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NEUROPHARMACOLOGY
-Amino-3-hydroxy-5-methyl-4-isoxazole Propionate (AMPA)/Kainate Glutamate Receptors Regulate the Deficit in Brain Reward Function Associated with Nicotine Withdrawal in Rats
Department of Neuropharmacology, The Scripps Research Institute, La Jolla, California (P.J.K., A.M.); and Nervous System Research, Novartis Biomedical Institutes, Basel, Switzerland (F.G.)
Received March 25, 2003; accepted May 16, 2003.
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Abstract |
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 Top Abstract Materials and MethodsResultsDiscussionReferences |
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-amino-3-hydroxy-5-methyl-4-isoxazole
propionate (AMPA)/kainate receptor antagonist
2,3-dihydroxy-6-nitro-7-sulfamoylbenzo(f)quinoxaline (NBQX; 0.01-1
mg/kg) precipitated withdrawal-like threshold elevations in nicotine-dependent
but not control rats, whereas 6-methyl-2-[phenylethynyl]-pyridine (MPEP;
0.01-3 mg/kg) and dizocilpine (MK-801; 0.01-0.2 mg/kg), antagonists at
metabotropic glutamate 5 and N-methyl-D-aspartate
receptors, respectively, did not. Overall, these data demonstrate that mGluII
receptors play an important role in the reward deficits associated with
nicotine withdrawal. Furthermore, it is likely that mGluII receptors generate
this reward deficit, at least in part, by decreasing glutamate transmission at
AMPA/kainate receptors.
; Kenny and Markou,
2001). Nicotine withdrawal was shown to precipitate a deficit in
brain reward function, as measured by elevations in intracranial
self-stimulation (ICSS) reward thresholds, similar to that observed in rats
undergoing withdrawal from other major drugs of abuse
(Epping-Jordan et al., 1998).
Moreover, avoidance and alleviation of this deficit in brain reward function
has been proposed as a major motivational factor contributing to craving,
relapse, and continued tobacco consumption in human smokers
(Epping-Jordan et al., 1998;
Kenny and Markou, 2001). In
contrast to the intense investigations into the mechanisms by which acute
nicotine produces its rewarding effects, little is known concerning the
mechanisms mediating the reward deficits associated with nicotine
withdrawal.
Most drugs of abuse have been shown to stimulate excitatory glutamatergic
transmission throughout brain reward circuitries
(Kalivas and Duffy, 1998;
Wolf et al., 2000). Increases
in glutamatergic transmission have been shown to play an important role in
mediating the positive reinforcing actions of addictive drugs
(Harris and Aston-Jones,
2003). Indeed, it is thought that nicotine elicits its rewarding
actions, at least in part, by activating nicotinic acetylcholine receptors
located on glutamate terminals in the ventral tegmental area (VTA), thereby
potentiating excitatory glutamatergic transmission in this reward-relevant
brain site and increasing mesoaccumbal dopamine transmission
(Mansvelder and McGehee,
2000). Accordingly, blockade of glutamatergic transmission reduced
nicotine's stimulatory action on mesoaccumbens dopamine transmission
(Schilstrom et al., 1998) and
attenuated the rewarding actions of nicotine and other drugs of abuse
(Chiamulera et al., 2001;
Laviolette and van der Kooy,
2003; Paterson et al.,
2003).
It has been suggested that the neuroadaptations that occur during prolonged
exposure to drugs of abuse, which give rise to the deficits in brain reward
function associated with withdrawal, may reside in the same neural elements
that mediate the acute rewarding actions of these drugs
(Koob and Le Moal, 2001).
Indeed, in contrast to nicotine's acute stimulatory effects, nicotine
withdrawal attenuated mesoaccumbens dopamine transmission
(Hildebrand et al., 1997), an
action likely to contribute to the reward and motivational deficits associated
with nicotine withdrawal (Kenny and
Markou, 2001). Therefore, because increases in excitatory
glutamatergic transmission are believed to play an important role in the
reinforcing actions of acute nicotine, we hypothesized that withdrawal from
nicotine is associated with decreased glutamatergic transmission in brain
reward circuitries, which contributes to the reward deficits observed during
withdrawal. To test this hypothesis, the effects of a group II metabotropic
glutamate (mGluII) receptor agonist were examined in nicotine-treated and
control rats. mGluII receptors, comprising of mGlu2 and mGlu3 receptors, are
inhibitory autoreceptors located on glutamate terminals throughout the
mesocorticolimbic system, where they act to decrease excitatory glutamatergic
transmission (Bonci et al.,
1997; Wigmore and Lacey,
1998). Because mGluII receptor agonists decrease glutamatergic
transmission in brain reward circuitries
(Manzoni and Williams, 1999),
we predicted that activation of these receptors would precipitate ICSS
threshold elevations in nicotine-dependent rats similar to those observed in
rats during spontaneous nicotine withdrawal, whereas blockade of these
receptors would reverse the threshold elevations associated with spontaneous
nicotine withdrawal. To further investigate the role of glutamatergic
transmission in nicotine withdrawal, we also examined whether direct blockade
of glutamatergic transmission at postsynaptic NMDA, AMPA/kainate, and
metabotropic glutamate 5 (mGlu5) receptors precipitated withdrawal-like ICSS
threshold elevations in nicotine-dependent rats.
