Abstract
The expression and contribution of μ (MOPR) and δ opioid receptors (DOPR) in polymodal nociceptors have been recently challenged. Indeed, MOPR and DOPR were shown to be expressed in distinct subpopulation of nociceptors where they inhibit pain induced by noxious heat and mechanical stimuli, respectively. In the present study, we used electrophysiological measurements to assess the effect of spinal MOPR and DOPR activation on heat-induced and mechanically induced diffuse noxious inhibitory controls (DNICs). We recorded from wide dynamic range neurons in the spinal trigeminal nucleus of anesthetized rats. Trains of 105 electrical shocks were delivered to the excitatory cutaneous receptive field. DNICs were triggered either by immersion of the hindpaw in 49°C water or application of 300 g of mechanical pressure. To study the involvement of peptidergic primary afferents in the activation of DNIC by noxious heat and mechanical stimulations, substance P release was measured in the spinal cord by visualizing neurokinin type 1 receptor internalization. We found that the activation of spinal MOPR and DOPR similarly attenuates the DNIC and neurokinin type 1 receptor internalization induced either by heat or mechanical stimuli. Our results therefore reveal that the activation of spinal MOPR and DOPR relieves both heat-induced and mechanically induced pain with similar potency and suggest that these receptors are expressed on polymodal, substance P-expressing neurons.
Introduction
In peripheral tissues, noxious mechanical, thermal, and chemical stimuli are detected by nociceptors and converted to action potentials by lightly myelinated Aδ and nonmyelinated C-fibers (Julius and Basbaum, 2001; Stein and Lang, 2009). Unlike other sensory receptors, most nociceptors are thought to be polymodal (Perl, 1996; Cain et al., 2001) (i.e., sensitive to both heat and mechanical noxious stimuli) (Julius and Basbaum, 2001). Until recently, discrimination between different pain modalities was therefore considered to happen primarily at spinal and/or supraspinal sites (Perl, 2007). Indeed, recent findings revealed that noxious stimuli of various natures specifically activate different neuronal pathways and, consequently, that the distinction between pain modalities would instead occur at the level of primary afferents (Abrahamsen et al., 2008; Cavanaugh et al., 2009; Scherrer et al., 2009). In particular, this model suggests that heat and mechanical sensitivity are processed by distinct subpopulations of primary afferent fibers. Indeed, in mice, a subpopulation of lightly myelinated Aδ fibers (Koltzenburg et al., 1997; Cain et al., 2001) and nonpeptidergic unmyelinated IB4-positive C-fibers (Cavanaugh et al., 2009; Scherrer et al., 2009) were shown to be specific mechanosensitive nociceptors. By contrast, peptidergic IB4-negative C-fibers expressing substance P and calcitonin gene-related peptide preferentially mediate heat sensitivity (Cavanaugh et al., 2009; Scherrer et al., 2009).
Adding to the controversy, Scherrer et al. (2009) had recently reported that, in mice, the δ opioid receptors (DOPRs) were absent from peptidergic nociceptors expressing μ opioid receptors (MOPRs). In support of a role of primary afferents in the discrimination of pain modalities, they further showed that activation of spinal DOPR preferentially inhibits mechanical pain, whereas activation of spinal MOPR preferentially inhibits thermal pain (Scherrer et al., 2009). However, numerous studies have shown that the selective activation of MOPR with [D-Ala2, N-Me-Phe4, Gly5-ol]-enkephalin (DAMGO) injected at the level of the spinal cord can efficiently alleviate both heat-induced (Porreca et al., 1984; Malmberg and Yaksh, 1992; Nagasaka and Yaksh, 1995; Kondo et al., 2005; Scherrer et al., 2009; van Rijn et al., 2012) and mechanically induced pain (Nichols et al., 1995; Sluka et al., 2002; Kondo et al., 2005; Chen and Pan, 2006; van Rijn et al., 2012). Similarly, the activation of spinal DOPR was shown to relieve heat (Stewart and Hammond, 1994; Tseng et al., 1997; Qiu et al., 2000; Cahill et al., 2001, 2003; Morinville et al., 2003; Gendron et al., 2007a,b; Beaudry et al., 2009; Overland et al., 2009; Dubois and Gendron, 2010) and mechanical pain (Miaskowski et al., 1990, 1991; Sutters et al., 1990; Holdridge and Cahill, 2007; Scherrer et al., 2009; Otis et al., 2011). Therefore, a more thorough investigation of the role of spinal MOPR and DOPR and their ability to inhibit various pain modalities is required.
