Functional Downregulation of P2X3 Receptor Subunit in Rat Sensory Neurons Reveals a Significant Role in Chronic Neuropathic and Inflammatory Pain

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The Journal of Neuroscience, September 15, 2002, 22(18):8139-8147

Functional Downregulation of P2X₃ Receptor Subunit in Rat Sensory Neurons Reveals a Significant Role in Chronic Neuropathic and Inflammatory Pain
Jane Barclay¹, Sadhana Patel¹, Gabriele Dorn², Glen Wotherspoon¹, Sarah Moffatt¹, Louise Eunson¹, Samir Abdel'al², Francois Natt², Jonathan Hall², Janet Winter¹, Stuart Bevan¹, William Wishart², Alyson Fox¹, and Pam Ganju¹
¹ Novartis Institute for Medical Sciences, London WC1E 6BS, United Kingdom, and ² Functional Genomics, Novartis Pharma AG, CH-4002 Basel, Switzerland

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The excitation of nociceptive sensory neurons by ATP released in injured tissue is believed to be mediated partly by P2X₃receptors. Although an analysis of P2X₃ knock-out mice has revealedsome deficits in nociceptive signaling, detailed analysis of therole of these receptors is hampered by the lack of potent specificpharmacological tools. Here we have used antisense oligonucleotides(ASOs) to downregulate P2X₃ receptors to examine their role inmodels of chronic pain in therat.
ASOs and control missense oligonucleotides (180 µg/d) were administered intrathecally to naive rats for up to 7 d via a lumbarindwelling cannula attached to an osmotic minipump. Functionaldownregulation of the receptors was confirmed by $alpha$ $beta$ -methyleneATP injection into the hindpaw, which evoked significantly lessmechanical hyperalgesia as early as 2 d after treatment with ASOsrelative to controls. At this time point, P2X₃ protein levelswere significantly downregulated in lumbar L4 and L5 dorsal rootganglia. After 7 d of ASO treatment, P2X₃ protein levels werereduced in the primary afferent terminals in the lumbar dorsalhorn of the spinalcord.
In models of neuropathic (partial sciatic ligation) and inflammatory (complete Freund's adjuvant) pain, inhibition of thedevelopment of mechanical hyperalgesia as well as significantreversal of established hyperalgesia were observed within 2 dof ASO treatment. The time course of the reversal of hyperalgesiais consistent with downregulation of P2X₃ receptor protein andfunction.
This study demonstrates the utility of ASO approaches for validating gene targets in in vivo pain models and provides evidencefor a role of P2X₃ receptors in the pathophysiology of chronicpain.

Key words: dorsal root ganglia; P2X₃; P2X_2/3; neuropathic pain; inflammatory pain; antisense oligonucleotide; $alpha$ , $beta$ -methylene ATP

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Since the first description of pain produced by the application of the purine ATP into a human blister base preparation (Bleehenand Keele, 1977), there has been accumulating evidence supportinga nociceptive role for extracellular ATP (Burnstock and Wood,1996; Dunn et al., 2001). ATP released by exocytosis or cell lysisafter tissue injury may activate primary sensory afferent neuronsvia ATP-gated cation channels, termed P2X. Of the seven P2X channelsubunits identified to date, P2X₃ subunit-containing receptors(either homomeric or heteromeric combination of P2X₃ and P2X₂receptors: P2X_2/3) are expressed predominantly in nociceptivesensory neurons (Chen et al., 1995; Lewis et al., 1995) and arethought to mediate ATP nociceptive signaling. P2X₃ receptor proteinis exported from the soma of dorsal root ganglia (DRG) neuronsto peripheral terminals in the skin and viscera (Bradbury et al.,1998) and to central terminals projecting into inner lamina IIof the dorsal horn of the spinal cord (Vulchanova et al., 1997,1998; Llewellyn-Smith and Burnstock, 1998). ATP has been shownto depolarize isolated DRG neurons (Bean et al., 1990) and excitethe peripheral terminals of primary afferent neurons (Dowd etal., 1998; Hamilton and McMahon, 2000; Rong et al., 2000). Inthe spinal cord, ATP may act at presynaptic P2X₃ receptors, facilitatingglutamate release from primary afferents (Gu and MacDermott, 1997;Khakh and Henderson, 1998; Tsuda et al., 1999), as well as atpostsynaptic receptors (including P2X₁, P2X₂, P2X₄, P2X₅, andP2X₆ receptors) located on second-order neurons (Fyffe and Perl,1984; Salter and Henry, 1985; Sawynok and Sweeney, 1989; Li andPerl, 1995; Bardoni et al., 1997; Stanfa et al., 2000).

