Analysis of Mecamylamine Stereoisomers on Human Nicotinic Receptor Subtypes

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Vol. 297, Issue 2, 646-656, May 2001

Analysis of Mecamylamine Stereoisomers on Human Nicotinic Receptor Subtypes

Roger L. Papke, Paul R. Sanberg and R. Douglas Shytle

Department of Pharmacology and Therapeutics, University of Florida, Gainesville, Florida (R.L.P.); and Departments of Neurosurgery and Psychiatry and the Neuroscience Program, University of South Florida College of Medicine, Tampa, Florida (P.R.S., D.S.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

Because mecamylamine, a nicotinic receptor antagonist, is used so often in nicotine research and because mecamylamine mayhave important therapeutic properties clinically, it is importantto fully explore and understand its pharmacology. In the presentstudy, the efficacy and potency of mecamylamine and its stereoisomerswere evaluated as inhibitors of human $alpha$ 3 $beta$ 4, $alpha$ 3 $beta$ 2, $alpha$ 7, and $alpha$ 4 $beta$ 2nicotinic acetylcholine receptors (nAChRs), as well as mouse adulttype muscle nAChRs and rat N-methyl-D-aspartate (NMDA) receptorsexpressed in Xenopus oocytes. The selectivity of mecamylaminefor neuronal nAChR was manifested primarily in terms of slow recoveryrates from mecamylamine-induced inhibition. Neuronal receptorsshowed a prolonged inhibition after exposure to low micromolarconcentrations of mecamylamine. Muscle-type receptors showed atransient inhibition by similar concentrations of mecamylamine,and NMDA receptors were only transiently inhibited by higher micromolarconcentrations. Mecamylamine inhibition of neuronal nAChR wasnoncompetitive and voltage dependent. Although there was littledifference between S-(+)-mecamylamine and R-( $-$ )-mecamylamine interms of 50% inhibition concentration values for a given receptorsubtype, there appeared to be significant differences in the off-ratesfor the mecamylamine isomers from the receptors. Specifically,S-(+)-mecamylamine appeared to dissociate more slowly from $alpha$ 4 $beta$ 2and $alpha$ 3 $beta$ 4 receptors than did R-( $-$ )-mecamylamine. In addition, itwas found that muscle-type receptors appeared to be somewhat moresensitive to R-( $-$ )-mecamylamine than to S-(+)-mecamylamine. Together,these findings suggest that in chronic (i.e., therapeutic) application,S-(+)-mecamylamine might be preferable to R-( $-$ )-mecamylamine interms of equilibrium inactivation of neuronal receptors with decreasedside effects associated with muscle-typereceptors.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Mecamylamine is widely used as a broad-spectrum antagonist of neuronal nicotinic acetylcholine (ACh) receptors (nAChRs) and,despite its common usage, questions still exist as to its precisespecificity and mechanisms of action. The present study evaluatesthe effects of mecamylamine on a wide range of nAChRs and additionallyevaluates whether the stereoisomers of this drug augment the specificityor efficacy for desired therapeuticeffects.

In the context of therapeutics, mecamylamine (Inversine) was developed and characterized by Merck (Darmstadt, Germany) asa ganglionic blocker with clinically significant hypotensive actions(Stone et al., 1956). Unique characteristics of mecamylamine,including exceptional oral efficacy, rapid onset, long durationof action, and nearly complete absorption from the gastrointestinaltract, made mecamylamine, at that time, a more desirable antihypertensivemedication than the existing ganglionic blockers (Baer et al.,1956).

Despite mecamylamine's efficacy in the treatment of hypertension, its side effects resulting from broad parasympathetic inhibitionat antihypertensive doses reduced its popularity in the treatmentof essential hypertension. However, in addition to its peripheralganglionic blocking actions, mecamylamine crosses the blood-brainbarrier and functions as a cholinergic antagonist specific toneuronal nicotinic receptor subtypes (Varanda et al., 1985; Martinet al., 1989, 1993; Banerjee et al., 1990). Because mecamylaminereadily blocks most of the physiological, behavioral, and reinforcingeffects of nicotine, it has become the most commonly used of allneuronal nAChR-specific inhibitors in basic nicotine research(Martin et al., 1989, 1993) and has been reported to be effectiveas an aid to smoking cessation (Tennant et al., 1984; Rose etal., 1994, 1998).

Since nicotine has both agonist and antagonistic properties, nicotinic receptor antagonists, such as mecamylamine, may alsobe useful for a wide range of nicotine-responsive neuropsychiatricdisorders. For example, mecamylamine, like nicotine, has alsobeen reported to possibly augment neuroleptic therapy of Tourette'ssyndrome (Sanberg et al., 1998). In addition, growing evidencesuggests that nicotinic receptor activation may also be involvedwith the actions of other drugs of abuse, including psychostimulantsand alcohol. It has been reported that mecamylamine prevents theinduction of locomotor sensitization to amphetamine in mice (Karleret al., 1996), and low doses of mecamylamine were recently foundto reduce cue-induced craving in human cocaine abusers (Reid etal., 1999). Furthermore, several preclinical studies have reportedthat mecamylamine reduces the behavioral and reinforcing effectsof alcohol in animals (Blomqvist et al., 1996, 1997; Ericson etal., 1998; Nadal et al., 1998).

