Is the Reduced Efficacy of Morphine in Diabetic Rats Caused by Alterations of Opiate Receptors or of Morphine Pharmacokinetics?

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Vol. 285, Issue 1, 63-70, April 1998

Is the Reduced Efficacy of Morphine in Diabetic Rats Caused by Alterations of Opiate Receptors or of Morphine Pharmacokinetics?

C. Courteix, P. Bourget¹, F. Caussade², M. Bardin³, F. Coudore, J. Fialip and A. Eschalier³

Equipe NPPUA, Laboratoire de Pharmacologie, Faculté de Pharmacie, F-63001 Clermont-Ferrand Cedex, France

	Abstract

Top Abstract Introduction Methods Results Discussion References

Because it generally is admitted that neuropathic pain is resistant to opioid analgesia, we investigated the effect of morphineon hyperalgesia in streptozocin-induced diabetes in rats. Theantinociceptive effect of morphine (0.5-4 mg/kg i.v.) on mechanical(paw pressure test), thermal (tail immersion test) and chemical(formalin test) hyperalgesia was reduced. To clarify the mechanismsinvolved in the alteration of morphine analgesia, the bindingcharacteristics of mu and delta receptor agonists and the pharmacokineticsof morphine and its glucuronide metabolites morphine 3-glucuronideand morphine 6-glucuronide were determined. K_D and B_max valuesfor [³H][D-Ala²,(Me)Phe⁴, Gly(ol)⁵]enkephalin and [³H][D-Pen²,D-Pen⁵]enkephalin to cerebral mu and delta opiate receptors were notaltered by diabetes. Likewise, the plasma maximal concentrationof morphine and metabolites, as well as the area under the curve,did not differ between diabetic and normal rats. Only the totalclearance and the apparent volume of distribution of morphinewere increased in diabetic rats, which suggests that the diabetes-inducedglycosylation of proteins might increase the distribution of morphinein the aqueous compartment. These data indicate that the reducedanalgesic effect of morphine caused by diabetes cannot be explainedby a decrease in opiate-receptor affinity or density but ratherby kinetic alteration of morphine (increase of total clearanceand of volume of distribution in comparison with healthy animals).

	Introduction

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Neuropathic pain is an important complication of diabetes and clinical studies have reported the difficulty of managing iteven though antidepressants have been shown to be partially effective.The response of chronic neuropathic pain to opioid treatment iscontroversial and according to some authors, neuropathic painis intrinsically nonresponsive to opioids (Arnér and Meyerson,1988a, b), and to others, underdosing opioid medication may beresponsible for this poor activity (Portenoy et al., 1990). Experimentalmodels of diabetes have been described as relevant models of chronicpain with alterations of pain sensitivity (Calcutt et al., 1996;Courteix et al., 1993; Kamei et al., 1991; Lee and McCarty, 1990),less ability to depend physically on morphine (Shook and Dewey,1986) and poor response to opioids administered systemically (Courteixet al., 1994; Raz et al., 1988; Simon and Dewey, 1981; Simon etal., 1981) or supraspinally (Kamei et al., 1992; Suh et al., 1996).

The mechanisms by which diabetes alters morphine potency are not clear, and few explanations have been proposed. Alterationof opiate receptor affinity for [³H]naloxone has been described in brain membranes from diabetic(db/db) mice (Morley et al., 1981). Dysfunction of the supraspinalmediation of opiate analgesia (Kamei et al., 1992) and decreaseof the release of serotonin from the bulbospinal pathways (Suhet al., 1996) known to be activated by morphine (Widgor and Wilcox,1987) have been reported in diabetic rats. However, other hypotheses,poorly or never investigated in the streptozocin-induced diabeticrat model, could account for the reduced efficacy of opiates.Reduced ability of opioid drugs to bind to mu and/or delta opiatereceptors could occur, which may be revealed by a decrease inthe binding characteristics of appropriate ligands to opiate receptors,or modifications of the pharmacokinetics of morphine could occur,such as reduced production of M6G which possesses a greater potencythan morphine as a mu opioid agonist (Abbott and Palmour, 1988;Gong et al., 1991, 1992; Pasternak et al., 1987) or a lesser amountof the active drug because of an increase of its elimination.

First, this study compared the antinociceptive potency of morphine to relieve pain caused by mechanical (pressure), thermal(warm and cold) and chemical (formalin injection) stimuli in STZ-induceddiabetic rats and normal rats. The use of various stimuli ledto the determination of a complete spectrum of the antinociceptiveeffect of morphine taking into account that differences in theeffect of opiates, according to the nature of the stimulation,have been described (Hill, 1994; Millan, 1986). Moreover, thedifferent reactions assessed (i.e., paw withdrawal, tail withdrawal,paw elevation and paw licking) provided an opportunity to studythe action of morphine at different sites of integration of pain(i.e., spinal or supraspinal). Second, to investigate possibleopioid receptor changes induced by diabetes, the binding characteristicsof [³H]DAMGO and [³H]DPDPE to mu and delta opiate receptors, respectively, were determinedin diabetic and normal animals. Third, because the metaboliteM6G is a long-lasting and powerful analgesic in animals (Gonget al., 1991) and humans (Abbott and Palmour, 1988; Portenoy etal., 1992; Sullivan et al., 1989) and binds to mu and delta opiatereceptors (Hucks et al., 1992), and because M3G, another metaboliteof morphine, may antagonize the antinociceptive effect of morphine(Ekblom et al., 1993), we compared the metabolism of morphinein diabetic and normal rats. Furthermore, the usual plasma pharmacokineticparameters were determined.

	Methods

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Animals and Induction of Diabetes

Male Sprague-Dawley rats (Charles River France, Cléon, France) weighing 200 to 250 g were used. They were housed three percage under standard laboratory conditions, and given food andwater ad libitum. Because some suffering might result from thisexperiment, the IASP Committee for Research and Ethical IssuesGuidelines (Zimmermann,1983) were followed.

The rats were rendered diabetic with an intraperitoneal injection of STZ (75 mg/kg) (Zanosar, Upjohn, St. Quentin en Yvelines,France) dissolved in distilled water. Diabetes was confirmed 4weeks later by measurement of tail vein blood glucose levels withAmes Dextrostix and a reflectance colorimeter (Ames Division,Miles Laboratories, Puteaux, France). Only rats with a final bloodglucose level $>=$ 14 mM were included in the study.

