Differential Activation and Desensitization of Sensory Neurons by Resiniferatoxin

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Volume 17, Number 14, Issue of July 15, 1997 pp. 5622-5628
Copyright ©1997 Society for Neuroscience

Differential Activation and Desensitization of Sensory Neurons by Resiniferatoxin

Geza Acs, Tamas Biro, Peter Acs, Shayan Modarres, and Peter M. Blumberg
Molecular Mechanisms of Tumor Promotion Section, Laboratory of Cellular Carcinogenesis and Tumor Promotion, National Cancer Institute, National Institutes of Health, Bethesda, Maryland 20892

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Recently, with use of rat dorsal root ganglion (DRG) neurons we have been able to dissociate the binding affinities of vanilloidsfrom their potencies to induce ⁴⁵Ca uptake, which suggests the existence of distinct classes ofthe vanilloid receptor (Acs et al., 1996). In the present study,we have demonstrated that the ultrapotent capsaicin analog resiniferatoxin(RTX) desensitized rat DRG neurons to the subsequent inductionof ⁴⁵Ca uptake by capsaicin and RTX with affinity and cooperativitysimilar to that found for [³H]RTX binding, contrasting with a ~10-fold weaker potency andlack of cooperativity to induce ⁴⁵Ca uptake. Likewise, the competitive antagonist capsazepine inhibitedRTX-induced desensitization with potency similar to that for inhibitionof specific [³H]RTX binding, whereas the potency of capsazepine was ~10-foldhigher for inhibiting RTX-induced ⁴⁵Ca uptake. Finally, the noncompetitive antagonist ruthenium redinhibited both the RTX-induced desensitization and ⁴⁵Ca uptake but showed ~60-fold selectivity for inhibiting RTX-induceddesensitization. The RTX-induced desensitization was not associatedwith loss of specific [³H]RTX binding, suggesting lack of gross cell toxicity. In contrastto RTX, capsaicin caused desensitization with a potency correspondingto that for ⁴⁵Ca uptake and did so in a noncooperative manner. Unlike the RTX-induceddesensitization, the desensitization by capsaicin was blockedby ruthenium red only at doses that blocked ⁴⁵Ca uptake and depended on external calcium. Our findings providefurther support for the existence of vanilloid receptor subtypeson DRG neurons with distinct pharmacology and distinct patternsof desensitization.
Key words: dorsal root ganglion neurons; capsaicin; resiniferatoxin; desensitization; [³H]RTX binding; ⁴⁵Ca uptake; capsazepine; ruthenium red; pain; rat

INTRODUCTION

A subpopulation of primary afferent neurons, located in the dorsal root and trigeminal ganglia, can be defined by their selectivesusceptibility to the effects of capsaicin (Buck and Burks, 1986;Holzer, 1991), the major pungent ingredient of hot peppers ofthe plant genus Capsicum.

Several years ago we found that resiniferatoxin (RTX), a naturally occurring irritant tricyclic diterpene (Hergenhahn et al.,1975) that combines structural features of the phorbol ester tumorpromoters and of capsaicin, functions as an ultrapotent capsaicinanalog (Szallasi and Blumberg, 1989). Qualitatively, RTX inducesa pattern of responses generally similar to those observed forcapsaicin (Szallasi and Blumberg, 1989). RTX and capsaicin differ,however, in their relative potencies for different responses (Blumberget al., 1993).

As observed for capsaicin, after initial excitation, RTX treatment also leads to desensitization to subsequent RTX application;in addition, desensitization by either compound leads to cross-desensitizationto the other (Blumberg et al., 1993). It was postulated decadesago that pungency of capsaicin analogs is proportional to thedesensitization that follows (Jancso, 1968); however, this doesnot seem to be the case for RTX. For example, similar concentrationsof RTX and capsaicin cause contraction of isolated rat urinarybladder, but RTX shows a 1000-fold higher potency to induce desensitization(Maggi et al., 1990). Moreover, RTX, but not capsaicin, can desensitizethe pulmonary J1 receptors of the rat without previous excitation(Szolcsanyi et al., 1990).

[³H]RTX shows specific, saturable binding to membranes of sensory afferent neurons, displaying appropriate tissue, species,and pharmacological specificity to represent the vanilloid receptor(Blumberg et al., 1993; Acs et al., 1994a,b). Specific [³H]RTX binding by the above membrane preparations displays sigmoidalsaturation kinetics, indicating apparent positive cooperativity(Acs et al., 1994a,b).

