Insulin Attenuates Formalin-Induced Nociceptive Response in Mice through a Mechanism that Is Deranged by Diabetes Mellitus

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Vol. 281, Issue 1, 315-321, 1997

Insulin Attenuates Formalin-Induced Nociceptive Response in Mice through a Mechanism that Is Deranged by Diabetes Mellitus

Nobuaki Takeshita and Isamu Yamaguchi

Basic Research Group, Tsukuba Research Laboratories, Fujisawa Pharmaceutical Co. Ltd., 5-2-3 Tokodai, Tsukuba, Ibaraki 300-26, Japan

	Abstract

Top Abstract Introduction Methods Results Discussion References

Although hypoglycemic doses of insulin (0.24-7.5 U/kg s.c.) did not significantly change acetic acid-induced writhing in mice,they dose-dependently attenuated formalin-induced nociceptiveresponses, and their effects were more potent on the second phase(ID₅₀ = .62 U/kg) than on the first (ID₅₀ > 7.5 U/kg). Intracerebroventriculardoses of insulin (250-1000 µU/animal) mimicked the effects ofthe s.c. dose, but caused little change in blood glucose levels.The antinociceptive activity of insulin (0.75 U/kg, s.c.) in theformalin test was significantly inhibited by naloxone (10 mg/kgi.p., an opiate receptor antagonist), sulpiride (10 mg/kg i.p.,a dopamine 2 receptor antagonist), pindolol (1 mg/kg i.p., a 5-hydroxytryptamine1 receptor antagonist) and ketanserin (1 mg/kg i.p., a 5-hydroxytryptamine2 receptor antagonist), but not by 3-tropanyl-indole-3-carboxylate(1 mg/kg i.p., a 5-hydroxytryptamine 3 receptor antagonist). Insulinalso exerted antinociception in streptozotocin-induced diabeticmice and genetically diabetic db/db mice which, however, wereless sensitive (ID₅₀s around 7.5 U/kg) to the of insulin effectthan normal mice. The results suggest that insulin attenuateschronic rather than acute pains through a mechanism mediated bydopamine, 5-hydroxytryptamine and opioids. The antinociceptivepathway appears to be deranged by diabetes mellitus.

	Introduction

Top Abstract Introduction Methods Results Discussion References

Davis et al. (1956) were the first to report that insulin-induced hypoglycemia potentiated the antinociceptive action of morphinein the rat tail-flick test. This was confirmed by later studiesdemonstrating that insulin potentiates the antinociceptive effectsof sodium salicylates (Wisniewski and Zarebski, 1968) and morphine(Singh et al., 1983), while Simon and Dewey (1981) and Simon etal. (1981) reported that streptozotocin- induced diabetic miceand rats as well as genetically diabetic db/db mice are significantlyless sensitive to the antinociceptive effect of morphine in thetail-flick test. This evidence indicated that blood glucose levelsaffect pain perception mechanisms, and has given a theoreticalbasis for the hyperalgesia in diabetic patients.

The abovementioned experiments measure transient pain induced by brief exposure to physical stresses, although the most frequentlyencountered complaints in patients are of continuous pain, usuallyof pathological origin. The formalin test was originally describedin rats and cats by Dubuisson and Dennis (1977), and the s.c.injection of formalin produced a biphasic pain response in rats.Several lines of evidence have indicated that the first phaserepresents a phasic pain response to direct stimulation of thenerve endings, and the second phase represents a tonic pain responseto subsequent inflammation (Dubuisson and Dennis, 1977; Shibataet al., 1989). However, only a few drugs have been studied inthe formalin test, especially for their effects in diabetic animals(Acton et al., 1992; Calcutt et al., 1994; Takeshita et al., 1995;Takeshita and Yamaguchi, 1995).