Investigation of the role of P2X₃ subunit-containing receptor activation in vivo is hampered by the lack of selective antagonists.Subplantar application of the agonists ATP and $alpha$ , $beta$ -methylene ATPinto the naive rat hindpaw has been shown to elicit thermal hyperalgesiaand nocifensive behavior that can be inhibited by selective desensitizationwith $alpha$ , $beta$ -methylene ATP, implicating a role for a combination ofP2X₃, P2X_2/3, and P2X₁ receptors (Bland-Ward and Humphrey, 1997).

Evidence for a direct physiological role of P2X₃ homomeric and P2X_2/3 heteromeric receptors has come from studies on P2X₃receptor null-mutant mice (Cockayne et al., 2000; Souslova etal., 2000). These mice respond normally to acute noxious, thermal,and mechanical stimuli but display attenuated responses to non-noxious"warming" stimuli and show reduced formalin-induced nocifensivebehaviors. In addition, their phenotype includes a marked urinarybladder hyporeflexia (Vlaskovska et al., 2001) and, somewhat unexpectedly,increased hyperalgesia after peripheral inflammation of thehindpaw.

Little is known of the role of P2X₃ receptors in neuropathic pain, despite evidence that P2X₃ mRNA levels are altered afternerve injury (Novakovic et al., 1999; Bradbury et al., 1998; Decosterdand Woolf, 2000; Tsuzuki et al., 2001). It is conceivable thatsympathetic nerves, which sprout into DRG after nerve injury (Ramerand Bisby, 1997), provide a source of ATP that activates P2X₃receptors in thesoma.

Given the lack of specific P2X₃ receptor antagonists, we have used specific antisense oligonucleotides (ASOs) (Dorn et al.,2001) to investigate the effects of reducing the expression levelsof P2X₃ receptor subunit-containing receptors in inflammatoryand neuropathic pain models in therat.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antisense oligonucleotides. The ASOs against the P2X₃ subunit that were used in this study were characterized essentiallyas described (Dorn et al., 2001). Briefly, a fully phosphodiester18-mer with five nucleotides at the 3' and 5' ends modified with2'-O-(2-methoxyethyl) (MOE) groups was synthesized using phosphoramiditechemistry (Martin and Natt, 2000), HPLC-purified, and characterizedby electrospray mass spectrometry and capillary gel electrophoresis.The sequences that were used are as follows: ASO, 5'-ctc caT CCAGCC Gag tga-3', and missense oligonucleotide, (MSO), 5'-cta caGCCA TCC Gcg tga-3'; lowercase letters represent 2'-MOE and uppercaseletter represent DNA. In vitro experiments confirmed the abilityof the P2X₃ ASOs to downregulate P2X₃ receptor mRNA levels (Dornet al., 2001). P2X₃ ASOs have no effect on P2X₂ receptor mRNAlevels (data not shown). The ability to downregulate P2X₃ receptormRNA levels is lost when more than two to three conservative mutationsare introduced to produce the MSO (Dorn et al., 2001).

Animal models. All experiments were performed according to Home Office (United Kingdom) guidelines and with approval of thelocal Novartis Animal Welfare and EthicsCommittee.

Neuropathic pain. The partial sciatic ligation model of neuropathic pain was used as described previously (Seltzer et al.,1990; Fox et al., 2001; Patel et al., 2001). Briefly, male Wistarrats (120-140 gm) were anesthetized, the left sciatic nerve wasexposed at mid-thigh level through a small incision, and one-thirdto one-half of the nerve thickness was tightly ligated with a7.0 silk suture. The wound was closed with sutures and clips anddusted with antibiotic powder. In sham animals the sciatic nervewas exposed but not ligated, and the wound was closed as before.Mechanical hyperalgesia was assessed by measuring paw withdrawalthresholds of both hindpaws to an increasing pressure stimulususing an Analgesymeter (Ugo-Basile, Milan, Italy). The cutoffwas set at 250 gm, and the endpoint was taken as paw withdrawal,vocalization, or overt struggling. Mechanical allodynia was assessedby measuring withdrawal thresholds to non-noxious mechanical stimuliapplied with custom-made von Frey hairs to the plantar surfaceof both hindpaws. Animals were placed individually into wire mesh-bottomcages, with groups of six tested concurrently, and allowed toacclimatize for ~30 min. Von Frey hairs were tested in ascendingorder of force with a single trial of up to 6 sec for each hairuntil a withdrawal response was established; cutoff was at 20.6gm. This was confirmed as the withdrawal threshold by testinga lack of response to hair with the next lowest force. Each animalwas tested only once, in random order. The statistical significanceof mechanical hyperalgesia and allodynia data obtained from thedifferent experimental animal groups was analyzed using ANOVAfollowed by Tukey's honest significant difference (HSD)test.

$alpha$ , $beta$ -methylene ATP (0.1 or 1.0 µmol in 10 µl) was given by intraplantar injection to the contralateral hindpaw on the finalday of the experiment, and paw withdrawal thresholds to mechanicalstimuli were measured 0.5 and 1.0 hrlater.