Control (normal) rats received only distilled water.

Behavioral Study

Test procedures. Mechanical stimulus: the paw pressure test. The rats were submitted to the paw pressure test described previously by Randalland Selitto (1957). Nociceptive thresholds, expressed in grams,were measured with a Ugo Basil analgesimeter (Apelex; tip diameterof probe, 1 mm; weight, 30 g) by applying an increasing pressureto the left hind paw until withdrawal (cut-off was 750 g). TheAUCs of the score variations were calculated by the trapezoidalrule to compare the global effect of morphine between normal anddiabetic rats. The use of score variations (threshold values obtainedfor each experimental time-predrug threshold value) was justifiedby the difference in predrug threshold values between the twogroups.

Thermal stimuli: the tail immersion test. Before and every 30 min after drug injections, the tail of the rat was immersedin a warm (46°C, diabetic and normal rat) and a cold non-noxious(10°C, only diabetic rats, to assess thermal allodynia) waterbath until tail withdrawal or signs of struggle were observed(cut-off time was 15 sec). Before the test, each animal was adaptedto be handled. Percent MPE was calculated from the following formula:%MPE = (postdrug reaction time $-$ predrug reaction time) × 100/(15 $-$ predrug score).

Chemical stimulus: the formalin test. The rats were placed individually in plexiglass cages (40 × 40 × 40 cm) during 15 minto be adapted to the environment. Three mirrors were placed behindthe lateral walls to facilitate the observation. Five minutesafter drug injection, a subdermal injection of 50 µl of a formalinsolution (5% in saline) was given into the dorsal surface of theleft forepaw, and the animals were returned immediately to thechamber. Each animal was observed for 45 min. Pain-related behaviorwas categorized with respect to its severity with a numericalscale as described by Dubuisson and Dennis (1977)

. Four positionsof the injected paw were gauged and affected by a numerical scoreas follows: 0 = the injected paw is pressed normally on the floor;1 = the injected paw is allowed to make contact with the floorbut little weight is placed upon it; 2 = the paw is kept off thefloor; 3 = the injected paw is vigorously licked or chewed. Anaverage pain intensity score ranging from 0 to 3 was then calculated,according to the weight-scores technique of Dubuisson and Dennis(1977)

by multiplying the amount of time (in seconds) spent ineach category by the numerical value, summing these products anddividing by the total interval time (180 sec). An analgesic drugwould tend to elicit lower pain scores.

Treatment protocol and experimental design. Tests took place 4 weeks after the induction of diabetes. Only rats in which the reduction in pain scores at week 4 of diabeteswas more than 15% of the value obtained in normal rats (exceptfor the formalin test) were included. The animals were submittedto the nociceptive test (paw pressure or tail immersion) beforedrug injection. Once two stable threshold values were obtained,morphine or saline (NaCl, 0.9%) was injected i.v. in the caudaltail vein. Rats were arranged randomly in cages, each rat receivingeither morphine or saline in the same volume (0.1 ml/100g b.wt.).

Different doses of morphine were administered (0.5, 1, 2 or 4 mg/kg i.v.) and the experiments were performed blind by themethod of equal blocks with randomization of treatments (n = 7for each treatment). Different animals were used for each testand treatment.

Statistical analysis. Statistical significance was assessed with a two-way analysis of variance followed, when the F value was significant, by aDunnett's test to analyze the time course of the effect. Significantdifferences between normal and diabetic groups were determinedby a Student's t test. The significance level was .05.

Binding Study

Preparation of membranes. Diabetic and normal rats were decapitated and whole brains (mu opioid receptors) or cerebral cortex (delta opioid receptors)were removed rapidly and placed on ice. The first preparationstep is common to the two types of structure. The cerebral structureswere homogenized in 10 volumes (w/v) of ice-cold 50 mM Tris-HClbuffer (pH 7.7) with a Ultra Turrax homogenizer. The homogenateswere centrifuged at 48,340 × g (Beckman J2-21 M/E) for 15 minat 4°C, the pellets resuspended in 10 volumes of fresh Tris-HClbuffer and incubated at 37°C for 40 min to dissociate any receptor-boundendogenous opioid peptides. The homogenates were centrifuged againas described above. For the study of mu opioid receptors, thefinal pellet was used immediately and resuspended in 30 volumesof fresh Tris-HCl buffer to yield a final protein concentrationof 0.5 mg/ml. For the study of delta opioid receptors, the preparationwas frozen ( $-$ 70°C) until the day of use. After thawing, the pelletwas resuspended in 50 volumes of fresh Tris-HCl buffer to yielda final protein concentration of 0.1 mg/ml.

Protein concentrations were determined according to Lowry et al. (1951)

, with bovine serum albumin as standard.

Receptor binding assay. For the delta receptors, membrane suspension (0.5 mg protein/ml) was incubated with 1 to 60 nM [³H]DPDPE (25 Ci/mmol, Amersham, Les Ulis, France) in the absenceand presence of 10 µM naloxone (Sigma, St. Quentin Fallavier,France) for determination of nonspecific binding.

For mu receptors, membrane suspension (0.1 mg protein/ml) was coincubated with 0.3 to 11 nM [³H]DAMGO (60 Ci/mmol, Amersham, Les Ulis, France). Binding in thepresence of 1 µM naloxone (Sigma, St. Quentin Fallavier, France)was used to determine the nonspecific binding.

Incubations were performed in triplicate in Tris-HCl buffer at 25°C for 60 min. The reaction was terminated by filtrationthrough Whatman GF/B filters that were washed twice with 5 mlof ice-cold Tris-HCl buffer (50 mM, pH 7.7). Radioactivity wasmeasured by liquid scintillation spectrometry using a Betamaticcounter (efficiency of counting = 60%).

Data analysis. Specific binding was defined as total binding minus nonspecific binding. Data of saturation experiments were analyzed withthe programs EDBA (McPherson, 1983, 1985) and LIGAND (Munson andRodbard, 1980).

Pharmacokinetic Study

Sample collection. Diabetic (n = 9) and normal (n = 9) rats received an i.v. injection of 4 mg/kg of morphine hydrochloride. Blood samples werecollected at different times (5, 15, 30, 60, 90, 120 min afterthe injection) by intracardiac puncture under light anesthesia(halothane, 0.01% thymol). All samples were centrifuged (3000× g at 4°C for 10 min) and stored at $-$ 40°C until the assay.