Using the formalin test, we recently found that the antinociceptive activity of morphine was significantly reduced in STZ-induceddiabetic mice, but was not changed in the genetically diabeticdb/db mice compared with their controls (Takeshita et al., unpublishedobservation). Although hyperglycemia is common in both STZ-induceddiabetic mice and db/db mice, the latter are hyperinsulinemic,and the former are hypoinsulinemic (Coleman and Hummel, 1967;Kodama et al., 1994). This in combination with the evidence citedabove led us to hypothesize that hyperinsulinemia in the db/dbmice might have potentiated the analgesic effect of morphine andcompensated for the attenuated pain perception mechanism due tohyperglycemia. During the course of a study on the synergism betweenmorphine and insulin, we found that insulin injection per se inducesantinociception in the formalin test.

We report on the mechanism of action of insulin in normal mice, and compare the antinociceptive effect of insulin in STZ-induceddiabetic and genetically diabetic db/db mice.

	Methods

Top Abstract Introduction Methods Results Discussion References

Materials

Bovine pancreas insulin, (±)-pindolol hydrochloride, naloxone hydrochloride and streptozotocin (STZ) were obtained from SigmaChemical Co. (St. Louis, MO). Ketanserin tartrate was from ResearchBiochemical Inc. (Natick, MA). Formalin and acetic acid were fromWako Pure Chemical Industries Ltd. (Osaka, Japan). Sulpiride and3-tropanyl-indole-3-carboxylate hydrochloride (ICS205-930) weresynthesized in our laboratory. Insulin, ketanserin, naloxone andICS205-930 were dissolved in saline. Pindolol and sulpiride weredissolved in 1% tartaric acid, adjusted to pH 7 with 1N NaOH anddiluted in saline. STZ was dissolved in 2 mM citrate buffer atpH 4.5. Formalin and acetic acid were diluted in saline. Sulpiride,naloxone, pindolol, ketanserin and ICS205-930 were administeredi.p. 30 min before the injection of insulin.

Animals

All mice were housed at 22 ± 1°C and 55 ± 5% humidity under a 12 hr light/12 hr dark cycle and given free access to waterand food ad libitum.

Normal mice. Male ddY strain mice (5 wk of age, SLC, Shizuoka, Japan) were purchased and used for the formalin test and the acetic acidwrithing test at the age of 7 wk (body weight, around 35 g).

STZ-induced diabetic mice. Two hundred mg/kg of STZ were injected i.p. to the 5-wk-old male ddY mice. Ten days later blood was obtained from the orbitalsinus and plasma glucose levels were determined by a commercialkit (Glucose B-test Wako, Wako Pure Chemical Industries, Ltd.Osaka, Japan). We used mice with blood glucose levels of >400mg/dl. The formalin-test was performed 2 wk after administrationof STZ. The body weight of the mice was around 27 g.

Genetically diabetic mice. Female C57BL/KsJ-db/db mice (6 wk of age, The Jackson Laboratory, Bar Harbor, ME) were purchased. The formalin test was performedwith 9- to 10-week-old mice (body weight around 44 g) becausehyperglycemia became steady at 7 to 8 wk of age. Blood was obtainedfrom the orbital sinus and plasma glucose levels were determinedby the commercial kit described above. We used db/db mice withblood glucose levels of >400 mg/dl.

Formalin Test

We used the formalin test previously published by Hunskaar et al. (1985) with slight modifications (Takeshita et al., 1995).Each mouse was placed in a observation chamber 5 min before theinjection of diluted formalin to allow acclimation to the newenvironment. Ten µl of 1% formaldehyde in saline were administeredinto the left hindpaw with an Ito microsyringe (Shizuoka, Japan).Each animal was then returned to the observation chamber and nociceptiveresponse was recorded for a period of 30 min. The summation oftime (sec) spent in licking and biting of the paw that receivedinjections during each 5 min block was measured as an indicatorof the pain response. The duration of responses in the first 10min and that from 10 to 30 min represent first and second phases,respectively. Insulin was injected s.c. and i.c.v. 20 and 10 minbefore injection of formalin, respectively. This test was performedin a temperature- and humidity-controlled (22 ± 1°C, 55 ± 5%)room.

