Characterization of Nicotinic Acetylcholine Receptors That Modulate Nicotine-Evoked [3H]Norepinephrine Release from Mouse Hippocampal Synaptosomes

doi:10.1124/mol.106.024513

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First published on May 30, 2006; DOI: 10.1124/mol.106.024513

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Mol Pharmacol 70:967-976, 2006

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Characterization of Nicotinic Acetylcholine Receptors That Modulate Nicotine-Evoked [³H]Norepinephrine Release from Mouse Hippocampal Synaptosomes

Layla Azam, and J. Michael McIntosh

Departments of Biology (L.A., J.M.M.) and Psychiatry (J.M.M.), University of Utah, Salt Lake City, Utah

Received March 15, 2006; accepted May 30, 2006

Abstract

Top
Abstract
Materials and Methods
Results
Discussion
References

Nicotine's modulation of hippocampal noradrenergic neurotransmissionmay contribute to its mnemonic properties, but the nicotinicacetylcholine receptor (nAChR) subtypes that modulate terminalrelease of norepinephrine are unknown. In the present study,we used a number of subtype-selective ${alpha}$ -conotoxins in combinationwith nicotinic receptor subunit-deficient mice to characterizenAChRs that modulate [³H]nore-pinephrine release from synaptosomes.The results indicate that at least two populations of nAChRscontribute to this release: a novel ${alpha}$ 6( ${alpha}$ 4) $beta$ 2 $beta$ 3 $beta$ 4 subtype and an ${alpha}$ 6( ${alpha}$ 4) $beta$ 2 $beta$ 3subtype. These are distinct from subtypes that modulate synaptosomalnorepinephrine release in the rat hippocampus in which an ${alpha}$ 6/ $beta$ 2and/or ${alpha}$ 6/ $beta$ 4 ligand binding interface is not present. Whereas ${alpha}$ -conotoxin MII fully inhibits nicotine-evoked [³H]norepinephrinerelease in mouse, it is ineffective in blocking [³H]norepinephrinerelease in rat. Block of [³H]norepinephrine release by ${alpha}$ -conotoxinBuIA, a toxin that kinetically distinguishes between $beta$ 2- and $beta$ 4-containing nAChRs, was partially reversible in mouse but irreversiblein rat. This indicates that in contrast to rat, mouse nAChRsare made of both $beta$ 4 and non- $beta$ 4-containing populations. Resultsfrom $beta$ 2 and $beta$ 4 null mutant mice confirmed this conclusion, indicatingthe presence of the $beta$ 2 subunit in all nAChRs and the presenceof the $beta$ 4 subunit in a subpopulation of nAChRs. In addition,both ${alpha}$ 4 and $beta$ 3 subunits are essential for the formation of functionalnAChRs on mouse noradrenergic terminals. Cytisine, a ligandformerly believed to be $beta$ 4-selective, was a highly effectiveagonist for ${alpha}$ 6 $beta$ 2-containing nAChRs. The sum of these results suggestsa possible novel nAChR subtype that modulates nor-adrenergicneurotransmission within the mouse hippocampus.

Presynaptic nicotinic acetylcholine receptors (nAChRs) modulaterelease of many neurotransmitters within the central nervoussystem, including dopamine (DA), serotonin, GABA, and norepinephrine(NE) (Wonnacott, 1997

). The nicotinic receptors regulating DArelease from striatal terminals have been extensively characterizedin both rats and mice. In both species, at least two types ofnAChR subtypes have been identified based on sensitivity to ${alpha}$ -conotoxin (CTX) MII (Kulak et al., 1997

; Grady et al., 2002

)and ${alpha}$ -CTX PIA (Azam and McIntosh, 2005

). Knockout studies haveshown that both subtypes require the $beta$ 2 subunit, because nicotine-evoked[³H]DA release is completely abolished in $beta$ 2-null mutant mice(Grady et al., 2001

; Salminen et al., 2004

). Knockout and immunoprecipitationstudies have identified at least four different subtypes onthe DAergic terminals: ${alpha}$ 6 $beta$ 2 $beta$ 3, ${alpha}$ 6 ${alpha}$ 4 $beta$ 2 $beta$ 3, ${alpha}$ 4 $beta$ 2, and ${alpha}$ 4 ${alpha}$ 5 $beta$ 2 (Zoli et al.,2002

; Champtiaux et al., 2003

In contrast to the striatal DAergic system, there are limiteddata on nicotinic regulation of hippocampal noradrenergic neurotransmissionin rats (Sacaan et al., 1996; Sershen et al., 1997; Fu et al.,1998) and a lack of data in mice. Nicotinestimulated [³H]NErelease from rat hippocampal synaptosomes is insensitive toblock by ${alpha}$ -CTX MII and partially blocked by the ${alpha}$ 3 $beta$ 4-selective ${alpha}$ -CTX AuIB (Kulak et al., 1997; Luo et al., 1998). The rat locusceruleus (LC), which provides the sole noradrenergic projectionto the hippocampus, expresses a variety of nAChR subunits, including ${alpha}$ 3- ${alpha}$ 7 and $beta$ 2- $beta$ 4 (Winzer-Serhan and Leslie, 1997; Lena et al., 1999;Vincler and Eisenach, 2003). Besides ${alpha}$ 3 $beta$ 4, the involvement ofother nAChR subtype(s) in nicotine-stimulated [³H]NE releasefrom rat hippocampal synaptosomes remains unknown.

Several novel nAChR subtype-selective ${alpha}$ -conotoxins have recentlybeen discovered, including ${alpha}$ -CTX PIA and ${alpha}$ -CTX BuIA (Dowell etal., 2003; Azam et al., 2005). ${alpha}$ -CTX PIA has been used in thecharacterization of nAChRs that regulate [³H]DA release fromstriatal synaptosomes and confirmed a role for ${alpha}$ 6-containingsubtypes (Azam and McIntosh, 2005). ${alpha}$ -CTX BuIA can kineticallydistinguish between $beta$ 2- and $beta$ 4-containing nAChRs (Azam et al.,2005). In the present study, we used these toxins in combinationwith subunit null-mutant mice to characterize murine nAChRsthat modulate [³H]NE release. To our knowledge, this is thefirst pharmacological characterization of nAChRs on mouse hippocampalnoradrenergic terminals. The results indicate that at leasttwo different nAChR subtypes are involved. In addition, thereare substantial species differences between mice and rats inboth the pharmacology and developmental regulation of nAChRsubtypes that modulate hippocampal [³H]NE release.

Materials and Methods

Top
Abstract
Materials and Methods
Results
Discussion
References

Materials. The chemicals were obtained from the following sources:(-)nicotine hydrogen tartrate, pargyline HCl, bovine serum albumin,ascorbic acid, and nisoxetine HCl were from Sigma (St. Louis,MO); [³H]NE (L-[ring-2,5,6-³H]norepinephrine; 52-53 Ci/mmol)was from PerkinElmer Life and Analytical Sciences (Boston, MA);and Ecolume scintillation cocktail was from MP Biomedicals (Irvine,CA). ${alpha}$ -Conotoxins were synthesized as described previously (Cartieret al., 1996; McIntosh et al., 2004; Azam et al., 2005).

