ERK MAP Kinase Activation in Superficial Spinal Cord Neurons Induces Prodynorphin and NK-1 Upregulation and Contributes to Persistent Inflammatory Pain Hypersensitivity

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (140)

Citing Articles via Google Scholar

Google Scholar

Articles by Ji, R.-R.

Articles by Woolf, C. J.

Search for Related Content

PubMed

PubMed Citation

Articles by Ji, R.-R.

Articles by Woolf, C. J.

Previous Article  |  Next Article

The Journal of Neuroscience, January 15, 2002, 22(2):478-485

ERK MAP Kinase Activation in Superficial Spinal Cord Neurons Induces Prodynorphin and NK-1 Upregulation and Contributes to Persistent Inflammatory Pain Hypersensitivity
Ru-Rong Ji, Katia Befort, Gary J. Brenner, and Clifford J. Woolf
Neural Plasticity Research Group, Department of Anesthesia and Critical Care, Massachusetts General Hospital and Harvard Medical School, Boston, Massachusetts 02129

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activation of ERK (extracellular signal-regulated kinase) MAP (mitogen-activated protein) kinase in dorsal horn neurons ofthe spinal cord by peripheral noxious stimulation contributesto short-term pain hypersensitivity. We investigated ERK activationby peripheral inflammation and its involvement in regulating geneexpression in the spinal cord and in contributing to inflammatorypain hypersensitivity. Injection of complete Freund's adjuvant(CFA) into a hindpaw produced a persistent inflammation and asustained ERK activation in neurons in the superficial layers(laminae I-IIo) of the dorsal horn. CFA also induced an upregulationof prodynorphin and neurokinin-1 (NK-1) in dorsal horn neurons,which was suppressed by intrathecal delivery of the MEK (MAP kinasekinase) inhibitor U0126. CFA-induced phospho-ERK primarily colocalizedwith prodynorphin and NK-1 in superficial dorsal horn neurons.Although intrathecal injection of U0126 did not affect basal painsensitivity, it did attenuate both the establishment and maintenanceof persistent inflammatory heat and mechanical hypersensitivity.Activation of the ERK pathway in a subset of nociceptive spinalneurons contributes, therefore, to persistent pain hypersensitivity,possibly via transcriptional regulation of genes, such as prodynorphinand NK-1.

Key words: ERK; MAP kinase; prodynorphin; neurokinin-1; spinal cord; inflammatory pain

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Input to the spinal cord dorsal horn from high-threshold nociceptors induces central sensitization, a heterosynaptic facilitationthat outlives the initiating stimulus for tens of minutes andthat plays a major role in the generation of immediate postinjurypain hypersensitivity (Woolf, 1983). The increased neuronal excitabilityappears to result from post-translational regulation, such asphosphorylation, of key membrane receptors and channels (Woolfand Salter, 2000; Ji and Woolf, 2001).

Recently, we showed that ERK (extracellular signal-regulated kinase), a member of the MAPK (mitogen-activated protein kinase)family, is activated with a short latency (<1 min) in superficialdorsal horn neurons by noxious but not by innocuous stimuli. Thisactivation contributes to short-term (<1 hr) pain hypersensitivity(Ji et al., 1999). Because the involvement of ERK activation ingenerating acute pain hypersensitivity can be detected well beforeany transcriptional change manifests, ERK activation in the spinalcord, as in the hippocampus (English and Sweatt, 1997; Impey etal., 1998, 1999; Winder et al., 1999), is likely to contributeto short-term changes in neuronal excitability by post-translationalregulation.

Activated ERK is also, however, translocated to the nucleus in which it phosphorylates the transcription factor cAMP element-bindingprotein (CREB), via the CREB kinase Rsk2, subsequently activatingcAMP response element (CRE)-mediated gene expression (Xing etal., 1996; Impey et al., 1998; Obrietan et al., 1999). ERK activationis required for long-term potentiation and long-term memory (Englishand Sweatt, 1997; Atkins et al., 1998; Impey et al., 1998, 1999).However, apart from immediate early genes such as c-fos, the specifictarget genes regulated by ERK responsible for long-lasting synapticplasticity are primarily unknown (Xia et al., 1996; Sgambato etal., 1998).

Injection of irritant chemicals into a hindpaw of the rat produces a localized tissue inflammation and inflammatory pain hypersensitivity(Stein et al., 1988; Dubner and Ruda, 1992). Peripheral inflammationresults in the transcriptional activation of many genes in dorsalhorn neurons (Hunt et al., 1987; Wisden et al., 1990; Dubner andRuda, 1992; Ji et al., 1994, 1995; Mannion et al., 1999; Woolfand Costigan, 1999, Samad et al., 2001), among which, prodynorphinand the substance P receptor neurokinin-1 (NK-1) have been intensivelystudied (Iadarola et al., 1988; Ruda et al., 1988; Schafer etal., 1993; McCarsson and Krause, 1994; Abbadie et al., 1996).Increased prodynorphin expression after inflammation has beensuggested to be involved in the inflammation-induced enhancedexcitability and subsequent development of expanded dorsal hornneuronal receptive fields (Hylden et al., 1991; Dubner and Ruda,1992). Several lines of evidence suggest that NK-1 in the dorsalhorn also plays an important role in inflammatory pain hypersensitivity(Traub, 1996; De Felipe et al., 1998; Ma et al., 1998; Woolf etal., 1998).

Noxious stimulation and inflammation induce CREB phosphorylation in dorsal horn neurons (Ji and Rupp, 1997; Messersmith etal., 1998), as well as ERK activation (Ji et al., 1999). CRE sitesare present, moreover, in the promoter regions of both the prodynorphinand NK-1 genes (Hershey et al., 1991; Cole et al., 1995). Thisraises the possibility that the ERK pathway may play a role inregulating expression of CRE-containing genes, such as prodynorphinand NK-1, in the dorsal horn after inflammation and in this waycontribute to altered pain sensitivity. We now investigatedthis.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals and drugs. Adult male Sprague Dawley rats (230-300 gm) were used according to Massachusetts General Hospital AnimalCare institutional guidelines. Animals were anesthetized withpentobarbital (50 mg/kg, i.p.). Complete Freund's adjuvant (CFA)(100 µl) was injected into the plantar surface of a hindpaw. Forintrathecal drug delivery, a polyethylene-10 catheter was implantedinto the intrathecal space of the spinal cord at the lumbar enlargement,and 10 µl of the MEK (MAP kinase kinase) inhibitor U0126 (1 µg;dissolved in 10% DMSO; Calbiochem, La Jolla, CA) was administered.DMSO (10%) was injected as vehicle control. For sustained drugdelivery, an Alzet osmotic pump (3 d pump, 1 µl/hr) was filledwith the MEK inhibitor U0126 (0.5 µg/ml) in 50% DMSO, and thecatheter of the pump was implanted intrathecally at least 3 hrbefore CFA injection. DMSO (50%) was used as vehiclecontrol.

