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Vol. 285, Issue 1, 208-215, April 1998
Center for Studies in Behavioral Neurobiology, Department of Psychology, Concordia University, Montreal, Quebec, Canada
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Abstract |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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In the present study, we examined the effects of dopamine (DA) receptor antagonists infused into the nucleus accumbens septi (NAS) on analgesia induced by intra-ventral tegmental area (VTA) infusions of the substance P (SP) analog, DiMe-C7 or morphine and intra-NAS infusions of amphetamine. Rats received intra-NAS infusions of either the mixed DA receptor antagonist flupenthixol (1.5 or 3.0 µg/0.5 µl/side; DiMe-C7 only), the DA D1/D5 receptor antagonist SCH 23390 (0.1 µg/0.5 µl/side; DiMe-C7 only) or the DA D2-type receptor antagonist raclopride (1.0, 3.0 or 5.0 µg/0.5 µl/side). Ten minutes later, rats received intra-VTA infusions of DiMe-C7 (3.0 µg/0.5 µl/side) or morphine (3.0 µg/0.5 µl/side) or intra-NAS infusions of amphetamine (2.5 µg/0.5 µl/side). Animals were then administered the formalin test for tonic pain. Intra-NAS raclopride prevented analgesia induced by intra-VTA DiMe-C7, intra-VTA morphine and intra-NAS amphetamine. Similarly, intra-NAS flupenthixol or SCH 23390 attenuated the analgesia induced by intra-VTA DiMe-C7. These findings suggest that tonic pain is inhibited, at least in part, by enhanced DA released from terminals of mesolimbic neurons. Furthermore, the evidence that SP and opioids in the VTA mediate stress-induced analgesia suggests that the pain-suppression system involving the activation of mesolimbic DA neurons is naturally triggered by exposure to stress, pain or both.
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Introduction |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Midbrain
ascending DA neurons, arising from the cell bodies of the VTA and
projecting to various forebrain structures such as the prefrontal
cortex, NAS and amygdala, play an important role in mediating the
suppression of tonic or persistent pain. Infusions into the VTA of the
tachykinin neuropeptide SP (Altier and Stewart, 1993
, 1997) or morphine
(Franklin, 1989; Manning et al., 1994) induce analgesia in
the formalin test for tonic pain. Intra-VTA infusions of either an SP
or an opioid receptor antagonist block the analgesia induced by
exposure to stress in the formalin test (Altier and Stewart, 1996; N. Altier and J. Stewart, unpublished observations), suggesting that SP-DA
and opioid-DA interactions are important in stress-induced analgesia. Amphetamine and morphine administered systemically induce analgesia in
the formalin test, and these effects are attenuated by either pretreatment with DA receptor antagonists (Morgan and Franklin, 1991)
or DA-depleting 6-OHDA lesions of the VTA (Morgan and Franklin, 1990).
There are several reasons to believe that the analgesia induced by SP,
morphine and amphetamine in the formalin test is mediated, at least in
part, by the release of DA from terminals in the NAS. SP interacts in
an excitatory way with midbrain DA neurons projecting to the NAS (see
Kalivas, 1985, for review), and intra-VTA infusions of SP enhance DA
metabolism in the NAS (e.g., Cador et al., 1989), as do those of the metabolically stable SP analog DiMe-C7 (Elliott et al., 1986) and the highly selective SP (NK-1) receptor
agonist GR-73632 (Elliott et al., 1991). Similarly, SP or
DiMe-C7 administered systemically increase extracellular levels of DA
in the NAS, as assessed by in vivo microdialysis (Boix
et al., 1992a, 1992b). Other studies show that intra-VTA
administration of SP, DiMe-C7 or GR-73632 stimulates locomotor activity
(e.g., Eison et al., 1982; Elliott and Iversen,
1986; Elliott et al., 1991; Stinus et al., 1978)
and that this response can be blocked by either intra-NAS infusions of
the DA receptor antagonist haloperidol or 6-OHDA lesions of the NAS
(Kelley et al., 1979).
