Functional Interactions between Tumor and Peripheral Nerve: Changes in Excitability and Morphology of Primary Afferent Fibers in a Murine Model of Cancer Pain

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The Journal of Neuroscience, December 1, 2001, 21(23):9367-9376

Functional Interactions between Tumor and Peripheral Nerve: Changes in Excitability and Morphology of Primary Afferent Fibers in a Murine Model of Cancer Pain
David M. Cain¹, Paul W. Wacnik², Michelle Turner⁴, Gwen Wendelschafer-Crabb³, William R. Kennedy³, George L. Wilcox², and Donald A. Simone¹^,⁵
Departments of ¹ Oral Science, ² Pharmacology, ³ Neurology, ⁴ Neuroscience, and ⁵ Psychiatry, University of Minnesota, Minneapolis, Minnesota 55455

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We used a murine model to investigate functional interactions between tumors and peripheral nerves that may contribute topain associated with cancer. Implantation of fibrosarcoma cellsin and around the calcaneus bone produced mechanical hyperalgesiaof the ipsilateral paw. Electrophysiological recordings from primaryafferent fibers in control and hyperalgesic mice with tumor revealedthe development of spontaneous activity (0.2-3.4 Hz) in 34% ofcutaneous C-fibers adjacent to the tumor (9-17 d after implantation).C-fibers in tumor-bearing mice exhibited a mean decrease in heatthreshold of 3.5 ± 0.10°C. We also examined innervation of theskin overlying the tumor. Epidermal nerve fibers (ENFs) were immunostainedfor protein gene product 9.5, imaged using confocal microscopy,and analyzed in terms of number of fibers per millimeter of epidermallength and branching (number of nodes per fiber). Divergent morphologicalchanges were linked to tumor progression. Although branching ofENFs increased significantly relative to control values, in laterstages (16-24 d after implantation) of tumor growth a sharp decreasein the number of ENFs was observed. This decay of epidermal innervationof skin over the tumor coincided temporally with gradual lossof electrophysiological activity in tumor-bearing mice. The developmentof spontaneous activity and sensitization to heat in C-fibersand increased innervation of cutaneous structures within the first2 weeks of tumor growth suggest activation and sensitization ofa proportion of C-fibers. The decrease in the number of ENFs observedin later stages of tumor development implicates neuropathic involvementin this model of cancerpain.

Key words: tumor; cancer pain; primary afferent fibers; epidermal nerve fibers; murine model; hyperalgesia

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cancer is often accompanied by pain that increases with metastatic infiltration and destruction. The pain is particularlydifficult to treat in advanced stages of the disease and whentumors infiltrate bone or nerve. Improved treatment for cancerpain is dependent on understanding the mechanisms by which tumorgrowth causes pain. To investigate neurobiological mechanismsunderlying cancer pain, we have used a mouse model to investigatefunctional interactions between tumors and peripheral nerve thatmay contribute to cancer-evoked pain and hyperalgesia. This modelis predicated on the implantation of fibrosarcoma cells into theC3H strain of mouse (Schwei et al., 1999; Honore et al., 2000a,b;Wacnik et al., 2000). Implantation of tumor-inducing cells intothe intramedullary space of the mouse femur produces a bone cancermodel that compares well with aspects of human bone cancer, e.g.,increased osteoclast activity preceding bone destruction and hyperalgesiathat is attenuated by morphine. Pathological cellular effectsof metastatic bone destruction in the spinal cord include hypertrophyof astrocytes, increased internalization of the substance P receptor,increased expression of c-fos protein in lamina I of the spinalcord after non-noxious palpation of the bone and deep tissuesin tumor-bearing mice, and increased expression of the prohyperalgesicopioid peptide dynorphin in the deep spinal laminae ipsilateralto the side of bone destruction (Schwei et al., 1999; Honore etal., 2000a,b). Because pain in human patients with bone cancertends to increase in relation to bone destruction induced by osteoclastactivity (Clohisy and Ramnaraine, 1998), inhibition of osteoclast-mediatedbone resorption diminishes pain-related behaviors by halting osteoclastdevelopment and activation (Honore et al., 2000b).

In the companion paper in which a similar model was used (Wacnik et al., 2001), implantation of tumor-inducing cells in andaround the calcaneus bone produced osteolysis and cutaneous mechanicaland cold hyperalgesia. It was also shown that endothelin-1 (ET-1),which is known to cause nociceptive behavior and excite primaryafferent fibers (Davar et al., 1998; Fareed et al., 2000), isreleased from the fibrosarcoma. We hypothesized that enhancedexcitability would occur in C-fibers because tumors produced anincrease in internalization of substance P receptors in spinalneurons (Schwei et al., 1999), and most of the substance P releasedin the spinal cord is from small-caliber afferent fibers (Mantyhet al., 1995; Allen et al., 1997, 1999). In addition, growth factors(Bonetti et al., 1997; Tsujino et al., 1997) released from tumorsor physical properties associated with tumors, such as compression,may result in structural modification of nerve fibers leadingto abnormal activity. We reasoned that either proliferation ofnerve fibers, particularly unmyelinated endings, or nerve degenerationwould contribute to increased excitability. We therefore quantifiedthe effects of tumor development on epidermalinnervation.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects
A total of 113 adult (>6 weeks old) male C3H mice weighing 20-29 gm were used. Because the cell line (NCTC clone 2472) usedto induce tumors in the mouse cancer pain model was derived fromC3H mice, this strain is optimally tumorigenic. Animals were obtainedfrom the National Institutes of Health, housed on a 12 hr light/darkschedule, and given ad libitum access to food and water. All animalprocedures were approved by the Animal Care Committee of the Universityof Minnesota, and experiments were conducted according to theguidelines set forth by the International Association for theStudy ofPain.