In the present study, we investigated whether spinal MOPR and DOPR differentially regulate thermal and mechanical pain by assessing the effects of intrathecal DAMGO and deltorphin II on both diffuse noxious inhibitory controls (DNICs) and spinal neurokinin type 1 (NK1) receptor internalization triggered by thermal and mechanical noxious stimulations of the rat hindpaws.
Materials and Methods
Animals
Studies in rats.
Adult male Sprague Dawley rats weighting 250–300 g (from Charles River Laboratories) were maintained on a 12 h light/dark cycle. Laboratory food and water were available ad libitum. Experiments were approved by the animal care committees at the Université d'Auvergne-Clermont 1 (Comité d'Éthique en Matière d'Expérimentation Animale Auvergne CE 26-12) and the Université de Sherbrooke (protocol 242-10). All procedures were in compliance with the policies and directives of the Canadian Council on Animal Care and guidelines from both the International Association for the Study of Pain and the Directives of the European Parliament and the Council on the protection of animals used for scientific purposes (Dir.2010/63/UE).
Studies in mice.
Adult male C57BL/6 mice (20–25 g: Charles River Laboratories) were housed in groups of four and maintained on a 12 h light/dark cycle. Laboratory food and water were available ad libitum. Experiments were approved by the animal care committee at the Université de Sherbrooke (protocol 242-10). All procedures were in compliance with the policies and directives of the Canadian Council on Animal Care and guidelines from the International Association for the Study of Pain. The experiments were designed to minimize the number of animals used and their suffering.
Drugs
DAMGO-enkephalin acetate salt (Tocris Bioscience, batch 22; and Sigma-Aldrich, lot BCBB7749), a MOPR-selective agonist, and deltorphin II (Dlt II) (American Peptide, lot M08048T1; and Sigma-Aldrich, lot 079K8741), a DOPR-selective agonist, were dissolved in saline solution (0.9% NaCl). The drugs were injected intrathecally either by lumbar catheterization for electrophysiological studies (5 μg of DAMGO in a volume of 10 μl; corresponding to 9.7 nmol and 8 μg of Dlt II in a volume of 10 μl; corresponding to 10.2 nmol) or lumbar puncture for NK1 receptor internalization studies (5 μg of DAMGO in a volume of 30 μl and 10 μg of Dlt II in a volume of 30 μl; corresponding to 12.7 nmol). To ascertain drug specificity and selectivity, respectively, for MOPR and DOPR, in the electrophysiological studies, naloxone 0.4 mg/kg intravenously, a nonselective opioid antagonist, and naltrindole 4 mg/kg intravenously, a DOPR-selective antagonist, were injected via the jugular vein. Selectivity of DAMGO and Dlt II in the NK1 receptor internalization studies was demonstrated in a previous study (Beaudry et al., 2011).
Electrophysiological recordings
Animal preparation
As previously described (Lapirot et al., 2011), the rats were anesthetized with 2% halothane in a NO2/O2 mixture (2:1). After intramuscular injection of 100 μg atropine sulfate, the trachea was cannulated. The carotid artery and external jugular vein were catheterized. The animals were then paralyzed by intravenous perfusions of vecuronium bromide (2.4 mg/h) and artificially ventilated with volume-controlled pumps (54–55 strokes/min). The levels of O2, N2O, and end-tidal CO2 (3.5–4.5%) were monitored by an anesthetic gas analyzer (Dräger Vamos) during the entire experimental period. These parameters were digitally displayed and under the control of alarms. The arterial catheter was attached to a calibrated pressure transducer (UFI) connected to an amplifier (Stoelting) for continuous monitoring of the mean arterial blood pressure (90–110 mmHg). The analog output from the blood pressure amplifier was connected to a computer data sampling system (Cambridge Electronics Design 1401 computer interface). The heart rate was continuously monitored, and cutaneous vascularization was periodically checked by observing the color of the paw extremities and the rapidity by which they regained normal color after pressure application. The colorectal temperature was kept constant at 38 ± 0.5°C with a feedback-controlled heating blanket. The surgical level of anesthesia was verified by a stable mean arterial blood pressure and a constant heart rate during noxious stimulation.
