Innervation Territories of Mechano-Insensitive C Nociceptors in Human Skin

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Innervation Territories of Mechano-Insensitive C Nociceptors in Human Skin

R. Schmidt,¹ M. Schmelz,² C. Weidner,² H. O. Handwerker,² and H. E. Torebjörk¹

¹Department of Clinical Neurophysiology, University of Uppsala, 751 85 Uppsala, Sweden; and ²Department of Physiology and Experimental Pathophysiology, Universitätsstr 17, University of Erlangen/Nürnberg, Germany

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Schmidt, R., M. Schmelz, C. Weidner, H. O. Handwerker, and H. E. Torebjörk. Innervation Territories of Mechano-Insensitive C Nociceptors in Human Skin. J. Neurophysiol. 88: 1859-1866, 2002. Microneurographic recordings were obtained in the peroneal nerve from 20 mechano-insensitive units (CMi) and six mechano-heatresponsive C units (CMH) in healthy human subjects. Their innervationterritories in the skin of the leg or foot were assessed by transcutaneouselectrical stimulation with a pointed probe at intensities of10 to 100 mA (0.2 ms) and, when applicable, by mechanical vonFrey hair stimulation. Electro-receptive fields (eRFs) of CMHunits had a median area of 1.95 cm² when mapped with 10 mA that coincided approximately with mechano-receptivefields (mRFs) as mapped with a 750-mN von Frey hair. Fifty-milliamperestimuli increased the eRFs to 3.08 cm² in a concentric manner. This was probably due to current spreadsince these units are known to have low electrical thresholds.Further increase of the stimulus strength to 70 or 100 mA increasedthe eRFs only marginally. Mechano-insensitive units had much smallereRFs (median: 0.35 cm²) than CMH units when mapped with the same pointed probe at 10mA (n = 13). The receptive territories consisted of one distinctspot or of several spots separated by distances of more than 1cm. However, when mapping stimuli of 50 mA were applied, eRFsbecame continuous and grew to a median area of 5.34 cm², i.e., larger than those of CMHs. The borders of eRFs of CMiunits were significantly more irregular compared with CMH units.A further increase of the stimulus intensity to a maximum of 100mA only marginally enlarged the eRFs. The CMi units could be activatedby heat or chemical substances applied inside the 50-mA eRF, indicatingthat receptive nerve endings were mapped. Responsiveness to thesestimuli was inhomogeneous within the eRFs. It was concluded thatinnervation territories of CMi units in human skin exceed thoseof CMH units in size by a factor of approximately 3. The widelybranched terminals underlying the large fields are consistentwith a role of this nociceptor class in axon reflex flare andpreclude a role in exact spatial discrimination of noxiousstimuli.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

In the last decade, mechano-insensitive C fibers (CMi units) were discovered in human skin (Schmidt et al. 1995). They clearlydiffer from the long known mechano-responsive C-nociceptors (CMHunits) by structural and functional characteristics (Schmelz etal. 2000a,b; Schmidt et al. 2000; Weidner et al. 1999). Thesemechano-insensitive units have been called "sleeping nociceptors"because they are not excited even by von Frey hairs of 750 mNbut become mechano-responsive on inflammation. They have beenshown to play a dominant role for encoding of painful stimulisuch as intracutaneous capsaicin injection and tonic pressureand for induction of primary and secondary hyperalgesia (Schmelzet al. 2000b; Schmidt et al. 2000). Furthermore, they apparentlymediate the axon reflex flare by neuropeptide release from theiraxon terminals on stimulation (Schmelz et al. 2000a) because CMHunits have too small receptive fields (Schmidt et al. 1997) toaccount forit.

The present study is the first quantitative assessment of the innervation territories of CMi units compared with those ofmechano-responsive units. The innervation territories of the latterhave already been assessed in a previous study (Schmidt et al.1997) in which we used electrical stimuli (constant current, 10mA, or constant voltage, 80-100 V) that turned out to be supramaximalfor mechanoresponsive units but insufficient to excite all branchesof mechano-insensitive fibers. For comparing the field sizes ofboth unit classes, we had to increase stimulus intensities inthe present study. Part of this work has been published in abstractform before (Schmidt et al. 1998).