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Materials and Methods |
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TopAbstractMaterials and MethodsResultsDiscussionReferences |
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Drugs. (-)-Nicotine hydrogen tartrate salt ([-]-1-methyl-2-[3-pyridyl] pyrrolidine) and dizocilpine ([+]-MK-801 hydrogen maleate; [(5R,10S)-(+)-5-methyl-10,11-dihydro-5H-dibenzo(a,d)cyclohepten-5,10-imine hydrogen maleate]) were purchased from Sigma-Aldrich (St. Louis, MO); LY341495 (2S-2-amino-2-[1S,2S-2-carboxycyclopropan-1-yl]-3-[xanth-9-yl]propionic acid) and NBQX disodium (2,3-dihydroxy-6-nitro-7-sulfamoylbenzo(f)quinoxaline disodium) were purchased from Tocris Cookson (Ballwin, MO). LY314582 (the racemic mixture of LY354740 [(+)-2-aminobicyclo(3.1.0)hexane-2,6-dicarboxylic acid]) and 6-methyl-2-[phenylethynyl]-pyridine (MPEP) were synthesized by one of the coauthors (F. Gasparini). Drugs were prepared immediately before each administration. For systemic administration, all drugs were dissolved in sterile water and administered by intraperitoneal injection, in a volume of 1 ml/kg body weight, 30 min before the experimental session. For direct intra-VTA administration, LY314582 was dissolved in artificial cerebrospinal fluid of the following composition: 126.6 mM NaCl, 27.4 mM NaHCO3, 2.4 mM KCl, 0.5 mM KH2PO4, 0.89 mM CaCl2, 0.8 mM MgCl2, 0.48 mM Na2HPO4 and 7.1 mM glucose, pH 7.4. Rats received intra-VTA injections immediately before the initiation of the experimental session. Unless otherwise stated, drug doses refer to the salt form.
Apparatus. Intracranial self-stimulation training and testing took
place in 16 Plexiglas operant chambers (25 x 31 x 24 cm) (MED
Associates, St. Albans, VT). The floors of the operant chambers were
constructed of parallel aluminum rods spaced 1.25 cm apart. One wall contained
a metal wheel manipulandum that required 0.2 N force to rotate it one-quarter
of a turn. The wheel (5 cm in width) extended out of the wall 
3 cm. Each
testing chamber was enclosed within a light- and sound-attenuated chamber (62
x 63 x 43 cm). Intracranial stimulation was delivered by constant
current stimulators (Stimtech model 1200; San Diego Instruments, San Diego,
CA). Subjects were connected to the stimulation circuit through flexible
bipolar leads (Plastics One, Roanoke, VA) attached to gold-contact swivel
commutators (model SL2C; Plastics One) mounted above the chamber. The
stimulation parameters, data collection, and all test session functions were
controlled by a microcomputer.
Placement of Electrodes and Cannulas. Rats were anesthetized by
inhalation of 1 to 3% halothane in oxygen and positioned in a stereotaxic
frame (Kopf Instruments, Tujunga, CA). The incisor bar was adjusted to 5 mm
above the interaural line, and the skull exposed. Stainless steel bipolar
electrodes (11 mm in length) were implanted into the posterior lateral
hypothalamus (AP -0.5 mm from bregma; ML ±1.7 mm; DV 8.3 mm from dura),
according to the atlas of Pellegrino et al.
(1979). For the VTA infusion
experiment, bilateral stainless steel guide cannulas (23-gauge, 14 mm in
length) were implanted 3 mm above the VTA (AP -3.2 mm from bregma; ML
±1.7 mm; DV 5.3 mm from skull surface; angle of 10° from midline),
at the same time that ICSS electrodes were implanted. Four indentations were
made in the skull to accommodate screws that together with the application of
dental acrylic, held the electrode and cannulas in place. Cannulas were kept
patent using 14-mm-long stainless steel stylets (30-gauge). Animals were
allowed to recover from surgery for at least 7 days before training in the
ICSS paradigm.