Immunohistochemistry. Rats were deeply anesthetized with pentobarbital (120 mg/kg, i.p.) and perfused through the ascendingaorta with saline, followed by 4% paraformaldehyde with 1.5% picricacid. L4-L5 spinal cord segments were dissected and post-fixedfor 2-4 hr. Transverse spinal cord sections (free floating, 30µm) were cut and processed for immunohistochemistry using theABC method as described previously (Ji et al., 1995, 1999). Briefly,sections were blocked with 2% goat serum in 0.3% Triton X-100for 1 hr at room temperature (RT) and incubated overnight at 4°Cwith primary antibody. The sections were then incubated for 2hr with biotinylated secondary antibody (1:200) and 1 hr withABC complex (1:50; Vector Laboratories, Burlingame, CA) at RT.Finally, the reaction product was visualized with 0.05% DAB-0.002%hydrogen peroxide in 0.1 M acetate buffer, pH 6.0, containing2% ammonium nickel sulfate for 2-5 min. Some sections were processedwith immunofluorescence by incubating overnight with primary antibodyand 1 hr at RT with FITC-conjugated secondary antibody (1:300;Jackson ImmunoResearch, West Grove, PA). The following antibodieswere used: anti-phospho-ERK (pERK) (also called anti-pMAPK; anti-rabbit,1:500; New England Biolabs, Beverly, MA), anti-pERK (monoclonal;1:300; New England Biolabs), anti-NK1 (anti-rabbit; 1:3000; Oncogene,Sciences, Uniondale, NY), and anti-prodynorphin (anti-guinea pig;1:3000; kindly provided by Dr. R. Elde, University of Minnesota,Minneapolis, MN). Double immunofluorescence was performed by incubatinga mixture of primary antibodies (mouse anti-pERK-rabbit anti-NK1or rabbit anti-pERK-guinea pig anti-prodynorphin), followed bya mixture of corresponding secondary antibodies conjugated witheither Cy3 orFITC.

In situ hybridization. Animals were rapidly sacrificed in a CO₂ chamber, and L4-L5 spinal cord segments were removed and cuton a cryostat at a thickness of 20 µm. A vector (pSP65) with a1.7 kb prodynorphin insert was kindly provided by Dr. Linda Kobierski(Harvard Medical School). Antisense RNA probe, and the correspondingsense control probe, were labeled by in vitro transcription usinglinearized DNA templates for prodynorphin and digoxigenin (DIG)labeling mixture for 2 hr at 37°C. Hybridization was processedas described previously (Ji et al., 1998). Tissue sections wereair dried for 2 hr, fixed in 4% paraformaldehyde for 15 min, andacetylated in acetic anhydride (0.25%) for 10 min. Sections wereprehybridized for 2 hr at RT and then incubated in hybridizationbuffer overnight at 60°C. After hybridization, sections were washedin decreasing concentrations of SSC (2×, 1×, and 0.2×) for 2 hrtotal. Sections were then blocked with 2% goat serum for 1 hrand incubated overnight at 4°C with alkaline phosphatase-conjugatedanti-DIG antibody (1:5000; Boehringer Mannheim, Indianapolis,IN). Finally, the sections were visualized in 75 µg/ml nitroblue-tetrazolium-chloride,50 µg/ml 5-bromo-4-chloro-3-indolyl-phosphate, and 0.24 mg/mllevamisole for 2-24hr.

RNase protection. Dynorphin cDNA was generated by reverse transcription-PCR from rat DRG total RNA, using primers 5'-TGGAAAAGCCCAGCTCCTAGACCCT-3'and 5'-TTCCTCGTGGGCTTGAAGTGTGAAA-3' and cloned into pCRII (Invitrogen,San Diego, CA). The plasmid was linearized with EcoRV, and anantisense probe was synthesized using Sp6 RNA polymerase and labeledwith [³²P]UTP (800 Ci/mmol; NEN, Boston, MA). RNase protection assays(RPAs) were performed using the RPA III (Ambion, Austin, TX) protocol,as reported previously (Samad et al., 2001). Briefly, 10 µg ofRNA samples were hybridized with labeled probe overnight at 42°Cand then digested with RNase A/RNase T1 mix in RNase digestionbuffer for 30 min at 37°C. Finally, samples were separated ondenaturing acrylamide gel and exposed to x-ray films. A $beta$ -actinprobe was used for each sample as loadingcontrols.

Western blot. Animals were sacrified, and dorsal horns of the L4-L5 spinal segments were rapidly removed and homogenized witha hand-held pellet pestle in lysis buffer containing a cocktailof phosphatase inhibitors (100×) and proteinase inhibitors (25×;Sigma, St. Louis, MO). For NK-1 protein, the dorsal horns weredirectly homogenized in boiling SDS sample buffer (100 mM Tris,pH6.8, 2% SDS, 20% glycerol, 10% $beta$ -mercaptoethanol, and 0.1% bromophenolblue). Protein samples were separated on SDS-PAGE gel (4-15% gradientgel; Bio-Rad, Hercules, CA) and transferred to polyvinylidenedifluoride filters (Millipore, Bedford, MA). The filters wereblocked with 3% milk and incubated overnight at 4°C with polyclonalanti-pERK (1:1000; New England Biolabs) or anti-NK-1 (1:5000;Oncogene Sciences) primary antibody. The blots were incubatedfor 1 hr at RT with HRP-conjugated secondary antibody (1:3000;Amersham Biosciences, Arlington Heights, IL) and visualized inECL solution (NEN, Boston, MA) for 1 min and exposed onto hyperfilms(Amersham Biosciences) for 1-30 min. The blots were then incubatedin stripping buffer (67.5 mM Tris, pH 6.8, 2% SDS, and 0.7% $beta$ -mercaptoethanol)for 30 min at 50°C and reprobed with polyclonal anti-ERK or anti-CREBantibody (1:3000; New England Biolabs) as loadingcontrols.

Behavioral analysis. Animals were habituated to the testing environment daily for 2 d before baseline testing. Except forthe heat test, all of the animals were placed on an elevated wiregrid. For mechanical allodynia, the plantar surface of the hindpawwas stimulated with a series of von Frey hairs. The thresholdwas taken as the lowest force that evokes a brisk withdrawal response.For heat hyperalgesia, the plantar surface of a hindpaw was exposedto a beam of radiant heat through a transparent Perspex surface(Hargrevas et al., 1988). The withdrawal latency was recorded,with a maximum 15 sec as cutoff. The withdrawal latency was averagedover threetrials.