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Subjects

The experiments were performed in 20 healthy human subjects, 14 men and 6 women (age range, 20-32 yr). All subjects gave theirinformed consent according to the Declaration of Helsinki andthe study was approved by the ethics committees of the Universitiesof Uppsala and Erlangen/Nürnberg.

Search for C-fiber responses

Microneurography techniques were employed for recording from cutaneous C fibers in the peroneal nerve, innervating the skinof the lower leg and the dorsum of the foot and toes. The searchprocedure for single C fibers and the mapping of their receptivefields has been described before in detail (Schmelz et al. 1995;Schmidt et al. 1995; Torebjörk and Hallin 1974). Briefly, a tungstenmicroelectrode was inserted into a skin fascicle of the peronealnerve at knee or ankle level. The innervation territory of theimpaled fascicle was identified by multifiber responses of largemechano-receptive fibers to touching the skin. Single transcutaneouselectrical stimuli from an insulated stimulator (0.3-Hz, 0.2-ms,50-mA constant-current pulses, DS7A, Digitimer) were applied withinthe innervation territory of the impaled fascicle via a pointedsteel electrode (1 mm diam), which was moved on the skin untila long-latency C-fiber response was obtained. Two tungsten microelectrodes(0.2 mm diam) were inserted intracutaneously approximately 5 mmapart at the skin site from where the C-fiber response had beenelicited. Pulses of moderate intensity (0.2 ms, 1-20 mA) suprathresholdfor C-fiber activation were then applied through these needlesfor repetitive intracutaneous stimulation. The C-unit responseswere recorded on-line by a PC computer via an interface card (DAP,Microstar) using the SPIKE/SPIDI software package (Forster andHandwerker 1990). Traces triggered by the intracutaneous pulseswere displayed successively from top to bottom on the computerscreen.

Conduction velocity measurements

The latencies of C-fiber responses to the first electrical pulse delivered through the intracutaneous needle electrodes aftera rest period of at least 2 min were used for computing the conductionvelocities. The shortest distance between the stimulating electrodesin the skin and the recording electrode in the nerve was measuredin millimeter. Room temperature was kept constant at 22-24°C throughouttheexperiments.

Classification of C units by the "marking" technique

For subclassification of C fibers, repetitious intradermal stimulation at 0.25 Hz was used. After a minute or so the latenciesof C responses would stabilize at latencies characteristic foreach fiber in a multifiber recording (Torebjörk and Hallin 1974).Activation of a C fiber by additional natural or electrical stimulationwould result in activity dependent slowing of impulse conduction,seen as a transient increase in latency, followed by a slow recoveryafter the end of the stimulus (Fig. 1).

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Fig. 1. The "marking method" used for mapping the electro-receptive field (eRF). A: intracutaneous needles were inserted for regular 0.25-Hz electrical stimulation. Conditioning transcutaneous electrical pulses (pen) delivered in the vicinity of the needles were interposed between regular pulses for mapping the eRF. B: regular pulses through intracutaneous needles within the receptive field every 4 s (stimulus artifacts under straight arrow) evoked responses of the unit at a stable latency. When additional electrical pulses through a surface probe were applied within the eRF, additional action potentials (left curved arrow) were generated causing delayed responses to the regular pulses and a slow recovery (right curved arrow). C: schematic drawing of an electroreceptive field. Fifty-milliampere electrical square wave pulses were applied to the skin through a pointed probe. Points where the unit was activated are marked with filled circles, and points where A was tested but not activiated are marked with open circles.

In this way C units were shown to be afferent by their responsiveness to mechanical, thermal, or chemical stimuli (Torebjörk1974). Sympathetic C fibers could be classified by their activationrelated to sympathetic reflexes caused, e.g., by arousal stimuli(Hallin and Torebjörk 1974). It has been proven in a previousstudy that this "marking" method is sensitive enough to allowdetection of just one extra impulse in a stimulated C fiber (Schmelzet al. 1995). This means that the technique is useful for classificationof C units, for threshold determinations, and for mapping theextensions of the innervation territories. Due to the long conductiondistances (20-50 cm), slight differences in conduction velocitiescaused latency separation of multiple C fibers recorded in oneintraneural site. There was never any ambiguity which unit respondedto a particular stimulus even if two or more units had adjacentor even overlapping innervationterritories.

