Spinal Prostaglandins Are Involved in the Development But Not the Maintenance of Inflammation-Induced Spinal Hyperexcitability

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The Journal of Neuroscience, November 15, 2001, 21(22):9001-9008

Spinal Prostaglandins Are Involved in the Development But Not the Maintenance of Inflammation-Induced Spinal Hyperexcitability
Enrique Vasquez, Karl-Jürgen Bär, Andrea Ebersberger, Barbara Klein, Horacio Vanegas, and Hans-Georg Schaible
Institut für Physiologie I, Universität Jena, D-07740 Jena, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Prostaglandins (PGs) are local mediators of several functions in the CNS. Both primary afferent neurons and intrinsic cellsin the spinal cord produce PGs, with a marked upregulation duringperipheral inflammation. Therefore, the significance of spinalPGs in the neuronal processing of mechanosensory information washerein investigated. In anesthetized rats, the discharges of spinalnociceptive neurons with input from the knee joint were extracellularlyrecorded. Topical administration of prostaglandin E₂ (PGE₂) tothe spinal cord facilitated the discharges and expanded the receptivefield of dorsal horn neurons to innocuous and noxious pressureapplied to the knee joint, the ankle, and the paw, thus mimickinginflammation-induced central sensitization. Conversely, topicaladministration of the PG synthesis inhibitor indomethacin to thespinal cord before and during development of knee joint inflammationattenuated the generation of inflammation-induced spinal neuronalhyperexcitability. However, after development of inflammation,the responses of spinal neurons to mechanical stimuli were onlyreduced by systemic indomethacin but not by indomethacin appliedto the spinal cord. Thus, spinal PG synthesis is important forthe induction and initial expression but not for the maintenanceof spinal cord hyperexcitability. Spinal PGE₂ application facilitateddorsal horn neuronal firing elicited by ionophoretic deliveryof NMDA, suggesting that an interaction of PGs and NMDA receptorsmay contribute to inflammation-induced central sensitization.However, after development of inflammation, spinal indomethacinfailed to reduce responses to ionophoretic delivery of NMDA orAMPA, suggesting that such an interaction is not required forthe maintenance of centralsensitization.

Key words: central sensitization; glutamate; pain; nociception; NSAID; prostaglandin

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Prostaglandins (PGs) are local mediators in a variety of functions in the CNS as well as in peripheral tissues. Considerableinformation has emerged in recent years regarding the involvementof spinal cord PGs in pain and central sensitization (Vanegasand Schaible, 2001). Indeed, cyclooxygenases 1 and 2 (COX-1 andCOX-2), the enzymes that form prostaglandin E₂ (PGE₂) and otherPGs from arachidonic acid, are expressed in both dorsal root ganglia(DRGs) and the spinal cord (Willingale et al., 1997; Inoue etal., 1999). Both isoforms of COX are expressed constitutively,but in particular COX-2 is markedly upregulated in the spinalcord during acute and chronic peripheral inflammation (Beicheet al., 1996, 1998a; Hay and de Belleroche, 1997; Hay et al.,1997; Goppelt-Struebe and Beiche, 1998; Ebersberger et al., 1999;Samad et al., 2001). In the spinal cord, there is a basal releaseof PGE₂ as well as an increased release after noxious stimulation,such as electrical pulses (Ramwell et al., 1966), noxious heat(Coderre et al., 1990), subcutaneous formalin (Malmberg and Yaksh,1995a,b; Hua et al., 1999; Muth-Selbach et al., 1999), and peripheralinflammation (Yang et al., 1996a; Hay et al., 1997; Hay and deBelleroche, 1998; Ebersberger et al., 1999; Gühring et al., 2000).Conversely, intrathecal administration of PGE₂ causes allodyniaand hyperalgesia in awake animals (Taiwo and Levine, 1988; Udaet al., 1990; Minami et al., 1994a, 1996; Malmberg et al., 1995a,b;Nishihara et al., 1995; Ferreira and Lorenzetti, 1996). Finally,antinociceptive nonsteroidal anti-inflammatory drugs (NSAIDs),such as indomethacin, inhibit PG synthesis not only in the inflamedperipheral tissues but also in the spinal cord, an effect thatmay contribute to their antinociceptive action (Vanegas and Schaible,2001).

Curiously, the effects of PGs on spinal dorsal horn neuronal firing have until now received only scant attention (Vanegasand Schaible, 2001), although this activity is precisely the drivefor segmental and suprasegmental reflexes as well as for the thalamocorticaltransmission that leads to the perception of pain. In the presentexperiments, we therefore determined the effects of spinally appliedPGE₂ on the responses of nociceptive dorsal horn neurons to naturalmechanical innocuous and noxious stimulation of the knee and otherperipheral tissues. We further investigated whether there is aninteraction between PGE₂ and glutamatergic synaptic transmissionin the spinal dorsal horn. Finally, we tested whether spinal applicationof a COX inhibitor influences the development and maintenanceof inflammation-induced hyperexcitability of nociceptive neuronsto mechanosensory stimuli, because mechanical hyperalgesia (pressurehypersensitivity) is an important pain symptom of jointinflammation.

Parts of this work have been published previously in abstract form (Vasquez et al., 2000, 2001).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation
Experiments were performed on 75 male Wistar rats (200-350 gm; University of Jena, Jena, Germany) anesthetized with sodiumthiopentone (Trapanal; initial dose of 85-115 mg/kg, i.p.; BYKGulden Ltd., Konstanz, Germany). The trachea was cannulated, andcatheters were inserted into the common carotid artery and theexternal jugular vein. The animals breathed spontaneously, anda gentle jet of oxygen was blown toward the opening of the trachealcannula. Body temperature was kept at 37°C by means of a feedback-controlledsystem. Additional intraperitoneal injections of thiopentone (20-50mg/kg) were given when necessary to achieve a sufficiently deeplevel of anesthesia as assessed by the absence of corneal or legwithdrawal reflexes. Mean arterial blood pressure was stable at90-120 mmHg. Spinal cord segments L1-L4 were exposed by laminectomy.The dura mater was opened, and a thin-walled, elliptic rubberring (~3 × 5 mm) was tightly sealed with silicone gel onto thesurface of the cord. This ring thus formed a trough with ~30 µlcapacity over the spinal segments in which the recordings wereto be performed. This trough was immediately filled with Tyrode'ssolution. A solution of 3% agar in Tyrode's solution was pouredaround the trough to seal and stabilize the surgicalarea.
In 51 rats, an inflammation was induced in the left knee joint, either at the beginning of the experiment before recordings(n = 33 rats) or during the recording session while an ipsilateralneuron was being monitored (n = 18 rats). With this purpose, a27 gauge needle was introduced through the patellar ligament,and 70 µl of a 4% kaolin suspension (Sigma, Deisenhofen, Germany)was slowly injected into the articular cavity. Then, the jointwas slowly flexed and extended for 15 min. Thereafter, 70 µl ofa 2% carrageenan solution (Sigma) was injected, and the jointwas moved for another 5min.