Inflammatory pain. Male Sprague Dawley rats (200-250 gm) were cannulated as described below, and 24 hr after cannulation,25 µl complete Freund's adjuvant (CFA) was injected into one hindpaw.This induces a mechanical hyperalgesia and allodynia that developsafter a few hours and lasts up to 7 d. Paw withdrawal thresholdswere measured just before CFA injection and then daily for the7 d of ASO treatment. A 0.1 µmol dose of $alpha$ , $beta$ -methylene ATP wasgiven by intraplantar injection to the contralateral hindpaw onthe final day of the experiment. Paw withdrawal thresholds tomechanical hyperalgesia were measured 0.5 and 1.0 hr afteradministration.

Administration of P2X₃ oligonucleotides. ASOs and MSOs were administered intrathecally via an indwelling cannula that wasinserted 24 hr before or 14 d after sciatic nerve ligation or24 hr before CFA injection. Rats were anesthetized, and an incisionwas made in the dorsal skin just lateral to the midline and ~10mm caudal to the ventral iliac spines. A sterile catheter (polyethylenePE10 tubing) was inserted via a guide cannula (20 gauge needle)and advanced 3 cm cranially in the intrathecal space approximatelyto the L1 level. The catheter, which was inserted subcutaneouslyin the left or right flank, was then connected to an osmotic minipump(Alzet) delivering P2X₃ receptor ASO, MSO, or saline (1 µl/h,7 d). The incision was closed with wound clips and dusted withantibiotic powder. Preliminary experiments determined 180 µg/das a maximal tolerated dose. No evidence of neurotoxicity suchas paralysis, vocalization, or anatomical damage to the spinalcord was noted at this dose. Delivery of ASOs to the DRG cellbodies was initially confirmed using a fluorescently labeled ASO;an unlabelled version was used in all subsequentexperiments.

To assess whether intrathecal cannulation produced any nonspecific damage, a control group of naive animals that were cannulatedand received saline was included. Additionally, contralateralthresholds were always measured, which would provide an indicationof any nonspecificdamage.

Tissue and section preparation. Tissue fixation by perfusion with paraformaldehyde and cryopreservation was performed as describedpreviously (Wotherspoon and Winter, 2000). L4 and L5 DRGs fromthe left-hand side of naive animals were dissected for in situhybridization. The L4/L5 level of spinal cord was dissected forimmunohistochemistry (IHC) analysis. DRG sections were cut toa thickness of 10 µm using a cryostat (Bright Instrument Co. Ltd.,Cambridgeshire, UK) and thaw-mounted onto Superfrost poly-L-lysine-coatedslides (VWR International Ltd., Dorset, UK) and air dried. Sectionsto be analyzed by RNA in situ hybridization were stored directlyat $-$ 80°C. Spinal cord sections were freshly cut as required to30 µm and were free floated in PBS before processing forIHC.

Immunohistochemistry in spinal cord. Before IHC, sections were incubated with 10% normal donkey serum for 1 hr to reduce nonspecificstaining. Spinal cord sections were incubated in primary antibodyfor 48 hr. Primary antibodies used were P2X₃ receptor (rabbitanti-rat P2X₃ receptor; Neuromics catalog number RA10109-50; 1:10000dilution) and calcitonin gene-related peptide (CGRP) (sheep anti-ratCGRP, Affiniti; 1:1000 dilution). All dilutions were in PBT (PBS,0.1% Triton X-100, and 0.02% sodium azide). Sections were incubatedfor 2 hr in secondary antibodies: fluorescein (FITC)-conjugatedAffiniPure F(ab')₂ fragment donkey anti-rabbit IgG and rhodamine(TRITC)-conjugated AffiniPure F(ab')₂ fragment donkey anti-sheepor anti-guinea pig IgG, diluted in PBT at 1:200 (Jackson ImmunoResearch,West Grove, PA). Sections were washed three times for 5 min inPBS before and after the secondary antibody incubations. Sectionswere mounted in PBS/glycerol (1:3) containing 25 mg/ml diazobicyclo-2,2-octane(Sigma, St. Louis, MO) as an anti-fading agent. Images of antibody-stainedsections were captured using a Nikon Eclipse 800 fluorescent microscopeattached to a Hamamatsu cooled CCD camera and image capturingsystem using Image Pro Plus software (Media Cybernetics). Therelevant filter blocks that were used depended on the fluorescentmarker conjugated to the secondary antibody. Samples from eachanimal were processed for IHC and analyzed simultaneously (foursections per slide) to allow accurate comparisons. A negativecontrol where the primary antibody was replaced with PBT was includedin all experiments. Immunoreactivity was quantified by drawingaround the whole section using Image Pro Plus software (MediaCybernetics) and determining the mean fluorescence intensity.CGRP immunoreactivity was used to normalize P2X₃ receptor proteinlevels in spinal cordsections.