Tissue Preparation. Adult male Sprague-Dawley rats (SimonsenLaboratories, Gilroy, CA) were kept two per cage on a 12:12-hlight/dark cycle, with food and water available ad libitum.Male and female Sprague-Dawley rat pups (2-3 weeks old) werekept in the cage with the dam, and both sexes were used forthe experiments. C57BL/6J wild-type and null mutant mice thatwere bred onto C57BL/6J background were provided by The Institutefor Behavioral Genetics (University of Colorado, Boulder, CO)and were used by permission from Dr. Arthur Beaudet (BaylorCollege of Medicine, Baylor, TX). The breeding triads (two femalerats, one male rat) were kept in the same cage and were allowedto mate. Only the first-generation pups for each genotype wereused for the experiments. For each experiment, hippocampi from2 adult male rats between 60 and 90 days old, 6 postnatal ratsbetween 14 to 21 days old, or 2 to 3 adult male mice or 4 to6 mice pups (male and female) between 14 and 20 days old wereused. The animals were decapitated, and brains were removedquickly. This procedure was approved by the Institutional AnimalCare and Use Committee and is consistent with federal guidelines.Synaptosomes were prepared as described by Azam and McIntosh(2005). In brief, the hippocampus was quickly dissected on iceand placed in ice-cold 0.32 M sucrose buffer, pH 7.4 to 7.5.The dissected hippocampus was homogenized by 14 gentle up anddown strokes, followed by centrifugation at 1000g for 10 minat 4°C. The supernatant was centrifuged at 12,000g for 20min at 4°C. The resulting P2 pellet was resuspended in 2ml of Krebs-HEPES buffer (superfusion buffer) with compositionof 128 mM NaCl, 2.4 mM KCl, 1.2 mM KH₂PO₄, 0.6 mM MgSO₄, 3.2mM CaCl₂, 25 mM HEPES, 10 mM glucose, and supplemented with1 mM ascorbic acid, 0.1 mM pargyline, and 0.1 mg/ml bovine serumalbumin. The synaptosomes were incubated for 10 min at 37°Cto equilibrate with the superfusion buffer, followed by another10-min incubation with 0.13 µM [³H]NE (specific activity,52-53 Ci/mmol) at 37°C. For the experiment determining uptakespecificity, 0.6 µM nisoxetine HCl was present in thebuffer throughout the preincubation and incubation periods.The synaptosomes were centrifuged at 3500 rpm for 5 min to getrid of excess radiolabeled NE. The pellet was resuspended in4 ml of superfusion buffer, and 1 ml was transferred into eachof four conical tubes containing 3 ml of superfusion bufferand subsequently loaded into the superfusion chambers containing13-mm diameter A/E glass fiber filters (Gelman Sciences, AnnArbor, MI). One tube of the final synaptosomal preparation (4ml total volume) contained enough synaptosomes for six chambersof the superfusion apparatus.

Superfusion. The superfusion system had 12 identical channelsand was set up as described in Kulak et al. (1997), except theperistaltic pumps were switched to Brandel pumps. Once synaptosomeswere loaded into the superfusion apparatus, they were washedfor 20 min with either superfusion buffer alone or buffer plusvarying concentrations of the toxins at a rate of 0.5 ml/min.For studies in which the reversibility of ${alpha}$ -CTX BuIA or ${alpha}$ -CTXAuIB was examined, synaptosomes were first perfused with buffercontaining toxin for 20 min and subsequently perfused for anadditional 10 or 20 min with toxin-free buffer. After the washperiod, 2-min fractions were collected in 6-ml polypropylenevials containing 4 ml of Ecolume scintillation cocktail. Atthe end of the third 2-min fraction, a 1-min pulse of nicotine,nicotine plus toxin, cytisine, or cytisine plus toxin was applied,followed by a 10-min wash with superfusion buffer alone. Inexperiments examining the reversibility of toxins, no toxinwas present when the nicotine or cytisine pulse was appliedafter the toxin washout period. At the end of the superfusion,filters containing the synaptosomes were taken out and placeddirectly in vials containing 4 ml of Ecolume to determine total[³H]NE uptake. Radioactivity collected in each fraction wasquantitated by liquid scintillation spectroscopy with a Beckman5801 liquid scintillation counter (tritium efficiency, approximately50%).

Data Analysis. Throughout this article, tritium release is presumedto correspond directly to amounts of radiolabeled transmitterrelease, as it has been shown previously that tritium releasedby nAChR agonists is proportional to total radiolabeled transmitterreleased (Rapier et al., 1988).

To account for experimental variations in tissue amount, releasewas calculated relative to the baseline. Baseline release wasdetermined as the average of two fractions before (fractions2 and 3) and two fractions after (fractions 6 and 7) the peakrelease (fractions 4 and 5). Average baseline was subtractedfrom the evoked release and the resulting values divided bythe baseline to yield the evoked release as a percentage overbaseline. The percentage release above baseline in fractions4 and 5 were then added together to yield total evoked release(or area under the curve). Because the total [³H]NE uptake amongchambers within each experiment was very consistent (less than10% deviation), it was assumed that a similar amount of tissuewas loaded into each chamber. For all data, except those inFig. 1B, the percentage release over baseline was normalizedto average release by 100 µM nicotine (or cytisine incase of Fig. 9) alone or to release by 100 µM nicotinein wild-type mice, as indicated. The IC₅₀ value for ${alpha}$ -CTX BuIAinhibition was determined by nonlinear regression analysis usingPrism (GraphPad Software Inc., San Diego, CA). All statisticalanalysis was performed with Prism. Toxin effects were analyzedby one-way analysis of variance, followed by Dunnett's posthoc test for comparisons with nicotine control.

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Fig. 1. Total [³H]NE uptake and release profile in adult and postnatal rat and mouse. A, total synaptosomal [³H]NE uptake, shown as counts per minute (CPM), is similar in postnatal mouse and rat and adult mouse but significantly higher in adult rat. ^*, p < 0.05, Dunnett's post hoc test with adult rat as control. Values are mean ± S.E.M. from three experiments. B, representative nicotine-evoked [³H]NE release profile from hippocampal synaptosomes of rat and mouse. Adult and postnatal (2-3 weeks old) rats display similar [³H]NE release above baseline in response to 100 µM nicotine. In contrast, although postnatal (2-3 weeks old) mice show nicotine-evoked [³H]NE release, adult mice do not display significant release above baseline. Values are averages from three experiments. Nic, nicotine.

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Fig. 9. Cytisine (Cyt) stimulation of [³H]NE release from WT and $beta$ 4-/- mouse hippocampal synaptosomes. Percentage of release above baseline is normalized to 100 µM cytisine control (100%). A, ${alpha}$ -BuIA blocks cytisine-stimulated release in WT mouse by more than 80%; however, this block, although still significant, is mostly reversed after a 20-min toxin washout period. B, ${alpha}$ -BuIA inhibits cytisine-stimulated [³H]NE release in $beta$ 4-/- mouse, but its block is fully reversed after a 20-min washout. ^*, p < 0.05; ^***, p < 0.001, significantly different from 100 µM cytisine control, Dunnett's post hoc test. Values are mean ± S.E.M. from three experiments.

	Results

Top Abstract Materials and Methods Results Discussion References

Uptake Specificity. The total [³H]NE uptake into hippocampalsynaptosomes prepared from mouse and rat hippocampus is shownin Fig. 1A. Tissue from postnatal rat and mouse and adult mousedisplayed similar [³H]NE uptake. Synaptosomes from adult rat,however, displayed significantly higher [³H]NE uptake (^*p <0.05, Dunnett's post hoc test with adult rat as control). Todetermine the extent of [³H]NE uptake into non-noradrenergicterminals within the mouse hippocampus, the synaptosomes wereexposed to 0.6 µM nisoxetine, a potent and specific inhibitorof the NE transporter, before incubation with radiolabeled neurotransmitter.Similar to rat hippocampal synaptosomes (Barik and Wonnacott,2006

), total [³H]NE uptake into synaptosomes prepared from mousehippocampus was reduced by 80 ± 1.1%, suggesting thatthe majority of radiolabeled NE is taken up by noradrenergicterminals. In addition, 100 µM nicotine stimulated only9.3 ± 4.2% [³H]NE release above baseline from synaptosomesexposed to 0.6 µM nisoxetine, suggesting that almost allof radiolabeled NE release from mouse hippocampal synaptosomesoccurs from noradrenergic terminals.

