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Vol. 282, Issue 3, 1181-1186, 1997
-Aminobutyric AcidA Receptors
Monash University, Department of Anesthesia, Monash Medical Centre, Clayton, Victoria, Australia 3168
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Abstract |
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 Top
Abstract
Introduction
Methods
Results
Discussion
References
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In this study, we investigated the interaction of propofol (a compound
used widely as an intravenous anesthetic) with 
-aminobutyric acidA (GABAA) and
delta opioid receptors at the level of the spinal cord.
Nociceptive thresholds were measured in rats through the use of
electrical current testing (ECT) and tail-flick latency. Full recovery
from sedation occurred 36.3 ± 1.7 min (mean ± S.E.M.; n = 20) after 40 mg/kg propofol i.p. Forty minutes
after administration, there was residual antinociception when assessed
by ECT but not when assessed by noxious heat. The ECT antinociceptive
effects of propofol at tail but not neck sites were suppressed by
intrathecal injection of the GABAA antagonists
bicuculline and SR-95531 and the delta opioid antagonist
naltrindole. These results suggest that there is an interaction between
propofol and antagonists at receptors in the caudal segments of the
spinal cord responsible for tail innervation. Antagonist dose-response
curves were compared with those for suppression of intrathecal
midazolam-induced antinociception. All intrathecal antagonists reversed
the antinociceptive effect of propofol with the same dose-response
curves as those previously obtained for suppression of the effect of
intrathecal midazolam. We conclude that propofol, when given
intraperitoneally, produces antinociception in rats through an
interaction with spinal GABAA receptors. This
combination leads to activation of a spinal cord system involving a
delta opioid receptor; the same mechanisms involved with
midazolam-induced spinal antinociception.
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Introduction |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Several
commonly used general anesthetics, sedatives and anxiolytics
(barbiturates, steroid derivatives, alcohols, benzodiazepines and
inhalational anesthetics) possess the ability to modulate GABAA receptors in the central nervous system
(Lambert et al., 1995
). GABA is the most widely distributed
and abundant inhibitory neurotransmitter in the central nervous system.
It activates either the chloride-linked GABAA or
the second-messenger-coupled GABAB receptor (Yeh
and Grigorenko, 1995). There is a substantial amount of evidence to
suggest that supraspinal GABAA receptors are
important sites for the pharmacological action of many of the
nonvolatile and volatile general anesthetics and sedatives (Jones
et al., 1995). GABA has also been implicated in the spinal
cord control of nociception (Nadeson et al., 1996), but the
precise role of the GABAA receptor in analgesia
remains unresolved.
Molecular biological studies have identified the
GABAA receptor as a macromolecular complex. It
consists of five subunits with many similarities to the nicotinic
acetylcholine receptor complex. Five types of subunit have been
described: alpha, beta, gamma,
delta and rho, and multiple variants for each of
these classes have been identified (alpha, 3beta,
2gamma, 1delta and 2rho). Cloning
studies have shown that a number of combinations of these subunits may
play a role in GABAergic neurotransmission in the central nervous
system (Olsen and Tobin, 1990; Tobin et al., 1991; Wafford
et al., 1993). The GABAA receptor
complex contains a number of distinct binding sites for ligands,
including GABA, benzodiazepines, barbiturates, picrotoxin and
t-butylbicyclophosphorothionate (Sieghart, 1992).
Propofol [2,6-diisopropylphenol (Diprivan)], a sterically hindered
phenol derivative, has become used widely as an intravenous anesthetic.
This drug is unrelated structurally to any other general anesthetic and
is the most short acting of the commercially available intravenous
agents. Studies have suggested that propofol produces anesthesia by
acting at GABAA receptors (Jones et
al., 1995; Sanna et al., 1995). A study by Hales and
Lambert (1991) showed that propofol potentiated the amplitude of
membrane currents elicited by the local application of GABA. These
results are consistent with biochemical data showing that propofol
increases [3H]GABA binding and GABA-induced
Cl
flux while decreasing
[35S]t-butylbicyclophosphorothionate
binding in rat brain through a bicuculline-sensitive mechanism (Sanna
et al., 1995). The early evidence indicated that modulation
of GABAA receptors by propofol resembled the
action of other general anesthetics such as barbiturate and steroid
derivatives. However, in recent studies, Concas et al.