The basis for the differences in the pattern of responses to capsaicin and RTX and the divergence between the stimulatoryand desensitizing potencies of vanilloids has remained unresolved.Consistent with the existence of receptor subclasses (Holzer,1991; Blumberg et al., 1993), different vanilloid analogs showdifferent potencies for receptor binding and for induction of⁴⁵Ca uptake in dorsal root ganglion (DRG) neurons when assayed undersimilar conditions (Acs et al., 1996). Likewise, both RTX andcapsaicin bind to DRG neurons in a positive cooperative fashionbut induce ⁴⁵Ca uptake in a noncooperative manner (Acs et al., 1996).

In the present study, we have examined whether we can identify any responses in the DRG neurons linked to the high-affinityRTX receptor as defined by [³H]RTX binding. We conclude that this site mediates desensitizationof ⁴⁵Ca uptake to subsequent vanilloid challenge. We further demonstratethat stimulation of the ⁴⁵Ca uptake site by capsaicin can alternatively desensitize thecells to subsequent vanilloid challenge. These two pathways ofdesensitization show different sensitivities to ruthenium redand different dependence on external Ca²⁺. On the one hand, our findings strengthen the evidence for multiplevanilloid receptors; on the other hand, they help rationalizethe extensive evidence for the complexity of "desensitization"in response to vanilloids (Holzer, 1991).

MATERIALS AND METHODS
Female Sprague Dawley rats (6-8 weeks old, 150-160 gm body weight) were purchased from NCI-FCRDC (Frederick, MD). Animalswere allowed to access food and water ad libitum throughout thecourse of the experiments. Animal protocols were approved by theAnimal Care and Use Subcommittee, Division of Basic Sciences,National Cancer Institute. [³H]RTX (37 Ci/mmol) was synthesized by the Chemical Synthesis andAnalysis Laboratory, NCI-FCRDC. ⁴⁵Ca (CaCl₂, 23.55 mCi/mg) was purchased from DuPont NEN (Boston,MA). Nonradioactive RTX and capsazepine were from LC Laboratories(Woburn, MA). Capsaicin was from Sigma (St. Louis, MO). Rutheniumred was purchased from Research Biochemicals International (Natick,MA).

Cell cultures. Rat DRG neuron cultures were prepared as described (Acs et al., 1995, 1996). Animals were decapitated underCO₂ anesthesia. The spinal columns were removed aseptically, andDRGs from all levels were dissected out and collected in ice-coldDMEM (Life Technologies, Gaithersburg, MD) containing 0.5% heat-inactivatedfetal bovine serum (Life Technologies), 1 mM sodium pyruvate,and 25 mM HEPES. Ganglia were digested with 0.125% collagenase(Sigma) in DMEM for 90 min at 37°C and then for an additional90 min in fresh collagenase solution. Ganglia were washed twicewith DMEM containing 25 mM HEPES and 1 mM sodium pyruvate andwere triturated through a flame-polished Pasteur pipette to forma single cell suspension. The cells were pelleted through a cushionof DMEM containing 15% fatty acid-free bovine serum albumin (BSA)(Sigma) to remove myelin debris. Cells were then washed threetimes with serum-free DMEM and resuspended in the same medium,and the number of viable cells was determined by the Trypan-bluedye exclusion test. Cells were then plated into MultiScreen-DV96-well filtration plates (Millipore, Marlborough, MA) at a densityof ~5 × 10³ cells/well in 100 µl of serum-free medium.

For desensitization experiments, cells were incubated at 37°C in the presence of RTX or capsaicin for the indicated timesbefore measurement of induction of ⁴⁵Ca uptake. Alternatively, the cells in suspension were treatedwith RTX and competing ligands (capsazepine or ruthenium red).After incubation at 37°C for 6 hr, cells were washed three timeswith serum-free DMEM containing 0.25 mg/ml BSA and then challengedwith either capsaicin or RTX to induce ⁴⁵Ca uptake. The efficacy of the washing procedure was quantitatedin the following way. Cells were incubated in the presence of250 pM [³H]RTX (the concentration of RTX used in most experiments for inducingdesensitization) for 6 hr. The radioactivity in the cell suspensionwas determined before washing and after each washing step by scintillationcounting. According to these experiments, ~95% of the added radioactiveRTX was removed by this washing procedure from the suspension(see insert in Fig. 5). The number of viable cells was then determined.Cells were then plated into Multiscreen-DV 96-well filtrationplates at a density of ~5 × 10³ cells/well in 100 µl serum-free medium and used for ⁴⁵Ca uptake and [³H]RTX binding assays.
Fig. 5. Differential inhibition by ruthenium red of capsaicin and RTX-induced desensitization of rat DRG neurons. Cells were incubatedwith either 250 pM RTX or 1 µM capsaicin for 6 hr in the presenceof 60 nM or 2 µM ruthenium red, washed three times with serum-freeDMEM containing 0.25 mg/ml BSA to remove the pretreatment compounds,and then challenged with 3 µM capsaicin to induce ⁴⁵Ca uptake. The return of the ⁴⁵Ca uptake response in the presence of ruthenium red representsthe inhibition of desensitization. Points represent mean valuesfrom sets of eight determinations in a single experiment; errorbars indicate SEM. Two additional experiments yielded similarresults.
[View Larger Version of this Image (49K GIF file)]

