 2). Moxonidine had no obvious effect on the basalrates of absorption from the jejunum or ileum at the two lowerdoses, 0.36 µmol/kg (0.1 mg/kg) and 1.08 µmol/kg (0.3 mg/kg),but significantly enhanced the fluid transport rate by 124 ± 21%(n = 6) in the jejunum and 45 ± 13% (n = 6) in the ileum at 3.6µmol/kg (1.0 mg/kg). Moxonidine also produced a biphasic effecton MAP consisting of a transient hypertension followed by prolongedhypotension. The depressor effect of moxonidine remained stableduring the 20-min period of intestinal perfusion. The MAP measuredat the midpoint of perfusions were 110 ± 2 (.36 µmol/kg, P < .001,n = 5), 99 ± 5 (1.08 µmol/kg, P < .001, n = 6) and 85 ± 4 (3.6µmol/kg, P < .001, n = 5) compared with the control of 130 ± 3mm Hg (n = 12).

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Fig. 2. Effects of i.v. injection of moxonidine on the rate of net absorption from the jejunum and ileum. Rats were injected i.v.with saline (open columns), moxonidine 0.36 µmol/kg (hatched columns),1.08 µmol/kg (cross-hatched columns) and 3.6 µmol/kg (filled columns).**, P < 0.01; ***, P < 0.001 vs. the individual control (Dunnett'st test). Values are mean ± S.E.M. of 5 to 16 rats.

Effects of moxonidine and UK 14,304 on the responses to yohimbine and efaroxan. Intravenous injection of the selective alpha-2 adrenoceptor antagonist yohimbine and I₁/alpha-2 receptor antagonist efaroxancaused a decrease in the rate of fluid absorbed from both thejejunum and ileum (table 2). Yohimbine at 10 µmol/kg (3.9 mg/kg)and efaroxan at 10 µmol/kg (2.5 mg/kg) reduced absorption to 17± 41 (n = 8) and 13 ± 63 (n = 5) µl/g in 20 min, respectively,in the jejunum, and 173 ± 31 and 131 ± 50 (n = 5) µl/g in 20 min,respectively, in the ileum.

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TABLE 2
Effects of the alpha-2 adrenoceptor antagonist yohimbine and I₁/alpha-2 receptor antagonist efaroxan on the proabsorptiveactions of moxonidine and UK 14,304

Pretreatment with yohimbine and efaroxan at doses of 10 µmol/kg i.v. each attenuated the proabsorptive effects of moxonidine3.6 µmol/kg and UK 14,304 1 µmol kg i.v. (table 2).

The effect of the putative endogenous I receptor agonist agmatine. Infusion of agmatine into the aortic arch via the left common carotid artery resulted in an infusion-dependent decrease inthe rate of net fluid absorption from both jejunum and ileum (fig.3). Agmatine at 0.1 µmol/min (0.02 mg/min, total dose of 2.1 mg/kg)had no effect on the fluid transport rates in both jejunum andileum (n = 5) compared to the controls, but at 0.3 µmol/min (0.07mg/min, total dose of 6.3 mg/kg) and 1.0 µmol/min (0.23 mg/min,total dose of 21.1 mg/kg), there were significant decreases influid transport rates to 79 ± 20 and 95 ± 20 (n = 5) µl/g in 20min, respectively, in the jejunum, and 232 ± 23 and 176 ± 54 (n= 5) µl/g in 20 min, respectively, in the ileum. No further reductionswere observed from both jejunum and ileum at higher infusion ratesof agmatine. Agmatine had no effect on MAP at all infusion ratesused.

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Fig. 3. Effects of i.a. infusions of agmatine on the rate of net absorption from the jejunum and ileum. Rats were administrated withsaline (i.a., open columns), agmatine 0.1 µmol/min (shaded columns),0.3 µmol/min (hatched columns), and 1 µmol/min (filled columns).*, P < 0.05; **, P < 0.01 vs. the individual control (Dunnett'st test). Values are mean ± S.E.M. of 5 to 16 rats.

Secretion Induced by VIP

Infusion of VIP (0.8 µg/min i.a.) starting 5 min before and continuing during the 20-min perfusion totally reversed watertransport from net absorption to secretion. The values were 265± 17 µl/g in 20 min secreted into the lumen of the jejunum and368 ± 33 µl/g in 20 min secreted by the ileum (n = 10 for bothregions, table 3).

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TABLE 3
Effects of the alpha-2 adrenoceptor antagonist yohimbine and I₁/alpha-2 receptor antagonist efaroxan on the antisecretoryactions of moxonidine and UK 14,304.
Secretion was induced by i.a. infusion of VIP at 0.8 µg/min.