Determination of mechanical and heat thresholds

A set of calibrated von Frey nylon filaments (Stoelting, Chicago, IL) was used to quantify mechanical thresholds. The forcesexerted by these filaments were 1.5-750 mN (0.8-18 bar; tip diameterof 0.15-0.71 mm). The lowest force that elicited a "marking" responsefrom the receptive field of a unit was regarded as the mechanicalthreshold.

Heat stimuli were delivered from a halogen lamp feedback controlled by a thermocouple attached to the skin (Beck et al. 1974).Skin temperature was increased by 0.25°C/s from an adapting temperatureof 32°C to tolerance level at 50-52°C. The temperature leadingto activation of the unit was noted. Because the electrical stimuliwere delivered every fourth second, a response to heating couldpossibly be overestimated by up to 1°C. In 17/20 CMi units, heatthresholds were measured in two or more spots within the eRF toassess possible variability of thermalresponsiveness.

Responsiveness to chemical stimulation

Histamine (20 mC) or acetylcholine (60 mC) was applied by iontophoresis within receptive fields of CMi units using a standardizedapplicator, 5 mm in diameter (Magerl et al. 1990). For five CMiunits, this application was repeated at different sites withinthe receptive field to assess variability of the response. Forfive CMi units, histamine was also applied outside the 50-mA eRF.The CMH units were not tested with thesesubstances.

Mapping of mechano-receptive fields

The extensions of the mechano-receptive fields (mRFs) were mapped with a stiff von Frey hair of 750 mN. The mRFs were mappedwith stimulation points spaced by about 2 mm. A skin area witha radius of at least 2.5 cm around the intracutaneous needle electrodeswas searched to maintain mapping of the whole mRF in cases ofdiscontinuity. Each point from which mechanical stimuli activatedthe respective C unit was marked on the skin byink.

Mapping of electro-receptive fields

The extension of the electro-receptive fields (eRF) was mapped as described before (Schmidt et al. 1997). For this purpose,the tip of a pointed steel electrode was moistened with sodiumchloride or electrode gel and gently contacted to the skin forpseudo-unipolar electrical stimulation. A metal plate (20 cm²) on the skin more than 10 cm away was used as reference electrode.The stimulation points were spaced by about 2-3 mm. A skin areawith a radius of at least 2.5 cm around the intracutaneous needleelectrodes was searched. After identifying an eRF in this regiona radius of at least 1 cm around, the eRF was searched. Mappingwas performed at 50 mA for all units. For 13/20 CMi units and6/6 CMH units, mapping was also performed at 10 mA. In some cases,70- and 100-mA pulses were also used, if tolerated by the subjects.Each point from which transcutaneous electrical stimuli activatedthe respective C unit was marked on the skin with different colorsfor different current strengths. A complete mapping of eRFs atdifferent intensities could take up to 4 h. Not surprisingly,in many instances the unit was lost during the mapping, due toinvoluntary withdrawal movements or muscle jerks in particularat the higher stimulationintensities.

At the end of an experiment, the marks were transferred to a transparent sheet, and the contours of differently marked mRFand eRF of each unit were scanned into computer for determiningthe areas and circumferences by a dedicated computer program (Dept.Physiology 1, Erlangen). The quotient circumference/square rootof area was calculated to indicate the degree of irregularityor roundness of the eRFs (a figure of maximal roundness, i.e.,a circle, produces a quotient of 3.55, and higher values indicateincreasing degrees of irregularity of the eRFs.)

The maximal diameter for each stimulation intensity was measured. Further we measured the maximal extension of the 50-mA eRFperpendicular to the maximal diameter, the maximal extension inthe proximo-distal direction, and the maximal extension in themedio-lateraldirection.

Location of units

Units were allocated to one of three regions of the cutaneous innervation territory of the peroneal nerve: the dorsum of thetoes except the ungual phalanges and the lateral part of the littletoe, the dorsum of the foot up to the malleoli, and the distallateral half of the lower leg. The upper half of the lower legwas covered by the preamplifier equipment and could not be usedfor recording. Each unit was classified as belonging to one ofthese skinareas.

