The Involvement of the Tetrodotoxin-Resistant Sodium Channel Nav1.8 (PN3/SNS) in a Rat Model of Visceral Pain

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The Journal of Neuroscience, November 1, 2001, 21(21):8690-8696

The Involvement of the Tetrodotoxin-Resistant Sodium Channel Na_v1.8 (PN3/SNS) in a Rat Model of Visceral Pain
Naoki Yoshimura¹^,², Satoshi Seki², Sanja D. Novakovic³, Elda Tzoumaka³, Vickie L. Erickson², Kristin A. Erickson², Michael B. Chancellor¹, and William C. de Groat²
Departments of ¹ Urology and ² Pharmacology, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania 15261, and ³ Neurobiology Unit, Roche Bioscience, Palo Alto, California 94304

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study investigated the effect of inhibiting the expression of Na_v1.8 (PN3/SNS) sodium channels by an antisenseoligodeoxynucleotide (ODN) on bladder nociceptive responses inducedby intravesical acetic acid infusion in rats. Animals were injectedintrathecally with either Na_v1.8 antisense or mismatch ODN. Controlcystometrograms under urethane anesthesia during intravesicalsaline infusion exhibited intercontraction intervals (ICIs) thatwere significantly longer in antisense-treated rats than in mismatchODN-treated rats. Intravesical infusion of 0.1% acetic acid inducedbladder hyperactivity as reflected by a 68% reduction in ICIsin mismatch ODN-treated rats but did not significantly reduceICIs in antisense-treated rats. The number of Fos-positive cellsafter acetic acid administration were significantly reduced inthe L6 spinal cord from antisense-treated animals, compared withmismatch ODN-treated animals. In addition, Na_v1.8 immunoreactivitywas reduced in L6 dorsal root ganglion neurons in the antisense-treatedrat. In patch-clamp recordings, the conductance density of TTX-resistantsodium currents in dissociated bladder afferent neurons that werelabeled by axonal transport of a fluorescent dye, Fast Blue, injectedinto the bladder wall was also smaller in antisense-treated ratsthan in mismatch ODN-treated rats, whereas no changes were observedin TTX-sensitive currents. These results indicate that the Na_v1.8TTX-resistant sodium channels are involved in the activation ofafferent nerves after chemical irritation of the bladder. Thesechannels represent a new target for the treatment of inflammatorypain from visceral organs such as the urinarybladder.

Key words: dorsal root ganglion; tetrodotoxin; Na_v1.8 sodium channels; urinary bladder; acetic acid; inflammation; antisense oligodeoxynucleotide

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

It has been shown in humans as well as in animals that tissue inflammation in visceral organs such as the urinary bladdercan sensitize afferent nerves and thereby elicit painful sensationsas well as hyperactivity of the inflamed organs (Stillwell andBenson, 1988; Häbler et al., 1990; Sengupta and Gebhart, 1994;Dmitrieva and McMahon, 1996; Dmitrieva et al., 1997). For example,interstitial cystitis, a chronic inflammatory disorder of theurinary bladder, is characterized by urinary frequency, urgency,and severe suprapubic pain (Ho et al., 1997). Intravesical applicationof capsaicin or resiniferatoxin, substances that desensitize C-fiberafferents, reduced the painful bladder symptoms in these patients(Lazzeri et al., 1996, 2000). It is also known that bladder hyperreflexiainduced by chemical irritation of the bladder in rats is suppressedby pretreatment with capsaicin (Maggi et al., 1992; Yu and deGroat, 1999). Thus it seems reasonable to assume that suppressionof activity of C-fiber afferent pathways can be effective in treatingpain arising from visceral organs such as the urinarybladder.

Our previous studies showed that capsaicin-sensitive C-fiber afferent neurons innervating the bladder and colon predominantlyexpress high-threshold sodium currents and action potentials thatare resistant to tetrodotoxin (TTX) (Yoshimura et al., 1996; Yoshimuraand de Groat, 1997; Yoshimura, 1999) and that C-fiber bladderafferent neurons with TTX-resistant action potentials become hyperexcitablein rats with chronic cystitis induced by cyclophosphamide (Yoshimuraand de Groat, 1999). Therefore, suppression of TTX-resistant actionpotentials might be a useful approach for treating visceralpain.

