Suppressed Injury-Induced Rise in Spinal Prostaglandin E2 Production and Reduced Early Thermal Hyperalgesia in iNOS-Deficient Mice

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The Journal of Neuroscience, September 1, 2000, 20(17):6714-6720

Suppressed Injury-Induced Rise in Spinal Prostaglandin E₂ Production and Reduced Early Thermal Hyperalgesia in iNOS-Deficient Mice
Hans Gühring¹, Manfred Görig¹, Mehmet Ates¹, Ovidiu Coste¹, Hanns Ulrich Zeilhofer¹, Andreas Pahl¹, Klaus Rehse², and Kay Brune¹
¹ Department of Experimental and Clinical Pharmacology and Toxicology, D-91054 Erlangen, Germany and ² Department of Pharmaceutical Chemistry, D-14195 Berlin, Germany

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

It is widely accepted that peripheral injury increases spinal inducible cyclooxygenase (COX-2) expression and prostaglandinE₂ (PGE₂) formation as key mediators of nociceptive sensitization.Here, we used inducible nitric oxide synthase (iNOS) gene-deficient(iNOS $-$ / $-$ ) mice to determine the contribution of iNOS-derived nitricoxide (NO) to this process. iNOS $-$ / $-$ mice exhibited reduced thermalhyperalgesia after zymosan injection. Spinal NO and PGE₂ formationboth remained at baseline levels, in contrast to wild-type (wt)mice. In wt mice reduced hyperalgesia similar to that seen iniNOS $-$ / $-$ mice was induced by local spinal, but not by systemictreatment with the iNOS inhibitor L-NIL, suggesting that the reducedheat sensitization in iNOS $-$ / $-$ mice was attributable to the lackof spinal rather than peripheral iNOS. Two additional observationsindicate that the antinociceptive effects of iNOS inhibition aredependent on a loss of stimulation of PG synthesis. First, intrathecalinjection of the COX inhibitor indomethacin, which exerted pronouncedantinociceptive effects in wt mice, was completely ineffectivein iNOS $-$ / $-$ mice. Second, treatment with the NO donor RE-2047 notonly completely restored spinal PG production and thermal sensitizationin iNOS $-$ / $-$ mice but also its sensitivity to indomethacin. In bothtypes of mice induction of thermal hyperalgesia was accompaniedby similar increases in COX-1 and COX-2 mRNA expression. The stimulationof PG production by NO therefore involves an increase in enzymaticactivity, rather than an alteration of COX gene expression. Theseresults indicate that NO derived from spinal iNOS acts as a fastinductor of spinal thermalhyperalgesia.

Key words: nitric oxide; inducible nitric oxide synthase; zymosan; thermal hyperalgesia; paw edema; spinal microdialysis; L-NIL; RE-2047; prostaglandins; cyclooxygenase

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Acute tissue damage is often accompanied by the fast development of hyperalgesia and allodynia (Andrew and Greenspan, 1999).Both peripheral mechanisms at the site of injury and central processesparticularly in the spinal cord contribute to this phenomenon.Prostaglandins (PGs) (Yaksh and Malmberg, 1993; Brune, 1994) aswell as nitric oxide (NO) (Lawand et al., 1997) are produced inresponse to tissue damage peripherally and centrally. WhereasPGs are generally accepted to play a dominant role in nociceptivesensitization (Bley et al., 1998), the role of NO is less clear.Also some authors claim of an anti-nociceptive action of NO (Goettland Larson, 1996; Hamalainen and Lovick, 1997), most favor a pro-nociceptiveactivity (Malmberg and Yaksh, 1993; Kawabata et al., 1994; Chenand Levine, 1999). Part of this controversy may arise from theexistence of three different isoenzymes of NO synthase (NOS) (Gonzalez-Hernandezand Rustioni, 1999), which may have distinct effects on nociception,and from the lack of specific inhibitors for these different isoforms.In the CNS including the spinal cord, NO is thought to be primarilyproduced by the neuronal isoform of NOS (nNOS) (Downen et al.,1999). However, endothelial NOS is also found in neurons (Weiet al., 1999) and under certain conditions, e.g., after tissuedamage (Sinz et al., 1999), inducible NOS (iNOS) can be expressedin the CNS (Meller et al., 1994; Lee and Brosnan, 1996; Barkeret al., 1998). Therefore, all three NO-generating isoenzymes appearto be possible sources of NO in theCNS.