The animals were placed in a stereotaxic frame with the head fixed in a ventroflexed position (incisor bar dropped 5 mm under the standard position) by means of an adapted metallic bar. For spinal trigeminal subnucleus oralis (Sp5O) recordings, a craniotomy was performed on the right side at the level of the occipitoparietal suture, and the dura mater was removed.
For the lumbar catheterization, a 2 cm longitudinal skin incision was made directly over the L5–L6 lumbar vertebrae. The subcutaneous soft tissue was eliminated, and the skin incision was drawn to the dorsal midline. The paravertebral muscles were separated to expose the L5 and L6 vertebrae. A curved Friedman-Pearson rongeur (F.S.T.) was used to break the spinal crest of the L6 vertebrae and then expose the dura. We cut a rat intrathecal polyurethane short catheter (Alzet, Durect) into 4.5-cm-long 28G tubing. A Teflon-coated, stainless steel stylet guided the catheter into the subarachnoid space from the lumbar spinal column (L5–L6) to the thoracic spinal column (T12–T13). DAMGO (5 μg) or Dlt II (8 μg) was injected via this catheter over a period of 2 s. Appropriate placement of the catheter was verified by dissecting the animals at the end of the experiment. After the surgery, the level of halothane was reduced to 0.6–0.7% and maintained during the entire recording period.
Recordings
Unitary extracellular recordings were made from the right Sp5O with glass micropipettes (7–10 MΩ) filled with a mixture of 5% NaCl and pontamine sky blue. The brainstem was explored 2.4–3.0 mm laterally to the midline and between the frontal planes AP −1.1 and AP −2.6 mm from the interaural line (Paxinos and Watson, 1997). Single-unit activities were amplified and displayed on oscilloscopes. The activities went into a window discriminator connected to a CED 1401plus interface (Cambridge Electronic Design) and a PC computer (Spike 2.06 software), which allowed sampling and analysis of the spontaneous and evoked neuronal activity. Wide-dynamic range (WDR) neurons were recognized based on their responses to mechanical non-noxious (brushing with a soft brush) and noxious (pinch with forceps) stimulations of their receptive fields as previously described (Dallel et al., 1999). Specifically, each neuron that responded in a graded manner with increasing firing rates to the stimulus range from non-noxious to noxious intensity was classified as a WDR cell. Once a neuron was identified, electrical square-wave stimuli (2 ms duration) were applied through a pair of stainless steel needle electrodes subcutaneously placed into the center of the receptive field; the thresholds for eliciting A- and C-fiber-evoked responses were determined. In poststimulus time histograms (PSTHs), A- and C-fiber-evoked responses were distinguished by their latencies, but only C-fiber-evoked responses were considered in the detailed analysis. Previous research showed that burst discharges at latencies >30 ms are elicited by C-fibers (Hu, 1990; Dallel et al., 1999). Therefore, all spikes occurring between 30 and 200 ms after a stimulus were considered to be C-fiber-evoked.