Implantation techniques
Mice were placed in an enclosed chamber and anesthetized with halothane in preparation for cell implantation. When the animaldemonstrated nonresponsiveness to paw pinch, it was removed fromthe chamber and fitted with a facemask that continuously delivered1-2% halothane in an air/oxygen mixture throughout the surgery.The level of anesthesia was monitored throughout the procedureby responsiveness to paw pinch to ascertain satisfactory depthof anesthesia. Mice showing signs of permanent motor dysfunctionafter tumor implantation wereeuthanized.
NCTC clone 2472 connective tissue cells were obtained from American Type Cell Culture and maintained as described previously(Clohisy et al., 1996). The cells were grown to confluence in75 cm² flasks in NCTC 135 medium, pH 7.35, 10% horse serum, and passedone time weekly by a 1:4-6 split ratio. Cells were prepared forimplantation by first pouring off the medium and rinsing withPBS. Trypsin was then added for 5-10 min to detach cells fromthe flask and create a single-cell suspension. The enzymatic actionwas stopped with a sufficient volume of the appropriate culturemedium. The cells were then counted with a hemacytometer, pelleted,resuspended, rinsed in PBS, pelleted a second time, and resuspendedin PBS for implantation in a concentration of 2 × 10⁵ cells/10 µl.
Cells were injected unilaterally into and around the calcaneus bone in a volume of 10 µl. Injection required the single useof a 0.3 cc insulin syringe, whereupon the syringe was used bothto bore through the calcaneus bone (proximal to distal) and injectthe cells as the needle was withdrawn. This implantation protocolwas derived from a femur skeletal metastasis model that has beenused to study the cellular and biochemical mechanisms mediatingbone destruction at the tumor site (Clohisy et al., 1996).

Behavioral studies: measurement of hyperalgesia
To ensure that all mice with tumor used in the electrophysiological studies were hyperalgesic, withdrawal responses evokedby a von Frey monofilament (3.4 mN bending force) were obtainedfrom the hindpaw of each animal. Mice were placed on a wire meshplatform, covered with a hand-sized container, and allowed toacclimate to their surroundings for a minimum of 30 min beforetesting. The von Frey monofilament was applied to the plantarsurface of the hindpaw at random locations. Withdrawal responsefrequency was measured from 6-10 trials. For each trial, the filamentwas applied at 1-5 sec intervals. Withdrawal response frequencieswere obtained for 3 d before tumor cell implantation and at variousdays after implantation. Mechanical hyperalgesia was defined asan increase in withdrawal frequency at least two SDs greater thanthe SD of the baseline mean. For electrophysiological study, wefurther restricted selection of mice with tumor to those animalsthat exhibited a withdrawal frequency $>=$ 80% for at least 2 consecutivedays.

