Ionic Basis of Cold Receptors Acting as Thermostats

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The Journal of Neuroscience, May 15, 2002, 22(10):3994-4001

Ionic Basis of Cold Receptors Acting as Thermostats
Makoto Okazawa^*, Keizo Takao^*, Aiko Hori, Takuma Shiraki, Kiyoshi Matsumura, and Shigeo Kobayashi
Division of Biological Information, Department of Intelligence Science and Technology, Graduate School of Informatics, Kyoto University, Kyoto 606-8501, Japan

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

When temperature (T) of skin decreases stepwise, cold fibers evoke transient afferent discharges, inducing cold sensationand heat-gain responses. Hence we have proposed that cold receptorsat distal ends of cold fibers are thermostats to regulate skinT against cold. Here, with patch-clamp techniques, we studiedthe ionic basis of cold receptors in cultured dorsal root ganglion(DRG) neurons of rats, as a model of nerve endings. Cells thatincreased cytosolic Ca²⁺ level in response to moderate cooling were identified as neuronswith cold receptors. In whole-cell current-clamp recordings ofthese cells, in response to cooling, cold receptors evoked a dynamicreceptor potential (RP), eliciting impulses briefly. In voltage-clamprecordings (-60 mV), step cooling induced an inward cold current(I_cold) with inactivation, underlying the dynamic RP. Ca²⁺ ions that entered into cells from extracellular side inducedthe inactivation. Analysis of the reversal potential implied thatI_cold was nonselective cation current with high Ca²⁺ permeability. Threshold temperatures of cooling-induced Ca²⁺ response and I_cold were different primarily among cells. In outside-outpatches, when T decreased, single nonselective cation channelsbecame active at a critical T. This implies that a cold receptoris an ion channel and acts as the smallest thermostat. Becausethese thermal properties were consistent with that in cold fibers,we conclude that the same cold receptors exist at nerve endingsand generate afferent impulses for cold sensation and heat-gainbehaviors in response tocold.

Key words: cold receptor; thermostat; sensor; dorsal root ganglion; phase transition; ionic basis; patch-clamp; thermoregulation

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In mammals, heating and cooling of local areas in the hypothalamus, medulla oblongata and spinal cord evoke different heat-lossand heat-gain responses, respectively (Carlisle and Ingram, 1973;Chai and Lin, 1973; Lipton, 1973; Roberts and Mooney, 1974). Thus,multiple thermostats in the CNS regulate core T with differentthermoregulatory effectors (Satinoff, 1978).

In the CNS, there are warm- and cold-sensitive neurons (Nakayama et al., 1963; Hardy et al., 1964; Simon and Iriki, 1971;Inoue and Murakami, 1976), the firing rates (FRs) of which increasewith a rise and fall in T, respectively. According to the traditionalassumption in physiology (Adrian, 1928), both neurons have beenassumed to be sensors (or transducers) of Ts. Investigators hencesearched for the multiple thermostats except for these sensorneurons (Hammel et al., 1963; Nakayama et al., 1963; Mitchellet al., 1970; Bligh, 1973) but failed to identify the thermostats(Satinoff, 1978; Kobayashi, 1989).

With extracellular electrodes, impulse activities of warm- and cold-sensitive neurons are recorded in hypothalamic slices(Kobayashi, 1986). The FRs show threshold, saturation, and transientresponses to step changes in T. Because T and FR are not in aone-to-one ratio, it is invalid to assume that both neurons aresensors. Instead, on the basis of control theory (Weyrick, 1975),we propose that warm- and cold-sensitive neurons are the multiplethermostats in the CNS that evoke thermoregulatory responses againstheat and cold, respectively (Kobayashi, 1989).

Heating and cooling of skin elicit afferent discharges in warm and cold fibers to evoke heat-loss and heat-gain activities,respectively (Benzinger, 1969; Crawshaw et al., 1975). Their FRsalso show threshold and transient responses to step changes inskin T (Hensel and Zotterman, 1951a; Hensel and Huopaniemi, 1969;Schaffer and Braun, 1992). Hence, we propose that warm and coldreceptors are peripheral thermostats against heat and cold, respectively(Kobayashi, 1989). A model study easily explains that centralthermostat neurons regulate core Ts and peripheral thermostatfibers regulate skin Ts with thermoregulatory effectors (Kobayashi,1989).