Morphine and its metabolites assay. Samples were assayed by high-performance liquid chromatography with an ion-pair formation that complied with the analyticalrecommendations of some authors (Derendorf and Kaltenbach, 1986;Zoer et al., 1986; Konishi et al., 1990). Extraction conditionsand limits of quantification for morphine were improved markedly.Morphine, N-ethylnormorphine (internal standard) and glucuronides(M3G and M6G) were purchased from Asta Medical Laboratories (Mérignac,France) and used without further purification. The method usedconsisted of a solid-liquid extraction procedure requiring BondElut C18 columns which need pretreatment (Varian, St. Quentinen Yvelines, France) and a connection to an Alltech vacuum manifoldsdevice (Alltech Chromatography, Templeuve, France). Plasma sample(0.5 ml) and internal standard (5.5 ng/ml in water, 50 µl) wereadded. The mobile phase, filtrated before use (HV 0.45-µm filters,Millipore, St. Quentin en Yvelines, France) was: 115 ml of acetonitrileand a dose of Pic B7 low UV reagent which were added to 885 mlof 0.01 M phosphate monobasic buffer (pH 2.1; adjusted with phosphoricacid). The samples were eluted at 30.2°C with heater equipmentat the constant flow rate of 1.2 ml/min. A 300 mm × 3.9 mm µBondapackdimethyloctadecylsilyl (10 µm) amorphous silica was used (Waters-Millipore).The equipment used was a Shimadzu two-piston LC 9A pump high-performanceliquid chromatograph (Touzard and Matignon, Vitry-sur-Seine, France)connected to a Perkin-Elmer ISS-100 autosampler (Perkin-Elmer,St. Quentin en Yvelines, France) combined, on the one hand, withan ESA Coulochem (model 5100A) electrochemical detector (detectionof both morphine and M6G, Touzard and Matignon), and on the otherhand, with a fluorescence spectrophotometer (detection of M3G)Merck F1050. To remove impurities in the mobile phase by electrolysis,the guard cell (ESA model 5020) was placed between the pump andthe automatic injector; its potential was set at +0.50 V. Detectionswere performed, on the one hand, with the ESA Coulochem operatingwith an oxidation voltage at +0.35 V (ESA analytical cell) andwith its sensitivity set at 100 nA full scale, and on the otherhand, with the fluorescence spectrophotometer ( $lambda$ _ex = 210 nm and $lambda$ _em = 350 nm). The response signals (height integrations, calculationsand plotting of the chromatograms) were carried out by a dataprocessor fitted with the I.C.S. PIC3 analytical software (InstrumentationConsommable Service, Toulouse, France).

The standards were prepared in pooled human plasma (12 drug-free volunteers) spiked with morphine and its related compoundsat concentrations ranging as follows: 1.345 to 29.93 ng/ml formorphine, 6.235 to 103.92 ng/ml for M6G and 101.64 to 1355.2 ng/mlfor M3G.

Each plasma sample was assayed in duplicate, and analytical in vivo and in vitro controls were determined.

Pharmacokinetic study. Data were analyzed by a noncompartmental method (Rowland, 1980). The programs used were Pharmac BD 1.0 and Siphar-Win. Terminalhalf-life (T_1/2, hours) was calculated by the equation: T_1/2 =ln2/ $beta$ . The area under the concentration-time curve from time zeroto time 2 h of the last sample (AUC_02h; ng·h/ml) was calculatedby the trapezoidal rule and was extrapolated to infinity. Themean residence time (M.R.T., h) was determined by the formulaof Yamaoka et al. (1978). The clearance (Cl, ml/min/kg) of morphinewas calculated by the following equation: Cl/F = Dose/AUC₀.The apparent volume of distribution (V_d, l/kg) was determinedas follows: V_d = Cl/ $beta$ . T_max, C_max and C_2h were experimental values.

Result expression and statistical analysis. Plasma concentrations are expressed in nanograms per milliliter. Results are expressed as mean ± S.E.M. Statistical significancewas assessed with a two-way analysis of variance, followed bya Dunnett's t test to analyze the time course of the effect whenthe F value was significant. Significant differences between normaland diabetic groups were determined by a Student's t test. Thesignificance level was .05.

	Results

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Effect of Morphine on Nociceptive Tests

Mechanical stimulus. Before morphine injection, withdrawal thresholds of normal rats (from 123.3 ± 4.8 to 134.3 ± 6.6 g) were significantly higher(P < .01) than those of diabetic rats (from 80.0 ± 2.9 to 82.9± 1.8 g). Morphine (2 and 4 mg/kg) dose-dependently and significantly(F = 3.254, P = .0009 and F = 4.813, P < .0001, respectively)increased thresholds in normal rats (fig. 1A). The maximum increaseat 40 min was +60 ± 21 g and +152 ± 32 g for 2 and 4 mg/kg morphine,respectively. This antinociceptive effect lasted 50 and 100 minafter the injection of 2 and 4 mg/kg, respectively.

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Fig. 1. Time course of the effect of several i.v. doses of morphine on mechanical pain thresholds in normal (A) and diabetic (B) rats. Paw withdrawal thresholds determined before (0) and after drug injection are expressed in grams. (C) Effect of morphine on pain thresholds in normal and diabetic rats. Results are expressed as the mean surface bounded by the time-course curves (AUC) of score variations (postdrug-predrug threshold values) calculated by the trapezoidal rule. Bars = S.E.; n = 7 for each morphine or saline-treated group. *P < .05 versus corresponding predrug values; $dagger$ P < .05 versus scores obtained in corresponding normal rats.

In diabetic rats a significant (F = 3.553, P = .0005) antinociceptive effect could be observed only at 4 mg/kg (fig. 1B).The maximum increase was +41 ± 16 g at 10 min, and the effectlasted 60 min after the injection.

The determination of the AUC bounded by the time-course curves of the variations of withdrawal thresholds (fig.1C) confirmedthe dose-dependent antinociceptive effect in diabetic and normalrats, and showed a significant difference between scores obtainedin normal and diabetic rats for 4 mg/kg.

