Interaction Between Histamine H3 Receptors and Other Prejunctional Receptor Systems in the Isolated Guinea Pig Duodenum,

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Vol. 281, Issue 1, 393-399, 1997

Interaction Between Histamine H₃ Receptors and Other Prejunctional Receptor Systems in the Isolated Guinea Pig Duodenum¹^,²

Enzo Poli, Cristina Pozzoli and Giulio Bertaccini

Institute of Pharmacology, School of Medicine, University of Parma, Parma, Italy

	Abstract

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The hypothesis that prejunctional histamine H₃ receptors and alpha-2 adrenoceptors interact with each other was assessed onthe cholinergic transmission of the guinea pig duodenum. Specificagonists acting at histamine H₃ receptors, alpha-2 adrenoceptorsand adenosine A₁ receptors, (R)- $alpha$ -methylhistamine (1 nM-1 µM),UK 14,304 (1 nM-1 µM) and N⁶-cyclopentyladenosine (0.1 nM-0.1 µM), respectively, inhibitedmuscle contractions evoked by electrical stimulation, the effectbeing antagonized by specific receptor blockers, thioperamideand clobenpropit (H₃ receptors), idazoxan and yohimbine alpha-2adrenoceptors) and 8-cyclopentyl-1,3-dimethylxanthine (A₁ receptors).The simultaneous activation of H₃ receptors and alpha-2 adrenoceptors,using EC₅₀ values of the specific agonists (UK 14,304: 30 nM;(R)- $alpha$ -methylhistamine: 20 nM), produced a combined effect thatdid not differ from the sum of the individual effects, a resultthat excluded the occurrence of interactions between these receptors.Conversely, the inhibition evoked by the coadministration of N⁶-cyclopentyladenosine (EC₅₀: 2.5 nm) and (R)- $alpha$ -methylhistamineor of N⁶-cyclopentyladenosine and UK 14,304 was significantly lower thanthe sum of the individual effects, which suggests that the correspondingprejunctional receptors interact with each other. No interactioncould be detected when threshold concentrations (EC_10-15)of the different agonists were simultaneously applied. These datashow a negative cooperativity between H₃ and A₁ receptors andbetween A₁ and alpha-2 receptors. Conversely, no evidence of positivecooperativity emerged, even when the different agonists were appliedat low or maximum concentrations. The lack of cross-reactivitybetween the respective agonists excludes an interaction at therecognition sites of the receptor moyeties. Therefore, these phenomenaare more likely to reflect interplays between second messengersor effectors involved in modulating the ACh release.

	Introduction

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Prejunctional (presynaptic) histamine H₃ receptors and alpha-2 adrenoceptors, localized on nerve endings of the peripheralnervous system, negatively modulate the release of different neuromediators,including ACh from the myenteric plexus (Trzeciakowski, 1987;Poli et al., 1991; Coruzzi et al., 1991) and NE from cardiac nervesor sympathetic neurons (Lipscombe et al., 1989; Malinowska andSchlicker, 1993; Endou et al., 1994). The activation of such receptorsystems limits both the action potential upstroke and the availabilityof free Ca⁺⁺ at the axoplasmic level, possibly by reducing Ca⁺⁺ transport through the neuronal-type Ca⁺⁺ channels (Endou et al., 1994; Poli et al., 1994; Schlicker etal., 1994) or by activating ATP-sensitive K⁺ channels (Ohkubo and Shibata, 1995). Irrespective of the mechanism,the activation of H₃ and alpha-2 receptors results in an attenuationof the exocytotic neurotransmitter release and, consequently,of the postsynaptic responses associated with nerve stimulation.

It has recently been demonstrated that histamine H₃ receptors and alpha-2 adrenoceptors, occurring at the noradrenergic nerveendings of the brain cortex, interact with each other in the modulationof NE release, showing a negative cooperativity when simultaneouslyactivated by selective agonists (Schlicker et al., 1992). Moreover,the effect induced by an H₃ receptor agonist is potentiated whenthe alpha-2 adrenoceptor is simultaneously blocked, which suggeststhat the negative cooperativity also occurs between an exogenouslyadded H₃ receptor agonist and endogenous NE (Schlicker et al.,1992).