Statistics

Measures are given as median and range. The data refers to the sample of units studied for the present work. However, we havea large sample of characterized units that have already been publishedin studies focusing on other questions. For the general propertiesof C fibers, like conduction velocity or receptive thresholds,and for eRFs of CMH units, an average of all fibers studied todate is provided in addition (indicated by running average, RA).Differences were tested by the Mann-Whitney U test or the Wilcoxontest for paired samples as stated in the text. Probability levelswere regarded significant at P < 0.05.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Sample of C units

A total of 26 C units were mapped. Six of them responded to von Frey filaments and heat radiation and were classified as CMHunits with a median mechanical threshold of 31 mN (range: 14-90mN, RA: 30 mN, 5.4-226 mN, n = 129) and a median heat thresholdof 41.0°C (range: 36.5-45.8°C, RA: 41.3°C, 35.6-49.5°C, n = 141).The conduction velocity was on average 1.0 m/s (median, range:0.85-1.07 m/s, RA: 0.97 m/s, 0.52-1.32 m/s, n = 155). Three ofthe six CMH units were located on the distal lower leg and threeon the proximal dorsum of the foot, close to theankle.

The other 20 units did not respond to stimulation with von Frey filaments of 750 mN and were hence classified as CMi. Theywere even not excited by penetration of the skin with a hypodermicneedle. Conduction velocity was on average 0.82 m/s (median, range:0.37-1.53 m/s, RA: 0.79 m/s, 0.47-1.29 m/s, n = 126). Of these,17 units were CH because they responded to heating (up to 52°C)with a median threshold of 48.6°C (range: 41.7-52.0°C, RA: 48.0°C,41.7-51.5°C, n = 52). Six CH units responded with more than 40"markings" to histamine iontophoresis and belonged therefore tothe subclass of "itch" units (Schmelz et al. 1997). Three CMiunits did not respond to heating (or histamine) and were classifiedas mechano-heat insensitive C nociceptors (CMiHi). They were provento be afferents by their pronounced activity dependent slowingclearly separating them from sympathetic efferents (Weidner etal. 1999). One of the total of 20 CMi units was located on a toe,13 on the foot dorsum and 6 on the lowerleg.

Conduction velocities and receptive thresholds were consistent with previous studies on larger samples of CMH and CMi units(Schmidt et al. 1997; Weidner et al. 1999).

Receptive fields of CMH units

eRFs OF CMH UNITS AT 10 mA. The eRFs of CMH units mapped with 10 mA had median areas of 1.95 cm² (range: 0.84-2.86 cm²; Fig. 2), which is not statistically different (Wilcoxon test)from the mRFs tested with 750 mN von Frey filaments (median: 1.87cm², range: 0.78-2.81 cm²). They had distinct borders. Moving the stimulus probe 1 mm acrossthe border drawn with pen on the skin was usually enough to reproduciblyactivate a unit or not. The borders of the 10 mA eRFs correspondedexactly to the 750-mN mRFs for most of the circumference of theCMH units. However, for parts of the circumference the 10-mA eRFsslightly exceeded the 750-mN mRF in four units. No CMH unit wasactivated by 750 mN outside the 10-mA eRF. Five of six CMH unitsexhibited one continuous 10-mA eRF. The remaining unit had twodistinct 10-mA eRFs separated by 2 mm. The 10-mA eRFs and 750-mNmRFs for the six CMH units are illustrated in Fig. 2A.

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Fig. 2. Electro- and mechano-receptive fields of mechano-heat-responsive (CMH) fibers. A: eRFs of 6 CMH units in response to 10-mA stimulation (black and white) and mechanoreceptive fields (mRFs) in response to 750 mN von Frey stimulation (black). For 2 units, the eRFs and mRFs coincided exactly. For 4 units, minor parts at the borders of the eRFs were not responsive to 750-mN von Frey stimulation. B: eRF of the same 6 mechano-responsive C units as shown in A mapped with electrical pulses of 10 mA (black) and 50 mA (crosshatched). Two units were also mapped with 70 mA (hatched) and 1 with 100 mA (white). Receptive fields located on the lower leg and foot are shown separately (top and bottom). The 50-mA fields are not much larger than the 10-mA fields in contrast to the mechano-insensitive units depicted in Fig. 3. The 10 mA eRFs for these mechano-responsive units are (in contrast to the mechano-insensitive units) mainly located near the center of the 50-mA receptive fields, suggesting that the 50-mA fields for these units may represent current spread rather than true anatomical receptive fields.