The TTX-resistant sodium channel Na_v1.8 (PN3/SNS) is preferentially expressed in small-sized nociceptive dorsal root ganglion(DRG) neurons (Arbuckle and Docherty, 1995; Akopian et al., 1996;Sangameswaran et al., 1996; Goldin et al., 2000; Waxman et al.,2000). It has been reported that suppression of Na_v1.8 channelswas effective in reducing pain induced by injury of somatic afferentaxons or tissue inflammation (Khasar et al., 1998; Porreca etal., 1999). However, it is not known whether Na_v1.8 sodium channelsare involved in activation of TTX-resistant sodium currents invisceral afferent neurons and in sensitization of visceral nociceptors.Thus we examined the effect of suppressing Na_v1.8 TTX-resistantsodium channels with an antisense oligodeoxynucleotide (ODN) ona rodent model of visceral pain induced by intravesical instillationof acetic acid (Birder and de Groat, 1992). We observed that intrathecalantisense ODN treatment decreased expression of Na_v1.8 sodiumchannels in lumbosacral DRG neurons, reduced TTX-resistant sodiumconductances in bladder afferent neurons, and suppressed bladdernociceptive responses induced by bladderirritation.

Preliminary results of this study have been reported previously in abstract form (Seki et al., 2000; Yoshimura et al., 2000).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animal preparation. Experiments were performed on adult female Sprague Dawley rats (170-200 gm). Care and handling of animalswere in accordance with institutional guidelines and approvedby the University of Pittsburgh Institutional Animal Care andUseCommittee.

An intrathecal catheter (PE-10) was implanted at the level of the L6-S1 spinal cord after a laminectomy at the Th11 vertebraunder halothane anesthesia. The distal end of the catheter wasfire sealed and placed subcutaneously. The rats were injectedintrathecally with either Na_v1.8 antisense or mismatch phosphodiesterODN (Life Technologies, Gaithersburg, MD) 3-4 d after intrathecalcatheter implantation. Antisense ODN (5'-TCC-TCT-GTG-CTT-GGT-TCT-GGC-CT-3')was directed against a unique sequence of the Na_v1.8 sodium channel(Porreca et al., 1999). The mismatch ODN (5'-TCC-TTC-GTG-CTG-TGT-TCG-TGC-CT-3')consisted of the antisense sequence, except that five pairs ofbases were switched. A dose of 45 µg of ODN dissolved in 8 µlof artificial CSF was injected through the intrathecal catheterunder halothane anesthesia twice a day for 3 d. The position ofthe intrathecal catheter was checked after the experiment to confirmthe location at the level of L6-S1 spinalcord.

Cystometry. Within 3-6 hr after the last injection of ODN solution, cystometry was performed under urethane anesthesia (1.2mg/kg, s.c.). A catheter (PE-50) was inserted via a midline abdominalincision into the bladder through the bladder dome, and then intravesicalpressure was measured to monitor bladder activity during continuousinfusion of saline solution (0.04 ml/min). After a control periodof 1-2 hr, the solution was switched to saline containing 0.1%acetic acid. Intercontraction intervals (ICIs), maximal contractionpressure, and pressure thresholds inducing reflex bladder contractionwere measured before and after intravesical infusion of aceticacid in both Na_v1.8 mismatch and antisense ODN-treatedrats.

Animal perfusion and tissue preparation. Two hours after infusion of acetic acid into the bladder, the animals were killedvia intracardiac perfusion with Krebs buffer followed by 4% paraformaldehydefixative. The L6 spinal cord and L6 DRGs were then removed andpost-fixed for 10-12 hr in the same fixative at 4°C. The spinalcords were placed in phosphate-buffered 30% sucrose solution overnightfor cryoprotection and embedded in OCT Tissue Tek. Alternate 42-µm-thickcryosections were cut and mounted on gelatin-coated slides forFos staining. DRGs were processed in xylene and ethanol solutionsand embedded in paraffin blocks for Na_v1.8 staining. Sections(4 µm thick) were cut, mounted, and air dried, first at room temperatureand then in a forced-air dryer (20 min, 60°C).