Thermal stimuli. Tail immersion in a 46°C water bath. Initial tail withdrawal delays were from 7.1 ± 0.5 to 8.7 ± 0.4 sec and from 5.3 ± 0.5to 6.1 ± 0.4 sec in normal and diabetic rats, respectively. Thesignificant difference (P < .01) between these scores confirmsthe diabetes-induced hyperalgesia (fig. 2, A and B).

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Fig. 2. Effect of several i.v. doses of morphine on tail withdrawal of normal (A) and diabetic (B) rats submitted to the tail immersion test in warm (46°C) water. Percentages of maximal possible effect (%MPE) are reported before (0) and after drug injections. Bars = S.E.; n = 7 for each morphine or saline-treated group. *P < .05, **P < .01, ***P < .001 versus corresponding predrug values.

Morphine dose-dependently increased the scores in normal rats (fig. 2A). Its antinociceptive effect corresponded to a MPEof 63 ± 19% for 1 mg/kg (F = 4.22, P = .0123), 79 ± 12% (F = 6.99,P = .0011) for 2 mg/kg and 88 ± 4% (F = 45.5, P < .0001) for 4mg/kg at 30, 30 and 120 min after the injection, respectively.

In diabetic rats (fig. 2B), only the doses of 2 and 4 mg/kg induced a significant antinociceptive effect, maximal at 30 and120 min, respectively (MPE = 52 ± 12% and 69 ± 4%, respectively).

Tail immersion in a 10°C water bath. Predrug values of the tail withdrawal threshold were from 5.6 ± 0.4 to 7.5 ± 1.2 secin diabetic rats (fig. 3). Morphine at the two lowest doses (0.5and 1 mg/kg) did not induce any significant effect. On the otherhand, 2 mg/kg morphine induced a significant antiallodynic effect(F = 19.84, P < .0001) from 30 to 120 min. The MPE was 92 ± 8%30 min after the injection.

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Fig. 3. Effect of several i.v. doses of morphine on tail withdrawal thresholds of diabetic rats submitted to the tail immersion test in cold (10°C) water. Percentages of maximal possible effect (%MPE) are reported before (0) and after drug injections. Bars = S.E.; n = 7 for each morphine or saline-treated group. *P < .05, *** P < .001 versus corresponding predrug values.

Chemical stimulus. Formalin-induced hyperalgesia was significantly (P < .05) more marked in diabetic (fig. 4B) than in normal (fig. 4A) rats.The scores of the first 3 min were 1.57 ± 0.16 and 1.93 ± 0.07in normal and diabetic animals, respectively. The duration ofthe first phase was longer in diabetics (0-18 min) than in normal(0-9 min) rats. In diabetic animals, hyperalgesia of the secondphase was significantly more intensive (P < .05) from the 18thto the 27th min than in normal rats.

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Fig. 4. Effect of i.v. morphine (2 mg/kg) on behavioral scores obtained after injection of formalin (5%) in the forepaw of normal (A) and diabetic (B) rats. Scores are the mean time (±S.E.M.) spent in the specific behavioral categories and affected by their category weights; bars = S.E.; n = 7 for each morphine- or saline-treated group. *P < .05, **P < .01, ***P < .001 versus scores obtained after NaCl (0.9%).

In normal rats, morphine (2 mg/kg) was ineffective on the acute phase but significantly decreased scores from the 27th tothe 45th min post-formalin injection. Compared with values obtainedin saline-treated rats, the decreases varied from 71 ± 19% to86.1 ± 13.9%.

In diabetic rats, morphine significantly reduced the scores of the two phases. The reduction of the first phase was 24 ± 10%at 0 to 3 min. The maximal scores obtained were similar to thoseof normal rats injected with saline (1.47 ± 0.18 and 1.57 ± 0.16,for the first 3-min block, respectively). Morphine significantlyreduced the scores of the second phase of 51 ± 14%, 60 ± 15% and74 ± 17%, 21 to 24, 33 to 36 and 42 to 45 min after the formalininjection, respectively. However, this effect is significantlylower (P < .05) than that observed in normal rats for the correspondingtimes.

[³H]DAMGO and [³H]DPDPE Binding

No significant difference was observed in the binding of [³H]DAMGO to brain mu receptors between normal and diabetic rats.K_D values were 1.52 ± 0.26 nM and 1.54 ± 0.45 nM, respectively,and B_max values were 189.3 ± 9.4 fmol/mg protein and 163.3 ± 22.1fmol/mg protein, respectively. The binding characteristics of[³H]DPDPE to delta receptors in diabetic rats were not significantlydifferent from those obtained in normal animals. The K_D and B_maxvalues were 5.71 ± 0.62 nM and 151.3 ± 9.8 fmol/mg protein, respectively,in diabetic rats, and 4.63 ± 0.29 nM and 129.7 ± 10.7 fmol/mgprotein, respectively, in normal rats.

Pharmacokinetics of Morphine and Its Metabolites

The pharmacokinetic parameters for morphine and its metabolites are shown in table 1. No significant variation was observedbetween diabetic and normal rats for C_max, T_1/2, AUC and MRT valuesof either morphine or its metabolites. However, morphine Cl andV_d were increased significantly in diabetic rats, whereas no significantchange was observed for its metabolites M3G and M6G between diabeticand normal animals.

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TABLE 1
Pharmacokinetic parameters for morphine and its metabolites in diabetic (D) and normal (N) rats

	Discussion

Top Abstract Introduction Methods Results Discussion References

The present results in STZ-treated rats confirm that diabetes induces alterations of nociceptive thresholds and clearly indicatethat morphine-induced analgesia is attenuated in diabetic animals,whatever the nature (mechanical, thermal, chemical) or the intensity(noxious or non-noxious) of the applied stimulation and the levelof integration (spinal or supraspinal) of the response. This univocalresult distinguishes this model from the model described by Bennettand Xie (1988). In this model of neuropathic pain in which a chronicconstrictive nerve injury produces allodynia and hyperalgesia,the efficacy of opioids is increased (Attal et al., 1991) or reduced(Yamamoto and Yaksh, 1992) according to the stimuli (mechanicaland thermal, respectively).