We have recently employed a functional test to study peripheral histamine H₃ receptors and alpha-2 adrenoceptors in the gut(Coruzzi et al., 1991; Poli et al., 1993; Poli et al., 1994).These receptors negatively modulate the cholinergic nerve activityin the isolated, electrically driven guinea pig duodenum withoutaffecting muscle contractions evoked by exogenous ACh (Coruzziet al., 1991). It was also shown that the activation of H₃ receptorsand alpha-2 adrenoceptors, but not of adenosine A₁ receptors,results in a Ca⁺⁺-dependent inhibition of neurogenic responses (Poli et al., 1994).These finding suggested a postreceptor mechanism of prejunctionalinhibition coupled with H₃ and alpha-2 receptors, possibly consistentwith a restriction of Ca⁺⁺ fluxes through neuronal-type channels (Poli et al., 1994).

Thus the purposes of the present study were 1) to test the hypothesis that alpha-2 adrenoceptors and H₃ receptors interactin modulating the activity of intestinal cholinergic nerves and2) to demonstrate possible interactions between the former tworeceptors and adenosine A₁ receptors.

	Materials and Methods

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The inhibitory effects mediated by histamine H₃ receptors and other prejunctional receptor systems on the cholinergic transmissionwere studied, using the isolated guinea pig duodenum, accordingto a previously described technique (Coruzzi et al., 1991; Poliet al., 1993; Poli et al., 1994).

Animal procedure. Male albino guinea pigs (300-400 g) were killed by cervical dislocation. The whole duodenum was rapidly removed and placedinto a dissection disc containing oxygenated (95% O₂ and 5% CO₂)Krebs-Henseleit solution of the following composition (mM): NaCl113; KCl 4.7; CaCl₂ · 2H₂O 2.5; KH₂PO₄ 1.2; MgSO₄ · 7H₂O 1.2;NaHCO₃ 25 and dextrose 11.5 (pH 7.4-7.5).

Segments of the whole duodenum (~20 mm in length) were tied at both ends, set up, at 37°C, into 10-ml organ chambers containingKrebs-Henseleit solution of the composition described above (pH7.4 ± 0.1) and suspended under a passive load of 0.7 g, whichproduced a constant stretch throughout the entire experiment.Longitudinal contractions were recorded isotonically on a pen-writingpolygraph (Basile, Milan) and measured as a change in length ofthe preparations.

EFS. A pair of coaxial platinum electrodes were positioned 10 mm apart the longitudinal axis of the preparations. Single square-wavepulses (0.5 msec in duration, 50 V at 150-200 mA intensity) weredelivered to the tissues every 10 sec. For each experiment, theintensity was adjusted to the level that gave 70% to 80% of themaximum tissue response to EFS. In these conditions, tetrodotoxin-and atropine-sensitive twitch responses were obtained (Coruzziet al., 1991), a result that suggests the involvement of ACh releasedfrom cholinergic neurons of the myenteric plexus.

Evaluation of drug effects. Agonists were cumulatively administered by addition of logarithmically increasing concentrations to the bath fluid, or bysingle administration of EC₅₀ concentrations (those that gave50% of the absolute maximum effect obtainable with the agonist,irrespective of its efficacy). When MHA was used, the experimentswere carried out in the presence of H₁ and H₂ receptor blockers(pyrilamine and famotidine 1 µM) to prevent the activation ofH₁ and H₂ receptors by concentrations of the compound higher than10 µM (Arrang et al., 1987; Endou et al., 1994). To avoid possibledesensitization phenomena at the level of H₃ receptors (Coruzziet al., 1991), a single concentration-response curve to MHA wascarried out in the same preparation. In the case of clonidine,UK 14,304, adenosine and CPA, it was possible to construct severalconcentration-response curves in the same preparation, providedthat 60 to 90 min elapsed between drug administrations.

From each animal, 3 to 4 segments of the duodenum were used, one for control experiments and the others for experiments withdifferent nutrient fluids or specific pharmacological tools (seebelow). Pilot experiments were carried out to exclude macroscopicdifferences in the reactivity of the different portions of theintestinal segments to EFS and in their sensitivity to drugs.