Measurement of ⁴⁵Ca uptake by DRG neurons. Freshly dissociated cells in MultiScreen-DV 96-well filtration plates were incubatedin a total volume of 0.25 ml of serum-free DMEM (containing 1.8mM CaCl₂) in the presence of 0.25 mg/ml BSA (included to stabilizethe compounds in the aqueous solution), 1 µCi/ml ⁴⁵Ca, and increasing concentrations of the different compounds for20 min at 37°C (Acs et al., 1995, 1996). Cells were then washedfive times with ice-cold DMEM by filtration using a MultiScreenVacuum Manifold (Millipore). Filters were dried under a heat lampand punched out into scintillation vials using MultiScreen disposablepunch tips, and the radioactivity was determined by scintillationcounting. For each data point in each experiment, eight wellswere assayed.

Analysis of ⁴⁵Ca uptake data. Analysis of the ⁴⁵Ca uptake experiments was performed as described previously (Acs et al., 1996)by computer fit to the Hill equation (Endrenyi et al., 1975).In the case of experiments performed on RTX or capsaicin-pretreatedcells, desensitization was defined as the difference (in dpm/well)between the increase in ⁴⁵Ca uptake in these and in control cells after challenge by capsaicinor RTX. The decrease in the ⁴⁵Ca uptake induced by vanilloids was plotted against the pretreatmentconcentration of RTX, and the data were fitted to the Hill equation.Data from competition experiments in which the effect of the desensitizingcompound was antagonized by either a competitive (capsazepine)or a noncompetitive (ruthenium red) antagonist were fitted tothe modified Hill equation (Davis et al., 1977). Data were fittedto the equations using the computer program MicroCal Origin 3.5(MicroCal Software, Northampton, MA). For the statistical analysisof the curve fitting to the experimental data, the $chi$ ² test of goodness of fit was used.

Measurement of [³H]RTX binding by DRG neurons. For [³H]RTX binding assays, cells were plated into Multiscreen-DV 96-well filtrationplates (Acs et al., 1996). Immediately after plating, 150 µl ofDMEM containing 0.25 mg/ml BSA, [³H]RTX, and nonradioactive ligands was added to each well containingthe 100 µl cell suspension, and the plates were incubated in triplicatefor 60 min at 37°C. Plates were then chilled on ice, and 1 mgof $alpha$ ₁-acid glycoprotein (AGP, Sigma) in 50 µl of ice-cold serum-freeDMEM was added to each well to reduce nonspecific binding (Szallasiet al., 1992). Cells were then washed four times with DMEM (200µl/well) containing 0.5 mg/ml AGP by filtration using a MultiScreenVacuum Manifold (Millipore). Filters were dried under a heat lampand punched out into scintillation vials using MultiScreen disposablepunch tips, and the bound radioactivity was determined by scintillationcounting. Binding was expressed as femtomoles/10³ cells; nonspecific binding was determined in the presence of1 µM nonradioactive RTX.

RESULTS
The potencies of RTX and capsaicin to stimulate the uptake of calcium into rat DRG neurons were determined in the presenceof 1 µCi/ml ⁴⁵Ca. As expected, both ligands induced a dose-dependent increasein ⁴⁵Ca uptake by the cells with ED₅₀ values of 1.24 ± 0.02 nM forRTX and 316 ± 47 nM for capsaicin (mean ± SEM for four experimentseach). Hill coefficients for the dose-response curves were closeto unity (1.08 ± 0.07 and 1.02 ± 0.06 in the case of RTX and capsaicin,respectively; mean ± SEM for four experiments) (p > 0.05; Student'st test), suggesting a noncooperative mechanism of action. Thesevalues agreed well with those determined previously (Acs et al.,1996).