Despite the significance in T sensation or thermoregulation, the ionic and molecular basis of warm and cold receptors hasnot well been characterized, compared with other types of sensoryreceptors. We have analyzed the ionic basis of warm-sensitiveneurons in thin hypothalamic slices with patch-clamp techniques(Hori et al., 1999). Capsaicin receptor (VR1) (Caterina et al.,1997) and its homolog VRL1 (Caterina et al., 1999), cloned fromdorsal root ganglion (DRG), respond to noxious heat. In contrast,the ionic basis of central or peripheral cold receptors has notbeen characterized. Cooling raises the intracellular Ca²⁺ ion level ([Ca²⁺]_i) in cultured DRG cells (Suto and Gotoh, 1999). This suggeststhat cold receptors exist at cell bodies as well as nerve endingsin sensory cells. In this study, we analyzed the ionic basis ofthe cold receptors in cultured DRG cells of rats, as a model ofnerve endings, with [Ca²⁺]_i measurements (Okazawa et al., 2000) and patch-clamp techniques(Hori et al., 1999). Recently, Reid and Flonta (2001) reportedon cold current; however, ion selectivity of cold currents andsingle-channel profiles have not beencharacterized.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Procedures were similar to those reported previously (Okazawa et al., 2000). Wistar rats (2-14 d old) were anesthetized withdiethyl ether and decapitated. DRGs were isolated and placed inCa²⁺-free Krebs' solution (see below) containing 0.25% collagenaseat 37°C for 90 min. Thereafter, they were incubated in Krebs'solution containing 0.25% trypsin at 37°C for 15 min, washed inDMEM (Invitrogen), and dissociated by trituration. The DRG cellswere then plated on coverslips (5 × 5 mm) coated with poly-L-lysineand cultured in DMEM containing penicillin (100 U/ml), streptomycin(0.1 mg/ml), 2 mM L-glutamine, nerve growth factor (100 ng/ml;Roche Diagnostics), and 10% fetal bovine serum (Hyclone) at 37°Cin a humidified atmosphere containing 5% CO₂ for 1-6 d beforerecordings.

Cultured cells were loaded with 5 µM fura-2 AM (Dojindo) at 30°C for 1 hr. After washing with Krebs' solution containing (inmM): 136 NaCl, 5 KCl, 2 CaCl₂, 2 MgCl₂, 10 glucose, 10 HEPES,pH 7.4 adjusted with ~4 NaOH, the cell-bearing coverslip was attachedwith silicone grease to the bottom of a recording chamber mountedon the stage of an upright fluorescence microscope (BS50WI, Olympus).Cells in the chamber were perfused with Krebs' solution by gravity.With a digital image analysis system (AQUACOSMOS; Hamamatsu Photonics),we detected the [Ca²⁺]_i image of cultured DRG cells every 4 sec except for those inFigure 1F (170 msec) and Figure 5 (2 sec). Cell T was monitoredwith a thermocouple (0.3 mm in diameter) close tocells.

For cold stimulation, T was decreased from 30-32°C (normal skin temperature) to 13-16°C in Figures 1-4, because these cellshave been assumed to be a model of skin receptors. At 30-32°C,however, responses sometimes started just after cooling, and itwas difficult to identify threshold temperatures. To clarify thresholdtemperatures, T was decreased from 38-40°C to 13-16°C in Figures5-7.

Patch-clamp recordings were similar to those in previous studies (Kobayashi and Takahashi, 1993; Hori et al., 1999). In Figures1-2, Krebs' solution was used as the extracellular solution. Forhigh K⁺ solution, 70 mM NaCl in Krebs' solution was replaced with equimolarKCl (see Fig. 1). For Ca²⁺-free Krebs' solution, 2 mM CaCl₂ in Krebs' solution was removed.The standard bath solution to analyze ion channels (see Figs.3-4, 6-7) was as follows (in mM): 136 NaCl, 10 HEPES, 10 glucose,pH 7.4 adjusted with ~4 NaOH. To make the Ca²⁺-containing solution in Figure 3, 2 mM Ca²⁺ was added to the standard bath solution. Bath solution to exploreCa²⁺ permeability in Figure 4D was as follows (in mM): 122 NaCl, 10CaCl₂, 0.1 CdCl₂ to suppress voltage-operated Ca²⁺ channels (VOCs), 10 HEPES, 10 glucose, pH 7.4 adjusted with ~4NaOH. In inside-out patch recordings (see Fig. 7F,G), 2 mM EGTAwas added to the standard bath solution to keep it in Ca²⁺-free condition, and 2 mM EGTA and 1.5 mM CaCl₂ were added tothe standard bath solution to keep it at 200 nM [Ca²⁺]_i according to the MAXCHELATOR program (C. Patton, Stanford University:http://www.stanford.edu/~cpatton/maxc.html).

The pipette solution for impulse recordings (see Fig. 1F) was Krebs' solution. The patch pipette in Figure 2 was filled witha solution containing (in mM): 122 K-gluconate, 14 KCl, 9 NaCl,1 MgCl₂, 0.2 EGTA, and 10 HEPES adjusted to pH 7.4 with ~4 KOH.The patch pipette in Figures 3A, 4A,B,D, 6, and 7A-E was filledwith a low Cl solution containing (in mM): 120 Cs-Aspartate, 16 CsCl, 10 HEPES,pH 7.4 adjusted with ~4 CsOH. In Figure 3B, the pipette solutionwas the low Cl solution containing 10 mM BAPTA. In Figures 4D, 7F, and G, thepipette was filled with a solution in which 10 mM glucose wasremoved from the standard bathsolution.