Figure 1B shows a representative profile of nicotine-evoked[³H]NE release in adult and postnatal rats and mice. Adult andpostnatal rats exhibited similar [³H]NE release above baselineupon stimulation by 100 µM nicotine, despite the lowertotal [³H]NE uptake in postnatal rats (Fig. 1A). Postnatal mouseexhibited lower nicotine-evoked [³H]NE release than did ratat the same age. Adult mouse exhibited a comparatively low levelof nicotine-evoked [³H]NE release, despite similar total [³H]NEuptake to both postnatal mouse and rat (Fig. 1, A and B). Whencalculated as the area under the curve, adult and postnatalrats exhibited 199 ± 16% and 215 ± 39% [³H]NErelease above baseline, respectively, and adult and postnatalmice release was 20 ± 2.2% and 78 ± 4.5% abovebaseline, respectively (p < 0.001, postnatal mouse releasesignificantly different from adult mouse, Student's t test).

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Fig. 2. Concentration-response curve of ${alpha}$ -CTX BuIA inhibition of nicotine-stimulated [³H]NE release from adult rat hippocampal synaptosomes. Percentage of release above baseline is normalized to 100 µM nicotine control (100%). Inhibition by ${alpha}$ -CTX BuIA is significant at concentrations $≥$ 10 nM and complete at 1 µM. The IC₅₀ value for inhibition is 88 nM (confidence interval, 57-136 nM) with a Hill coefficient of 1.1 ± 0.23. ^***, p < 0.001, Dunnett's post hoc test with 100 µM nicotine alone as control. Values are mean ± S.E.M. from at least three experiments.

The $beta$ 4 Subunit Is Implicated in All of the nAChRs that Modulate[³H]NE Release from Adult Rat Hippocampal Synaptosomes. To furtherassess the contribution of the $beta$ 4 subunit to nicotinic modulationof [³H]NE release from the adult rat hippocampus, we took advantageof a novel ${alpha}$ -conotoxin, ${alpha}$ -CTX BuIA, that kinetically distinguishesbetween $beta$ 2^* (^* indicates the presence of other subunits) and $beta$ 4^* nAChRs. Block of rat, human, and mouse nAChRs by this toxinis rapidly reversed in subtypes that have an ${alpha}$ x/ $beta$ 2 interface (t_1/2for recovery from block <1.5 min for all except ${alpha}$ 6 $beta$ 2 $beta$ 3, wheret_1/2 ${approx}$ 10 min); in contrast, its block is very slowly reversedin nAChRs containing an ${alpha}$ x/ $beta$ 4 interface (t_1/2 > 30 min) (Azamet al., 2005

). ${alpha}$ -CTX BuIA dose-dependently inhibited [³H]NE releasefrom adult rat hippocampal synaptosomes evoked by 100 µMnicotine, with an IC₅₀ value of 88 nM (95% confidence interval,57-136 nM) and Hill slope of 1.1 ± 0.23. At a concentrationof 1 µM, ${alpha}$ -CTX BuIA completely inhibited nicotine-evoked[³H]NE release (Fig. 2). The reversibility of toxin inhibitionwas next examined. After superfusing the synaptosomes with ${alpha}$ -CTXBuIA for 20 min, the synaptosomes were washed with toxinfreebuffer. As shown in Fig. 3A, even after a 20-min wash with toxin-freebuffer, nicotine-evoked [³H]NE release did not recover fromthe level of initial toxin block. To ascertain that the lackof reversibility was a true toxin-dependent effect rather thanan artifact of the experimental procedure, the reversibilityof the block by ${alpha}$ -CTX AuIB was also examined. ${alpha}$ -CTX AuIB blocks ${alpha}$ 3 $beta$ 4 nAChRs more potently than ${alpha}$ 6 $beta$ 4 nAChRs, with IC₅₀ values of0.5 ± 0.14 µM and >5 µM, respectively(5 µM toxin blocks rat ${alpha}$ 6 $beta$ 4 nAChRs expressed in Xenopuslaevis oocytes by 35.6 ± 2.7%, n = 5). Toxin block israpidly reversed for both subtypes (t_1/2 < 1.5 min) (Luoet al., 1998

; L. Azam, unpublished observations). ${alpha}$ -CTX AuIB(5 µM) blocked nicotine-evoked [³H]NE release from adultrat hippocampal synaptosomes by $~$ 50%. A 10-min wash with toxin-freebuffer was sufficient to completely reverse the partial inhibitionof nicotine-evoked [³H]NE release by ${alpha}$ -CTX AuIB (Fig. 3B).

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Fig. 3. Reversibility of ${alpha}$ -CTX BuIA and ${alpha}$ -CTX AuIB block of nicotine-evoked [³H]NE release from adult rat hippocampal synaptosomes. Percentage of release above baseline is normalized to 100 µM nicotine control (100%). A, ${alpha}$ -CTX BuIA (100 nM and 1 µM) inhibition of nicotine-stimulated [³H]NE is not reversed after a 10- or 20-min wash with toxin-free buffer. The "control" bars represent release in presence of the toxin without a toxin-free wash. B, ${alpha}$ -CTX AuIB blocks nicotine-evoked [³H]NE release from adult rat hippocampal synaptosomes by 50%, but in contrast to ${alpha}$ -CTX BuIA, the block is completely reversed after a 10-min wash with toxin-free buffer. ^***, p < 0.001, significantly different from 100 µM nicotine control, Dunnett's post hoc test. Values are mean ± S.E.M. from at least three experiments. Nic, nicotine.

Nicotinic-Receptor Modulation of [³H]NE Release in C57BL/6JMice Is Developmentally Regulated. As discussed above, in adultrat hippocampal synaptosomes, nicotine maximally evoked [³H]NErelease at 200% above baseline. In contrast, in adult C57BL/6Jmouse synaptosomes, 100 µM nicotine only stimulated [³H]NErelease at 20 ± 2.2% above baseline, with no additionalrelease at 300 µM nicotine. However, a 1-min pulse of25 mM K⁺ stimulated [³H]NE release at 528 ± 10.3% abovebaseline, indicating that the hippocampal terminals of adultmice have the exocytotic machinery required for neurotransmitterrelease. The lower level of nicotine evoked [³H]NE release inadult mouse was not further investigated.

In contrast to adult mouse, 2- to 3-week-old pups displayedsignificantly higher nicotine-evoked [³H]NE release (Fig. 1B).Nicotine (100 µM) stimulated [³H]NE release at 78 ±4.5% above baseline, with no additional release observed at300 µM nicotine. Therefore, the pharmacological characterizationof nicotine-evoked [³H]NE release in both wild-type (WT) andnull mutant mice was carried out during the second to thirdpostnatal week at a nicotine concentration of 100 µM.Thus, the results drawn from these studies do not necessarilyapply to adult mouse.