Acetic Acid Writhing Test

Writhing was induced by an i.p. injection of 120 mg/kg of acetic acid (0.6% in saline solution) 20 min after s.c. injectionof insulin. The mice were placed individually in observation chambersimmediately after the acetic acid injection, and 3 min later thenumber of writhes produced by each mouse was counted for 10 min.

Procedure for i.c.v. Injections

Intracerebroventricular injection essentially followed a previously published method (Haley and McCormick, 1957). Insulinwas delivered in a volume of 5 µl using a Hamilton microsyringe(Hamilton Company, Reno, NV). To minimize leakage of the solution,we injected the volume over a period of 15 sec and left the needlein place for a further 15 sec. After some practice using a dye,we found little difficulty in reproducibly localizing drugs intracerebroventricularly.

Time Course Studies of Blood Glucose after Insulin Injection

Insulin (s.c.: 0.75 U/kg; i.c.v.: 1000 µU) was injected to mice and blood was taken from the orbital sinus s.c. at pre, 20,30 and 50 min, and i.c.v. at pre, 10, 20 and 40 min. Plasma wasobtained by centrifuging the blood. Plasma glucose was determinedwith the commercially available kit described above.

Statistical Analysis

The results are presented as the mean ± S.E., and statistical significance of differences between groups was analyzed by meansof analysis of variance followed by Dunnett's t test or by theunpaired t test where indicated. P < 0.05 were considered significant.The ID₅₀ values (i.e., the dose of drugs that reduced formalin-inducednociceptive response by 50% relative to control values) were estimatedfrom individual experiments by using the linear regression methodsin a computer program produced in our laboratory.

	Results

Top Abstract Introduction Methods Results Discussion References

Effects of insulin on nociceptive responses induced by formalin and acetic acid in normal mice. Although insulin tended to attenuate the acetic acid-induced writhing in normal mice in a dose-dependent fashion (fig. 1),even the largest dose (7.5 U/kg) gave only 19% inhibition, andthe overall dose effect of the drug was not statistically significant(F4,35 = 0.68, P > .05).

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Fig. 1. Effects of insulin on acetic acid-induced writhing responses in normal ddY mice. Insulin was administered (s.c.) 20 min beforethe acetic acid injection. Each value represents mean ± S.E.(n= 8). Columns represent number of writhes for 10 min from 3 minafter the acetic acid injection.

A s.c. injection of diluted formalin to the hindpaw of mice induced biphasic nociceptive responses such as licking and bitingof the paw that was injected. Treatment with insulin did not changethe pattern of responses, but dose-dependently attenuated theresponse time at each 5 min period (fig. 2). The total responsetime are shown in figure 3; the overall dose effects of insulinwere statistically significant for both the first (F4,45 = 3.82,P < .01) and the second phases (F4,45 = 27.07, P < .001). Theactivity of insulin was more potent on the latter than on theformer; 7.5 U/kg caused only 39% inhibition of the first phase,but almost completely abolished the second phase (ID₅₀ = 0.62U/kg).

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Fig. 2. Time course of biphasic nociceptive responses after injection of formalin in normal ddY mice. Insulin was administered (s.c.)20 min before formalin injection. Each value (mean ± S.E., n =10) represents duration of biting and licking responses per 5min.

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Fig. 3. Dose-response of insulin effect on formalin-induced nociceptive responses in figure 2. First phase (hatched columns) and secondphase (closed columns) represent the sum of biting and lickingresponses during 0 to 10 min and 10 to 30 min after injectionof formalin, respectively. Dunnett's t test for multiple comparisonssubsequent to analysis of variance was used for evaluation. Statisticalsignificance at *P < .05 and ***P < .001.