Recording and mechanical stimulation
Using glass-insulated carbon filaments for extracellular recording, individual neurons were identified by spike shape andheight. The action potentials were continuously monitored on adigital oscilloscope to guarantee that the same neuron was recordedthroughout. The signal was also fed into a window discriminator,the output of which was processed by an analog-to-digital interfaceand a personal computer so that peristimulus time histograms couldbe constructed. Action potentials were also stored on hard diskby means of the Spike/Spidi software (Forster and Handwerker,1990). Final spike discrimination was performed off-line accordingto shape and size. Dorsal horn neurons were chosen for study ifthey responded to pressure applied to the ipsilateral, left kneebut did not respond to brushing or squeezing of the skin overthe knee. The size of, and the threshold within, receptive fieldswere determined using stimulation of the skin (brushing or squeezingof skin folds with forceps) and of the deep tissue (manual compressionof joints and muscles). Mechanical test stimuli of two standardintensities were then applied to the knee, the ankle, and thepaw. Each test stimulus lasted for 15 sec. A calibrated mechanicaldevice (CORREX; Haag-Streit, Bern, Switzerland) was used for compressionof the knee joint in the mediolateral axis; for innocuous intensity,a 1.9 N/40 mm² holding pressure was applied, and for noxious intensity (feltpainful when applied to the experimenter's fifth finger), theknee was compressed with 7.8 N/40 mm² (or with 5.9 N/40 mm² when the response was very strong). Two modified crocodile clipswith teeth filed away and jaws wrapped in tape were used to applymediolateral compression of the ankle joint and dorsoventral compressionof the middle of the paw (1.1 N/20 mm² for innocuous stimulation, and 5.8 N/20 mm² for noxiousstimulation).

Ionophoretic delivery of glutamatergic agonists
In one set of experiments, we used the ionophoretic administration of AMPA (Research Biochemicals, Deisenhofen, Germany) andNMDA (Research Biochemicals) close to the neurons. A carbon filament,glass-insulated microelectrode was glued onto a multibarrel glassmicropipette so that their tips ended together. The carbon microelectrodewas used for recording of extracellular unitary action potentialsfrom nociceptive dorsal spinal neurons with input from the knee(see above). The multibarrel micropipette was used for ionophoresis.One barrel was filled with AMPA (10 mM in 155 mM NaCl, pH 7.5,adjusted with NaOH), and another one was filled with NMDA (50mM in 115 mM NaCl, pH 7.5, adjusted with NaOH). Two other barrelswere filled with NaCl; one of them (1 M) served for automaticcurrent balancing, and the other (165 mM) served for control ofcurrent application. Ejection currents for NMDA and AMPA werenegative, and positive retaining currents of 25 nA were used betweenejectionperiods.

Experimental protocols
Effect of spinally applied PGE₂ on responses to mechanical stimulation. In the first set of experiments (15 rats, one neuronper rat), we tested the effects of PGE₂ on the responses of spinalcord neurons to mechanical stimulation of the left knee, ankle,and paw. Innocuous and noxious test stimuli were applied sequentiallyto the knee, the ankle, and the paw. This sequence was repeatedevery 5 min, even when the manipulations described below werebeing performed. The neuronal baseline responses were establishedwith the vehicle solution (0.07% ethanol in Tyrode's solution)in the spinal trough, and, when the responses were stable, thelast 25 min before application of PGE₂ were taken as the predrugcontrol period. After having established the baseline responses,the spinal trough was rinsed and filled with 30 µl of a solutioncontaining PGE₂ (100 ng/µl; Cayman Chemical, Ann Arbor, MI). Thisdose of PGE₂ was chosen from behavioral experiments using intrathecalapplication of PGE₂ (Vanegas and Schaible, 2001). The mechanicalstimulation of knee, ankle, and paw was continued, and, after50 min, the PGE₂ solution was replaced by the vehicle solution.The responses to mechanical stimulation were continued for another25-50 min to observe recovery. In four experiments, the effectof the vehicle alone was tested and found to benought.
In some experiments, PGE₂ was applied a second time while the same cell (four experiments) or another cell (eight experiments)was being recorded. The same procedure was used with another eightrats, but in these experiments, the knee joint had been inflamed5-10 (on average 7) hours before the recordingsstarted.
Effect of the application of the COX inhibitor indomethacin. In the second set of experiments, we studied the effect of spinallyadministered indomethacin on the development and maintenance ofinflammation-evoked mechanical hyperexcitability of dorsal hornneurons. To study its effect on development of hyperexcitability,indomethacin was applied before the inflammation was induced.In eight rats (one neuron per rat), the responses of the neuronsto mechanical stimulation of knee, ankle, and paw (see above)were monitored for 25 min. Then, indomethacin (Calbiochem, BadSoden, Germany) was administered at a dose of 8 mM (Vanegas andSchaible, 2001) into the spinal trough, and the responses to mechanicalstimulation were tested for another 25 min. Thereafter, the inflammationwas induced (see above), and the responses to stimulation of knee,ankle, and paw were followed for another 4 hr still in the presenceof indomethacin. Another 10 rats were used to assess the developmentof hyperexcitability in the absence of indomethacin. In theseanimals, only the vehicle (10 mM Na₂HPO₄, 17.65 mM NaOH, and 63.4mM NaCl, pH 7.5, adjusted with HCl) was administered to the spinalcord while the responses to mechanical stimulation of knee, ankle,and paw were monitored before (25 min) and after induction ofinflammation (4hr).
To study the effect of indomethacin on the maintenance of spinal cord hyperexcitability, an inflammation was induced first,and the recordings from neurons with knee input were started 5-10hr thereafter (eight rats). The responses to mechanical stimulationof the knee, ankle, and paw were assessed for a period of 50 min,with vehicle (see above) on the spinal cord. Then, indomethacin(8 mM) was applied to the spinal cord surface, and the responsesto the mechanical test stimuli were monitored for 100 min duringwhich indomethacin was on the cord. Thereafter, indomethacin (4mg/kg) was given intraperitoneally, and the protocol was continuedfor another 50min.
Effect of PGE₂ and indomethacin on glutamatergic responses. In the third set of experiments (nine rats with normal knee and12 rats with inflamed knee, one neuron per rat), we tested whetherthe application of PGE₂ to the surface of the spinal cord wouldalter the responses to ionophoretic administration of AMPA orNMDA. Once a neuron had been characterized, ionophoretic applicationof AMPA or NMDA was started. After a variable number of seconds,the neuron began to fire, and ionophoretic application was thenmaintained for 10 sec after the first evoked spike. An ejectioncurrent was chosen such that it reproducibly induced clear responsesthat could be modulated in both directions (increase or decrease).Application of AMPA or NMDA began every 60 sec and was repeateduntil a stable baseline of 50 min duration was obtained. Then,PGE₂ (100 ng/µl) was administered for 50 min, and the applicationof AMPA or NMDA was performed. Finally, the responses were monitoredafter washout of PGE₂ for 50min.
In another five rats with an inflammation in the knee joint, the effect of indomethacin on the responses to AMPA and NMDAwas tested. AMPA and NMDA were administered ionophoretically for50 min as described above, and then indomethacin (8 mM) was administeredinto the spinal trough and the responses to AMPA and NMDA werecontinued for 50 min. Thereafter, indomethacin was replaced byTyrode's solution, and the responses to AMPA and NMDA were recordedfor another 50min.
Data analysis. The responses to pressure stimuli were calculated by subtracting the ongoing activity in the preceding 15 sec(if any) from the total activity during an innocuous or a noxioustest stimulus. To evaluate the effects of PGE₂ on the responsesto mechanical stimulation, we averaged all of the test responsesto each type of stimulus in the 25 min preceding drug application(baseline), as well as the test responses during the last 25 minof PGE₂ application. Values are given in mean ± SE. Baseline andPGE₂ values were compared by using the Wilcoxon matched-pairssigned rank test. A similar procedure was used for the evaluationof the effects of PGE₂ on the responses to NMDA and AMPA. Theresponses in the last 25 min before PGE₂ (baseline) were averagedand normalized to 100%, and the values in the last 25 min of PGE₂application were expressed as percentage of baseline. A similarprocedure was used to analyze effects ofindomethacin.
In experiments in which we assessed the effects of indomethacin on the development of inflammation-induced hyperexcitability,the baseline responses before inflammation were averaged (mean± SE). After injection of kaolin into the knee, the responsesto each stimulus within every hour after kaolin were averaged,and the baseline responses were subtracted. For statistical analysis,we compared the increase of the responses in the nontreated andthe indomethacin-treated animals at corresponding intervals of1 hr using the Mann-Whitney U test. In all statistical tests,significance was acknowledged if p < 0.05.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