Osmotic Mini-Pump Surgery. Rats were anesthetized by inhalation of 1
to 3% halothane in oxygen and prepared with Alzet osmotic mini-pumps [model
2ML4 (28 day); Alza, Palo Alto, CA] placed subcutaneously (back of the animal
parallel to the spine). Pumps were filled with either sterile water or
nicotine salt solution. The concentration of the nicotine salt solution was
adjusted according to animal body weight, resulting in delivery of 9 mg/kg/day
(3.16 mg/kg, free base). This dose of nicotine maintains stable plasma levels
(44 ng/ml) comparable with those obtained in human smokers consuming
approximately 30 cigarettes per day
(Benowitz, 1988). After
mini-pump implantation (or removal), the surgical wound was closed with 9-mm
stainless steel wound clips (BD Biosciences Primary Care Diagnostics, Sparks,
MD) and treated with topical antibiotic (Bacitracin) ointment.
ICSS Reward Threshold Procedure. Animals were trained to respond
according to a modification of the discrete-trial current-threshold procedure
of Kornetsky and Esposito
(1979). Briefly, a trial was
initiated by the delivery of a noncontingent electrical stimulus. This
electrical reinforcer had a train duration of 500 ms and consisted of 0.1-ms
rectangular cathodal pulses that were delivered at a frequency of 50 to 100
Hz. The frequency of the stimulation was selected for individual animals so
that current-intensity thresholds of each subject were within 85 to 160 µA,
and thus allowed both threshold elevations and lowerings to be detected. This
frequency was held constant throughout the experiment. A one-quarter turn of
the wheel manipulandum within 7.5 s of the delivery of the noncontingent
electrical stimulation resulted in the delivery of an electrical stimulus
identical in all parameters to the noncontingent stimulus that initiated the
trial. After a variable intertrial interval (7.5-12.5 s, average of 10 s),
another trial was initiated with the delivery of a noncontingent electrical
stimulus. Failure to respond to the noncontingent stimulus within 7.5 s
resulted in the onset of the intertrial interval. Responding during the
intertrial interval delayed the onset of the next trial by 12.5 s. Current
levels were varied in alternating descending and ascending series. A set of
three trials was presented for each current intensity. Current intensities
were altered in 5-µA steps. In each testing session, four alternating
descending and ascending series were presented. The threshold for each series
was defined as the midpoint between two consecutive current intensities that
yielded "positive scores" (animals responded for at least two of
the three trials) and two consecutive current intensities that yielded
"negative scores" (animals did not respond for two or more of the
three trials). The overall threshold of the session was defined as the mean of
the thresholds for the four individual series. Each testing session was
30 min in duration. The time between the onset of the noncontingent
stimulus and a positive response was recorded as the response latency. The
response latency for each test session was defined as the mean response
latency of all trials during which a positive response occurred. After
establishment of stable ICSS reward thresholds, rats were tested in the ICSS
procedure once daily except for the spontaneous nicotine withdrawal experiment
when rats were tested at time points according to the experimental design.
Intracerebral Injection Procedure. All injections were administered bilaterally in a volume of 0.5 µl/side given over 66 s through 17-mm injectors. The injectors were connected to calibrated polyethylene-10 tubing preloaded with drug solution and protruded 3 mm below the ends of the cannulas into the VTA. After infusion, the injectors were kept in place for an additional 60 s to allow for drug diffusion and to minimize diffusion along the injection tract when pulling out the injector. Injectors were then removed and replaced with 14-mm wire stylets, and the animals were placed directly into the ICSS testing apparatus. Injections were made using a microinfusion pump (model 975; Harvard Apparatus Inc., Holliston, MA).
Systemic Drug Administration Experiments. These experiments
investigated whether nicotine withdrawal, as measured by elevations in ICSS
thresholds, could be precipitated in nicotine-treated rats by systemic
administration of an agonist at mGluII receptors (LY314582), or antagonists at
mGlu5 (MPEP), NMDA (dizocilpine), or AMPA/kainate (NBQX) glutamate receptors.
For each drug tested, rats were trained in the ICSS paradigm until stable
baseline responding was achieved, defined as 
10% variation in thresholds
for three consecutive days and requiring approximately 14 days of daily
testing. In each case, drug-naïve rats were then assigned to two separate
groups such that there was no difference in mean baseline ICSS thresholds or
body weight between groups. One group was then prepared with subcutaneous
osmotic mini-pumps delivering vehicle and the second group with mini-pumps
delivering 9 mg/kg/day nicotine hydrogen tartrate (3.16 mg/kg/day nicotine
free base). There was a minimum 7-day interval after mini-pump implantation,
during which ICSS reward thresholds continued to be measured daily, before the
effect of any systemically administered drug on reward thresholds was
evaluated. This time period was sufficient to produce robust elevations in
thresholds in nicotine-treated but not vehicle-treated rats upon abrupt
removal of mini-pumps (i.e., spontaneous withdrawal) or administration of
nicotinic receptor antagonists (i.e., precipitated withdrawal;
Epping-Jordan et al., 1998).