Statistical analysis and data presentation. Data from experimental and control populations were compared statistically usingKruskal-Wallis ANOVA with Dunn's multiple comparisons post-test.

Western blot analysis of P2X₃ receptors in DRG. L4 and L5 DRG were dissected from naive rats treated with ASO, MSO, or salineand snap-frozen on dry ice. Samples were prepared by crushingin a small pestle and mortar followed by homogenization in 100µl lysis buffer [50 mM Tris-HCl, pH 8, 150 mM NaCl, 5 mM EDTA,pH 8, 1% Triton, 1% SDS, 1:100 aprotinin-solution, 1 mM PMSF (bothSigma)]. Lysates were passed 10 times through a 0.6 × 30 gaugeneedle and centrifuged for 10 min at 14,000 rpm. Fifty microgramsof solubilized proteins from the supernatant fraction were mixedwith 3× loading buffer (187.5 mM Tris-HCl, pH 6.8, 30% glycerol,6% SDS, 0.3% Bromophenol blue) subjected to SDS-PAGE through aBio-Rad 4-20% Tris-glycine gel. Proteins were electrophoreticallytransferred on to a nitrocellulose membrane (Schleicher & Schuell,Dassel, Germany). After blocking for 1 hr with 5% milk powderin 1× TBS-T (10 mM Tris, pH 8.0, 150 mM NaCl, 0.05% Tween 20),the blot was incubated overnight with the P2X₃ receptor primaryantibody (Neuromics) at a dilution of 1:2000 in TBS-T. The filterwas incubated with a horseradish peroxidase-conjugated donkeyanti-rabbit IgG secondary antibody (Pierce (Perbio), Cheshire,UK), diluted 1:2000 in TBS-T, and then developed by enhanced chemiluminescence(ECL, Amersham Biosciences) and detected on film (ECL-Hyperfilm,Amersham Biosciences) according to the manufacturer's instructions.To check for variation in sample loading, the same blot was thenwashed and incubated overnight with a 1:2000 dilution of mouseanti-transferrin receptor primary antibody (Zymed, San Francisco,CA), followed by incubation with a 1:2000 dilution of horseradishperoxidase-conjugated goat anti-mouse IgG (Pierce) secondary antibodyand then detected usingECL.

P2X₃ receptor mRNA analysis by digoxigenin-labeled RNA in situ hybridization. To visualize the level of P2X₃ receptor mRNAin DRG neurons, digoxigenin (DIG)-labeled RNA in situ hybridizationwas performed. A 930 bp (EagI-EcoRV) fragment was subcloned froma P2X₃ receptor plasmid (nucleotide 583-1513; GenBank accessionnumber X90651) into pBluescript KSII+ (Stratagene). DNA fromthe subclone (P2X3-7) was prepared (QiaFilter maxiprep kit, Qiagen)and linearized with EagI or EcoRV (New England Biolabs, Beverly,MA) for the antisense and sense probes, respectively. DIG-labeledriboprobes were prepared from the linearized plasmids using T3polymerase (antisense) or T7 polymerase (sense) with a DIG RNAlabeling kit (Roche Diagnostics) as instructed. An aliquot (4µl) was checked by agarose gel electrophoresis, and the rest waspurified using a Quick Spin column (Roche Diagnostics) followedby overnight ethanol precipitation. The dried RNA pellet was resuspendedin 50 µl of 10 mM DTT solution and stored at $-$ 80°C. In situ hybridizationand color development were performed as described previously (Eisenstatet al., 1999). After color development, slides were washed inPBS and mounted as described for the IHC. In situ hybridizationimages were quantified using the method described above, exceptthat optical density wasmeasured.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Downregulation of P2X₃ receptors in naive animals

ASO treatment of naive animals (n = 6) for 7 d resulted in a functional downregulation of peripheral P2X₃ receptors as demonstratedby an abolition of mechanical hyperalgesia evoked by an intraplantarinjection of 0.1 µmol $alpha$ , $beta$ -methylene ATP into the hindpaw (Fig.1). The same dose of $alpha$ , $beta$ -methylene ATP injected into the hindpawof animals treated with saline or MSO evoked significant, similarlevels of mechanical hyperalgesia (Fig. 1).

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Figure 1. Inhibition of $alpha$ , $beta$ -methylene ATP evoked mechanical hyperalgesia in the hindpaw of naive rats after a 7 d treatment with P2X₃ receptor ASO, MSO, or saline. Paw withdrawal thresholds were measured before cannulation on day 0 and immediately before and 0.5 and 1 hr after administration of 0.1 µM $alpha$ , $beta$ -methylene ATP. Each point represents the mean ± SEM from three animals per treatment group. *p < 0.05 compared with saline treatment by ANOVA followed by Tukey's HSD test performed on gram threshold data.