To define the role of NO in spinal processing of nociceptive information more clearly, we investigated nociceptive sensitizationin genetically modified mice deficient in the iNOS isoenzyme (iNOS $-$ / $-$ mice). For this purpose, we adapted the Hargreaves model of thermalhyperalgesia (Hargreaves et al., 1988) to mice and developed atechnique for spinal microdialysis in mice. We showed that iNOS $-$ / $-$ mice exhibit a delay in thermal sensitization and lack the risein spinal PG production, which is normally observed in responseto peripheral nociceptivestimulation.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Assessment of thermal hyperalgesia. A modified Hargreaves plantar test (Hargreaves et al., 1988) was used to assess thermalhyperalgesia in mice. A metal grid bottom instead of a glass floorin the observation cage and 10.5 × 13.0 × 4.5 cm boxes to restrictanimal movement were used. Zymosan A (Sigma, Deisenhofen, Germany)was injected subcutaneously into the plantar side of right hindpaws,and paw withdrawal latencies (PWL) were determined on exposureof the paws to a defined thermal stimulus were measured usinga commercially available apparatus (Hargreaves Test Ugo BasileBiological Research Apparatus, Comerio,Italy).

Mice were kept in the test cages for 1 d to allow accommodation. On day 2, each mouse was tested several times to gain baselinePWL. On day 3 thermal hyperalgesia was assessed for 8 hr starting15 min after subcutaneous zymosan injection (3.0 mg/ml in 20 µlof PBS, containing NaCl 8 gm/l, Na₂HPO₄ 2.9 gm/l, KCl 0.2 gm/l,KH₂ PO₄ 0.24 gm/l). Experiments were performed in air conditionedrooms (22°C) between 12 A.M. and 8 P.M. In some experiments theassessment of thermal hyperalgesia was continued for 7 d (onemeasurement per day). Right (injected) and left (noninjected)paws were measured alternately in intervals of 5-10 min. At 1hr intervals, PWL wereaveraged.

Under control conditions, PWL were identical in wt (10.40 ± 0.35 sec; n = 40) and iNOS $-$ / $-$ mice (10.25 ± 0.20 sec; n = 18).In an initial set of experiments, zymosan (20 µl) was tested inconcentrations of 12.0, 6.0, or 3.0 mg/ml. Zymosan injection causeda dose-dependent increase in areas [PWL × observation interval[seconds × hours]; calculated using the linear trapezoidal rulefor each mouse] between right and left hindpaw PWL from 0.17 ±1.75 (PBS) to 10.10 ± 1.81 (3.0 mg/ml) to 17.47 ± 2.55 (6.0 mg/ml)and to 23.30 ± 2.22 (12.0 mg/ml). Injection of vehicle did notaffect nociceptive behavior in any of the experiments. For allsubsequent tests an intermediate zymosan concentration of 3.0mg/ml was used for the detection of pro-nociceptive and anti-nociceptiveeffects.

Animals. Male iNOS $-$ / $-$ mice weighing 26.7 (22.9-36.8) gm [mean (range)] with the genetic background of C57/Bl6 mice and maleC57/Bl6 mice (wt) weighing 21.2 (19.6-26.1) gm were used for allexperiments. Breeding pairs of iNOS $-$ / $-$ mice (Laubach et al.,1995) were obtained from The Jackson Laboratory (Bar Harbor, ME).INOS $-$ / $-$ mice show no major abnormalities (Laubach et al., 1995;MacMicking et al., 1995; Wei et al., 1995). Mice were housed undera 12 hr light/dark cycle and cared for according to the guidelinesof the Institutional Animal Care and Use Committee. Water andfood were given ad libitum.

Application of drugs. All drugs were dissolved in isotonic, physiological solvents. Indomethacin was dissolved as describedelsewhere (Shen and Winter, 1977). Briefly, for a 10 mM solution,17.9 mg of indomethacin, 15.3 mg of Na₂CO₃ × 10 H₂O, and 5 mlof artificial CSF (ACSF) consisting of (in mM): 151.1 Na⁺, 2.6 K⁺, 0.9 Mg²⁺, 1.3 Ca²⁺, 122.7 Cl, 21.0 mM HCO3, 2.5 mM HPO4, and 3.5 dextrose, pH 7.20, was used. Intraperitoneal drug orvehicle (PBS) injections (50 µl) were given into the lower leftabdominal quadrant. Intrathecal injections were performed accordingto Hylden and Wilcox (1980). In brief, mice were anesthetizedwith isoflurane, and 5 µl of drug containing solutions or vehicle(ACSF) were injected into the spinal subarachnoid space betweenL5 and L6 30 min before the administration of zymosan using a26 gauge needle mated to a 10 µl Hamilton syringe. Mice showingneurological abnormalities were excluded. We added 1% black ink(Pelikan, Hannover, Germany) to all solutions used for intrathecalinjections. Proper intrathecal injections were verified by inspectionof slices of the spinal cord after lumbarlaminectomy.