Fos staining. Spinal cord sections were processed by an avidin-biotin complex (ABC) method for the Fos protein with antibodiespurchased from Oncogene Science (Cambridge, MA), as describedpreviously (Birder and de Groat, 1992; Kakizaki et al., 1996).Briefly, sections were incubated in Fos antiserum (1:15,000) for30 min at room temperature and then for 72 hr at 4°C. Sectionswere then exposed to biotinylated secondary antibody (Vector,Burlingame, CA; 1:600) and ABC reagent (Vector), each for 1 hrat room temperature. Tissue sections were then mounted on gelatin-coatedslides, dehydrated in graded ethanol rinses, cleared in xylene,and coverslipped with Permount. Control sections in which primaryantibody was replaced with 0.4% Triton X-100 were negative. Analysiswas performed on the L6 spinal cord segment, because in the previousstudies the largest number of Fos-positive cells after bladderirritation was located in this segment (Birder and de Groat, 1992;Kakizaki et al., 1996). Cells exhibiting Fos immunoreactivitywere counted in four spinal cord regions: medial dorsal horn (MDH),lateral dorsal horn (LDH), dorsal commissure (DCM), and laterallaminas V-VII containing the sacral parasympathetic nucleus (SPN).Counts of Fos-positive cells were performed on both sides of thespinal cord and presented as average numbers persection.

Na_v1.8 staining. After deparaffinization in xylene and ethanol solutions, DRG sections were preincubated in potassium PBS(KPBS) containing 20% normal goat serum (NGS) and 0.2% TritonX-100 (1 hr, room temperature), and then incubated in KPBS containing5% NGS, 0.2% Triton X-100, and Na_v1.8 antibodies at 1:50 dilution(overnight, 4°C). The specificity of this antibody for Na_v1.8has been demonstrated previously (Novakovic et al., 1998). Thenext day, sections were washed in KPBS containing 0.1% bovineserum albumin and 0.1% Triton X-100 (2 hr, room temperature),incubated in the secondary antibody solution (biotinylated anti-rabbitIgG 1:200, Vecstatin Elite Kit; 1 hr, room temperature), washedagain, and then incubated with peroxidase ABC (1:50, 90 min, roomtemperature). After a few washes with 0.1 M KPB, the stainingpattern was visualized with a DAB substrate reaction (Zymed Laboratories,San Francisco, CA). Tissue sections were then washed, dehydratedin a series of ethanols and xylenes, and mounted with Krystalon.Images were obtained with a Nikon Microphot SA microscope andthe IPLab Spectram (Sigma Analytics). Thereafter, in randomlyselected DRG sections, cell size and labeling intensity measurementswere made on all cell profiles that exhibited a nucleus (~120-150cells per animal; n = 4 animals) using Scion Image software (ScionCorporation). The perimeter of each neuron profile was traced,and the cross-sectional area including the nuclear region wascalculated. Neurons were then analyzed for mean labeling intensityof Na_v1.8 staining. For the measurement of labeling intensity,the nucleus region was excluded. Na_v1.8 staining intensity ofeach neuron was estimated by subtracting nonspecific staining.The latter was determined by sampling the staining intensitiesof large-diameter neurons (average of six neurons per section)that were similar to those of cells labeled with preabsorbed antibodies(i.e., negative staining for Na_v1.8protein).

Electrical recording. In four animals in each group treated with either Na_v1.8 mismatch or antisense ODN, L6-S1 DRGs weredissociated enzymatically into single neurons, and TTX-resistantsodium currents were measured using patch-clamp recording techniques.The population of DRG neurons that innervate the urinary bladderwere labeled by retrograde axonal transport of a fluorescent dye,Fast Blue (4% w/v) (Polyloy, Gross Umstadt, Germany) injectedinto the wall of the bladder in halothane-anesthetized animals(Yoshimura et al., 1994, 1998). The dye was injected with a 29gauge needle at three to six sites on the dorsal surface of thebladder (5-6 µl per site; total volume of 20-30 µl). Each injectionsite was washed with saline to minimize contamination of adjacentorgans with the dye. Particular care was taken to avoid injectionsinto the lumen, major blood vessels, or overlying fascial layers.Our previous studies (Keast and de Groat, 1992; Yoshimura et al.,1998) using these techniques showed that nonspecific labelingof neurons caused by the leakage of dye isnegligible.