Molecular analysis of the P2X₃ receptor ASO-, MSO-, and saline-treated animals (n = 3) revealed a downregulation of P2X₃ receptormRNA in the soma of DRG neurons. Nonradioactive in situ hybridizationin DRG neurons showed a visible reduction in P2X₃ receptor mRNAsignal after treatment with P2X₃ ASO but not saline or MSO (Fig.2A). Quantification of the in situ hybridization images (n = 4per L4/L5 DRG per animal) indicated that the P2X₃ receptor mRNAlevels were significantly reduced (p < 0.001) in P2X₃ receptorASO-treated animals compared with that of the saline- and MSO-treatedgroups (Fig. 2B).

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Figure 2. Molecular analysis of P2X₃ receptor mRNA expression levels in naive rats after a 7 d treatment with P2X₃ receptor ASO, MSO, or saline. A, Representative DRG sections from saline-, ASO-, and MSO-treated animals after nonradioactive RNA in situ hybridization with a P2X₃ probe. Presence of P2X₃ receptor mRNA is indicated by dark-staining cells. P2X₃ receptor mRNA levels are visibly reduced after ASO but not saline or MSO treatment. Scale bar, 200 µm. B, Quantification of P2X₃ receptor mRNA expression levels in the soma of DRG neurons visualized by in situ hybridization. P2X₃ receptor mRNA levels are expressed in arbitrary units. Each bar represents the mean ± SEM of 24 sections (4 sections per L4 and L5 DRG taken from 3 animals per treatment group). P2X₃ receptor ASO but not saline or MSO treatment decreases P2X₃ receptor mRNA expression levels. ***p < 0.001 compared with saline treatment by Kruskal-Wallis ANOVA with Dunn's multiple comparisons post-test.

P2X₃ receptor immunoreactivity in inner lamina II of the dorsal horn of the spinal cord was visibly reduced in P2X₃ receptorASO-treated animals compared with saline- or MSO-treated groups(Fig. 3A). Quantification of P2X₃ receptor immunoreactivity, normalizedto that of CGRP (four sections per animal; n = 3 per group) (Fig.3B), indicated that P2X₃ receptor protein expression levels inASO-treated animals were significantly reduced (p < 0.001) comparedwith those of the saline- and MSO-treated groups. Absolute P2X₃receptor protein levels that were not normalized to CGRP levelsalso showed significantly reduced levels in ASO-treated animalscompared with MSO- and vehicle-treated animals (data not shown).

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Figure 3. P2X₃ protein expression levels in the dorsal horn of lumbar spinal cord in naive rats after a 7 d treatment with P2X₃ receptor ASO, MSO, or saline. A, Representative images of P2X₃ receptor immunoreactivity in dorsal horn sections of lumbar (L4/L5) spinal cord from animals treated with saline, ASO, or MSO. Red band of P2X₃ immunoreactivity in lamina II is visibly reduced in ASO-treated animals (top panel). Coimmunostaining with CGRP (green) shows that equivalent regions of each spinal cord were analyzed. Scale bar, 200 µm. B, Quantification of P2X₃ protein expression levels in the dorsal horn of the spinal cord. Protein levels are expressed in arbitrary units. Each bar represents the mean ± SEM of 12 sections (4 sections per animal and 3 animals per treatment group). ***p < 0.001 compared with saline treatment by Kruskal-Wallis ANOVA with Dunn's multiple comparisons post-test.

Effect of ASO treatment on neuropathic and inflammatory hyperalgesia

The effect of P2X₃ receptor ASO treatment was evaluated in models of neuropathic and inflammatory pain. Intrathecal administrationof P2X₃ receptor ASO, initiated 24 hr before partial sciatic nerveligation, produced a significant inhibition in the developmentof mechanical hyperalgesia (p < 0.05, compared with MSO or saline)within 2 d of surgery that reached 50% inhibition by the finalreading on day 7 (Fig. 4A). Contralateral paw withdrawal thresholdswere not affected by surgery or ASO treatment (Fig. 4B).

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Figure 4. Effect of P2X₃ receptor ASO, MSO, or saline treatment on development of mechanical hyperalgesia in a rat model of neuropathic pain. Four groups (n = 6) of animals were cannulated and infused with P2X₃ receptor ASO, MSO, or saline for 7 d. Twenty-four hours after cannulation, the sciatic nerve was partially ligated in three groups, whereas the fourth saline-treated group was maintained as a control for the effects of cannulation. Mechanical hyperalgesia was assessed on ipsilateral (A) and contralateral (B) hindpaws before cannulation and then daily until day 7. Each point represents the mean ± SEM from six animals per treatment group. *p < 0.05 compared with neuropathic saline-treated group by ANOVA followed by Tukey's HSD test performed on gram threshold data.