The present study investigates the selectivity of mecamylamine and its stereoisomers by using the genes cloned from the nervoussystem, which code for nicotinic acetylcholine receptor subunits.The nAChRs are known to be formed by the association of five monomericsubunits. The neuronal nAChR gene family include nine proteinsdesignated as $alpha$ subunits ( $alpha$ 2- $alpha$ 10) and three proteins designatedas $beta$ subunits ( $beta$ 2- $beta$ 4) (Papke, 1993; Elgoyhen et al., 1994, 2001).Except for $alpha$ 7 subunits that may form functional homomeric receptors,most nicotinic receptors found in the mammalian central nervoussystem require at least one type of $alpha$ and one type of $beta$ subunitto form functional nAChR channels. Neuronal nAChRs are both structurallyand phylogenetically related to the nicotine receptors of theneuromuscular junction. The mature muscle-type nAChRs containtwo $alpha$ 1 subunits, one $beta$ 1 subunit, one $delta$ subunit, and one $epsilon$ subunit(Mishina et al., 1986).

This study specifically evaluated the efficacy and potency of highly pure R-( $-$ )-mecamylamine and S-(+)-mecamylamine on human $alpha$ 3 $beta$ 4, $alpha$ 4 $beta$ 2, $alpha$ 3 $beta$ 2, and $alpha$ 7 receptors expressed in Xenopus oocytesand compared their activity to that of racemic mecamylamine. Thevoltage dependence and reversibility of inhibitory activity wasalso investigated. Since prior research in this lab suggestedthat a residual inhibition of receptors by mecamylamine is stillpresent after a 5-min wash period (Webster et al., 1999), it washypothesized that the persistence of block (an indirect indicationof the dissociation rate) might prove to be an important distinguishingfeature of the stereoisomers. In addition, the report of finding"interesting differences" between the actions of mecamylaminestereoisomers in assays measuring neuromuscular transmission (Schoenenbergeret al., 1986) prompted our investigation of the inhibitory actionsof these stereoisomers at adult-type mouse muscle nAChRs expressedin Xenopusoocytes.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Chemicals. Fresh acetylcholine (Sigma, St. Louis, MO) stock solutions were made daily in Ringer's solution and diluted. Racemic-(±)-mecamylamine(N-2,3,3-tetramethylbicyclo[2.2.1]heptan-2-amine) and the stereoisomerswere supplied by Layton Biosciences (Menlo Park, CA). All otherchemicals for electrophysiology were obtained from Sigma (St.Louis,MO).

Preparation of RNA and Expression in Xenopus Oocytes. Mature (>9 cm) female Xenopus laevis African toads (Nasco, Ft. Atkinson, WI) were used as a source of oocytes. Before surgery,frogs were anesthetized by placing the animal in a 1.5 g/l solutionof MS222 (3-aminobenzoic acid ethyl ester) for 30 min. Eggs wereremoved from an incision made in the abdomen. The incisions weredisinfected with gentamicin, sutured with 4-0 gut, and the animalswere allowed to recover from the anesthesia in a humid environment.Postoperative animals were kept in isolation tanks and checkeddaily before return to thecolony.

After linearization and purification of cloned cDNA, RNA transcripts were prepared in vitro using the appropriate mMessagemMachine kit from Ambion, Inc. (Austin, TX). Harvested oocyteswere treated with collagenase from Worthington Biochemical Corporation(Freehold, NJ) for 2 h at room temperature in calcium-free Barth'ssolution (88 mM NaCl, 10 mM HEPES, pH 7.6, 0.33 mM MgSO₄, 0.1mg/ml gentamicin sulfate). Subsequently, stage 5 oocytes wereisolated and injected with 50 nl each of a mixture of the appropriatesubunit cRNAs. Recordings were made 1 to 7 days after injection,depending on the cRNAs beingtested.

Electrophysiology. Oocyte recordings were made with a Warner Instruments (Hamden, CT) OC-725C oocyte amplifier and RC-8 recording chamber interfacedto a Macintosh personal computer. Data were acquired using Labviewsoftware (National Instruments, Austin, TX) and filtered at arate of 6 Hz. Oocytes were placed in the recording chamber witha total volume of about 0.6 ml and perfused at room temperatureby frog Ringer's solution (115 mM NaCl, 2.5 mM KCl, 10 mM HEPES,pH 7.3, 1.8 mM CaCl₂) containing 1 µM atropine to inhibit potentialmuscarinic responses. A Mariotte flask filled with Ringer's solutionwas used to maintain a constant hydrostatic pressure for drugdeliveries and washes. Current electrodes were filled with a solutioncontaining 250 mM CsCl, 250 mM CsF, and 100 mM EGTA and had resistancesof 0.5 to 2 M $Omega$ . Voltage electrodes were filled with 3 M KCl andhad resistances of 1 to 3 M $Omega$ .

Drugs were diluted in perfusion solution and loaded into a 2-ml loop at the terminus of the perfusion line. A bypass of thedrug-loading loop allowed bath solution to flow continuously whilethe drug loop was loaded, and then drug application was synchronizedwith data acquisition by using a two-way electronic valve. Therate of bath solution exchange and all drug applications was 6ml/min. We have previously shown that this protocol delivers abrief but essentially complete solution exchange around the surfaceof the oocyte (Papke and Thinschmidt, 1998

). A double-loop protocolwas used for the determination of concentration-response relationships.With this method, the cells were first equilibrated for 12 s ina solution of the inhibitor alone and then tested with the coapplicationof ACh and theinhibitor.

Experimental Protocols and Data Analysis. Current responses to drug application were studied under two-electrode voltage clamp at a holding potential of $-$ 50 mV unlessotherwise noted. Holding currents immediately before agonist applicationwere subtracted from measurements of the peak response to agonist.All drug applications were separated by a wash period of 5 minunless otherwise noted. At the start of recording, all oocytesreceived two initial control applications of ACh. Subsequent drugapplications were normalized to the second ACh application tocontrol for the level of channel expression in each oocyte. Thesecond application of control ACh was used to minimize the affectsof rundown that occasionally occurred after the initial ACh-evokedresponse. To measure residual inhibitory effects, an experimentalapplication of ACh with inhibitor or of inhibitor alone was followedby a second application of ACh alone and compared with the preapplicationcontrol ACh response. Means and standard errors (S.E.M.) werecalculated from the normalized responses of at least four oocytesfor each experimentalconcentration.