Nicotine Modulation of [³H]NE Release from Postnatal C57BL/6JWT Mouse Hippocampal Synaptosomes Is Mediated by a Mixed Populationof $beta$ 2- and $beta$ 4-Containing nAChRs. Similar to adult rat, 1 µM ${alpha}$ -CTX BuIA almost completely inhibited [³H]NE release from 2-to 3-week-old WT mouse hippocampal synaptosomes. However, incontrast to adult rat (where inhibition was pseudoirreversible),the inhibition by ${alpha}$ -CTX BuIA was partially reversed after toxinwashout (Fig. 4A), suggesting the presence of both $beta$ 2 (without $beta$ 4) and $beta$ 4-containing nAChRs.

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Fig. 4. ${alpha}$ -CTX BuIA inhibition of nicotine-evoked [³H]NE release from postnatal mouse and rat hippocampal synaptosomes. Percentage of release above baseline is normalized to 100 µM nicotine control (100%). A, 1 µM ${alpha}$ -CTX BuIA blocks [³H]NE release from mouse hippocampal synaptosomes, and its block is partially reversed after 10- and 20-min washes with toxin-free buffer. B, 1 µM ${alpha}$ -BuIA almost completely blocks nicotine-evoked [³H]NE release from postnatal rat hippocampal synaptosomes, but its block is not reversed, even after a 20-min wash with toxin-free buffer. ^***, p < 0.001, significantly different from 100 µM nicotine control, Dunnett's post hoc test. Values are mean ± S.E.M. from at least three experiments. Nic, nicotine.

To further characterize the identity of the nAChR subtypes thatregulate [³H]NE release from postnatal WT mouse hippocampalsynaptosomes, release was examined in the presence of threesubtype-selective ${alpha}$ -conotoxins: ${alpha}$ -CTX MII (selective for ${alpha}$ 3 $beta$ 2, ${alpha}$ 6 $beta$ 2^*,and ${alpha}$ 6 $beta$ 4 nAChRs) (Cartier et al., 1996

; Vailati et al., 1999

;Champtiaux et al., 2002

), ${alpha}$ -CTX PIA (selective for ${alpha}$ 6 $beta$ 2^* and ${alpha}$ 6 $beta$ 4nAChRs) (Dowell et al., 2003

), and ${alpha}$ -CTX AuIB [selective for ${alpha}$ 3 $beta$ 4 (Luo et al., 1998

) > ${alpha}$ 6 $beta$ 4]. In contrast to adult rat, where ${alpha}$ -CTX MII does not inhibit [³H]NE release (Kulak et al., 1997

;Luo et al., 1998

), 100 nM ${alpha}$ -CTX MII almost completely blockednicotine-evoked [³H]NE release from postnatal mouse hippocampalsynaptosomes (Fig. 5A). ${alpha}$ -CTX PIA (10 nM), a concentration thatblocks ${alpha}$ 6 $beta$ 2^* nAChRs by $~$ 85% and blocks ${alpha}$ 6 $beta$ 4 nAChRs by $~$ 20%, but onlyblocks ${alpha}$ 3 $beta$ 2by $~$ 10% (Dowell et al., 2003

), inhibited nicotine-evoked[³H]NE release by 80 ± 9.4% (Fig. 5A). ${alpha}$ -CTX AuIB, at5 µM, blocked nicotine-evoked [³H]NE release by 14 ±3.8% (Fig. 5A). Because the ${alpha}$ -CTX AuIB-sensitive fraction wasquantitatively similar to the ${alpha}$ -CTX PIA-insensitive release,both toxins were coapplied to determine whether the ${alpha}$ -CTX PIA-insensitivecomponent could be eliminated by ${alpha}$ -CTX AuIB. Coapplication of10 nM ${alpha}$ -CTX PIA and 5 µM ${alpha}$ -CTX AuIB did not produce a greaterinhibition than that seen with 10 nM ${alpha}$ -CTX PIA alone (Fig. 5A).

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Fig. 5. Effect of selective antagonists on nicotine-evoked [³H]NE release from WT postnatal mouse and postnatal rat hippocampal synaptosomes. Percentage of release above baseline is normalized to 100 µM nicotine control (100%). A, ${alpha}$ -CTX MII completely blocks nicotine-evoked [³H]NE release from postnatal mouse hippocampal synaptosomes, whereas ${alpha}$ -CTX PIA blocks release by $~$ 80%. ${alpha}$ -CTX AuIB blocks release by only approximately 15%. Coapplication of ${alpha}$ -CTX PIA and ${alpha}$ -CTX AuIB does not produce a greater inhibition than ${alpha}$ -CTX PIA alone. B, ${alpha}$ -CTX MII is ineffective in blocking nicotine-evoked [³H]NE release from postnatal rat hippocampal synaptosomes, whereas ${alpha}$ -CTX PIA significantly potentiates release. ${alpha}$ -CTX AuIB blocks release by $~$ 30%. ^*, p < 0.05; ^***, p < 0.001, significantly different from 100 µM nicotine control, Dunnett's post hoc test. Values are mean ± S.E.M. from at least three experiments.

To ascertain whether the difference in the pharmacology of nicotinicregulation of [³H]NE release between mice and rats was due toage differences, nicotine-evoked [³H]NE release was examinedin 2- to 3-week-old rat pups. Similar to adult rats, 1 µMBuIA almost completely and irreversibly inhibited nicotine-evoked[³H]NE release from postnatal rat hippocampal synaptosomes (Fig. 4B). ${alpha}$ -CTX MII (100 nM) was ineffective in blocking nicotine-evoked[³H]NE release from hippocampal synaptosomes of rat pups (Fig. 5B)in contrast to the complete block in postnatal mice (Fig. 5A). ${alpha}$ -CTX AuIB (5 µM) partially but significantly blocked [³H]NErelease. We were surprised to find that 10 nM ${alpha}$ -CTX PIA potentiated[³H]NE release (Fig. 5B). This was not further investigated.

The ${alpha}$ 4, $beta$ 2, and $beta$ 3 Subunits Are Critical Components of nAChRs thatModulate [³H]NE Release from Postnatal C57BL/6J Mouse HippocampalSynaptosomes. To further elucidate the role of the differentsubunits in nAChRs that modulate [³H]NE release from postnatalmouse hippocampal terminals, mutant mice lacking a specificnAChR subunit were examined for nicotine modulation of hippocampal[³H]NE release. Nicotine-evoked [³H]NE release was abolishedin $beta$ 2-null mutant mice ( $beta$ 2-/-) and significantly decreased in ${alpha}$ 4-/- and $beta$ 3-/- mice (Fig. 6). It is interesting that nicotine-evoked[³H]NE release in $beta$ 4-/- pups was similar to the level in theWT (Fig. 6), despite the fact that the partial reversibilityof ${alpha}$ -CTX BuIA indicated the presence of the $beta$ 4 subunit in a subpopulationof nAChRs that modulate [³H]NE release in WT pups (see above).However, ${alpha}$ -CTX BuIA block was fully reversed in $beta$ 4-/- pups (Fig. 7B),suggesting the presence of the $beta$ 2 subunit in all nAChRs. In addition, ${alpha}$ -CTX AuIB failed to block [³H]NE release in $beta$ 4-/- mice (Fig. 7A),consistent with ${alpha}$ -CTX AuIB being inactive on $beta$ 2-containing nAChRs(Luo et al., 1998).