Tissue samples. After completion of the Hargreaves test, mice were killed under CO₂ anesthesia by intracardial puncture anddecapitation. Hindpaws and the thoracolumbar segment of the spinalcord were removed for morphological and biochemical analyses.After intra-articular disconnection at the ankle joint, rightand left hindpaws were weighed. Differences in paw weight ( $Delta$ PW)were used to measure edemaformation.

Spinal microdialysis. The dialysis tube was constructed from a Cuprophan hollow fiber (outer diameter, 216 µm) with a 36 kDamolecular weight cutoff (Hospal, Nuernberg, Germany). This fiberwas connected at one side to a polyethylene (PE) tube (inner diameter,0.4 mm; outer diameter, 0.8 mm) using cyanacrylate glue (number448 Stabiloplast; Renfert, Chemietechnik, GmbH). A small metalspike was inserted into the other side and fixed with a quick-settingcyanacrylate glue (UHU, Buehl,Germany).

Mice were deeply anesthetized with isoflurane (1.5-2.0% vol; Abbott GmbH, Wiesbaden, Germany) and placed on an electronicallycontrolled heating pad (37°C; CMA/Microdialysis, Stockholm, Sweden).After cutaneous incision of the thoracolumbar region, superficialand deep dorsal lumbar fascia were slit, and muscle tissue wasremoved from the vertebrae T12-L1. The dialysis tube was introducedthrough the intervertebral joints between the thoracic and lumbarsegments. All accessible parts of the dialysis tube were coveredwith cyanacrylate glue. After cutting the spike, the free endof the hollow fiber was connected to another PE tube using thesame cyanacrylate adhesive. Afterward mice were surgically sewedand permanently anesthetized with urethane (~750 mg/kg, i.p.).

The PE tube was connected to a microdialysis pump (CMA 100; CMA/Microdialysis), and ACSF was perfused at a flow rate of 3µl/min. ACSF was bubbled with carbogen (5% CO₂ and 95% O₂) andkept at 37°C during the experiments. Samples were collected at30 min intervals in Eppendorf cups kept on ice and finally storedat $-$ 70°C for subsequent analysis of PGE₂, as well as NO₂ and NO₃ (NO_x) as the breakdown products of NO. After a washout periodof 30 min, baseline samples were collected for 1.5 hr every 30min. Thereafter, 20 µl of zymosan (3.0 mg/ml) was injected subcutaneouslyinto the right hindpaw, and samples were collected for another4 hr. After mice were killed, the proper placement of microdialysistubes was verified by perfusion with black ink (Pelikan), andsubsequent microscopicexamination.

NO_x and PGE₂ measurements. NO production was assessed indirectly by determining NO degradation products after reduction ofNO₃ to NO₂ with nitrate reductase (Cytochrome; Sigma) by the Griess reaction-dependentmethod described elsewhere (Green et al., 1981). We incubated50 µl of perfusion samples with 50 µl of modified Griess reagent(Sigma), and the absorption was recorded at 540 nm (Flow Titertec,Multiscan Plus MK11; ICN Biochemicals, Frankfurt,Germany).

Tissue samples obtained from the spinal cord and from the hindpaws were weighed, transferred into 99.5% methanol (1 mg oftissue to 10 µl of methanol), and shaken for 2 hr at room temperature.We transferred 100 µl of the supernatants into Eppendorf cups,and methanol was evaporated. The remaining pellet was dissolvedin 100 µl of enzyme immunoassay (EIA) buffer. We incubated 20µl of the microdialysis perfusion samples with 80 µl of enzymeimmunoassay (EIA) buffer for PGE₂measurements.

All further steps were performed as described in the Cayman Chemical Company PGE₂ EIA Kit - Monoclonal, calibration range:1000-7.8 pg/ml (Cayman Chemicals, Ann Arbor, MI). Measurementwas completed by using an ELISA reader (Flow Titertec, MultiscanPlus MK11; ICN Biochemicals) with an absorbency maximum at 405nm.

RT-PCR. Immediately after preparation, tissue samples of the right hindpaw and spinal cord segment L4 were snap frozen with800 µl of lysis buffer (Qiagen, Hilden, Germany) in liquid nitrogen,stored at $-$ 70°C, and homogenized with a microshredder. RNA wasisolated using the RNeasy-kit (Qiagen). Real-time RT-PCR was usedto determine expression of mouse-actin, COX-1, and COX-2 mRNA.TaqMan probes were labeled at the 5' end with the reporter dyemolecule FAM (6-carboxy-fluorescein; emission $lambda$ , 518 nm), andat the 3' end with the quencher dye molecule TAMRA (6-carboxy-tetramethyl-rhodamine,emission $lambda$ , 582 nm). In addition, the 3' end was phosphorylatedto prevent extension of the probe duringPCR.