Separate groups of nicotine-treated rats and their corresponding
nicotine-naive control group were then injected intraperitoneally with the
mGluII receptor agonist LY314582 (0, 2.5, 0.5, and 7.5 mg/kg; n = 9
nicotine, n = 11 control), the mGlu5 receptor antagonist MPEP (0,
0.01, 0.05, and 0.1 mg/kg; n = 8 nicotine, n = 7 vehicle or
0, 0.5, 1, 2, and 3 mg/kg; n = 13 nicotine, n = 13 vehicle),
the NMDA receptor antagonist dizocilpine (0, 0.01, 0.05, 0.1, 0.175, and 0.2
mg/kg; n = 10 nicotine, n = 9 control), or the AMPA/kainate
receptor antagonist NBQX (0, 0.01, 0.025, 0.05, 0.075, 0.1, 0.5, and 1 mg/kg;
n = 10 nicotine, n = 12 control) according to
within-subjects Latin-square designs and ICSS thresholds were evaluated 30 min
later. A minimum of 48 h was allowed between each injection in the
Latin-square design, during which ICSS thresholds continued to be measured
daily, to ensure that ICSS thresholds returned to baseline levels before the
next drug administration. The doses of LY314582 and MPEP were chosen based on
a previous study demonstrating that 
10 mg/kg LY314582 and 3 mg/kg MPEP
elevated ICSS thresholds in drug-naïve rats
(Harrison et al., 2002). For
the potential demonstration of statistical interaction effects, it was
important to include doses of the test drugs that did not alter thresholds
under baseline conditions.
Intraventral Tegmental Area Administration Experiment. After stable
baseline ICSS responding was achieved (10% variation in threshold for
three consecutive days), rats (n = 15) with bilateral cannulas
directed toward the VTA were allocated to two groups such that there were no
differences in mean baseline reward thresholds or body weight between groups.
One group was then prepared with subcutaneous osmotic mini-pumps delivering
vehicle and a second group with mini-pumps delivering nicotine (3.16 mg/kg/day
nicotine free-base). Animals again were tested in the ICSS paradigm each day
for 7 days before drug treatment. Both groups of rats were then injected
directly into the VTA, as described above, with LY314582 (0, 10, 50, and 100
ng/side; n = 7 nicotine, n = 8 control) according to a
within-subjects Latin square design, and ICSS reward thresholds were evaluated
immediately postinjection. There was a minimum 48-h interval between each
injection, during which ICSS thresholds continued to be measured, to allow
thresholds to return to baseline levels before further drug tests. At the
conclusion of the experiment, all animals were anesthetized and their brains
removed and immediately placed on ice. The brains were cut in 50-µm
sections, and placements of the injectors and the electrodes were examined
(Fig. 1 for histological
verification of injection sites). Only those rats with injection tips located
within the VTA were included in statistical analyses.
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Spontaneous Nicotine Withdrawal Experiment. Osmotic mini-pumps were
surgically removed from nicotine-treated rats (n = 15) (defined as
rats having been prepared with mini-pumps delivering 3.16 mg/kg/day nicotine
free-base for at least 7 days) or corresponding control rats (n = 17;
rats prepared with vehicle-containing mini-pumps). All rats were then tested
in the ICSS procedure at 12, 18, 24, 36, 48, and 72 h after the removal of
osmotic mini-pumps. These time points were chosen based on the time course of
threshold elevations previously observed during spontaneous nicotine
withdrawal after removal of nicotine-delivering osmotic mini-pumps
(Harrison et al., 2001). Based
on the ICSS reward thresholds obtained at the 12-h time point,
nicotine-withdrawing rats were allocated to two groups such that there was no
difference in the magnitude of reward threshold elevations between each group
(117.67 ± 3.1%, n = 8; 119.93 ± 3.5%, n = 7).
Similarly, control rats were allocated to two groups such that there was no
difference in mean reward thresholds between these groups (106.45 ±
5.2%, n = 7; 103.63 ± 3.6%, n = 10). Thirty min
before being tested at the 18-h time point, one group of nicotine withdrawing
and one group of control rats were injected with LY341495 (1 mg/kg); the
remaining rats were injected with vehicle.
Statistical Analyses. Mean raw thresholds and response latencies (± S.E.M.) are presented for each experiment in the results section. For all experiments, except the spontaneous nicotine withdrawal experiment, percentage of change from baseline reward threshold was calculated by expressing the drug-influenced raw threshold scores as a percentage of the previous day's threshold (i.e., a drug-free baseline threshold). These percentages of baseline scores were subjected to two-factor repeated-measures analyses of variance (ANOVA), with treatment drug dose as the within-subjects factor and pump content (nicotine or control) as the between-subjects factor. For the spontaneous nicotine withdrawal experiment, percentage change from baseline reward threshold was calculated by expressing the threshold scores obtained at each time point during withdrawal as a percentage of thresholds for each rat on the day immediately before mini-pump removal. These percentages of baseline scores were subjected to three-factor repeated measures ANOVA. The within-subjects factor was the time after mini-pump removal, and the two between-subjects factors were pump content (nicotine or vehicle) and acute drug treatment (LY314582 or vehicle). For all experiments, response latency data were analyzed in the same manner as the threshold data. After statistically significant effects in the ANOVAs, post hoc comparisons among means were conducted with the Fisher's least significant difference test. The level of significance was set at 0.05.