Effects of i.c.v. insulin on formalin-induced nociceptive response. An i.c.v. injection of insulin did not change the biphasic pattern of formalin-induced nociception, but attenuated the responsetime at each 5-min period (fig. 4). The total response time areshown in figure 5; the overall dose effect of insulin was statisticallysignificant for the second phase (F3,28 = 4.72, P < .01). Themaximal and statistically significant inhibition (57%) was obtainedat 1000 µU. The overall dose effect of insulin on the first phasewas not statistically significant (F3,28 = 0.13, P > .05).

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Fig. 4. Time course of biphasic nociceptive responses after injection of formalin in normal ddY mice. Insulin was administered (i.c.v.)10 min before formalin injection. Each value (mean ± S.E., n =8) represents duration of biting and licking responses per 5 min.

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Fig. 5. Dose-response of insulin effect on formalin-induced nociceptive responses in figure 4. First phase (hatched columns) and secondphase (closed columns) represent the sum of biting and lickingresponses during 0 to 10 min and 10 to 30 min after injectionof formalin, respectively. Dunnett's t test for multiple comparisonssubsequent to analysis of variance was used for evaluation. Statisticalsignificance at *P < .05.

Blood glucose levels after the treatment with insulin. Twenty minutes after a s.c. injection of insulin (0.75 U/kg) plasma glucose levels were significantly lowered by 29% comparedwith the saline treated group (fig. 6a). There was also a statisticallysignificant difference between the two at 30 min but not at 50min.

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Fig. 6. Time course changes in blood glucose levels after injection of insulin. Each value represents mean ± S.E. (n = 6-8). a; s.c.injection, b; i.c.v. injection. Open symbols: Injection of vehicle;closed symbols: injection of insulin. Dunnett's t test for multiplecomparisons subsequent to a repeated measurements analysis ofvariance was used for evaluation. Statistical significance at**P < .01, ***P < .001.

No significant changes in plasma glucose levels were obtained by i.c.v. injection of insulin (1000 µU), and there were nostatistically significant differences between the vehicle- andinsulin-treated groups at any time points. (fig. 6b).

Effects of naloxone and sulpiride on the antinociceptive activity of insulin in normal mice. Reproducing the abovementioned results, a s.c. injection of insulin (0.75 U/kg) significantly inhibited the second phase ofthe formalin test in normal mice (compare saline-saline with insulin-salinein figure 7).

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Fig. 7. Effects of pretreatment with naloxone and sulpiride on insulin (0.75 U/kg, s.c.) analgesia in formalin-induced tonic painresponses. a; Naloxone, b; sulpiride. Naloxone (10 mg/kg) andsulpiride (10 mg/kg) were injected i.p. 30 min before administrationof insulin. The nociceptive responses represent the summationof biting and licking responses during 10 to 30 min after injectionof formalin. Each value represents mean ± S.E. (n = 10-13). *P< .05, ***P < .001: Student's t test.

Treatment with naloxone (10 mg/kg i.p., an opiate receptor antagonist) per se did not significantly change the nociceptiveresponse to the formalin injection (compare saline-saline withsaline-naloxone in fig. 7a), but it greatly reduced the antinociceptiveactivity of insulin; insulin inhibited the formalin-induced nociceptiveresponse by 74% in the saline-treated mice and by 26% in the naloxone-treatedones. The latter change (saline-naloxone vs. insulin-naloxone)was not statistically significant.

Similarly, treatment with sulpiride (10 mg/kg i.p., a DA2 receptor antagonist) per se did not significantly change the nociceptiveresponse to the formalin injection, but it greatly reduced theantinociceptive activity of insulin (fig. 7b). The differencebetween the saline-sulpiride and insulin-sulpiride groups wasnot statistically significant.

Effects of pindolol, ketanserin and ICS205-930 on the antinociceptive activity of insulin in normal mice. In the three sets of experiments in normal mice, a s.c. injection of insulin (0.75 U/kg) induced comparable and statisticallysignificant inhibition of the second phase of the formalin test(fig. 8).