Experimental design
Sequences of 105 electrical stimuli (0.66 Hz) were applied to the receptive field at 3 times the threshold for C-fiber activation every 10 min. DNICs were triggered by alternatively immersing one hindpaw into a 49°C water bath or applying a mechanical pressure of 300 g to the other hindpaw with calibrated forceps between the 36th and 60th stimuli (i.e., for 37.5 s) (see Fig. 1A). The pressure of 300 g was determined from pilot electrophysiological experiments, which showed that this was the minimal pressure required to induce a reduction of at least 40% of C-fiber-evoked action potentials. This pressure is also in the range of the pressures reached in the Randall-Selitto's test in which 400 g (Chen and Pan, 2006; Sibilia et al., 2012) or higher pressures (Miaskowski et al., 1991; Muthuraman and Singh, 2011) are commonly used as a cutoff. Only one hindpaw at a time received a noxious stimulation, and the order of application of the noxious stimulation was alternated for each animal. For example, for one animal, we began with the thermal stimulus and then proceeded with the mechanical stimulus. For another animal, we instead began with mechanical stimulation, followed with thermal stimulation and so forth. Thus, when all the tested animals were considered, the effects of 5 μg DAMGO or 8 μg Dlt II on both heat-induced and mechanically induced DNICs were tested 10, 20, 30, and 40 min after the administration of the opioid. To ascertain the drug specificity in the observed effects, naloxone (0.4 mg/kg intravenously), a nonselective opioid receptor antagonist, was injected 50 min after the administration of DAMGO in animals. For the Dlt II-injected rats, naltrindole (4 mg/kg intravenously), a DOPR-selective antagonist, was used.
The analyses were performed as previously described (Lapirot et al., 2011). Briefly, in each sequence, the PSTHs determined from the 21st to 35th responses were used for studying the unconditioned response (before noxious stimulation; control period), and those derived from responses 36th to 105th were used for studying the DNICs. To assess the inhibitory effect of noxious heat or a mechanical stimulus, only the 46th–60th responses were considered because responses induced between the 36th–45th noxious stimuli correspond to the time required (5–10 s) to reach the maximal inhibitory effects. In each sequence, PSTHs derived from the 46th–60th (DNIC effect) were normalized to PSTHs derived from the 21st to 35th responses (unconditioned response; control period). The inhibitory effect of the DNIC was computed as the percentage decrease in the number of C-fiber-evoked action potentials.
DAMGO (5 μg in 10 μl) or Dlt II (8 μg in 10 μl) was intrathecally injected after two stable control sequences were recorded (i.e., variation in unconditioned C-fiber response <10%). Each rat received only one injection of DAMGO or Dlt II.
NK1 receptor internalization
Animal perfusion
Studies in rats.
The animals were deeply anesthetized in an induction cage with 5% isoflurane–95% medical air mixture (the anesthetic used in Sherbrooke) and maintained during the entire procedure with 2% of the same anesthetic distributed via a mask. In those experiments, DAMGO (5 μg in 30 μl), Dlt II (10 μg in 30 μl), or saline was administered via direct lumbar puncture using a technique with a high success rate that was previously described by others (Fairbanks, 2003) and extensively used in our laboratory (Beaudry et al., 2009, 2011; Otis et al., 2011). Briefly, a 30-gauge 0.5-inch needle mounted on a Luer tip Hamilton syringe (VWR) was inserted into the L5–L6 intervertebral space of the anesthetized animal (at the level of the cauda equina), and the injection was performed over a period of 2 s. Appropriate placement of the needle was confirmed by observing a brief twitch of the tail. DAMGO, Dlt II, or saline was intrathecally injected 10 min before application of either heat stimulation at 49°C or a mechanical pressure of 300 g for 38 s on the right hindpaw. As previously described (Beaudry et al., 2011), 10 min after the noxious stimulation (i.e., 20 min after DAMGO, Dlt II, or saline injection), the animals were perfused through the aortic arch with 500 ml of 4% PFA and 0.18% picric acid in 0.1 m phosphate buffer with pH 7.4 at 4°C. The spinal cord was then removed, postfixed in the same solution for 1 h, and cryoprotected for 48 h in a solution of 30% sucrose in 0.2 m phosphate buffer. The lumbar segment of the spinal cord was snap frozen in isopentane at −45°C and stored at −80°C until sectioning. The lumbar segments of the spinal cord were sliced in transverse sections (30 μm thick) on a frozen microtome, and immunolabeling of NK1 receptors was performed on free-floating sections. Briefly, the slices were incubated for 30 min at room temperature in 1% sodium borohydride diluted in PBS to quench aldehyde-induced fluorescence present in tissues and thoroughly rinsed. The sections were incubated overnight at 4°C in a rabbit anti-NK1 receptor polyclonal antibody (directed against the C-terminal of NK1 receptors of rat origin, amino acids 393–407; Sigma-Aldrich) diluted 1:5000 in a solution containing 3% normal goat serum and 0.3% Triton X-100 in PBS. The slices were washed in PBS and then incubated with a fluorescent goat anti-rabbit secondary antibody (Alexa-488, Invitrogen) diluted 1:1000 in PBS for 1 h at room temperature.