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Fig. 6. Nicotine-evoked [³H]NE release from hippocampal synaptosomes of WT (+/+) and nAChR subunit null-mutant mice. Percentage of release above baseline is normalized to release by 100 µM nicotine in WT mice (100%). $beta$ 4-/- mice show the same amount of [³H]NE release as the WT mice. However, release is abolished in hippocampal synaptosomes of $beta$ 2-/- mice, whereas it is significantly reduced in ${alpha}$ 4-/- and $beta$ 3-/- mice. ^***, p < 0.001 Dunnett's post hoc test, with WT release as control. Values are mean ± S.E.M. from at least three experiments.

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Fig. 7. Effect of selective antagonists on nicotine-evoked [³H]NE release from postnatal $beta$ 4-/- mouse hippocampal synaptosomes. Percentage of release above baseline is normalized to 100 µM nicotine control (100%). A, both ${alpha}$ -CTX MII and ${alpha}$ -CTX PIA inhibit nicotine-evoked [³H]NE release, whereas ${alpha}$ -CTX AuIB is ineffective in inhibiting this release. B, ${alpha}$ -CTX BuIA block of nicotine-evoked [³H]NE release from $beta$ 4-/- mouse hippocampal synaptosomes is almost completely reversed after 10- and 20-min washes with toxin-free buffer. ^***, p < 0.001, Dunnett's post hoc test with 100 µM nicotine alone as control. Values are mean ± S.E.M. from three experiments. Nic, nicotine.

Nicotine-evoked [³H]NE release was pharmacologically examinedin synaptosomes from mouse pups that lack either the ${alpha}$ 4orthe $beta$ 3 subunit. In ${alpha}$ 4-/- pups, release was decreased by almost 80%relative to the WT (Fig. 6, 8A), suggesting that the ${alpha}$ 4 subunitis present in a large proportion of functional nAChRs on hippocampalterminals. The residual release in these animals was completelyblocked by ${alpha}$ -CTX MII and ${alpha}$ -CTX BuIA and blocked approximately76% by ${alpha}$ -CTX PIA (Fig. 8A). In the $beta$ 3-/- pups, [³H]NE releasewas decreased by almost 90% relative to the WT. The residualrelease was not sensitive to any of the ${alpha}$ -CTXs (Fig. 8B).

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Fig. 8. Effect of ${alpha}$ -CTX MII, ${alpha}$ -CTX PIA, and ${alpha}$ -CTX BuIA on nicotine-evoked [³H]NE release from hippocampal synaptosomes of ${alpha}$ 4-/- and $beta$ 3-/- postnatal mice. Percentage of release above baseline is normalized to release by 100 µM nicotine in WT mice (100%). A, ${alpha}$ -CTX MII and ${alpha}$ -CTX BuIA completely inhibit the residual [³H]NE release in ${alpha}$ 4-/-mice. Although ${alpha}$ -PIA inhibits the release by $~$ 80%, this inhibition does not reach significance. B, nicotine-evoked [³H]NE release is almost completely abolished in $beta$ 3-/- mice. The residual release is not sensitive to block by any of the toxins. Values are mean ± S.E.M. from three experiments. Nic, nicotine.

We also examined whether the developmental decline in nicotine-evoked[³H]NE release observed in WT mice also occurs in $beta$ 4-/- mice.Similar to WT mouse, $beta$ 4-/- adult mouse displayed only 16.9 ±10.5% release above baseline in response to 100 µM nicotine,with no additional release (16.6 ± 4%) at 300 µMnicotine. Cytisine Is an Efficacious Agonist at $beta$ 2-Containing

nAChRs Present on Mouse Noradrenergic Terminals.Cytisine isa nAChR agonist formerly reported to be highly efficacious at $beta$ 4-containing nAChRs (Luetje and Patrick, 1991; Chavez-Noriegaet al., 1997; Colquhoun and Patrick, 1997) but only poorly efficaciousat $beta$ 2-containing nAChRs (Papke and Heinemann, 1994). In WT mousehippocampal synaptosomes, 100 µM cytisine was 90 ±6% as efficacious as nicotine in stimulating [³H]NE release. ${alpha}$ -CTX BuIA almost completely inhibited cytisine-stimulated [³H]NErelease in WT mouse, and this block was reversed by 80.5 ±3.4% after a 20-min wash with toxin-free buffer (Fig. 9A), suggestingthe involvement of mostly $beta$ 2-containing nAChRs. The high efficacyof cytisine at $beta$ 2-containing nAChRs was further confirmed in $beta$ 4-/- mice. In these mice, 100 µM cytisine was 82 ±6% as efficacious as nicotine in stimulating [³H]NE release.This release was almost completely blocked by 1 µM ${alpha}$ -CTXBuIA, and the block was fully reversed after a 20-min wash withtoxin-free buffer (Fig. 9B).

Discussion

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Abstract
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In this study, we used a combination of novel subtype-selectiveligands and nAChR subunit knockout mice to examine the molecularcomposition of nAChRs that modulate hippocampal [³H]NE release.To our knowledge, this is the first report to examine nicotine-evoked[³H]NE release in mouse hippocampus. The data indicate speciesdifferences in both the developmental and pharmacological profilesof nAChRs in mouse versus rat. Although nicotine-evoked [³H]NErelease during the second to third postnatal week is similarto adult levels in rats (Leslie et al., 2002; current study),NE release decreases with age in mice. A first major pharmacologicaldifference between the two species is that mouse nAChRs arepotently blocked by ${alpha}$ 6^*-selective antagonists, whereas rat nAChRsare not. Second, in addition to a population of $beta$ 2- and $beta$ 4-containingnAChRs, there is a separate subpopulation of only $beta$ 2-containingnAChRs on mouse noradrenergic terminals, whereas in the rat,all nAChRs seem to contain a $beta$ 4 subunit. The results from thepresent study are summarized in Table 1.

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TABLE 1 Composition of nAChR subtypes expressed on hippocampal noradrenergic terminals of rat and mouse

For each subtype, the percentage contributing to NE release has been determined from the portion of the release that is sensitive to the particular subtype-selective ${alpha}$ -conotoxin.

nAChRs on Rat Hippocampal Noradrenergic Terminals. Previouswork identified a subpopulation of ${alpha}$ 3 $beta$ 4-like nAChRs in nicotine-evoked[³H]NE release from adult rat hippocampal synaptosomes (Clarkeand Reuben, 1996; Luo et al., 1998). In the present study, itwas shown that the $beta$ 4 subunit is present in most, if not all,nAChRs that modulate nicotine-evoked [³H]NE release in bothadult and postnatal rats, as evidenced by the pseudoirreversibleblock by ${alpha}$ -CTX BuIA. In addition, there is an absence of nAChRsthat have an ${alpha}$ 6/ $beta$ xor ${alpha}$ 3/ $beta$ 2 subunit interface in both developmentaltime points, as evidenced by the lack of block by ${alpha}$ -CTX MII (Kulaket al., 1997; Luo et al., 1998). The partial block by 5 µM ${alpha}$ -CTX AuIB indicates the presence of a population of ${alpha}$ 3 $beta$ 4^* and/or ${alpha}$ 6 $beta$ 4^* nAChRs. However, lack of block by ${alpha}$ -CTX MII excludes the ${alpha}$ 6 $beta$ 4^* subtype. This is in contrast to LC nAChRs that modulateadult rat hippocampal NE release. Microinjection of ${alpha}$ -CTX MIIand ${alpha}$ -CTX AuIB into the LC blocks hippocampal NE release by 67and 44%, respectively. Coadministration of the two toxins doesnot produce a greater inhibition than ${alpha}$ -CTX MII, suggesting thepresence of nAChRs with both the $beta$ 2 and the $beta$ 4 subunits (Fu etal., 1999). The greater inhibition by ${alpha}$ -CTX MII suggests thepossible presence of additional ${alpha}$ 3 $beta$ 2^* and/or ${alpha}$ 6 $beta$ 2^* subtype(s), without $beta$ 4, that are not sensitive to block by ${alpha}$ -CTX AuIB. The presentfindings, together with those of Fu et al. (1999), indicatethat systemic nicotine stimulates hippocampal NE release bytargeting different subtypes of nAChRs that are present in ratLC and on rat hippocampal NE terminals.