All neurons with knee input were located in segments L1-L4 at depths of 700-1200 µm (mean of 954 µm), thus mainly in the deepdorsal horn. Typically, the receptive field also included deeptissues of the thigh and lower leg. In 42 rats with normal joints,29 of 42 neurons were wide dynamic range neurons that respondedto innocuous and noxious stimulation of the knee in a graded manner,and 13 of 42 neurons were nociceptive specific and responded onlyto noxious pressure applied to the knee and other tissues. In20 of these 42 neurons, the receptive field extended to the ankleand, in eight neurons, further to the paw. Three of these neuronshad cutaneous receptive fields located on the thigh and/or thelower leg. Spontaneous activity was usually absent. In the sampleof 33 neurons with input from the inflamed knee joint, 26 neuronswere wide dynamic range, and seven were nociceptive-specificneurons.

Effect of PGE₂ on the responses of spinal cord neurons

The effects of spinally applied PGE₂ on the responses of dorsal horn neurons to mechanical stimulation of the ipsilateralhindlimb were studied in 15 neurons. Figure 1 shows the responsesto innocuous and noxious pressure applied to the knee joint, theankle, and the paw. During baseline stimulation the spinal cordtrough was filled with vehicle solution. When this was replacedby the PGE₂ solution (100 ng/µl), the responses to both innocuousand noxious pressure showed a gradual increase. When the PGE₂-containingsolution was replaced by the vehicle, the responses declined slowly.However, recovery was incomplete in most of the neurons (thisis indicated by the large SE in the post-PGE₂ period).

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Figure 1. Effect of PGE₂ on the responses of dorsal horn neurons to mechanical stimulation of the ipsilateral knee joint, ankle, and paw. Each symbol shows the mean ± SE of the responses. nox., Noxious pressure; innoc., innocuous pressure. During the first 25 min, only vehicle solution was in the spinal cord trough. This was replaced for 50 min (shaded area) by a solution containing PGE₂ (100 ng/µl).

For statistical analysis, we compared the average responses in the last 25 min of PGE₂ application versus the average baselineresponses by using the Wilcoxon matched-pairs signed rank test.The increase of the responses was significant for innocuous (p< 0.005) and noxious (p < 0.001) pressure applied to the knee(n = 15 neurons), for innocuous (p < 0.005) and noxious (p < 0.01)pressure applied to the ankle (n = 12 neurons), and for innocuous(p < 0.05) and noxious (p < 0.05) pressure applied to the paw(n = 7 neurons). The number of neurons for knee was greater thanfor ankle or paw because their receptive fields did not alwaysextend to these latter regions. Interestingly, however, PGE₂ applicationcaused an expansion of the receptive field in some neurons. Thus,under PGE₂, three neurons that did not respond to ankle stimulationinitially became responsive to noxious compression of the ankle,and three neurons whose receptive field did not include the pawinitially became responsive to noxious stimulation of the paw.After PGE₂, the responses increased in both nociceptive-specificand wide dynamic rangeneurons.

In four experiments, a second application of PGE₂ was made during recording from the same neuron, 2 hr 15 min after the firstapplication. In eight additional experiments, a second neuronwas identified ~2 hr after the protocol with the first neuronhad been completed, and the same protocol was performed with thenew neuron. In contrast to the first application of PGE₂, thesecond administration did not change the responses to mechanicalstimulation (n = 12) (Fig. 2).

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Figure 2. Effect of PGE₂ (shaded area) when spinally applied after a previous application of PGE₂. The graph displays the responses of 12 spinal cord neurons to noxious (nox.) and innocuous (innoc.) pressure onto the knee joint. Same type of display as in Figure 1.