One week after dye injection into the bladder, freshly dissociated neurons from DRGs were removed from halothane-anesthetizedanimals (Yoshimura et al., 1996; Yoshimura and de Groat, 1997).Briefly, L6 and S1 DRGs were dissected and incubated in a bathfor 25 min at 35°C with 5 ml of DMEM (Sigma, St. Louis, MO) containing0.3 mg/ml trypsin (Type 3, Sigma), 1 mg/ml collagenase (Type 1,Sigma), and 0.1 mg/ml deoxyribonuclease (Type 4, Sigma). Trypsininhibitor (Type 2a, Sigma) was then added to neutralize the activityof trypsin. Individual DRG cell bodies were isolated by triturationand then plated on poly-L-lysine-coated 35 mm Petri dishes. Dye-labeledprimary afferent neurons that innervate the urinary bladder wereidentified using an inverted phase-contrast microscope (Nikon,Tokyo, Japan) with fluorescent attachments (UV-1A filter; excitationwavelength, 365 nm). G $Omega$ -seal whole-cell recordings were performedat room temperature (20-22°C) on each freshly dissociated labeledneuron in a culture dish that usually contained two to five labeledcells among a few hundred unlabeled neurons. The internal solutionused during current-clamp recordings of sodium currents contained(in mM) NaCl 10, CsF 125, CaCl₂ 1, MgCl₂ 2, EGTA 10, HEPES 10,Mg-ATP 4, and GTP (Tris Salt) 0.3, adjusted to pH 7.4 with CsOH(310 mOsm). Patch electrodes had resistances of 1-4 M $Omega$ when filledwith the internal solution. Neurons were superfused at a flowrate of 1.5 ml/min with an external solution containing (in mM):NaCl 40, tetraethylammonium (TEA)-Cl 95, MgCl₂ 10, CaCl₂ 0.03,4-aminopyridine 5, HEPES 10, and D-glucose 10, adjusted to pH7.4 with TEA-OH (340 mOsm). All recordings were made with an Axopatch-1Dpatch-clamp amplifier (Axon Instruments, Foster City, CA), anddata were acquired and analyzed by PCLAMP software (Axon Instruments).The peak amplitudes of the currents were measured and convertedto sodium conductances by means of the following equation: G_Na= I_Na/(V_test $-$ V_rev), where G_Na is the sodium conductance, I_Nais the sodium current, V_test is the test potential, and V_rev isthe reversal potential for the sodium current. To correct thesodium conductance for cell size, the TTX-resistant and TTX-sensitivesodium conductances for each cell were normalized with respectto cell membrane capacitances that were obtained by reading thevalue for whole-cell input capacitance neutralization directlyfrom theamplifier.

Analysis. All data are expressed as means ± SEM. Statistical differences between data were determined by Mann-Whitney U test.A level of p < 0.05 was considered to be statisticallysignificant.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cystometry

Control cystometrograms performed by infusing saline into the bladder revealed that ICIs were significantly (p < 0.05) longerin antisense-treated rats than in mismatch ODN-treated rats (9.7± 1.2 vs 6.7 ± 0.8 min) (Figs. 1, 2). Subsequent intravesicalinfusion of 0.1% acetic acid induced bladder hyperactivity, reducingICIs to 2.2 ± 0.3 min (68% reduction; p < 0.01) in mismatch ODN-treatedrats (n = 8). However, in Na_v1.8 antisense ODN-treated rats (n= 8), the ICI after intravesical acetic acid infusion was reducedby 38% to 6.0 ± 1.0 min, which was not significantly different(p = 0.65) from the ICI before acetic acid treatment (9.7 ± 1.2min) (Figs. 1, 2). Mean pressure thresholds (8.7 ± 0.7 vs 9.3± 0.8 cmH₂O) and bladder contraction pressure (36.7 ± 3.7 vs 34.2± 2.9 cmH₂O) were not significantly different in mismatch andantisense ODN-treated animals.

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Figure 1. Effects of intravesical infusion of 0.1% acetic acid on cystometrograms in rats treated with mismatch or antisense oligodeoxynucleotide (ODN) for Na_v1.8 sodium channels. Note that in an antisense-treated rat, acetic acid-induced bladder hyperactivity was suppressed.

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Figure 2. Effects of intravesical infusion of acetic acid on intercontraction intervals (ICI) in rats treated with mismatch (n = 8) or antisense ODN (n = 8). Note that in antisense ODN-treated rats, the ICI in the control period is significantly longer and a reduction in the ICI after acetic acid infusion is significantly smaller, when compared with mismatch ODN-treated rats. *p < 0.05, **p < 0.01.