Studies in mice.
Mice were deeply anesthetized as described for rats. They then received a noxious heat (immersion in a 49°C water bath) or mechanical (application of a 200 g pressure) stimulation for 38 s on their right hindpaw. Ten minutes after mice had received the noxious stimulation, they were intracardially perfused with 30 ml of 4% PFA and 0.18% picric acid in 0.1 m phosphate buffer with pH 7.4 at 4°C. The spinal cord was then removed, postfixed in the same solution for 2 h, and cryoprotected for 48 h in a solution of 30% sucrose in 0.2 m phosphate buffer. The lumbar segment (L4–L6) of the spinal cord was snap frozen in isopentane at −45°C and stored at −80°C until sectioning. The dorsal part of the L4–L6 spinal cord segment was cut on a cryostat into 8–10 serial 20-μm-thick horizontal sections to examine superficial laminae I–II. Horizontal sections were directly mounted on HistoBond adhesive microscope slides (VWR), and immunohistochemistry was performed directly on the slides. Briefly, the slices were thawed at room temperature before rehydration for 10 min in PBS. They were then incubated for 30 min at room temperature in 0.1 m glycine diluted in PBS to quench aldehyde-induced fluorescence present in tissues and rinsed. The sections were incubated overnight at 4°C, in a humid container, with the anti-NK1 receptor polyclonal antibody (1:5000) solution described above. The slices were washed in PBS and then incubated with the fluorescent secondary antibody (1:1000) solution for 1 h at room temperature.
The proportion of spinal cord neurons exhibiting internalized NK1 receptors was quantified by a previously described method (Abbadie et al., 1997; Marvizon et al., 2003; Kondo et al., 2005; Nazarian et al., 2008; Beaudry et al., 2011). Briefly, we used an epifluorescence microscope (Leica DM4000B; Leica Microsystem) to count NK1 receptor-like immunoreactive cell bodies. Neurons with and without NK1 receptor internalization located in the superficial lamina I were counted, and the percentage of NK1 receptor immunoreactive cells with internalization was calculated. The number of neurons with NK1 receptor internalization was determined by averaging the counts made in 3–5 rats per condition (14–18 sections per animal) or 4 or 5 mice per condition (3–6 sections per animal). During the counting procedure, the observer was unaware of the treatment received by the animals. A neuron was considered having internalized NK1 receptors if the membrane was barely labeled and if >50 vesicle-like fluorescent puncta were observed in the cell body. The results were expressed as the mean ± SEM.
For the purpose of illustrating our observations, representative confocal images were collected with the Olympus Fluoview 1000 (FV1000) laser-scanning confocal microscope fitted with an U Plan S-Apo 60× (1.35 NA) oil-immersion objective.
Calculations and statistical analysis
The calculations were performed with Excel 2007 (Microsoft), graphs were created with SigmaPlot 11.0, and statistical analyses were performed with Prism GraphPad 5.0. The data are expressed as the mean ± SEM. p values are presented in the figure legends.