In a previous study, we examined the eRFs of mechanoresponsive units with relatively weak stimulus intensities (10 mA or 80-100V) (Schmidt et al. 1997

). Because these results also revealeda good correspondence of eRF and mRF, they are comparable to thenew results obtained at 10 mA in this study. Therefore we alsogive numbers of a combined sample of these two studies in thepresent work. All 83 CMH units together had a median receptivefield size of 1.01 cm² (range: 0.16-5.11 cm²) and a median diameter of 17 mm (range: 6-47 mm). The medianarea of the six CMH units in the present study (1.95 cm²) is close to the value (1.83 cm²) found for the lower leg in the previousstudy.

HIGH-INTENSITY eRFs OF CMH UNITS. Mapping the 6/6 CMH units with 50-mA electrical pulses produced slightly larger eRFs as compared with 10 mA (Fig. 2). Forunits with irregular 10-mA eRFs, the gaps and indentations ofthe eRFs tended to be filled out. The median area of the 50-mAfields increased to 3.08 cm² (range 1.15-3.66 cm²) and the median diameter from 24.4 to 28.7 mm. Increasing thestimulation intensity to 70 and 100 mA tended to produce a smallconcentric growth of the eRFs (Figs. 2B and 4).

Receptive fields of CMi units

eRFs OF CMi UNITS AT 10 mA. Stimulation at 10 mA in 13/20 CMi units produced small eRFs in all units tested. The median area was 0.35 cm² (range: 0.1-1.74 cm²). The units were excited at one or several small spots (median3, range: 1-7, Fig. 3). Chemical or thermal excitability couldregularly be found outside the 10 mA eRF. If the 10-mA eRF consistedof multiple spots, their closest borders had a median distanceof 5 mm (range: 3-45 mm) for the two closest spots and of 25 mm(range: 3-45 mm) for two most distant spots.

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Fig. 3. Electroreceptive fields of mechano-insensitive C-fibers. Electroreceptive fields of heat-responsive (CH) and -unresponsive (CMiHi, marked) mechano-insensitive C fibers on the lower leg, the foot, and the toes are depicted proximal side up. The 50-mA (crosshatched, tested for all units) fields were much larger than the 10-mA (black) fields but 70 (hatched) and 100 mA (white) produced relatively little further increase in the electroreceptive fields, suggesting that 50, 70, or 100 mA reflects the true anatomical receptive field. Note that even for 100 mA, no proximal elongation of the eRF indicative of the axonal stem is visible. There were no major differences in electroreceptive fields based on location (leg, foot, or toes) or histamine responsiveness (His). Ten-milliampere mapping stimuli produced an eRF in the units tested $---$ units lacking a black area in the figure were not tested at 10 mA. Units lacking a 70- or 100-mA field in the figure were not tested with these intensities.

HIGH-INTENSITY eRFs OF CMi UNITS. Stimulation with 50-mA pulses in 20/20 CMi units revealed fairly large irregular eRFs often with small "satellites" outsidethe main territory. The median area was 5.34 cm² (range: 1.1-14.2 cm²) and the median diameter was 46.6 mm (range: 21.0-78.6). Thisis larger than for CMH units (median area: 3.1 cm², median diameter: 28.7 mm, U test, P = 0.0013).

Further increase of the mapping intensity to 70 mA in 11 units and to 100 mA in 4 units produced little further increase inareas of eRFs (Figs. 3 and 4).

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Fig. 4. Summary of electro-receptive field size of CMH and CMi fibers. Raw data (thin lines) and medians ± quartile (thick lines) are depicted for CMi (n = 20) and CMH (n = 6) units. Note that the areas of the CMi units grew considerably when the current intensity was increased from 10 to 50 mA, whereas the areas of the CMH units changed only little with increasing current intensity.