Dose-dependent antisecretory effect of moxonidine. Intravenous injection of moxonidine caused a dose-related inhibition of the VIP-induced fluid secretion in both jejunum andileum (fig. 4). The effect of the highest dose of moxonidine extendedto complete reversal of the VIP-induced effect in the jejunum,but in the ileum, it only blocked the secretory component of theresponse to VIP.

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Fig. 4. Inhibition by moxonidine (i.v.) of VIP-induced secretion in the rat jejunum and ileum. The open columns indicate the controlvalues of fluid secretion in response to i.a. infusion of VIPat 0.8 µg/min. Hatched columns are responses of rats administratedwith moxonidine at 0.036 µmol/kg, cross-hatched columns at 0.36µmol/kg, and filled columns at 3.6 µmol/kg. ***, P < 0.01 vs.the individual control (Dunnett's t test). Values are mean ± S.E.M.of 4 to 10 rats.

Comparison of the antisecretory with the proabsorptive effect of moxonidine. Moxonidine (3.6 µmol/kg i.v.) enhanced basal absorption by 239 ± 41 µl/g in 20 min in the jejunum and by 164 ± 47 µl/g in20 min in the ileum (n = 6, for actual values see table 2). Inanimals infused with VIP, the same dose of moxonidine reversedsecretion by 426 ± 26 µl/g in 20 min in the jejunum and by 277± 11 (n = 4) in the ileum (for actual values see table 3). Theantisecretory effect of moxonidine was significantly greater thanthe proabsorptive effect in the jejunum (P < .01, Student's unpairedt test). Although not statistically significant, the antisecretoryeffect of moxonidine also appeared larger than the proabsorptiveeffect in the ileum (P = .09).

Effects of moxonidine and UK 14,304 on the responses to yohimbine and efaroxan. Yohimbine and efaroxan did not affect the values of VIP-induced secretion in either jejunum or ileum, when tested separatelyat doses of 10 µmol/kg (P > .05, n = 3). The results of agonist-antagonistinteraction experiments are shown in table 3, where, yohimbineand efaroxan significantly antagonized the inhibitory effect exertedby moxonidine (3.6 µmol/kg) and UK 14,304 (1 µmol/kg) on VIP-inducedsecretion in the jejunum and ileum (P < .001, n = 5 in both regions).The degree of antagonism of yohimbine and efaroxan was similaragainst moxonidine and UK 14304.

Effect of the putative endogenous I receptor agonist agmatine. The antisecretory activity of agmatine was tested at the low dose (0.1 µmol/min) because higher infusion rates decreased therate of absorption in the rat intestine, an action contrary tothat of moxonidine and UK 14,304. Infusion of agmatine, togetherwith VIP, starting 5 min before and continuing during the 20-minperfusion did not influence the rate of secretion induced by VIP.The values were $-$ 286 ± 53 µl/g in 20 min in the jejunum (n = 5)and $-$ 345 ± 58 µl/g in 20 min in the ileum (n = 5) vs. correspondingvalues of $-$ 265 ± 17 and $-$ 368 ± 33 µl/g in 20 min in animals infusedwith VIP alone (P > 0.05, student's unpaired t test).

	Discussion

Abstract Introduction Methods Results Discussion References

The I receptors are now generally recognized as a unique set of nonadrenergic, high-affinity binding sites for a number ofagents that also specifically bind to alpha-2 adrenoceptors (Regunathanand Reis, 1996). It has been suggested that I₁ receptors are importantin mediating the hypotensive actions of clonidine, moxonidineand rilmenidine and may regulate renal sodium and water excretion(see the introduction). However, the involvement of I₁ receptorsin cardiovascular and renal functions are not fully accepted.For example, the results of studies in conscious rats and rabbitsargued in favour of alpha-2 adrenoceptors as sites of mediatinghypotensive actions of clonidine, rilmenidine and moxonidine (Hiebleand Kolpak, 1993; Szabo et al., 1993; Urban et al., 1994, 1995).Also, experiments conducted in conscious dogs provided no supportfor a role of I receptors in regulation of renal function (Evansand Anderson, 1995).

The starting point for the present study was that there are reports showing moxonidine inhibits gastric acid secretion throughactivation of I₁ receptors (Carlisle et al., 1995; Glavin andSmyth, 1995). Also, agmatine is an endogenous ligand for alpha-2adrenoceptors and I receptors (Li et al., 1994) and is widelydistributed in rat organs, particularly in the stomach and smallintestine (Raasch et al., 1995). A series of experiments was designedto investigate whether agmatine and moxonidine could regulatefunctions of the intestine and, if so, determine the receptorsby which they might exert their effects. The effects of moxonidineon intestinal motility and fluid transport were compared withthose of the pure alpha-2 adrenoceptor agonist UK 14,304. It isreasonable to presume that if moxonidine and UK 14,304 acted throughdifferent receptors, then the profiles of their effects mightbe expected to differ. Moreover, it would also be expected thatif the effects of moxonidine were mediated by I receptors, theywould be relatively resistant to antagonism by the alpha-2 adrenoceptorantagonists yohimbine and EEDQ.