There also is evidence that morphine and other mu opioid
receptor agonists act to increase DA release in the NAS. For example, DA metabolism in the NAS is increased after intra-VTA infusions of
opioids (Kalivas et al., 1983; Kalivas and
Richardson-Carlson, 1986; Latimer et al., 1987), as is
extracellular DA in the NAS after systemic injections of morphine and
other mu opioid receptor agonists (e.g., Di
Chiara and Imperato, 1988; Spanagel et al., 1990). Intra-VTA
infusions of mu opioid receptor agonists stimulate locomotor
activity (Joyce et al., 1981; Kalivas et al.,
1983; Latimer et al., 1987), and this effect is blocked by
either intra-NAS DA receptor antagonists or lesions made to the NAS
(Stinus et al., 1980; Kalivas et al., 1983).
Studies have also shown that the rewarding effects of opioids are
associated with the release of DA in the NAS from terminals of midbrain
ascending neurons (e.g., Kiyatkin et al., 1993).
Other studies show that systemic or intra-VTA administration of
mu agonists elicit conditioned place preference, and that
electrolytic or 6-OHDA lesions of the NAS block this effect
(e.g., Phillips and LePiane, 1980; Kelsey et al.,
1989; Bals-Kubik et al., 1993; Shippenberg et
al., 1993).
Finally, amphetamine is known to elevate extracellular levels of DA in
the NAS (e.g., Sharp et al., 1987; Di Chiara and
Imperato, 1988) to enhance locomotor activity and to have rewarding
properties. Amphetamine-induced hyperactivity and self-administration
are greatly reduced by 6-OHDA lesions of the NAS (Kelly et
al., 1975; Kelly and Iversen, 1976; Lyness et al.,
1979) and by infusions of DA receptor antagonists into the NAS
(Pijnenburg et al., 1975; van den Boss et al.,
1988). It has also been shown that infusions of amphetamine into the
NAS induce conditioned place preference and self-administration (Carr
and White, 1983; Hoebel et al., 1983; Phillips et
al., 1994) and stimulate locomotor activity (Pijnenburg et
al., 1976).
Thus, the evidence that SP, morphine and amphetamine act to increase DA
transmission in mesolimbic neurons, that all are effective at
attenuating tonic pain and that intra-NAS infusions of amphetamine elicits analgesia in the formalin test (Altier and Stewart, 1993) suggests that the analgesia induced by intra-VTA tachykinins and opioids and intra-NAS amphetamine are due, at least in part, to enhanced DA release in the NAS from terminals of midbrain ascending neurons. The following experiments were designed, therefore, to examine
the involvement of DA in the NAS in the analgesia induced by these
compounds in the formalin test. To this end, we studied the effect of
pretreatment with DA receptor antagonists infused into the NAS on the
analgesia induced by intra-VTA infusions of either the SP analog,
DiMe-C7, or morphine and by infusions of amphetamine in the NAS.
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Materials and Methods |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Subjects, housing and habituation. Naive male Wistar rats weighing 350 to 375 g (Charles River Canada, St. Constant, Quebec, Canada) served as subjects. On arrival, they were housed individually in stainless-steel cages. They had continuous access to food and water and were maintained on a 12-hr light-dark cycle (lights on at 9:00 p.m. and off at 9:00 a.m.). All testing took place during the dark portion of the light-dark cycle. On each of the 4 days before testing, all animals were handled for at least 1 min. On each of the 2 days before formalin testing, all animals were handled and habituated to the various testing procedures to be used on the test day, except that neither intracranial nor formalin injections were administered.
Apparatus. The formalin test cubicles, 30 × 30 × 30 cm, were made of clear Plexiglas. A mirror was mounted beneath the floor of the cubicle at a 45 degree angle to allow an unobstructed view of the rats' paws.
Surgery.