(1991, 1992) identified a binding site for
[3H]propofol in rat brain that differs from
either the steroid or barbiturate recognition sites
Studies have shown that positive modulation of the
GABAA receptor in the spinal cord can cause
antinociception in vivo (Edwards et al., 1990;
Nadeson et al., 1996). No in vivo studies
investigating the role of propofol and GABAA
receptors in spinal cord have been reported. In the present study, we
investigate the interaction of propofol injected intraperitoneally with
GABAA receptors at the level of the spinal cord.
We used two GABAA antagonists (bicuculline and
SR-95531) injected i.t. to investigate this interaction. These results
suggested the same spinal GABAA receptors were
responsible for i.p. propofol antinociception as those involved with
spinally mediated antinociception after i.t. midazolam (Goodchild
et al., 1996). Spinal delta opioid receptors are
also involved with midazolam-induced antinociception. We therefore
investigated the involvement of spinal cord delta opioid
receptors with propofol-induced antinociception by attempting to
suppress the effects with the delta-selective opioid
antagonist naltrindole.
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Methods |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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This work was carried out with the permission of the Monash
University Standing Committee on Ethics in Animal Experimentation (SCEAE Project No. 93017). In all experiments, attention was paid to
ethical guidelines for the investigation of experimental pain in
conscious animals (Zimmerman, 1983)
Surgical techniques.
Male Wistar rats (weight, 180-200 g)
were anesthetized with halothane in oxygen-enriched air
(FiO2 = 0.4) and a Portex catheter (i.d.,
0.28 mm; o.d., 0.61 mm) was implanted under aseptic surgical conditions
into the lumbar subarachnoid space to lie adjacent to lower lumbar and
sacral segments of the spinal cord as previously described(Edwards
et al., 1990).
Test for recovery from sedation. Twenty rats (180-200 g; 10 with and 10 without i.t. catheter) were tested for the presence of the righting reflex and competency to perform the Rotarod test. These tests were used to assess the time taken for full recovery from sedation after an i.p. injection of 40 mg/kg propofol (Diprivan; ICI, Melbourne, Victoria, Australia). The rats were naive with no previous exposure to the Rotarod test. They were placed on the Rotarod accelerator treadmill (Ugo Basile 7650 accelerator Rotarod, Ugo Basile, Varese, Italy) set at the minimal speed for two training sessions of 1 to 2 min at intervals of 30 to 60 min. After this conditioning period, the animals were placed onto the Rotarod at a constant speed of 25 rpm. As the animal took grip of the drum, the accelerator mode was selected on the treadmill (i.e., the rotation rate of the drum was increased linearly at 20 rpm every minute thereafter). The time was measured from the start of the acceleration period until the rat fell off the drum; this was the control (pretreatment) performance time for each rat. The maximum running time was 30 sec. This test was performed on each rat four times with an interval of 30 min between each run. The mean performance time was calculated as an average of the last three control performance times.
The animals were then injected i.p. with propofol (40 mg/kg). The time taken for the animal to lose and regain the righting reflex was recorded. Once the animal had regained the ability to turn over from the supine to the prone position, it was placed on the Rotarod with the test parameters used in the control (pretreatment) period. The time taken for the animal to achieve its own mean performance time was recorded. Because there was no significant difference in the sedative profile between rats with and those without an i.t. catheter (see Results), the results from all 20 rats were combined to calculate an average recovery time. In subsequent experiments on age- and weight-matched rats, we waited for full recovery from the sedative effect of i.p. propofol for a period equal to this average plus 1 S.D. of the mean before continuing with nociceptive testing. Thus, all nociceptive threshold measurements made in subsequent experiments after i.p. propofol were made in rats that would show no signs of sedation or anesthesia (P < .05).Nociceptive tests.
Experiments were performed on 38 rats
with chronically implanted lumbar subarachnoid catheters. The animals
were placed in a restrainer that was covered to exclude distracting
sights and sounds. Nociceptive thresholds were measured with ECT and
the TFL as previously described (Edwards et al., 1990;
Nadeson et al., 1996).