For each of the receptor subtypes tested, a control ACh concentration was selected that was sufficient to stimulate the receptorsto a level representing a reasonably high value of p_open at thepeak of the response while minimizing rundown with successiveACh applications. For potent use-dependent inhibitors, we havefound that such conditions were adequate to achieve maximal inhibition(Papke et al., 1994

; Francis and Papke, 1996

). The control AChconcentrations used were 30 µM ACh for $alpha$ 4 $beta$ 2, 100 µM ACh for $alpha$ 3 $beta$ 4,30 µM ACh for $alpha$ 3 $beta$ 2, 300 µM ACh for $alpha$ 7, and 3 µM ACh for $alpha$ 1 $beta$ 1 $delta$ $epsilon$ .These correspond to the EC₃₀, EC₁₀, EC₁₅, EC₅₀, and EC₅₀, respectively,for thesereceptors.

For concentration-response relations, data were plotted using Kaleidagraph 3.0.2 (Abelbeck Software; Reading, PA), and curveswere generated from the Hill equation (Webster et al., 1999

<UP>Response</UP>=<FR><NU>I<SUB><UP>max</UP></SUB>[<UP>agonist</UP>]<SUP>n</SUP></NU><DE>[<UP>agonist</UP>]<SUP>n</SUP>+(<UP>EC<SUB>50</SUB></UP>)<SUP>n</SUP></DE></FR>

where I_max denotes the maximal response for a particular agonist/subunit combination, and n represents the Hill coefficient.Negative Hill slopes were applied for the calculation of IC₅₀values.

For the analysis of ACh concentration-response relationships in the presence and absence of mecamylamine (i.e., competitionexperiments), data were initially normalized based on controlACh responses, as described above. Data were subsequently scaledby a factor relating the efficacy of control ACh responses tothe maximum responses obtained with ACh.

Calculations of net charge during evoked responses were made by integration of the current responses for 200 s after the initialdeflection from baseline. Specifically, raw data values for experimentalresponses were imported into a template Excel spreadsheet alongwith the raw data for the corresponding ACh controls obtained5 min before the experimental response. Each record included ashort (0.5 s) interval of baseline that was used for offset correction.Peaks and areas were then calculated for both the experimentaland control responses, and the experimental values were expressedrelative to their respectivecontrols.

For experiments assessing voltage-dependence of inhibition, oocytes were voltage-clamped at a holding potential of either $-$ 40 mV or $-$ 90 mV, and a control application of ACh alone was delivered.The holding potential was then kept at the designated voltagefor the coapplication of ACh with mecamylamine. Residual inhibitionwas evaluated with a subsequent application of ACh alone at thetest potential, after a 5-min washperiod.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Inhibition of nAChR Subtypes by Mecamylamine Stereoisomers. Racemic mecamylamine and its stereoisomers were tested for their ability to inhibit the ACh-evoked responses of $alpha$ 4 $beta$ 2, $alpha$ 3 $beta$ 4, $alpha$ 3 $beta$ 2, and $alpha$ 7 type receptors expressed in Xenopus oocytes. Rawdata traces showing the effect of 10 µM mecamylamine stereoisomerson these receptor subtypes are shown in Fig. 1. To prevent confoundingthe effect of changing both ACh and mecamylamine concentrationsduring the rising phase of the evoked responses, cells were firstpre-equilibrated with mecamylamine before ACh was applied in thecontinuing presence of mecamylamine (see Materials and Methods).As shown in Fig. 1, 10 µM of either mecamylamine stereoisomerproduced significant inhibition of the nAChR subtypes. Additionally,for each of the $beta$ subunit-containing receptor subtypes, therewas a marked decrease in subsequent control responses to ACh whenit was applied 5 min after exposure to mecamylamine. A summaryof the residual inhibition produced by 10 µM mecamylamine is shownin Fig. 2. The residual inhibition was greatest for $beta$ 2-containingreceptors and least for $alpha$ 7 receptors. There was no stereo-selectivityapparent in the 5-min recovery data. The time dependence of recoveryis considered further below.

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Fig. 1. Effect of mecamylamine (Mec) on neuronal nAChR. A, representative traces showing the effect of the two mecamylamine stereoisomers on ACh-evoked currents in $alpha$ 4 $beta$ 2-expressing oocytes. The traces illustrate initial control responses to 30 µM ACh alone (application indicated by black bar) and then the application of 30 µM ACh in the presence of 10 µM mecamylamine (open bar). B, representative traces showing the effect of the two mecamylamine stereoisomers (10 µM) on currents evoked by 100 µM ACh in $alpha$ 3 $beta$ 4-expressing oocytes. C, representative traces showing the effect of the two mecamylamine stereoisomers (10 µM) on currents evoked by 30 µM ACh in $alpha$ 3 $beta$ 2-expressing oocytes. D, representative traces showing the effect of the two mecamylamine stereoisomers (10 µM) on currents evoked by 300 µM ACh in $alpha$ 7-expressing oocytes. In each panel, the third trace in each row shows the response to a control ACh application 5 min after the application of mecamylamine.

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Fig. 2. Residual effects of mecamylamine (Mec) on ACh control responses. Control ACh responses 5 min after the coapplication of 10 µM mecamylamine to $alpha$ 4 $beta$ 2 receptors (A), $alpha$ 3 $beta$ 4 receptors (B), $alpha$ 3 $beta$ 2 receptors (C), and $alpha$ 7 receptors (D). Control ACh concentrations used for these receptor subtypes were 30 µM, 100 µM, 30 µM, and 300 µM, respectively. Each bar represents the average normalized responses of four to seven cells.

