alpha -Adrenoceptor-Mediated Prejunctional Effects of Chloroethylclonidine in the Canine Saphenous Vein

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Vol. 282, Issue 3, 1326-1330, 1997

$alpha$ -Adrenoceptor-Mediated Prejunctional Effects of Chloroethylclonidine in the Canine Saphenous Vein¹

Serafim Guimarães, Maria Q. Paiva and Oduvaldo Pereira²

Institute of Pharmacology and Therapeutics, Faculty of Medicine, 4200-Porto, Portugal

	Abstract

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The present study was undertaken to look for the effect of chloroethylclonidine (CEC) on prejunctional alpha-2 autoreceptorsof the canine saphenous vein. The effect was tested on tritiumoverflow evoked by electrical stimulation from tissues preloadedwith 0.2 µM ³H-norepinephrine. Yohimbine (3-300 nM) and CEC (1-125 µM) increasedand UK-14,304 reduced the overflow of tritium evoked by 300 pulses(1 Hz). The maximal increase of tritium overflow caused by yohimbinewas much higher than that caused by CEC: 3.82 and 1.74 times,respectively. CEC (5 µM) abolished both the inhibition causedby UK-14,304 and the enhancement of tritium overflow caused byyohimbine. However, when CEC was added after yohimbine, it reducedthe electrically evoked overflow of tritium, the maximal effectbeing a reduction of tritium overflow by 35%. Prazosin (1-100nM) did not change either the inhibitory effect of UK-14,304 orthe facilitatory effect of CEC. These results suggest that CECacts on two different subtypes of prejunctional alpha-2 autoreceptors;on one of them it acts as an antagonist and increases the electricallyevoked overflow of tritium (and inhibits both the effect of UK-14,304and yohimbine); on the other it acts as an agonist and reducesthe electrically evoked overflow of tritium. Alternatively, onecan admit that CEC is able to inhibit alpha-2 autoreceptors, whichcauses an increase of the transmitter release, and to activatea nonadrenergic inhibitory receptor thus causing a reduction ofthe transmitter release.

	Introduction

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Chloroethylclonidine was described by Leclerc et al. (1980) as the first example of an alpha adrenoceptor agonist with anirreversible effect. Later on, CEC was found to bind irreversiblyto alpha-1B adrenoceptors and is now used both in binding andfunctional studies as an antagonist in the current definitionof alpha-1 subtypes (Han et al., 1987; Minneman et al., 1988).More recently CEC was found to be an irreversible agonist at postjunctionalalpha-2 adrenoceptors of the canine saphenous vein; this effectinvolved the activation of receptors that differ from those activatedby UK-14,304 (Nunes and Guimarães, 1992, 1993; Low et al., 1994).

Apart from the postjunctional effects of CEC, there is evidence for its action on prejunctional adrenoceptors. In the ratvas deferens, CEC reduces the release of norepinephrine and ofa purinergic co-transmitter by irreversible stimulation of prejunctionalalpha-2 adrenoceptors, and this effect is prevented by pretreatmentwith rauwolscine (Bültmann and Starke, 1993). Also in vivo (inthe pithed rat), CEC (25 µg/kg) significantly reduced the pressorresponse to electrical stimulation of spinal sympathetic nervesand this inhibitory effect was antagonized by idazoxan, whichindicates that CEC activates prejunctional alpha-2 autoreceptors(Vargas et al., 1994)

The present investigation was undertaken to study the effect of CEC on prejunctional alpha adrenoceptors of the canine saphenousvein.

A preliminary report of these results was presented at the 8th Meeting on Adrenergic Mechanisms (Guimarães and Paiva, 1994)

	Materials and Methods

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Tissue preparations. In the municipal dog pound, mongrel dogs, 10 to 16 kg in weight, of either sex, were anesthetized with pentobarbitone sodium(30 mg/kg). Immediately after removal, the saphenous veins wereplaced in small vials containing aerated (95% O₂ and 5% CO₂) andcold Krebs-Henseleit solution of the following composition (mM):NaCl, 118.6; KCl, 4.70; CaCl₂, 2.52; KH₂PO₄, 1.18; MgSO₄, 1.23;NaHCO₃, 2.50; glucose, 10; ascorbic acid, 0.57; disodium EDTA,0.027 (Guimarães et al., 1987). The animals were sacrificed byan overdose of pentobarbitone sodium (100 mg/kg). The veins werethen transported to the laboratory where they were helically cutinto small strips (of about 2.5 × 25 mm) which were preincubatedfor 30 min in medium containing 1 mM pargyline (to inhibit monoamineoxidase), 40 µM hydrocortisone and 50 µM U-0521 (3,4-dihydroxy-2-methylpropiophenone)(to inhibit extraneuronal removal of norepinephrine) (Guimarãeset al., 1978). Hydrocortisone and U-0521 were also kept in themedium for the remainder of the experiment. After preincubation,the vessel segments were exposed for 60 min to ³H-norepinephrine (0.2 µM).