Results
Characteristics of trigeminal WDR neurons
Seventeen WDR neurons were recorded within the Sp5O to test the effect of DAMGO (n = 8) and Dlt II (n = 9) on noxious heat and mechanical stimulations. None of the neurons exhibited spontaneous activity. All of them had ipsilateral receptive fields that included the intraoral or perioral region. They were sensitive to both innocuous and noxious mechanical stimuli and responded by increasing their firing rates as the stimulus intensity increased into the noxious range. When 2-ms-long percutaneous electrical stimuli were applied to the center of the receptive fields of the neurons, responses attributable to peripheral activation of A- and C-fibers could be observed (data not shown). The longest latency responses (89 ± 3.7 ms, n = 17) were C-fiber-evoked. Indeed, the computed conduction velocity (∼0.5 m/s) was in the range of those previously reported for C-fibers (Hu, 1990; Dallel et al., 1999; Coste et al., 2008a,b; Lapirot et al., 2011). In addition, long latency responses could only be evoked by high intensity stimulations (mean threshold, 10.3 ± 0.8 mA, n = 17), and they exhibited windup. Figure 1A illustrates the experimental design used for the electrophysiological assays. As shown in Figure 1 (examples), immersion of the hindpaw in a 49°C water bath (Fig. 1B) or application of a 300 g pressure (Fig. 1C) between the 36th and 60th electrical stimulus induced a strong inhibition of C-fiber-evoked firing of Sp5O WDR neurons. This inhibition reflects the activation of DNICs.
The effects of intrathecal DAMGO and Dlt II injection on the DNIC induced by a noxious heat stimulus
All tested neurons were under the influence of the DNICs. The C-fiber-evoked responses of all those neurons were strongly depressed by the application of noxious heat stimulation (49°C) to one of the hindpaws (Fig. 2A,E, examples).
Regarding the experiments with DAMGO (n = 8), quantitative analysis showed that noxious heat stimulation induced a mean inhibition of 89 ± 4% before the injection of the drug. The intrathecal injection of DAMGO (5 μg) alone (i.e., without the heterotopic conditioning stimulus) has no effect on the C-fiber-evoked responses of trigeminal WDR neurons (Fig. 2B; see also Fig. 4B, between the first and the 36th electrical stimuli), but the injection strongly reduced the inhibitory effect induced by noxious heat stimulation of the hindpaw (Fig. 2B). Ten to 20 and 30–40 minutes after the administration of DAMGO, the inhibitions of C-fiber-evoked responses during heat application were 33 ± 7% and 32 ± 8%, respectively (Fig. 2D). Indeed, spinally administered DAMGO induced reductions of 62 ± 8% and 65 ± 9% of the DNICs (p < 0.0001, F = 20.30, one-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test). The specificity of the effects of intrathecally administered DAMGO upon the DNIC was tested by administering the opiate antagonist naloxone. For all the tested neurons, systemic administration of naloxone (intravenous injection, 0.4 mg/kg) antagonized the effect of DAMGO, indicating that it was opioid receptor-mediated (Fig. 2C,D). Immersion of one of the hindpaw of the rats in the water bath reduced by 87 ± 5% the C-fiber-evoked action potentials of Sp5O WDR neurons. As for DAMGO, the intrathecal injection of Dlt II (8 μg) alone (i.e., without the heterotopic conditioning stimulus) has no effect on the C-fiber-evoked responses of trigeminal WDR neurons (Fig. 2F; see also Fig. 4F, between the first and the 36th electrical stimuli), but the injection strongly reduced the inhibitory effect induced by noxious heat stimulation of one hindpaw (Fig. 2F). Ten to 20 and 30–40 minutes after the administration of Dlt II, the inhibitions of C-fiber-evoked responses during heat application were 36 ± 8% and 55 ± 8%, respectively (Fig. 2H). Indeed, spinally administered Dlt II induced reductions of 56 ± 11% and 38 ± 8% of the DNICs (p < 0.0001, F = 13.81, one-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test). The selectivity of the effects of intrathecally administered Dlt II upon the heat-induced DNIC was tested by administering the DOPR-selective antagonist naltrindole. For all the tested neurons, systemic administration of naltrindole (intravenous injection, 4 mg/kg) antagonized the effect of Dlt II, indicating that it was DOPR-mediated (Fig. 2G,H).
In an interesting way, the effects of spinally administered DAMGO and Dlt II (at equimolar doses), when compared together, show no significant difference in their ability to reduce the activation of heat-induced DNICs (p = 0.1451, F = 2.36, two-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test).