We used 25 µl of reaction mixture, which contained 2 µl of template, 5 µl of 10 × PCR buffer (100 mM Tris, pH 8.3, 500 mMKCl), 3 µl of Mn(OAc)₂, 0.3 µl of dATP, dCTP, dGTP, and dUTP,0.1 µl of Diagonal DNA polymerase, 0.05 µl of each primer, 0.05µl of the TaqMan probe, and 14.55 µl of sterile water for thePCR. For RT-PCR and detection of fluorescence signals the ABIPrism 7700 SDS analytical thermal cycler (Perkin-Elmer, FosterCity, CA) was used. Thermal cycle conditions were: 2 min at 50°C,30 min 60°C, 5 min 95°C, and then 45 cycles (15 sec at 94°C, 1min at 60°C).

The emission of the reporter dye was compared with that of the quenching dye during PCR amplification and the increase offluorescence signals, $Delta$ Rn, was calculated as: $Delta$ Rn = (Rn⁺) $-$ (Rn) [Rn⁺ = ratio of reporter and quencher dye at any given time duringa reaction; Rn = ratio of reporter and quencher baseline emission]. Referringto a standard RNA a threshold was defined indicating the exponentialphase of the fluorescent signal increase. The C_T value, whichcorrelates to the number of RNA copies present at the start ofPCR according to the references of PE Applied Biosystems (UserBulletin 2; ABI PRISM 7700 Sequence Detection System, 1997) wasdetermined as the amplification cycle number when the $Delta$ Rn of asample intersected this threshold value. The quantity of mRNAwas given as $Delta$ C_T, which was calculated as $Delta$ C_T = C_T^{gene of interest} $-$ C_T^-actin
mRNA.

iNOS mRNA transcripts were analyzed in spinal cord tissue (thoracolumbar segment) homogenates according to a protocol previouslydescribed in detail (Deckert-Schluter et al., 1995). Primer sequenceswere described previously (Deckert-Schluter et al., 1998; compareTable 1) and were synthesized by TIB MOLBIOL (Berlin, Germany).Briefly, total mRNA was extracted as described above. After reversetranscription of mRNA using the Superscript RT kit (Life Technologies,Frederick, MD) PCR reactions were conducted in a final volumeof 25 µl of using the AmpliTaq Gold kit from PE Biosystems (Weiterstadt,Germany). Conditions are: 1 × 2 min 95°C; 45 × 1 min 95°C, 1 min58°C, 1 min 72°C; 1 × 7 min 72°C. The PCR product was visualizedby electrophoresis on 1.5% agarose gels.


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Table 1. Primer sequences

Statistical analysis. Results are expressed as the mean ± SEM. The statistical analyses of the behavioral experiments wereperformed using one-way ANOVA followed by post hoc Bonferronitest (the $alpha$ level was set to 0.05) or by a Student's t test (p< 0.05 was considered statisticallysignificant).

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

iNOS-derived NO facilitates development of spinal hyperalgesia

A modification of the Hargreaves test was used to assess thermal hyperalgesia in wt and iNOS $-$ / $-$ mice. Both types of mice exhibiteda time-dependent sensitization to noxious heat in response toplantar zymosan injection. At the time point of maximum thermalhyperalgesia, PWL were reduced from ~10 sec under control conditionsto ~3 sec after zymosan injection. In wt mice, however, maximumsensitization occurred after 3 hr, whereas that of iNOS $-$ / $-$ micewas not reached until 8 hr (Fig. 1). Wild type-like thermal sensitizationcould be restored in iNOS $-$ / $-$ mice by treatment with the NO-donorRE-2047 (3-methyl-N-nitroso-sydnone-5-imine; a generous gift fromProf. Rehse, Department of Pharmaceutical Chemistry, Berlin, Germany)(Rehse and Ciborski, 1995) in a dose-dependent manner. At thehighest dose of RE-2047 hyperalgesia in iNOS $-$ / $-$ mice was indistinguishablefrom that of wt mice, confirming that the reduced thermal sensitizationin iNOS $-$ / $-$ mice was caused by the absence of NO generated by iNOS(Fig. 2).

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Figure 1. Time course of zymosan-induced thermal hyperalgesia in iNOS $-$ / $-$ mice. Development with time of PWL in iNOS $-$ / $-$ (n = 12; open circles) and wt mice (n = 12; black circles) after intraperitoneal administration of PBS and after injection of 3.0 mg/ml zymosan subcutaneously into the right hindpaw. Left PWLs (black lines) were similar for both lines of mice. Different PWL (*p < 0.05) indicate reduced heat sensitization after zymosan injection in iNOS $-$ / $-$ mice. Data are expressed as means ± SEM.