During inflammation of peripheral tissues, the milieu in the spinal cord is modified such that excitatory synaptic transmissionbecomes more efficient and spinal nociceptive neurons become hyperexcitable.Furthermore, endogenous release of PGE₂ is increased (see introductoryremarks). In view of the above results with a second PGE₂ application,in eight neurons we tested the effects of PGE₂ on the responsesto mechanical stimulation when the knee joint had been inflamedfor 5-10 (on average 7) hours. When applied during inflammation,PGE₂ increased the neuronal responses to mechanical stimuli, butthe effects were smaller than in non-inflamed animals (Fig. 3).However, this comparison reached statistical significance onlyfor knee stimulation (p < 0.05; one-sided; Mann-Whitney U test).

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Figure 3. PGE₂-induced changes in the responses to mechanical stimulation of knee, ankle, and paw in rats with non-inflamed knees and in rats with inflammation of the stimulated knee joint. The columns show the mean ± SE increase of the responses above baseline in the last 25 min of the PGE₂ application. *p < 0.05, significant difference between increase above baseline in rats with normal knees and rats with inflamed knees.

Effect of indomethacin on the development and maintenance of inflammation-induced hyperexcitability

In these experiments, we addressed the role of endogenous spinal PGs in the induction and maintenance of inflammation-inducedhyperexcitability for mechanical stimuli. The PG synthesis inhibitorindomethacin that reduces stimulus-evoked PGE₂ release from spinalcord (Malmberg and Yaksh, 1994) was applied into the spinal trough.Figure 4 illustrates the experiments in which indomethacin wasgiven before induction and during development of inflammation.First, we recorded the baseline responses, and then we inducedthe knee inflammation by injection of kaolin and carrageenan (K/C)and monitored the neurons for another 4 hr. Indomethacin was given25 min before kaolin was injected and had no immediate effecton neuronal responses. Indeed, in five neurons, the average responseto noxious pressure onto the knee joint before indomethacin was273 ± 89 impulses/15 sec and after indomethacin was 260 ± 93 impulses/15sec. However, indomethacin attenuated the inflammation-inducedchanges. Figure 4 shows the responses to noxious and innocuouspressure applied to the knee and ankle in nontreated control animalsand in animals that received indomethacin in the spinal trough.In all graphs, the responses in the baseline period were set tozero, and the values after K/C express the increase of the responsesabove baseline. In the untreated rats, we observed a pronouncedincrease of the responses to mechanical stimulation of the injectedknee (showing peripheral sensitization and ensuing spinal cordactivation and sensitization) and of the non-inflamed ankle (showingcentral sensitization) within the 4 hr of knee inflammation (Fig.4, open squares). The circumference of the injected knees increasedon average from 43 to 50 mm. In contrast, when indomethacin waspresent in the spinal trough before and during development ofknee inflammation, there was no increase in the responses to innocuousor noxious stimulation of the non-inflamed ankle or to innocuousstimulation of the injected knee. The responses to noxious pressureon the knee showed a small but significant increase. For statisticalanalysis, we compared for all stimuli the values obtained in eachof the 4 hr after induction of inflammation (Mann-Whitney U test).In neurons from rats without indomethacin, the responses to mechanicalstimulation of the inflamed knee and of the non-inflamed anklewere significantly larger than in rats with indomethacin treatment(Fig. 4). In rats with spinal indomethacin, the circumferenceof the injected knees increased on average from 44 to 50 mm (sameas in control experiments).

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Figure 4. Effect of spinal application of indomethacin on the development of inflammation-induced hyperexcitability of spinal cord neurons. The graphs show the changes of the responses to noxious (nox.) and innocuous (innoc.) pressure ipsilaterally applied to the knee and to the ankle in the 4 hr after induction of inflammation in the knee by intra-articular injection of K/C. When the spinal trough was filled with vehicle solution (open squares) or with indomethacin (filled squares), the baseline (BL) values before K/C were set to zero, and the values after K/C injection show the mean ± SE change of all of the responses within each hourly interval compared with baseline. For stimulation of the knee joint, each value shows at least the averaged responses from seven animals and for stimulation of the ankle at least from four animals.

The inflammation induced by K/C and the resulting hyperexcitability of spinal cord neurons reach a plateau after 5-6 hr, i.e.,the responses usually do not further increase after this time(Neugebauer et al., 1993). In additional experiments, we testedthe effect of indomethacin when the compound was given after developmentof inflammation (Fig. 5). Indomethacin (8 mM) was administeredto the spinal cord 6-11 hr after induction of inflammation. Althoughindomethacin was applied to the spinal cord for 100 min, no reductionof the responses to knee stimulation was noted, nor were the responsesto stimulation of the ankle and paw reduced. These data thereforesuggest that inhibition of spinal PG synthesis after developmentof inflammation does not influence central sensitization. Whenindomethacin was given intraperitoneally at a later time, theresponses to pressure onto the knee showed a progressive reduction.When the last three values after intraperitoneal injection ofindomethacin were compared with the last three values before intraperitonealinjection of indomethacin, the reduction of the responses to noxiouspressure was statistically significant for noxious pressure (p< 0.05; Wilcoxon matched-pairs signed rank test; n = 6 neurons).This is probably attributable to extraspinal effects of indomethacin.

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Figure 5. Effects of indomethacin on neuronal responses after development of hyperexcitability. The recordings started 6-11 hr after induction of inflammation in the ipsilateral knee joint. Each symbol represents the mean ± SE of the responses of spinal cord neurons to innocuous (innoc.) and noxious (nox.) pressure onto the knee joint under spinal application and subsequent intraperitoneal administration of indomethacin.

Effect of PGE₂ on the responses to AMPA and NMDA

Behavioral experiments have shown that the hyperalgesia evoked by PGE₂ can be blocked by antagonists at NMDA and non-NMDAreceptors (Minami et al., 1994b; Nishihara et al., 1995a). Furthermore,NMDA receptors are thought to be key players in the generationand maintenance of inflammation-induced hyperexcitability (Woolfand Thompson, 1991; Neugebauer et al., 1993). Thus, an interactionbetween PGE₂ and glutamatergic synaptic transmission is of particularinterest. We therefore studied whether the application of PGE₂would influence responses of spinal cord neurons to the applicationof AMPA and NMDA, the agonists at ionotropic glutamate receptors.Neurons that responded to mechanical stimulation of the knee jointwere stimulated by the ionophoretic administration of AMPA orNMDA. The knee joint was either normal or inflamed. Figure 6 showsthe effects of PGE₂ on the responses of neurons to AMPA or NMDA.The line graphs show the average responses to each test applicationof AMPA or NMDA. The columns display the average responses inthe 25 min before PGE₂, the responses in the last 25 min of PGE₂application, and the responses after washout of PGE₂, expressedas percentage of baseline. The baseline responses were obtainedwhile Tyrode's solution was in the spinal cord trough. In animalswith normal knees (Fig. 6, top), only the responses to NMDA showeda significant increase (p < 0.05; Wilcoxon matched-pairs signedrank test) during application of PGE₂. However, when the kneewas inflamed, both the responses to AMPA and to NMDA (Fig. 6,bottom) showed marked progressive increases (for AMPA, p < 0.005;for NMDA, p < 0.005; Wilcoxon matched-pairs signed rank test).