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Fig. 8. Effects of pretreatment with pindolol, ketanserin and ICS205-930 on insulin (0.75 U/kg, s.c.) analgesia in formalin-inducedtonic pain responses. a; Pindolol, b; ketanserin, c; ICS205-930.These compounds (1 mg/kg) were injected i.p. 30 min before administrationof insulin. The nociceptive responses represent the summationof biting and licking responses during 10 to 30 min after injectionof formalin. Each value represents mean ± S.E. (n = 10-16). *P< .05, ***P < .001: Student's t test.

Treatment with pindolol (1 mg/kg i.p., a 5-HT1 receptor antagonist) per se did not significantly change the nociceptive responseto the formalin injection (compare saline-vehicle with saline-pindololin fig. 8a), but it reduced the antinociceptive activity of insulin;insulin inhibited the formalin-induced nociceptive response by56% in the vehicle-treated mice and by 26% in the pindolol-treatedones, and the latter change (saline-pindolol vs. insulin-pindolol)was not statistically significant.

Treatment with ketanserin (1 mg/kg i.p., a 5-HT2 receptor antagonist) per se did not significantly change the nociceptiveresponse to the formalin injection (compare saline-saline withsaline-ketanserin in fig. 8b), but it greatly reduced the antinociceptiveactivity of insulin; insulin inhibited the formalin-induced nociceptiveresponse by 69% in the saline-treated mice and by 30% in the ketanserin-treatedones. The latter change (saline-ketanserin vs. insulin-ketanserin)was not statistically significant.

Treatment with ICS205-930 (1 mg/kg i.p., a 5-HT3 receptor antagonist) per se affected neither the nociceptive response tothe formalin injection (compare saline-saline with saline-ICS205-930in fig. 8c), nor the antinociceptive activity of insulin. Insulininhibited the response by 66% in the saline-treated mice (saline-salinevs. insulin-saline) and 47% in the ICS205-930-treated ones (saline-ICS205-930vs. insulin-ICS205-930). Both of the changes were statisticallysignificant.

Effects of insulin on the formalin-induced nociceptive response in STZ-induced diabetic mice. The biphasic pattern of formalin-induced nociception was not changed in STZ-induced diabetic mice compared with normal ddYmice, although the response time of the second phase was attenuatedin the former (compare fig. 9 with fig. 2). Insulin attenuatedthe response time of the second phase with minimal effects onthat of the first phase (fig. 9). The total response times areshown in figure 10; the overall dose effect of insulin was statisticallysignificant for the second phase (F4,45 = 3.05, P < .05) but notfor the first phase (F4,45 = 0.82, P > .05). The ID₅₀ for theformer was around 7.5 U/kg.

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Fig. 9. Time course of biphasic nociceptive responses after injection of formalin in STZ-treated ddY mice. Insulin was administered(s.c.) 20 min before the formalin injection. Each value (mean± S.E., n = 10) represents duration of biting and licking responsesper 5 min.

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Fig. 10. Dose-response of insulin effect on formalin-induced nociceptive responses in figure 9. Insulin was administered (s.c.) 20min before formalin injection. First phase (hatched columns) andsecond phase (closed columns) represent the sum of biting andlicking responses during 0 to 10 min and 10 to 30 min after injectionof formalin, respectively. Dunnett's t test for multiple comparisonssubsequent to analysis of variance was used for evaluation. Statisticalsignificance at **P < .01.

Effects of insulin on the formalin-induced nociceptive response in genetically diabetic db/db mice. The biphasic pattern of formalin-induced nociception was not changed in genetically diabetic db/db mice compared with normalddY mice, although the nociceptive responses were attenuated inthe former (compare fig. 11 with fig. 2). Insulin attenuated thesecond phase with minimal effects on the first phase (fig. 11).The total response times are shown in figure 12; the overall doseeffect of insulin was statistically significant for the secondphase (F4,45 = 4.37, P < .01) but not for the first phase (F4,45= 0.97, P > .05). The ID₅₀ for the former was around 7.5 U/kg.