As reported previously on vocalization thresholds (Courteix et al., 1994), 2-fold higher doses of morphine are necessary toincrease withdrawal thresholds in diabetic rats in comparisonwith normal rats. This demonstrates that both spinal (paw withdrawal)and supraspinal (vocalization) responses are depressed in diabeticrats. This alteration of both spinal and supraspinal responsesto pain was reported also by Kamei et al. (1992) with use of thetail-pinch (supraspinal response) and tail-flick (spinal response)tests in STZ diabetic mice. In the same way, an alteration ofcontent and/or release of endogenous opioid peptides at both spinaland supraspinal levels as well as changes in their interactionwith opiate receptors has been suggested in diabetic mice (Ramabadranet al., 1989). Taken together, literature data and the presentresults show that diabetes induces a generalized alteration thatmodifies the activity of morphine at the spinal and supraspinallevel.

The reduced efficacy of morphine was confirmed by use of a thermal nociceptive stimulation (tail immersion in a 46°C waterbath). The dose of 1 mg/kg was devoid of activity in diabeticrats, whereas it increased tail withdrawal latency in normal rats.Furthermore, the MPE values obtained with 2 and 4 mg/kg morphinewere significantly lower in diabetic (52 ± 12% and 69 ± 4%, respectively)than in normal rats (79 ± 12% and 88 ± 4%, respectively). Theneed to reach the dose of 2 mg/kg to alleviate thermal allodynia(cold stimulation) confirms the poor sensitivity to morphine ofdiabetic animals. For the dose of 2 mg/kg, the activity of morphinewas more effective in countering allodynia (MPE = 92 ± 5%) thanin reducing hyperalgesia caused by warm stimulation (MPE = 52± 12%). The impairment of morphine efficacy in thermal pain testsagrees with previous results of Simon and Dewey (1981) and Simonet al. (1981) which showed that acute or chronic hyperglycemiareduced the antinociceptive effect of morphine subcutaneouslyadministered in the tail-flick test. Raz et al. (1988) by useof the hot plate test also showed a reduction of morphine analgesiain hyperglycemic rats. The intracerebroventricular injection ofmorphine resulted in an alteration of the response mediated bysupraspinal mu opiate receptors measured by the tail-flick assay(Kamei et al., 1992; Suh et al., 1996). Finally, Ramabadran etal. (1989), with use of the same test but with a stimulus temperatureof 50°C, demonstrated that the hyperalgesic response to naloxonewas abolished in diabetic mice.

In the formalin test, the scores of the two phases were significantly greater in diabetic rats than in normal rats as describedpreviously by Malmberg et al. (1993). Morphine significantly decreasedresponses in both the early and the late phase of the formalintest in diabetic rats. In normal rats, an antinociceptive effectwas reached only on the late phase; the lack of effect of morphineon the early phase was inconsistent with literature data (Dubuissonand Dennis, 1977) even though morphine-induced score reductionof the first phase is usually lower than that of the second phase.Despite this discrepancy, the comparison between normal and diabeticrats clearly shows a significantly lower decrease in the secondphase scores after morphine injection in diabetic rats than innormal animals.

To resolve whether prolonged hyperglycemia affects the affinity and the density of brain mu and delta receptors, we investigatedthe saturation curves of tritiated DAMGO and DPDPE to membranepreparations from diabetic and normal rats. Whole brain and totalcortex were used to give a general approach of the effect of STZtreatment on cerebral opioid receptors, assuming that if alterationsoccurred, they would be revealed on total brain or cortex. Thus,the reduction of the analgesic activity of morphine in diabeticrats cannot be explained by a variation of K_D and B_max valuesfor mu and delta opioid receptors, because no significant changeis evident in comparison with K_D and B_max values for both opioidreceptor subtypes in normal rats. However, although the differencesin mu and delta receptors were not statistically significant,the density of the mu binding sites was reduced by approximately14% by STZ treatment. On the other hand, B_max for DPDPE on deltareceptors seemed to be (but not significantly) increased by approximately17%. These data suggest that the opioid receptor populations areimbalanced after STZ treatment. The use of another methodology(i.e., membrane pretreatment with Na⁺ and GDP and binding in presence of GDP), as recently describedby Liu-Chen et al. (1995), could have revealed small changes inreceptor binding. However that may be, our conditions are thesame as used by Adams et al. (1987), who successfully have reportedalterations (a 20-31% reduction) in mu binding sites in rat braininduced by $beta$ -funaltrexamine treatment. Finally, because our studycarried out in whole-brain homogenate did not show changes ofopioid receptor binding, it is also possible that uncoupling ofG-protein with the mu opiate receptor and/or changes in mu opiatereceptor-associated second messenger systems might result in thereduced effectiveness of morphine, as suggested by Mao et al.(1995) in an animal model of neuropathic pain.

Because the relationship between opioid concentration and analgesic efficacy is steep (Levine et al., 1983), the pharmacokineticbehavior of morphine, M3G and M6G, was considered in additionto opiate receptor exploration. In normal rats, the obtained morphineCl, V_d and T_1/2 values are similar to those reported by Hasselströmet al. (1996). The amount of M6G formed after the administrationof morphine is negligible (Hasselström et al., 1996) or absent(Coughtrie et al., 1989) in rats, compared with the amount ofM6G found in humans (Coughtrie et al., 1989; Stain et al., 1995).In our study, morphine was converted to M3G as the major metabolite.However, the M3G and M6G kinetic parameters reported (Hasselströmet al., 1989) were obtained after injection of each metaboliteand consequently cannot be compared with ours.

In diabetic rats, some pharmacokinetic parameters of morphine such as V_d and Cl are modified. The increase of V_d might becaused by glycosylation of plasma proteins, reported previouslyin diabetic patients (Gwilt et al., 1991), which can alter theprotein binding and increase the unbound fraction of morphine.Because morphine and glucuronides are hydrophilic compounds, highamounts may be attracted in aqueous compartments. Thus, it ispossible that the amount of morphine in blood crossing the brain-bloodbarrier and present in the central nervous system is reduced.The existence of a relationship between the intensity of analgesiaand the levels of morphine and its glucuronide metabolites inthe cortical extracellular fluid (Barjavel et al., 1995) has beendemonstrated by use of the microdialysis procedure. Consequently,a much greater fraction of morphine might reach the biophase innormal rats than in diabetic rats, which explains the differenceof potency of the drug.

Total clearance of morphine also is increased. This probably is not related to variations of hepatic metabolism despite thepreviously described impaired metabolic activity of hepatocytesfrom STZ rats toward xenobiotics (Favreau and Schenkman, 1988)but rather may be related to the well-known modifications of renalfunction described in humans (Gwilt et al., 1991), especiallythe increase of glomerular filtration occurring in early diabetesmellitus. The higher total clearance observed in diabetic ratsthan in normal rats clearly means that frequent doses will berequired to maintain the same blood concentration in the two groupsof animals as it is the rule in humans (Mather, 1987).