Electrophysiological studies
Electrophysiological recording from primary afferent fibers. A total of 86 mice were used in electrophysiological experiments(control, n = 42; mice with tumor, n = 44). Of the mice with tumor,only those determined to be hyperalgesic to mechanical stimuliwere used. Animals were sedated with acepromazine maleate (20mg/kg, i.p.) and anesthetized with sodium pentobarbital (Nembutal,48 mg/kg, i.p.). Supplemental doses of sodium pentobarbital (15mg/kg) were given as needed to maintain areflexia. Hair was removedfrom one hind limb and an incision was made on the dorsal aspectof the lower leg in the skin overlying the tibial nerve. Afterthe gastrocnemius muscle was surgically removed, the skin wassutured to a metal ring (inner diameter 1.3 cm) to form a basinthat was filled with warm mineral oil. The tibial nerve was dissectedfrom connective tissue and placed on a small, mirrored platformfor separation of nerve fibers. To prevent leakage of oil fromthe recording basin, a rubber-based polysulfide impression material(COE-FLEX, GC America Inc.) was applied externally around thering to the skin of the hind limb and allowed to set for ~20 minto form a hard seal. The epineurium of the tibial nerve was openedusing a miniature scalpel, and small fascicles were cut to allowthe proximal ends to be spread out on the platform for separationwith fine jewelersforceps.
Nerve fascicles were teased apart, and fine filaments were placed on a silver-wire recording electrode maneuvered by a micromanipulator.Extracellular recordings were obtained only from single fibersthat could be easily discriminated according to amplitude andshape. Action potentials were amplified, audio monitored, displayedon an oscilloscope, and stored on a VCR before being sent to aPC computer for data acquisition. Evoked responses were analyzedoff-line using a customized data analysis program (LabVIEW, version5.1). An amplitude window discriminator was used to separate actionpotentials of the fiber under study from those of other fibersand from background noise. However, recordings typically consistedof one afferentfiber.
Identification of primary afferent fibers. The receptive fields (RFs) of cutaneous afferent fibers were identified using mechanicalstimuli. Mechanical stimulation proceeded by a graduated approachbeginning with large and soft stimulation with a cotton swab orthe experimenter's fingers, followed by mild pinching with curvedserrated forceps. Once a fiber was isolated, the location of itsRF was identified using a small glass probe (1 mm diameter) ora suprathreshold von Frey monofilament, or both. The RF locationwas then marked on the skin with a felt-tip pen and reconstructedon a drawing of the mousehindpaw.
Conduction velocity. By electrical stimulation of the RF of each isolated fiber, the conduction latency and distance of actionpotentials between the RF and the recording electrode were determinedfor calculation of conduction velocity. Two fine needle electrodes(30 gauge) were inserted into the skin on opposite sides adjacentto the RF. Square-wave pulses (duration 0.2 msec, 0.5 Hz) weredelivered at a stimulating voltage 1.5 times the voltage requiredto evoke a threshold response. Average conduction latencies werepreviously obtained from compound action potentials so that fiberswith conduction velocities $>=$ 1.3 m/sec were classed as myelinatedand subdivided into A $delta$ -fibers (1.3-13.6 m/sec) and A $beta$ -fibers (>13.6m/sec). Fibers with conduction velocities <1.3 m/sec were identifiedas C-fibers.
Mechanical stimulation. To ensure that recordings were obtained exclusively from fibers innervating cutaneous RFs rather thanfrom deeper units innervating muscle, the skin surrounding theRF was gently grasped with curved forceps and lifted. Only fibersthat discharged primarily while the skin around the RF was liftedabove the underlying tissue and lightly squeezed were consideredto be cutaneous units. At the time of unit isolation, toes andjoints were manipulated to identify proprioceptive units, whichwere not studied further. Individual fibers were classed accordingto general response properties, including conduction velocity,waveform, and response to gradations of various mechanical stimulisuch as light stroking with cotton swab and applied pressure witha round-tipped glass rod. Mechanical thresholds were determinedusing calibrated von Frey monofilaments (Stoelting) and were expressedas the minimum force (in milliNewtons) needed to evoke a responsein at least 50% of the trials. The range of von Frey filamentsused in this study exerted bending forces from 0.1 to 177.5 mN.Low-threshold mechanoreceptors (A $beta$ fibers) were identified aseither rapidly adapting (RA) or slowly adapting (SA) by applyingconstant force using a suprathreshold von Frey monofilament (73mN bending force) that was secured to a microdrive and manuallylowered onto the RF for 10sec.
Thermal stimulation. Thermal stimuli were delivered by a Peltier-type thermode controlled by a customized software program.Heat stimuli ranging from 35 to 51°C were presented in ascendingsteps of 2°C from a base temperature of 32°C. Each stimulus wasapplied for 5 sec duration with an interstimulus interval of 60sec. The rise and fall of each thermal stimulus presented was20°C/sec. After a period of at least 5 min, cold stimuli (eachof 10 sec duration) were presented in descending increments of4°C from 28°C to $-$ 12°C and were applied with a ramp rate of 5°C/sec.An interstimulus interval of 160 sec occurred between each incrementof coldstimulation.
The relatively large contact area of the thermode (contact area 1 cm²), which was attached to a manipulator, facilitated a firm contactwith the RF. For A $delta$ - and C-units, the thermode was lowered ontothe RF exerting pressure just sufficient to elicit a response,thus assuring the proper angle and position of the thermode overthe RF. Then, the thermode was delicately adjusted (by manipulator)until the mechanically induced response ceased yet a visible indentationof the skin wasmaintained.
Fiber classification. The procedure used to classify mouse primary afferent fibers has been described previously (Cain etal., 2001). Briefly, mechanoreceptors were considered RA if theyexhibited an abrupt response to the onset (and offset) of mechanicalstimuli but failed to maintain discharge during the 10 sec trial.SA mechanoreceptors were those that discharged throughout the10 sec period ofstimulation.
Nociceptors were characterized according to responses evoked by noxious mechanical, heat, and cold stimuli. In the absenceof a response to the applied range of thermal stimuli, A $delta$ andC nociceptors were classed as mechanonociceptors (AM and CM, respectively).Nociceptors excited by heat, but not cold, were classed as mechanoheatnociceptors (AMH, CMH), and those responding to cold but not heatwere classed as mechanocold nociceptors (AMC, CMC). Nociceptorsexcited by both types of thermal stimuli, mechanoheat/mechanocoldnociceptors, were designated AMHC or CMHC. AMH nociceptors exhibitingresponse thresholds $<=$ 51°C were subclassed as AMH type II fibers.Those A $delta$ nociceptors not responsive during initial heat trialswere exposed (up to three times) to 53°C for 30 sec to inducesensitization to heat. If these nociceptors subsequently respondedto heat, they were classified as AMH type I (Meyer et al., 1985;Treede et al., 1992).

Studies of epidermal innervation
Twenty-seven C3H mice (11 control, 16 hyperalgesic mice with tumor) were used to identify possible effects of tumor growthon density and branching of epidermal nerve fibers (ENFs). Afterinjection with pentobarbital (60 mg/kg, i.p.), a punch biopsywas obtained from the skin overlying the heel of the left hindpaw and fixed in Zamboni's solution (2% paraformaldehyde, 0.2%picric acid in PBS, pH 7.6, for 24 hr at 4°C, then cryoprotectedin 0.1 M PBS, pH 7.4, containing 20% sucrose and stored at 4°Cuntil furtherprocessing.
Biopsies were sectioned at 30 µm and washed free-floating in PBS with 0.3% Triton X-100 and 5% normal donkey serum (NDS) for1 hr, then incubated in primary antisera overnight at 4°C. Rabbitantisera to protein gene product (PGP) 9.5 (Ultraclone, Isle ofWight, UK) and goat antisera to type IV collagen (Southern BiotechnologyAssociates, Inc., Birmingham, AL) were used. All primary antibodieswere diluted in PBS with 0.3% Triton X-100 and 1% NDS. The followingday the sections were washed three times with the same dilutingsolution and incubated with donkey anti-rabbit antibodies conjugatedto Cy-3 and donkey anti-goat antibodies conjugated to Cy-2 (JacksonImmunoResearch, West Grove, PA; 1:200) overnight at 4°C. Afteradditional rinses in the diluting solution, sections were adheredto coverslips with 1% Nobel agar (Sigma, St. Louis, MO), dehydratedin ethanol, cleared in methyl-salicylate, and mounted on slideswith DPX (Fluka, Buchs, Switzerland). Fluorescent samples wereviewed with an epifluorescence-equipped Nikon Microphot-SA microscopeusing appropriate filters. Selected sections were imaged witha CARV non-laser Confocal Microscope System (ATTO Instruments,Rockville, MD). Images were collected in successive frames of1 µm serial optical sections (Z-series) through the thicknessof the sections using a 40× oil Zeiss plan apochromat objective(numerical aperture 1.3). Each Z-series of images was either projectedinto a single in-focus image and printed with a Kodak ColorEasethermal dye diffusion printer or used as a Z-series for quantificationof nervefibers.
Quantitative analyses of ENFs were conducted as described previously (Kennedy et al., 1996). The number of ENFs and nodesper fiber in epidermal images was counted using a 40× objectivewith a Nikon Microphot-SA fluorescent microscope. Epidermal innervationwas evaluated from Z-series stacks of PGP 9.5-immunostained ENFs,and the images were analyzed with Neurolucida software (MicroBrightfield,Colchester, VT) by tracing nerve fibers in three dimensions. IndividualENFs were counted after they passed through the basement membraneso that branching occurring within the epidermis did not increasethe number of ENFs counted. Fiber counts per millimeter lengthof epidermis were standardized for section thickness (25 µm) andexpressed as the number of fibers per millimeter ofepidermis.