Evaluation of receptor interactions Protocol I. The interaction between two different prejunctional receptors was evaluated on the basis of the effects elicited by the respectiveagonists, administered alone or in combination. Preparations werestimulated as described above. Then ED₅₀s of two agonists (agonistA and agonist B) were tested separately, and the respective effects(effect A and effect B) were measured. After washout and completerecovery of contraction to EFS (60-90 min), the agonists werecoadministered, and we obtained the combined effect (effect [A+ B]). Then "effect [A + B]" was compared with the algebraic sum"effect A + effect B," which represents the expected effect foradditivity. Significant deviations from additivity, determinedby statistical comparison (see below), were taken as evidenceof cooperativity between receptors.

The possible interaction between prejunctional receptors was also investigated at concentrations of agonists near to the thresholdvalue. Concentrations that gave 10% to 15% of the maximum effectof each agonist were extrapolated from the respective concentration-responsecurves and applied as we have described for EC₅₀s.

Protocol II. Other kinds of experiments were performed to test whether previous activation of a prejunctional receptor could modify theeffects evoked by activation of a second receptor. In these experiments,the current strength of the electrical pulses was calibrated ata level (~150 mA) that gave 55% to 60% of the maximum tissue responsivityto EFS. Typically, we constructed the concentration-response curveof an agonist and then left the tissue to recover after washoutbefore applying a single concentration of a second agonist. Oncethe maximum effect was reached, the current strength was raised(usually from 150 to 270 mA) to restore a predrug level of twitchresponse, after the application of the second agonist, and thenthe concentration-response curve of the former agonist was reconstructedin the presence of the second agonist (see fig. 3 for more details).The adjustment of the current strength was made to compensatefor inhibition of the electrically evoked response by one of thetwo interacting agonists and hence to reproduce a predrug levelof neurogenic contraction. This procedure was designed to excludethe possibility of experimental artifacts due to the decreaseof neurogenic response and to make it possible to evaluate a truereceptor interaction (Schlicker et al., 1992).

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Fig. 3. Typical experiment showing the effects of UK 14,304 before and after near-maximum concentrations of MHA and reversal of inhibitoryeffect of MHA by raising current strength (from 150 to 270 mA).Concentrations of drugs are expressed in nanomoles per liter.Vertical calibration represents the isotonic shortening of duodenalmuscle in response to EFS. x: stop stimulation and washout.

Statistical analysis. Results are given as means ± S.E.M. Comparisons between two sets of data were made by Student's t test for paired or unpaireddata. When more than two groups were compared, the analysis ofvariance was used. In all these tests, P < .05 was consideredstatistically significant. The potency of the different agonistson EFS-induced contractions was expressed by the EC₅₀ value (seeabove). Confidence limits 95% (CL₉₅) of the geometric mean ofthe individual EC₅₀ values were then provided.

When the affinity of receptor antagonists was measured, pA₂ values were calculated according to Schild's method (Kenakin,1987

). Arithmetic means ± CL₉₅ of these values were provided.

Drugs. The following drugs and chemicals were used in this study: yohimbine hydrochloride, pyrilamine maleate (mepyramine), atropinesulfate, tetrodotoxin (citrate buffer) and adenosine (base) (SigmaChemical Co., St. Louis, MO), THEO (Merck, Darmstadt, FRG) andCPA, UK 14,304 (5-bromo-N-(4,5-dihydro-1H-imidazol-2-y1)-6-quinoxalinamine,also known as bromoxidine), idazoxan hydrochloride, 8-cyclopentyl-1,3-dipropylxantine(free base) and thioperamide maleate (RBI, Natick, MA). Famotidine(free base) was a gift of Sigma-Tau, Roma, Italy; (R)- $alpha$ -methylhistaminedihydrochloride was generously provided by Dr. J. C. Schwartz(Centre Paul Broca de l'INSERM, Paris, France); and the H₃ receptorligands immepip dihydrobromide (VUF 4708) and clobenpropit dihydrobromide(VUF 9153) were synthesized by Prof. H. Timmermann (Vrije Universiteit,Amsterdam, the Netherlands).