Peristalsis. It is well established that peripheral alpha-2 adrenoceptors mediate inhibition of small intestinal contraction by inhibitingacetylcholine release from enteric cholinergic nerves (Andrejaket al., 1980; Coupar and Liu, 1996; Doherty and Hancock, 1983;Wikberg, 1977). It has been shown recently that the alpha-2 adrenoceptorsin the rat ileum are the alpha-2D subtype, which when activatedby agonists results in inhibition of peristalsis (Liu and Coupar,1996). The present study showed that alpha-2 adrenoceptors, butnot I receptors, were responsible for moxonidine mediating inhibitionof intestinal motility. First, this was substantiated by comparingIC₅₀ and relative potency values of agonists used in the presentexperiments with those obtained in previous reports. The IC₅₀value of clonidine for inhibition of peristalsis was 2.8 nM (Liuand Coupar, 1996). This shows that the relative potencies forclonidine, moxonidine and rilmenidine at inhibiting the peristalticreflex are in accordance with their relative affinities at alpha-2adrenoceptor binding sites of the bovine ventrolateral medulla(1:12:52 vs. 1:19:47) but are quite different to their relativeaffinity at I₁- binding sites (vs. 1:2:6) (Ernsberger et al.,1993). Second, the affinity values (apparent pK_B values)of the selective alpha-2 adrenoceptor antagonist yohimbine againstmoxonidine, rilmenidine and UK 14,304 were the same, suggestingthat these three compounds acted at the same receptors. Third,the pK_B values of the I₁/alpha-2 antagonist efaroxanat the low (0.01 µM) and high (1 µM) concentration against moxonidine(7.66 and 7.86) and UK 14,304 (8.03 and 7.96) were consistent.These values are correspondent to the affinity of efaroxan atthe alpha-2 binding sites in bovine rostral ventrolateral medulla(pK_i = 7.72-8.22) but not at the I binding sites (pK_i = 9.82-9.96)(Haxhiu, et al., 1994). Fourth, the alkylating agent EEDQ almostabolished the inhibitory effect of both moxonidine and UK 14,304on peristalsis. EEDQ is a useful tool because it inactivates brainalpha-2 adrenoceptors in vivo and in vitro without influencingI receptors (Pineda et al., 1993; Ruiz-Ortega et al., 1995; Szaboet al., 1996). The final evidence discounting the presence offunctional I receptors in the control of peristalsis was obtainedfrom the series of experiments using the putative endogenous ligandagmatine. In these experiments, agmatine failed to mimic the effectof moxonidine and UK 14,304, as in the case of rat vas deferensand guinea pig ileum, which are tissues containing alpha-2 adrenoceptors(Pinthong et al., 1995). It was reported by Holt and Baker (1995)that agmatine was a substrate for DAO but not for monoamine oxidaseand the metabolism of agmatine by DAO was inhibited by aminoguanidine.Hence, administration of a DAO inhibitor may increase endogenousagmatine levels and lead to a detectable biological response.The potential effect of agmatine on peristalsis, however, wasnot revealed in the presence of aminoguanidine (1 µM). The possibilityof agmatine being an alpha-2 adrenoceptor antagonist has beenruled out because the potency of UK 14,304 in suppressing theperistaltic reflex was not affected by the presence of agmatine(100 µM).

Fluid transport. The influence of the I₁/alpha-2 agonist moxonidine and putative endogenous I receptor agonist agmatine on intestinal fluidtransport by the small intestine was investigated under basalconditions and during active secretion induced by intra-arterialinfusion of VIP. This part of the study also supplied no functionalrole for I receptors in mediating fluid transport.

Intravenous administration of moxonidine resulted in a dose-dependent increase in the rate of basal fluid absorption thatwas more pronounced in the jejunum than ileum. This effect iscongruent with the previously reported effects of noradrenalineand UK 14,304 (Liu and Coupar, 1997

). The proabsorptive effectof the highest dose of moxonidine (3.6 µmol/kg i.v) was blockedby yohimbine and efaroxan (both 10 µmol/kg i.v) to the same extentas that of UK 14,304 (1 µmol/kg i.v). If moxonidine acted throughI receptors, then yohimbine would be anticipated to antagonizethe effect of moxonidine to a much lesser extent than that ofthe alpha-2 adrenoceptor agonist UK 14,304, whereas efaroxan wouldbe more potent against moxonidine than against UK 14,304.