Quantification and statistics. Eight nonadjacent sections from the L4-L5 lumbar spinal cord were randomly selected, and thenumbers of immunoreactive or mRNA-positive neuronal profiles inthe superficial laminae and/or deep laminae of the dorsal hornin each section were counted (under a 20× object field) by anobserver blind to the treatment. The values from the eight sectionswere averaged for each animal. The data are represented as mean± SEM. For RNase protection and Western blots, each experimentwas repeated at least twice, and, in all cases, the same resultswere obtained. The density of specific bands was measured witha computer-assisted imaging analysis system (IP Lab software)and normalized against a loading control. Differences betweengroups were compared using Student's t test or ANOVA, followedby Fisher's PLSD. For nonparametric data, Mann-Whitney U testwas applied. The criterion for statistical significance was p< 0.05.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

ERK activation by peripheral inflammation

To investigate whether ERK is activated by peripheral inflammation, we injected 100 µl of CFA into the plantar surface ofa hindpaw under pentobarbital anesthesia (50 mg/kg, i.p). Thisproduced an area of localized swelling, erythema, and hypersensitivityto mechanical and thermal stimuli, which persisted for the durationof the experiment (48 hr). The inflammation induced by the CFAinjection resulted in the induction of pERK in neurons in themedial superficial dorsal horn on the ipsilateral side of thelumbar enlargement (Fig. 1a,b). No induction was found in thecontralateral spinal cord (Fig. 1a). Intraplantar injection ofsaline (100 µl) only induced a very weak pERK induction (datanot shown). The CFA-induced pERK was found only in neurons; allpERK cells expressed neuronal-specific nuclear protein, a markerfor neuronal cells (data not shown). The pERK-labeled neuronswere predominantly localized in laminae I-IIo, and the pERK waspresent in the nucleus, cytoplasm, and dendrites, as reportedpreviously (Ji et al., 1999). The number of pERK neurons peakedat 10 min but remained elevated with a slow decline for 48 hr(Fig. 1c). This temporal pattern differs substantially from thetransient (<2 hr) ERK activation evoked by intraplantar capsaicin(Ji et al., 1999). ERK activation by CFA was confirmed by Westernblot analysis. The phosphorylation level of both ERK1 (44 kDa)and ERK2 (42 kDa) increased in the ipsilateral dorsal horn comparedwith the contralateral side at 30 min and 6 hr (Fig. 1d). BecauseERK is only activated in a small subset of dorsal horn neurons,Western blot is less sensitive than immunohistochemistry in detectingERK activation in the superficial dorsal horn.

View larger version (41K):
[in this window]
[in a new window]
Figure 1. CFA induces a sustained activation of ERK. a, A low-magnification image showing induction of ERK phosphorylation in laminae I-IIo neurons of the ipsilateral spinal cord (indicated with an arrowhead) 10 min after CFA injection into a hindpaw. Scale bar, 200 µm. b, A high-magnification image of a, showing ERK activation in the medial superficial dorsal horn of the ipsilateral spinal cord 10 min after CFA injection. Scale bar, 50 µm. c, Time course of pERK induction after CFA administration measured by the number of pERK-positive neurons in the superficial (I-IIo) layers of the ipsilateral dorsal horn. Data are represented as mean ± SEM (n = 3). d, Western blot showing increased ERK phosphorylation of both ERK1 (44 kDa) and ERK2 (42 kDa) in the ipsilateral (I) dorsal horn compared with contralateral (C) side, 30 min and 6 hr after CFA injection. The bottom panel indicates levels of total ERK1 and ERK2, as loading controls. Fold represents comparative levels over the corresponding contralateral side after normalizing for loading.

Because pERK reached a peak level very rapidly (10 min) after the CFA injection, we tested whether the CFA also produced hyperalgesiaat this time. CFA (100 µl) injected into the plantar surface ofhindpaw in awake rats produced both immediate erythema and a rapidheat hyperalgesia. The paw-withdrawal latency (in seconds) decreasedby 60% (from 10.8 ± 0.4 to 4.3 ± 0.7; p < 0.01; t test; n = 3)and 50% (from 9.7 ± 1.2 to 4.9 ± 1.3; p < 0.05) at 10 and 30 min,respectively. Saline-injected rats did not show any heathypersensitivity.

Prodynorphin induction by inflammation

To investigate changes in the expression of prodynorphin in response to inflammation, we used RPA, in situ hybridization,and immunohistochemistry. The peripheral inflammation resultedin a substantial upregulation of prodynorphin mRNA in the ipsilateralspinal dorsal horn 24 and 48 hr after CFA injection, as detectedby the RPA (Fig. 2a). With the in situ hybridization, many stronglylabeled prodynorphin mRNA-labeled neurons were found both in thesuperficial and deep layers of the ipsilateral dorsal horn 24hr after CFA injection, whereas on the contralateral side, onlya few weakly labeled neurons were detected (Fig. 2b). An increasein the number of prodynorphin peptide immunoreactive neurons wasalso found in the superficial and deep dorsal horn 48 hr afterthe CFA-induced inflammation (Fig. 2c).

View larger version (54K):
[in this window]
[in a new window]
Figure 2. CFA induces prodynorphin upregulation in the dorsal horn. a, An RNase protection assay reveals an increase in prodynorphin mRNA in the ipsilateral dorsal horn 24 and 48 hr after CFA injection. Fold represents comparative levels over control after normalizing for loading. b, In situ hybridization indicates an increased expression of prodynorphin mRNA in ipsilateral superficial and deep dorsal horn neurons 24 hr after CFA. Scale bar, 50 µm. c, Increased number of prodynorphin-immunoreactive neurons was induced in the ipsilateral superficial and deep dorsal horn by CFA injection at 48 hr. Scale bar, 50 µm.

ERK activation and prodynorphin expression

We then investigated whether prodynorphin mRNA expression in the dorsal horn is regulated by ERK activation. A specific andpotent MEK inhibitor, U0126 (Favata et al., 1998), was intrathecallyinjected twice (1 µg), 30 min before and 6 hr after intraplantarCFA injection. This reduced the CFA-induced prodynorphin mRNAincrease in the ipsilateral dorsal horn, as detected by the RPA(Fig. 3a). The CFA-evoked increase in the number of prodynorphinmRNA-positive neurons in the superficial dorsal horn was alsodecreased by U0126 (2× 1 µg) without any effect on the numberof labeled neurons in the deep laminae, as detected by in situhybridization (Fig. 3b,c).

View larger version (102K):
[in this window]
[in a new window]
Figure 3. ERK activation regulates prodynorphin expression. a, Partial suppression of the CFA-induced increase in prodynorphin mRNA in the dorsal horn at 24 hr by U0126 (1 µg, intrathecally injected 30 min before and 6 hr after CFA). Fold represents comparative levels over control after normalizing for loading. b, Quantification of prodynorphin mRNA-positive neurons in laminae I-II and III-VI of the ipsilateral dorsal horn 24 hr after CFA injection. *p < 0.001, compared with control; +p < 0.001, compared with CFA (n = 4). c, In situ hybridization showing an inhibition of the CFA-induced increase in prodynorphin mRNA-labeled neurons in the superficial dorsal horn by U0126 24 hr after CFA injection. Scale bar, 50 µm.