We had reported previously (Acs et al., 1996) that RTX displayed 24-fold greater potency for specific binding to DRG neuronsthan for induction of ⁴⁵Ca uptake. We were interested in how the low concentrations ofRTX, at which binding was measured, affected the induction of⁴⁵Ca uptake on subsequent capsaicin treatment. We first determinedthe effect of RTX pretreatment for different time intervals on⁴⁵Ca uptake after challenge with capsaicin. Preincubation of theneurons with 100 pM (a concentration close to the K_d value ofRTX for receptor binding) and 250 pM RTX (a concentration thatalmost saturates RTX binding sites) (Acs et al., 1996) for 10min had no effect on the level of ⁴⁵Ca uptake when the cells were stimulated with 3 µM capsaicin (adose that by itself induces a maximal stimulation of ⁴⁵Ca uptake by the cells) (Acs et al., 1995, 1996) (Fig. 1A). Incontrast, a significant decrease of ⁴⁵Ca uptake (20.8 ± 1.3 and 33.6 ± 2.1% decrease compared with controluptake, respectively; mean ± SEM for three experiments each) (p< 0.05; Student's t test) was observed in both cases after 30min of preincubation with RTX. A maximal effect of RTX pretreatment(55.7 ± 3.3 and 91.2 ± 1.8% decrease in ⁴⁵Ca uptake in the case of 100 and 250 pM RTX pretreatment, respectively,compared with control cells; mean ± SEM for three experimentseach) was reached in both cases by 5 hr of preincubation. On thebasis of the above results, a 6 hr preincubation time was usedin the subsequent experiments to induce maximal desensitizationto RTX.
Fig. 1. Inhibition of ⁴⁵Ca uptake in rat DRG neurons after RTX pretreatment. A, Time course of the effect of RTX pretreatment on ⁴⁵Ca uptake. Cells were pretreated with 100 pM ( $square$ ) and 250 pM ( $black-square$ )resiniferatoxin and then challenged with 3 µM capsaicin. Two additionalexperiments yielded similar results. B, Comparison of dose-responsecurves for induction of ⁴⁵Ca uptake, [³H]RTX binding, and desensitization by RTX in rat DRG neurons.Data are expressed as uptake values above baseline for RTX-induced⁴⁵Ca uptake ( $open circle$ ) and as specifically bound [³H]RTX ( $triangle$ ) when binding was determined. Desensitization was definedas the difference (in dpm/well) in ⁴⁵Ca uptake between pretreated and control cells challenged withcapsaicin. In the case of desensitization ( $black-square$ ), cells were pretreatedwith different concentrations of RTX for 6 hr and then challengedwith 3 µM capsaicin. Points represent mean values from sets ofeight determinations in a single experiment; error bars indicateSEM. The theoretical curves were calculated by fitting the measuredvalues to the Hill equation. In the case of ⁴⁵Ca uptake and desensitization, three additional experiments ineach case yielded similar results. The dose-response curve for[³H]RTX binding is a single experiment, yielding binding parameterssimilar to those we found previously (Acs et al., 1996).
[View Larger Version of this Image (17K GIF file)]

To determine the concentration dependence of RTX-induced desensitization, neurons were incubated with different concentrationsof RTX for 6 hr. This procedure resulted in a dose-dependent reductionin the level of ⁴⁵Ca uptake after challenge with 3 µM capsaicin (Fig. 1B). Fittingthe desensitization curves (see Materials and Methods) to theHill equation yielded an apparent K_d value for desensitizationof 81 ± 5 pM and a Hill coefficient of 1.51 ± 0.11 (mean ± SEMfor four experiments), suggesting positive cooperativity of RTXaction. The potency of RTX for desensitization thus was ~10-foldhigher than that for induction of ⁴⁵Ca uptake and was similar to its affinity for receptor binding(47 ± 4 pM) (Acs et al., 1996). Moreover, RTX desensitized thecells in a positive cooperative fashion $---$ with a Hill coefficientsimilar to that determined in receptor binding assays (1.78 ±0.12) (Acs et al., 1996) $---$ as opposed to its noncooperative actionin ⁴⁵Ca uptake induction assays.

In the above experiments, we desensitized with RTX and challenged with capsaicin. In other experiments we challenged the 250pM RTX-pretreated cells with as high a dose of RTX as 200 nM.The K_d and Hill coefficient values for desensitization were similarto those after capsaicin challenge (K_d and Hill coefficient valueswere 91 ± 6 nM and 1.62 ± 0.24, respectively; mean ± SEM for fiveexperiments).

The desensitization of ⁴⁵Ca uptake was independent of the challenging dose of capsaicin or RTX. Pretreatment of the neuronswith 250 pM RTX (a concentration that by itself induced only 11.7± 1.5% of maximal ⁴⁵Ca uptake response; mean ± SEM for four experiments) almost completely(92.1 ± 2.8%; mean ± SEM for four experiments, for challenge by3 µM capsaicin) abolished the induction of ⁴⁵Ca uptake by capsaicin up to a concentration of 6.4 µM (data notshown). Likewise, pretreatment of the cells with 250 pM RTX for6 hr also abolished the ⁴⁵Ca uptake induced by 200 nM RTX by 90.3 ± 3.1% (mean ± SEM forfive experiments) (data not shown). These results suggest thatthe decrease in ⁴⁵Ca uptake stimulated by a subsequent challenge could not be attributedto competition at the site coupled to the ⁴⁵Ca uptake. Further support for this conclusion comes from experimentsin which the cells were washed three times after RTX preincubationimmediately before the capsaicin challenge (this procedure removed>95% of the 250 pM RTX used for pretreatment) (for details, seeMaterials and Methods). The washing had no effect on the levelof desensitization caused by the pretreatment (data not shown).We conclude that the RTX-induced desensitization does not requirethe continuous presence of RTX on the receptors.