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Results |
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TopAbstractMaterials and MethodsResultsDiscussionReferences |
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Ventral Tegmental Area Administration of the mGluII Receptor Agonist LY314582 Precipitated Elevations in ICSS Reward Thresholds in Nicotine-Treated but Not Control Rats. Mean (±S.E.M.) raw reward thresholds before intra-VTA administration of LY314582 for control and nicotine-treated rats were 115.3 ± 12.2 and 113.5 ± 19.0 µA, respectively. Mean (±S.E.M.) raw response latencies for control and nicotine-treated rats were 3.55 ± 0.29 and 3.15 ± 0.13 s, respectively. Bilateral microinfusion of LY314582 (10-100 ng/side) directly into the VTA significantly elevated reward thresholds in nicotine-treated but not control rats (Fig. 3). Again, there were significant effects of group [F(1,13) = 4.81, p < 0.05], dose [F(3,39) = 4.77, p < 0.01], and a significant group x dose interaction [F(3,39) = 3.82, p < 0.05]. Post hoc analyses revealed that doses of 50 and 100 ng/side LY314582 were sufficient to elevate reward thresholds in nicotine-treated rats without affecting thresholds in control rats. LY314582 had no effect on response latencies [F(3,39) = 1.94, N.S.] in nicotine-treated or control rats after VTA administration (data not shown).
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The mGluII Receptor Antagonist LY341495 Attenuated the Elevations in ICSS Thresholds Associated with Spontaneous Nicotine Withdrawal. Mean (±S.E.M.) raw reward thresholds prior to mini-pump removal for control and nicotine-treated rats were 105.9 ± 7.8 and 105.9 ± 11.0 µA, respectively. Mean (±S.E.M.) raw response latencies for control and nicotine-treated rats were 3.38 ± 0.1 and 3.36 ± 0.13 µA, respectively. Withdrawal from chronic nicotine treatment produced robust ICSS threshold elevations compared with control rats [F(1,27) = 15.3, p < 0.001] (Fig. 4A). Analysis of the significant group x dose x time interaction [F(5,135) = 3.3, p < 0.02] revealed the following. Nicotine-treated rats injected with vehicle demonstrated robust reward threshold elevations that reached a peak 24 h after mini-pump removal (Fig. 4A). However, administration of LY341495 30 min before the 18-h time point significantly attenuated the elevations in reward thresholds in nicotine-withdrawing rats (p < 0.001) (Fig. 4A), without affecting thresholds in control rats (Fig. 4B). LY341495 had no effect on response latencies at any time point after injection [F(1,27) = 0.43, N.S.] in nicotine-treated or control rats (data not shown).
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The NMDA Receptor Antagonist Dizocilpine Lowered ICSS Thresholds
Similarly in Nicotine-Treated and Control Rats. Mean (±S.E.M.) raw
reward thresholds before treatment with the NMDA receptor antagonist
dizocilpine for control and nicotine-treated rats were 88.9 ± 9.1 and
86.9 ± 3.2 µA, respectively. Mean (±S.E.M.) raw response
latencies for control and nicotine-treated rats were 3.32 ± 0.06 and
3.10 ± 0.06 µA, respectively. As can be seen in
Fig. 5A, dizocilpine (MK-801;
0.01-0.2 mg/kg) lowered ICSS reward thresholds in nicotine-treated and control
rats [F(6,66) = 7.5, p < 0.0001], and there
was no group x dose interaction [F(6,66) = 1.2,
N.S.]. Doses of dizocilpine 0.2 mg/kg caused disruption in performance in
the ICSS paradigm in both groups such that rats no longer responded for
self-stimulation, and therefore doses higher than 0.2 mg/kg were not tested.
Furthermore, dizocilpine did not precipitate withdrawal-like elevations in
reward thresholds in nicotine-treated rats at any dose tested. Dizocilpine
significantly increased response latencies [F(6,72) = 2.9,
p < 0.05]. Post hoc analysis demonstrated that as the dose of
dizocilpine increased, so too did response latency, particularly in control
rats, suggesting that performance was increasingly impaired at higher doses of
dizocilpine (Fig. 5B).