Possible candidates for the ${alpha}$ -CTX AuIB-resistant nAChRs on rathippocampal noradrenergic terminals are those that contain an ${alpha}$ 4/ $beta$ 4 or ${alpha}$ 2/ $beta$ 4 interface. However, in light of the absence of ${alpha}$ 2mRNA in both postnatal and adult LC (Lena et al., 1999; Vinclerand Eisenach, 2003), the ${alpha}$ 2 $beta$ 4^* subtype can be excluded. The ${alpha}$ 4subunit mRNA and protein have been detected in the rat LC (Lenaet al., 1999; Vincler and Eisenach, 2003). The $beta$ 2 subunit mayalso be present on the terminals, but the irreversible blockby ${alpha}$ -CTX BuIA suggests that any $beta$ 2-containing nAChRs must alsocontain a $beta$ 4 subunit at the other ligand binding interface. Thepresence of the putative structural subunits ${alpha}$ 5 and $beta$ 3 in thesenAChRs is also a possibility, especially because the mRNA forboth subunits has been detected in the LC (Lena et al., 1999).

nAChRs on Mouse Hippocampal Noradrenergic Terminals. We wereable to perform much more detailed studies in the mouse hippocampusbecause of the availability of nAChR subunit-deficient mice.In contrast to postnatal and adult rats, results from the nullmutant mice indicated that all nAChRs that regulate nicotine-evoked[³H]NE release contain a $beta$ 2 subunit. A large proportion of thesenAChRs also contain the $beta$ 3 and/or the ${alpha}$ 4 subunits (Table 1). InWT mice, partial reversibility of block by ${alpha}$ -CTX BuIA indicatedthe presence of both $beta$ 4^* and $beta$ 2^*(without $beta$ 4) nAChR subtypes. The $beta$ 2 subunit, however, seemed to be able to compensate for the $beta$ 4 subunit in $beta$ 4-/- mice, as evidenced by the lack of a decreasein the total amount of [³H]NE release, lack of effect of ${alpha}$ -CTXAuIB, and, most notably, the complete reversibility of ${alpha}$ -CTXBuIA inhibition.

In WT mice, block of [³H]NE release by the ${alpha}$ 6 $beta$ x/ ${alpha}$ 3 $beta$ 2-selective ${alpha}$ -CTXMII and the ${alpha}$ 6 $beta$ x selective ${alpha}$ -CTX PIA indicated that most, if notall, receptors also contain an ${alpha}$ 6 subunit. The lack of coadditivityof inhibition by 10 nM ${alpha}$ -CTX PIA and 5 µM ${alpha}$ -CTX AuIB suggestsa common site of action, possibly the ${alpha}$ 6 $beta$ 4^* rather than an ${alpha}$ 3 $beta$ 4^*subtype. However, the presence of a small population of ${alpha}$ 6( ${alpha}$ 3) $beta$ 4^*subtype that is sensitive to block by both ${alpha}$ -CTX AuIB and ${alpha}$ -CTXPIA cannot be ruled out. This is in contrast to the rat, whereapproximately half of nicotine-evoked [³H]NE release is modulatedby ${alpha}$ 3 $beta$ 4^* but not ${alpha}$ 6 $beta$ 4^* or ${alpha}$ 6 ${alpha}$ 3 $beta$ 4^* nAChRs (Luo et al., 1998).

To further investigate the pharmacology of nAChRs on mouse noradrenergicterminals, cytisine, a ligand formerly believed to only activate $beta$ 4-containing nAChRs with high efficacy (Luetje and Patrick,1991; Chavez-Noriega et al., 1997; Colquhoun and Patrick, 1997),was used. More recent studies, however, have shown that cytisinebinds to ${alpha}$ -CTX MII-sensitive sites, although with low affinity(Whiteaker et al., 2000). In addition, one study has demonstratedthat cytisine is as efficacious as nicotine and acetylcholinein activating ${alpha}$ -CTX MII-sensitive nAChRs that modulate [³H]DArelease from mouse striatal synaptosomes (Salminen et al., 2004).Similar to the latter study, in the present study, cytisinewas nearly as efficacious as nicotine in stimulating [³H]NErelease from WT hippocampal synaptosomes. In addition, cytisinewas also effective in stimulating [³H]NE release from hippocampalsynaptosomes of $beta$ 4-/- mice, where all of the nAChRs contain the ${alpha}$ 6 $beta$ 2 interface and are ${alpha}$ -CTX MII-sensitive. These results confirmthat cytisine is a highly efficacious agonist at the ${alpha}$ 6 $beta$ 2^* nAChRspresent on mouse noradrenergic terminals.

Nicotine-evoked [³H]NE release was significantly reduced inmice lacking the ${alpha}$ 4 subunit, suggesting that along with the $beta$ 2subunit, the ${alpha}$ 4 subunit is a critical component of the majorityof nAChRs that stimulate [³H]NE release in postnatal mouse hippocampus.The residual release in ${alpha}$ 4-/- mice is abolished by 100 nM ${alpha}$ -CTXMII and by $~$ 80% by 10 nM ${alpha}$ -CTX PIA. This suggests that the smallresidual release in ${alpha}$ 4-/- mice may be mediated by a populationof ${alpha}$ 6 $beta$ 2 $beta$ 3( $beta$ 4) receptors that is still functional in the absenceof the ${alpha}$ 4 subunit.

Deletion of the $beta$ 3 subunit largely eliminates nicotineevoked[³H]NE release from mouse hippocampal synaptosomes. This resultsuggests that almost all of the nAChRs on mouse noradrenergicterminals contain a $beta$ 3 subunit. It has been shown that the ${alpha}$ -CTXMII-sensitive component of nicotine-evoked [³H]DA release fromstriatal synaptosomes is substantially reduced in $beta$ 3-/- adultmice (Cui et al., 2003; Salminen et al., 2004). In light ofthe finding that nicotine-evoked [³H]NE release from hippocampusof mouse pups was completely ${alpha}$ -CTX MII-sensitive (current study),the loss of the [³H]NE release in $beta$ 3-/- is consistent with theidea that this subunit is a critical component of native ${alpha}$ -CTXMII-sensitive nAChRs that modulate catecholamine release inthe central nervous system. It has recently been shown thatthe deletion of the $beta$ 3 subunit decreases the number of ${alpha}$ 6-containingnAChRs on mouse DAergic terminals (Gotti et al., 2005), indicatingthat ${alpha}$ 6 and $beta$ 3 subunits coparticipate in the formation of nativenAChRs.

Additional Implications. NE is a neurotransmitter that is importantfor attentiveness, working memory, and learning. Compounds thatenhance memory also increase the release of NE within the hippocampus(Lee et al., 1993; Lee and Ma, 1995). The cognitive-enhancingproperties of nicotine may, in part, be mediated by the releaseof NE within the hippocampus. SIB-1553A, a nicotinic receptorligand with selectivity for $beta$ 4-containing nAChRs, improves attentionand working memory in both rats and mice (Bontempi et al., 2001,2003; Terry et al., 2002). The beneficial effects of SIB-1553Aon working memory/attention may be mediated, in part, by releaseof acetylcholine (Bontempi et al., 2001; Rao et al., 2003b)and/or NE within the hippocampus (Rao et al., 2003a). The resultsof the present study, which indicate the presence of the $beta$ 4 subunitin nAChRs that modulate [³H]NE release in both rat and mousehippocampus, provide additional support for the latter.