As shown in Figure 1B, [³H]RTX displayed specific binding to rat DRG neurons. At 4 nM [³H]RTX, a concentration sufficient to saturate the receptors, thereceptor density in control cells was 0.140 ± 0.002 fmol/10³ cells. This value agreed well with those determined previously(Acs et al., 1996). Under similar conditions, in cells pretreatedwith 250 pM RTX for 6 hr and in cells to which 250 pM RTX wasadded immediately before the binding assay, we determined similarvalues of specifically bound [³H]RTX of 0.129 ± 0.002 and 0.125 ± 0.001 fmol/10³ cells, respectively. When we determined the density of RTX bindingsites after washing the cells three times after RTX pretreatment,we observed values of specifically bound [³H]RTX of 0.139 ± 0.002 and 0.141 ± 0.008 fmol/10³ cells, respectively. In neither case did the pretreated cellssignificantly differ from the corresponding control (p > 0.05;Student's t test). We conclude that the observed decrease in ⁴⁵Ca uptake after RTX pretreatment could not be attributed to thedownregulation of the vanilloid receptor as detected by the [³H]RTX binding assay. This observation further demonstrates thelack of toxicity of the 6 hr incubation with 250 pM RTX. Likewise,the number of viable neurons was not changed after RTX treatment,and the baseline uptake of ⁴⁵Ca was the same in pretreated and control cells (data not shown).

As observed previously (Acs et al., 1996), the competitive antagonist capsazepine (Bevan et al., 1992; Szallasi et al., 1993)inhibited stimulation of ⁴⁵Ca uptake by 500 nM capsaicin in a noncooperative fashion. K_iand Hill coefficient values were 291 ± 31 nM and 0.98 ± 0.03,respectively (mean ± SEM for three experiments). Capsazepine likewiseinhibited ⁴⁵Ca uptake into rat DRG neurons induced by 200 nM RTX with similarK_i and Hill coefficient values of 351 ± 39 nM and 1.07 ± 0.08(mean ± SEM for four experiments) (data not shown).

To determine whether capsazepine also acted as an antagonist of RTX-induced desensitization, we pretreated the cells with250 pM RTX and different concentrations of capsazepine for 6 hr,washed them three times, and then challenged them with 200 nMRTX. This high challenging concentration of RTX (~200-fold itsK_d for induction of ⁴⁵Ca uptake) was used to assure complete displacement of capsazepinefrom both the ⁴⁵Ca uptake site and the specific [³H]RTX binding site. Using the washing protocol (see Materialsand Methods), we were able to show that capsazepine inhibitedthe RTX-induced desensitization in a dose-dependent fashion (Fig.2), yielding a K_i of 3.66 ± 0.71 µM and a Hill coefficient valueof 1.83 ± 0.11 (mean ± SEM for four experiments), suggesting apparentpositive cooperativity. These data are in good accord with theK_i and Hill coefficient values of capsazepine for inhibiting specific[³H]RTX binding to DRG neurons (3.16 ± 0.21 µM and 1.72 ± 0.11,respectively) (Acs et al., 1996) and contrast with the respectivevalues of capsazepine for blocking RTX-induced ⁴⁵Ca uptake (see above). By itself, capsazepine did not cause desensitization.
Fig. 2. Inhibition of RTX-induced desensitization of rat DRG neurons by capsazepine. Cells were incubated in the presence of 250 pMRTX and different concentrations of capsazepine for 6 hr. Cellswere then washed three times with serum-free DMEM containing 0.25mg/ml BSA to remove the above compounds and were then challengedwith 200 nM RTX to induce ⁴⁵Ca uptake ( $black-square$ ). Cells not treated with either RTX or capsazepine( $open circle$ , control) or treated with only 250 pM RTX for 6 hr ( $square$ ) areshown as control values. Points represent mean values from setsof eight determinations in a single experiment; error bars indicateSEM. The theoretical curve was calculated by fitting the measuredvalues to the Hill equation. Two additional experiments yieldedsimilar results.
[View Larger Version of this Image (23K GIF file)]