The concentration-response analyses for human $alpha$ 4 $beta$ 2, $alpha$ 3 $beta$ 4, $alpha$ 3 $beta$ 2, and $alpha$ 7 nAChR are shown in Fig. 3. The IC₅₀ values are givenin Table 1. The mecamylamine compounds were most potent at inhibiting $alpha$ 3 $beta$ 4 receptors and least potent at inhibiting $alpha$ 7 receptors. Thereappeared to be very little difference between the R-( $-$ )-isomersand S-(+)-isomers at any of these receptor subtypes in terms ofpotency for inhibition.

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Fig. 3. Concentration-response relationships for the effects of mecamylamine (Mec) and its stereoisomers on neuronal nAChR. A, concentration-response relationship for mecamylamine's inhibition of the peak currents of $alpha$ 4 $beta$ 2 receptors when 30 µM ACh was coapplied with mecamylamine at the indicated concentrations. Data from each oocyte were normalized to that cell's response to 30 µM ACh alone. B, concentration-response relationship for mecamylamine's inhibition of the peak currents of $alpha$ 3 $beta$ 4 receptors when 100 µM ACh was coapplied with mecamylamine at the indicated concentrations. Data from each oocyte were normalized to that cell's response to 100 µM ACh alone. C, concentration-response relationship for mecamylamine's inhibition of the peak currents of $alpha$ 3 $beta$ 2 receptors when 30 µM ACh was coapplied with mecamylamine at the indicated concentrations. Data from each oocyte were normalized to that cell's response to 30 µM ACh alone. D, concentration-response relationship for mecamylamine's inhibition of the peak currents of $alpha$ 7 receptors when 300 µM ACh was coapplied with mecamylamine at the indicated concentrations. All cells were pre-equilibrated with mecamylamine, at the indicated concentration, for 10 s before the coapplication of agonist with antagonist. Each point represents the average normalized response of four to seven cells.

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TABLE 1
IC₅₀ values

The Selectivity of Mecamylamine for Neuronal nAChR. To confirm the selectivity of mecamylamine for neuronal nAChR over muscle-type nAChR, we also examined the effects of R-( $-$ )-mecamylamineand S-(+)-mecamylamine on adult-type $alpha$ 1 $beta$ 1 $delta$ $epsilon$ receptors, using mousecDNA clones. Mecamylamine could produce a transient inhibitionof muscle-type receptor responses with a potency roughly comparablewith that for the inhibition of $alpha$ 4 $beta$ 2 receptors (Fig. 4 and Table1). There was a tendency for R-( $-$ )-mecamylamine to produce moreinhibition of muscle-type receptors than S-(+)-mecamylamine; howeverthe difference was only significant at the 1 µM concentration(unpaired t test p < 0.05). In contrast to the inhibition of $beta$ subunit-containing neuronal receptors, the inhibition of musclereceptors was fully reversed after a 5-min wash (Fig. 4B).

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Fig. 4. Effect of mecamylamine (Mec) on ACh-evoked currents in oocytes expressing the $alpha$ 1 $beta$ 1 $delta$ $epsilon$ subunits of the adult muscle-type nAChR. A, concentration-response relationship for mecamylamine's inhibition of the peak currents of muscle-type receptors when 30 µM ACh was coapplied with mecamylamine at the indicated concentrations. Data from each oocyte were normalized to that cell's response to 3 µM ACh alone. All cells were pre-equilibrated with mecamylamine at the indicated concentration for 10 s before the coapplication of agonist with antagonist. Each point represents the average normalized response of at least four cells. B, amplitude of 3 µM ACh control responses obtained 5 min after the application of ACh and mecamylamine at the indicated concentrations. In contrast to the residual inhibition seen with neuronal nAChR receptors, the inhibition of muscle-type receptors was essentially fully reversible.

The effects of R-( $-$ )-mecamylamine and S-(+)-mecamylamine were also evaluated on oocytes coexpressing the NMDA receptor subunitsNR1 and NR2b. The NR1 subunit, which is ubiquitous throughoutthe brain, produces robust functional responses when coexpressedwith the NR2b subunit and activated by glutamate and the coagonistglycine (Fig. 5). The NR2b subunit in vivo is selectively presentin the forebrain with high levels of expression in the cerebralcortex and hippocampus, as well as the septum, caudate putamen,and olfactory bulb (Ozawa et al., 1998

), making the combinationof NR2b with NR1 relevant for both cognitive and motor functionsin the central nervous system. As shown in Fig. 5, whereas bothmecamylamine stereoisomers applied at a concentration of 100 µMcould produce a transient inhibition of NMDA receptor responsesto the coapplication of 10 µM glutamate + 10 µM glycine (p < 0.001),this effect was reversible after a 5-min wash. NMDA receptor responsesobtained in the presence of mecamylamine were also analyzed interms of net charge. Analysis of net charge for neuronal nAChRstended to show a somewhat greater effect than analysis of peakcurrent (see below), whereas for NMDA receptors inhibition ofnet charge was no greater than inhibition of peak currents (Fig.5A). The rapid reversibility of mecamylamine block was apparentin the response rebounds seen as mecamylamine was washed fromthe bath (Fig. 5B).