Relative permeability of monovalent cation (X⁺) to Cs⁺ (P_X/P_Cs) was calculated as P_X/P_Cs = exp (V_rev F/RT_abs), where V_rev isthe reversal potential, F is Faraday's constant, R is the universalgas constant, and T_abs is the absolute temperature. Relative permeabilityof Ca²⁺ to Cs⁺ (P_Ca/P_Cs) was calculated as described previously (Virginio etal., 1998).

Data were sampled at 0.4 kHz (whole-cell recording) or 2 kHz (single-channel recording) with MacLab software (AD Instruments)and analyzed with Igor Pro (WaveMetrics). Values were displayedas mean ± SEM. Statistical significance was obtained with unpairedttest.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of cells with cold receptors

We searched for cells with cold receptors using [Ca²⁺]_i in cultured DRG cells (Fig. 1). A high K⁺ solution increased [Ca²⁺]_i in neurons (Okazawa et al., 2000; Rusznak et al., 2000) (datanot shown). Step cooling (Fig. 1D, bottom) rapidly increased [Ca²⁺]_i in a few cells (13.5%) (B) of the neurons from a basal levelof 69.0 ± 4.8 nM (mean ± SEM; n = 32) to a peak of 422.4 ± 2.9nM (D, top). These cells were small in the cell body (10-25 µmin diameter), which was similar to the previous report (Suto andGotoh, 1999). After the peak, [Ca²⁺]_i slowly decreased despite a cessation of cooling.

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Figure 1. Cooling-induced [Ca²⁺]_i responses in cultured DRG cells. A-C, Microscopic views of cells in the same field. A, B, [Ca²⁺]_i in pseudocolor. A, Control level of [Ca²⁺]_i. B, Cooling-induced [Ca²⁺]_i increase in two cells (arrowheads). We identified them as cold-receptor cells. Arrow indicates one of the cold-insensitive cells. C, Nomarski image of cells. Scale bar, 20 µm. D, Time course of [Ca²⁺]_i responses to cooling (bottom) in cold-receptor cells (top) and cold-insensitive cells (middle). E, Pathway of Ca²⁺ ions to induce [Ca²⁺]_i increase in response to cooling. Top, Control; middle, cooling-induced [Ca²⁺]_i response (left) decreased under Ca²⁺-free condition (right). Bottom, Cooling-induced [Ca²⁺]_i response (left) decreased by Cd²⁺ (right), blocker of voltage-operated Ca²⁺ channels. F, Simultaneous recording of impulses (middle) and [Ca²⁺]_i increase (top). Impulses were recorded using a cell-attached pipette filled with Krebs' solution. [Ca²⁺]_i was measured at a high rate (170 msec). $open circle$ , [Ca²⁺]_i surge after impulses before cooling; , [Ca²⁺]_i surge after the first impulse at the onset of cooling.

We studied the Ca²⁺ source that elicited the [Ca²⁺]_i increase in response to cooling (Fig. 1E). In the middle traces, the cooling-induced[Ca²⁺]_i response (left) disappeared (right) under Ca²⁺-free conditions (3.1 ± 1.1% of controls; n = 18). This suggestedthat the influx of extracellular Ca²⁺ ion caused the [Ca²⁺]_i increase, consistent with the previous findings (Suto and Gotoh,1999). In the bottom traces, the cooling-induced [Ca²⁺]_i response (left) was inhibited (right) by Cd²⁺ ions, a blocker of VOCs (Hoehn et al., 1993; Gotoh et al., 1999).The residual response was 3.0 ± 1.2% of controls (n = 17) at thetime of peak response, suggesting that the VOC is a main pathwayfor [Ca²⁺]_iresponse.

Cell-attached patch recording of impulses activating VOC and [Ca²⁺]_i measurement were performed simultaneously in the same cold-receptorcells (n = 4) (Fig. 1F) (Sugimori and Llinas, 1990). Before cooling,this cell evoked spontaneous impulses (Fig. 1F, middle), and [Ca²⁺]_i surges ( $open circle$ ) occurred immediately after the impulses (top). WhenT was decreased (bottom), the impulse activities increased vigorously.A [Ca²⁺]_i surge () was identified at the first impulse after cooling.Thereafter, [Ca²⁺]_i increased rapidly with impulse activities. These results showthat the [Ca²⁺] responses reflect impulseactivities.

We performed whole-cell current-clamp recordings in cells with [Ca²⁺]_i responses (Fig. 2A, middle). In response to step cooling, membranepotential depolarized from the resting potential ( $-$ 65.1 ± 0.6mV; n = 7) to a peak ( $-$ 32.2 ± 5.2 mV) and slowly decreased. Byanalogy with other receptors, cooling-induced depolarization maybe a receptor potential (RP), showing dynamic response. When theRP became above threshold of excitation, cells generated actionpotentials (APs) repetitively. However, even when the depolarizationcontinued, firing activities soon decreased (Fig. 2A, top), probablybecause of inactivation of voltage-gated Na⁺ channels (Hille, 1992). Such a marked dynamic response of FRwas similar to that of impulses recorded extracellularly in coldfibers in vivo (Hensel and Zotterman, 1951a; Schafer et al., 1982;Schaffer and Braun, 1992). In contrast, cells without [Ca²⁺]_i responses did not respond to cooling (n = 13) (Fig. 2B).