Fos staining

After bladder irritation by intravesical infusion of acetic acid, Fos-positive cells were identified in the MDH, LDH, DCM,and SPN areas of the L6 spinal cord (Fig. 3). The largest numberof Fos-positive cells was located in the DCM area in both groupsof animals. The total number of Fos-positive cells in the L6 spinalcord after bladder irritation in antisense ODN-treated animalswas significantly smaller (p < 0.01) than in mismatch ODN-treatedanimals (20.6 ± 1.1 vs 61.2 ± 2.6 cells per section). The numbersof Fos-positive cells were significantly (p < 0.01) smaller inthe DCM (6.3 ± 1.1 vs 25.8 ± 2.4), MDH (2.5 ± 0.6 vs 13.0 ± 2.6),LDH (1.5 ± 0.6 vs 6.1 ± 1.2), and SPN (8.3 ± 1.0 vs 14.9 ± 2.1cells per section) regions of the L6 spinal cord from antisense-treatedanimals, compared with mismatch ODN-treated animals (Fig. 3).

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Figure 3. Effects of Na_v1.8 antisense ODN on c-fos expression in the L6 spinal cord after intravesical infusion of acetic acid. A, Photomicrographs of Fos staining in transverse sections of the L6 spinal cord from rats treated with mismatch (left panel) and antisense (right panel) ODN. B, Histograms of the number of Fos-positive cells after intravesical acetic acid infusion. DCM, Dorsal commissure; DH, dorsal horn; SPN, sacral parasympathetic nucleus; CC, central canal. *p < 0.01.

Na_v1.8 staining

In four mismatch and four antisense ODN-treated rats, 445 and 421 DRG neuron profiles were measured, respectively. The cross-sectionalareas of cell profiles were divided into three groups accordingto their measured area: small (<700 µm²; 174 and 169 cells), medium (700-1200 µm²; 133 and 121 cells), and large (>1200 µm²; 138 and 131 cells) in mismatch and antisense ODN-treated rats.In mismatch ODN-treated rats, the highest intensity of labelingfor Na_v1.8 was found in small-sized DRG neurons, whereas medium-sizedneurons had lower intensity of staining, and the staining intensityof large-sized neurons was minimal (Fig. 4), as reported previouslyin untreated rats (Novakovic et al., 1998). In Na_v1.8 antisense-treatedrats, the mean intensity of Na_v1.8 labeling in small- and medium-sizedneurons was significantly decreased by 44 and 46%, respectively,compared with the labeling intensity in mismatch ODN-treated rats,indicating the reduction of Na_v1.8 channel protein expressionafter antisense ODN treatment (Fig. 4B).

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Figure 4. Immunolabeling of Na_v1.8 TTX-resistant sodium channels in L6 DRG. A, Photomicrographs of Na_v1.8 immunostaining in rat treated with mismatch (left panel) or antisense (right panel) ODN. Scale bar, 50 µm. B, Averaged Na_v1.8 labeling intensity in L6 DRG neurons with small, medium, and large cross-sectional somal areas. Note that labeling intensity is greater in small-sized neurons and significantly reduced after antisense treatment in small- to medium-sized neurons. *p < 0.01.

Sodium currents in bladder afferent neurons

As reported previously, in the majority of small-sized (<30 µm diameter or 765 µm² cross-sectional area) bladder afferent neurons, inward sodiumcurrents elicited from the holding potential of $-$ 60 mV were mainlyinsensitive to TTX (1 µM) (Yoshimura et al., 1996; Yoshimura andde Groat, 1997). In this population of bladder afferent neurons,the peak amplitude of sodium currents was measured in presenceof 1 µM TTX. The calculated sodium conductances were then normalizedwith respect to cell membrane capacitances. The maximum conductancedensity of TTX-resistant sodium currents at the holding potentialof $-$ 60 mV in bladder afferent neurons was significantly (p < 0.05)smaller in antisense ODN-treated rats than in mismatch ODN-treatedrats (1.9 ± 0.5 vs 4.1 ± 0.9 nS/pF; n = 15) (Fig. 5). The valuesfor membrane voltages at half-maximal activation of TTX-resistantcurrents calculated by the Boltzmann equation in antisense andmismatch ODN-treated rats ( $-$ 11.2 and $-$ 10.7 mV, respectively) werenot different from those reported in our previous studies (Yoshimuraet al., 1996; Yoshimura and de Groat, 1997). In contrast, large-sized(>30 µm or 765 µm²) bladder afferent neurons expressed TTX-sensitive sodium currentsthat comprised >60% of the total sodium currents elicited by depolarizingpulses to 0 mV from the holding potential of $-$ 60 mV (Yoshimuraand de Groat, 1997). In these neurons (n = 12), TTX-sensitivesodium currents were isolated by the subtraction of the currentsafter TTX application from those before TTX application. The maximumconductance density of TTX-sensitive sodium currents at the holdingpotential of $-$ 60 mV in antisense ODN-treated rats (3.9 ± 0.8 nS/pF)was not different from the conductance density (4.0 ± 0.7 nS/pF)in mismatch ODN-treated rats.