; Nadeson et al., 1996). These changes were standardized as a ratio of
control (predrug administration) as previously described (Nadeson
et al., 1996; Serrao et al., 1989b). The TFL was
expressed as %MPE with the cutoff time set at 15 sec to avoid damage
to the tail. Both ECT and TFL were measured every 5 min, and the order
of tests was TFL, tail ECT and then neck ECT.
Measurement of antinociceptive effect of propofol.
ECT and
TFL were assessed every 5 min until three stable consecutive control
readings had been obtained. An i.p. injection of propofol 40 mg/kg
(n = 10) was then administered, and rats allowed to
recover from the effect of propofol for 40 min (the mean recovery plus
1 S.D. assessed by the Rotarod test in the previous group of age- and
weight-matched rats). Nociceptive values were then measured every 5 min
for 60 min (fig. 1, protocol 1).
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Experiments using antagonist. The involvement of spinal cord GABAA and delta opioid receptors with the antinociceptive effect of i.p. propofol was investigated in 38 rats with chronically implanted i.t. catheters. Experiments were performed on each rat once daily, up to 6 successive days. These animals were placed in a restrainer as above, and protocol 2 in figure 1 was followed. Nociceptive thresholds using ECT (neck and tail) were measured every 5 min until three consecutive stable readings had been obtained at each skin site. Propofol (40 mg/kg i.p.) was then given, and the rats remained in the restrainer. After full recovery from propofol-induced sedation, the residual antinociceptive effects were assessed before and after i.t. administration of bicuculline methiodide (Sigma Chemical, St. Louis, MO), SR-95531 (Research Biochemicals, Natick, MA) or naltrindole HCl (Research Biochemicals) (see protocol 2). The volume of the antagonist injected i.t. was 5 µl. This was chosen so that spread of the drug in the cerebrospinal fluid was minimized and its effect would therefore be restricted to the lumbosacral spinal cord; all antagonists were also dissolved in a slightly hyperbaric 6% dextrose solution for the same reason. To confirm this restriction of the drug effect, ECT was measured at both skin sites every 5 min. A change in the tail ECT after i.t. drug without a change in the neck ECT would indicate that the action of the drug was confined to the caudal segments of the spinal cord responsible for tail innervation.
A range of doses of antagonist were used: bicuculline (1 × 1012 to 5 × 1011
mol), SR-95531 (1 × 1012 to 5 × 1011 mol) and naltrindole (5 × 1011 to 5 × 108
mol). The effect of the antagonists was calculated as a percentage suppression of the response to propofol alone (mean of Y1 + Y2 + Y3 in
protocol 2, fig. 1) using the following equation:
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; Nadeson et al., 1996)
for the suppression of antinociception induced by i.t. midazolam.
Controls.
Experiments conducted in which 5 × 1011 mol bicuculline (n = 6),
5 × 1011 mol SR-95531 (n = 6) or 5 × 108 mol naltrindole
(n = 6) was administered i.t. but without prior i.p.
propofol. This was done to determine whether these compounds had any
effects on ECT or TFL when given alone.
Statistical analysis. All statistical comparisons between groups were made using Student's unpaired t test or one-way analysis of variance as appropriate. A value of P < .05 was considered statistically significant. ED50 values were calculated by applying a nonlinear regression to each line using the STATISTICA computer program.
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Results |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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All animals exhibited positive lidocaine tests after each experiment, indicating that the drugs injected down the catheters had been given into the i.t. space. No rat showed overt signs of neurological damage during the series of experiments by either loss of motor power or spontaneous occurrence of anesthesia in the tail.
Recovery from sedation after i.p. propofol. Propofol (40 mg/kg i.p.) caused no loss of righting reflex, but it did cause decreased performance in the Rotarod test. Table 1 shows the time (mean ± S.E.M.) taken to lose and recover performance in the Rotarod test after i.p. propofol (40 mg/kg) for a group of normal rats (n = 10) and rats with i.t. catheters (n = 10). There was no significant difference in the recovery times between rats with and without i.t. catheters. In pooled data for the two groups, full recovery from sedation measured by the Rotarod test occurred at 36.3 ± 1.7 min (mean ± S.E.M.) after i.p. propofol. In subsequent experiments, all nociceptive readings were taken 40 min (36.3 min + 3.6 min, which is 1 S.D. from the mean) after i.p. propofol.
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Antinociceptive effect of propofol.