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Figure 2. Whole-cell properties of cultured DRG cells. A, B, Current-clamp recordings of the membrane potential. A, Cold-receptor cell identified by cooling-induced [Ca²⁺]_i increase. Step cooling (bottom) induced a depolarizing receptor potential (RP) with inactivation, which elicited action potentials (AP) briefly at the onset of cooling (middle). The time scale was expanded to show APs (top). Because of cooling-induced dynamic RP and impulses, this cell could not be a sensor. Instead, this cell acted as a thermostat, which generated RPs leading to impulses in response to cooling. B, Cells without a cooling-induced [Ca²⁺]_i increase. Cooling did not induce RPs or impulses. C, D, Voltage-clamp recordings of the membrane current at $-$ 60 mV. C, Cold-receptor cell with a cooling-induced [Ca²⁺]_i increase. Step cooling induced inward current (I_cold) with inactivation, underlying dynamic responses of RPs in current-clamp recordings (A). D, Cold-insensitive cell without a cooling-induced [Ca²⁺]_i response. Cooling did not induce current.

To investigate the ionic basis of the RP, we performed whole-cell voltage-clamp recordings ( $-$ 60 mV) in cells with a [Ca²⁺]_i response. When cooled stepwise, a cold-receptor cell inducedan inward current with inactivation (Fig. 2C). The current maybe similar to that reported recently (Reid and Flonta, 2001),and we called the current I_cold. Peak I_cold was $-$ 25.1 ± 3.3 pA/pF(n = 19). This indicated that whole-cell conductance, the reversalpotential of which was at a potential depolarized from $-$ 60 mV,became active in response to cooling. These results imply thatI_cold underlies the RP in current-clamp recordings. In contrast,cooling did not induce a current in cells without a [Ca²⁺]_i response (Fig. 2D) (n = 14). Thus, we identified cells witha [Ca²⁺]_i response as neurons with cold receptors, and we identifiedcells without a [Ca²⁺]_i response as cold-insensitive neurons. In the following experiments,we analyzed characters of the cooling-induced [Ca²⁺]_i response and I_cold.

Effects of Ca²⁺ ions on I_cold

When the intravenous Ca²⁺ ion level decreases, cooling-induced FR increases in cold fibers (Schafer et al., 1982; Schaffer andBraun, 1992). Thus, we studied the effects of the extracellularCa²⁺ ion level, [Ca²⁺]_o, on I_cold at $-$ 60 mV (Fig. 3A). The duration of cooling wasprolonged to show the inactivation process in full, compared withFigure 2C. When [Ca²⁺]_o was normal (2 mM) (Fig. 3A, left), step cooling induced inwardI_cold to a peak, which was soon inactivated. At 60 sec after peak,I_cold was 17.0 ± 4.1% of the peak current (n = 4). In Ca²⁺-free solution (Fig. 3A, center), in contrast, cooling inducedI_cold without inactivation. When [Ca²⁺]_o was returned to normal, inactivation recovered. The ratio ofmaximum I_cold in the Ca²⁺-free solution to the peak in normal solution was 1.73 ± 0.38(n = 4). Thus, extracellular Ca²⁺ ions at normal level inactivated I_cold, which was consistentwith the above in vivo findings (Schafer et al., 1982; Schafferand Braun, 1992) and the patch-clamp study (Reid and Flonta, 2001).This indicates that Ca²⁺-induced inactivation of I_cold causes the dynamic response ofRP (Fig. 2A). To clarify whether Ca²⁺ ions affect I_cold from the intracellular or extracellular side,we added the Ca²⁺ ion chelator, BAPTA (10 mM), to the pipette solution. When cytosolicCa²⁺ was chelated with BAPTA, I_cold increased to $-$ 68.1 ± 12.7 (pA/pF)without inactivation (n = 4), even in the presence of extracellular2 mM Ca²⁺ ions (Fig. 2B). These results imply that Ca²⁺ ions that enter through I_cold conductance (Fig. 4D) affect I_coldfrom the intracellular side.

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Figure 3. Effects of extracellular Ca²⁺ ions on I_cold. A, I_cold was inactivated in Ca²⁺-containing bath solution (left). Duration of cooling was prolonged to clarify the inhibitory process, compared with Figure 2. In Ca²⁺-free solution, I_cold did not show inactivation (center). When bath solution was returned to Ca²⁺-containing solution, inactivation of I_cold recovered (right). These responses were obtained in the same cell. B, When 10 mM BAPTA was included in a pipette, I_cold was not inactivated in Ca²⁺-containing bath solution.