Similar experiments were performed with the noncompetitive vanilloid receptor antagonist ruthenium red (Amann and Maggi, 1991).When applied together with RTX, ruthenium red blocked the ⁴⁵Ca uptake into the cells induced by 200 nM RTX in a dose-dependentfashion, with an ED₅₀ of 790 ± 40 nM (mean ± SEM for three determinations)(Fig. 3); this value agreed well with those reported previously(Maggi et al., 1988). Furthermore, when administered togetherwith 250 pM RTX during the 6 hr pretreatment, ruthenium red hada biphasic effect on ⁴⁵Ca uptake induced by a subsequent challenge with 200 nM RTX. Atlower concentrations ruthenium red inhibited RTX-induced desensitization,which was reflected by the increased ⁴⁵Ca uptake into the cells. At higher concentrations, however, rutheniumred inhibited the ⁴⁵Ca uptake induced by the challenging dose of RTX. When the cellswere washed three times after pretreatment with RTX and rutheniumred, the second phase of the above curve was eliminated (no rutheniumred was present in the assay to block ⁴⁵Ca uptake) (Fig. 3). In these latter experiments ruthenium redinhibited 250 pM RTX-induced desensitization with an ED₅₀ of 14± 2 nM (mean ± SEM for three determinations), a value markedlydifferent (~60-fold difference in potencies) from that determinedfor the inhibition of induction of the ⁴⁵Ca uptake. The ability of ruthenium red to inhibit selectivelythe RTX-induced desensitization is of great importance. It arguesstrongly that the desensitization observed in response to RTXdoes not reflect simply a long-term consequence of limited Ca²⁺ influx occurring at a concentration of ligand below the ED₅₀for stimulation of ⁴⁵Ca uptake.
Fig. 3. Effect of ruthenium red on RTX-induced ⁴⁵Ca uptake and on RTX-induced desensitization in rat DRG neurons. Cells were incubatedin the presence of 250 pM RTX and different concentrations ofruthenium red for 6 hr and then challenged with 200 nM RTX ( $black-square$ ).To evaluate the effect of ruthenium red just on desensitization,after the above incubation cells were washed three times withserum-free DMEM containing 0.25 mg/ml BSA to remove the pretreatmentcompounds before the cells were challenged to induce ⁴⁵Ca uptake ( $down-triangle$ ). To measure the effect of ruthenium red just on⁴⁵Ca uptake, varying concentrations of ruthenium red and 200 nMRTX were applied together, and ⁴⁵Ca uptake was determined ( $open circle$ ). Points represent mean values fromsets of eight determinations in a single experiment; error barsindicate SEM. The theoretical curve for blocking the RTX-induced⁴⁵Ca uptake was calculated by fitting the measured values to themodified Hill equation, whereas data for blocking the RTX-induceddesensitization was fitted to the Hill equation. Two additionalexperiments yielded similar results.
[View Larger Version of this Image (25K GIF file)]

The motivation for the above studies was to determine whether we could identify any responses that were coupled to the vanilloidreceptor subtype detected by [³H]RTX binding. We conclude that this receptor subclass is associatedwith desensitization of subsequent ⁴⁵Ca uptake in response to vanilloid challenge. These studies donot address the converse issue, whether the vanilloid receptorsubtype detected by ⁴⁵Ca uptake can also induce desensitization. We therefore treatedthe cultured DRG neurons with capsaicin, which is selective forinducing ⁴⁵Ca uptake and has weaker affinity for the receptor defined byspecific [³H]RTX binding, and we determined the effect of capsaicin pretreatmenton the subsequent ⁴⁵Ca uptake induced by vanilloid challenge. The stimulation of ⁴⁵Ca uptake was inhibited by capsaicin pretreatment with an ED₅₀of 445 ± 46 nM (Fig. 4A). This value compares closely with theED₅₀ for induction of ⁴⁵Ca uptake by capsaicin, 316 ± 47 nM, and is thus markedly lowerthan that for inhibition of [³H]RTX binding by capsaicin (K_i of 4.9 µM) (Acs et al., 1996).Furthermore, capsaicin induced desensitization in a noncooperativemanner (with a Hill coefficient of 0.89 ± 0.15; mean ± SEM forthree experiments), similar to its action on inducing ⁴⁵Ca uptake (see above) and in contrast to the displacement of [³H]RTX binding (Hill coefficient of 1.81) (Acs et al., 1996).
Fig. 4. A, Comparison of dose-response curves for induction of ⁴⁵Ca uptake, desensitization, and displacement of [³H]RTX binding by capsaicin in rat DRG neurons. Data are expressedas dpm/well values over baseline for capsaicin-induced ⁴⁵Ca uptake ( $open circle$ ). In the case of desensitization ( $black-square$ ), cells werepretreated with different concentrations of capsaicin for 6 hrand then challenged with 3 µM capsaicin. Desensitization was definedas the difference (in dpm/well) in ⁴⁵Ca uptake between pretreated and control cells challenged withcapsaicin. For comparison, the capsaicin dose-response curve fordisplacement of [³H]RTX binding (dotted line), determined previously by us (Acset al., 1996), was plotted. Points represent mean values fromsets of eight determinations in a single experiment; error barsindicate SEM. The theoretical curves were calculated by fittingthe measured values to the Hill equation. Two additional experimentsin each case yielded similar results. B, Extracellular Ca²⁺ dependence of the capsaicin-induced desensitization of rat DRGneurons. Cells were incubated with either 250 pM RTX or 1 µM capsaicinfor 4 hr in medium that contained 1.8 mM, 0.9 mM, or 0.45 mM Ca²⁺. After incubation, cells were washed with serum-free DMEM containing1.8 mM Ca²⁺ and challenged with 3 µM capsaicin to induce ⁴⁵Ca uptake. Data were expressed as percentage values of control⁴⁵Ca uptake determined on untreated cells in the same medium. Theexternal Ca²⁺ dependence of desensitization is indicated by the return of the⁴⁵Ca uptake response. Points represent mean values from sets ofeight determinations in a single experiment; error bars indicateSEM. Two additional experiments yielded similar results.
[View Larger Version of this Image (19K GIF file)]