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Fig. 5. NMDA receptors containing NR1 and NR2b subunits. Effect of mecamylamine stereoisomers on NMDA receptor currents. Oocytes expressing NR1 and NR2b subunits were tested for the effects of S-(+)-mecamylamine and R-( $-$ )-mecamylamine at the indicated concentrations. NMDA receptor responses were activated by 10 µM glutamate (glut.) + 10 µM glycine (gly.), and data are normalized to the cells' initial responses to glutamate and glycine. A, solid bars represent the effect of mecamylamine on peak current amplitudes during the coapplication. Open bars represent the net charge calculated during the coapplication response. Hatched bars represent the peak amplitude of control glutamate/glycine responses after a 5-min wash. Data represent the average values for at least four cells under each condition with either S-(+)-mecamylamine (left) or R-( $-$ )-mecamylamine (right). B, raw data from an experiment testing the effect of 100 µM S-(+)-mecamylamine and R-( $-$ )-mecamylamine on NMDAR1 + NMDAR2b receptors. Note the large rebound currents occurring with the washout of mecamylamine, consistent with the relief of open channel block. In order to control for the intrinsic variability of the control responses, statistical analyses were based on t test comparisons between experimental data and repeated glutamate controls (i.e., sequential responses to the applications of 10 µM glutamate + 10 µM glycine). The peak amplitude of the repeated NMDA receptor controls were 0.958 ± 0.062 of the previous control responses, and the area of the repeated NMDA receptor controls were 1.042 ± 0.007 of the previous controls. *p < 0.05, **p < 0.01, and ***p < 0.001. Unmarked bars are not significantly different from corresponding glutamate controls at the 0.05 level.

Recovery Time Course. Since significant residual inhibition was detected after a 5-min washout for all neuronal nAChR other than $alpha$ 7, we conductedrecovery time course experiments in which we obtained an initialinhibition of greater than 50% with the coapplication of 10 µMR-( $-$ )-mecamylamine or S-(+)-mecamylamine and ACh at the controlconcentration (see above), and then followed the recovery of responsewith control ACh applications repeated at 5-min intervals. Asshown in Fig. 6, for $beta$ 2-containing receptors, recovery from mecamylamine-inducedinhibition seemed to follow simple exponential kinetics. For $alpha$ 3 $beta$ 2receptors, both R-( $-$ )-mecamylamine and S-(+)-mecamylamine hadtime constants of recovery of about 33 ± 4 min, which was similarto the time constant of recovery for S-(+)-mecamylamine at $alpha$ 4 $beta$ 2.The $tau$ for R-( $-$ )-mecamylamine on $alpha$ 4 $beta$ 2 receptors was somewhat faster(23 ± 1.2 min). Note that although inhibition of $alpha$ 4 $beta$ 2 receptorsduring the initial coapplication was not significantly differentbetween cells treated with R-( $-$ )-mecamylamine or S-(+)-mecamylamine,at each time point represented in Fig. 6A there was significantlyless residual inhibition for the cells treated with R-( $-$ )-mecamylaminethan with S-(+)-mecamylamine (p < 0.05 at 5 and 25 min, and p< 0.01 at other time points).

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Fig. 6. The recovery of ACh control responses. Cells were monitored for their responses to control applications of ACh at 5-min intervals after 10 µM mecamylamine (Mec) was coapplied with ACh on: A, $alpha$ 4 $beta$ 2 receptors; B, $alpha$ 3 $beta$ 2 receptors; and C, $alpha$ 3 $beta$ 4 receptors. Data from each oocyte were normalized to that cell's response to ACh alone. Each point represents the average normalized response of at least four cells.

In contrast to the $beta$ 2-containing receptors, the recovery of $alpha$ 3 $beta$ 4 receptors did not follow simple exponential kinetics. Thereappeared to be a fast phase over the first 15 min ( $tau$ = 19 ± 3.4min and 12 ± 1.3 min for S-(+)-mecamylamine and R-( $-$ )-mecamylamine,respectively). However, after the first 15 min, no further recoverywas observed. This would suggest that mecamylamine may exert twoqualitatively different forms of inhibition on $alpha$ 3 $beta$ 4receptors.

Competition Studies. To determine whether mecamylamine produced inhibition of neuronal nAChR through a mechanism that is noncompetitive with ACh,we conducted ACh concentration-response studies of $alpha$ 4 $beta$ 2 and $alpha$ 3 $beta$ 4receptors in the absence or presence of either S-(+)-mecamylamineor R-( $-$ )-mecamylamine (Table 2). Data were analyzed both in termsof peak currents and in terms of the net charge during the entireevoked response (see Materials and Methods). Data were normalizedto the peak or net charge of corresponding control ACh responses.As shown in Fig. 7, both forms of analysis indicate that the inhibitionproduced by the mecamylamine stereoisomers was not surmountedby increasing the ACh concentration and that the relative amountof inhibition produced by a fixed concentration of mecamylaminewas relatively constant over a wide range of ACh concentrations.

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TABLE 2
Curve fits from competition experiments (Fig. 7)

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Fig. 7. Competition studies. A, ACh concentration response curves for $alpha$ 4 $beta$ 2 receptors were determined with ACh alone or ACh coapplied with 3 µM S-(+)-mecamylamine or R-( $-$ )-mecamylamine. Data were initially normalized to the 30 µM ACh responses obtained in the same cells and then scaled by the ratio of 30 µM ACh control responses to the maximal ACh responses, obtained with 3 mM ACh. Each point represents the average normalized response of at least four cells. Data in the left plot show the effect of mecamylamine (Mec) on peak currents. Data in the right plot show the effect of mecamylamine on the net charge during a coapplication of ACh and mecamylamine, normalized to the net charge in the responses to ACh alone. B, ACh concentration-response curves for $alpha$ 3 $beta$ 24 receptors were determined with ACh alone or ACh coapplied with 3 µM S-(+)-mecamylamine or R-( $-$ )-mecamylamine. Data were initially normalized to the 100 µM ACh responses obtained in the same cells and then scaled by the ratio of the 100 µM ACh control responses to the maximal ACh responses, obtained with 3 mM ACh. Each point represents the average normalized response of at least four cells. Data in the left plot show the effect of mecamylamine on peak currents. Data in the right plot show the effect of mecamylamine on the net charge during a coapplication of ACh and mecamylamine, normalized to the net charge in the responses to ACh alone.