Thus, both the increase of morphine Cl, which results in a nonsignificant reduction of morphine AUC by approximately 37%,and the increase of morphine V_d, which results in a high diffusionof morphine in the aqueous compartment, can lead to a reductionof available morphine and to a decrease of its amount in the targetorgans, i.e., in the central nervous system. These two processmay explain the reduced effect of morphine, despite the unmodifiedT_1/2. The examination of experimental values obtained from thepaw pressure test and plasma morphine levels tended to show thathigher morphine levels would be necessary in diabetic rats toobtain the same pharmacological effect as observed in normal rats.

The present study fails to show any change in morphine metabolism. For morphine, phase II reactions are the most importantmetabolic reactions, and glucuronidation is the major reactionin humans, but this process is species dependent (Xu et al., 1993).Taking into account (1) the increased $beta$ -glucuronidase activityobserved in diabetes (Rao et al., 1989) and (2) the previouslyreported increase of glucuronidation of the hydroxylated metabolitesof amitriptyline in STZ-induced diabetic rats (Coudoré et al.,1996), increases of M3G and M6G were expected, and the unchangedpharmacokinetics of morphine glucuronides observed in this studywas surprising. Nevertheless, M3G/morphine and M6G/morphine AUCratios obtained in diabetic rats (5.10 and 0.20, respectively)tends to be higher than those obtained in normal rats (2.93 and0.16, respectively). It is possible that an increase of glucuronidationmay occur but that it is compensated by the increase of morphineand/or glucuronide elimination. Because glucuronide pharmacokineticparameters remain unchanged, this phenomenon does not influencemorphine analgesic activity. However, in rats, despite contradictoryreports, morphine glucuronidation, especially in the 6-positionseems to be deficient (Oguri et al., 1990; Kuo et al., 1991) andeventual modifications may be not observed. Specific in vitrostudies on morphine metabolism with hepatocytes from STZ-diabeticrats and in vivo behavioral studies with direct administrationof M6G and M3G would be necessary.

Study of phase I metabolism was impossible because levels of oxided metabolites, N-demethylated morphine and morphine-N-oxide,or of the O-methylated metabolite, codeine, were not assessed.However, the oxidation reaction minor pathways of morphine metabolismand the activity of the specific cytochrome P450 involved in theformation of codeine, i.e., cytochrome P2D6, were unchanged inhuman diabetes mellitus (Bechtel et al., 1988), contrary to thoseobserved with other cytochrome P450 isoenzymes in STZ-diabeticrats (Favreau and Schenkman, 1988).

To conclude, the data reported herein confirm that diabetes-induced hyperglycemia alters pain sensitivity by inducing mechanical,thermal and chemical hyperalgesia and thermal allodynia. Theyshow that this metabolic trouble reduced the antihyperalgesicand antiallodynic activity of morphine whatever the nature ofstimulus applied and the level of integration of pain reaction.This reduced efficacy is not caused by significant changes inthe binding parameters for brain mu and delta opiate receptors.The meaningful explanation is in the pharmacokinetic alterationof morphine (increase in V_d and Cl) which could lead to the reductionof morphine levels in central nervous system. However, furtherinvestigations are needed to determine the involvement of someendogenous systems that are involved in opiate analgesia. Then,the recent demonstration of the decrease in morphine antinociceptioncaused by activation of N-methyl-D-aspartate receptors (Mao etal., 1995) and of the modulatory role of antiopioid peptides (neuropeptideFF or cholecystokinin) in acute and chronic pain states (Gouardèreset al., 1996; Stanfa et al., 1994, respectively) would justifyspecific studies in diabetic rats.

	Footnotes

Accepted for publication December 12, 1997.

Received for publication April 29, 1997.

¹ Current address: Service de Pharmacie Clinique, Institut Gustave-Roussy, 39, rue Camille Desmoulins, F-94805 Villejuif, CedexFrance.

² Current address: Laboratoires UPSA, 128 rue Danton, F-92506 Rueil-Malmaison.

³ Current address: Equipe NPPUA, Laboratoire de Pharmacologie Médicale, Faculté de Médecine, Place H. Dunant, BP 38, F-63001Clermont-Ferrand Cedex 1.

Send reprint requests to: C. Courteix, Laboratoire de Pharmacologie, Faculté de Pharmacie, Place H. Dunant BP 38, F-63001 Clermont-Ferrand, France.

	Abbreviations

AUC, area under the curve; C_max, maximal concentration; Cl, total clearance; i.v., intravenously; MPE, maximum possible effect; MRT, mean residence time; M3G, morphine-3-glucuronide; M6G, morphine-6-glucuronide; S.E.M., standard error of the mean; STZ, streptozocin; T_1/2, elimination half-life time; T_max, delay to reach C_max; V_d, apparent volume of distribution; DAMGO, [D-Ala²,(Me)Phe⁴,Gly(ol)⁵]enkephalin; DPDPE, [DPen²,D-Pen⁵]enkephalin.