Perifusion experiments. The vessel segments were mounted in 1-ml glass chambers between two platinum electrodes and perifused with amine-free medium(aerated and at 37°C) moving from bottom to top at a flow rateof 0.8 ml/min. From t = 100 min (t = 0 being the onset of theperifusion) the perifusion fluid was collected continuously as5-min samples. Transmural electrical stimulation (1 Hz, 2 ms,100 V, for 5 min; Stimulator II X, Hugo Sachs Elektronik, March-Hugstetten,Germany) was applied at min 120 (S₁), 170 (S₂), 220 (S₃), 270(S₄) and 320 (S₅).In addition to hydrocortisone and U-0521, cocaine(12 µM) was also present in the perifusion fluid from 90 min onward.

To test the effect of UK-14,304 [5-bromo-6-(imidazoline-2-ylamino-quinoxaline)], chloroethylclonidine or yohimbine, each ofthese drugs was used alone, being added cumulatively to the perifusionfluid in concentrations increasing by about half-log increments.These additions were made 20 min (UK-14,304 or yohimbine) or 30min (chloroethylclonidine) before S₃, S₄ and S₅. To study theinfluence of yohimbine on the effect of UK-14,304 or CEC, yohimbinewas added to the perifusion fluid 20 min before S₁ and left inthis fluid for the remainder of the experiment. Likewise, to studythe influence of CEC on the effect of UK-14,304 or yohimbine,CEC was added to the perifusion fluid 30 min before S₁ and leftin this fluid for the remainder of the experiment.

For the calculation of the overflow elicited by electrical stimulation, those samples were taken into account in which theoutflow of tritium exceeded that in the last prestimulation sample;usually this applied to the three or four samples collected duringand after stimulation. The spontaneous outflow measured in thelast prestimulation sample was assumed to represent the spontaneousoutflow in subsequent samples; it was subtracted from the outflowdetermined in stimulation and poststimulation samples. Fractional³H-efflux/min was calculated by dividing ³H-efflux in each 5-min sample by tritium present in the tissueat the onset of the respective collection period and by 5. Thefractional release was calculated by dividing evoked tritium overflowby tritium present in the tissue at the beginning of the stimulationperiod. Drug effects are expressed as percentage of the fractionalrelease of tritium evoked by S₃ (or S₄ or S₅) over that evokedby S₂. Each result was corrected for tissue-dependent changesas determined in parallel drug-free control experiments.

IC_50% represents the concentration of the agonist that reduces the evoked overflow of tritium by 50% and EC_50%represents the concentration of the antagonist that increasesthe evoked overflow by 50%. Both IC_50% and EC_50%values were determined by interpolation between the two nearestpoints from the 50% values of the concentration-response curves.

Determination of tritium in the overflow and in the tissue. Radioactivity was measured by liquid scintillation counting (liquid scintillation counter 1209 Rackbeta LKB Wallac, Turku,Finland) in 2-ml aliquots of perifusate or 0.5 ml of tissue extract+ 1.5 ml of Krebs-Henseleit solution. The extraction was madein 3 ml of 0.1 M perchloric acid during 18 h.

Statistical analysis. Results are expressed as arithmetic means ± S.E.M. or as geometric means with 95% confidence limits. One-way analysis of variancewas used to test differences between unpaired results. A probabilitylevel of .05 or less was considered statistically significant.