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Figure 5. Effects of Na_v1.8 antisense ODN on TTX-resistant sodium currents in bladder afferent neurons. A, Superimposed traces of TTX-resistant sodium currents elicited by depolarizing pulses to 10 mV from the holding potential of $-$ 60 mV in neurons from rats treated with mismatch and antisense ODN. B, Maximum conductance densities of TTX-resistant sodium currents. In rats treated with antisense ODN, the conductance density of TTX-resistant sodium currents (n = 15 neurons) was significantly smaller compared with rats with mismatch ODN treatment (n = 15 neurons). *p < 0.05.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results obtained in this study indicate that intrathecal Na_v1.8 antisense ODN treatment reduced TTX-resistant sodium channelNa_v1.8 expression in lumbosacral DRG neurons as well as the TTX-resistantsodium conductance in bladder afferent neurons. The treatmentalso suppressed bladder hyperactivity and c-fos expression inthe spinal cord induced by chemical irritation of the urinarybladder. Because the ICIs during cystometry under urethane anesthesiain mismatch ODN-treated rats were not different from those inuntreated rats reported in our previous studies (Ozawa et al.,1999), inhibitory effects of antisense ODN on bladder pain responsesare not likely to be caused by toxic or nonspecific effects ofrepeated injections of ODN. This is also supported by previousstudies (Porreca et al., 1999), which revealed that intrathecalinjections of the same sequence of Na_v1.8 antisense ODN producedonly a transient depression of the allodynia and hyperalgesiainduced in rats by sciatic nerve injury. Thus it is assumed thatNa_v1.8 channels are involved in sensitization of bladder afferentnerves induced by noxious stimuli and that suppression of Na_v1.8channels could be a new modality for the treatment of painfulbladder symptoms and/or bladderhyperactivity.

Previous studies demonstrated that TTX-resistant sodium channels are responsible for action potentials in a subpopulationof afferent neurons (Elliott and Elliott, 1993; Ogata and Tatebayashi,1993, Arbuckle and Docherty, 1995; Yoshimura et al., 1996). TheTTX-resistant sodium channel (Na_v1.8) has been cloned from ratDRG neurons, and the expression of these channels is confinedto the capsaicin-sensitive, small-sized DRG neurons (Arbuckleand Docherty, 1995; Akopian et al., 1996; Sangameswaran et al.,1996; Dib-Hajj et al., 1998; Waxman et al., 2000). It has alsobeen documented that TTX-resistant sodium channels are presentin central axon terminals of afferent nerves (Novakovic et al.,1998) and participate in action potential initiation in slow-conductingC-fiber afferents (Jeftinija, 1994; Gu and MacDermott, 1997).

Our previous studies revealed that most bladder afferent neurons exhibit TTX-resistant sodium currents and action potentialsand are capsaicin-sensitive (Yoshimura et al., 1996; Yoshimura,1999; Yoshimura and de Groat, 1999). In addition, most (>95%)of the capsaicin-sensitive bladder afferent neurons from normalrats were the C-fiber type (unmyelinated) that did not stain withantibodies for the 200 kDa subunit of neurofilament (Yoshimuraet al., 1998). The latter marker is specifically expressed inDRG neurons with myelinated axons (Lawson et al., 1993). Onlya small proportion (5%) of neurofilament-positive, myelinatedA $delta$ -fiber bladder afferent neurons are sensitive to capsaicin (Yoshimuraet al., 1998). Thus, it is likely that bladder afferent neuronsthat predominantly express TTX-resistant sodium currents are capsaicin-sensitiveC-fiberneurons.