Shape of 50-mA eRFs of CMH and CMi units

The median circumference/square root area quotient for the 50-mA eRFs of CMH units was 5.0 (range: 4.35-5.82), indicatinga more rounded shape than for CMi units with a median quotientof 7.2 (range: 5.1-10.8). The latter were thus significantly moreirregular in shape (U test, P = 0.002). There was no differencein 50-mA eRF area between CMi units on the lower leg (median area:5.91 cm², n = 6) or foot (median area: 5.08 cm², n = 14). This is in contrast to the proximo-distal size diminutionin CMH units as shown previously (Schmidt et al. 1997). The mediandiameters of 50-mA eRFs of CMi units were also similar (48 mm)on the foot and the lower leg. The maximal diameters were about50% larger than the perpendicular diameters. The direction ofthe maximal extent seemed to be randomly orientated (Table 1).

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Table 1. Diameters of 50-mA eRFs of the 20 CMi units in different directions related to region

Discrepancy between 10- and 50-mA eRFs in CMi and CMH units

The eRFs of CMi units grow in an irregular and discontinuous manner when increasing the stimulus intensity from 10 to 50 mAand the most distant part of a 50-mA field could be quite remotefrom its closest 10-mA field. In contrast, the eRFs of CMH unitsgrow little and in a more regular concentric manner. To illustratethis numerically, the maximal distance from the outer border ofthe 50-mA eRF to the nearest outer border of the 10-mA eRF wasmeasured for all the 13 CMi and 6 CMH units that were mapped withboth these intensities. We named this measure the "10-50 eRF distance."For CMi units, the median 10- to 50-eRF distance was 22.7 mm (range:4.6-33.2 mm). For CMH units, the corresponding median distancewas 3.4 mm (range: 2.4-5.7 mm). The difference is statisticallysignificant (U test, P = 0.0009). Even after normalizing thesedata by dividing 10- to 50-eRF distance with the mean diameterof the 50-mA eRFs to compensate for the difference in size betweenCMi and CMH units, the difference remained highly significant(U test, P = 0.007).

Variability of chemical and heat responsiveness inside the eRFs

Temperature thresholds were measured at multiple locations within the eRFs of all CH units except three. In some units, activationthresholds to heat and chemical responsiveness showed considerablevariations even inside the eRFs of a single unit as shown in Fig.5 (e.g., the 2 lower units). Maximal differences between heatthresholds were 42.7 versus 52 and 41.7 versus 50.2. The localtemperature thresholds and responsiveness to chemicals were notclearly related to whether the units were excited by 10-mA oronly by 50-mA electrical pulses through a pointed probe at thelocation where heat or chemical stimulation was applied.

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Fig. 5. Responsiveness to natural stimulation inside and outside the electro-receptive field of CMi fibers. Six examples of electroreceptive fields of CMi units are depicted using the same method to indicate responsiveness to electrical stimuli as in Fig. 3. $open circle$ , temperature thresholds at tested locations within the eRFs or responsiveness to histamine and acetylcholine when applied at multiple sites inside or outside the eRFs.

Histamine iontophoresis applied outside the 50-mA eRFs for five CMi units wasnegative.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The most important findings in this paper are the differences in size and shape of innervation territories between CMH andCMi fibers, the latter being larger and moreirregular.

Reliability and validity of the mapping procedure

Innervation territories of individual C units were mapped by transcutaneous electrical stimulation delivered from a pointedprobe. In all experiments, the marking technique was employedto make sure that responses of an individual unit were not confusedwith those of other fibers having overlapping innervation territories.To address the question whether the eRF as assessed here correspondedwith the distribution of receptive nerve endings mechanical, heator chemical stimuli were applied within the electrically mappedinnervationterritories.

In CMH units, the eRFs were compared with the mechanical receptive fields (mRFs) mapped with von Frey hairs suprathresholdfor all mechano-responsive C fibers (750 mN). Mechanical stimuliaffect stretch activated membrane channels in the C-fiber terminals,and the mRFs represent the distribution of those channels in theterminal arborization of theunits.

The substrate stimulated by transcutaneous electrical stimulation is not as obvious as that of mechanical stimulation. Whereasmechanical, thermal, and chemical stimuli excite the nerve fiberat its receptive terminals, an electrical stimulus might activateit further proximally. However, we did not observe elongationsof eRFs in the proximal direction which would have been the caseif the parent axon would have been activated. In monkey, Meyeret al. (1991) found such elongation as a correlate of the parentaxon at high stimulus intensities, whereas a sudden distal thresholddecrease indicated the border of the innervation territory. Inawake humans, the current necessary to excite the parent axonseems to exceed the tolerance level probably due to the thickinsulatingsubcutis.