Seven to 10 days after arrival, rats were
anesthetized with an injection of sodium pentobarbital (Somnotol, 65 mg/kg i.p.; MTC Pharmaceuticals, Cambridge, Ontario, Canada). When
required, anesthesia was supplemented with methoxyflurane (Metofane;
Pitman-Moore, Mississauga, Ontario, Canada). Animals receiving a DA
receptor antagonist in the NAS followed by intra-VTA DiMe-C7 or
morphine were implanted with four cannulae. First, 21-mm-long, 22-gauge guide cannulae (Plastics One, Roanoke, VA) were implanted bilaterally 1.0 mm above the VTA and aimed at the following coordinates: 
5.7 mm
posterior to bregma, +0.6 mm lateral from the midline and 7.4 mm
ventral from the dura mater (Paxinos and Watson, 1986). The stereotaxic
arms were angled laterally at 15 degrees from the perpendicular, and
the skull was level between lambda and bregma (i.e., flat
skull position). Five stainless-steel screws were secured to the skull,
and the VTA cannulae were anchored to the skull with dental acrylic
cement applied around them without blocking bregma from view. The
incisor bar was then set 5.0 mm above the interaural line, and cannulae
were angled at 10 degrees from the perpendicular. The 19-mm-long,
22-gauge guide cannulae were implanted bilaterally 1.0 mm above the NAS
at the following coordinates: +3.0 mm anterior from bregma, +1.4 mm
lateral from midline and 6.3 mm ventral from the skull surface
(Pellegrino et al., 1967). Cannulae were anchored with
dental acrylic cement. Animals receiving infusions into the NAS of
raclopride followed by amphetamine were implanted with cannulae in the
NAS using the same coordinates stated above. Before surgery, all
animals received 0.6 mg/kg s.c. of atropine sulfate (Glaxo
Laboratories, Montreal, Quebec, Canada). After surgery, 28-gauge
stainless-steel obturators (Plastics One) were inserted into the guide
cannulae. These extended 1.0 mm beyond the tip of the guide cannulae.
On recovery under a heat lamp, rats were housed individually in
standard plastic cages with wire tops and allowed a 7-day recovery
period before habituation to testing procedures was begun.
Formalin test.
Tonic pain was induced by a subcutaneous
injection of 0.05 ml of 2.5% formalin into the plantar surface of one
hind paw. Pain responses were recorded once every 5 sec for 60 min
using a time-sampling procedure. Thus, 12 observations were made per
minute. The intensity of pain was rated according to four behavioral
categories, using a scale of 0 to 3: a score of 0, if the rat walked or
sat normally with weight placed equally on both hindpaws; 1, if the rat
favored the injured paw (e.g., if it limped); 2, if the rat
held the injured paw off the floor, with at most the nails touching the
floor; and 3, if the rat chewed or licked the injured paw. The scores used for each time point were based on the mean for each animal of all
the pain scores taken over a 3-min period. This weighted-scores method
of rating formalin pain responses has been validated previously (Coderre et al., 1993). In all cases, the observer was blind
as to which animals received a drug and which received the vehicle.
Drugs.
The doses used to induce analgesia in these
experiments were based on previous findings. The SP analog DiMe-C7
(Sigma Chemical, St. Louis, MO) was dissolved in acid saline (pH 6.05)
and infused bilaterally into the VTA at a dose of 3.0 µg/0.5
µl/side (Altier and Stewart, 1993, 1997). Stock volumes (5.0 µl) of
this compound and its vehicle were aliquoted into polypropylene vials
and frozen at 70°C. Solutions were thawed within 30 min of the
infusions. Morphine sulfate (BDH, Québec, Canada) was dissolved
in saline and infused bilaterally into the VTA at a dose of 3.0 µg/0.5 µl/side (Manning et al., 1994).
D-Amphetamine sulfate (SmithKline Beecham, Oakville,
Ontario, Canada) was dissolved in saline and infused bilaterally into
the NAS at a dose of 2.5 µg/0.5 µl/side (Altier and Stewart, 1993).
). Raclopride
(Astra Pharma, Mississauga, Ontario, Canada) was dissolved in saline
and infused bilaterally into the NAS at doses of 1.0, 3.0 and 5.0 µg/0.5 µl/side.
Intracranial microinjections. After removal of the obturators, 28-gauge stainless-steel internal injector cannulae extending 1.0 mm beyond the tip of the guide cannulae were inserted and held in place in the guide cannulae by a brass screw cuff. The injector cannulae were connected via polyethylene tubing to 1-µl Hamilton syringes. Compounds were administered in unrestrained rats in a volume of 0.5 µl/side over 60 sec. The injectors remained in place for an additional 120 sec to allow diffusion of the solutions around the injection site. Obturators were immediately replaced after removal of the injectors. To prevent intracranial infections, all internal injector cannulae and obturators were wiped with 70% alcohol and dried immediately before being inserted into the guide cannulae.