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Figure 4. Ion selectivity of I_cold conductance. The I-V curve of I_cold was drawn by application of a ramp-voltage command from 50 to $-$ 100 mV (0.6 sec). A-C, I-V curves in the absence of Ca²⁺ ions in external solution. A, In the standard bath solution (140 Na⁺), the I-V curve showed outward rectification. Reversal potential was 0.42 ± 0.75 mV (n = 16). Replacement of Na⁺ by NMDG abolished inward current (0 Na⁺), indicating that NMDG⁺ or Cl ions were not permeant. When half of the Na⁺ ions were replaced with NMDG⁺ ions (70 Na⁺), reversal potential shifted close to the value estimated by the Nernst equation. B, Replacement of extracellular 140 mM Na⁺ with equimolar Li⁺ or K⁺ did not significantly shift the reversal potential. C, When internal and external cations were 140 mM Na⁺, the reversal potential did not shift significantly. D, I-V curve in the presence of 10 mM Ca²⁺ in external solution. Partial replacement of extracellular Na⁺ with Ca²⁺ shifted the reversal potential to a positive potential.

Ion selectivity of I_cold channels

We studied ionic selectivity of I_cold conductance by drawing current-voltage (I-V) curves during cooling-induced currents.A set of voltage steps (25, 0, $-$ 25, $-$ 50, $-$ 75, and $-$ 100 mV; 600msec) was applied from a holding potential of 50 mV. Current evokedat each step was constant for 600 msec (n = 5). On the basis oftime-independency, we obtained I-V curves with ramp-voltage commandschanging from 50 to $-$ 100 mV for 600 msec (Fig. 4) (Kobayashi andTakahashi, 1993). In a standard bath solution (140 Na⁺), the I-V curve showed outward rectification (Fig. 4A). The reversalpotential was 0.42 ± 0.75 mV (n = 16), implying that I_cold conductancewas nonselective cation conductance. When 140 mM Na⁺ was replaced with equimolar N-methyl-D-glucamine (NMDG⁺) (0 Na⁺), the inward current disappeared (n = 4). This suggested thatNMDG⁺ or Cl ions were not permeant through the conductance. When half ofthe Na⁺ was replaced with equimolar NMDG⁺ (70 Na⁺), the reversal potential shifted to $-$ 15.9 ± 0.3 mV (n = 4), closeto the value ( $-$ 16.8 mV) estimated by the Nernst equation. When140 mM of Na⁺ was replaced with equimolar Li⁺ or K⁺ (Fig. 4B), the reversal potentials did not shift significantly(Li⁺: $-$ 1.3 ± 1.1 mV, n = 5; K⁺: 0.8 ± 1.0 mV, n = 5). When internal and external cations were140 mM Na⁺, the reversal potential did not shift significantly (0.0 ± 0.7mV, n = 4), suggesting that the inward and outward Na⁺ ion permeability was the same (Fig. 4C). In the presence of 10mM Ca²⁺ in bath solution, the reversal potential shifted to a positivepotential (6.8 ± 0.8 mV; n = 4), indicating that I_cold channelwas more permeable to the divalent cations than monovalent cations(P_Na:P_Li:P_K:P_Cs:P_Ca = 1.02:0.95:1.04:1.00:8.36).

Threshold responses of cooling-induced [Ca²⁺]_i increase

The threshold response is a crucial feature of a thermostat. We studied the cooling-induced threshold responses of [Ca²⁺]_i increases (Fig. 5) reflecting impulse activities. T was decreasedfrom 38-40°C to 13-16°C in several steps. When T decreased belowthreshold, [Ca²⁺]_i increased transiently (overshoot) and relaxed to a level abovebasal level. Transient responses in [Ca²⁺]_i may correspond to cooling-induced impulses for a short time(Fig. 2A). When T was decreased stepwise, [Ca²⁺]_i showed overshoots repeatedly, similar to firing rate activitiesin cold fibers in vivo (Dostrovsky and Hellon, 1978). The distributionsof threshold temperatures (27.4 ± 0.6°C; n = 67) (Fig. 5B) wereskewed to high temperatures. To investigate whether the thresholdtemperature depends on the changing speed of T, T was decreasedgradually (Fig. 5C). When T decreased below the thresholds, the[Ca²⁺]_i increase showed a long-lasting response. Here, the distributionsof threshold temperatures (27.0 ± 0.5°C; n = 72) became more symmetrical(Fig. 5D). However, the mean threshold temperatures were not significantlydifferent between the two experiments.

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Figure 5. Threshold responses of [Ca²⁺]_i increase reflecting impulse activities. A, Simultaneous recordings of [Ca²⁺]_i responses in two cells on the same coverslips. T was decreased stepwise (bottom). When T decreased below the threshold, [Ca²⁺]_i increased with dynamic responses at the onset of cooling (top). When T was decreased further to lower steps, [Ca²⁺]_i repeatedly increased with overshoots at the onset of cooling. In another cell (middle), [Ca²⁺]_i increase showed dynamic responses at a lower threshold temperature. B, Histogram of threshold temperatures recorded following the same procedure as in A. C, Simultaneous recordings of [Ca²⁺]_i responses in three cells on the same coverslips. T was decreased gradually. When T decreased below a threshold, [Ca²⁺]_i increase showed a long-lasting response. D, Histogram of threshold temperatures recorded following the same procedure as in C.