In addition to its role as a neurotransmitter, NE acts as aneurotrophic factor in the immature central nervous system,regulating cell proliferation, differentiation, and synaptogenesis.In the rat cerebellum, another late-maturing structure, nicotine-evoked[³H]NE release is significantly higher during the second tothird postnatal week compared with the adult, similar to thesituation observed in the present study for the mouse hippocampus(O'Leary and Leslie, 2003). The authors attributed the transient[³H]NE release to key developmental events occurring duringthe period of observed peak release. It is possible that similardevelopmental events also occur in the mouse hippocampus duringthe postnatal period when nicotine-evoked [³H]NE release isobserved.

Acknowledgements

We thank Dr. Arthur Beaudet at Baylor College of Medicine (Houston,TX) for permission to use the null mutant mice, Natalie Meinerzat IBG (University of Colorado, Boulder, CO) for providing uswith the wild-type and null mutant C57BL/6J mice, and TracyDelVelcchio at IBG for the genotyping.

Footnotes

This work was supported by National Institutes of Health grantDA016835 (to L.A.), DA015663 (Institute for Behavioral Genetics),and MH53631 (to J.M.M.).

This work was previously presented in part at the 2003 Societyfor Neuroscience Annual Meeting, Program 248.12; Nov 8-12, 2003;New Orleans, LA.

ABBREVIATIONS: nAChR, nicotinic acetylcholine receptor; CTX,conotoxin; DA, dopamine; LC, locus wild-type.

Address correspondence to: Dr. Layla Azam, Department of Biology, University of Utah, 257 S 1400 E, Salt Lake City, UT 84112. E-mail: layla_azam{at}yahoo.com

References

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Abstract
Materials and Methods
Results
Discussion
References

Azam L, Dowell C, Watkins M, Stitzel JA, Olivera BM, and McIntosh JM (2005) Alpha-conotoxin BuIA, a novel peptide from Conus bullatus, distinguishes among neuronal nicotinic acetylcholine receptors. J Biol Chem 280: 80-87.[Abstract/Free Full Text]

Azam L and McIntosh JM (2005) Effect of novel ${alpha}$ -conotoxins on nicotine-stimulated [³H]dopamine release from rat striatal synaptosomes. J Pharmacol Exp Ther 312: 231-237.[Abstract/Free Full Text]

Barik J and Wonnacott S (2006) Indirect modulation by ${alpha}$ 7 nicotinic acetylcholine receptors of noradrenaline release in rat hippocampal slices: interaction with glutamate and GABA systems and effect of nicotine withdrawal. Mol Pharmacol 69: 618-628.[Abstract/Free Full Text]

Bontempi B, Whelan KT, Risbrough VB, Lloyd GK, and Menzaghi F (2003) Cognitive enhancing properties and tolerability of cholinergic agents in mice: a comparative study of nicotine, donepezil, and SIB-1553A, a subtype-selective ligand for nicotinic acetylcholine receptors. Neuropsychopharmacology 28: 1235-1246.[CrossRef][Medline]

Bontempi B, Whelan KT, Risbrough VB, Rao TS, Buccafusco JJ, Lloyd GK, and Menzaghi F (2001) SIB-1553A, (±)-4-[[2-(1-methyl-2-pyrrolidinyl)ethyl]thio]phenol hydrochloride, a subtype-selective ligand for nicotinic acetylcholine receptors with putative cognitive-enhancing properties: effects on working and reference memory performances in aged rodents and nonhuman primates. J Pharmacol Exp Ther 299: 297-306.[Abstract/Free Full Text]

Cartier GE, Yoshikami D, Gray WR, Luo S, Olivera BM, and McIntosh JM (1996) A new ${alpha}$ -conotoxin which targets ${alpha}$ 3 $beta$ 2 nicotinic acetylcholine receptors. J Biol Chem 271: 7522-7528.[Abstract/Free Full Text]

Champtiaux N, Gotti C, Cordero-Erausquin M, David DJ, Przybylski C, Lena C, Clementi F, Moretti M, Rossi FM, Le Novere N, et al. (2003) Subunit composition of functional nicotinic receptors in dopaminergic neurons investigated with knockout mice. J Neurosci 23: 7820-7829.[Abstract/Free Full Text]

Champtiaux N, Han ZY, Bessis A, Rossi FM, Zoli M, Marubio L, McIntosh JM, and Changeux JP (2002) Distribution and pharmacology of alpha 6-containing nicotinic acetylcholine receptors analyzed with mutant mice. J Neurosci 22: 1208-1217.[Abstract/Free Full Text]

Chavez-Noriega LE, Crona JH, Washburn MS, Urrutia A, Elliott KJ, and Johnson EC (1997) Pharmacological characterization of recombinant human neuronal nicotinic acetylcholine receptors h ${alpha}$ 2 $beta$ 2, h ${alpha}$ 2 $beta$ 4, h ${alpha}$ 3 $beta$ 2, h ${alpha}$ 3 $beta$ 4, h ${alpha}$ 4 $beta$ 2, h ${alpha}$ 4 $beta$ 4 and h ${alpha}$ 7 expressed in Xenopus oocytes. J Pharmacol Exp Ther 280: 346-356.[Abstract/Free Full Text]

Clarke PB and Reuben M (1996) Release of [³H]-noradrenaline from rat hippocampal synaptosomes by nicotine: mediation by different nicotinic receptor subtypes from striatal [³H]-dopamine release. Br J Pharmacol 117: 595-606.[Medline]

Colquhoun LM and Patrick JW (1997) Alpha3, beta2, and beta4 form heterotrimeric neuronal nicotinic acetylcholine receptors in Xenopus oocytes. J Neurochem 69: 2355-2362.[Medline]

Cui C, Booker TK, Allen RS, Grady SR, Whiteaker P, Marks MJ, Salminen O, Tritto T, Butt CM, Allen WR, et al. (2003) The beta3 nicotinic receptor subunit: a component of alpha-conotoxin MII-binding nicotinic acetylcholine receptors that modulate dopamine release and related behaviors. J Neurosci 23: 11045-11053.[Abstract/Free Full Text]

Dowell C, Olivera BM, Garrett JE, Staheli ST, Watkins M, Kuryatov A, Yoshikami D, Lindstrom JM, and McIntosh JM (2003) Alpha-conotoxin PIA is selective for alpha6 subunit-containing nicotinic acetylcholine receptors. J Neurosci 23: 8445-8452.[Abstract/Free Full Text]

Fu Y, Matta SG, James TJ, and Sharp BM (1998) Nicotine-induced norepinephrine release in the rat amygdala and hippocampus is mediated through brainstem nicotinic cholinergic receptors. J Pharmacol Exp Ther 284: 1188-1196.[Abstract/Free Full Text]

Fu Y, Matta SG, McIntosh JM, and Sharp BM (1999) Inhibition of nicotine-induced hippocampal norepinephrine release in rats by alpha-conotoxins MII and AuIB microinjected into the locus coeruleus. Neurosci Lett 266: 113-116.[CrossRef][Medline]