	Results

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Effects mediated by prejunctional H₃, alpha-2 and A₁ receptors. The activation of H₃ alpha-2 and A₁ receptors by a series of specific or nonspecific agonists induced a concentration-dependentinhibition of EFS-evoked contractions of the guinea pig duodenum.The efficacy of the H₃ receptor agonist MHA (fig. 1 and table1) was lower (~60% of maximum inhibition of EFS-evoked twitchresponses), compared with the alpha-2 agonist UK 14,304 or withthe A₁ agonist CPA, both of which compounds produced an almostcomplete damping of the cholinergic response. Also, the new agonistfor H₃ receptors, immepip (Barnes et al., 1993; Vollinga et al.,1994), incompletely suppressed the cholinergic response. Conversely,a complete inhibition was attained with the endogenous A₁/A₂ receptoragonist adenosine, and the alpha-2 agonist clonidine showed apartial agonistic activity, compared with UK 14,304. The potencyand the efficacy of these agonists are listed in table 1. Noneof these compounds modified the contractile effect of exogenousACh, even at the maximum inhibitory concentrations affecting EFS-evokedresponses. An example is shown in figure 1, which considers onlythe effect of CPA.

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Fig. 1. Left plot: Inhibitory effect of CPA, UK 14,304, MHA and immepip on the amplitude of twitch responses of the isolated guineapig duodenum. Data are the mean ± S.E.M. of 5 to 8 experiments.On abscissa: molar concentration of drugs; on ordinate: percentof the predrug contractions evoked by EFS, taken as 100%. Rightpanel: Original recordings showing the effects of CPA on the cholinergicresponses evoked by EFS (upper) and by exogenous ACh. Verticalcalibration represents the isotonic shortening of duodenal musclein response to EFS. Concentrations of drugs are expressed in nanomolesper liter. x: stop stimulation and washout; w: washout.

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TABLE 1
EC₅₀ values and efficacy of different prejunctionally acting receptor agonists for their inhibitory activity on EFS-evokedmuscle contractions

Interactions among H₃, alpha-2 and A₁ receptors. From the concentration-response curves of figure 1, we extrapolated the concentrations of prejunctional receptor agonistsgiving 10% to 15% of the respective maximum effects, and the followingvalues were chosen for MHA, CPA and UK 14,304, respectively: 3nM, 0.5 nM and 3 nM.

As shown in figure 2A, the combined effect of all these agonists did not significantly differ from the algebraic sum of theindividual effects, a result that suggests a lack of interactionat these levels of concentration.

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Fig. 2. Inhibitory effect of CPA (grid columns), UK 14,304 (UK) (white columns) and MHA (horizontally barred column) obtained by singleadministration or by coadministration (black columns) of two ofthese agonists. A) The following concentrations, which representthe approximate EC_10-15 of each agonist, were used: MHA:3 nM; UK 14,304: 3 nM; CPA: 0.5 nM. B) The EC₅₀ value of eachdrug was used (see table 1). Hatched columns represent the inhibitionvalue expected for additivity of the individual effects. Dataare the mean ± S.E.M. of 6 to 9 experiments. On ordinate: percentof response to EFS, considering the predrug level to be 100%.* indicates significant difference (P < .05) from the value expectedfor additivity.

When the H₃ agonist MHA and the alpha-2 agonist UK 14,304 were coadministered at concentrations corresponding to their respectiveEC₅₀ values (see table 1), the inhibitory activity was equivalentto the sum of the inhibitions exerted by the individual drugs(fig. 2B). By contrast, when either UK 14,304 or MHA was coadministeredwith CPA, the inhibition obtained was significantly lower (P <.05) than the sum of the inhibitions produced by the individualdrugs (fig. 2B).

When immepip was tested in place of MHA, we still observed an additive effect when it was combined with UK 14,304 and a reducedeffect when it was combined with CPA (not shown).

We further investigated the cooperativity among receptors by using concentrations of agonists higher than the EC₅₀ values.Near-maximum concentrations of agonists could not be applied simultaneously,the expected inhibition of EFS-induced responses being higherthan 100%. Therefore, the interactions among H₃, alpha-2 and A₁receptors were measured in conditions where the current strengthwas raised, to reproduce a predrug level of muscle response, afterthe application of one agonist (see "Materials and Methods").The protocol represented in figure 3, which considers only themodification of the effect of UK 14,304 by MHA, was used. Theapplication of MHA (0.3 µM) did not modify the concentration-responsecurve of UK 14,304 or of CPA (figs. 3 and 4). CPA (3 nM), in turn,significantly reduced the effects of MHA but not those of UK 14,304.By contrast, UK 14,304 (30 nM) did not cause any change in theeffects of MHA but significantly reduced the effects of CPA (fig.4).