In a model of established neuropathic hyperalgesia, 7 d of treatment with P2X₃ receptor ASO produced a significant 33% reversalof mechanical hyperalgesia (p < 0.05) (Fig. 5A) that was evidentwithin 2 d of treatment. Again, there was no effect of ASO treatmenton contralateral paw thresholds during the treatment period (Fig.5B).

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Figure 5. Effect of P2X₃ receptor ASO, MSO, or saline treatment on established mechanical hyperalgesia in a rat model of neuropathic pain. The sciatic nerve was partially ligated in three groups of six animals. On day 13, all three groups were cannulated and treated with P2X₃ receptor ASO, MSO, or saline for 7 d. An addition saline group was set up on the same day as a control for cannulation. Mechanical hyperalgesia was assessed on ipsilateral (A) and contralateral (B) hindpaws before surgery and then daily from days 13-20. Each point represents the mean ± SEM from six animals per treatment group. *p < 0.05 compared with neuropathic saline treatment group by ANOVA followed by Tukey's HSD test performed on gram threshold data.

P2X₃ receptor ASO treatment had no effect on either the development of mechanical allodynia (Fig. 6A) or the allodynia inthe model of established neuropathic pain (Fig. 6B).

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Figure 6. Effect of P2X₃ receptor ASO, MSO, or saline treatment on the development and maintenance of mechanical allodynia in a rat model of neuropathic pain. A, Mechanical allodynia was assessed in the ipsilateral and contralateral (data not shown) hindpaws of animals described in Figure 4 before cannulation and then daily until day 6. Each point represents the mean ± SEM from six animals per treatment group. No significant difference was detected on the development of mechanical allodynia. B, Mechanical allodynia was assessed in the ipsilateral and contralateral (data not shown) hindpaws of animals described in Figure 5 before surgery and then daily from days 13-20. Each point represents the mean ± SEM from six animals per treatment group. No significant difference was detected on the maintenance of mechanical allodynia.

In the inflammatory pain model, intrathecal administration of P2X₃ receptor ASO for 7 d, initiated 24 hr before the injectionof CFA into the hindpaw, produced a 25% attenuation in the developmentof mechanical hyperalgesia (p < 0.05) (Fig. 7A). Contralateralwithdrawal thresholds were not affected by ASO treatment (Fig.7B). The development of mechanical allodynia was not reduced byP2X₃ receptor ASO treatment (data not shown).

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Figure 7. Effect of P2X₃ receptor ASO, MSO, or saline treatment on the development of mechanical hyperalgesia in the complete Freund's adjuvant (CFA) model of inflammatory pain. Four groups (n = 6) of animals were cannulated and infused with P2X₃ receptor ASO, MSO, or saline for 7 d. Twenty-four hours after cannulation, three groups received an intraplantar stimulus of CFA into the hindpaw, and the fourth saline group was maintained as a control for cannulation. Mechanical hyperalgesia was assessed on ipsilateral (A) and contralateral (B) hindpaws before cannulation and then daily until day 7. Each point represents the mean ± SEM from six animals per treatment group. *p < 0.05 compared with CFA saline treatment group by ANOVA followed by Tukey's HSD test performed on gram threshold data.

Antisense treatment results in incomplete receptor knockdown

In all of the above investigations, functional downregulation of P2X₃ receptors was assessed in the contralateral "untreated"hindpaw using an injection of $alpha$ , $beta$ -methylene ATP (0.1 and 1 µmol)on the final day of the experiment (Fig. 8). These doses of $alpha$ , $beta$ -methyleneATP were chosen selectively to activate P2X₃ and P2X_2/3 receptorson the basis of previous published studies (Tsuda et al., 2000).In experiments examining the development of neuropathic pain,ASO but not MSO or saline treatment abolished the mechanical hyperalgesiaevoked by 0.1 µmol $alpha$ , $beta$ -methylene ATP (Fig. 8) and attenuated (66%relative to predose) the mechanical hyperalgesia evoked by 1 µmol $alpha$ , $beta$ -methylene ATP (Fig. 8). Similarly, ASO but not MSO or salinetreatment abolished the mechanical hyperalgesia evoked by a 0.1µmol dose of $alpha$ , $beta$ -methylene ATP on established neuropathic painand the development of inflammatory hyperalgesia (data not shown).