Figure
2 shows time-response curves for the
antinociceptive effect of propofol assessed using ECT (measured at neck
and tail) and TFL. Propofol produced a rise in electrical current
threshold in the tail (R = 2.26 ± 0.27 × control; mean ± S.E.M., n = 6) and in the neck
(R = 2.09 ± 0.27 × control; mean ± S.E.M., n = 6) without affecting TFL (%MPE = 9.77 ± 9.81; mean ± S.E.M., n = 6). The
antinociception produced by propofol assessed using ECT was sustained
for 60 min (the end of the testing period allowed under ethics
committee license) after full recovery from propofol-induced sedation.
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Reversal of propofol antinociception by antagonists.
All three
antagonists produced suppression of the residual antinociceptive
effects of propofol in the tail but not the neck. Figure
3 shows one such response as a
time-response curve, the mean ± S.E.M. from six experiments in
which bicuculline (5 × 1011 mol)
suppressed the antinociceptive effect of propofol assessed using ECT at
the tail skin site but not the neck.
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; Nadeson et al., 1996) and by
propofol in the experiments reported here. The dose-response curves for
the two GABAA antagonists suppressing the
antinociceptive effect of propofol were different. These curves were
fitted to a nonlinear regression model using a statistical computer
program (STATISTCA), and the ED50 values for
these effects were calculated. The curves describing the suppression of
the antinociception induced by i.t. midazolam were coincident with
those describing the suppression by the antagonist of the i.p. propofol
effects (Goodchild et al., 1996; Nadeson et al.,
1996).
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Controls.
Intrathecal injections of bicuculline (5 × 1011 mol), SR-95531 (5 × 1011 mol) or naltrindole (5 × 108 mol) alone or the vehicles (10% intralipid
for i.p. propofol and 6% dextrose for i.t. injections) caused no
change in antinociceptive response assessed by either ECT or TFL values
at the doses used (table 2).
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Discussion |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Propofol is a commonly used anesthetic that has been shown to
enhance GABA-mediated synaptic inhibition in a number of neuronal systems (Hales and Lambert, 1991). In our experiments, an i.p. injection of propofol (40 mg/kg) caused rats to become sedated but not
lose consciousness. Full recovery from the sedative effects as measured
by the Rotarod test took ~35 min, after which the animals had resumed
all normal grooming and feeding behavior. Nociceptive tests were
carried out 40 min after the i.p. injection of propofol to assess
whether any residual (subanesthetic/sedative) concentrations of
propofol caused any antinociceptive effects. Although the rats in which
nociceptive thresholds were measured could not be subjected to the
Rotarod test while in the restrainer, it is likely that they recovered
from the sedative effects of i.p. propofol (40 mg/kg) similarly to the
rats in the previous group; they were obtained from the same batch and
were the same age and weight. In addition, it was possible to observe
them while they were in the restrainer, and they showed no signs of
sedation. The residual brain concentrations of propofol (40 mg/kg) that were probably present were therefore not sufficient to cause a noticeable change in conscious level.
After full recovery from sedation, the residual concentrations of propofol produced a rise in both neck and tail ECT values with no change in TFL. This antinociceptive effect was long lasting, and no appreciable reduction was noticed for 50 min after time had been allowed for full recovery from sedation. Because this antinociceptive effect occurred in the absence of any detectable anesthesia or sedation, it can be suggested that the systemic concentration of propofol needed to maintain antinociception is far lower than that required to induce or sustain anesthesia or sedation. However, full recovery and return of nociceptive thresholds to base-line values had occurred by the following day before the next experiment in the series.
In the present study, it is clear that propofol acts similarly to i.t.
midazolam in that it has no modulatory role in the nociceptive pathway
activated by noxious heat stimulation. Previous studies have shown that
the results from a number of different nociceptive tests can yield
contrasting results. For example, midazolam, a benzodiazepine, also
causes spinally mediated antinociception when given i.t. in our model
(Nadeson et al., 1996); this drug causes a rise in tail ECT
without a change in TFL. This is in contrast to i.t. fentanyl, which
causes antinociception when assessed by both tests (Serrao et
al., 1989a). It seems likely that the ECT activates different
nociceptive afferents to those stimulated by the TFL test.