We next compared the dependence of the desensitization induced by either RTX or capsaicin on the concentration of Ca²⁺ in the medium. Because the DRG neurons show toxicity to prolongedincubation in the absence of extracellular Ca²⁺, we determined that desensitization in media containing decreasedCa²⁺ concentrations after 4 hr preincubation (Fig. 4B). Desensitizationby 250 pM RTX was not affected by the change in the concentrationof Ca²⁺ in the medium, whereas desensitization by 1 µM capsaicin wasreduced in media containing a decreased concentration of Ca²⁺.

Finally, consistent with the desensitization in response to capsaicin reflecting the induction of ⁴⁵Ca uptake, we compared the ability of ruthenium red to block thecapsaicin and RTX-induced desensitization. We examined concentrationsof ruthenium red that were three- to fourfold the ED₅₀ for blockingRTX-induced desensitization and ⁴⁵Ca uptake (60 nM and 2 µM, respectively). Only the latter concentrationinhibited the desensitization induced by 1 µM capsaicin; in contrast,the desensitization induced by 250 pM RTX was already inhibitedby 60 nM ruthenium red, as expected (Fig. 5). We conclude thatcapsaicin induces desensitization through a mechanism distinctfrom that of RTX. The capsaicin-induced desensitization is linkedto the enhanced Ca²⁺ influx; the RTX-induced desensitization is mediated by the receptordetected by specific [³H]RTX binding.

DISCUSSION
Our findings cogently argue for the existence of two pharmacologically defined classes of vanilloid receptors, for which wesuggest the designation R(TX)-type and C(apsaicin)-type. The distinctpharmacology of these two receptor subclasses had already beendemonstrated in our comparison of [³H]RTX binding and ⁴⁵Ca uptake in intact DRG neurons (Acs et al., 1996). In the presentstudy, we have extended the evidence by showing that a biologicalresponse, desensitization in response to RTX, quantitatively agreeswith the pharmacology for the R-type receptor. We further showthat ruthenium red, a noncompetitive vanilloid antagonist, showsmarkedly different affinity for blocking responses through theR- and C-type receptors.

A critical issue was whether the desensitization induced by RTX could simply have been a consequence of a low level of ⁴⁵Ca uptake induced by RTX occupying a small fraction of the C-typereceptors. Three findings argue against this explanation. First,ruthenium red was much more potent for blocking the RTX-induceddesensitization compared with ⁴⁵Ca uptake. Second, the RTX-induced desensitization showed no dependenceon external Ca²⁺, in contrast to the desensitization by capsaicin. Finally, desensitizationin response to capsaicin was observed only with an ED₅₀ correspondingto that for induction of ⁴⁵Ca uptake, not at a concentration an order of magnitude lower.

Elegant previous studies have established that capsaicin-induced desensitization is largely dependent on external Ca²⁺ (Santicioli et al., 1987; Cholewinski et al., 1993; Dochertyet al., 1996). Our results with capsaicin are consistent withthese observations and provide further support for distinct mechanismsof desensitization mediated by the R- and C-type vanilloid receptors.Obviously, the ability to separate responses through these twopathways in DRG neurons will depend on ligands of appropriateselectivity and on their use at appropriate concentrations. Athigher concentrations, RTX will also act on the C-type receptorsand capsaicin on the R-type. An alternative approach for analysiswould be to find systems in which only one receptor subtype isexpressed. Elsewhere, we will describe characterization of vanilloidresponses in a series of non-neuronal cell lines. In these cells,we observe only C-type receptors and not R-type receptors, andthe C-type receptors display characteristics quantitatively similarto those described here (T. Biro, M. Maurer, S. Modarres, N. E.Lewin, C. Brodie, G. Acs, P. Acs, R. Paus, and P. M. Blumberg,unpublished observations).