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Figure 2. NO donor restores thermal hyperalgesia in iNOS $-$ / $-$ mice. Intraperitoneal injection of RE-2047, a metabolic NO-donor, in doses increasing from 5 (black diamonds) to 15 (gray diamonds) and 45 mg/kg (open diamonds) antagonized the restored heat sensitization of iNOS $-$ / $-$ mice. The difference of heat sensitization between wt (black circles) and iNOS $-$ / $-$ mice (open circles) after intraperitoneal administration of PBS is drawn as dotted lines.

To determine whether the lack of iNOS in the peripheral tissue or in the CNS was responsible for reduced early thermal hyperalgesia,we used the selective iNOS inhibitor L-NIL (L-N6-(I-iminoethyl)-lysinehydrochloride; Alexis Biochemicals, Gruenberg, Germany; Mooreet al., 1994) and took advantage of its inability to penetratethe blood-brain barrier in significant amounts (U. Werner, B.Layh, K. Brune, H. and Guehring, unpublished observations). Inthis series of experiments we compared the effects of L-NIL aftersystemic peripheral (intraperitoneal) and local spinal (intrathecal)injection in wt mice. After intraperitoneal injection at dosesranging from 15.0 to 135.0 mg/kg L-NIL effectively reduced edemaand PGE₂ production in the zymosan-injected paw, but had no effecton thermal hyperalgesia (Fig. 3A, Table 2). Increases in theweight of the injected paws were 35.2 ± 3.0% and 48.7 ± 2.1% inL-NIL and vehicle-treated mice, respectively. A similar differencewas found for the PGE₂ content in the zymosan-injected paws, whichwas 25.6 ± 5.0 pg/mg in L-NIL treated and 54.6 ± 2.7 pg/mg incontrol mice. As expected, L-NIL was completely ineffective iniNOS $-$ / $-$ mice. Both paw edema formation and PGE₂ production inL-NIL-treated mice were not significantly different from thosefound in iNOS $-$ / $-$ mice (edema, 30.25 ± 4.14%; PGE₂, 23.3 ± 1.9pg/mg).

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Figure 3. Effects of peripheral versus spinal injection of L-NIL on thermal hyperalgesia in wt mice. A, In wt mice (open diamonds) the selective iNOS inhibitor L-NIL administered intraperitoneally was without any effect even in doses ranging from 5 to 135 mg/kg. The difference of heat sensitization between wt (black circles) and iNOS $-$ / $-$ mice (open circles) after intraperitoneal administration of PBS is drawn as dotted lines. Data are expressed as mean ± SEM. B, In contrast to A drugs were administered intrathecally. Intrathecal administration of L-NIL (0.1 µM) to wt mice (black diamonds) reduced heat sensitization significantly to the level of iNOS $-$ / $-$ mice. Differences in heat sensitization between wt (black circles) and iNOS $-$ / $-$ mice (open circles) were also observed after acute intrathecal injection of ACSF (5 µl). Data are expressed as means ± SEM.


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Table 2. Thermal hyperalgesia after intraperitoneal administration of drugs

By contrast, when L-NIL (0.1 µM; 5 µl) was injected intrathecally the development of zymosan-induced sensitization was significantlyretarded compared to vehicle (ACSF; 5 µl)-treated animals andindistinguishable from that of iNOS $-$ / $-$ mice (Fig. 3B). The latterfinding indicates that the lack of spinal rather than of peripheraliNOS was responsible for the observed delay in thermal hyperalgesia.Interestingly, neither L-NIL nor the nonspecific NOS inhibitorL-NAME (NG-nitro-L-arginine methyl ester; Alexis Biochemicals,Gruenberg, Germany; Amir and English, 1991) affected heat sensitizationin iNOS $-$ / $-$ mice (Table 3), indicating that nNOS and eNOS didnot significantly contribute to zymosan-induced thermal hyperalgesia.


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Table 3. Thermal hyperalgesia after intrathecal administration of drugs

To investigate whether the facilitating action of iNOS on thermal hyperalgesia was related to the COX system in the spinalcord, we compared the effects of spinal COX inhibition in iNOS $-$ / $-$ and wt mice. In wt mice intrathecal injection of the COX inhibitorindomethacin (Sigma) reduced thermal hyperalgesia in a dose-dependentmanner (Fig. 4A). This antinociceptive effect was completely absentin iNOS $-$ / $-$ mice (Table 3, Fig. 4B) but was restored after substitutionof NO with RE-2047, suggesting that the increase in spinal PGE₂production after zymosan injection required NO, which in wt miceis produced by spinal iNOS.