Drugs. Chloroethylclonidine hydrochloride (RBI, Natick, MA); cocaine hydrochloride (Uquipa, Lisboa, Portugal); hydrocortisone 21-hemisuccinate(Sigma, St. Louis, MO); ³H-7-( $-$ )-norepinephrine (12.4 Ci·mmol¹) (New England Nuclear, Dreieich, Germany); pargyline hydrochloride(Sigma); U-0521 (3,4-dihydroxy-2-methyl-propiophenone; UpjohnKalamazoo, MI); UK-14,304 [5-bromo-6-(imidazoline-2-ylamimo-quinoxaline)](Pfizer, Seixal, Portugal); yohimbine hydrochloride (Sigma)

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

In the first series of experiments, vein strips prelabeled with ³H-norepinephrine were stimulated electrically five times; eachstimulation period (S₁ to S₅) consisted of a train of 300 pulses(1 Hz). In the absence of drugs, the spontaneous outflow of tritiumdecreased slowly with time. However, the fractional rate of loss(spontaneous outflow per min divided by tritium content of thetissue) remained constant as in previous studies (Guimarães etal., 1978). The fractional rate of spontaneous tritium outflowimmediately before S₂ was 0.000162 ± 0.000006/min (n = 30) andthe overflow elicited by S₂ amounted to 0.332 ± 0.017% (n = 42)of tritium content of the tissue. In the absence of drugs, theevoked overflow expressed in % of tissue content (see "Materialsand Methods") remained approximately constant from S₁ to S₅ incontrol experiments (for example, ratio S₅/S₂ = 0.99 ± 0.10; n= 5).

Effect of UK-14,304. In most of the experiments, UK-14,304 was added cumulatively to the perifusion fluid; three concentrations were used per strip:3, 10 and 30 nM or 10, 30 and 100 nM. The first, the second andthe third addition were made 20 min before S₃, S₄ and S₅, respectively.UK-14,304 caused concentration-dependent reductions of tritiumoverflow evoked by electrical stimulation with an IC_50%value of 16.9 (14.6; 19.7) nM, (n = 5). The maximal effect ofUK-14,304 was a reduction of tritium overflow by 77.0 ± 5.3% (n= 6) (fig. 1).

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Fig. 1. Canine saphenous vein. Effect of UK-14,304 on tritium overflow evoked by electrical stimulation (1 Hz, 2 ms, 100 V, during5 min) from the tissue preloaded with ³H-norepinephrine (0.2 µM): (- $bullet$ -) in the absence of any treatment;( $---$ $open circle$ $---$ ) in the presence of CEC (5 µM); (- $black-triangle$ -) in the presence ofyohimbine (100 nM). CEC and yohimbine were added 30 and 20 minbefore S₁, respectively, and were present for the remainder ofthe experiment. The fractional release in the presence of CECand in the presence of yohimbine was 1.41 and 3.82 times higherthan in controls, respectively. Means ± S.E. from five or sixexperiments. * Significantly different from corresponding control(P < .05).

Effect of CEC. CEC did not change the fractional rate of spontaneous tritium outflow. In some experiments cumulative concentration-responsecurves were determined for the effect of CEC (1-125 µM) on theelectrically evoked overflow of tritium. As for UK-14,304, onlythree concentrations were used per experiment: 1, 5 and 25 µMor 5, 25 and 125 µM. The first addition of CEC (1 or 5 µM) wasperformed 30 min before S₃, the second (5 or 25 µM) 30 min beforeS₄ and the third (25 or 125 µM) 30 min before S₅. As shown infigure 2, CEC (1-125 µM) caused a concentration-dependent increaseof the electrically evoked overflow of tritium, its EC_50%being 14.1 (5.1;39.3) µM (n = 6). The maximal effect of CEC wasobtained with 125 µM and increased the evoked overflow by a factorof 1.74 (1.45;2.09) (n = 6).

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Fig. 2. Canine saphenous vein. Effect of CEC on tritium overflow evoked by electrical stimulation (1 Hz, 2 ms, 100 V, during 5 min)from the tissue preloaded with ³H-norepinephrine (0.2 µM), in the absence (- $bullet$ -) and in the presence(- $open circle$ -) of yohimbine (100 nM). Yohimbine was added 20 min beforeS₁ and was present for the remainder of the experiment. CEC wasadded cumulatively, each addition being made 30 min before theelectrical stimulation. The fractional release in the presenceof yohimbine was 3.82 times higher than in controls. Means ± S.E.from four experiments.

In some experiments, the influence of CEC on UK-14,304 effects was studied. In these experiments CEC was added to the perifusionfluid 30 min before S₁ and left in this fluid for the remainderof the experiment. Under these conditions, 5 µM CEC abolishedthe inhibitory effect of UK-14,304 (3-100 nM) (fig. 1).