ERK activation and NK-1 expression

In agreement with previous studies (Abbadie et al., 1996, 1997), we observed increased NK-1 immunoreactivity in the superficialdorsal horn after CFA-induced inflammation using both immunohistochemistryand Western blot analysis (Fig. 4a,c). However, in contrast tothe previous studies (Abbadie et al., 1997; Honore et al., 1999),we found more NK-1-expressing cells after inflammation comparedwith our control (Fig. 4a,b). This discrepancy is attributableto the different detection thresholds for NK-1-positive neurons;our quantification, based on standard DAB staining, did not includeweakly stained cells in control animals. These cells would bedetected with confocal microscopy (Abbadie et al., 1997; Honoreet al., 1999). The increase in NK-1-immunoreactive neurons wedetected in lamina I (Fig. 4a) reflects the increase in stainingintensity seen by others (Abbadie et al., 1997; Honore et al.,1999) in this lamina. To explore whether ERK activation is involvedin the NK-1 upregulation, the MEK inhibitor U0126 was deliveredintrathecally before the induction of inflammation via an osmoticpump (0.5 µg · µl¹ · hr¹ for 2 d). MEK inhibition suppressed the CFA-induced elevationof NK-1-immunoreactive neurons in the superficial dorsal horn(Fig. 4a,b). A Western blot analysis confirmed this (Fig. 4c).The NK-1 antibody recognized a single band of ~46 kDa, which correspondsto the predicted molecular weight of cloned NK-1 receptor (Hersheyand Krause, 1990).

View larger version (65K):
[in this window]
[in a new window]
Figure 4. ERK activation regulates NK-1 expression. a, Suppression of the CFA-induced increase in NK-1 immunoreactivity in the medial superficial dorsal horn at 48 hr by U0126 delivered via an osmotic pump. Scale bar, 50 µm. b, Quantification of the numbers of NK-1 neurons in laminae I-IIo of the ipsilateral dorsal horn 48 hr after CFA injection. *p < 0.001, compared with control; +p < 0.001, compared with CFA (n = 5). c, Western blot indicates that the CFA-induced NK-1 increase in the dorsal horn at 24 hr is inhibited by U0126 (1 µg, intrathecally injected 30 min before and 6 hr after CFA injection). CREB, a constitutively expressed protein, was used as a loading control. Fold represents comparative levels over control after normalizing for loading.

To test whether the pERK-positive neurons and prodynorphin $---$ NK-1-expressing neurons belong to same subset of dorsal horn cells,we performed double immunofluorescence for pERK-prodynorphin andfor pERK-NK-1. Almost all prodynorphin- and NK-1-positive neuronsin the superficial dorsal horn also express pERK 24 hr after CFAinjection (Fig. 5).

View larger version (72K):
[in this window]
[in a new window]
Figure 5. ERK is activated in a subset of prodynorphin- and NK-1-expressing neurons. pERK (red) is primarily colocalized with prodynorphin (green; left) and NK-1 (green; right) in the medial superficial dorsal horn 24 hr after CFA injection. Arrows indicate double-labeled neurons. Scale bar, 20 µm.

ERK activation and persistent inflammatory pain

To examine the functional consequences of ERK activation and its downstream effects on prodynorphin and NK-1 upregulation,we tested whether inhibition of ERK activation modified inflammatorypain hypersensitivity. Intrathecal administration of U0126 (1µg) into non-inflamed animals, like another MEK inhibitor PD 98059(Ji et al., 1999), produced no significant change in basal painsensitivity measured in terms of mechanical withdrawal threshold(108% of the vehicle control) and heat withdrawal latency (113%of vehicle control), when tested 30 min after the administration.However, intrathecal administration of U0126 via an osmotic pump(0.5 µg · µl¹ · hr¹), started before the CFA injection and maintained for 48 hr,significantly reduced the inflammation-induced heat and mechanicalhypersensitivity measured at 24 and 48 hr (Fig. 6a,b).

View larger version (21K):
[in this window]
[in a new window]
Figure 6. Sustained infusion of an MEK inhibitor reduces CFA-induced inflammatory pain. The MEK inhibitor U0126 delivered by osmotic pump (0.5 µg · µl¹ · hr¹) before CFA injection reduces thermal hyperalgesia (a) and mechanical allodynia (b) 24 and 48 hr after CFA injection. These were measured by paw-withdrawal latency and paw-withdrawal threshold, respectively, and expressed as percentage of pre-CFA baseline measurements of vehicle control (50% DMSO). *p < 0.01, compared with corresponding vehicle control (n = 8).

Acute pain hypersensitivity (10-60 min after an intraplantar formalin injection) is reduced by inhibition of ERK activation,presumably by preventing post-translational changes (Ji et al.,1999). ERK activation by CFA could conceivably contribute to inflammatorypain hypersensitivity by either maintaining ongoing post-translationalchanges or inducing transcription of genes, such as prodynorphinand NK-1. In the former case, blocking ERK activation in establishedinflammation would be expected to reduce the pain hypersensitivitywithin tens of minutes as the substrates were dephosphorylated.If the contribution of ERK activation were through transcription,however, inhibiting ERK activation would be expected to have noimmediate effect but rather a delayed effect. To test this, weintrathecally injected U0126 (1 µg) in rats with established inflammation(24 hr after CFA injection) and tested pain hypersensitivity 30min, 6 hr, and 24 hr after the U0126 injection. Neither heat hyperalgesianor mechanical allodynia was significantly affected by such post-treatmentwhen tested at 30 min (Fig. 7a,b). However, the post-treatmentdecreased heat hyperalgesia at 24 hr and mechanical allodyniaat 6 hr (Fig. 7a,b), indicating a long-latency contribution ofERK activation to the maintenance of persistent inflammatory pain.