Data analyses
Electrophysiology. Action potentials and discriminated spikes were stored on videotape and on a laboratory computer for off-lineanalysis. Thermal stimuli, including ascending and descendingramps and the time at which they were reached, were also digitizedand stored. An additional channel stored a digitized trace ofvoltage from a footswitch used to identify the time of mechanicalstimulation for characterization of rapidly and slowly adaptingresponses.
Differences in mechanical threshold among fiber types were determine using the Kruskal-Wallis ANOVA and Mann--Whitney U tests.The responses of A $delta$ - and C-fibers to thermal stimuli were analyzedon the basis of the number of impulses and the frequency, i.e.,discharge rate (from first to last evoked impulse) evoked by eachstimulus. The LabVIEW software files were reviewed for each thermalstimulus trial. To obtain the discharge frequency, the exact numberof spikes was divided by the time difference between the firstspike and the last spike in response to each thermal stimulus.The mean was computed from the discharge frequency totals obtainedfor each temperature stimulus for either A $delta$ - or C-fibers. Frequencycould not be calculated for responses consisting of a single impulse.Differences in response thresholds for heat and cold between fibertypes were analyzed using a one-way ANOVA and Newman-Keuls posthoc comparisons. Responses of C-fibers evoked by suprathresholdheat stimuli were analyzed by within-and-between-subjects ANOVAperformed on the log of spikes + 1 to homogenizevariability.
Morphology. The Mann-Whitney rank sum test was used to assess whether the number of ENFs per millimeter length of epidermisand the branching (nodes per fiber) differed significantly. $chi$ ² tests were used to determine the proportion of ENFs having nobranching, one node per fiber, or two or more nodes per fiber.A probability of <0.05 was considered significant for statisticalcomparisons.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

As shown in a related study in this issue (Wacnik et al., 2001), the fibrosarcoma tumor caused progressive destruction ofthe calcaneus bone. Hematoxylin and eosin staining showed thatby post-implantation day 6 (PID 6) the edge of the calcaneus bonewas irregular, and bone had deteriorated with tumor progression.Also, there was no indication that tumor cells invaded skin ornerve up to PID 12. Results showed a continuous progression intumor diameter from day 3 (4 mm) to day 10 (4.5 mm), whereuponthe rate increased and by day 15 heel width reached an average5.5 mm (naive width 3.3 mm) and maximal width of 8.2 mm in mice>PID20.

Hyperalgesia in mice with tumors

Sarcoma tumor cell implantation into the heel of 125 C3H/He mice was associated with mechanical hyperalgesia beginning PID7. Mechanical hyperalgesia was measured using a von Frey monofilamentwith a bending force of 3.8 mN applied to the plantar surfaceof the hindpaw. The hyperalgesia developed with tumor growth fromPID 6 through PID 15. In control mice, the frequency of withdrawalfrom the von Frey filament was 10-20%, whereas the comparablevalues in tumor-bearing mice were 80-100%.

Responses of primary afferent fibers

Recordings were obtained in the present study from a total of 190 primary afferent fibers, all of which were excited by mechanicalstimuli applied to RFs located on glabrous skin. In control mice,84 fibers were studied, of which 30 were identified as C-fibers,21 as A $delta$ -fibers, and 33 as A $beta$ -fibers. Response properties weresimilar to those described in an earlier study of afferent fibersin the mouse tibial nerve (Cain et al., 2001). In addition, 106fibers were isolated in mice with tumor, 50 were identified asC-fibers, 26 as A $delta$ -fibers, and 30 as A $beta$ -fibers. All of the C-fibersin mice with tumor were recorded at PID 8-17, except for one eachat PID 19 and 20. Both A $delta$ - and A $beta$ -fibers in mice with tumor werealso evenly distributed between PID 8 and PID 17, and one A $beta$ -fiberwas recorded at PID 21. Fibers that were completely tested withheat and cold stimulation paradigms were further grouped accordingto temperature sensitivity (Table 1).