Effect of yohimbine. When used alone, yohimbine (3-300 nM) was added cumulatively to the perifusion fluid according to the schedule which was similarto that for UK-14,304 and CEC; 3, 10 and 100 nM were used in someexperiments and 10, 30 and 300 nM in others. The first additionof yohimbine to the perifusion fluid was made 20 min before S₃and the subsequent ones 20 min before S₄ and S₅. As shown in figure3, yohimbine increased the overflow of tritium evoked by electricalstimulation in a concentration-dependent manner. The EC_50%of yohimbine was 3.1 (1.2; 7.9) nM, (n = 4) and its maximal effectincreased the electrically evoked overflow of tritium by a factorof 3.82 (3.06; 4.39) (n = 6) (fig. 3). When CEC (5 µM) was addedto the perifusion fluid before yohimbine (see "Materials and Methods")it abolished this enhancing effect of yohimbine (fig. 3).

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Fig. 3. Canine saphenous vein. Effect of yohimbine on tritium overflow evoked by electrical stimulation (1 Hz, 2 ms, 100 V, during5 min) from the tissue preloaded with ³H-norepinephrine (0.2 µM) in the absence (- $bullet$ -) and in the presence(- $open circle$ -) or CEC (5 µM). CEC was added to the perifusion fluid 30min before S₁ and was present for the remainder of the experiment.Yohimbine was added cumulatively, each addition being made 20min before the electrical stimulation. The fractional releasein the presence of CEC was 1.41 times higher than in controls.Means ± S.E. from four or five experiments. *Significantly differentfrom the corresponding value obtained in the absence of CEC.

When yohimbine (100 nM) was added to the perifusion fluid before the other drugs under study (see "Materials and Methods")it abolished the inhibitory effect of UK-14,304 (3-100 nM) (fig.1) and reversed that of CEC which became inhibitory (fig. 2).The maximal inhibitory effect of CEC after yohimbine reduced tritiumoverflow by 35.2 ± 5.8% (n = 2).

Effect of prazosin. When used alone, prazosin (1-100 nM) did not change either the spontaneous efflux of tritium or its overflow elicited by electricalstimulation. In concentrations up to 100 nM, prazosin also didnot change either the inhibitory effect of UK-14,304 (3-100 nM)or the facilitatory effect of CEC (5-125 µM). At the concentrationof 1 µM, prazosin caused a small but significant displacementof the concentration-response curve of CEC to the right (fig.4).

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Fig. 4. Canine saphenous vein. Influence of CEC on tritium overflow evoked by electrical stimulation (1 Hz, 2 ms, 100 V, during 5min) from tissues preloaded with ³H-norepinephrine (0.2 µM) in the absence (control) (- $bullet$ -) and inthe presence of prazosin: 1 nM (- $open circle$ -), 10 nM (- $black-diamond$ -), 100 nM (- $black-square$ -)and 1 µM (- $black-triangle$ -). Means ± S.E. from four experiments. *Significantlydifferent from the control.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

In the first study of the effects of CEC at the prejunctional level it was shown that in the rat vas deferens CEC reducedthe release of noradrenaline by irreversible activation of prejunctionalalpha-2 adrenoceptors (Bültmann and Starke, 1993). In the presentstudy it was shown that CEC, in a concentration-dependent way,increased the overflow of tritium evoked by electrical stimulationof the canine saphenous vein, which indicates that CEC inhibitsprejunctional alpha adrenoceptors in this tissue. Furthermore,CEC abolished the concentration-dependent reduction of the electricallyevoked overflow of tritium caused by the selective alpha-2 adrenoceptorUK-14,304 confirming that CEC inhibits prejunctional alpha-2 autoreceptorsin the canine saphenous vein. This is the first report of an antagonisticaction of CEC at prejunctional alpha-2 adrenoceptors.