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Fig. 4. Inhibitory effect of CPA, UK 14,304 and MHA, first given alone and subsequently administered in the presence of each of theother two agonists. Control curves (Co) were constructed to low-currentstrength (typically 150 mA); the combined effect was tested afterreversal of inhibition by raising the current strength at 270mA, according to the scheme represented in figure 3. Data arethe mean ± S.E.M. of 5 to 8 experiments. On abscissa: molar concentrationof drugs; on ordinate: percent of the predrug contractions evokedby EFS. * indicates significant difference (P < .05) from thecorresponding control value.

Maximum or supramaximum concentrations of UK 14,304 or CPA could not be applied in these experiments, because we obtaineda complete damping of the cholinergic response that could notbe restored by raising the current strength. Only MHA could betested up to 3 to 10 µM, but even at these concentrations, theeffect of UK 14,304 was not modified (not shown).

Effect of specific blockers on the agonist-induced prejunctional effects. To ascertain whether the cooperativity between CPA and UK 14,304 or MHA reflects cross-reactions at the recognition sitesof receptors, we tested each of these agonists in the presenceof the corresponding receptor blockers and in the presence ofblockers acting at the other receptors.

The effects of MHA, of UK 14,304 and of CPA were antagonized only by the corresponding blockers: THIO (H₃), idazoxan (alpha-2)and DPCPX (A₁). In all cases, the antagonism was surmountable(data not shown). In a result similar to its antagonism by THIO(pA₂ value ± CL₉₅: 7.99 ± 0.69, data from Coruzzi et al., 1991

),the effect of MHA was antagonized by the new H₃ receptor blockerCLO (Barnes et al., 1993

; Vollinga et al., 1994

). CLO exertedan insurmountable antagonism. This latter compound completelyabolished the effect of maximum concentrations of MHA at 10 nMwithout influencing the effect of alpha-2 or A₁ agonists (datanot shown).

Effects of the H₃, alpha-2 and A₁ receptor antagonists on the EFS-evoked cholinergic response. The possible role of endogenous ligands in modulation of the ACh release, as a factor in the cooperativity between A₁ andalpha-2 or H₃ receptors, was tested with specific blockers forprejunctional receptors on the contractile response to EFS.

The amplitude of EFS-evoked twitch responses was slightly but significantly enhanced (P < .05) by the H₃ receptor antagonistsTHIO and CLO (fig. 5A) at concentrations known to block the MHA-inducedeffect (see above). The amplitude of the cholinergic responsesafter THIO and CLO, at the maximum facilitatory concentrations(1 and 0.01 µM, respectively), was not enhanced by further cross-administrationof CLO and THIO, respectively (fig. 5A).

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Fig. 5. Effect of THIO, CLO, DPCPX, THEO, IDAZ and yohimbine (YO) on the amplitude of muscle contractions evoked by EFS. Data representthe mean ± S.E.M. of 5 to 12 experiments. On ordinate: percentof the cholinergic response to EFS, considering the predrug levelto be 100%. The concentrations of drugs are expressed in micromolesper liter. n.s.: not statistically significant; *: P < .05, comparedwith the respective control (Co) value.

Conversely, the A₁ receptor antagonist DPCPX, but not the nonselective antagonist THEO, strongly enhanced the amplitude ofthe cholinergic responses (fig. 5B). Furthermore, the facilitatoryeffect of DPCPX was not significantly affected by THEO, nor didDPCPX induce any change in the effect of THEO (fig. 5B).

The alpha-2 adrenoceptor antagonists idazoxan and yohimbine, in turn, did not produce any modification of the cholinergicresponse up to concentrations of 1 µM (fig. 5C).

	Discussion

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The use of specific agonists to activate H₃ receptors, alpha-2 adrenoceptors and A₁ receptors reveals the occurrence of negativecooperativity between some, but not all, of the presynaptic heteroreceptorsthat control ACh release from the intrinsic excitatory nervesof the isolated guinea pig duodenum. In fact, alpha-2 adrenoceptorsand H₃ receptors do not interact with each other, whereas adenosineA₁ receptors interact with both of them. This is suggested bythe additivity of the inhibitory actions of the specific alpha-2adrenoceptor agonist UK 14,304 and the specific H₃ receptor agonistMHA, and by a reduced inhibition when both agonists were combinedwith the A₁ receptor agonist CPA. These interactions occur whenagonists are applied at EC₅₀ or more; at lower concentrations(near to threshold), no evidence of cooperativity between receptorsemerged.