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Figure 6. Effects of PGE₂ on the responses of spinal cord neurons to the ionophoretic application of AMPA or NMDA. Neurons in the top panels were in animals with normal joints, and neurons in the bottom panels were in rats with inflammation of the ipsilateral knee joint. The line graphs below the column diagrams show the responses to each test application of AMPA or NMDA, averaged in the total sample of neurons. For each neuron, responses are expressed as percentage of the average of all its responses during baseline. Each square represents the mean ± SE of the response of all neurons to one AMPA application (left) or one NMDA application (right). The column diagrams display the average response in the 25 min before PGE₂, the average responses in the last 25 min of PGE₂ application (shaded area), and the average responses after washout of PGE₂, expressed as percentage of baseline. *p < 0.05 versus baseline.

To test whether a reduction of endogenous spinal PGs would alter the activation of glutamate receptors after inflammationis established, we tested the effect of spinal application ofindomethacin on the responses to AMPA and NMDA. As with mechanicalstimulation, indomethacin (8 mM) was administered 6-11 hr afterinduction of inflammation. Figure 7 shows that neither the responsesto AMPA nor the responses to NMDA were significantly changed inthe presence of indomethacin.

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Figure 7. Effects of indomethacin on responses to AMPA or NMDA after development of hyperexcitability. The recordings started 6-11 hr after induction of inflammation in the ipsilateral knee joint. Graphs illustrate the effects of topical administration of indomethacin to the spinal cord on the responses of dorsal horn neurons to ionophoretically administered AMPA or NMDA. Each symbol displays one neuron.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the present study, topical application of PGE₂ to the spinal cord enhanced the responses of dorsal horn neurons to mechanicalstimuli and expanded their receptive fields. These effects mimicthe central sensitization that develops during knee joint inflammation.Spinal application of indomethacin before and during developmentof knee joint inflammation did not prevent the inflammation inthe knee but markedly attenuated the generation of hyperexcitabilityin spinal cord neurons. Administration of indomethacin 6-11 hrafter development of inflammation, however, did not reduce theenhanced responses. Thus, endogenous PG synthesis in primary afferentneurons and/or spinal cord seems necessary and sufficient forthe induction of central sensitization but not for its maintenance.Topical application of PGE₂ to the spinal cord enhanced the responsesof nociceptive neurons to the ionophoretic application of NMDA,thus suggesting that PGE₂ interaction with glutamatergic synaptictransmission contributes to the PG role in central sensitization.However, application of indomethacin after development of inflammationdid not reduce responses to ionophoretically administered NMDAand AMPA, again suggesting that after establishment of inflammationspinal PG synthesis is not essential for glutamatergicsensitivity.

Prostaglandins and the increase in responsiveness of spinal cord neurons

The effects of PGE₂ on neurons in vitro as well as on animal behavior have been studied extensively (Vanegas and Schaible,2001). However, we have herein investigated the effects of PGE₂on nociceptive neuronal discharges, i.e., messages that may leadto perception and behavioral responses, elicited by "natural"innocuous and noxious stimuli. As mentioned, PGE₂ induced a patternof effects on spinal cord neurons similar to that of central sensitizationin general and of inflammation-induced hyperexcitability in particular.After PGE₂, like during peripheral inflammation (Woolf 1983; Hyldenet al., 1989; Neugebauer and Schaible, 1990; Dougherty et al.,1992), and in agreement with behavioral experiments (see introductoryremarks), the neurons showed an increased firing to noxious mechanicalstimulation, which may lead to primary mechanical hyperalgesia,a decrease in the excitation threshold, and thus enhanced or novelresponses to innocuous stimulation, which may lead to allodynia,and an expansion of the receptive field, which is typical of centralsensitization and may lead to secondary mechanical hyperalgesia.Preliminary experiments show that butaprost, an EP2 agonist, producessimilar effects as PGE₂ in a dose-dependentmanner.

We also studied herein the consequences of reducing the effect of PGs during the induction of inflammation, because in inflammation,PG synthesis and release in the spinal cord are upregulated (seeintroductory remarks). Local transmitters and modulators may contributeto this upregulation, because NMDA (Sorkin, 1993), kainic acid(Yang et al., 1996b), substance P (Hua et al., 1999), depolarizationby K⁺ (Dirig et al., 1997), and capsaicin (Dirig and Yaksh, 1999) havebeen shown to stimulate PG synthesis and release in the spinalcord (Vanegas and Schaible, 2001). During inflammation, interleukin-1 $beta$ -mediatedinduction of COX-2 may be particularly important (Samad et al.,2001). Because no specific antagonists are available for PG receptors,we applied indomethacin, a COX-1/COX-2 inhibitor, to the spinalcord before the inflammation began. This significantly attenuatedthe development of inflammation-induced neuronal hyperexcitability.Plausibly, the initial production of PGs in primary afferentsand/or spinal cord intrinsic elements is essential for the fulldevelopment of spinal cord plasticity. Indomethacin also reduceswindup of dorsal horn neuronal discharges to electrical C-fiberstimulation (Willingale et al., 1997) and the discharges of dorsalhorn neurons after subcutaneously applied formalin (Chapman andDickenson, 1992). Although these and the present results are takenas attributable to COX inhibition, contribution by non-COX targetscannot be excluded (Vanegas and Schaible, 2001).

Effects of PGE₂ on the responses to AMPA and NMDA

The results discussed above could arise from a PG effect on presynaptic elements, e.g., primary afferent terminals, or onpostsynaptic elements, e.g., intrinsic spinal neurons. PGE₂ actson G-protein-coupled receptors (EP1-4), and DRG neurons expressEP1 (Oida et al., 1995), EP3 (Sugimoto et al., 1994; Oida et al.,1995; Beiche et al., 1998b), and EP4 receptors (Oida et al., 1995),whereas spinal cord neurons express EP2 receptors (Kawamura etal., 1997). Thus, the spinal effects of naturally released orexperimentally applied PGE₂ on nociception may be exerted on boththe primary afferents and dorsal hornneurons.