We also evaluated whether mecamylamine behaved as a partial agonist for the neuronal nAChR subtypes tested. S-(+)-mecamylamineand R-( $-$ )-mecamylamine were applied to receptors over a wide rangeof concentrations (10 nM-100 µM) in the absence of ACh. No agonistactivity was detected within the limits of our systems' sensitivity(approximately 0.1% of the ACh controls, data notshown).

Voltage Dependence of Inhibition. We evaluated the voltage dependence of inhibition by R-( $-$ )-mecamylamine and S-(+)-mecamylamine in coapplication experiments.Specifically, cells were held at either $-$ 40 mV or $-$ 90 mV and testedfor their responses to control concentrations of ACh (see above).After a 5-min wash, mecamylamine was coapplied with ACh. Cellswere then washed for 5 min and tested again for their responseto a second control ACh application. Cells were held at the indicatedholding potential throughout the entire procedure. Through theuse of a coapplication protocol rather than a preincubation procedure(as with the concentration-response curve experiments describedabove), we can evaluate both the voltage dependence of the onsetof inhibition (Fig. 8, t = 0 data) and the voltage dependenceof recovery, presumably representing the off-rates of the drugs(Fig. 8, t = 5 data). Note that the data in Fig. 8 represent theeffects of mecamylamine on amplitude of the peak currents relativeto the amplitude of the peak currents of control applicationsof ACh before mecamylamine was applied. The mecamylamine concentrationstested in these coapplication experiments were 10 µM for $alpha$ 7 receptors,5 µM for $alpha$ 4 $beta$ 2 and $alpha$ 3 $beta$ 2 receptors, and 1 µM for $alpha$ 3 $beta$ 4 receptors.As shown in Fig. 8 (A and B), there was significant voltage dependencefor the off-rate of both R-( $-$ ) and S-(+)-mecamylamine with $alpha$ 4 $beta$ 2and $alpha$ 3 $beta$ 4 receptors (p < 0.01). Significant effects of voltage(p < 0.01) were detected in the t = 0 peak responses only forS-(+)-mecamylamine on $alpha$ 7 (Fig. 8C) and R-( $-$ )-mecamylamine on $alpha$ 3 $beta$ 4(Fig. 8D). With $alpha$ 3 $beta$ 2 receptors, only the off-rate of S-(+)-mecamylamineshowed significant voltage dependence (p < 0.01), although theoff-rate of R-( $-$ )-mecamylamine showed a trend toward significance(p = 0.0505). In general, these results suggest that the bindingsite for mecamylamine may be deep enough into the membrane's electricfield to slow the dissociation of mecamylamine when the cell ishyperpolarized.

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Fig. 8. Voltage dependence of mecamylamine (Mec)-induced inhibition of peak currents. Mecamylamine was coapplied with agonist at either $-$ 40 or $-$ 90 mV. Inhibition was calculated relative to initial control ACh responses and measured during the coapplication (t = 0) or after a 5 min wash (t = 5). Concentrations of mecamylamine used were: A, 5 µM for $alpha$ 4 $beta$ 2 receptors; B, 1 µM for $alpha$ 3 $beta$ 4 receptors; C, 5 µM for $alpha$ 3 $beta$ 2 receptors; and D, 10 µM for $alpha$ 7 receptors. Each point represents measurements from at least four cells. Columns marked with a double asterisk were determined to be significantly different from the corresponding $-$ 40 mV control data at p < 0.01 by unpaired t tests.

The results presented in Fig. 8 suggested relatively little effect of voltage on the inhibition of peak currents by mecamylamine.However, with use-dependent inhibitors, the effect of the drugcan accumulate throughout the period of activation. Therefore,to further investigate the effect of voltage on the onset of inhibitionof neuronal nAChR by mecamylamine, we also analyzed the net chargeassociated with the coapplication of ACh and mecamylamine at differentvoltages. As shown in Fig. 9, when net charge was used as themeasure of receptor response, significant effects of voltage weredetected for the initial inhibition of $alpha$ 4 $beta$ 2 receptors by bothR-( $-$ )-mecamylamine and S-(+)- mecamylamine, for $alpha$ 3 $beta$ 2 receptorsby S-(+)-mecamylamine, and for $alpha$ 3 $beta$ 4 receptors by R-( $-$ )-mecamylamine.