Such results at least in part contrast with the view that two (or more) inhibitory presynaptic (prejunctional) receptor systems,occurring at the same nerve endings, display a negative cooperativity.Although the exact molecular mechanism(s) is (are) lacking, examplesof such cooperativity can be found between receptors in centralas well as in peripheral tissues, including dopamine D₂ receptorsand alpha-2 adrenoceptors in perivascular nerves (Friedman andDuckles, 1995) and adenosine A₁ and kappa opioid receptors incortical nerve endings (Limberger et al., 1988).

Schlicker et al. (1992) found a negative cooperativity between presynaptic alpha-2 adrenoceptors and H₃ receptors that controlthe release of ³H-NE from adrenergic nerves of the brain cortex. Whether suchdiscrepancy with our results is a consequence of the differentexperimental conditions (contraction vs. release experiments)cannot be easily established. It is possible that prejunctional/presynapticreceptor interactions preferentially involve the respective autoreceptorand a heteroreceptor, rather than two heteroreceptors.

One factor that could contribute significantly to this difference is the state of activation of the interacting receptors,because it has been shown that the block of activated, but notof nonactivated, alpha-2 receptors potentiates (Schlicker et al.,1989) or unmasks (Schlicker et al., 1990) the inhibitory effectmediated by H₃ receptors on the release of NE from rat and pigtissues. Histamine and purines (either ATP or its metabolite adenosine),together with NE, play a role as inhibitory neuromediators inthe gut (for reviews see Burks, 1994; Wood, 1994). Therefore,these substances, when released from noncholinergic nerves ortissue stores, could influence the activity of exogenously appliedagonists at the respective receptor.

To investigate this possibility, we performed experiments with antagonists acting at H₃, alpha-2 and A₁ receptors in an attemptto determine whether such receptors are activated by the correspondingendogenously released agonists. THIO and CLO (H₃) and DPCPX (A₁),have a facilitatory effect on the neurogenic contractions, whereasthe nonspecific A₁ receptor blocker THEO (at nonspasmolytic concentrations)did not produce any facilitation. The effect of each H₃ antagonistis apparently consistent with H₃ receptor blockade, being absentin preparations pretreated with the other H₃ antagonist. Theseresults, together with the finding that the nonspecific H₃ blockerimpromidine may enhance the release of ACh (Poli et al., 1991),suggest that H₃ receptors are activated by endogenous histamine,released in response to EFS. The use of other specific antagonistsfor A₁ receptors will clarify whether this system is really activatedby endogenous purines or whether DPCPX enhances the cholinergicresponse through a nonspecific mechanism.

On the other hand, the observed negative cooperativity cannot be simply a consequence of interactions with endogenous ligands,because NE does not appear to be released from enteric nervesin response to EFS (perhaps the frequency of stimuli applied tothe preparations is too low to activate sympathetic nerve endings),but alpha-2 receptors, much like H₃ receptors, do interact withA₁ receptors.

Schlicker et al., (1992), but not others (Imamura et al., 1994) found a potentiation of the inhibitory activity mediated byH₃ receptors when an alpha-2 adrenoceptor antagonist was addedsimultaneously. In our conditions, specific antagonists for alpha-2and H₃ (and also A₁) receptors, modify only the effect mediatedby the corresponding receptor, while leaving unaffected the effectsmediated by other receptors. Therefore, H₃ receptors and alpha-2adrenoceptors occurring at the cholinergic endings of the myentericplexus represent separate entities, which modulate in the sameway, and probably with a similar (but not necessarily identical)molecular mechanism, the release of ACh from excitatory nervesof the gut (Poli et al., 1994).