The evidence for presynaptic targets is considerable. For example, PGE₂ enhances the release of substance P and calcitoningene-related peptide (CGRP) from cultured or native DRG neuronsthat is evoked by various chemical stimuli (Nicol et al., 1992;Andreeva and Rang, 1993; Vasko et al., 1993, 1994; Hingtgen andVasko, 1994; Southall et al., 1998). Conversely, NSAIDs diminishthe stimulus-induced release of substance P and CGRP from DRGneurons or spinal cord slices because this release is facilitatedby PGs (Andreeva and Rang, 1993; Vasko et al., 1994). Furthermore,PGE₂ application increases the frequency but not the amplitudeof miniature EPSCs mediated by AMPA receptors in spinal cord neurons(Minami et al., 1999). Recently, however, Baba et al. (2001) showedthat PGE₂ excites spinal cord intrinsic neuronsdirectly.

Here we show for the first time that PGE₂ increases firing of intrinsic neurons elicited by AMPA or NMDA. When the knees werenormal, PGE₂ caused a significant facilitation of firing to applicationof NMDA close to the neurons. This is of particular interest becausethe activation of NMDA receptors of dorsal horn neurons is thoughtto be a key mechanism in the induction of central sensitization(see above) and in particular the increase in mechanosensitivity(Neugebauer et al., 1993). When the joint was inflamed, PGE₂ inducedfacilitated responses to AMPA and NMDA. This could result frompresynaptic but also from postsynaptic effects of PGE₂. For example,PGE₂ might release compounds from primary afferents (e.g., substanceP) that facilitate the responses to glutamate receptor agonists.Alternatively or additionally, the sensitivity of postsynapticneurons to PGE₂ might increase during inflammation attributableto, for example, EP receptor sensitization. However, because theresponses to AMPA and NMDA were not reduced by indomethacin afterinflammation was established, a facilitation of glutamatergicsynapses by endogenous PGs does not seem to be the mechanism wherebycentral sensitization is maintained (see alsobelow).

Role of prostaglandins after development of inflammation

Unexpectedly, when the inflammation was established, the responses of spinal cord neurons to mechanical stimulation (and theresponses to AMPA or NMDA) were not reduced by spinal administrationof indomethacin. However, the responses to mechanical stimuliwere reduced after systemic administration of indomethacin. Becauseinhibition of PG synthesis by indomethacin is rapid, we shouldhave seen a reduction of the responses after spinal applicationif the continuous production of PGs in the spinal cord were importantfor the maintenance of hyperexcitability to mechanical stimuliduring inflammation. Interestingly, Dirig et al. (1998) observedno reduction of thermal hyperalgesia with intrathecal administrationof S(+)-ibuprofen or the specific COX-2 inhibitor SC58125 3 hrafter induction of carrageenan inflammation. It thus seems thatspinal PG synthesis is not required for the maintenance of centralsensitization, at least in the time period studied, and that analgesiceffects of NSAIDs in this period are exerted at sites other thanspinal targets, at least with respect to mechanical stimulation.Such targets could be the inflamed knee joint (Heppelmann et al.,1986) and supraspinal structures (Vanegas et al., 1997).

The lack of effect of spinal indomethacin after establishment of inflammation could have several reasons. First, there mightbe no additional spinal PG synthesis after the initial PG production,and hence indomethacin would not act. This seems unlikely, becauseupregulation of COX-2 in the spinal cord begins in the first hoursof inflammation and lasts for many hours or days (Vanegas andSchaible, 2001). Second, PGs and/or other spinal mediators might,as inflammation progresses, cause persistent changes, includinga decrease in the sensitivity of spinal neurons to PGs. Indeed,the effects of PGE₂ on the responses to mechanical stimulationwere not fully reversible, a second application of PGE₂ in thesame experiment did not further enhance these responses, and theeffects of PGE₂ on these responses were much less pronounced inrats with a knee inflammation. Thus, PGE₂ could initiate cellularevents that induce long-term changes in synaptic transmissionthat may contribute to the persistence of central sensitization.Because the activation of PG receptors sets in motion second messengersystems and enhances, for example cAMP (Vanegas and Schaible,2001), it is likely that second messengers could induce theselong-term changes. A desensitization of PG receptors or alterationsin the transduction cascade may be part of these effects. It shouldbe noted, however, that exogenous PGE₂ enhanced the responsesto AMPA and NMDA in the spinal cord of rats with inflamed knees,so that a total insensitivity of neurons to PGE₂ is unlikely,and other explanations should be sought in thefuture.

In all, the present results highlight the involvement of PGs in the facilitation of somatosensory neuronal discharges, particularlyduring induction of central sensitization. A direct and/or indirectfacilitation of glutamatergic synapses might underlie this effect,but other molecular players seem to be responsible for the sustainedcentralhyperexcitability.

  FOOTNOTES

Received May 2, 2001; revised Aug. 28, 2001; accepted Aug. 30, 2001.

This work was supported by Deutsche Forschungsgemeinschaft Grant Scha 404/11-1. E.V. held fellowships from the Deutscher AkademischerAustauschdienst and the Venezuelan Consejo Nacional de InvestigacionesCientíficas y Técnicas. We thank G. Cuny for skillful assistancewith the laboratorywork.
Correspondence should be addressed to Dr. Hans-Georg Schaible, Institut für Physiologie I der Universität Jena, Teichgraben8, D-07740 Jena, Germany. E-mail: schaible{at}mti-n.uni-jena.de.