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Fig. 9. Voltage dependence of mecamylamine (Mec)-induced inhibition of net charge during the coapplication of ACh and either S-(+)-mecamylamine or R-( $-$ )-mecamylamine. Mecamylamine was coapplied with agonist at either $-$ 40 or $-$ 90 mV. Inhibition of net charge was calculated relative to the net charge in the initial control ACh responses. Representative traces are shown to the right of the bar graphs. Drug applications were 12 s in duration and correspond to the bars. Note that the rapidly desensitizing $alpha$ 7 receptor-mediated responses are shown at an expanded time scale. In all cases, the response obtained in the presence of mecamylamine is shown as the thin line contained within the thick line that corresponds to the control ACh response obtained 5 min before the ACh/mecamylamine coapplication. The concentrations of mecamylamine used were: A, 5 µM for $alpha$ 4 $beta$ 2 receptors; B, 1 µM for $alpha$ 3 $beta$ 4 receptors; C, 5 µM for $alpha$ 3 $beta$ 2 receptors; and D, 10 µM for $alpha$ 7 receptors. Each point represents measurements from at least four cells. Analysis was conducted on the same responses that were represented in Fig. 8 in terms of peak amplitude. However, more significant effects of voltage were revealed when the data were analyzed in terms of net charge rather than peak currents. Columns marked with a double asterisk were determined to be significantly different from the corresponding $-$ 40 mV control data at p < 0.01 by unpaired t tests.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Most previous in vitro studies investigating mecamylamine's mode of action have found its inhibitory activity to be voltage-dependent,which suggests that it functions as an open channel blocker (Ascheret al., 1979; Varanda et al., 1985; Fieber and Adams, 1991). Thus,mecamylamine is generally thought of as a noncompetitive antagonistproducing inhibition by binding to sites other than the agonistactivation site (Francis and Papke, 1996). However, Ascher etal. (1979) also found that inhibition of parasympathetic gangliaof the rat was lessened when the drug was coapplied at high agonistconcentrations, an observation that is more consistent with acompetitive mechanism of inhibition. Moreover, Bertrand et al.(1990) reported that the inhibitory effects of mecamylamine onheterologously expressed chick $alpha$ 4 $beta$ 2 receptors was voltage independent,yet present only after coapplication with an agonist. Previousresearch by this lab suggests that mecamylamine's inhibition ofrat $alpha$ 3 $beta$ 4 receptors is voltage dependent, which is consistent withopen channel block (Webster et al., 1999). Moreover, analysisof point mutations indicated that residues at the 6' positionwithin the $beta$ subunit TM2 domain may be important for mecamylamine'sinhibitory properties (Webster et al., 1999).

In a recent study investigating the effects of mecamylamine on human AChRs expressed in Xenopus oocytes, Chavez-Noriega etal. (1997) found that a single concentration of mecamylamine (3µM) produced approximately 50% inhibition of $alpha$ 2 $beta$ 2, $alpha$ 4 $beta$ 2, and $alpha$ 7receptors and between 75 and 90% inhibition at $alpha$ 3 $beta$ 4, $alpha$ 3 $beta$ 2, $alpha$ 4 $beta$ 4,and $alpha$ 2 $beta$ 4 receptors. However, these findings were difficult tointerpret since it was not clear which of four possible nicotinicagonists were used for each subunit combination tested, and onlya single concentration of mecamylamine wasinvestigated.

Our results indicate that for $beta$ subunit-containing receptors, the effects of mecamylamine are long-lived and use-dependent.Although the slow reversibility of mecamylamine's effects is mostapparent in our recovery studies, our concentration/response analysesprimarily measure the onset of inhibition over a relatively briefperiod of activation. This implies that our IC₅₀ estimates, whichare based only on a single period of activation during which inhibitionaccumulates, are not likely to reflect equilibrium IC₅₀ valuesthat, if feasible to measure, would be considerably lower. Itmay be the case that previous reports, which have suggested higherpotency for inhibition by mecamylamine, may have been affectedby the accumulation of inhibition with the repeated activationof the receptors. A similar consideration could account for whyour apparent IC₅₀ values for $beta$ subunit-containing neuronal receptorsdo not differ as much as might be expected from the apparent valuesfor muscle-type receptors. Specifically, since the off-rate ofmecamylamine from muscle-type receptors is probably at least 10times faster than for the neuronal $beta$ subunit-containing receptors,our IC₅₀ measurements should approximate the equilibrium IC₅₀values for muscle receptors, while underestimating the equilibriumIC₅₀ of the $beta$ subunit-containing neuronal receptors. Likewise,for the same reason, the rapid reversibility of mecamylamine'sblock of $alpha$ 7 receptors would be consistent with the relativelysmall effects of mecamylamine on neuronal $alpha$ 7-type receptors (Frazieret al., 1998).

In general, previous studies of mecamylamine have used a racemic mixture comprising the optical isomers R-( $-$ )-mecamylamineand S-(+)-mecamylamine hydrochloride. The few previous studiesaimed at investigating the pharmacology of these two isomers havegenerally found little or no difference in potency or efficacy.For example, Stone et al. (1962) compared the effects of S-(+)-mecamylaminehydrochloride with racemic mecamylamine hydrochloride on nicotine-inducedconvulsions and pupil dilation in mice and found essentially nosignificant differences between the two compounds. They concludedthat "optical isomerism does not play a significant role in determiningthe degree of activity". Suchocki et al. (1991) also investigatedthe actions of R-( $-$ )-mecamylamine and S-(+)-mecamylamine hydrochloridein assays measuring nicotine-induced depression of spontaneouslocomotor activity and antinociception. They found that both opticalisomers had similar potency in blocking the antinociception causedby nicotine, whereas the potency of the S-(+)-mecamylamine isomerin blocking the nicotine-induced depression of spontaneous locomotoractivity could not be determined because S-(+)-mecamylamine, likenicotine, also induced depression of spontaneous locomotor activity.Despite some evidence for agonist activity of the S-isomer ofmecamylamine, these investigators also concluded that opticalisomerism does not play a significant role in determining theinhibitory activity of mecamylamine. However, Schoenenberger etal. (1986) reported finding "interesting differences" betweenthe actions of R-( $-$ )-mecamylamine and S-(+)-mecamylamine hydrochloridein assays measuring neuromuscular transmission, but the detailsregarding these differences were not described nor everpublished.