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Figure 4. Effects of indomethacin in wt and iNOS $-$ / $-$ mice. A, Intrathecal injection of indomethacin, a nonselective COX inhibitor, in ascending doses of 0.1 (black diamonds) to 1.0 (gray diamonds) and 10.0 mM (open diamonds) decelerated the development of thermal hyperalgesia of wt mice. Intrathecal injection was performed to exclude the possibility of a decreased production of prostaglandins in the inflamed hindpaws during systemic application of COX inhibitors. Wt (black circles) and iNOS $-$ / $-$ mice (open circles) after acute intrathecal injection of ACSF (5 µl). Data are expressed as mean ± SEM. B, Intrathecal injection of indomethacin 10.0 mM (black triangle) antagonized the development of thermal hyperalgesia after intraperitoneal pretreatment with the NO donor RE-2047 (45 mg/kg). iNOS $-$ / $-$ mice after intraperitoneal pretreatment with 45 mg/kg RE-2047 and after intrathecal injection of ACSF (black diamonds) served as controls. Thermal hyperalgesia in iNOS $-$ / $-$ mice was not affected after intraperitoneal pretreatment with PBS and intrathecal pretreatment with indomethacin 10.0 mM (black triangle). Wt (black circles) and iNOS $-$ / $-$ mice (open circles) after acute intrathecal injection of 5 µl of ACSF (dotted lines). Data are expressed as means ± SEM.

Spinal NO_x and PGE₂ formation

The difference in heat sensitization between wt and iNOS $-$ / $-$ mice was already present 1 hr after zymosan injection. BecauseiNOS is generally considered not to be constitutively expressedin the CNS, the fast rise in NO production after zymosan injectionwould require an at least equally fast induction of iNOS expression.We have therefore analyzed the expression of iNOS mRNA duringthe early phase of hyperalgesia development by RT-PCR (Fig. 5).Significant amounts of iNOS mRNA were detected 30 and 60 min afterzymosan injection and 120 min after zymosan injection in separateexperiments (data not shown). As expected, iNOS mRNA was absentunder control conditions and in iNOS $-$ / $-$ mice after zymosan injection.

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Figure 5. Early iNOS mRNA expression in wt mice. iNOS mRNA expression in spinal cord of wt and iNOS $-$ / $-$ mice after zymosan injection into the right hindpaw. In wt but not in iNOS $-$ / $-$ mice, iNOS mRNA was increased in thoracolumbar segment of spinal cord even 0.5 (3 of 6 mice) and 1 hr (6 of 6 mice) after peripheral inflammation. $beta$ -actin RT-PCR product level served as control. This figure represents one of two independent experiments.

To further elucidate the role of iNOS in the spinal mechanisms of heat sensitization and its relation to the COX pathway weperformed spinal microdialysis to measure NO and PGE₂ productionin the spinal cord in response to zymosan injection. In a firstseries of experiments we tested whether insertion of the microdialysisprobe was sufficient to induce spinal PG formation. In these experiments,PBS instead of zymosan was injected subcutaneously into the righthindpaw. Under these conditions only a modest increase in PGE₂was induced in wt mice (from 18.4 ± 1.9 to 26.3 ± 2.5 pg/ml).

When zymosan was injected, both PGE₂ and NO degradation products (NO_x,, i.e., NO₂ and NO₃) increased in wt mice. NO_x concentrations reached their maximumalready after 1 hr and thus closely paralleled the developmentof iNOS-dependent hyperalgesia (Fig. 6A). By contrast, PGE₂ showeda more prolonged increase, exhibiting a continuous rise over thewhole observation period of 4 hr (Fig. 6B).

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Figure 6. Spinal microdialysis in wt and iNOS $-$ / $-$ mice. A, Time course of percentile NO_x level changes in the spinal cord of wt mice (black circles) and iNOS $-$ / $-$ mice (open circles) after subcutaneous injection of 3.0 mg/ml zymosan into the right hindpaw. Samples were collected via microdialysis of the thoracolumbar segment. In wt mice zymosan injection led to a rapid increase of breakdown products of NO, whereas only a slight increase of NO_x was observed in iNOS $-$ / $-$ mice. After treatment with RE-2047, an NO donor, NO_x levels in the spinal cord of iNOS $-$ / $-$ mice increased (open diamonds). Black triangles represent NOx levels in wt mice after injection of PBS instead of zymosan into the right hindpaw. Data are expressed as means ± SEM. B, Time course of the percentile PGE₂ changes in the spinal cord of wt (black circles) and iNOS $-$ / $-$ mice (open circles). The additional curve (black diamonds) shows the changes of PGE₂ levels after injection of RE-2047 intraperitoneally into iNOS $-$ / $-$ mice. Black triangles represent wt mice after PBS administration into the right hindpaw instead of zymosan. Data are expressed as means ± SEM.