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Fig. 11. Time course of biphasic nociceptive responses after injection of formalin in genetically diabetic db/db mice. Insulin wasadministered (s.c.) 20 min before the formalin injection. Eachvalue (mean ± S.E., n = 10) represents duration of biting andlicking responses per 5 min.

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Fig. 12. Dose-response of insulin effect on formalin-induced nociceptive responses in figure 11. First phase (hatched columns) and secondphase (closed columns) represent the sum of biting and lickingresponses during 0 to 10 min and 10 to 30 min after injectionof formalin, respectively. Dunnett's t test for multiple comparisonssubsequent to analysis of variance was used for evaluation.

	Discussion

Top Abstract Introduction Methods Results Discussion References

It is a novel and interesting finding that insulin strongly attenuated the second phase of the formalin-induced nociceptiveresponse in our study. Although the experimental data demonstratingthat insulin per se has analgesic effects are still scanty, thismay possibly be ascribed to the nature of methods used. Most behavioralstudies concerning pain transmission use tests determining acuteor phasic pain induced by thermal, mechanical or chemical stimuli.The formalin test was originally described in rats and cats byDubuisson and Dennis (1977), and a s.c. injection of formalinproduced a biphasic pain response in rats. Several lines of evidencehave indicated that the first phase represents a phasic pain responseto direct stimulation of the nerve endings, and the second phaserepresents a tonic pain response to subsequent inflammation (Dubuissonand Dennis, 1977; Shibata et al., 1989). We thus speculate thatinsulin, which resembles mild analgesics such as paracetamol andacetylsalicylic acid (Hunskaar et al., 1985), induces specificmodulation of tonic pain compared with phasic pain. The assumptionis supported, in part, by the present finding that insulin hada less potent effect on the first phase of the formalin test andon the acetic acid-induced writhing test than on the second phaseof the formalin test. However, there is clinical evidence thatnormal subjects with higher insulin levels show an elevated thresholdfor thermal nociceptive stimuli (Delaney et al., 1994) and thatinsulin effectively blocks diabetic pain (Samanta and Burden,1985). In addition to the effects of insulin on sensory nervefunction (Delaney et al., 1994) and on glucose metabolism (Samantaand Burden, 1985), the mild analgesic action of insulin may alsobe responsible for its clinical effects. In this respect, it isinteresting to note that amitriptyline and tiapride, which areclinically effective for painful diabetic neuropathy, specificallyattenuated the second phase of the formalin test (Acton et al.,1992, Takeshita et al, 1995). Further, Calcutt et al. (1994) havesuggested that animal studies using the formalin test might beuseful in elucidating the etiology of painful diabetic neuropathy.

An i.c.v. injection of insulin dose-dependently attenuated only the second phase of the formalin test, but it did not significantlylower the blood glucose levels even at the largest dose. The degreeof the change by 1000 µU/animal i.c.v. was comparable to thatby 0.75 U/kg s.c., i.e., the i.c.v. dose was calculated to beabout 20 times more potent than the s.c. dose because the bodyweight of the mice was around 35 g. However, it has been reportedthat insulin receptors are widely distributed in the central nervoussystem (Havrankova et al., 1978; Pacold and Blackard, 1979), andthat peripherally administered insulin crosses the blood-brainbarrier to reach the central nervous system (Wallum et al., 1987;Steffens et al., 1988). This evidence, taken together, favours,the view that the central nervous system is the site of the antinociceptiveaction of insulin. However, as there is still a possibility thats.c. and i.c.v. insulin activate different mechanisms, furtherstudies are needed to clarify the point.