Design and procedure. On the test day, rats received either bilateral intra-VTA infusions of DiMe-C7 (3.0 µg/0.5 µl/side) or morphine (3.0 µg/0.5 µl/side) or bilateral intra-NAS infusions of amphetamine (2.5 µg/0.5 µl/side). Ten minutes before these intracranial infusions, all rats were pretreated with bilateral intra-NAS infusions of either raclopride (1.0, 3.0 or 5.0 µg/0.5 µl/side), SCH 23390 (0.1 µg/0.5 µl/side; DiMe-C7 only), flupenthixol (1.5 or 3.0 µg/0.5 µl/side; DiMe-C7 only) or saline. Rats received a subcutaneous injection of 0.05 ml of 2.5% formalin into the plantar surface of one hindpaw immediately after the last intracranial infusion. Rats assigned to conditions flupenthixol-DiMe-C7 and saline-DiMe-C7 (fig. 1), SCH 23390-DiMe-C7 and saline-DiMe-C7 (fig. 2), raclopride-DiMe-C7 and saline-DiMe-C7 (fig. 3), raclopride-morphine and saline-morphine (fig. 4) and raclopride-amphetamine and saline-amphetamine (fig. 5) were tested in the formalin test using a counterbalanced within-subjects design. Thus, animals were tested twice in the formalin test at a 1-week interval. Either the right or left hindpaw was injected on successive tests. Rats assigned to all the remaining conditions were tested in the formalin test once, using a between-subjects design.
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Histology. After completion of the experiments, rats were deeply anesthetized with chloral hydrate (1 ml i.p.) and perfused transcardially with the injectors in place with 0.9% saline followed by 10% formalin. Brains were then removed and stored in 10% formalin for at least 1 week. Histological verification of cannulae tip placements was subsequently determined on 30-µm thionine-stained coronal sections.
Statistical analyses. To verify whether DiMe-C7, morphine and amphetamine induced significant analgesia and whether pretreatment with the DA receptor antagonists had any effects on its own, separate two-way ANOVAs were conducted with treatment group (vehicle-drug vs. antagonist-vehicle vs. vehicle-vehicle) as the between-subjects variable and time (10 postinfusion time points) as the within-subjects variable; because most of the effects of the drugs occurred within the first 30 min of testing, only the first 10 postinfusion time points were included in the analyses. All analyses were followed, if appropriate, by Tukey's post hoc test for overall differences between groups. Unless otherwise specified, two-way ANOVAs were conducted with pretreatment condition (antagonist-drug vs. vehicle-drug) and time (10 postinfusion time points) as within-subjects variables to examine the effects of pretreatment with the DA receptor antagonists on the analgesia induced by DiMe-C7, morphine and amphetamine. Tests for simple main effects were used, if appropriate, to analyze the differences at each time point between the two conditions. Data from an animal were included in the analyses only if the injector tips were located within 0.5 mm of the target area.
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Results |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Effect of intra-NAS flupenthixol on DiMe-C7-induced analgesia. Figure 1 shows the effect of intra-NAS pretreatment with two doses (1.5 or 3.0 µg/0.5 µl/side) of the mixed DA receptor antagonist flupenthixol on the analgesic effect of DiMe-C7 (3.0 µg/0.5 µl/side) infused into the VTA. Separate ANOVAs conducted for treatment group (saline-DiMe-C7 vs. saline-vehicle vs. flupenthixol-vehicle) by time for each dose of flupenthixol (fig. 1, A and B) revealed significant effects for treatment group, F(2,15) = 60.954, P < .0001 and F(2,16) = 43.194, P < .0001, respectively. As seen by comparing groups saline-DiMe-C7 and saline-vehicle (fig. 1, A and B), intra-VTA DiMe-C7 significantly attenuated pain scores (P < .05) for ~30 min. A three-way ANOVA conducted with dose (1.5 or 3.0 µg/0.5 µl/side) as the between-subjects variable and pretreatment condition (flupenthixol-DiMe-C7 vs. saline-DiMe-C7) and time as within-subjects variables revealed a significant main effect of pretreatment condition, F(1,9) = 5.64, P < .05.