Next we investigated whether the effects of reduced NO formation on nociceptive sensitization might be secondary to a suppressionof PGE₂ formation. iNOS $-$ / $-$ mice lacked not only the zymosan-inducedincrease in NO, but also showed reduced spinal PGE₂ formation.The rise in PGE₂ production was much smaller compared to thatin wt mice. As described above the NO donor RE-2047 reconstitutedwt-like hyperalgesia in iNOS $-$ / $-$ mice. As shown in Figure 6A, RE-2047not only increased spinal NO_x concentrations, but also restoredspinal PGE₂ formation (Fig. 6B).

We analyzed whether the expression of COX-1 or COX-2 differs in iNOS $-$ / $-$ and wt mice. Time course of COX-1 and COX-2 mRNA expressionand of the PGE₂ concentration in spinal cord tissue was followedfor 7 d. As shown in Figure 7A, increases in PGE₂ concentrationsreached their maximum 8 hr after zymosan injection, declined,and came back to baseline levels after 7 d. In iNOS $-$ / $-$ mice therise in PGE₂ was again largely suppressed, and only at 8 hr amodest increase in PGE₂ was seen.

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Figure 7. PGE₂ concentration and COX-1 and COX-2 mRNA expression in spinal cord tissue. A, Time course of absolute PGE₂ levels in the spinal cord tissue samples of wt (black circles) and in iNOS $-$ / $-$ (open circles) mice after zymosan injection into the right hindpaw. PGE₂ measurement was performed from tissue samples after perfusion with 100 ml of ice-cold PBS. Data are expressed as means ± SEM. B, Time course of real time RT-PCR measurement of spinal COX-1 (circles) and COX-2 (squares) mRNA expression in wt (black) and iNOS $-$ / $-$ (open) mice after peripheral administered zymosan. There are no differences between COX mRNA expression in both lines of mice. Data are expressed as means ± SEM.

In contrast to the striking difference in PGE₂ production seen between iNOS $-$ / $-$ and wt mice, COX-1 and COX-2 mRNA expressionwere very similar in both types of mice. This suggests that theNO-induced rise in PGE₂ levels was attributable to an increasein COX-1 and/or COX-2 enzymatic activity, rather than to alteredgeneexpression.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Our data indicate that NO production from iNOS in the spinal cord immediately follows the early induction of peripheral tissuedamage and inflammation. This process occurs in parallel to thedevelopment of thermal hyperalgesia and is required for the increasein spinal PGE₂ production. Our data therefore attribute a decisiverole to iNOS in the early phase of development of thermalhyperalgesia.

It appears that NO production immediately after peripheral tissue damage is predominantly iNOS-derived. This is corroboratedby our results, which show an induction of iNOS mRNA in the spinalcord as early as 30 min after zymosan injection. Furthermore,administration of L-NAME intrathecally into iNOS $-$ / $-$ mice was withoutany effect with regard to thermal hyperalgesia. This stronglyargues against an extensive contribution of nNOS or eNOS. Observationsof Clark et al. (1996), MacNaughton et al. (1998), Haddad et al.(1995), and Salvemini et al. (1995) of an early iNOS expressionalso support our results. Reconstitution of the fast developmentof hyperalgesia by the NO donor RE-2047 (Rehse and Ciborski, 1995)demonstrates the importance of early NO production. To relatethis to the lack of iNOS genes, we injected the selective iNOSinhibitor L-NIL into wt mice; it reduced development of thermalhyperalgesia. The dose of L-NIL chosen (0.1 µM; 5 µl) does notaffect the other NOS isoforms (Moore et al., 1994). Furthermore,our results support previous studies showing that selective pharmacologicalinhibition of iNOS attenuates thermal hyperalgesia in rats (Osborneand Coderre, 1999). Only when given intrathecally did L-NIL inhibitNO production in the spinal cord and result in antinociceptiveeffects. These data indicate that only spinal iNOS-derived NOproduction correlates with antinociceptive activity. Interestingly,a substantial part of thermal hyperalgesia was insensitive toinhibition of iNOS and is also considered insensitive to COX inhibition.This insensitivity becomes dominant during the late phase of thermalsensitization ~8 hr after zymosan injection. It is likely thatboth peripheral mechanisms such as sensitization of capsaicinreceptors (Caterina et al., 1997; Kress and Zeilhofer, 1999) andcentral mechanisms independent from PG and NO contribute to thislatephase.