View larger version (19K):
[in this window]
[in a new window]
Figure 7. Post-treatment with an MEK inhibitor has a delayed effect on inflammatory pain. U0126 (1 µg) or vehicle (10% DMSO) was intrathecally administered 24 hr after CFA injection. Heat hyperalgesia (a) and mechanical allodynia (b) were tested 30 min, 6 hr, and 24 hr after the administration of the U0126. *p < 0.05, compared with corresponding vehicle control (n = 10). The data are expressed as percentage of pre-CFA baseline measurements of vehicle control.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

ERK activation in nociceptive dorsal horn neurons

Peripheral inflammation induced, after a short latency, a persistent activation of ERK in laminae I-IIo neurons of the ipsilateralsuperficial dorsal horn. Inhibition of this activation, usingan MEK inhibitor, blocked elevation of prodynorphin and NK-1 expressionin this particular subset of dorsal horn neurons, as well as reducedinflammatory pain hypersensitivity. pERK was induced by CFA inthe same subset of dorsal horn neurons that express prodynorphinand NK-1. Many NK-1- and dynorphin-expressing neurons in laminaI are projection neurons (Nahin et al., 1989; Marshall et al.,1996). Projection neurons in lamina I exhibit an enlargement oftheir receptive fields after CFA-induced inflammation (Dubnerand Ruda, 1992). A targeted loss of NK-1-expressing neurons inlamina I has been shown to abolish inflammatory pain (Nicholset al., 1999). These studies indicate a critical role for theaforementioned superficial neurons in the reaction of the CNSto inflammation. A particular subset of C-nociceptor fibers, thosethat are NGF-responsive, and TrkA- and neuropeptide-expressing,terminate in laminae I and IIo, in an area overlapping the neuronsthat show ERK activation. Another subset of C-fibers, those thatrespond to the glial cell line-derived neurotrophic factor familyof growth factors and are characterized by selective binding ofthe IB4 lectin, terminate in lamina IIi (Averill et al., 1995;Molliver et al., 1997). The neurons these fibers contact, manyof which contain PKC $gamma$ (Malmberg et al., 1997), do not show ERKactivation after capsaicin or CFA injection (R.-R. Ji et al.,unpublished observations). The role of ERK in regulating painhypersensitivity is, therefore, restricted to a particular subsetof nociceptive dorsal horn neurons, only those located in laminaeI-IIo, and this activation is likely to reflect activation onlyof TrkA-expressing C-fibers.

Transcriptional regulation in response to ERK activation

pERK was found in the nucleus of neurons after CFA injection (Fig. 1a), pointing to a possible transcriptional role for theactivated kinase. Unlike the transient activation (lasting <2hr) induced after capsaicin injection (Ji et al., 1999), CFA producedpersistent ERK activation (Fig. 1c). The sustained ERK activationafter CFA injection is associated with persistent upregulationof prodynorphin mRNA (lasting >48 hr) (Fig. 2a), whereas the transientpERK induced by capsaicin is associated with a shorter-lastingupregulation of prodynorphin mRNA (<6 hr; R.-R. Ji and C. J. Woolf,unpublished observation). ERK activation is likely to regulatethe expression of prodynorphin and NK-1, both of which are CRE-containinggenes, via CREB phosphorylation. CREB is required for dopamine-inducedexpression of prodynorphin in striatal neurons (Cole et al., 1995)and is phosphorylated in NK-1 receptor-expressing neurons afternoxious stimulation (Anderson and Seybold, 2000). Interestingly,a CRE site has been shown to mediate a long-term sensitizationof nociceptive neurons in Aplysia (Lewin and Walters, 1999).

ERK activation and inflammatory pain hypersensitivity

U0126 is a potent and selective MEK inhibitor (Favata et al., 1998), achieving inhibition of ERK activation even in the faceof strong activators, such as phorbol esters, whereas other majorsignal transduction pathways are not affected (Roberson et al.,1999). This inhibitor has not only been used in in vitro studies(Roberson et al., 1999) but also in in vivo studies (Han and Holtzman,2000; Kuroki et al., 2001). At the dose we used, we did not findobvious toxicity of this inhibitor, animals behaved normally,and locomotion was unaffected. Although basal pain sensitivitywas not affected by the inhibitor, persistent inflammatory painwas reduced. This could conceivably result from either preventingsome post-translational change mediated by the ERK signal transductionpathway, as for acute pain hypersensitivity (Ji et al., 1999),or a reduction in transcription of target genes, such as prodynorphinand NK-1. The involvement suggested by a number of different studies,of both the NK-1 receptor and prodynorphin in pain mechanisms,together with their regulation by ERK activation, is compatiblewith a hypothesis that ERK activation after inflammation contributesto pain hypersensitivity by regulating gene transcription. Thetemporal profile of the effect of blocking ERK activation representsadditional support. The acute pain hypersensitivity establishedwithin minutes of intraplantar formalin can be reduced by preventingERK activation (Ji et al., 1999), an effect that is too quick(<1 hr) to be mediated by an inhibition of transcription and islikely therefore to represent some post-translational change downstreamof the activated ERK. At present, it is not clear what the substratefor such post-translational change is, but it may well be an ionchannel or receptor, such as the NMDA or AMPA receptor (Woolfand Salter, 2000). Such post-translational changes underlie theinduction and maintenance of central sensitization, a use-dependentplasticity that outlasts its initiating stimulus by tens of minutes(Woolf, 1983; Woolf and Wall, 1986). If inflammatory hypersensitivitywere a manifestation only of a central sensitization maintainedby ongoing afferent input from the inflamed tissue, then blockingthe initiation of central sensitization, by inhibiting an ERK-mediatedphosphorylation, should reduce the hypersensitivity over a periodsof tens of minutes as the key proteins were dephosphorylated.The fact that MEK inhibition during established inflammation hadno immediate effect, but rather only reduced mechanical and thermalhypersensitivity 6-24 hr later, argues that the role of ERK activationmay well be via transcriptionalregulation.

Dynorphin and NK-1 contribute to inflammatory pain hypersensitivity

A temporal correlation has been shown previously between the expression of prodynorphin and NK-1 and development of inflammatorypain hypersensitivity (Iadarola et al., 1988; Abbadie et al.,1996). Unlike other opioid peptides, intrathecal injection ofdynorphin does not produce analgesia (Laughlin et al., 1997).Dynorphin has actually been found to be pronociceptive in somepathological pain states. For example, dynorphin A antiserum reducesthe pain hypersensitivity after nerve injury (Nichols et al.,1997; Wegert et al., 1997; Malan et al., 2000), and neuropathicpain does not persist in prodynorphin knock-out mice (Wang etal., 2001). The pronociceptive action of dynorphin appears tobe the result of its nonopioid actions (Laughlin et al., 1997),including an activation of NMDA receptors sufficient to induceexcitotoxicity (Dubner and Ruda, 1992).

Inflammation induces NK-1 receptor upregulation in dorsal horn neurons and upregulation of its ligand, the neuropeptide substanceP, in primary afferent neurons (Noguchi et al., 1988; Abbadieet al., 1996) (also see Woolf et al., 1998). NK-1 antagonistshave been shown to reduce inflammatory pain (both hyperalgesiaand mechanical allodynia) in several different animal models (Neumannet al., 1996; Ren et al., 1996; Traub, 1996; Ma et al., 1998;Woolf et al., 1998; Trafton and Basbaum, 2000), including NK-1knock-out mice (De Felipe et al., 1998). The increased amountand internalization of the NK-1 receptor on the dendrites of dorsalhorn neurons in response to noxious and innocuous stimuli afterinflammation indicates that this receptor is activated by substanceP in response to peripheral stimuli (Abbadie et al., 1997).