The present study showed that treatment with Na_v1.8 antisense ODN, which decreased expression of Na_v1.8 channel protein inDRG neurons and reduced the TTX resistant sodium conductance inbladder afferent neurons, suppressed the nociceptive responsesinduced by chemical irritation of the bladder. This anti-nociceptiveeffect in Na_v1.8 antisense-treated rats is similar to that observedin previous studies in rats in which C-fiber bladder afferentswere desensitized by pretreatment with systemic capsaicin (Maggiet al., 1992; Yu and de Groat, 1999). Therefore, it is reasonableto assume that activation of bladder nociceptors and/or nociceptiveinput to the spinal cord is dependent on activation of Na_v1.8channels in C-fiber bladder afferentnerves.

The present study also demonstrated that, in addition to nociceptive mechanisms, Na_v1.8 channels are likely to be involvedin activation of mechanosensitive afferents induced by non-noxiousbladder distension. This conclusion is based on the finding thatantisense treatment increased the ICIs during control cystometrywhen saline was infused into the bladder. Previous studies revealedthat systemic capsaicin pretreatment produced a similar increasein ICIs or bladder capacity, or both, in urethane-anesthetizedrats (Santicioli et al., 1985; Yu and de Groat, 1999), indicatingthat activity in C-fiber bladder afferents modulates reflex voiding.This is consistent with the reports that some C-fiber bladderafferent fibers in rats are not only nociceptive, but also mechanosensitive(Sengupta and Gebhart, 1994; Dmitrieva and McMahon, 1996).

Various evidence has indicated that alterations in sodium channel expression in afferent neurons contribute at least in partto neuronal hyperexcitability after nerve injury. For example,in an animal model of neuropathic pain induced by sciatic nerveligation, the redistribution and accumulation of Na_v1.8 sodiumchannel protein from DRG cell bodies to nerve fibers proximalto the injury site have been implicated as an important mechanismfor ectopic discharges of injured nerves. Under the same conditions,the level of Na_v1.8 mRNA in DRG neurons was not altered (Novakovicet al., 1998). A recent study (Porreca et al., 1999) providedfurther support for this idea by demonstrating that Na_v1.8 antisensetreatment that reduced the level of Na_v1.8 channel protein inDRG neurons suppressed hyperalgesia in the same neuropathic painmodel. However, in another model of neuropathic pain induced bysciatic nerve transection (axotomy), TTX-resistant sodium currentswere significantly reduced in small-sized DRG neurons along withthe reduction in the level of Na_v1.8 mRNA and protein expression.In concert with the reduction in TTX-resistant sodium channelexpression, TTX-sensitive sodium channel expression was upregulated(Black et al., 1999; Waxman et al., 2000). A similar increasein TTX-sensitive sodium channels and decrease in TTX-resistantsodium channels occurred in bladder afferent neurons in spinalcord injured rats that exhibited bladder hyperreflexia (Yoshimuraand de Groat, 1997). Because TTX-sensitive sodium channels areactivated at lower thresholds (Elliott and Elliott, 1993; Ogataand Tatebayashi, 1993; Yoshimura et al., 1996; Yoshimura and deGroat, 1997), a switch in sodium channel expression from TTX-resistantto TTX-sensitive types would be expected to contribute to thephenotypic changes in bladder afferent neurons after spinal cordinjury (Yoshimura and de Groat, 1997; Yoshimura, 1999) or theincreased excitability in injured DRG neurons in an axotomy-inducedneuropathic pain model (Black et al., 1999; Waxman et al., 2000).Therefore, plasticity in TTX-resistant and -sensitive sodium channelsmight contribute to sensory and reflex changes in various pathophysiologicalconditions.

An involvement of Na_v1.8 sodium channels has also been implicated in the hyperalgesia induced by tissue inflammation. In ratmodels of inflammatory pain induced by carrageenan injection intothe hindpaw, Na_v1.8 expression in DRG neurons increased alongwith an increase in TTX-resistant sodium current amplitude (Tanakaet al., 1998). It has also been reported that pretreatment withNa_v1.8 antisense ODN suppressed prostaglandin E₂ (PGE₂)- and completeFreund's adjuvant (CFA)-induced hyperalgesia in the hindpaw ofrats (Khasar et al., 1998; Porreca et al., 1999). PGE₂ is knownto be a chemical mediator that can induce changes in the voltagedependence of TTX-resistant sodium channels, resulting in hyperexcitabilityof DRG neurons (England et al., 1996; Gold et al., 1996). In addition,Na_v1.8 knock-out mice that lack functional Na_v1.8 channels exhibitedanalgesia to noxious mechanical stimuli and reduced inflammatoryhyperalgesia (Akopian et al., 1999). Thus it seems likely thatNa_v1.8 channels are involved at least in part in the developmentof inflammatory pain in somatic afferentpathways.