In wt mice, COX inhibition by indomethacin and disruption of the iNOS gene resulted in virtually indistinguishable antinociceptiveeffects. In iNOS $-$ / $-$ mice, indomethacin failed to display an antinociceptiveeffect. Antinociceptive activity could be restored in these miceby adding back NO with the NO donor RE-2047. These results demonstratethat the production of spinal PGE₂ requires spinal NO and thatspinal iNOS-derived NO appears to mediate thermal hyperalgesialargely if not solely via an increase in spinal PGE₂ formation.In this respect, our data support previous evidence that PGs arekey mediators of thermal hyperalgesia (Minami et al., 1994; Ferreiraand Lorenzetti, 1996; Yamamoto and Nozaki-Taguchi, 1997). We alsoconfirmed findings that hindpaw inflammation produces enhancedPG levels in the spinal cord (Yang et al., 1996; Hay and de Belleroche,1997; Ichitani et al., 1997; Yamamoto and Nozaki-Taguchi, 1997;Dirig and Yaksh, 1999; Ebersberger et al., 1999).

In line with several studies, we could show that PG production in the spinal cord is modulated positively by NO release andis diminished by lack of NO production (Salvemini et al., 1994,1995; Salvemini, 1997; but see also Hamilton and Warner, 1998).Substitution of NO by RE-2047 completely reconstituted PGE₂ productionin iNOS $-$ / $-$ mice as well as nociceptive responses in the behavioraltests, indicating once again that iNOS-derived NO amplifies PGproduction at spinal level. Moreover, the constitutive baselinemRNA expression (Beiche et al., 1996, 1998) and zymosan-inducedexpression of COX-2 were similar in both types of mice in thedorsal horn of the spinal cord. Consequently, it appears plausibleto attribute to iNOS-derived NO a pivotal role as a trigger ofspinal enzymatic PGproduction.

PGE₂ and NO production did not run in parallel. NO exhibited a fast peak within ~1 hr, whereas increases in PGE₂ occurredat a markedly prolonged time scale. Our results suggest that PGE₂production is not attributable to increased COX-1 or COX-2 expression.It may be speculated that the enhanced early PG production iscaused by a free radical driven modulation of phospholipase A₂activity and therefore of the concentration of arachidonic acid,which is the rate-limiting substrate of PG production (but seealso Zingarelli et al., 1997; Sahnoun et al., 1998). However,a direct or indirect interaction of NO or one of its metaboliteswith the COX-1 or COX-2 proteins by enhancing their enzymaticactivity is also possible (Salvemini, 1997). In either case onewould assume that the NO-induced change in COX enzyme activityoutlasts the rise in spinal NO, e.g., via sustained changes inenzyme activity of COX-1, COX-2, or phospholipase A₂.

An intriguing question raised by our study is whether inhibition of iNOS provides a novel target for analgesic therapy. Ourexperiments have shown that inhibition of iNOS via gene disruptionor by selective drugs almost completely abolishes the PG-mediatedpart of thermal hyperalgesia. With the possible exception of inhibitionof resistance to certain microbial agents, iNOS $-$ / $-$ mice are notonly viable but also show no major abnormalities indicating thatpharmacological inhibition of iNOS may be considered as largelysafe. The use of iNOS inhibitors as analgesics would be largelylimited by the fact that they would have to be administered veryearly, before spinal PG production has beentriggered.

Our data also indicate that NO donors reaching the CNS may be enhancers of pain development and in this respect be problematic.This observation is in line with findings of Urban et al. (1999),Inoue et al. (1997), and Aley et al. (1998) (but see also Laurettiet al., 1999) and should be subjected to furtherresearch.

Our data offer no clues indicating whether the decrease of NO production seen in our animals before hyperalgesia reaches itspeak is of importance for the later normalization of hyperalgesiathat goes along with healing processes in the damaged tissue (Reichneret al., 1999).

In summary, we have shown that NO generated by iNOS not only plays an important role as a mediator of tissue inflammationacting in peripheral tissue, but that it also serves an importantrole in the spinal cord, where it triggers PGE₂ formation, enhancesCOX-2 activity, and facilitates the development of thermal andpossibly other forms ofhyperalgesia.

  FOOTNOTES

Received Feb. 23, 2000; revised June 7, 2000; accepted June 16, 2000.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB 353, A1). We thank Dr. Ivan Otterness, visiting professorof the department, for the helpful suggestions and corrections.We acknowledge the professional help of Tanja Mittmann, AlexandraSchmauss, and IsabellaKolberg.
H.G. and M.G. contributed equally to thiswork.

Correspondence should be addressed to Dr. Hans Guehring, Department of Experimental and Clinical Pharmacology and Toxicology,Fahrstrasse 17, D-91054 Erlangen, Germany. E-mail: guehring{at}pharmakologie.uni-erlangen.de.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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