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Figure 8. Inhibition of $alpha$ , $beta$ -methylene ATP evoked mechanical hyperalgesia in the contralateral hindpaw of neuropathic rats after a 6 or 7 d treatment with P2X₃ receptor ASO, MSO, or saline. On the final experimental day, $alpha$ , $beta$ -methylene ATP was administered by intraplantar injection to the contralateral hindpaws of the animals described in Figure 4. Paw withdrawal thresholds were determined before and 0.5 hr after $alpha$ , $beta$ -methylene ATP administration. Doses of 0.1 or 1.0 µmol were used. In each case the mean ± SEM of the mean paw withdrawal thresholds of n = 6 per treatment group are shown. In all cases ASO treatment results in a significant inhibition of the development of $alpha$ , $beta$ -methylene ATP-evoked mechanical hyperalgesia. *p < 0.05 compared with saline treatment group by ANOVA followed by Tukey's HSD test performed on gram threshold data. However, the 100% inhibition seen in the ASO-treated group at the 0.1 µmol dose is reduced to 66% relative to predose values at a higher 1.0 µmol dose.

In all of the pain models, mechanical hyperalgesia was significantly reversed 2 d after ASO treatment. To assess whether P2X₃receptor ASO treatment could cause a functional downregulationof P2X₃ receptor that might directly account for this relativelyfast reversal, $alpha$ , $beta$ -methylene ATP-induced mechanical hyperalgesiawas evaluated in naive rats after treatment with ASO for 2 d.A significant reduction (45% relative to predose) in 1 µmol $alpha$ , $beta$ -methyleneATP-induced mechanical hyperalgesia was observed in ASO-treatedrelative to saline- or MSO-treated rats (Fig. 9A). Furthermore,immunoblot analysis of the DRG from these naive rats showed avisible downregulation of P2X₃ receptor after treatment with ASOrelative to MSO or saline treatment for 2 d (Fig. 9B).

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Figure 9. A, Inhibition of $alpha$ , $beta$ -methylene ATP evoked mechanical hyperalgesia in the hindpaw of naive rats after a 2 d treatment with P2X₃ receptor ASO, MSO, or saline. Paw withdrawal thresholds were measured before cannulation on day 0 and immediately before and 1 hr after administration of 1 µmol $alpha$ , $beta$ -methylene ATP. Each point represents the mean ± SEM from six animals per treatment group. *p < 0.05 compared with saline treatment by ANOVA followed by Tukey's HSD test performed on gram threshold data. B, P2X₃ receptor protein levels in DRG are reduced in ASO relative to MSO or saline groups after 2 d of treatment in naive rats. L4 and L5 DRG were isolated and pooled from naive rats and evaluated by Western blot analysis. Immunoblots were reprobed for transferrin to control for protein loading. Representative results are shown for three saline-, MSO-, and ASO-treated animals.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The aim of the present study was to investigate the effects of downregulating P2X₃ receptors in rat models of chronic inflammatoryand neuropathic pain using ASO technology. We have demonstratedthat P2X₃ receptor oligonucleotides, previously characterizedextensively by Dorn et al. (2001), can be reproducibly deliveredto lumbar DRG and spinal cord neurons via an indwelling intrathecalcannula attached to an osmotic minipump. We observed no signsof neurotoxicity from the surgical procedure such as paralysis,vocalization, or gross anatomical changes in the spinal cord.In addition, there was no evidence of neurotoxicity from the chemicalcomposition [phosphodiester flanked by 2'-O-(2-methoxyethyl) groups]or the dose (180 µg/d) of oligonucleotidesadministered.

Delivery of P2X₃ receptor ASO, but not MSO or saline, for 7 d produced significant reduction of P2X₃ message in the DRG aswell as P2X₃ receptor protein in inner lamina II of the dorsalhorn of the spinal cord in naive animals. This was consistentwith the reduced mechanical hyperalgesia evoked by intraplantaradministration of $alpha$ , $beta$ -methylene ATP into the hindpaw at this timepoint, demonstrating a functional downregulation of P2X₃ receptorsin peripheral terminals of sensoryneurons.

In the Seltzer et al. (1990) model of neuropathic pain, ASO treatment significantly reduced the development of mechanicalhyperalgesia and partially reversed established mechanical hyperalgesia.Similarly, ASO treatment inhibited the development of CFA-inducedmechanical hyperalgesia. These ASO effects were evident only inthe ipsilateral paws in the pain models, whereas no significantchanges in nociceptive indices were observed in the contralateralpaws or indeed in any MSO- or saline-treated groups. Althougholigonucleotide treatment of neuropathic and inflammatory animalswas maintained for up to 7 d, a partial reversal of mechanicalhyperalgesia in these models was observed as early as 2 d afterASO application. We were able to demonstrate a reduction in P2X₃receptor protein expression in DRG as well as a functional downregulationof P2X₃ receptor in the periphery, measured by injecting $alpha$ , $beta$ -methyleneATP into the hindpaw, after 2 d of ASO administration in naiveanimals. Taken together, these data are consistent with the hypothesisthat the rapid reversal of mechanical hyperalgesia, observed inthe pain models, can be directly attributed to the downregulationof P2X₃receptor.