	References

Top Abstract Introduction Methods Results Discussion References

Abbott FV and Palmour RM (1988) Morphine-6-glucuronide: Analgesic effects and receptor binding profile in rats. Life Sci 43: 1685-1695[Medline].
Adams JU, Andrews JS, Hiller JM, Simon EJ and Holtzman SG (1987) Effects of stress and $beta$ -funaltrexamine pretreatment on morphine analgesia an opioid binding in rats. Life Sci 41: 2835-2844[Medline].
Arnér S and Meyerson BA (1988a) Lack of analgesic effect of opioids on neuropathic and idiopathic forms of pain. Pain 33: 11-23[Medline].
Arnér S and Meyerson BA (1988b) Reply to Howard Fields on "Can opiates relieve neuropathic pain ?" Pain 35: 366-367.
Attal N, Chen YI, Kayser V and Guilbaud GL (1991) Behavioural evidence that systemic morphine may modulate a phasic pain-related behaviour in a rat model of peripheral mononeuropathy. Pain 47: 65-70[Medline].
Barjavel MJ, Scherrmann J-M and Bhargava HN (1995) Relationship between morphine analgesia and cortical extracellular fluid levels of morphine and its metabolites in the rat: a microdialysis study. Br J Pharmacol 116: 3205-3210[Medline].
Bechtel CY, Joanne C, Grandmottet M and Bechtel RP (1988) The influence of insulin-dependent diabetes on the metabolism of caffeine and the expression of the debrisoquin oxidation phenotype. Clin Pharmacol Ther 44: 408-417[Medline].
Bennett GJ and Xie YK (1988) A peripheral mononeuropathy in rat that produces pain disorders like those seen in man. Pain 33: 87-107[Medline].
Calcutt NA, Jorge MC, Yaksh TL and Chaplan SR (1996) Tactile allodynia and formalin hyperalgesia in streptozotocin-diabetic rats: effects of insulin, aldose reductase inhibition and lidocaine. Pain 68: 293-299[Medline].
Coudoré F, Besson A, Courteix C, Eschalier A, Lavarenne J and Fialip J (1996) Pharmacokinetics of amitriptyline and its demethylated and hydroxylated metabolites in streptozocin-induced diabetic rats. Gen Pharmacol 5: 803-807.
Coughtrie MWH, Ask B, Rane A, Burchell B and Humes R (1989) The enantioselective glucuronidation of morphine in rats and humans. Evidence for the involvement of more than one UDP-glucuronosyltransferase isoenzyme. Biochem Pharmacol 38: 3273-3280[Medline].
Courteix C, Eschalier A and Lavarenne J (1993) Streptozocin-induced diabetic rats: behavioural evidence for a model of chronic pain. Pain 53: 81-88[Medline].
Courteix C, Bardin M, Chantelauze C, Lavarenne J and Eschalier A (1994) Study of the pharmacological sensitivity of the diabetes-induced pain model in rats to a range of analgesics. Pain 57: 153-160[Medline].
Derendorf H and Kaltenbach M (1986) Coulometric high-performance liquid chromatographic analysis of morphine in biological fluids. J Pharm Sci 75: 1198-1200[Medline].
Dubuisson D and Dennis SG (1977) The formalin test: A quantitative study of the analgesic effects of morphine, meperidine and brain stem stimulation in rats and cats. Pain 4: 161-174[Medline].
Ekblom M, Gardmark M and Hammarlund-Udenaes M (1993) Pharmacokinetics and pharmacodynamics of morphine-3-glucuronide in rats and its influence on the antinociceptive effect of morphine. Biopharm Drug Dispos 14: 1-11[Medline].
Favreau LV and Schenkman JB (1988) Composition change in hepatic microsomal cytochrome P450 during onset of streptozocin-induced diabetes and during insulin treatment. Diabetes 37: 577-584[Abstract].
Gong QL, Hedner J, Björkman R and Hedner T (1992) Morphine-3-glucuronide may functionally antagonize morphine-6-glucuronide induced antinociception and ventilatory depression in the rat. Pain 48: 249-256[Medline].
Gong QL, Hedner T, Hedner J, Bjorkman R and Nordberg G (1991) Antinociceptive and ventilatory effects of the morphine metabolites: Morphine-6-glucuronide and morphine-3-glucuronide. Eur J Pharmacol 193: 47-56[Medline].
Gouardères C, Jhamandas K, Sutak M and Zajac J-M (1996) Role of opioid receptors in the spinal antinociceptive effects of neuropeptide FF analogues. Br J Pharmacol 117: 493-501[Medline].
Gwilt PR, Nahhaas RR and Tracewell WG (1991) The effects of diabetes mellitus on pharmacokinetics and pharmacodynamics in humans. Clin Pharmacokinet 20: 477-490[Medline].
Hasselström J, Svensson JO, Wiesenfield-Hallin Z, Yue Q-Y and Xu X-J (1996) Disposition and analgesic effects of systemic morphine, morphine-6-glucuronide and normorphine in rat. Pharmacol Toxicol 79: 40-46[Medline].
Hill RG (1994) Pharmacological considerations in use of opioids in the management of pain associated with nonterminal disease states. Pain Rev 1: 47-61.
Hucks D, Thompson PI, McLoughlin L, Joel SP, Patel N, Grossman A, Rees L and Slevin ML (1992) Explanation at the opioid receptor level for differing toxicity of morphine and morphine-6-glucuronide. Br J Cancer 65: 122-126[Medline].
Kamei J, Ohhashi Y, Aoki T and Kasuya Y (1991) Streptozotocin-induced diabetes in Mice reduces the nociceptive threshold, as recognized after application of noxious mechanical stimuli but not for thermal stimuli. Pharmacol Biochem Behav 39: 541-544[Medline].
Kamei J, Ohhashi Y, Aoki T, Kawasima N and Kasuya Y (1992) Streptozocin-induced diabetes selectively alters the potency of analgesia produced by µ-opioid agonists, but not by $partial$ - and K-opioid agonists. Brain Res 571: 199-203[Medline].
Konishi M and Hashimoto H (1990) On-line clean-up system of plasma sample for simultaneous determination of morphine and its metabolites in cancer patients by high-performance liquid chromatography. J Pharm Sci 79: 379-383[Medline].
Kuo CK, Hanioka N, Hoshikawa Y, Oguri K and Yoshimura H (1991) Species difference of site-selective glucuronidation of morphine. J Pharmacobio-Dyn 14: 187-193[Medline].
Lee JH and McCarty RC (1990) Glycemic control of pain threshold in diabetic and control rats. Physiol Behav 47: 225-230[Medline].
Levine J, Gordon NC, Poole T and Benowitz N (1983) Relationship of duration of analgesia to opioid pharmacokinetic variables. Brain Res 289: 391-394[Medline].