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Table 1. Response characteristics of primary afferent fibers

Spontaneous activity

Unlike C-fibers in control mice in which none of the 30 C-fibers exhibited ongoing activity, 34% (17 of 50) of C-fibers inmice with tumor discharged action potentials spontaneously. Ratesof spontaneous activity ranged from ~0.2-3.4 Hz with a mean rateof 1.2 Hz ± 0.24 Hz. The peak discharge, the maximal rate of dischargeof a fiber based on the shortest time interval between two actionpotentials, was 28.2 Hz. Figure 1 illustrates the ongoing activityof three C-fibers (A, B, and C) accompanied (see below) by threesuperimposed traces verifying the constant response latency usedto determine the conduction velocity of the fiber. Some C-fibersin mice with tumor displayed an intermittent bursting patternof spontaneous activity (Fig. 1C).

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Figure 1. Representative examples of spontaneous activity and conduction latency of three C-fibers recorded in skin overlying a fibrosarcoma tumor. A, Top, Spontaneous activity of this nociceptor occurred generally at a steady rate of ~1 Hz. A, Bottom, Three superimposed oscilloscope traces showing constant conduction latency evoked by electrical stimulation at the RF. B, A second C-fiber with a slower (0.15 Hz) rate of spontaneous activity. C, Spontaneous activity of this nociceptor occurred in bursts of three to five action potentials. Arrows indicate stimulus artifact. The 10 sec calibration below the spontaneous activity in C applies to all three traces of ongoing activity. Calibrations of individual conduction latencies are shown under the overlaid traces of constant conduction velocity.

The presence of spontaneous activity, in addition to being limited to C-fibers in mice with tumor, increased with tumor progression.Logistic regression analysis indicated that ongoing activity,which was observed first in 33% (1 of 3) of C-fibers at PID 9,peaked significantly at 83% (5 of 6) of the C-fibers recordedat PID 17 (p < 0.033). When the percentage of C-fibers with spontaneousactivity was calculated as a function of day after implantation,82% (14 of 17) of such fibers were found to occur in the rangeof PID 13-17. Among later PID mice, electrophysiological responsivenessof all types of primary afferents in the nerve decreased sharply,thus making the isolation of single fibers difficult, and thisphysiological change coincided with the onset of the disappearanceof ENFs as reported below (see Morphology of epidermal nervefibers).

There was no obvious relationship between specific characteristics of the spontaneous activity and the functional class ofC-fiber. Among the spontaneously active fibers, one was classedas CM, one as CMC, five as CMH, and four as CMHC. The functionalclasses of the other six spontaneously active C-fibers were notcompletely identified; however, all responded to mechanicalstimuli.

The RFs of spontaneously active C-fibers were generally located in close proximity to the tumor, specifically, 88% (15 of17) were on the plantar surface within 2 mm of the visible tumorperiphery, whereas the RFs of two spontaneously active C-fiberswere found on the toes (~3.5 mm from the edge of the tumor). Nospontaneous activity was found between either A $beta$ - or A $delta$ -fibersin thisstudy.

Responses evoked by thermal and mechanical stimuli

Heat thresholds were determined for 18 C-fibers (from 18 mice with tumor) and 17 heat-sensitive C-fibers (from 13 controlmice). Thresholds of C-fibers in mice with tumor were obtainedfrom PID 8 (n = 2; mean 39°C) to PID 17 (n = 1; 35°C). Althoughno correlation was found between heat threshold and PID, the meanresponse threshold of C-fibers to heat was significantly 3.5°Clower (p < 0.01) in mice with tumor (38.3°C ± 0.7; n = 18) relativeto control mice (41.8 ± 1.0; n = 17), as shown in Figure 2. Incontrol mice, 41% (7 of 17) of the C-fibers had response thresholdsbelow 40°C compared with 78% (14 of 18) of the C-fibers in micewith tumor. In addition, responses of C-fibers evoked by suprathresholdheat stimuli (Fig. 3A) were greater in mice with tumor than incontrol mice (p < 0.01), and the number of impulses between controland tumor for stimulus temperatures of 37-49°C showed a significanttemperature-dependent difference (p < 0.01). Thus, sensitizationto heat was manifested as a decrease in response threshold andan increase in number of impulses evoked by suprathreshold heatstimuli. The histogram in Figure 4 differentiates between heatthresholds of non-spontaneously active and spontaneously activeC-fibers in tumor-bearing mice. Although the difference in heatthresholds between control and tumor mice was significant, nodifference occurred between quiescent and spontaneously activeC-fibers in tumor mice. The ranges of response thresholds to heatfor C-fibers without and with spontaneous activity were 35-47and 35-39°C, respectively.

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Figure 2. Mean (±SE) response threshold for heat and cold in control (unfilled columns) and in mice with fibrosarcoma tumors (filled columns). The mean heat threshold of C-fibers in control mice was 41.8 ± 1.09°C compared with 38.3 ± 10.72°C in mice with tumor (p = 0.011). * indicates a significant difference from control. The cold threshold of C-fibers in mice with tumor was 11.2 ± 2.4°C compared with 10.2 ± 2.67°C in control mice.

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Figure 3. Stimulus response curves for C-fibers in control mice ( $open circle$ ) and mice with tumor () indicating mean (±SE) number of impulses in response to thermal stimuli. A, C-fibers discharged a greater number of impulses to heat stimuli 37-47°C in mice with tumor than in control mice. B, No significant difference was observed in C-fiber discharge to cold stimuli between control mice and mice with tumor.

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Figure 4. Mean (±SE) thermal threshold in control mice (black) and nonspontaneously active and spontaneously active C-fibers in mice with tumor. The asterisk (left columns) indicates a significant difference in mean heat thresholds between control and mice with tumor, but thresholds of C-fibers in tumor mice with spontaneous activity did not differ from those without it. Right columns, Neither the presence of tumor nor ongoing activity appeared to have an effect on cold thresholds of C-fibers.