Threshold responses of I_cold in whole-cell recordings

We analyzed threshold responses of I_cold (Fig. 6), corresponding to that of RP (Fig. 2). In whole-cell voltage-clamp modes( $-$ 60 mV), T was decreased stepwise (Fig. 6A,B). When T decreasedbelow the thresholds, cells generated I_cold slightly (A). WhenT was decreased further to lower steps, I_cold vigorously increasedto a peak and then rapidly decreased. The repeated responses maycorrespond to the repeated [Ca²⁺]_i responses (Fig. 5A). The threshold temperatures (28.7 ± 0.8°C;n = 12) were similar to that (28.7°C) reported by others (Reidand Flonta, 2001) and not significantly different from that (27.4°C)of the [Ca²⁺]_i response (Fig. 5B). These results suggested that when T wasdecreased stepwise below threshold, cold receptors working asa thermostat increased whole-cell conductance with overshoot,leading to the dynamic RP in current-clamp recordings.

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Figure 6. Threshold responses of I_cold in whole-cell voltage-clamp recordings ( $-$ 60 mV). A, B, Cells with different threshold temperatures in the Ca²⁺-containing solution. A, T was decreased stepwise. When T decreased below the threshold (arrow), this cell generated inward I_cold slightly. When T was decreased to a lower step, I_cold vigorously increased to a peak and then rapidly deceased as in Figure 3A. B, Another cell with a low threshold temperature. C, I_cold in Ca²⁺-free solution. T was decreased gradually. Below the threshold (T_th), inward I_cold increased with a T decrease and reached saturation. T_th was 25.5°C. D, Relation between T (bottom scale) and I_cold in the box in C. $open circle$ , Experimental values. Top scale shows $Delta$ T (=T $-$ T_th). Because of the threshold response, I_cold was expressed by two equations. I_cold = 0, if $Delta$ T > 0. I_cold = S ( $Delta$ T), if $Delta$ T < 0. S ( $Delta$ T) is an increasing function with saturation.

To investigate threshold responses without inactivation, I_cold was recorded under Ca²⁺-free conditions (Fig. 6C). When T decreased below the threshold(T_th), I_cold increased and reached a saturated level ( $-$ 33.1 ±8.5 pA/pF; n = 5). The threshold temperatures (27.5 ± 1.3°C; n= 5) were not significantly different from the above recordings(28.7°C), suggesting that external Ca²⁺ ions did not affect threshold temperatures of I_cold.

The relation between T and I_cold in Figure 6C is shown in Figure 6D. We introduced a temperature difference, $Delta$ T (=T $-$ T_th).The top scale shows $Delta$ T. When T is above T_th, $Delta$ T > 0. When T isbelow T_th, $Delta$ T < 0. Because of the threshold response, I_cold isexpressed by two equations: I_cold = 0, when $Delta$ T > 0; I_cold = S( $Delta$ T), when $Delta$ T <0.

S( $Delta$ T) is an increasing function with saturation in the Ca²⁺-free condition; thus, I_cold depends on a negative value of $Delta$ T. Thisimplies that a cold cell acts as a thermostat, the output of whichdepends on negative $Delta$ T (Weyrick, 1975; Kobayashi, 1989).

Single-channel properties of cold receptors

We investigated single-channel properties of cold receptors in excised patch recordings of cold-receptor cells (Fig. 7). Ata holding potential of 60 mV, when T decreased gradually (Fig.7A), single-channel activities suddenly appeared at a criticaltemperature (T_c). During the active phase, open and closed statesalternated at random. When the channel was open, a unit currentflowed outward. Thus, a phase transition from silent to activephases occurred at T_c. In 23 patches from 17 cells, T_c was 22.6± 1.1°C, significantly (p < 0.05) lower than T_th of whole-cellcurrents (27.5°C). I-V profiles of the unit currents showed outwardrectification (Fig. 7B,C), similar to that of whole-cell currents(Fig. 4). The reversal potential was $-$ 1.1 ± 0.74 mV (n = 7), implyingthat they were nonselective cation channels. These similaritiesof I-V profiles suggested that the unit currents were elementsof the whole-cell I_cold current. Thus, cooling-activated channelswere recorded in cell-free patches without cytosol, suggestingthat cold receptors were ionotropic receptors with nonselectivecation channel properties.