Liu-Chen L-Y, Yang H-H, Li S and Adams JU (1995) Effect of intracerebroventicular $beta$ -funaltrexamine on µ-opioid receptors binding in the rat brain: Consideration of binding condition. J Pharmacol Exp Ther 273: 1047-1056[Abstract/Free Full Text].
Lowry OH, Rosebrough NJ, Farr AL and Randall RJ (1951) Protein measurement with the folin phenol reagent. J Biol Chem 193: 265-269[Free Full Text].
Malmberg AB, Yaksh TL and Calcutt NA (1993) Antinociceptive effects of GM1 ganglioside derivative Agf 44 on the formalin test in normal and streptozotocin- diabetic rats. Neurosci Lett 161: 45-48[Medline].
Mather LE (1987) Opioid pharmacokinetics in relation to their effects. Anaesthesiol Intensive Care Med 15: 15-22.
Mao J, Price DD and Mayer DJ (1995) Mechanisms of hyperalgesia and morphine tolerance: a current view of their possible interactions. Pain 62: 259-274[Medline].
McPherson GA (1983) A practical computer-based approach to the analysis of radioligand binding experiments. Comput Programs Biomed 17: 107-114[Medline].
McPherson GA (1985) Analysis of radioligand binding experiments: a collection of computer programs for the IBM PC. J Pharmacol Methods 14: 313-228[Medline].
Millan MJ (1986) Multiple opioid systems and pain. Pain 27: 303-347[Medline].
Morley GK, Mooradian AK, Levine AD and Morley JE (1984) Mechanisms of pain in diabetic peripheral neuropathy. Effect of glucose on pain perception in humans. Am J Med 77: 79-82[Medline].
Morley JE, Levine AS, Hess SA, Brown DM and Handwerger BS (1981) Evidence for in vivo and in vitro modulation of the opiate receptor by glucose. Soc Neurosci Abstr 7: 854.
Munson PJ and Rodbard D (1980) Ligand: A versatile computerized approach for characterization of ligand-binding systems. Anal Biochem 107: 1247-1254.
Oguri K, Hanioka N and Yoshimura H (1990) Species difference in metabolism of codeine urinary excretion of codeine glucuronide, morphine-3-glucuronide and morphine-6-glucuronide in mice, rats, guinea pigs and rabbits. Xenobiotica 20: 683-688[Medline].
Pasternak GW, Bodnard RJ, Clark JA and Inturrisi CE (1987) Morphine-6-glucuronide, a potent mu agonist. Life Sci 41: 2845-2849[Medline].
Portenoy RL, Foley KM and Inturrisi CE (1990) The nature of opioid responsiveness and its implications for neuropathic pain: New hypotheses derived from studies of opioid infusions. Pain 43: 273-286[Medline].
Portenoy RK, Thaler HT, Inturrisi CE, Friedlander-Klar H and Foley KM (1992) The metabolite morphine-6-glucuronide contributes to the analgesia produced by morphine infusion in patients with pain and normal renal function. Clin Pharmacol Ther 51: 422-431[Medline].
Ramabadran K, Bansinath M, Turndorf H and Puig MM (1989) The hyperalgesic effect of naloxone is attenuated in streptozocin-diabetic mice. Psychopharmacology 97: 169-174[Medline].
Randall LO and Selitto JJ (1957) A method for measurement of analgesic activity on inflamed tissue. Arch Int Pharmacodyn 61: 409-419.
Rao GMM, Morghom LO and Abukhris AA (1989) Serum beta-glycosidases in diabetes mellitus. Clin Physiol Biochem 7: 161-164[Medline].
Raz I, Hasdai D, Seltzer Z and Melmed RN (1988) Effect of hyperglycemia on pain perception and on efficacy of morphine analgesia in rats. Diabetes 37: 1253-1259[Abstract].
Shook JE and Dewey WL (1986) Morphine dependence and diabetes: The development of morphine dependence in streptozotocin-diabetic rats and spontaneously diabetic C57BL/Ksj mice. J Pharmacol Exp Ther 237: 841-847[Abstract/Free Full Text].
Simon GB and Dewey WL (1981) Narcotics and diabetes. I. The effects of STZ-induced diabetes on the antinociceptive potency of morphine. J Pharmacol Exp Ther 218: 318-323[Abstract/Free Full Text].
Simon GB, Borzelleca J and Dewey WL (1981) Narcotics and diabetes. II. STZ-induced diabetes selectively alters the potency of certain narcotic analgesics. Mechanism of diabetes: Morphine interaction. J Pharmacol Exp Ther 218: 324-329[Abstract/Free Full Text].
Stain F, Barjavel MJ, Sandouk P, Plotkine M, Scherrmann J-M and Bhargava HN (1995) Analgesic response and plasma and brain extracellular fluid pharmacokinetics of morphine and morphine-6- $beta$ -D-glucuronide in the rat. J Pharmacol Exp Ther 274: 852-857[Abstract/Free Full Text].
Stanfa LC, Dickenson A, Xu X-J and Wiesenfield-Hallin Z (1994) Cholecystokinin and morphine analgesia: variations on a theme. Trends Pharmacol Sci 15: 65-66[Medline].
Suh HW, Song D-K, Wie M-B, Jung J-S, Hong H-E, Choi S-R and Kim Y-H (1996) The reduction of the antinociceptive effect of morphine administered intracerebroventricularly is correlated with the decrease of serotonin release from the spinal cord in streptozocin-induced diabetic rats. Gen Pharmacol 27: 445-450[Medline].
Sullivan AF, McQuay HJ, Bailey D and Dickenson AH (1989) The spinal antinociceptive actions of morphine metabolites morphine-6-glucuronide and normorphine in the rat. Brain Res 482: 219-224[Medline].
Widgor S and Wilcox GL (1996) Central and systemic morphine-induced antinociception in mice: contribution of descending serotonergic and noradrenergic pathways. J Pharmacol Exp Ther 242: 90-95[Abstract/Free Full Text].
Xu BQ, Bjorneboe A, Ripel A, Aasmundstad TA, Christophersen AS and Morland J (1993) Ethylmorphine metabolism in isolated rat hepatocytes. Pharmacol Toxicol 73: 35-40[Medline].
Yamamoto T and Yaksh TL (1992) Studies on the spinal interaction of morphine and the NMDA antagonist MK-801 on the hyperesthesia observed in a rat model of sciatic mononeuropathy. Neurosci Lett 135: 67-70[Medline].
Yamaoka K, Nakagawa W and Uno T (1978) Statistical moments in pharmacokinetics. J Pharmacokinet Biopharm 6: 547-558[Medline].
Zimmermann M (1983) Ethical guidelines for investigations of experimental pain in conscious animals. Pain 16: 109-110[Medline].
Zoer J, Virgili P and Henry JA (1986) High-performance liquid chromatographic assay for morphine with electrochemical detection using an unmodified silica column with non-aqueous ionic eluent. J Chromatogr 382: 189-197[Medline].

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