In contrast, the mean cold threshold of C-fibers in mice with tumors (11.2°C ± 2.4; n = 15) compared closely with that ofcontrol mice (10.2°C ± 2.6; n = 14), and no difference in meanresponse threshold was observed. Similarly, responses of C-fibersevoked by suprathreshold cold stimuli, illustrated in Figure 3B,did not differ significantly between control mice and tumor-bearingmice. The histogram in Figure 4 further indicates that no significantdifference in cold thresholds was observed between nonspontaneouslyactive and spontaneously active C-fibers in mice with tumor. Therange of response thresholds to cold was 24C° to $-$ 4C° regardlessof whether the C-fiber was spontaneouslyactive.

In tumor-bearing mice, two heat-sensitive A $delta$ -fibers (AMH type II) had response thresholds of 47 and 43°C, respectively. Theseresponse thresholds are similar to those observed in control mice(Table 1). In addition, the mean threshold of five cold-sensitiveA $delta$ -fibers (AMC) in mice with tumor was 11.2°C ± 6.1 (range, $-$ 8to +28°C) compared with a mean of 3.0 ± 5.7°C from four cold-sensitiveA $delta$ -fibers in control mice. A larger sampling of responses of A $delta$ -fibersto cold reported in a previous study (Cain et al., 2001) founda mean cold threshold of 7.6 ± 3.8°C. Sensitivity of A $beta$ -fibersto heat and cold was nottested.

No significant differences were observed for mechanical threshold of C-fibers and A $delta$ -fibers between control mice and tumor-bearingmice. The median mechanical threshold of C-fibers in control mice(n = 30) was 24.4 mN, and the median mechanical threshold of C-fibersin mice with tumor (n = 50) was also 24.4 mN. The range of thesethresholds was 1.2-177.5 mN (control) and 2.1-111.5 mN in micewith tumor. The median mechanical thresholds of 47 A $delta$ -fibers (21from control mice, 26 from mice with tumor) are stated in Table1. For mice with tumor the median value was 5.2 mN compared with10.4 mN in control mice; however, this difference was not significant.The median mechanical threshold of A $beta$ -fibers in control mice was4.4 mN (range, 0.6-24.4 mN), which compared with a median of 1.18mN (range, 0.27-24.4 mN) in mice with tumor. This difference inmedian mechanical thresholds for A $beta$ -fibers was significant (p= 0.01). Sensitivity of A $beta$ -fibers to heat and cold was nottested.

Tibial nerve afferent fibers in mice with tumor underwent marked change in electrophysiological activity beyond 2 weeks oftumor growth. After PID 17 it became more difficult to recordactivity from individual primary afferents regardless of functionaltype, and by PID 20-24 fiber activity was rarely recorded. Thisdecrease of afferent activity correlated with prodigious tumorgrowth as measured by a maximal heel width of 8.2 mm in mice >PID20 (compared with 3.3 mm in control) and was consistent with degenerationof cutaneous nerve fibers observed in later stages of tumor growth(seebelow).

Morphology of epidermal nerve fibers

The earliest biopsies from mice with tumor were obtained at PID 8 and the latest at PID 24. Confocal images of ENFs in skinbiopsies are provided in Figure 5. These three representativeimages demonstrate the impact of tumor growth from normal (control)condition (left top) through PID 10 (left middle) to PID 24 (leftbottom). The denervation of the epidermis is evident in the latestages of tumor progression, e.g., PID 24 coincided with a substantialattenuation of electrophysiological activity in the tibial nerve.The branching of ENFs, defined as the number of nodes or bifurcationpoints per fiber, was quantified by computer-enhanced tracingsof individual PGP 9.5 immunoreactive fibers from biopsied skinsuperficial to a tumor or from the same heel region in controlmice. Figure 6A indicates a significant increase in ENF branchingin skin of mice with tumor, i.e., 0.27 ± 0.02 nodes per fibercompared with 0.13 ± 0.02 nodes per fiber in control mice (p <0.007).

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Figure 5. Effect of tumor growth on morphology of ENFs. Left panels, Confocal images of glabrous skin biopsies indicating ENFs (green) and basement membrane (BM) and blood vessels (red) from a control mouse (top), a mouse with tumor 10 d after implantation of tumor-inducing cells (PID 10, middle), and a mouse with tumor 24 d after implantation (PID 24, bottom). ENFs in control mouse (top left) show normal innervation with relatively little branching. Within 2 weeks of implantation, increased fiber branching is evident (middle left). After >3 weeks of tumor progression, extensive atrophy results in loss of most ENFs. The scale bar applies to each of the panels. Right three panels, Neurolucida tracings corresponding to the composite image stack of ENFs on the corresponding left panels. Each image stack consists of a Z-series acquired in 1 mm increments throughout the thickness of the section. Note that the standard criterion for quantifying the number of fibers restricted tracings to continuous fibers passing through the basement membrane. Fiber fragments such as some of those seen in the bottom left image, for example, were not quantified. Straight lines approximating the basement membrane underneath ENF tracings (right panels) were used to determine the epidermal length of the image stack for calculation of number of fibers per millimeter of epidermis. Different branches of individual fibers are illustrated by different colors.

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Figure 6. A, Effect of tumor growth on branching of ENFs and on epidermal innervation. Comparison of mean (±SE) branching (nodes per fiber) observed in biopsy images from control mice (0.14 nodes per fiber ± 0.02; n = 60) and mice with tumor (0.27 ± 0.03; n = 117). Significant difference is indicated by asterisk. B, The mean number of fibers per millimeter length of epidermis. The histogram shows a significant (asterisk) decline in the number of ENFs per millimeter of epidermis observed in biopsies from mice with tumor.