The present findings indicate that while the various neuronal nAChR differ in their sensitivity to inhibition by mecamylamineand its stereoisomers, there seems to be little difference betweenS-(+)-mecamylamine and R-( $-$ )-mecamylamine in terms of IC₅₀ valuesfor a given receptor subtype. However, there appeared to be somesignificant differences in the off-rates for the mecamylamineisomers from the receptors. Specifically, S-(+)-mecamylamine appearsto dissociate more slowly from $alpha$ 4 $beta$ 2 and $alpha$ 3 $beta$ 4 receptors than doesR-( $-$ )-mecamylamine.

Additionally, adult ( $alpha$ 1 $beta$ 1 $delta$ $epsilon$ ) muscle-type receptors appeared to be somewhat more sensitive to R-( $-$ )-mecamylamine than to S-(+)-mecamylamine.This differential sensitivity of muscle receptors to the mecamylaminestereoisomers may have important clinical implications. For example,Tennant et al. (1984) found that "weakness" was one of the mostintolerable side effects of mecamylamine when used as an aid tosmoking cessation. In addition, in a recent double-blind placebo-controlledstudy investigating the safety of mecamylamine as a monotherapyfor the treatment of Tourette's disorder, weakness was the mostcommon adverse experience reported by patients treated with mecamylamine.Patients were asked each week of the 8-week treatment study ifthey felt "fatigue or tiredness" (along with 113 other potentialside effects). Twenty-eight percent (8 of 29) of patients in themecamylamine group experienced this side effect versus 9% (3 of32) in the placebo group (Silver et al., 2000). Taken together,the combination of an increased inhibitory effect on neuronalreceptors and a decreased effect on muscle-type receptors, wouldsuggest that in chronic (i.e., therapeutic) application, S-(+)-mecamylaminemight be preferable to R-( $-$ )-mecamylamine, especially in termsof equilibrium inactivation of neuronal receptors, and with decreasedside effects associated with neuromusculartransmission.

Our competition experiments indicate that the mecamylamine stereoisomers are noncompetitive inhibitors of neuronal nAChR.This is consistent with our data that indicates that the inhibitionproduced by the mecamylamine isomers is voltage dependent, whichis consistent with previous findings from this lab (Webster etal., 1999), as well as others (Ascher et al., 1979; Varanda etal., 1985; Fieber and Adams, 1991; Giniatullin et al., 2000).

Although the kinetics of recovery suggest a single exponential process for $beta$ 2-containing receptors, the inhibition of $alpha$ 3 $beta$ 4receptors seems more complex. Recovery of $alpha$ 3 $beta$ 4 receptors occurredin two phases, one phase of which was too slow to resolve over30 min. This would suggest either multiple sites of action oran inhibition-dependent allosteric conversion of receptors toa long-lived inactivestate.

Our data provide an indication that S-(+)-mecamylamine may be a somewhat more desirable inhibitor of neuronal nAChR than R-( $-$ )-mecamylamine.However, a number of issues deserve further investigation. Recentin vivo studies suggest that mecamylamine has unique pharmacologicaleffects at relatively low doses. For example, low (0.1 mg/kg s.c.),but not higher, doses of mecamylamine were found to attenuatethe plasma corticosterone response to stress in rats (Newman etal., 2000) and improve executive cognitive function in aged primates(Terry et al., 1999). It would therefore be of interest to lookat the effects of mecamylamine and its stereoisomers on neuronalreceptors containing the $alpha$ 5 subunits, because these may bettermodel the properties of some ganglionic and brain-type receptors(Conroy et al., 1992; Vernallis et al., 1993; Conroy and Berg,1998). Additionally, other differences are likely to exist betweenthe receptors expressed in oocytes and those found in vivo, suchas additional complex subunit arrangements, post-translationalmodifications, etc. These factors might also impact the sensitivityof native neuronal receptors tomecamylamine.

Although some previous reports have suggested that mecamylamine's effects in the brain may involve NMDA receptors (O'Delland Christensen, 1988; McDonough and Shih, 1995), our data indicatethat at least for the rat subtype consisting of NR1 and NR2b subunits,inhibitory effects of mecamylamine would be small andtransient.

In conclusion, our results suggest that the new therapeutic potentials that have been proposed to exist for the central nervoussystem $---$ active nicotinic antagonists may be better realized ifwe take advantage of the stereochemistry of mecamylamine to targetmore selectively the nicotinic receptors of the brain. Also, ourstudies of mecamylamine and its stereoisomers illustrate thatthere still may be much to learn from old drugs when we approachthem with modern methodology and the refined perspective of molecularneurobiology.

	Acknowledgments

We thank Julia Porter and Jennifer Kruse for outstanding technical assistance. Clones for the human nicotinic receptor subunitswere kindly provided by Jon Lindstrom, mouse muscle clones wereprovided by Jim Boulter and Paul Gardner, and rat NMDA receptorsubunit clones were provided by Jane Sullivan. The authors arescientific consultants for Layton Bioscience, Inc., and R.D.D.and P.R.S. are coinventors on USF-owned patents (licensed to LaytonBioscience, Inc.) covering the use of mecamylamine stereoisomersfor various neuropsychiatricindications.

	Footnotes

Accepted for publication January 23, 2001.

Received for publication November 9, 2000.

This study was supported by Layton BioScience, Inc., and the USF I-4 CorridorProgram.

Send reprint requests to: Dr. Roger L. Papke, Associate Professor of Pharmacology and Therapeutics, P.O. Box 100267, 1600 S.W. Archer Rd., University of Florida, College of Medicine, Gainesville, FL 32610. E-mail: rpapke{at}college.med.ufl.edu

	Abbreviations

ACh, acetylcholine; nAChR, nicotinic acetylcholine receptor; EC₁₀, EC₁₅, EC₃₀, and EC₅₀, 10%, 15%, 30%, and 50% effective concentrations; IC₅₀, 50% inhibitory concentration; NMDA, N-methyl-D-aspartate.

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