On the basis of these results, we conclude that the negative cooperativity between A₁ receptors and H₃ or alpha-2 receptorsis a consequence of interactions taking place at the postreceptorlevel. Such cooperativity occurs when agonists are coadministered,or when one kind of receptor is stimulated, before the administrationof the agonist for the second receptor. Furthermore, we observedthat the interaction is of the nonreciprocal kind. In fact, theactivation of A₁ receptors, which apparently interact with bothalpha-2 and H₃ receptors, blunts only the effects elicited bythe activation of H₃ receptors, whereas alpha-2 receptor activation,in turn, limits those of A₁ receptors. It is evident from thesefindings that the mechanism underlying the interaction betweenthese prejunctional receptor systems differs with the differentreceptors (and, consequently, with the postreceptor events) involved.

In conclusion, we provide evidence of negative cooperativity between some, but not all, heteroreceptors involved in the controlof ACh release from the myenteric plexus, and we found no evidenceof positive cooperativity. These interactions occur when receptorsare activated by high concentrations (EC₅₀ or more) of exogenousagonists and seem to be due to cross-talk at the postreceptorlevel. Whatever the mechanism, these interactions could representa limiting factor in the pathophysiologic modulation of ACh releaseby substances occurring in the intestinal neuroimmune system,when simultaneously mobilized by neurohumoral and/or immunologicalstimuli (Wood, 1994).

	Acknowledgments

We are indebted to Mrs. S. Spaggiari for her skillful technical assistance in the experiments.

	Footnotes

Accepted for publication December 16, 1996.

Received for publication March 27, 1996.

¹ This work was supported by European Community (BIOMED 1 GRANT) and by C.N.R. (Rome-Italy).

² A preliminary version of these findings was presented at the meeting "Receptor Classification" held in Verona (Italy) in 1995and was published in the Abstract Book of the Symposium (p. 25).

Send reprint requests to: Giulio Bertaccini, Institute of Pharmacology, School of Medicine, University of Parma, Via Gramsci 14, I-43100 Parma, Italy.

	Abbreviations

CLO, clobenpropit; CPA, N⁶-cyclopentyladenosine; DPCPX, 8-cyclopentyl-1,3-dimethylxanthine; EFS, electrical field stimulation; IDAZ, idazoxan; MHA, (R)- $alpha$ -methylhistamine; NE, norepinephrine; THEO, theophylline; THIO, thioperamide.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