Conclusion

ERK activation has two roles in nociceptive plasticity in the dorsal horn: a short-latency contribution to acute noxious stimulus-inducedcentral sensitization and an involvement in the induction andmaintenance of inflammatory pain. The involvement of pERK in peripheralinflammatory pain hypersensitivity may be contributed to by itsregulation of prodynorphin and NK-1 expression, as well as othertarget genes. ERK activation plays, therefore, a pivotal rolein the functional plasticity and chemical phenotype of a groupof neurons in the superficial dorsal horn, determining the activationof particular effector responses to divergent inputs, which inturn contribute to alteredsensibility.

  FOOTNOTES

Received June 22, 2001; revised Oct. 3, 2001; accepted Oct. 26, 2001.

The work was supported by National Institutes of Health Grants RO1 NS38253 (C.J.W.) and RO1 NS40698 (R.R.J.). We thank SaraBillet for technical support, Dr. Linda Kobierski (MassachusettsGeneral Hospital) for the prodynorphin cDNA vector, and Dr. RobertElde (University of Minnesota) for prodynorphinantibody.
Correspondence should be addressed to Dr. Ru-Rong Ji, Neural Plasticity Research Group, Department of Anesthesia and CriticalCare, Massachusetts General Hospital, Harvard Medical School,149 13th Street, Room 4309, Charlestown, MA 02129. E-mail: ji{at}helix.mgh.harvard.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Abbadie C, Brown JL, Mantyh PW, Basbaum AI (1996) Spinal cord substance P receptor immunoreactivity increases in both inflammatory and nerve injury models of persistent pain. Neuroscience 70:201-209[ISI][Medline].
Abbadie C, Trafton J, Liu H, Mantyh PW, Basbaum AI (1997) Inflammation increases the distribution of dorsal horn neurons that internalize the neurokinin-1 receptor in response to noxious and non-noxious stimulation. J Neurosci 17:8049-8060[Abstract/Free Full Text].
Anderson LE, Seybold VS (2000) Phosphorylated cAMP response element binding protein increases in neurokinin-1 receptor-immunoreactive neurons in rat spinal cord in response to formalin-induced nociception. Neurosci Lett 283:29-32[Medline].
Atkins CM, Selcher JC, Petraitis JJ, Trzaskos JM, Sweatt JD (1998) The MAPK cascade is required for mammalian associative learning. Nat Neurosci 1:602-609[ISI][Medline].
Averill S, McMahon SB, Clary DO, Reichardt LF, Priestley JV (1995) Localization of trkA receptors in chemically identified subgroups of adult rat sensory neurones. Eur J Neurosci 7:1484-1494[ISI][Medline].
Cole RL, Konradi C, Douglass J, Hyman SE (1995) Neuronal adaptation to amphetamine and dopamine: molecular mechanisms of prodynorphin gene regulation in rat striatum. Neuron 14:813-823[ISI][Medline].
De Felipe C, Herrero JF, O'Brien JA, Palmer JA, Doyle CA, Smith AJ, Laird JM, Belmonte C, Cervero F, Hunt SP (1998) Altered nociception, analgesia and aggression in mice lacking the receptor for substance P. Nature 392:394-397[Medline].
Dubner R, Ruda MA (1992) Activity-dependent neuronal plasticity following tissue injury and inflammation. Trends Neurosci 15:96-103[ISI][Medline].
English JD, Sweatt JD (1997) A requirement for the mitogen-activated protein kinase cascade in hippocampal long term potentiation. J Biol Chem 272:19103-19106[Abstract/Free Full Text].
Favata M, Horiuchi KY, Manos EJ, Daulerio AJ, Stradley DA, Feeser WS, Van Dyk DE, Pitts WJ, Earl RA, Hobbs F, Copeland RA, Magolda RL, Scherle PA, Trzaskos JM (1998) Identification of a novel inhibitor of mitogen-activated protein kinase kinase. J Biol Chem 273:18623-18632[Abstract/Free Full Text].
Han BH, Holtzman DM (2000) BDNF protects the neonatal brain from hypoxic-ischemic injury in vivo via the ERK pathway. J Neurosci 20:5775-5781[Abstract/Free Full Text].
Hargrevas K, Dubner R, Brown F, Flores C, Joris J (1988) A new and sensitive method for measuring thermal nociception in cutaneous hyperalgesia. Pain 32:77-88[ISI][Medline].
Hershey AD, Krause JE (1990) Molecular characterization of a functional cDNA encoding the rat substance P receptor. Science 247:958-962[Abstract/Free Full Text].
Hershey AD, Dykema PE, Krause JE (1991) Organization, structure and expression of the gene encoding the rat substance P receptor. J Biol Chem 266:4366-4374[Abstract/Free Full Text].
Honore P, Menning PM, Rogers SD, Nichols ML, Basbaum AI, Besson JM, Mantyh PW (1999) Spinal substance P receptor expression and internalization in acute, short-term, and long-term inflammatory pain states. J Neurosci 19:7670-7678[Abstract/Free Full Text].
Hunt SP, Pini A, Evan G (1987) Induction of c-fos-like protein in spinal cord neurons following sensory stimulation. Nature 328:632-634[Medline].
Hylden JL, Nahin RL, Traub RJ, Dubner R (1991) Effects of spinal kappa-opioid receptor agonists on the responsiveness of nociceptive superficial dorsal horn neurons. Pain 44:187-193[ISI][Medline].
Iadarola MJ, Brady LS, Draisci G, Dubner R (1988) Enhancement of dynorphin gene expression in spinal cord following experimental inflammation: stimulus specificity, behavioral parameters and opioid receptor binding. Pain 35:313-326[ISI][Medline].
Impey S, Obrietan K, Wong ST, Poser S, Yano S, Wayman G, Deloulme JC, Chan G, Storm DR (1998) Cross talk between Erk and PKA is required for Ca²⁺ stimulation of CREB-dependent transcription and Erk nuclear translocation. Neuron 21:869-883[ISI][Medline].
Impey S, Obrietan K, Storm DR (1999) Making new connections: role of ERK/MAP kinase signaling in neuronal plasticity. Neuron 23:11-14[ISI][Medline].
Ji RR, Rupp F (1997) Phosphorylation of transcription factor CREB in rat spinal cord after formalin-induced hyperalgesia: relationship to c-fos induction. J Neurosci 17:1776-1785[Abstract/Free Full Text].
Ji RR, Woolf CJ (2001) Neruonal plasticity and signal transduction in nociceptive neurons: Implications for the initiation and maintenance of pathological pain. Neurobiol Dis 8:1-10[ISI][Medline].
Ji RR, Zhang X, Wiesenfeld-Hallin Z, Hokfelt T (1994) Expression of neuropeptide Y and neuropeptide Y (Y1) receptor mRNA in rat spinal cord and dorsal root ganglia following peripheral tissue inflammation. J Neurosci 14:6423-6434[Abstract].
Ji RR, Zhang X, Nilsson S, Wiesenfeld-Hallin Z, Hokfelt T (1995) Central and peripheral response to galanin induced by inflammation. Neuroscience 68:563-576[ISI][Medline].
Ji RR, Schlaepfer TE, Aizenman CD, Qiu D, Hung JC, Rupp F (1998) Repetitive transcranial magnetic stimulation activates specific neural regions. Proc Natl Acad Sci USA 95:15635-15640[Abstract/Free Full Text].
Ji RR, Baba H, Brenner G, Woolf CJ (1999) Nociceptive-specific activation of ERK in spinal neurons contributes to pain hypersensitivity. Nat Neurosci 2:1114-1119[ISI][Medline].
Kuroki Y, Fukushima K, Kanda Y, Mizuno K, Watanabe Y (2001) Neuroprotection by estrogen via extracellular signal-regulated kinase against quinolinic acid-induced cell death in the rat hippocampus. Eur J Neurosci 13:472-476[ISI][Medline].
Laughlin TM, Vanderah TW, Lashbrook J, Nichols ML, Ossipov M, Porreca F, Wilcox GL (1997) Spinally administered dynorphin A produces long-lasting allodynia: involvement of NMDA but not opioid receptors. Pain 72:253-260[ISI][Medline].
Lewin MR, Walters ET (1999) Cyclie GMP pathway is critical for inducing long-term sensitization of nociceptive sensory neurons. Nat Neurosci 2:18-23[ISI][Medline].