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The mGlu5 Receptor Antagonist MPEP Elevated ICSS Thresholds Similarly in Nicotine-Treated and Control Rats. Mean (±S.E.M.) raw reward thresholds before treatment with low doses of the mGlu5 receptor antagonist MPEP for control and nicotine-treated rats were 118.9 ± 9.3 and 98.4 ± 8.9 µA, respectively. Mean (±S.E.M.) raw response latencies for the low-dose MPEP experiment for control and nicotine-treated rats were 3.34 ± 0.09 and 3.43 ± 0.12 s, respectively. Mean (±S.E.M.) raw reward thresholds before treatment with high doses of MPEP for control and nicotine-treated rats were 112.9 ± 8.9 and 109.5 ± 8.5 µA, respectively. Mean (±S.E.M.) raw response latencies for the high-dose MPEP experiment for control and nicotine-treated rats were 3.27 ± 0.19 and 3.14 ± 0.07 s, respectively. Low doses of MPEP (0.01-0.1 mg/kg) did not affect ICSS reward thresholds [F(3,39) = 2.3, N.S.] or response latencies [F(3,39) = 0.4, N.S.] in nicotine-treated or control rats (data not shown). Higher doses of MPEP (0.5-3 mg/kg) elevated ICSS thresholds in nicotine-treated and control rats [F(4,96) = 8.4, p < 0.0001] (Fig. 6). However, MPEP elevated ICSS thresholds in both groups of rats by a similar magnitude (Fig. 6), and there was no group x dose interaction [F(4,96) = 0.7, N.S.]. MPEP (0.5-3 mg/kg) had no effect on response latencies [F(4,96) = 1.4, N.S.] in either group (data not shown).
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The AMPA/Kainate Receptor Antagonist NBQX Precipitated Elevations in ICSS Thresholds in Nicotine-Treated but Not Control Rats. Mean (±S.E.M.) raw reward thresholds prior to treatment with the AMPA/kainate receptor antagonist for control and nicotine-treated rats were 98.9 ± 10.0 and 98.5 ± 11.8 µA, respectively. Mean (±S.E.M.) raw response latencies for control and nicotine-treated rats were 3.21 ± 0.09 and 3.36 ± 0.15 µA, respectively. NBQX (0.01-1 mg/kg) significantly altered ICSS thresholds in nicotine-treated but not control rats (Fig. 7). This effect was reflected in a statistically significant effect of group [F(1,20) = 10.82, p < 0.005], a significant effect of dose [F(7,140) = 2.8, p < 0.01], and a significant group x dose interaction [F(7,140) = 2.11, p < 0.05]. Post hoc analysis revealed a bimodal action of NBQX on ICSS thresholds in nicotine-treated rats. Low doses of NBQX (0.025-0.1 mg/kg) elevated thresholds in nicotine-treated rats, whereas higher doses of NBQX (0.5-1 mg/kg) were less effective and did not significantly elevate thresholds compared with vehicle treatment (Fig. 7). NBQX had no effect on response latencies in nicotine-treated or control rats at any dose tested [F(7,140) = 0.31, N.S.] (data not shown).
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Discussion |
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TopAbstractMaterials and MethodsResultsDiscussionReferences |
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). The
present data strongly suggest a role for group II metabotropic glutamate
receptors in generating the reward deficits associated with nicotine
withdrawal by demonstrating that activation of mGluII receptors precipitated
ICSS threshold elevations in nicotine-dependent rats similar to those observed
during spontaneous nicotine withdrawal. Furthermore, activation of mGluII
receptors in the VTA also elevated thresholds in nicotine-dependent rats,
providing further support for an important role of the VTA in mediating the
actions of nicotine on reward pathways. Consistent with the above-mentioned
information, blockade of mGluII receptors attenuated the reward deficits in
rats undergoing spontaneous nicotine withdrawal. Previously, the mGluII
receptor agonist LY354740 was shown to attenuate the increased auditory
startle observed during spontaneous nicotine withdrawal
(Helton et al., 1997). One
possible explanation for these observations is that mGluII receptors located
in different brain sites may differentially regulate various aspects of
nicotine withdrawal.
Previously, the mGluII receptor agonist LY314582, which we found here to
elevate reward thresholds in nicotine-dependent rats at doses 7.5 mg/kg,
was shown to elevate ICSS thresholds in control rats at doses 10 mg/kg
(Harrison et al., 2002).
Therefore, the present observation that "sub-threshold" doses of
LY314582 precipitated withdrawal-like threshold elevations in
nicotine-dependent but not control rats suggests that negative regulation of
brain reward function by mGluII receptors was increased by prolonged nicotine
treatment. One mechanism through which nicotine elicits its reinforcing
effects is by increasing glutamatergic transmission in the VTA, thereby
potentiating mesoaccumbens dopamine transmission
(Schilstrom et al., 1998).