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Figure 7. Single I_cold channels in excised patch recordings. A-E, Outside-out single I_cold channel recordings. A, When T decreased gradually, single-channel activities started at a critical temperature (T_c), implying that phase transition from silent to active phases occurred at T_c. In this patch, T_c was 19°C. B, Cooling-activated unit currents at different holding potentials at 25°C. C, I-V curve of unit currents in B. Points are expressed in mean ± SEM. Unit conductance ( $gamma$ ) was 48.5 ± 1.0 pS at 60 mV (n = 7) and 23.3 ± 0.6 pS at $-$ 60 mV (n = 7). D, Cooling-induced changes in the size of unit currents. Unit current at 25°C was larger than that at 15°C. E, Relationship between T and unit conductance ( $gamma$ , log scale) at three holding potentials. Symbols represent mean ± SEM (n = 7-9). Regression lines were drawn by the least square method. $open circle$ , (60 mV): $gamma$ = 22.92 exp (0.03076T). , (30 mV): $gamma$ = 20.14 exp (0.03441T). , ( $-$ 60 mV): $gamma$ = 11.17 exp (0.03050T). F, Inside-out single I_cold channel recordings in the absence (1, 3) and presence (2) of 200 nM Ca²⁺ ions in bath solution. G, Open probability (NP_o) of the channels (F) plotted against time. Numbered traces in F were obtained at times indicated by respective numbers in G. Ca²⁺ ions (200 nM) decreased open probabilities reversibly.

When T was below T_c, the size of the unit current decreased with a fall in T (Fig. 7D). The relations between T and unit conductance( $gamma$ , log scale) were plotted in Figure 7E, indicating that $gamma$ wasexponentially related to T. Q₁₀ (the 10° T coefficient) was 1.36(60 mV), 1.41 (30 mV), or 1.36 ( $-$ 60mV).

Ca²⁺ ions affected I_cold from the intracellular side (Fig. 3B). To clarify whether Ca²⁺ ions directly inactivated the I_cold channel, we made an inside-outpatch configuration from cold-receptor cells. Single-channel activitiesof I_cold were also recorded in the inside-out patch mode (Fig.7F(1)) (n = 17). In three of five patches, 200 nM Ca²⁺ ions decreased the activities of I_cold channels (Fig. 7F(2)).After washout of Ca²⁺, channel activities recovered (Fig. 7F(3)). Open probabilities(NP_o) of the channels were plotted against time (Fig. 7G); 200nM Ca²⁺ ions inhibited the channel activities reversibly. However, suchan inactivation of I_cold channels was not observed in the remainingtwo patches. These results imply that intracellular Ca²⁺ ions partly inactivate single I_cold channels, but soluble substancesare also needed in the Ca²⁺-inducedinhibition.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

When skin T decreases stepwise, cold fibers evoke afferent discharges (Hensel and Zotterman, 1951a; Schaffer and Braun, 1992)to induce cold sensation or heat-gain responses (Benzinger, 1969;Crawshaw et al., 1975) for regulation of skin T. Hence we proposethat cold fibers themselves are thermostats of skin T againstcold (Kobayashi, 1989). Here we analyzed the ionic basis of coldreceptors in DRG neurons in place of nerveendings.

Cold receptors in DRG neurons are the model of that in nerve endings

In whole-cell current-clamp recordings of cold-receptor neurons in cultured DRG cells, moderate cooling induced dynamic RP,eliciting impulses for a short time (Fig. 2). In some cases, spontaneousactivities of discharges were observed (Fig. 1F). Such a dynamicresponse and spontaneous activities of discharges have been recordedin cold fibers (Hensel and Zotterman, 1951a; Schaffer and Braun,1992). When T was decreased to several steps, dynamic [Ca²⁺]_i responses reflecting FR were evoked each time (Fig. 5), whichwere similar to the properties of afferent impulses from coldfibers (Dostrovsky and Hellon, 1978). When the extracellular Ca²⁺ level was normal, I_cold was inactivated (Fig. 3), which was similarto the patch-clamp study (Reid and Flonta, 2001) and consistentwith the effects of Ca²⁺ ions on FR of cold fibers (Schafer et al., 1982; Schaffer andBraun, 1992). Menthol induced an increase in [Ca²⁺]_i and a receptor potential leading to impulses in a small populationof DRG neurons (Okazawa et al., 2000). Most of the cold-receptorneurons in this study responded to menthol (our unpublished observation).The observation is consistent with the report that cold fibersrespond to menthol (Hensel and Zotterman, 1951b; Schafer et al.,1986). Cold-receptor neurons were small in diameter, implyingthat cold receptors in DRG neurons are the adequate model of thatin nerveendings.

Effects of Ca²⁺ on I_cold

When the extracellular Ca²⁺ level was normal, I_cold was inactivated (Fig. 3). This may partially cause adaptation of cold-receptorcells (Fig. 2A). The inactivation disappeared by removing extracellularCa²⁺ ions (Fig. 3A). The disappearance by intracellular BAPTA (Fig.3B) indicates that Ca²⁺ influx causes inactivation of the I_cold channel. In inside-outconfigurations, the activities of the I_cold channel was suppressedby calcium ions (Fig. 7E,F), indicating that calcium ions directlyinactivate the I_cold channels. However, in two of five patches,no obvious inactivation was observed. This suggests that thereare other inactivation mechanisms of I_cold channels using calcium-sensitivecytosolic component such as calmodulin or $alpha$ -actinin (Krupp etal., 1999).