Effect of intra-NAS SCH 23390 on DiMe-C7-induced analgesia. Figure 2 shows the effect of intra-NAS pretreatment with the DA D1/D5 receptor antagonist SCH 23390 (0.1 µg/0.5 µl/side) on the analgesia induced by intra-VTA DiMe-C7 (3.0 µg/0.5 µl/side). The ANOVA conducted for treatment group (saline-DiMe-C7 vs. SCH 23390-saline vs. saline-vehicle) by time revealed a significant overall effect of treatment group, F(2,12) = 55.04, P < .0001. As shown by comparing groups saline-DiMe-C7 and saline-vehicle, intra-VTA infusions of DiMe-C7 induced significant analgesia for ~30 min after the formalin injection (P < .05). The ANOVA conducted for pretreatment condition (SCH 23390-DiMe-C7 and saline-DiMe-C7) by time revealed a significant effect of pretreatment condition, F(1,5) = 10.85, P < .05, indicating that intra-NAS infusions of SCH 23390 significantly attenuated the analgesic effect of intra-VTA DiMe-C7.
Effect of intra-NAS raclopride on DiMe-C7-, morphine- and
amphetamine-induced analgesia.
Figure 3 shows the effect of
intra-NAS pretreatment with escalating doses of raclopride on the
analgesia induced by intra-VTA infusions of DiMe-C7 (3.0 µg/0.5
µl/side). The ANOVAs conducted for treatment group (saline-DiMe-C7
vs. raclopride-vehicle vs. saline-vehicle) by
time for each dose of raclopride (fig. 3, A-C) revealed significant
overall treatment group effects, F(2,18) = 6.05, P < .01, F(2,17) = 67.72, P < .0001, and F(2,16) = 37.3, P < .0001, respectively. In each case, DiMe-C7 alone significantly reduced pain
scores (P < .05). A three-way ANOVA with dose (1.0, 3.0 or 5.0 µg/0.5 µl/side) as the between-subjects variable and pretreatment
condition (raclopride-DiMe-C7 or saline-DiMe-C7) and time as
within-subject variables revealed a significant main effect of
pretreatment condition, F(1,16) = 17.033, P < .001. As seen by
comparing conditions raclopride-DiMe-C7 (
) and saline-DiMe-C7 (
),
raclopride significantly blocked the analgesic effect induced by
DiMe-C7 only at the highest dose (P < .05). At this dose,
DiMe-C7-induced analgesia was blocked at all time points for 18 min
after the formalin injection. As seen by comparing groups
raclopride-vehicle (
) and saline-vehicle (
), raclopride
pretreatment alone was without effect on pain scores at any of the
doses tested.
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Discussion |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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The present findings indicate that DA D2-type receptor antagonism
in the NAS prevents the analgesia induced by SP, morphine and
amphetamine in the formalin test for tonic pain. More specifically, it
was found that pretreatment with the DA D2-selective receptor antagonist raclopride infused directly into the NAS blocks the analgesia induced by intra-VTA infusions of either the SP analog DiMe-C7 or morphine and of intra-NAS infusions of amphetamine. In the
case of DiMe-C7, animals were pretreated with three different doses of
raclopride, and a dose-dependent attenuation of DiMe-C7-induced analgesia was observed, with the highest dose (i.e., 5.0 µg/0.5 µl/side) resulting in a complete blockade of the analgesic
effect. Likewise, this highest dose of raclopride caused a complete
blockade of intra-VTA morphine- and intra-NAS amphetamine-induced
analgesia. These findings are in accordance with those of previous
studies implicating midbrain ascending DA neurons in the inhibition of tonic pain (Franklin, 1989; Morgan and Franklin, 1990; Manning et
al., 1994; Anderson and Rompré, 1996) and, more
specifically, implicating enhanced DA activity in the NAS in this
effect (Clarke and Franklin, 1992; Altier and Stewart, 1993).
Previous studies have reported that selective DA D2-type agonists
administered systemically induce analgesia in the formalin test (Morgan
and Franklin, 1991) and the vocalization after discharge test (Carr,
1984), the latter of which induces pain associated with significant
negative affect, as is the case with the formalin test. Selective DA
D2-type receptor antagonists administered systemically attenuate the
analgesia induced by systemic amphetamine, morphine and cocaine in the
formalin test (Lin et al., 1989; Morgan and Franklin, 1991)
and in the vocalization after discharge test (Paalzow and Paalzow,
1975; Carr, 1984). Our findings are consistent with those of these
previous studies implicating DA D2-type receptors in the inhibition of
tonic pain and indicate that the NAS is the neuroanatomical site where
these DA receptor subtypes mediate this response. The present findings
also extend those of previous studies by showing that DA D2-type
receptors in the NAS mediate the analgesia induced by morphine and
amphetamine when they are infused directly at sites within the
mesolimbic system, namely, in the VTA and NAS, respectively. Finally,
the results indicate that, as is the case for morphine and amphetamine,
DA D2-type receptors in the NAS also mediate the analgesic effects
induced by SP acting in the VTA.