Ma QP, Allochorne AJ, Woolf CJ (1998) Morphine, the NMDA receptor antagonist MK801 and tachykinin NK1 receptor antagonist RP67580 attenuate the development of inflammation-induced progressive tactile hypersensitivity. Pain 77:49-57[ISI][Medline].
Malan TP, Ossipov MH, Gardell LR, Ibrahim M, Bian D, Lai J, Porreca F (2000) Extraterritorial neuropathic pain correlates with multisegmental elevation of spinal dynorphin in nerve-injured rats. Pain 86:185-194[ISI][Medline].
Malmberg AB, Chen C, Susumu T, Basbaum AI (1997) Preserved acute pain and reduced neuropathic pain in mice lacking PKC gamma. Science 278:279-283[Abstract/Free Full Text].
Mannion RJ, Costigan M, Decosterd I, Amaya F, Ma QP, Holstege JC, Ji RR, Acheson A, Lindsay RM, Wilkinson GA, Woolf CJ (1999) Brain-derived neurotrophic factor-a centrally acting modulator of tactile stimulus-induced inflammatory pain hypersensitivity. Proc Natl Acad Sci USA 96:9385-9390[Abstract/Free Full Text].
Marshall GE, Shehab SA, Spike RC, Todd AJ (1996) Neurokinin-1 receptors on lumbar spinothalamic neurons in the rat. Neuroscience 72:255-263[ISI][Medline].
McCarsson KE, Krause JE (1994) NK-1 and NK-3 type tachykinin receptor mRNA expression in the rat spinal cord dorsal horn is increased during adjuvant or formalin-induced nociception. J Neurosci 14:712-720[Abstract].
Messersmith DJ, Kim DJ, Iadarola MJ (1998) Transcription factor regulation of prodynorphin gene expression following rat hindpaw inflammation. Mol Brain Res 53:260-269[Medline].
Molliver DC, Wright DE, Leitner ML, Parsadanian AS, Doster K, Wen D, Yan Q, Snider WD (1997) IB4-binding DRG neurons switch from NGF to GDNF dependence in early postnatal life. Neuron 19:849-861[ISI][Medline].
Nahin RL, Hylden JL, Iadarola MJ, Dubner R (1989) Peripheral inflammation is associated with increased dynorphin immunoreactivity in both projection and local circuit neurons in the superficial dorsal horn of the rat lumbar spinal cord. Neurosci Lett 96:247-252[Medline].
Neumann S, Doubell TP, Leslie T, Woolf CJ (1996) Inflammatory pain hypersensitivity mediated by phenotypic switch in myelinated primary sensory neurons. Nature 384:360-364[Medline].
Nichols ML, Lopez Y, Ossipov MH, Bian D, Porreca F (1997) Enhancement of the antiallodynic and antinociceptive efficacy of spinal morphine by antisera to dynorphin A (1-13) or MK-801 in a nerve-ligation model of peripheral neuropathy. Pain 69:317-322[ISI][Medline].
Nichols ML, Allen BJ, Rogers SD, Ghilardi JR, Honore P, Luger NM, Finke MP, Li J, Lappi DA, Simone DA, Mantyh PW (1999) Transmission of chronic nociception by spinal neurons expressing the substance P receptor. Science 286:1558-1561[Abstract/Free Full Text].
Noguchi K, Morita Y, Kiyama H, Ono K, Tohyama MA (1988) Noxious stimulus induces the preprotachykinin-A gene expression in the rat dorsal root ganglion: a quantitative study using in situ hybridization histochemistry. Brain Res 464:31-35[Medline].
Obrietan K, Impey S, Smith D, Athos J, Storm DR (1999) Circadian regulation of cAMP response element-mediated gene expression in the suprachiasmatic nuclei. J Biol Chem 274:17748-17756[Abstract/Free Full Text].
Ren K, Iadarola MJ, Dubner R (1996) An isobolographic analysis of the effect of N-methyl-D-aspartate and NK1 tachykinin receptor antagonists on inflammatory hyperalgesia in the rat. Br J Pharmacol 117:196-202[ISI][Medline].
Roberson ED, English JD, Adams JP, Selcher JC, Kondratick C, Sweat JD (1999) The mitogen-activated protein kinase cascade couples PKA and PKC to cAMP response element binding protein phosphorylation in area CA1 of hippocampus. J Neurosci 19:4337-4348[Abstract/Free Full Text].
Ruda MA, Iadarola MJ, Cohen LV, Young WS (1988) In situ hybridization histochemistry and immunohistochemistry reveal an increase in spinal dynorphin biosynthesis in rat model of peripheral inflammation and hyperalgesia. Proc Natl Acad Sci USA 85:622-626[Abstract/Free Full Text].
Samad A, Moore KA, Sapirstein A, Billet S, Allchorne A, Poole S, Bonventre JV, Woolf CJ (2001) An interleukin-1b-mediated induction of Cox-2 in the central nervous system contributes to inflammatory pain hypersensitivity. Nature 22:471-475.
Schafer MK, Nohr D, Krause JE, Weihe E (1993) Inflammation-induced upregulation of NK1 receptor mRNA in dorsal horn neurons. NeuroReport 4:1007-1010[ISI][Medline].
Sgambato V, Pages C, Rogard M, Besson MJ, Caboche J (1998) Extracellular signal-regulated kinase (ERK) controls immediate early gene induction on corticostrital stimulation. J Neurosci 18:8814-8825[Abstract/Free Full Text].
Stein C, Millan MJ, Herz A (1988) Unilateral inflammation of the hindpaw in rats as a model of prolonged noxious stimulation: alterations in behavior and nociceptive thresholds. Pharmacol Biochem Behav 31:445-451.
Trafton JA, Basbaum AI (2000) The contribution of spinal cord neurokinin-1 receptor signaling to pain. J Pain Suppl 1:57-65.
Traub RJ (1996) The spinal contribution of substance P to the generation and maintenance of inflammatory hyperalgesia in the rat. Pain 67:151-161[ISI][Medline].
Wang Z, Gardell LR, Ossipov MH, Vanderah TW, Brennan MB, Hochgeschwender U, Hruby VJ, Malan Jr TP, Lai J, Porreca F (2001) Pronociceptive actions of dynorphin maintain chronic neuropathic pain. J Neurosci 21:1779-1786[Abstract/Free Full Text].
Wegert S, Ossipov MH, Nichols ML, Bian D, Vanderah TW, Malan TP, Porreca Jr F (1997) Differential activities of intrathecal MK-801 or morphine to alter responses to thermal and mechanical stimuli in normal or nerve-injured rats. Pain 71:57-64[ISI][Medline].
Winder DG, Martin KC, Muzzio IA, Rohrer D, Chruscinski A, Kobilka B, Kandel ER (1999) ERK plays a regulatory role in induction of LTP by theta frequency stimulation and its modulation by b-adrenergic receptors. Neuron 24:715-726[ISI][Medline].
Wisden W, Errington ML, Williams S, Dunnett SB, Waters C, Hitchcock D, Evan G, Bliss TVP, Hunt SP (1990) Differential expression of immediate early genes in the hippocampus and spinal cord. Neuron 4:603-614[ISI][Medline].
Woolf CJ (1983) Evidence for a central component of post-injury pain hypersensitivity. Nature 306:686-688[Medline].
Woolf CJ, Costigan M (1999) Transcriptional and post-translational plasticity and the generation of inflammatory pain. Proc Natl Acad Sci USA 96:7723-7730[Abstract/Free Full Text].
Woolf CJ, Salter MW (2000) Neuronal plasticity: increasing the gain in pain. Science 288:1765-1769[Abstract/Free Full Text].
Woolf CJ, Wall PD (1986) Relative effectiveness of C primary afferent fibers of different origins in evoking a prolonged facilitation of the flexor reflex in the rat. J Neurosci 6:1433-1442[Abstract].
Woolf CJ, Mannion RJ, Neumann S (1998) Null mutations lacking substance: elucidating pain mechanisms by genetic pharmacology. Neuron 20:1063-1066[ISI][Medline].
Xia Z, Dudek H, Miranti CK, Greenberg ME (1996) Calcium influx via the NMDA receptor induces immediate early gene transcription by a MAPK/ERK-dependent mechanism. J Neurosci 16:5425-5436[Abstract/Free Full Text].
Xing J, Ginty DD, Greenberg ME (1996) Coupling of the RAS-MAPK pathway to gene activation by RSK2, a growth factor-regulated CREB kinase. Science 273:959-963[Abstract].