E.V. and H.V. are on leave from the Instituto Venezolano de Investigaciones Cientificas, Apartado 21827, Caracas 1020A,Venezuela.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Andreeva L, Rang HP (1993) Effect of bradykinin and prostaglandins on the release of calcitonin gene-related peptide-like immunoreactivity from the spinal cord in vitro. Br J Pharmacol 108:185-190[ISI][Medline].
Baba H, Kohno T, Moore KA, Woolf CJ (2001) Direct activation of rat spinal dorsal horn neurons by prostaglandin E2. J Neurosci 21:1750-1756[Abstract/Free Full Text].
Beiche F, Scheuerer S, Brune K, Geisslinger G, Goppelt-Struebe M (1996) Up-regulation of cyclooxygenase-2 mRNA in the rat spinal cord following peripheral inflammation. FEBS Lett 390:165-169[ISI][Medline].
Beiche F, Brune K, Geisslinger G, Goppelt-Struebe M (1998a) Expression of cyclooxygenase isoforms in the rat spinal cord and their regulation during adjuvant-induced arthritis. Inflamm Res 47:482-487[ISI][Medline].
Beiche F, Klein T, Nüsing R, Neuhuber W, Goppelt-Struebe M (1998b) Localization of cycloogygenase-2 and prostaglandin E2 receptor EP3 in the rat lumbar spinal cord. J Neuroimmunol 89:26-34[ISI][Medline].
Chapman V, Dickenson AH (1992) The spinal and peripheral roles of bradykinin and prostaglandins in nociceptive processing in the rat. Eur J Pharmacol 219:427-433[ISI][Medline].
Coderre TJ, Gonzales R, Goldyne ME, West ME, Levine JD (1990) Noxious stimulus-induced increase in spinal prostaglandin E2 is noradrenergic terminal-dependent. Neurosci Lett 115:253-258[Medline].
Dirig DM, Konin GP, Isakson PC, Yaksh TL (1997) Effect of spinal cyclooxygenase inhibitors in rat using the formalin test and in vitro prostaglandin E2 release. Eur J Pharmacol 331:155-160[ISI][Medline].
Dirig DM, Isakson PC, Yaksh TL (1998) Effect of COX-1 and COX-2 inhibition on induction and maintenance of carageenan-evoked thermal hyperalgesia in rats. J Pharmacol Exp Ther 285:1031-1038[Abstract/Free Full Text].
Dirig DM, Yaksh TL (1999) In vitro prostanoid release from spinal cord following peripheral inflammation: effects of substance P, NMDA and capsaicin. Br J Pharmacol 126:1333-1340[ISI][Medline].
Dougherty PM, Sluka KA, Sorkin LS, Westlund KN, Willis WD (1992) Neural changes in acute arthritis in monkeys. I. Parallel enhancement of responses of spinothalamic tract neurons to mechanical stimulation and excitatory amino acids. Brain Res Rev 17:1-13[Medline].
Ebersberger A, Grubb BD, Willingale HL, Gardiner NJ, Nebe J, Schaible H-G (1999) The intraspinal release of prostaglandin E2 in a model of acute arthritis is accompanied by up-regulation of cyclo-oxygenase-2 in the spinal cord. Neuroscience 93:775-781[ISI][Medline].
Ferreira SH, Lorenzetti BB (1996) Intrathecal administration of prostaglandin E2 causes sensitization of primary afferent neurons via the spinal release of glutamate. Inflamm Res 45:499-502[ISI][Medline].
Forster C, Handwerker HO (1990) Automatic classification and analysis of microneurographic spike data using a PC/AT. J Neurosci Methods 31:109-118[ISI][Medline].
Goppelt-Struebe M, Beiche F (1998) Cyclooxygenase-2 in the spinal cord: localization and regulation after a peripheral inflammatory stimulus. Adv Exp Med Biol 433:213-216.
Gühring H, Görig M, Ates M, Coste O, Zeilhofer HU, Pahl A, Rehse K, Brune K (2000) Suppressed injury-induced rise in spinal prostaglandin E2 production and reduced early thermal hyperalgesia in iNOS-deficient mice. J Neurosci 20:6714-6720[Abstract/Free Full Text].
Hay CH, de Belleroche JS (1997) Carrageenan-induced hyperalgesia is associated with increased cyclo-oxygenase-2 expression in spinal cord. NeuroReport 8:1249-1251[ISI][Medline].
Hay CH, de Belleroche JS (1998) Dexamethasone prevents the induction of COX-2 mRNA and prostaglandins in the lumbar spinal cord following intraplantar FCA in parallel with inhibition of oedema. Neuropharmacology 37:739-744[Medline].
Hay CH, Trevethick MA, Wheeldon A, Bowers JS, de Belleroche JS (1997) The potential role of spinal cord cyclooxygenase-2 in the development of Freund's complete adjuvant-induced changes in hyperalgesia and allodynia. Neuroscience 78:843-850[ISI][Medline].
Heppelmann B, Pfeffer A, Schaible H-G, Schmidt RF (1986) Effects of acetylsalicylic acid (ASA) and indomethacin on single groups III and IV units from acutely inflamed joints. Pain 26:337-351[ISI][Medline].
Hingtgen CM, Vasko MR (1994) Prostacyclin enhances the evoked-release of substance P and calcitonin gene-related peptide from rat sensory neurons. Brain Res 655:51-60[ISI][Medline].
Hua X-Y, Chen P, Marsala M, Yaksh TL (1999) Intrathecal substance P-induced thermal hyperalgesia and spinal release of prostaglandin E2 and amino acids. Neuroscience 89:525-534[ISI][Medline].
Hylden JLK, Nahin RL, Traub RJ, Dubner R (1989) Expansion of receptive fields of spinal lamina I projection neurons in rats with unilateral adjuvant-induced inflammation: the contribution of dorsal horn mechanisms. Pain 37:229-243[ISI][Medline].
Inoue A, Ikoma K, Morioka N, Kumagai K, Hashimoto T, Hide I, Nakata Y (1999) Interleukin-1 $beta$ induces substance P release from primary afferent neurons through the cyclooxygenase-2 system. J Neurochem 73:2206-2213[ISI][Medline].
Kawamura T, Yamauchi T, Koyama M, Maruyama T, Akira T, Nakamura N (1997) Expression of prostaglandin EP2 receptor mRNA in the rat spinal cord. Life Sci 61:2111-2116[ISI][Medline].
Malmberg AB, Yaksh TL (1994) Capsaicin-evoked prostaglandin E₂ release in spinal cord slices: relative effect of cyclooxygenase inhibitors. Eur J Pharmacol 271:293-299[ISI][Medline].
Malmberg AB, Yaksh TL (1995a) Cyclooxygenase inhibition and the spinal release of prostaglandin E2 and amino acids evoked by paw formalin injection: a microdialysis study in unanesthetized rats. J Neurosci 15:2768-2776[Abstract].