Still, there is a possibility of lateral spread of the electrical current such that remote nerve terminals are excited byhigh-intensity stimulation. Indeed, this seemed to be the casefor CMH units that are known to have low electrical thresholds(Weidner et al. 1999). The concentric expansion of the eRFs onincreasing the stimulus intensity from 10 to 50 mA as documentedhere seems to reflect such current spread. Comparing the eRFswith the mRFs mapped with a 750-mN von Frey hair revealed a goodcorrespondence for the 10-mA eRF and the 750-mN mRF, whereas theexpansion at 50 mA was always outside the mRF. Therefore for CMHunits that have fairly low electrical and mechanical thresholds(Weidner et al. 1999), both mapping procedures might lead to aslight overestimation of the respective receptive fields, mechanicalprobing by exciting remote endings through lateral stretch, andtranscutaneous electrical stimuli by currentspread.

The situation is completely different for CMi units. They have much higher transcutaneous electrical thresholds than CMHs.In a previous study, we found an average threshold of 60 mA (0.2ms pulses) for CMi units and 4 mA for CMH units when an iontophoresisprobe, 5 mm in diameter, was used for stimulation (Weidner etal. 1999). In this study, 10 mA applied through a pointed proberevealed small scattered eRFs that could not reflect the realsize of the innervation territories because thermal or chemicalstimuli could excite the units from areas outside. Therefore 50mA was used for mapping. This revealed a considerable expansionof the eRFs that now might better reflect the real size of theinnervation territories because thermal and chemical stimulationregularly excited the units from within this area. Increase ofthe stimulus intensity to 70 or 100 mA induced only minimal furtherextensions, possibly not due to current spread because of itsnonconcentric growth. In addition, 10-mA spots were found directlyadjacent (2 mm) to spots from which 100 mA did not elicit anyresponse of the recorded fiber. This also reflects that a gradualincrease of current does not induce a gradual increase of sizeas suggested by the current spread hypothesis but that the areasrecruited at very high stimulus intensities represent extremelyhigh-threshold branches of the terminal arborization. In otherwords, mapping with 50 mA probably leads to an underestimationof the real size of the innervation territories for the mechano-insensitiveunits. The statistically significant difference between the slightlyoverestimated 10-mA eRF areas of CMH units (median: 1.95 cm²) and the underestimated 50-mA eRFs of CMi (median: 5.34 cm²; U test, P < 0.01) reveals that CMi units have much wider branchesin human skin than CMH C nociceptors. This difference becomeseven more striking (median: 1.01 vs. 5.34 cm², U test, P < 0.0001) when comparing the present CMi materialwith a large sample of CMH units published previously (Schmidtet al. 1997).

Inhomogeneity of sensory properties within the eRF of CMi units

The mRF and 10-mA eRF of CMH units are usually highly congruent. Comparable responsiveness to natural stimulation is not easilytested in CMi units. Only part of the CMi units respond to a certainchemical stimulus or to heating, and the unresponsiveness mightbe attributed to a lack of receptor proteins or to a lack of terminalbranches at the examined position. Several CH units, proven tobe heat sensitive in at least one spot, were tested for theirheat thresholds in various other spots within their eRF (Fig.5). Heat thresholds were astonishingly variable within the eRF.For a few units, repetitive histamine or acetylcholine stimulationyielded a comparable variability. The responsiveness to thesestimuli was apparently not related to whether the stimulus wasapplied within the 10 or 50 mA part of the eRFs. This suggeststhat CH units may have inhomogenous receptive properties of theirendings within different parts of their innervation territoriesrather than only variation in depth or dimensions of the terminalbranches.

In five of the CMi units, histamine iontophoresis was applied outside the 50-mA eRF. None of these units was activated. Thissuggests that there are no receptive endings outside the eRFsof CMi units, although it is possible that some CMi units mayhave branches with extremely high electrical thresholds whichare not excited even by 50- to 100-mApulses.