Because mGluII receptors located in the VTA are presynaptic autoreceptors that
decrease glutamate transmission (Bonci et
al., 1997; Wigmore and Lacey,
1998), it is likely that the increased mGluII receptor sensitivity
in the VTA observed in nicotine-treated rats occurred in response to prolonged
activation of excitatory glutamate transmission by nicotine in this brain
site, perhaps to counter this effect. Thus, during nicotine withdrawal when
the stimulatory effects of nicotine on excitatory glutamate transmission were
no longer present, increased mGluII receptor function would be expected to
decrease glutamate transmission and thereby decrease the activity of this
brain reward substrate. Recent electrophysiological studies are consistent
with this hypothesis. For instance, chronic opiate treatment increased the
inhibitory effects of mGluII receptor agonists on excitatory glutamate
currents in VTA dopamine neurons (Manzoni
and Williams, 1999), and in nucleus accumbens neurons
(Martin et al., 1999).
Nevertheless, it is possible mGluII receptors are also located on
nonglutamatergic terminals (e.g., serotonergic and cholinergic neurons) and
that activation of mGluII receptors precipitated nicotine withdrawal by
decreasing the release of neurotransmitters other than glutamate. Indeed,
nicotine withdrawal-induced threshold elevations were attenuated by
coadministration of fluoxetine, a selective serotonin reuptake inhibitor, and
4-(2'-methoxyphenyl)-1-[2'(N-[2'-pyridinyl]-p-iodo-benzamido)ethyl]piperazine
(P-MPPI), a serotonin-1A receptor antagonist, suggesting that decreased
serotonergic transmission also contributes to the reward deficits associated
with nicotine withdrawal (Harrison et al.,
2001).
To further investigate a potential role of decreased glutamatergic
transmission in the reward deficits associated with nicotine withdrawal, we
examined whether antagonists at postsynaptic glutamate receptors precipitated
withdrawal-like threshold elevations in nicotine-dependent rats similar to
activation of mGluII receptors. At low doses the AMPA/kainate receptor
antagonist NBQX precipitated threshold elevations in nicotine-treated but not
controls rats. Under "normal" baseline conditions, AMPA receptors
are the primary regulators of excitatory glutamate transmission throughout the
mesoaccumbens reward pathway (Pennartz et
al., 1990). Furthermore, AMPA receptor overexpression in the VTA
increased, whereas AMPA receptor blockade decreased, the rewarding actions of
drugs of abuse (Carlezon et al.,
1997; Xi and Stein,
2002). These observations suggest that AMPA receptors positively
modulate brain reward function. Conversely, AMPA receptor antagonists elicit
an intrinsic rewarding action after VTA administration
(David et al., 1998),
suggesting that AMPA receptors may also negatively regulate brain reward
function under baseline conditions. Indeed, AMPA receptors are located on
dopamine and GABAergic neurons in the VTA (Wang and French,
1993,
1995), where they modulate
mesoaccumbens dopamine transmission in an opposite manner. Therefore, it is
possible that NBQX had no effects in control rats because it simultaneously
blocked populations of AMPA/kainate receptors that positively and negatively
regulate reward function. However, the sensitivity of nicotine-treated rats to
NBQX suggests a scenario in which the development of nicotine dependence led
to compensatory decreases in the number and/or function of those AMPA/kainate
receptors that positively regulate brain reward function, perhaps to counter
the prolonged stimulatory effects of nicotine on reward pathways. Consistent
with this hypothesis, prolonged nicotine exposure decreased AMPA receptor
immunoreactivity in the VTA and nucleus accumbens
(Lee et al., 2002).
Alternatively, it is possible that a "silent" population of
AMPA/kainate receptors was recruited during prolonged nicotine exposure
(Isaac et al., 1995),
resulting in increased regulation of reward circuitries by AMPA/kainate
receptors. Regardless of the mechanism, these data suggest that decreased
glutamatergic transmission at AMPA/kainate receptors contributes to the
threshold elevations observed in nicotine withdrawing rats.
There is considerable evidence that NMDA receptors play an important role
in mediating the stimulatory effects of nicotine on mesoaccumbens dopamine
transmission (Grillner and Svensson,
2000). Therefore, it might have been expected that prolonged
nicotine treatment may have resulted in adaptations in the function/number of
NMDA receptors such that their blockade precipitated withdrawal-like threshold
elevations in nicotine-dependent rats but not controls similar to AMPA/Kainate
receptor blockade. Nevertheless, this did not seem to be the case. Similar to
previous reports (Carlezon and Wise,
1993), NMDA receptor blockade lowered thresholds in
nicotine-dependent and control rats, indicating a rewarding action. At no dose
tested did the NMDA receptor antagonist dizocilpine elevate thresholds in
either nicotine-treated or control rats. Interestingly, dizocilpine tended to
lower thresholds by a greater magnitude in nicotine-treated rats, suggesting
they were slightly more sensitive to dizocilpine's reward-facilitating
effects. Furthermore, higher doses of dizocilpine elevated response latencies
in control but not nicotine-dependent rats, suggesting that prolonged nicotine
treatment attenuated the performance-disrupting effects of dizocilpine.