Gotti C, Moretti M, Clementi F, Riganti L, McIntosh JM, Collins AC, Marks MJ, and Whiteaker P (2005) Expression of nigrostriatal ${alpha}$ 6-containing nicotinic acetylcholine receptors is selectively reduced, but not eliminated, by $beta$ 3 subunit gene deletion. Mol Pharmacol 67: 2007-2015.[Abstract/Free Full Text]

Grady SR, Meinerz NM, Cao J, Reynolds AM, Picciotto MR, Changeux JP, McIntosh JM, Marks MJ, and Collins AC (2001) Nicotinic agonists stimulate acetylcholine release from mouse interpeduncular nucleus: a function mediated by a different nAChR than dopamine release from striatum. J Neurochem 76: 258-268.[CrossRef][Medline]

Grady SR, Murphy KL, Cao J, Marks MJ, McIntosh JM, and Collins AC (2002) Characterization of nicotinic agonist-induced [³H]dopamine release from synaptosomes prepared from four mouse brain regions. J Pharmacol Exp Ther 301: 651-660.[Abstract/Free Full Text]

Kulak JM, Nguyen TA, Olivera BM, and McIntosh JM (1997) Alpha-conotoxin MII blocks nicotine-stimulated dopamine release in rat striatal synaptosomes. J Neurosci 17: 5263-5270.[Abstract/Free Full Text]

Lee EH, Lee CP, Wang HI, and Lin WR (1993) Hippocampal CRF, NE, and NMDA system interactions in memory processing in the rat. Synapse 14: 144-153.[CrossRef][Medline]

Lee EH and Ma YL (1995) Amphetamine enhances memory retention and facilitates norepinephrine release from the hippocampus in rats. Brain Res Bull 37: 411-416.[CrossRef][Medline]

Lena C, de Kerchove D'Exaerde A, Cordero-Erausquin M, Le Novere N, del Mar Arroyo-Jimenez M, and Changeux JP (1999) Diversity and distribution of nicotinic acetylcholine receptors in the locus ceruleus neurons. Proc Natl Acad Sci USA 96: 12126-12131.[Abstract/Free Full Text]

Leslie FM, Gallardo KA, and Park MK (2002) Nicotinic acetylcholine receptor-mediated release of [³H]norepinephrine from developing and adult rat hippocampus: direct and indirect mechanisms. Neuropharmacology 42: 653-661.[CrossRef][Medline]

Luetje CW and Patrick J (1991) Both alpha- and beta-subunits contribute to the agonist sensitivity of neuronal nicotinic acetylcholine receptors. J Neurosci 11: 837-845.[Abstract]

Luo S, Kulak JM, Cartier GE, Jacobsen RB, Yoshikami D, Olivera BM, and McIntosh JM (1998) Alpha-conotoxin AuIB selectively blocks alpha3 beta4 nicotinic acetyl-choline receptors and nicotine-evoked norepinephrine release. J Neurosci 18: 8571-8579.[Abstract/Free Full Text]

McIntosh JM, Azam L, Staheli S, Dowell C, Lindstrom JM, Kuryatov A, Garrett JE, Marks MJ, and Whiteaker P (2004) Analogs of ${alpha}$ -conotoxin MII are selective for ${alpha}$ 6-containing nicotinic acetylcholine receptors. Mol Pharmacol 65: 944-952.[Abstract/Free Full Text]

O'Leary KT and Leslie FM (2003) Developmental regulation of nicotinic acetylcholine receptor-mediated [³H]norepinephrine release from rat cerebellum. J Neurochem 84: 952-959.[CrossRef][Medline]

Papke RL and Heinemann SF (1994) Partial agonist properties of cytisine on neuronal nicotinic receptors containing the $beta$ 2 subunit. Mol Pharmacol 45: 142-149.[Abstract]

Rao TS, Adams PB, Correa LD, Santori EM, Sacaan AI, Reid RT, Suto CM, and Vernier JM (2003a) In vitro pharmacological characterization of (±)-4-[2-(1-methyl-2-pyrrolidinyl)ethyl]thio]phenol hydrochloride (SIB-1553A), a nicotinic acetylcholine receptor ligand. Brain Res 981: 85-98.[CrossRef][Medline]

Rao TS, Reid RT, Correa LD, Santori EM, Gardner MF, Sacaan AI, Lorrain D, and Vernier JM (2003b) In vivo pharmacological characterization of (±)-4-[2-(1-methyl-2-pyrrolidinyl)ethyl]thiophenol hydrochloride (SIB-1553A), a novel cholinergic ligand: microdialysis studies. Brain Res 986: 71-81.[CrossRef][Medline]

Rapier C, Lunt GG, and Wonnacott S (1988) Stereoselective nicotine-induced release of dopamine from striatal synaptosomes: concentration dependence and repetitive stimulation. J Neurochem 50: 1123-1130.[Medline]

Sacaan AI, Menzaghi F, Dunlop JL, Correa LD, Whelan KT, and Lloyd GK (1996) Epibatidine: a nicotinic acetylcholine receptor agonist releases monoaminergic neurotransmitters: in vitro and in vivo evidence in rats. J Pharmacol Exp Ther 276: 509-515.[Abstract/Free Full Text]

Salminen O, Murphy KL, McIntosh JM, Drago J, Marks MJ, Collins AC, and Grady SR (2004) Subunit composition and pharmacology of two classes of striatal pre-synaptic nicotinic acetylcholine receptors mediating dopamine release in mice. Mol Pharmacol 65: 1526-1535.[Abstract/Free Full Text]

Sershen H, Balla A, Lajtha A, and Vizi ES (1997) Characterization of nicotinic receptors involved in the release of noradrenaline from the hippocampus. Neuroscience 77: 121-130.[CrossRef][Medline]

Terry AV Jr, Risbrough VB, Buccafusco JJ, and Menzaghi F (2002) Effects of (±)-4-[[2-(1-methyl-2-pyrrolidinyl)ethyl]thio]phenol hydrochloride (SIB-1553A), a selective ligand for nicotinic acetylcholine receptors, in tests of visual attention and distractibility in rats and monkeys. J Pharmacol Exp Ther 301: 284-292.[Abstract/Free Full Text]

Vailati S, Hanke W, Bejan A, Barabino B, Longhi R, Balestra B, Moretti M, Clementi F, and Gotti C (1999) Functional ${alpha}$ 6-containing nicotinic receptors are present in chick retina. Mol Pharmacol 56: 11-19.[Abstract/Free Full Text]

Vincler MA and Eisenach JC (2003) Immunocytochemical localization of the alpha3, alpha4, alpha5, alpha7, beta2, beta3 and beta4 nicotinic acetylcholine receptor subunits in the locus coeruleus of the rat. Brain Res 974: 25-36.[CrossRef][Medline]

Whiteaker P, McIntosh JM, Luo S, Collins AC, and Marks MJ (2000) ¹²⁵I- ${alpha}$ -conotoxin MII identifies a novel nicotinic acetylcholine receptor population in mouse brain. Mol Pharmacol 57: 913-925.[Abstract/Free Full Text]

Winzer-Serhan UH and Leslie FM (1997) Codistribution of nicotinic acetylcholine receptor subunit alpha3 and beta4 mRNAs during rat brain development. J Comp Neurol 386: 540-554.[CrossRef][Medline]

Wonnacott S (1997) Presynaptic nicotinic ACh receptors. Trends Neurosci 20: 92-98.[CrossRef][Medline]

Zoli M, Moretti M, Zanardi A, McIntosh JM, Clementi F, and Gotti C (2002) Identification of the nicotinic receptor subtypes expressed on dopaminergic terminals in the rat striatum. J Neurosci 22: 8785-8789.[Abstract/Free Full Text]