We have reported previously that chronic bladder inflammation induced hyperexcitability of capsaicin-sensitive C-fiber bladderafferent neurons (Yoshimura and de Groat, 1999). Although neuronalhyperexcitability in this visceral pain model seemed to be relatedto the reduction in potassium channel expression in the afferentneurons, the firing of hyperexcitable C-fiber bladder afferentneurons was still dependent on TTX-resistant sodium channels.Thus, the TTX-resistant sodium channel Na_v1.8 could be a targetfor treatment of inflammatory pain in visceral organs such asthe urinarybladder.

In the present study, Na_v1.8 antisense treatment did not completely suppress bladder hyperactivity induced by bladder irritation.This is probably attributable to incomplete suppression of Na_v1.8channel protein in DRG neurons after antisense treatment, as revealedby ~50% reduction in Na_v1.8 staining intensity in small- to medium-sizedDRG neurons from antisense-treated rats. However, an alternativeexplanation could be the presence of another type of TTX-resistantsodium channel (Na_v1.9 or NaN/SNS2), which is expressed in capsaicin-sensitive,small-sized DRG neurons (Dib-Hajj et al., 1998; Tate et al., 1998).Na_v1.9 sodium channels are reportedly upregulated in a chronicinflammatory condition induced by CFA injection into the rat hindpaw(Tate et al., 1998; Waxman et al., 2000). On the other hand, Na_v1.9channels are not likely to contribute to the development of neuropathicpain because antisense treatment that reduced the expression ofNa_v1.9 channel protein in DRG neurons did not change the behavioralresponses in nerve-injured rats (Porreca et al., 1999).

The relative contribution of the two types of TTX-resistant sodium channels (Na_v1.8 and Na_v1.9) to bladder sensory mechanismscan only be inferred from indirect evidence. Studies by otherinvestigators (Fjell et al., 1999, 2000) revealed that the twotypes of TTX-resistant channels were expressed in different typesof C-fiber afferent neurons: (1) Na_v1.8 in peptidergic, isolectinB4 (IB4)-negative neurons and (2) Na_v1.9 in nonpeptidergic, IB4-positiveneurons. We and other investigators (Bennett et al., 1996; Yoshimura,2001) found that IB4 staining was present in a smaller numberof bladder afferent neurons (10-20%) than in somatic afferentneurons (40%) innervating skin or striated muscles. Thus, it seemslikely that Na_v1.8 channels are more important than Na_v1.9 channelsin bladder nociceptivemechanisms.

In conclusion, the present study provides the first evidence that Na_v1.8 sodium channels are involved in sensitization ofC-fiber bladder afferents and in the triggering of nociceptiveresponses. It has been well documented that tissue inflammationin visceral organs can induce C-fiber afferent hyperexcitability,which contributes to painful sensations as well as hyperactivityof the inflamed visceral organs (Häbler et al., 1990; Senguptaand Gebhart, 1994; Dmitrieva and McMahon, 1996; Lazzeri et al.,1996, 2000; Yoshimura and de Groat, 1999). Therefore, the Na_v1.8TTX-resistant sodium channel could be a new target for the treatmentof chronic visceral painful disorders such as interstitialcystitis.

  FOOTNOTES

Received June 27, 2001; revised Aug. 14, 2001; accepted Aug. 21, 2001.

This work was supported by grants from the National Institutes of Health (DK 49430 and DK 57267) and the Spinal Cord ResearchFoundation, Paralyzed Veterans of America (1861-01/02).
Correspondence should be addressed to Dr. Naoki Yoshimura, Departments of Urology and Pharmacology, University of PittsburghSchool of Medicine, Kaufmann Medical Building, Suite 700, 3471Fifth Avenue, Pittsburgh, PA 15213. E-mail: nyos{at}pitt.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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