Surprisingly, in the presence of the classical selective alpha-2 adrenoceptor antagonist yohimbine, the effect of CEC wasreversed, a reduction of the overflow evoked by electrical stimulationbeing observed. This unexpected finding may be explained on thebasis of the existence of more than one kind of receptor for CEC.The first example of such a reversal phenomenon, the conversionof a pressor effect to exogenous epinephrine into a depressorone by ergotoxine, was observed in vivo and was described by Dale(1906). Only 42 years later this reversal phenomenon was interpretedby Ahlquist (1948) on the basis of the existence of two differenttypes of adrenoceptors. Some years later, such a reversal phenomenonwas also shown in isolated organs. In strips of saphenous veinpreviously contracted by prostaglandin F₂ in the presenceof phentolamine, epinephrine caused a concentration-dependentrelaxation; similarly, in strips preloaded with epinephrine andpreviously contracted by prostaglandin F₂ in the presenceof phentolamine, electrical stimulation caused frequency-dependentrelaxations. This inhibitory response to either exogenous or "endogenous" epinephrine was also interpreted on the basis of theexistence of two different kinds of receptors (Guimarães andPaiva, 1981a, b). The reversal observed in the present study mayalso show the existence of two different subtypes of alpha-2 adrenoceptorsat prejunctional level of the canine saphenous vein. When we comparethe reversal obtained in the present study with those referredto above, we have to take into account a disturbing factor, theincrease in norepinephrine concentration at the biophase causedby yohimbine in the present experiments. However, it is not easyto explain how this increase contributes to the reversal observed.The addition of the same drugs (yohimbine + CEC) by a reversedorder (CEC first) gave no place to any reduction of the electricallyevoked overflow despite the increase in norepinephrine concentrationat the biophase.

Based on functional studies with different agonists and antagonists in several tissues, evidence has been accumulated whichsupports the hypothesis that more than one subtype of alpha-2adrenoceptors exist prejunctionally. For example, Akers et al.(1991) showed that the antagonist potency of the compound SK&F104078 at prejunctional alpha-2 adrenoceptors is agonist- andtissue-dependent. Furthermore, Oriowo et al. (1991) proposed theexistence of two prejunctional alpha-2 adrenoceptor subtypes inthe rat vas deferens, one being sensitive to SK&F 104078 and anotherbeing insensitive to this compound.

CEC caused an enhancement of the overflow evoked by electrical stimulation which was smaller than that caused by yohimbine(1.74- and 3.82-fold, respectively). This difference between themaximal effects of these two antagonists may be explained if oneadmits that CEC acts simultaneously on two different populationsof prejunctional alpha adrenoceptors: as antagonist on one ofthem and as agonist on the other one. The final enhancement ofthe electrically evoked overflow of tritium caused by CEC wassmaller than that caused by yohimbine because it represents thealgebraic sum of an inhibitory effect (caused by the activationof one population of alpha adrenoceptors) and a facilitatory effect(caused by the blockade of the other population of alpha adrenoceptors).The capacity of CEC to be agonist on some alpha-2 adrenoceptorsand antagonist on others has already been reported. The above-discussedreversal of CEC effect, from a facilitatory (in the absence ofyohimbine) into an inhibitory one (in the presence of yohimbine),may be explained assuming that yohimbine blocks only one partof the prejunctional alpha-2 adrenoceptors in this tissue. Unpublishedresults (S. Guimarães and M.Q. Paiva) indicate that both oxymetazolineand UK-14,304 cause a reduction of the electrically evoked overflowof tritium in this tissue. However, these selective alpha-2 adrenoceptoragonists are differentially antagonized by yohimbine, exactlyas alpha-2 adrenoceptors in the rat vas deferens, a fraction ofwhich is sensitive to SKF 104078 and another is insensitive (Bylundand Iversen, 1990; Oriowo et al., 1991). Alternatively, one mayspeculate that, under control conditions, CEC inhibits alpha-2autoreceptors (thus causing an increase in the overflow of tritium)and that in the presence of the alpha-2 adrenoceptor antagonistyohimbine it activates some nonadrenergic receptor (imidazoline-,5-hydroxytryptamine-, dopamine receptor) the activation of whichcauses a decrease of tritium-evoked overflow.

The hypothesis that prejunctional alpha-1 adrenoceptors might be involved in the effect of CEC can be ruled out because prazosin,in concentrations up to 100 nM, did not change either the inhibitoryinfluence of UK-14,304 or the facilitatory influence of CEC. Accordingto Flavahan and Vanhoutte (1986), the pA₂ values for prazosinagainst alpha-1 adrenoceptor-mediated responses in isolated bloodvessels ranged from 10 pM to 10 nM. In earlier experiments carriedout in the saphenous vein, at postjunctional level the pA₂ valuesof prazosin were 7.65 and 6.02 for alpha-1 and alpha-2 adrenoceptor-mediatedresponses, respectively (Guimarães and Nunes, 1990). In the presentstudy, the concentrations of prazosin required to antagonize CECare as high as those required to block alpha-2 adrenoceptors.