Ionic basis of cold receptors

The reversal potential (near 0 mV) of I_cold is different from that (13.3 mV) reported by others (Reid and Flonta, 2001). Wecannot explain the discrepancy, because the ion compositions ofintracellular and extracellular solutions are not described intheir paper. The ion selectivity of the I_cold channel was Ca²⁺ > Cs⁺ ~ Li⁺ ~ K⁺ ~ Na⁺, indicating that the nonselective cation channel is permeableto both monovalent and divalent cations. Such a high permeabilityto Ca²⁺ has been reported in NMDA receptors (Burnashev et al., 1995)and the transient receptor potential (TRP) family, including TRP4 (Philipp et al., 1996), TRP6 (Inoue et al., 2001), and VR1 (Caterinaet al., 1997).

The I_cold channel is similar to VR1 in several ways. Extracellular Ca²⁺ ions inactivate channel activities, the I-V curve shows outwardrectification, and both are nonselective cation channels. Theunit conductance of cold-receptor channels (85.3 pS at 66 mV at44°C; extrapolated by thermal sensitivity of unit current in Fig.7E) is similar to heat-activated conductance (83.4 pS at 66 mVat 44°C) in VR1 (Tominaga et al., 1998).

I_cold current recorded in excised patches (Fig. 7) reveals that cooling directly activates cold channel without soluble secondmessengers. The Q10 of $gamma$ (1.36-1.41) is similar to that of theK⁺ (Rodriguez et al., 1998) and Cl channels (Pusch et al., 1997). This indicates that T dependenceof $gamma$ in I_cold channels is similar to that in other types of ionchannels.

Cold receptors act as thermostats against cold

Here we summarize the results and discuss the mechanism of how cold receptors act as thermostats against cold. In responseto step cooling, cold receptors in cultured DRG neurons eliciteda dynamic RP, which induced impulse trains briefly (Fig. 2). Theionic basis of the RP was analyzed. In whole-cell voltage-clamprecordings, cold receptors induced I_cold with inactivation, whenT decreased below threshold temperatures (Fig. 6A,B). An analysisof the reversal potential suggested that I_cold was a nonselectivecation current with high Ca²⁺ permeability. This implies that RP increases from resting potentialtoward ~0 mV, when whole-cell conductance is activated fully bycooling. Threshold temperatures of cooling-induced [Ca²⁺]_i response and I_cold were distributed widely (Figs. 5, 6). Wecannot explain the reason for the diversity at present, but thediversity might be caused by differences in channel modificationsuch as glycosylation (Kedei et al., 2001). Large differencesin threshold temperatures have been observed in warm- and cold-sensitiveneurons recorded extracellularly in hypothalamic slices (Kobayashi,1986). Thus, individual cold-receptor cells may be thermostatneurons against cold, having different threshold temperaturesas targets of T regulation (Kobayashi, 1989).

In outside-out patch recordings, when T decreased, a nonselective cation channel became active at a critical T (Fig. 7). Thisimplies that a cold receptor is an ion channel and acts as thesmallest thermostat against cold. Thus, the principle of thermostataction may be attributable to phase transition between silentand active phases occurring at a critical T in the channel. Whenmany cold receptors exist in a cell membrane, they will form awhole-cell thermostat against cold. Under Ca²⁺-free conditions, whole-cell current increased when T decreasedbelow threshold (Fig. 6D). In contrast, the unit size of singlechannels decreased with a fall in T when the channel was active(Fig. 7E). The discrepancy can be explained as follows. Whole-cellcurrent is equal to Np_oi, where N is the number of activated channels,p_o is open probability of the channels, and i is the size of unitcurrents. Because whole-cell current (Np_oi) greatly increaseswith a decrease in T (Fig. 6C,D), a cooling-induced increase inNp_o (activities of N channels) may be larger than an cooling-induceddecrease in i.

We conclude that the same cold receptors as identified in cultured DRG cells exist at nerve endings and generate RP to evokeafferent impulses for cold sensation or heat-gain responses inresponse tocold.

Note added in proof. While this paper was being revised, the molecular basis of cold receptors was reported (McKemy et al.,2002; Peier et al., 2002). Whole-cell properties of cooling-inducedcurrents in the cloned receptors were similar to results in thispaper.

  FOOTNOTES

Received Oct. 26, 2001; revised Feb. 28, 2002; accepted March 7, 2002.

^* M.O. and K.T. contributed equally to thiswork.

This study was supported by a grant-in-aid for scientific research from the Ministry of Education, Science, Sports and Cultureof Japan, and by Special Coordination Funds for Promoting Scienceand Technology from the Science and Technology Agency. We thankDr. S. Nakanishi for invaluable discussions about thismanuscript.

Correspondence should be addressed to Dr. Shigeo Kobayashi, Division of Biological Information, Department of IntelligenceScience and Technology, Graduate School of Informatics, KyotoUniversity, Sakyo-ku, Yoshida Honmachi, Kyoto 606-8501, Japan.E-mail skoba{at}i.kyoto-u.ac.jp.

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