Arrang, J. M., Garbarg, M., Lancelot, J. C., Lecomte, J. M., Pollard, H., Robba, M., Schunack, W. and Schwartz, J. C.: Highly potent and selective ligands for histamine H₃-receptors. Nature (Lond.) 327: 117-123, 1987[Medline].
Barnes, J. C., Brown, J. D., Clarke, N. P., Chapman, J., Evans, D. J. and O'Shaughnessy, C. T.: Pharmacological activity of VUF 9153, an isothiourea histamine H₃ receptor antagonist. Eur. J. Pharmacol. 250: 147-152, 1993[Medline].
Burks, T. F.: Neurotransmission and neurotransmitters. In Physiology of the Gastrointestinal Tract (3rd ed.) ed. by Leonard R. Johnson, pp. 211-242, Raven Press, New York, 1994.
Coruzzi, G., Poli, E. and Bertaccini, G.: Histamine receptors in isolated guinea pig duodenal muscle: H₃ receptors inhibit cholinergic neurotransmission. J. Pharmacol. Exp. Ther. 258: 325-331, 1991[Abstract/Free Full Text].
Endou, M., Poli, E. and Levi, R.: Histamine H₃-receptor signaling in the heart: Possible involvement of Gi/Go proteins and N-Type Ca²⁺ channels. J. Pharmacol. Exp. Ther. 269: 221-229, 1994[Abstract/Free Full Text].
Friedman, D. J. and Duckles, S. P.: Prejunctional interaction of $alpha$ ₂-adrenoceptors and D₂ dopamine receptors on perivascular sympathetic nerves. J. Auton. Pharmacol. 15: 27-35, 1995[Medline].
Imamura, M., Poli, E., Omonyi, A. T. and Levi, R.: Unmasking of activated histamine H₃-receptors in myocardial ischemia: Their role as regulators of exocytotic norepinephrine release. J. Pharmacol. Exp. Ther. 271: 1259-1266, 1994[Abstract/Free Full Text].
Kenakin, T. P.: Drug antagonism. In Pharmacologic Analysis of Drug-Receptor Interaction., ed. by T. P. Kenakin, pp. 205-244, Raven Press, New York, 1987.
Limberger, N., Spath, L. and Starke, K.: Presynaptic $alpha$ ₂-adrenoceptor, opioid $kappa$ -receptor and adenosine A₁-receptor interactions on noradrenaline release in rabbit brain cortex. Naunyn-Schmiedeberg's Arch. Pharmacol. 338: 53-61, 1988[Medline].
Lipscombe, D., Kongsamut, S. and Tsien, R. W.: $alpha$ ₂-Adrenergic inhibition of sympathetic neurotransmitter release mediated by modulation of N-type calcium-channel gating. Nature 340: 639-642, 1989[Medline].
Malinowska, B. and Schlicker, E.: Identification of endothelial H₁, vascular H₂ and cardiac presynaptic H₃ receptors in the pithed rat. Naunyn-Schmiedeberg's Arch. Pharmacol. 347: 55-60, 1993[Medline].
Ohkubo, T. and Shibata, M.: ATP-sensitive K⁺ channels mediate regulation of substance P release via the prejunctional histamine H₃-receptor. Eur. J. Pharmacol. 277: 45-49, 1995[Medline].
Poli, E., Coruzzi, G. and Bertaccini, G.: Histamine H₃-receptors regulate acetylcholine release from the guinea pig ileum myenteric plexus. Life Sci. 48: PL63-PL68, 1991[Medline].
Poli, E., Pozzoli, C., Coruzzi, G. and Bertaccini, G.: Histamine H₃-receptor-induced inhibition of duodenal cholinergic transmission is independent of intracellular cyclic AMP and GMP. Gen. Pharmacol. 24: 1273-1278, 1993[Medline].
Poli, E., Pozzoli, C., Coruzzi, G. and Bertaccini, G.: Signal transducing mechanism coupled to histamine H₃ receptors and alpha-2 adrenoceptors in the guinea pig duodenum: Possible involvement of N-type Ca⁺⁺ channels. J. Pharmacol. Exp. Ther. 270: 788-794, 1994[Abstract/Free Full Text].
Schlicker, E., Behling, A., Lummen, G., Malinowska, B. and Gothert, M.: Mutual interaction of histamine H₃-receptors and $alpha$ ₂-adrenoceptors on noradrenergic terminals in mouse and rat brain cortex. Naunyn-Schmiedeberg's Arch Pharmacol. 345: 639-646, 1992[Medline].
Schlicker, E., Fink, K., Hinterthaner, M. and Gothert, M.: Inhibition of noradrenaline release in the rat brain cortex via presynaptic H₃ receptors. Naunyn-Schmiedeberg's Arch. Pharmacol. 340: 633-638, 1989[Medline].
Schlicker, E., Kathmann, M., Detzner, M., Exner, H. J. and Gothert, M.: H₃ receptor-mediated inhibition of noradrenaline release: An investigation into the involvement of Ca²⁺ and K⁺ ions, G protein and adenylate cyclase. Naunyn-Schmiedeberg's Arch. Pharmacol. 350: 34-41, 1994[Medline].
Schlicker, E., Schunack, W. and Gothert, M.: Histamine H₃ receptor-mediated inhibition of noradrenaline release in pig retina discs. Naunyn-Schmiedeberg's Arch. Pharmacol. 342: 497-501, 1990[Medline].
Trzeciakowski, J. P.: Inhibition of guinea pig ileum contractions mediated by a class of histamine receptor resembling the H₃ subtype. J. Pharmacol. Exp. Ther. 243: 874-880, 1987[Abstract/Free Full Text].
Vollinga, R. C., de Koenig, J. P., Jansen, F. P. and Leurs, R.: A new potent and selective histamine H₃ receptor agonist, 4-(1H-Imidazolylmethyl)piperidine. J. Med. Chem. 37: 332-333, 1994[Medline].
Wood, J. D.: Physiology of the enteric nervous system. In Physiology of the Gastrointestinal Tract, (3rd ed.) ed. by Leonard R. Johnson, pp. 423-482, Raven Press, New York, 1994.

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Interaction Between Histamine H3 Receptors and Other Prejunctional Receptor Systems in the Isolated Guinea Pig Duodenum1,2

Interaction Between Histamine H₃ Receptors and Other Prejunctional Receptor Systems in the Isolated Guinea Pig Duodenum¹^,²