Copyright © 2002 Society for Neuroscience 0270-6474/02/222478-08$05.00/0

This article has been cited by other articles:

H.-Y. Peng, H.-M. Chang, S. Y. Chang, K.-C. Tung, S.-D. Lee, D. Chou, C.-Y. Lai, C.-H. Chiu, G.-D. Chen, and T.-B. Lin
Orexin-A modulates glutamatergic NMDA-dependent spinal reflex potentiation via inhibition of NR2B subunit
Am J Physiol Endocrinol Metab, July 1, 2008; 295(1): E117 - E129.
[Abstract] [Full Text] [PDF]

Y. Kawasaki, L. Zhang, J.-K. Cheng, and R.-R. Ji
Cytokine Mechanisms of Central Sensitization: Distinct and Overlapping Role of Interleukin-1{beta}, Interleukin-6, and Tumor Necrosis Factor-{alpha} in Regulating Synaptic and Neuronal Activity in the Superficial Spinal Cord
J. Neurosci., May 14, 2008; 28(20): 5189 - 5194.
[Abstract] [Full Text] [PDF]

T. Kohno, H. Wang, F. Amaya, G. J. Brenner, J.-K. Cheng, R.-R. Ji, and C. J. Woolf
Bradykinin Enhances AMPA and NMDA Receptor Activity in Spinal Cord Dorsal Horn Neurons by Activating Multiple Kinases to Produce Pain Hypersensitivity
J. Neurosci., April 23, 2008; 28(17): 4533 - 4540.
[Abstract] [Full Text] [PDF]

S. Pezet, F. Marchand, R. D'Mello, J. Grist, A. K. Clark, M. Malcangio, A. H. Dickenson, R. J. Williams, and S. B. McMahon
Phosphatidylinositol 3-Kinase Is a Key Mediator of Central Sensitization in Painful Inflammatory Conditions
J. Neurosci., April 16, 2008; 28(16): 4261 - 4270.
[Abstract] [Full Text] [PDF]

G.-D. Chen, M.-L. Peng, P.-Y. Wang, S.-D. Lee, H.-M. Chang, S.-F. Pan, M.-J. Chen, K.-C. Tung, C.-Y. Lai, and T.-B. Lin
Calcium/calmodulin-dependent kinase II mediates NO-elicited PKG activation to participate in spinal reflex potentiation in anesthetized rats
Am J Physiol Regulatory Integrative Comp Physiol, February 1, 2008; 294(2): R487 - R493.
[Abstract] [Full Text] [PDF]

S. Biswal, D. L. Resnick, J. M. Hoffman, and S. S. Gambhir
Molecular Imaging: Integration of Molecular Imaging into the Musculoskeletal Imaging Practice
Radiology, September 1, 2007; 244(3): 651 - 671.
[Abstract] [Full Text] [PDF]

K. A. Corrow and M. A. Vizzard
Phosphorylation of extracellular signal-regulated kinases in urinary bladder in rats with cyclophosphamide-induced cystitis
Am J Physiol Regulatory Integrative Comp Physiol, July 1, 2007; 293(1): R125 - R134.
[Abstract] [Full Text] [PDF]