It was also found that pretreatment with the selective DA D1/D5
receptor antagonist SCH 23390 infused into the NAS attenuates the
analgesic effects induced by the SP analog DiMe-C7 infused into the
VTA. Together with the findings on the effects of raclopride, this
finding suggests that SP acting in the VTA inhibits tonic pain by
causing the release of DA in the NAS from mesolimbic terminals, which,
in turn, stimulates both DA D1/D5 and DA D2-type receptors at this
site. The finding that DA D1/D5, in addition to DA D2-type, receptors
in the NAS mediate the analgesic effects induced by SP acting in the
VTA agrees with the results of other reports indicating that SCH 23390 administered systemically attenuates the analgesia induced by
amphetamine, morphine and cocaine in the formalin test (Lin et
al., 1989; Morgan and Franklin, 1991). It is likely that the NAS
is the site where DA D1/D5 receptors also mediate the analgesia induced
by morphine and amphetamine administered either systemically or into
the VTA or NAS, respectively, given the similarities reported in the
present study between the effects of DiMe-C7, morphine and amphetamine
on tonic pain and on the involvement of DA D2-type receptors in the NAS
in these effects. This remains, however, to be tested in the future.
Although the antagonism of either DA D1/D5 or D2-type receptors in the
NAS attenuated the analgesia induced by intra-VTA DiMe-C7, the DA
D2-type receptor antagonist raclopride appeared to be more effective
than the DA D1/D5 receptor antagonist SCH 23390. These findings suggest
that D2-type receptors may play a more important role than D1/D5
receptors in the NAS in the mediation of analgesia induced by the
activation of DA neurons. It could be that the dose of SCH 23390 used
was not high enough to induce a more potent attenuation of analgesia.
However, higher doses were not used because we were concerned that they
would induce sedation and motor impairment (Nakajima and Wise, 1987).
It was also found that intra-NAS infusions of the mixed DA receptor
antagonist flupenthixol attenuates the analgesia induced by intra-VTA
DiMe-C7. This finding is consistent with the results of previous
studies showing that the mixed DA receptor antagonists flupenthixol and
chlorpromazine administered systemically attenuate the analgesia
induced by systemic amphetamine, morphine and cocaine in the formalin
test (Lin et al., 1989; Morgan and Franklin, 1991). It is
interesting to note, however, that the attenuation of DiMe-C7-induced analgesia by intra-NAS flupenthixol within the range of doses used was
not as great as that seen after intra-NAS raclopride.
The present findings concerning the role of DA in the NAS on analgesia
induced by intra-NAS amphetamine test are consistent with those of
Clarke and Franklin (1992), who showed that bilateral 6-OHDA lesions of
the NAS attenuated the analgesia induced by systemic amphetamine in the
formalin test. In contrast to the present results, however, Clarke and
Franklin found that 6-OHDA lesions in the NAS did not reduce the
analgesic effect of systemically administered morphine in the formalin
test, whereas in the present study, reduced DA neurotransmission in the
NAS prevented the analgesia induced by intra-VTA morphine. There are
two possible reasons for this difference. It may be that the intra-NAS
infusions of the DA receptor antagonists used in the present
experiments were more effective in reducing DA transmission than the
6-OHDA lesions used by Clarke and Franklin, which were incomplete and
known to allow substantial recovery of DA function (see Castaneda
et al., 1990). Differences in the routes of morphine
administration might also account for the discrepancy. Indeed, it is
possible that the manipulations carried out in the study of Clarke and
Franklin aimed at decreasing DA transmission in the NAS did not block
morphine analgesia because the opioid given systemically elicited
analgesia by acting at several sites involved in modulating tonic pain. Morphine infused in the spinal cord (Malmberg and Yaksh, 1993) and at
several supraspinal sites other than the VTA, such as the posterior
hypothalamic area, periaqueductal gray and habenula, produces analgesia
in the formalin test (Cohen and Melzack, 1985; Manning et
al., 1994; Vaccarino and Chorney, 1994). In contrast, in the
present study, morphine analgesia may have been prevented successfully
by DA receptor antagonism in the NAS because the opioid was infused
directly into the VTA, thereby restricting the effect of the opioid on
tonic pain to midbrain ascending DA systems.