It is notable that at the maximum ASO dose administered (180 µg/d), significant but incomplete reversal of mechanical hyperalgesiain either the neuropathic or the inflammatory pain models is observed.This could reflect a partial role of P2X₃ receptors in nociceptivesignaling, or it may be the result of incomplete receptor "knockdown."ASO treatment does not commonly produce a total protein knockdown(Hallbook et al., 2000; Yoshimura et al., 2001). Incomplete receptordownregulation is consistent with the residual P2X₃ message andreceptor in DRG and spinal cord immunoreactivity observed in ASO-treatedanimals. Incomplete downregulation of P2X₃ receptors is also consistentwith the observed reduction, but not abolition, of mechanicalhyperalgesia evoked after an intraplantar injection of 1 µmol $alpha$ , $beta$ -methylene ATP into the contralateral hindpaw. This dose issimilar to concentrations of ATP reached in injured tissue. Ininflammatory pain states, persistent and augmented ATP responsesare observed, which suggests that significant endogenous ATP levelscontribute to the pathophysiology of pain (Hamilton and McMahon,2000).

It has been reported previously (Tsuda et al., 2000) that intraplantar injection of $alpha$ , $beta$ -methylene ATP into the hindpaw ofnaive rats elicits nocifensive behavior (paw licking), which isattributed to activation of peripheral P2X₃ receptors, as wellas mechanical allodynia, which was attributed to heteromeric P2X_2/3receptor activation. Although P2X₃ ASO treatment is predictedto downregulate all receptors containing P2X₃ subunits, includingP2X₃ homomers and P2X_2/3 heteromers (and formally P2X_1/3 homomers)(Torres et al., 1999; Petruska et al., 2000a), we observed noreversal on mechanical allodynia in either neuropathic or inflammatorypain states. One possible explanation for this observation isthat P2X₃ receptors do not mediate this modality in neuropathicand inflammatory pain states. It has been proposed that specificsubpopulations of DRG afferents, in particular the A-fiber low-thresholdmechanoreceptors, are involved in generation of allodynic behavior(Matzner and Devor, 1994; Campbell, 2001; Kim et al., 2001). Indeed,immunohistochemical techniques show that P2X₃ receptors are notlocalized to these neurons (Bradbury et al., 1998), suggestingthat these receptors may not have a role in mechanical allodynia.However, an equally likely possibility for our observations isthat there was insufficient downregulation of P2X₃ subunits toelicit a reversal of mechanicalallodynia.

Taken together, the findings in the present study show, for the first time, that P2X₃ ASO treatment produces a partial functionaldownregulation of peripheral P2X₃ receptors and a reduction inP2X₃ receptors in the DRG and the primary afferent terminals ofthe spinal cord that are associated with a significant, but partial,inhibition of mechanical hyperalgesia in models of inflammatoryand neuropathic pain. Previous studies using P2X₃ receptor null-mutantmice (Cockayne et al., 2000; Souslova et al., 2000) did not investigatethe effects of the absence of these receptors on neuropathic pain.They did report, however, that these mice show hypersensitivityto an inflammatory stimulus, which is clearly different from ourdata. The reason for this disparity is unclear. Cook and McCleskey,(2000) have suggested previously that the increased response tothe inflammatory stimulus in the null-mutant mice may have beena compensatory artifact of the gene knock-out approach. AlthoughSouslova et al., (2000) studied other P2X mRNA levels in the knock-outmice, protein and functional receptor levels were not examinedand neither were the levels of other transcripts that may havecontributed to the nociceptivemechanism.

In conclusion, our data indicate that homomeric P2X₃ and/or heteromeric P2X_2/3 receptors play a significant role in both neuropathicand inflammatory pain processing. We would propose that smallmolecule P2X₃ receptor antagonists would have a beneficial rolein alleviating neuropathic, inflammatory, and possibly mixed painconditions such as osteoarthritis and cancer pain. Moreover, specificP2X₃ receptor antagonists are also likely to reveal the extentof the role of homomeric P2X₃ and heteromeric P2X_2/3 receptorsin these painstates.

Additionally, this work validates the use of ASO technology for dissecting the role of receptor subunits in cases where noselective pharmacological tools areavailable.

  FOOTNOTES

Received Feb. 26, 2002; revised June 18, 2002; accepted June 20, 2002.

We are indebted to Dr. Katharine Walker, Dr. Laszlo Urban, and Clive Gentry for guidance with setting up the intrathecal cannulationfor antisense oligonucleotide delivery. We also thank Prof. JohnWood for the rat P2X₃ cDNAclone.

Correspondence should be addressed to Dr. Pam Ganju, Novartis Institute for Medical Sciences, 5 Gower Place, London WC1E 6BS,UK. E-mail: pam.ganju{at}pharma.novartis.com.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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