Which kind (kinds) of alpha-2 adrenoceptors are involved in these responses to UK-14,304, CEC and yohimbine in the saphenousvein is a question to which the present results give no answer.In the human saphenous vein, prejunctional alpha-2 adrenoceptorshave been characterized as alpha-2A adrenoceptors (Molderingsand Göthert, 1995). However, there are interesting differencesbetween human and canine saphenous veins at the prejunctionallevel. For example, whereas the canine saphenous vein is endowedwith prejunctional beta adrenoceptors mediating a facilitatoryinfluence on the transmitter release (Guimarães et al., 1978),the human saphenous vein is devoid of these receptors (Molderingset al., 1988); Moreover, although oxymetazoline did not act asan agonist, inhibiting the electrically evoked overflow of tritiumin the human saphenous vein (Molderings and Göthert., 1995),it acted as a potent agonist which concentration-dependently reducedthe overflow of tritium evoked by electrical stimulation in thesaphenous vein (M.Q. Paiva, A. Mota, D. Moura, S. Guimarães,unpublished results).

In conclusion, the present results suggest that, at prejunctional levels of the canine saphenous vein, there is more thanone kind of alpha-2 adrenoceptor which both participate in thefeedback regulation of norepinephrine release evoked by electricalstimulation; alternatively, it may be that the canine saphenousvein is endowed with alpha-2 adrenoceptors mediating an inhibitoryinfluence which is blocked by CEC and also with some kind of nonadrenergicreceptors also mediating an inhibitory effect which is activatedby CEC. These results also show that CEC cannot be taken as a"pure" alpha-1B antagonist, because in the canine saphenous vein,it inhibits alpha-2 adrenoceptor-mediated responses.

	Footnotes

Accepted for publication May 23, 1997.

Received for publication December 31, 1996.

¹ This work was supported by Junta Nacional de Investigação Científica e Tecnológica (JNICT)-Project number PECS/P/SAU/80/95,by PRAXIS/2/2.1/SAU/1293/95 and by Biomed 2 (EureCa project).

² Present address: Departamento de Farmacologia. I.B. Botucatu-UNESP, 18600 Botucatu, SP, Brasil.

Send reprint requests to: S. Guimarães, Institute of Pharmacology and Therapeutics, Faculty of Medicine, 4200-Porto, Portugal.

	Abbreviations

CEC, chloroethylclonidine; U-0521, 3,4-dihydroxy-2-methylpropiophenone.

	References

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S. Guimaraes and D. Moura
Vascular Adrenoceptors: An Update
Pharmacol. Rev., June 1, 2001; 53(2): 319 - 356.
[Abstract] [Full Text] [PDF]

A. Marjamaki, H. Frang, M. Pihlavisto, A.-M. Hoffren, T. Salminen, M. S. Johnson, J. Kallio, J. A. Javitch, and M. Scheinin
Chloroethylclonidine and 2-Aminoethyl Methanethiosulfonate Recognize Two Different Conformations of the Human alpha 2A-Adrenergic Receptor
J. Biol. Chem., July 30, 1999; 274(31): 21867 - 21872.
[Abstract] [Full Text] [PDF]

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				S. Guimaraes and D. Moura Vascular Adrenoceptors: An Update Pharmacol. Rev., June 1, 2001; 53(2): 319 - 356. [Abstract] [Full Text] [PDF]

				A. Marjamaki, H. Frang, M. Pihlavisto, A.-M. Hoffren, T. Salminen, M. S. Johnson, J. Kallio, J. A. Javitch, and M. Scheinin Chloroethylclonidine and 2-Aminoethyl Methanethiosulfonate Recognize Two Different Conformations of the Human alpha 2A-Adrenergic Receptor J. Biol. Chem., July 30, 1999; 274(31): 21867 - 21872. [Abstract] [Full Text] [PDF]

-Adrenoceptor-Mediated Prejunctional Effects of Chloroethylclonidine in the Canine Saphenous Vein1

$alpha$ -Adrenoceptor-Mediated Prejunctional Effects of Chloroethylclonidine in the Canine Saphenous Vein¹