In addition to the observation of a greater number of branch points in ENFs of mice with tumors, analysis was also made ofthe proportion of fibers that had a specific number of nodes perfiber in each mouse group. Figure 7 illustrates the proportionof ENFs in control mice and mice with tumors having no branchpoints, one branch point, or two or more branch points. Controlmice had a significantly higher proportion of ENFs having no branching(86 vs 75%; p < 0.01), whereas the percentage of ENFs containingeither one (13 vs 21%; p < 0.01) or two or more (1.5 vs 4%; p< 0.006) branch points was higher in mice with tumor (Fig. 7).

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Figure 7. For control mice and mice with tumor, the proportions of ENFs having no branching, one node per fiber, or two or more nodes per fiber are compared. Fibers having no branching were significantly more abundant in control mice. Conversely, ENFs exhibiting one or more than or equal to two branch points were significantly more prevalent in mice with tumor. Asterisks indicate significant differences among groups.

Conversely, the number of ENFs in mice with tumors declined with tumor growth. The most pronounced reduction of nerve fibersoccurred in the epidermis after PID 16, and indeed some skin associatedwith extensive tumor growth (>PID 20) was completely devoid ofintact fiber innervation in the epidermis. Figure 6B indicatesthe significant change in the number of fibers per millimeterlength of epidermis. Control mice exhibited a mean number of epidermalnerve fibers of 51.3 ± 2.7 compared with only 32.3 ± 1.8 fibersper millimeter length of epidermis in all tumor-bearing mice combinedacross times after implantation (p < 0.007).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neuronal sensitization refers to an increase in excitability characterized by spontaneous activity, lowered response thresholds,and increased response to suprathreshold stimuli, all of whichwere observed in the present study. The most conspicuous differencein the responses of primary afferent fibers in tumor-bearing micewas the high incidence of spontaneous activity in C-fibers. Ongoingactivity in unmyelinated and myelinated nociceptors has been associatedwith nerve injury (Meyer et al., 1985; Ali et al., 1999) or tissueinflammation (Kocher et al., 1987; Andrew and Greenspan, 1999).Clinical and experimental observations implicate spontaneous activityas a probable substrate of persistent neuropathic pain and progressivedegenerative neuropathies (Gracely et al., 1992; Sheen and Chung,1993). In addition, inflammatory pain may be evoked by the releaseof cytokines and growth factors (Woolf, 1996), thereby loweringnociceptor thresholds to the point at which body temperature andpressure of edema become adequate stimuli for excitation (Cesareand McNaughton, 1997; for review see, Sorkin and Wallace, 1999).Spontaneous activity may sustain central sensitization, whichincreases excitability of nociceptive spinal neurons (Cook etal., 1987; Willis, 1992; Woolf, 1992). That the spontaneous activityof C-fibers observed in the present study may be maintaining centralsensitization is consistent with the increased internalizationof substance P receptors in the spinal cord of mice with bonecancer (Schwei et al., 1999; Honore et al., 2000a).

Interestingly, we found no spontaneous activity in myelinated fibers in tumor-bearing mice. Studies involving peripheral nerveinjury in rats report ongoing activity in cutaneous myelinatedfibers (Boucher et al., 2000; Liu et al., 2000) and in fibersinnervating deep tissues (Proske et al., 1995; Michaelis et al.,2000). Recently it has been shown that spinal nerve injury evokesectopic activity originating in the distal terminals of neighboringuninjured C-fibers (Wu et al., 2001). Patterns of spontaneousactivity ranged from regular to bursting, similar to those inthe presentstudy.

Although we found that a proportion of C-fibers in mice with tumor were sensitized to heat, this was not accompanied by adecrease in mechanical threshold. Earlier studies also found thatinflammation or capsaicin lower heat, but not mechanical, thresholdsof C-fibers (Reeh et al., 1986; Kocher et al., 1987; Baumann etal., 1991). Recently, however, sensitization of cutaneous nociceptorsto mechanical stimulation after inflammation was documented usingsuprathreshold mechanical stimuli (Andrew and Greenspan, 1999).In the present study, responses of nociceptors to mechanical stimulithat were above response threshold were not evaluated. We thereforecannot be certain whether mechanical hyperalgesia in this modelis mediated primarily by nociceptor sensitization or by othermechanisms such as the sensitization of second-order sensory neuronsin the spinal cord, i.e., centralsensitization.

The observed decrease of mechanical thresholds for A $beta$ -fibers in mice with tumor may be attributable to stretching of the skinor to changes in compliance of the skin that accompanied tumorgrowth. By PID 24 the maximal size of the heel tumor width measured8.2 mm compared with 3.3 mm in control animals. Thus thresholdchanges of mechanoreceptors might have been induced indirectlyby changes in the mechanical properties of the skin. However,the lowered thresholds of mechanoreceptors might contribute tomechanical hyperalgesia if their activity impinged on sensitizednociceptive dorsal hornneurons.

The mechanisms underlying the spontaneous activity and sensitization of C-fibers in the present model are unknown. Excitabilityof nociceptors can be altered by such well known algogens as prostaglandins,bradykinin, histamine, certain cytokines, and trophic factors(for review, see Wacnik et al., 2000). The companion paper (Wacniket al., 2001) reports elevated release from the tumor of the peptideET-1. This finding is of interest because previous studies haveimplicated ET-1 in the transmission of nociceptive informationin both animals and humans (Raffa et al., 1991, 1996a,b; Davaret al., 1998; Fareed et al., 2000; Piovezan et al., 2000; Pomoniset al., 2001). In addition, it is secreted in high concentrationsby metastatic prostate and breast cancer cells (for review, seeGokin et al., 2001). Levels of ET-1 are also elevated in plasmaof men with prostate cancer (Nelson et al., 1995). Administrationof an ET-A receptor antagonist reduces cancer pain (Carducci etal., 1998) and decreases hyperalgesia in mice with this tumor(Wacnik et al., 2001). This evidence suggests that ET-1 may contributeto the tumor-evoked spontaneousactivity.