Recently, we reported that the small intestinal mucosa is under tonic proabsorptive influence from sympathetic nerves. Partof the evidence in support of this conclusion was that alpha-2adrenoceptor antagonists such as yohimbine and rauwolscine inducedantiabsorptive effects (Liu and Coupar, 1997

). In the currentstudy, efaroxan at 10 µmol/kg i.v. also induced reductions influid absorption from both the jejunum and ileum. Hence, efaroxanseems to act as an alpha-2 adrenoceptor antagonist under the conditionsof the present experiments.

The antisecretory effect of moxonidine was assessed by i.a. infusion of the directly acting secretagogue VIP. We reportedpreviously that the VIP-induced secretion was markedly reducedby UK 14,304, by an action mediated through an alpha-2D (or alpha-2A-like)adrenoceptor subtype (Liu and Coupar, 1997

). The present studyalso showed that moxonidine dose-dependently reversed the secretioninduced by VIP. The present results also showed that the antisecretoryeffect of moxonidine was larger than the proabsorptive effect.This might imply that stimulation of absorption and inhibitionof secretion are mediated at different levels along the crypt-villusaxis as has been proposed to explain the greater antisecretoryeffect compared with proabsorptive effect of UK 14,304 (Liu andCoupar, 1997

). Absorption and secretion are believed to be independentprocesses and it has been suggested that the crypt cells regulatesecretion while the villus cells are responsible for absorption(Welsh et al., 1982

). The results were in line with the findingby Paris et al. (1990)

that in rat jejunum epithelial cells therewas a greater density of alpha-2 adrenoceptors in the crypt thanvillus enterocytes. The present study also showed that the antisecretoryeffect of moxonidine was blocked by both yohimbine and efaroxan,and the degree of antagonism to moxonidine did not differ fromthat of UK 14,304.

The i.a. infusion of agmatine, in contrast to moxonidine and UK 14304, decreased the rate of basal fluid absorption in a dose-relatedmanner from both jejunum and ileum, the effect being equivalentto that produced by alpha-2 adrenoceptor antagonists. A low doseof agmatine (0.1 µmol/min), which did not show significant influenceon basal absorption, failed to reverse secretion induced by VIPin either region.

If agmatine is the endogenous agonist for I receptors and I receptors are involved in regulating fluid transport, then itcould be expected that the effect of agmatine and that of thespecific agonist moxonidine would be similar. The opposite effectsof agmatine and moxonidine are suggestive of different mechanismsof action for the two compounds. Because agmatine did not behaveas an alpha-2 adrenoceptor antagonist in the peristalsis experiments,the reason for its ability to decrease fluid absorption remainsunexplained in this study.

Discrepancies have been reported concerning the effects of agmatine as an endogenous agonist on I receptors. For instance,agmatine has been reported to activate I receptors mediating eitherinhibition of noradrenaline release in rabbit aorta (Molderingsand Gothert, 1995

) or increase of catecholamines release fromadrenal chromaffin cells (Li et al., 1994

). In contrast, it hasbeen suggested that agmatine acts as an inverse agonist ratherthan a true agonist at I receptors because it increased rat gastricsecretion and worsened gastric mucosal injury, effects oppositeto those of moxonidine (Glavin et al., 1995

; Glavin & Smyth, 1995

).It is of interest that these opposite effects noted for moxonidineand agmatine parallel those in the present study. Agmatine hasalso been found to lack activity at I sites in mediating insulinsecretion (Berdeu, et al., 1996

In conclusion, this study provides no support for a functional role of I receptors in regulating motility and fluid transportin the rat intestine. The effects of moxonidine on both functionscan be entirely explained on the basis of interactions with alpha-2adrenoceptors. The pharmacological characteristics of agmatineat alpha-2 adrenoceptors is not clear because its actions canbe attributed to neither agonism nor antagonism.

	Acknowledgments

We wish to thank Beiersdorf-Lilly and Servier Laboratories for their generous gifts of research compounds.

	Footnotes

Accepted for publication August 25, 1997.

Received for publication March 18, 1997.

Send reprint requests to: Dr. Ian M. Coupar, Department of Pharmaceutical Biology and Pharmacology, Victorian College of Pharmacy, Monash University, Parkville, Victoria, 3052, Australia. E-mail: ian.coupar{at}vcp.monash.edu.au

	Abbreviations

DAO, diamine oxidase; EEDQ, N-ethoxycarbonyl-2-ethoxy-1,2-dihydroquinoline; I, imidazoline; MAP, mean arterial pressure; UK 14, 304, 5-bromo-6-(2-imidazolin-2-yl-amino)-quinoxaline; VIP, vasoactive intestinal peptide; i.v., intravenous; i.a., intra-arterial; DMSO, dimethylsulfoxide.

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