Our findings help structure and interpret various observations by multiple groups in the vanilloid field. Szallasi and colleagues(1993) (Goso et al., 1993) have reported previously that specificRTX binding in some preparations, e.g., airways and colon, isof low affinity (K_d values for RTX are 250 pM and 3 nM, respectively)and lacks cooperativity; these characteristics might fit withthese measurements reflecting interaction at the lower affinity,⁴⁵Ca uptake-coupled receptor site. Interpretation had been cloudedsomewhat because of the difficulties in accurately defining thislow-affinity binding and the known variability in the cooperativitydepending on the conditions of membrane preparation (Szallasiand Blumberg, 1993). Like us, Walpole et al. (1996) found differencesbetween the structure-activity relations for ⁴⁵Ca uptake and RTX binding. In their case, however, binding wasperformed on membrane preparations, and because the general trendwas similar for both assays, they concluded that "the potenciesin the ⁴⁵Ca uptake assay are generally about 10-fold lower than bindingpotencies, presumably due to other processes, e.g., uptake intomitochondria being necessary for detection in this assay." Infact, the differences in structure-activity relations are impressive.If one compares the relative potency for binding versus ⁴⁵Ca uptake, the ratio (K_i/ED₅₀) is 0.04 for RTX compared with 15for capsaicin; RTX thus permits a 375-fold better selectivitythan does capsaicin for the high-affinity RTX binding site comparedwith the vanilloid receptor mediating ⁴⁵Ca uptake.

In biological systems, abundant evidence supports distinct structure-activity relations for different biological responsesfor vanilloids (Holzer, 1991). Such differences are evident notonly in comparisons between vanilloids of the RTX and capsaicinclasses, but also within each class. Thus, the vanilloid analogolvanil differentially induces desensitization compared with capsaicin(Dickenson et al., 1990; Dray et al., 1990). The dissection ofpatterns of biological response can be explained most readilyby receptor subtypes, although it is also clear that differencesin pharmacokinetics can complicate interpretation (Maggi et al.,1990).

Cellular studies of others likewise argue for vanilloid receptor heterogeneity. Liu and Simon (1994), for example, characterizedcurrents induced in single sensory neurons in response to capsaicinand RTX. At least one subset of currents was inducible by capsaicinbut not RTX (at the concentration examined), and furthermore,significant differences were found in the desensitization patternsof the different vanilloid-sensitive currents (Liu and Simon,1996).

The findings reported here have important implications. First, the evidence that vanilloids induce the activation of a nonvoltage-dependent,relatively nonselective cation channel in intact cells (Wood etal., 1988; Winter et al., 1990) and in single-channel patch-clamppreparations (Oh et al., 1996) has strongly supported the argumentthat the vanilloid receptor either is, or is closely associatedwith, this ion channel. Our findings suggest that a subset ofvanilloid receptors, namely those corresponding to the RTX selectivesubclass, have a different mechanism. Although further studieswill be required to define the mechanism for the R-type vanilloidreceptor, the potent inhibition of desensitization by rutheniumred argues for the involvement of calcium, consistent with activationof, e.g., the phosphoinositide pathway. In fact, the stimulationof the phosphoinositide pathway in DRG neurons after vanilloidtreatment has already been described (Harvey et al., 1995).

Elegant studies by Walpole and coworkers (1996) have helped define the structural constraints for activity of vanilloids ofthe capsaicin class and, to a lesser degree, those of the RTXclass. Because these analyses have used ⁴⁵Ca uptake as the measure of activity, it is clear that separateevaluation of structure-activity relations at the R-type vanilloidreceptor will be required. Because this latter receptor is coupledto desensitization without ⁴⁵Ca uptake, derivatives optimized for selectivity to this sitemay be of particular potential therapeutic interest. Conversely,vanilloid antagonists selective for the ⁴⁵Ca uptake site should permit enhanced selectivity when used incombination with a vanilloid agonist selective for the R-typereceptor. Indeed, on the basis of our limited knowledge of structure-activityrelations for the RTX-selective vanilloid receptor, we shouldbe able to enhance the selectivity of RTX by a factor of 10 bycoapplication with capsazepine.

FOOTNOTES

Received Feb. 7, 1997; revised April 29, 1997; accepted May 6, 1997.

G. Acs and T. Biro contributed equally to this work.

Correspondence should be addressed to Dr. Peter M. Blumberg, MMTP/LCCTP/NCI, Building 37, Room 3A01, 37 Convent Drive MSC4255, Bethesda, MD 20892-4255.

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