Another important finding of our study is that the antinociceptive effect of a systemic dose of insulin was significantlyinhibited by pretreatment with naloxone (10 mg/kg i.p., an opiatereceptor antagonist), sulpiride (10 mg/kg i.p., a DA2 receptorantagonist), pindolol (1 mg/kg i.p., a 5-HT1 receptor antagonist)and ketanserin (1 mg/kg i.p., a 5-HT2 receptor antagonist), butnot by that with ICS205-930 (1 mg/kg i.p., a 5-HT3 receptor antagonist).Pindolol and ketanserin effectively blocked the antinociceptiveeffect of meta-chlorophenylpiperazine (a 5-HT receptor agonist)in the formalin test (Takeshita and Yamaguchi, 1995), althoughsulpiride blocked the antinociceptive effect of FR64822 (a dopaminergicenhancer) in the acetic acid writhing test (Ohkubo et al., 1991).These results suggest that insulin causes antinociception throughan indirect activation of the opiate, DA2, 5-HT1 and 5-HT2 receptors.In line with this speculation, there have been papers demonstratingthat insulin injection releases brain amines including DA and5-HT (Gordon and Meldrum, 1970; Gupta et al., 1992).

The antinociceptive effects of insulin were less potent in db/db mice and STZ-treated mice than in normal ddY mice. The differencein insulin effects was too large (about 10-fold) to be ascribedto that in body weight (less than 2-fold) between the diabeticmice and the normal ddY mice. However, we have recently observedthat the antinociceptive effects of FR64822 (a dopaminergic enhancer,Ohkubo et al., 1991) are also reduced in both of these diabeticmodels (Takeshita et al., unpublished observation), whereas theeffects of serotonergic agents such as tiapride (Takeshita etal., 1995) and meta-chlorophenylpiperazine (Takeshita and Yamaguchi,1995) are not changed in mice compared with normal ddY mice. Thereforederangement of the dopaminergic antinociceptive pathway wouldappear to be responsible for the reduced activity of insulin inthe diabetic mice. In line with this assumption, it has been shownthat the brain DA synthesis rate is decreased in STZ-induced diabeticrats (Trulson and Himmel, 1983). Alternately, the following evidenceargues against the possibility that derangement of insulin- oropiate-receptor mechanisms is responsible for the change in theeffect of insulin. Although it is widely accepted that insulinreceptors in the periphery undergo up- and down-regulation, abalance of evidence indicates that insulin receptors in the centralnervous system do not undergo a similar regulation (Schwartz etal., 1992). Insulin binding to brain homogenates was not affectedby hyperinsulinemia or STZ-treatment (Havrankova et al., 1979;Pacold and Blackard, 1979). Also, naloxone binding in brain membraneswas not affected by the induction of diabetes via STZ or in db/dbmice compared with the nondiabetic control (Brase et al., 1987).

In conclusion, insulin attenuated specifically the second phase of formalin-induced nociception. An activation of centraldopaminergic, serotonergic and opioidergic pathways rather thansystemic hypoglycemia appears to be the mechanism of action. Someof the antinociceptive pathways initiated by insulin appear tobe attenuated in both the STZ-induced diabetic mice and the geneticallydiabetic db/db mice.

	Acknowledgments

The authors thank Dr. T. Ohashi for helpful advice during the preparation of this manuscript.

	Footnotes

Accepted for publication December 13, 1996.

Received for publication March 4, 1996.

Send reprint requests to: Dr. Nobuaki Takeshita, Basic Research Group, Tsukuba Research Laboratories, Fujisawa Pharmaceutical Co. Ltd., 5-2-3 Tokodai, Tsukuba, Ibaraki 300-26, Japan.

	Abbreviations

STZ, streptozotocin; ICS205-930, 3-tropanyl-indole-3-carboxylate; i.c.v., intracerebroventricular; 5-HT, 5-hydroxytryptamine (serotonin); DA, dopamine.

	References

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