An i.t. injection of the GABAA antagonist bicuculline or SR-95531 caused a dose-dependent reversal of the antinociceptive response to ECT in the tail but not in the neck. This differential effect suggests that there was no rostral spread of the antagonist in the CSF to the cervical levels of the spinal cord or higher because no effect was seen at the neck skin site. It can therefore be concluded that the antinociception produced by propofol is mediated through GABAA receptors at the level of the spinal cord because both GABAA antagonists could reverse the tail ECT rise. The antagonists did not reverse the antinociception after i.p. propofol at the neck skin sites. Because the antinociception in the tail site could be reversed by the spinal application of the antagonist, we may conclude that the effects were mediated by spinal cord mechanisms.
In experiments using the delta opioid antagonist naltrindole, a similar dose-dependent reversal of the antinociceptive effect of propofol measured by ECT was observed at the tail skin site but not at the neck site. This result suggests that propofol antinociception is also mediated by a spinal delta opioid receptor.
When using a particular antagonist, the dose-response curves for
suppressing the antinociceptive effect of midazolam given i.t. and
propofol given i.p. are the same. This was true for all three
antagonists used. When two different antinociceptive agents are
suppressed by the same antagonist with the same dose-response relationship and the same ED50, this implies that
the drugs are acting either directly or indirectly at the same receptor
(Mackay, 1994); that is, the two agents both bind to the receptor or
cause release of an endogenous neurotransmitter that binds to the same receptor as the antagonist drug.
This present study suggests that the antinociceptive effect of i.p.
propofol is mediated by the same GABAA receptors
as previously described for i.t. midazolam even though the drug is
given by a nonspinal parenteral (Goodchild et al., 1996).
Propofol, like midazolam, does not bind with delta opioid
receptors. However, both drugs must cause a release of endogenous
opioid peptides that bind with spinal cord delta opioid
receptors that were blocked by naltrindole. It is unclear whether
propofol binds directly with the spinal cord
GABAA receptors or exerts an indirect action. This could occur by activating brain systems with pathways descending to the spinal cord that then interact with spinal cord
GABAA receptors. To elucidate these questions
further, experiments using i.t. administered propofol are required. At
present, this is not possible because no suitable vehicle for the drug
is available for i.t. injection.
Antinociceptive effects of propofol have been reported in humans
(Anker-Moller et al., 1991), and there has been some
suggestion from in vitro studies that this action occurs
via modulation of GABAA receptors. Our
studies show that propofol causes antinociception in rats through
involvement of the same GABAA and
delta opioid receptor observed for midazolam. These
mechanisms suggest a possibility for potentiation of conventional
mu opioid analgesia. Midazolam, however, has to be given
i.t. to produce this effect (Yanez et al., 1990). The
current evidence suggests that this potentiation occurring at the level
of the spinal cord may be achieved with propofol without the necessity
of invading the i.t. space. This may be useful in humans, in whom one
is always wary of the possibility of neurological damage.
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Footnotes |
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Accepted for publication May 5, 1997.
Received for publication February 4, 1997.
Send reprint requests to: Prof. C. S. Goodchild, Monash University, Department of Anaesthesia, Monash Medical Centre, 246 Clayton Rd., Clayton, Victoria, Australia 3168.
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Abbreviations |
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ECT, electrical current threshold test;
GABA, -aminobutyric acid;
i.p., intraperitoneal;
i.t., intrathecal;
TFL, tail-flick latency;
%MPE, percentage of the maximal possible effect.
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References |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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ion channels modulated by multiple drug-binding sites.
Trends Pharmacol. Sci.
13: 446-450, 1992[Medline]. subunits in recombinant human -aminobutyric acidA/benzodiazepine receptors.
Mol. Pharmacol.
44: 437-442, 1993[Abstract].This article has been cited by other articles:
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, neck (ECT); 
, tail (ECT); 
, TFL (%MPE).
Values shown are mean ± S.E.M. (n = 6).
), SR-95531 (
, 
)
of the ECT antinociceptive effects of propofol (40 mg/kg i.p.; closed
symbols) and i.t. midazolam (47 nmol; open symbols). A, ECT tail skin
site. B, ECT neck skin site. ED50 values
calculated for each curve (STATISTCA) are bicuculline vs.
midazolam, 4.3 × 10