Organization of innervation territories

Innervation territories of several square centimeters can only be explained by extensive arborization of the nerve terminals.Anatomical evidence for branched nerve terminals that might evensupply distinct anatomical structures has been found in rats andcats (Heppelmann et al. 1990; Pierau et al. 1982; Taylor and Pierau1982). Distinct steps in response latency were found as functionalevidence for branched A $delta$ and C fibers in animal and human recordings(McMahon and Wall 1987; Peng et al. 1999; Ringkamp et al. 1998;Torebjörk and Hallin 1974). Our findings indicate that such branchestend to be concentrated on a confluent rounded area for CMH fibers,whereas for CMi fibers, the terminal arborization is widely distributed.Thus the CMi units had very irregular contours of their eRFs andoften showed satellites outside the main innervation territory.In addition many of the CMi units had discrete spots of fairlylow-threshold eRFs often eccentrically located within the high-thresholdregions possibly reflecting inhomogeneity in diameter or depthof the individualterminals.

Functional implications of different innervation territories

Recently we have shown that afferent cutaneous C fibers fall into two clearly different classes that in intact skin can bedistinguished by their responsiveness to mechanical stimulationwith von Frey hairs, the prior with a threshold of less than 200mN, the latter not even excitable by 750 mN or insertion of hypodermicneedles. Under pathophysiological conditions, this differencemay be blurred because CMi units often become responsive to mechanicalstimuli in inflamed skin (Schmidt et al. 1995). Since mechanicalthresholds of CMH units do not decrease in inflammation sensitizationof CMi units may be the underlying mechanism for primary mechanicalhyperalgesia (Schmelz et al. 1996). Alternatively, suprathresholdresponses could be enhanced also in CMH unit as shown before (Andrewand Greenspan 1999).

Mechanical responsiveness is not the only difference between the two classes of C nociceptors. Whereas discharge patternsof CMH units do not explain the intensity and time course of painin response to capsaicin injection or tonic pressure, dischargeof CMi units closely matches the perceived pain (Schmelz et al.2000b; Schmidt et al. 2000). Also the contribution to neurogenicflare responses is different. It is mediated by CMi units in humanskin, whereas there is only a minor contribution of CMH unitsto the axon reflex flare (Schmelz et al. 2000a). The extensionof the axon reflex flare induced by capsaicin injection, high-intensityelectrical stimulation or histamine of up to 15 cm in diametercan only be explained by large innervation territories of up to7.9 cm as shown for CMi units here. A subgroup of CMi units isparticularly sensitive to histamine and probably mediates itchsensations (Schmelz et al. 2000a). Six CH units responding tohistamine (marked with "His" in Fig. 3) were presented in thispaper.

It might be speculated that the small sizes of the innervation territories of CMH units and their proximo-distal decay wouldallow for more precise stimulus localization than the input fromCMi units with large territories. This notion is supported bythe finding, that localization of noxious events is fairly preciseon the foot and the dorsum of the hand with a pure C-fiber input(Jørum et al. 1989; Koltzenburg et al. 1993), whereas the twopoint discrimination for histamine induced itch is poor (Wahlgrenand Ekblom 1996).

In conclusion, innervation territories of CMi nociceptors are more irregular and much larger than the territories of CMH units.This spatial difference adds to the functional dichotomy betweenthe two major types of C nociceptors in human skin: mechano-insensitiveversus mechano-responsive.

	ACKNOWLEDGMENTS

This work was supported by the Swedish Medical Council, Project 5206, The Bank of Sweden Tercentenary Foundation (for H. O.Handwerker), the Max Planck Research Award for International Cooperation(for H. E. Torebjörk), the Swedish Foundation for Brain Research(for R. Schmidt), and the Deutsche Forschungsgemeinschaft (SFB353).

	FOOTNOTES

Address for reprint requests: R. Schmidt, University Hospital, Dept. of clinical neurophysiology, 751 85 Uppsala, Sweden.(E-mail: roland.schmidt{at}nc.uas.lul.se).

Received 5 November 2001; accepted in final form 3 June 2002.

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Innervation Territories of Mechano-Insensitive C Nociceptors in Human Skin

0022-3077/02 $5.00 Copyright © 2002 The American Physiological Society