Changes in nerve structure and innervation of the epidermis

The most striking morphological effect of tumor growth encountered in this study was the progressive atrophy of ENFs, as indicatedby a loss of immunoreactivity for PGP 9.5, which was measurable2 weeks after implantation of cancer cells. ENFs are unmyelinatedendings that are sensitive to the neurotoxic effect of capsaicinand have been shown to include nociceptors (Simone et al., 1998;Nolano et al., 1999). A particularly interesting finding was thatmice exhibited mechanical hyperalgesia at a time when there wassignificant loss of epidermal innervation. The implication thatdenervation may be associated with pain and hyperalgesia is inagreement with several recent clinical studies. It has been shownthat cutaneous innervation is reduced in several painful sensoryneuropathies (Holland et al., 1997), including diabetes (Levyet al., 1992), human immunodeficiency virus (McCarthy et al.,1995), painful burning feet (Periquet et al., 1999), Fabry disease(Scott et al., 1999), and most recently, in post-herpetic neuralgia(Oaklander et al., 1998; Oaklander, 2001). Oaklander (2001) hasdiscussed possible explanations for the paradox that a decreasein the number of neurons, up to a point, may enhance rather thandiminish nociceptive input. Developments in cancer mice observedin our study, i.e., the presence of ongoing C-fiber activity,increased number of impulses, and lowered response thresholdsto heat stimuli, accompanied ENF degeneration near the tumor siteof hyperalgesic mice >2 weeks after implantation. These changesin response to tissue injury may facilitate increased activationof second-order sensory neurons simultaneous to denervation ofthe skin and thus account for the hyperalgesia observed duringadvanced tumor progression. The loss of ENFs observed in cancermice provides direct evidence that this model of cancer pain hasa neuropathic component, at least in later stages. The persistenthyperalgesia observed despite a reduction in ENFs may be a manifestationof the functional redundancy inherent in nervous systems, wherebynear-normal function can be preserved after neuron injury as longas a certain minimum number of neuronssurvive.

A second morphological feature that occurred after tumor growth was increased branching of ENFs, which represent axonal sproutingat the nociceptive ending. Several studies have considered theeffects of axonal branching on action potential propagation, andthe general conclusion is that action potentials generated inone branch may propagate antidromically into other branches andcollide with action potentials generated there, leading to anocclusion of the action potential signal (Grossman et al., 1973;Stockbridge, 1988; Stockbridge and Stockbridge, 1988; Peng etal., 1999). Although the functional significance of increasedbranching of ENFs is unclear, one possibility is that an increasein branching of nociceptive terminals may add density to the sensorysurface area through proliferation of transduction channels and/orelevated availability of endogenous compounds, such as nerve growthfactor, involved in modulating excitability of nociceptors. Stuckyet al. (1999) showed that mice overexpressing nerve growth factorin skin have a 50% increase in unmyelinated nociceptors in thesaphenous nerve and a substantial increase in the percentage ofC-fibers responsive to heat. This may account in part for spontaneousactivity and sensitization of C-fibernociceptors.

Alternatively, the spontaneous activity coupled with the degenerative changes in ENFs observed in mice with tumor seems tobe consistent with the Wallerian degeneration hypothesis. Thishypothesis was proposed to account for spontaneous activity ofuninjured C-fibers commingling in the sciatic nerve with injuredfibers degenerating as a result of spinal nerve injury (Wu etal., 2001). Nerve injury produced by spinal nerve ligation ortransection may elicit release of substances such as nerve growthfactor from injured fibers that could be transported back to thedorsal root ganglion where novel expression of receptor proteinscould result in increasedexcitability.

Conclusions

A major impediment to understanding mechanisms underlying cancer pain has been the lack of appropriate animal models. Newmurine models of cancer pain are elucidating changes in biochemical,cellular, and physiological responses involved in the generationand maintenance of cancer pain. We show that tumor growth producesphysiological and morphological alterations in primary afferentfibers that are characterized by spontaneous activity, sensitizationof C-fiber nociceptors, and proliferation and subsequent degenerationof ENFs. These findings suggest that the observed behavioral hyperalgesiais mediated in part by sensitization of C-fibers. Furthermore,it is likely that central sensitization also occurs and may bemaintained by spontaneous activity of C-fibers. An understandingof the functional interactions between tumors and peripheral nerves,and the consequences that those interactions have on the CNS,may identify novel targets for development of new therapies forcancerpain.

  FOOTNOTES

Received June 11, 2001; revised Aug. 8, 2001; accepted Aug. 31, 2001.

This work was supported by National Institutes of Health Grants CA91007 and DA11471 (D.A.S.). We thank Dr. Denis R. Clohisyand Margaret L. Ramnaraine for culturing fibrosarcoma cells fortumor induction, Dr. Mona M. Selim for help with quantificationof epidermal nerve fibers, and Dr. Jim Hodges for advice on statisticalanalysis. We also appreciate the comments by Dr. Al Beitz andLaura Eikmeier on an earlier version of thismanuscript.
Correspondence should be addressed to Donald A. Simone, Department of Oral Science, University of Minnesota, 17-252 Moos Tower,515 Delaware Street SE, Minneapolis, MN 55455. E-mail: simon003{at}umn.edu.

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