Nevertheless, based on the present data it is unlikely that decreased
glutamatergic transmission at NMDA receptors contributes to the threshold
elevations associated with nicotine withdrawal.
Recently, mGlu5 receptors, which are primarily located postsynaptically
throughout the mesocorticolimbic system
(Wigmore and Lacey, 1998),
were shown to block the reinforcing effects of drugs of abuse, including
nicotine (Chiamulera et al.,
2001; Paterson et al.,
2003). Therefore, we also investigated the role of mGlu5 receptors
in nicotine withdrawal. At low doses, the mGlu5 receptor antagonist MPEP had
no effect on ICSS thresholds, whereas higher doses elevated thresholds in
nicotine-dependent and control rats (consistent with
Harrison et al., 2002).
Interestingly, MPEP tended to elevate thresholds by a greater magnitude in
nicotine-dependent rats compared with control. However, because no dose of
MPEP differentially elevated thresholds in nicotine-treated rats without also
elevating thresholds similarly in control rats, these data indicate that mGlu5
receptors regulate baseline brain reward function in control and
nicotine-treated rats, but are probably not involved in the threshold
elevations associated with nicotine withdrawal.
Perhaps the most parsimonious explanation of the present observations is
that prolonged, continuous nicotine exposure increased mGluII receptor
function, and decreased AMPA/kainate-mediated glutamate transmission in reward
circuitries, which contributed to the reward deficits observed during nicotine
withdrawal. In contrast, recent investigations demonstrated that repeated,
intermittent exposure to psychostimulants decreased mGluII function, and
increased AMPA receptor transmission in reward circuitries
(Giorgetti et al., 2001;
Xi et al., 2002). Thus, it is
possible that chronic nicotine and psychostimulant administration induce
different alterations in glutamatergic transmission. Alternatively, this
apparent discrepancy may be explained by the fact that the long-term
behavioral effects of drugs of abuse are related to the dosing administration
regimen (i.e., continuous or intermittent). Specifically, repeated
intermittent exposure to addictive drugs can result in a progressive
augmentation or "sensitization" in their behavioral effects
(Pierce and Kalivas, 1997;
Wolf, 1998). Conversely, more
continuous exposure similar to that used in the present study, and similar to
the pattern of prolonged nicotine exposure observed in smokers, engages
counteradaptive "opponent processes" that decrease the acute
behavioral effects of addictive drugs (i.e., "tolerance"), and
leads to the expression of an aversive withdrawal syndrome upon cessation
(Koob and Le Moal, 2001). It
has been proposed that sensitization may be important in the early stages of
drug addiction, when intake is intermittent, whereas tolerance and withdrawal
may be more important in later stages of drug dependence, as drug intake
progressively increases (Koob and Le Moal,
2001; Kenny et al.,
2003). Based on the above-mentioned information, it is an
interesting possibility that an initial increase, followed by a prolonged
decrease in glutamatergic transmission, mediated by mGluII and AMPA/kainate
receptors, may be involved in the initiation and maintenance of the
drug-taking habit, respectively. Thus, it will be of interest to investigate
whether other major drugs of abuse also increase the regulation of brain
reward function by mGluII receptors.
In conclusion, the present data suggest that mGluII receptors play an
important role in generating the reward deficits associated with nicotine
withdrawal. Furthermore, it is likely that mGluII receptors generated these
deficits, at least in part, by decreasing glutamate transmission at
AMPA/kainate receptors. Thus, because the reward deficits associated with drug
withdrawal are thought to play such a crucial role in drug addiction
(Ahmed et al., 2002;
Kenny et al., 2003), these
data suggest that mGluII and AMPA/kainate glutamate receptors may prove to be
useful therapeutic targets for the treatment of nicotine addiction.
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Acknowledgements |
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Footnotes |
|---|
Article, publication date, and citation information can be found at http://jpet.aspetjournals.org.
ABBREVIATIONS: ICSS, intracranial self-stimulation; VTA, ventral
tegmental area; mGluII, group II metabotropic glutamate receptor; NMDA,
N-methyl-D-aspartate; AMPA,
-amino-3-hydroxy-5-methyl-4-isoxazole propionate; mGlu5, metabotropic
glutamate 5 receptors; MK-801, dizocilpine; NBQX,
2,3-dihydroxy-6-nitro-7-sulfamoylbenzo(f)quinoxaline; MPEP,
6-methyl-2-[phenylethynyl]-pyridine; ANOVA, analysis of variance.
Address correspondence to: Dr. Athina Markou, Department of Neuropharmacology, CVN-7, The Scripps Research Institute, 10550 North Torrey Pines Rd., La Jolla, CA 92037. E-mail: amarkou{at}scripps.edu
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