Finally, it was found that intra-NAS infusions of raclopride, SCH 23390 and flupenthixol had no effect when given alone on pain responses in
the formalin test. Although these manipulations appeared to induce mild
hyperalgesia (i.e., increased pain responsiveness), this
effect was expected to be more pronounced given the evidence presented
here that DA plays a role in modulating tonic pain. It is possible,
however, that these manipulations were not effective at inducing the
expected hyperalgesic effects because pain scores, recorded after an
injection of 2.5% formalin, show a ceiling effect. In support of this
idea, it has been reported in a previous study that pain scores
recorded after the injection of 5.0% formalin do not differ from those
recorded after the injection of 2.5% formalin (Coderre et
al., 1993). These findings suggest that it might be worthwhile to
reexamine the effects DA receptors antagonists in the NAS on tonic pain
using a concentration of formalin lower than that used in the present
study.
It was observed in the present study that intra-VTA DiMe-C7, intra-VTA
morphine and intra-NAS amphetamine increased locomotor activity. The
issue is often raised that analgesia induced by drugs that increase
behavioral activation may be an artifact; that is, increased locomotor
activity may compete and interfere with the animals' ability to
display pain behavior, thereby accounting for the decreased pain
scores. There are several lines of evidence to suggest, however, that
locomotor activity and analgesia in the formalin test are dissociable.
First, there is a discrepancy in the time course between the
locomotor-stimulant and analgesic effects induced by SP, opioids and
amphetamine. More specifically, the locomotor-activating effects of
intra-VTA SP or DiMe-C7 (Kalivas, 1985), intra-VTA mu
receptor agonists (e.g., Joyce et al., 1981; Kalivas and Richardson-Carlson, 1986) and intra-NAS amphetamine (e.g., van den Boss et al., 1988) greatly outlast
the analgesic effects induced by similar pharmacological manipulations.
We compared the time course of the behavioral effects of intra-VTA
DiMe-C7 in formalin-treated animals and found that the SP analog
increased locomotor activity for at least 110 min, whereas analgesia
lasted for ~30 min (Altier, 1993), indicating that animals can
display pain behaviors despite high levels of locomotor activity. Other evidence that secondary motor effects do not interfere with an animal's ability to display pain behavior comes from studies showing that animals that are either cataleptic (Matthies and Franklin, 1992)
or hypoactive due to DA receptor antagonist pretreatment (Morgan and
Franklin, 1991) can display high pain scores in the formalin test.
Based on all these findings, it is unlikely that the analgesic effects
reported here are confounded by secondary motor effects.
In summary, the results of the present study indicate that blockade of
DA D2-type receptors in the NAS by raclopride prevents the analgesic
effects induced by either infusions into the VTA of the SP analog
DiMe-C7 or morphine or infusions of amphetamine into the NAS. It was
also found in tests with intra-VTA DiMe-C7 that intra-NAS infusions of
either the mixed DA receptor antagonist flupenthixol or the DA D1/D5
receptor antagonist SCH 23390 attenuate analgesia, although less
effectively. Together, these findings suggest that a mechanism
underlying the inhibition of tonic pain is the stimulation of DA
receptors in the NAS by DA released from terminals of mesolimbic
neurons. The evidence that SP and opioid receptors in the VTA play a
role in mediating stress-induced analgesia in the formalin test (Altier
and Stewart, 1996; N. Altier and J. Stewart, unpublished observations)
further suggests that the pain-suppression system involving the
activation of mesolimbic DA neurons is naturally triggered by exposure
to stress, pain or both through the release of SP and opioids in the
VTA.
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Footnotes |
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Accepted for publication December 22, 1997.
Received for publication September 12, 1997.
1 This work was supported by grants from the Medical Research Council of Canada and Fonds pour la Formation de Chercheurs et l'Aide à la Recherche (Québec).
Send reprint requests to: Dr. Jane Stewart, Center for Studies in Behavioral Neurobiology, Department of Psychology, Concordia University, 1455 de Maisonneuve Blvd. West, Montréal, Québec, Canada, H3G 1M8.
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Abbreviations |
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VTA, ventral tegmental area; DA, dopamine; NAS, nucleus accumbens septi; SP, substance P; 6-OHDA, 6-hydroxydopamine; ANOVA, analysis of variance.
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References |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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