Malmberg AB, Yaksh TL (1995b) The effect of morphine on formalin-evoked behaviour and spinal release of excitatory amino acids and prostaglandin E2 using microdialysis in conscious rats. Br J Pharmacol 114:1069-1075[ISI][Medline].
Minami T, Nishihara I, Uda R, Ito S, Hyodo M, Hayaishi O (1994a) Characterization of EP-receptor subtypes involved in allodynia and hyperalgesia induced by intrathecal administration of prostaglandin E2 to mice. Br J Pharmacol 112:735-740[ISI][Medline].
Minami T, Uda R, Horiguchi S, Ito S, Hyodo M, Hayashi O (1994b) Allodynia evoked by intrathecal administration of prostaglandin E2 to conscious mice. Pain 57:217-223[ISI][Medline].
Minami T, Okuda-Ashitaka E, Mori H, Ito S, Hayaishi O (1996) Prostaglandin D2 inhibits prostaglandin E2-induced allodynia in conscious mice. J Pharmacol Exp Ther 278:1146-1152[Abstract/Free Full Text].
Minami T, Okuda-Ashitaka E, Hori Y, Sakuma S, Sugimoto T, Sakimura K, Mishina M, Ito S (1999) Involvement of primary afferent C-fibres in touch-evoked pain (allodynia) induced by prostaglandin E2. Eur J Neurosci 11:1849-1856[ISI][Medline].
Muth-Selbach US, Tegeder I, Brune K, Geisslinger G (1999) Acetaminophen inhibits spinal prostaglandin E2 release after peripheral noxious stimulation. Anesthesiology 91:231-239[ISI][Medline].
Neugebauer V, Schaible H-G (1990) Evidence for a central component in the sensitization of spinal neurons with joint input during development of acute arthritis in cat's knee. J Neurophysiol 64:299-311[Abstract/Free Full Text].
Neugebauer V, Lücke T, Schaible H-G (1993) N-methyl-D-aspartate (NMDA) and non-NMDA receptor antagonists block the hyperexcitability of dorsal horn neurons during development of acute arthritis in rat's knee joint. J Neurophysiol 70:1365-1377[Abstract/Free Full Text].
Nicol GD, Klingberg DK, Vasko MR (1992) Prostaglandin E2 increases calcium conductance and stimulates release of substance P in avian sensory neurons. J Neurosci 12:1917-1927[Abstract].
Nishihara I, Minami T, Uda R, Ito S, Hyodo M, Hayaishi O (1995) Effect of NMDA receptor antagonists on prostaglandin E2-induced hyperalgesia in conscious mice. Brain Res 677:138-144[ISI][Medline].
Oida H, Namba T, Sugimoto Y, Ushikubi F, Ohishi H, Ichikawa A, Narumiya S (1995) In situ hybridization studies of prostacyclin receptor mRNA expression in various mouse organs. Br J Pharmacol 116:2828-2837[ISI][Medline].
Ramwell PW, Shaw JE, Jessup R (1966) Spontaneous and evoked release of prostaglandins from frog spinal cord. Am J Physiol 211:998-1004[Free Full Text].
Samad TA, Moore KA, Sapirstein A, Billet S, Allchorne A, Poole S, Bonventre JV, Woolf CJ (2001) Interleukin-1 $beta$ -mediated induction of Cox-2 in the CNS contributes to inflammatory pain hypersensitivity. Nature 410:471-475[Medline].
Sorkin LS (1993) IT ketorolac blocks NMDA-evoked spinal release of prostaglandin E2 (PGE2) and thromboxane B2 (TBXB2). Anesthesiology 79:A908.
Southall MD, Michael RL, Vasko MR (1998) Intrathecal NSAIDS attenuate inflammation-induced neuropeptide release from rat spinal cord slices. Pain 78:39-48[Medline].
Sugimoto Y, Shigemoto R, Namba T, Negishi M, Mizuno N, Narumiya S, Ichikawa A (1994) Distribution of the messenger RNA for the prostaglandin E receptor subtype EP3 in the mouse nervous system. Neuroscience 62:919-928[ISI][Medline].
Taiwo YO, Levine JD (1988) Prostaglandins inhibit endogenous pain control mechanisms by blocking transmission at spinal noradrenergic synapses. J Neurosci 8:1346-1349[Abstract].
Uda R, Horiguchi S, Ito S, Hyodo M, Hayaishi O (1990) Nociceptive effects induced by intrathecal administration of prostaglandin D2, E2, or F2alpha to conscious mice. Brain Res 510:26-32[ISI][Medline].
Vanegas H, Schaible H-G (2001) Prostaglandins and cyclooxygenases in the spinal cord. Prog Neurobiol 64:327-363[ISI][Medline].
Vanegas H, Tortorici V, Eblen-Zajjur A, Vasquez E (1997) PAG-microinjected dipyrone (metamizol) inhibits responses of spinal dorsal horn neurons to natural noxious stimulation in rats. Brain Res 759:171-174[Medline].
Vasko MR, Zirkelbach SL, Waite KJ (1993) Prostaglandins stimulate the release of substance P from rat spinal cord slices. Prog Pharmacol Clin Pharmacol 10:69-89.
Vasko MR, Campbell WB, Waite KJ (1994) Prostaglandin E2 enhances bradykinin-stimulated release of neuropeptides from rat sensory neurons in culture. J Neurosci 14:4987-4997[Abstract].
Vasquez E, Bär K-J, Ebersberger A, Klein B, Vanegas H, Schaible H-G (2000) Influence of PGE₂ on spinal nociceptive processing in rats with normal and inflamed knee joints. Soc Neurosci Abstr 26:732.6.
Vasquez E, Bär K-J, Ebersberger A, Vanegas H, Schaible H-G (2001) Spinal prostaglandin E₂ modifies the mechanosensitivity of spinal cord neurons and the development of inflammation-evoked hyperexcitability. Pflügers Arch 441:R156.
Willingale HL, Gardiner NJ, McLymont N, Giblett S, Grubb BD (1997) Prostanoids synthesized by cyclooxygenase isoforms in rat spinal cord and their contribution to the development of neuronal hyperexcitability. Br J Pharmacol 122:1593-1604[ISI][Medline].
Woolf CJ (1983) Evidence for a central component of post injury pain hypersensitivity. Nature 306:686-688[Medline].
Woolf CJ, Thompson SWN (1991) The induction and maintenance of central sensitization is dependent on N-methyl-D-aspartic acid receptor activation; implications for the treatment of post-injury pain hypersensitivity states. Pain 44:293-299[ISI][Medline].
Yang LC, Marsala M, Yaksh TL (1996a) Characterization of time course of spinal aminoacids, citrulline and PGE₂ release after carrageenan/kaolin-induced knee joint inflammation: a chronic microdialysis study. Pain 67:345-354[ISI][Medline].
Yang LC, Marsala M, Yaksh TL (1996b) Effect of spinal kainic acid receptor activation on spinal amino acid and prostaglandin E2 release in rat. Neuroscience 75:453-461[Medline].

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