The effects of intrathecal DAMGO and Dlt II injection on heat-induced NK1 receptor internalization
A well-known phenomenon is that, after the activation of peptidergic primary afferent fibers by noxious stimulation, substance P is released in the superficial laminae of the spinal cord, where it binds to and activates NK1 receptors. Upon activation, NK1 receptors are rapidly internalized (Mantyh et al., 1995; Abbadie et al., 1997; Marvizon et al., 2003; Nazarian et al., 2008; Beaudry et al., 2011). NK1 receptor internalization can therefore be used as an indication of the activation of peptidergic primary afferent fibers.
In the ipsilateral side of control rats, immunostaining of NK1 receptors in the rat spinal cord revealed intense immunofluorescent labeling located mainly at the cell surface of laminae I of the lumbar spinal cord (Fig. 3E; see Fig. 5E, first column; 15 ± 2% of lamina I neurons have internalized NK1 receptors). In animals pretreated with intrathecal saline, noxious heat stimulation (immersion of the right hindpaw in 49°C water bath during 38 s) induced NK1 receptor internalization in the majority of the lamina I neurons of the ipsilateral lumbar spinal cord (Fig. 3B,E; 72 ± 4% of laminae I neurons have internalized NK1 receptors). In contrast, only discrete NK1 receptor internalization was observed in the contralateral side of the spinal cord (Fig. 3A). Intrathecal DAMGO (Fig. 3C) and Dlt II (Fig. 3D) administered 10 min before noxious heat stimulation significantly decreased the proportion of neurons with internalized NK1 receptors to 37 ± 4% and 52 ± 3%, respectively (Fig. 3E). Those results correspond to a reduction of ∼49% for DAMGO and 28% for Dlt II, of laminae I neurons with internalized NK1 receptors. We found no significant difference between the effects of DAMGO and Dlt II on their ability to inhibit heat-induced NK1 receptor internalization (Fig. 3E) (p < 0.0001, F = 4.03, one-way ANOVA followed by Bonferroni's multiple-comparison test).
The effects of intrathecal DAMGO and Dlt II injection on the DNIC induced by a noxious mechanical stimulus
C-fiber-evoked responses were strongly depressed by the application of noxious mechanical (300 g) stimulation to the hindpaw (Fig. 4A,E, examples). For assays where DAMGO was tested, quantitative analysis showed a mean inhibition of 56 ± 8% of C-fiber-evoked firing of Sp5O neurons before the injection of the MOPR-selective agonist. After intrathecal injection of DAMGO (5 μg), the DNICs triggered by noxious mechanical stimulation of the hindpaw were strongly reduced (Fig. 4B). Figure 4D illustrates the results of the quantitative analysis. Ten to 20 min and 30–40 min after DAMGO injection, mechanically induced inhibition of C-fiber-evoked responses was 23 ± 9% and 29 ± 7%, respectively. The DNICs were therefore reduced by 64 ± 13% and 53 ± 7% (p < 0.0001, F = 22.90, one-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test). The specificity of the effects of intrathecally administered DAMGO upon the DNIC was tested by administering the opiate antagonist naloxone. For all the neurons tested, systemic administration of naloxone (intravenous injection, 0.4 mg/kg) antagonized the reduction of the DNIC induced by DAMGO (Fig. 4C,D).
In animals where Dlt II was tested (n = 9), application of a 300 g pressure to the hindpaw of the rats before the administration of the DOPR-selective agonist reduced by 57 ± 7% the C-fiber-evoked action potentials of Sp5O WDR neurons. The intrathecal injection of Dlt II strongly reduced the inhibitory effects evoked by noxious mechanical stimulation of the hindpaw (Fig. 4F). Ten to 20 and 30–40 minutes after the administration of Dlt II, the inhibitions of C-fiber-evoked responses during the 300 g pressure application were 28 ± 7% and 46 ± 11%, respectively (Fig. 4H). In brief, spinally administered Dlt II induced reductions of 51 ± 14% and 25 ± 13% of the DNICs. Indeed, the effect of Dlt II is only significant 10–20 min after its administration (p < 0.0002, F = 10.00, one-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test). The selectivity of the effects of intrathecally administered Dlt II upon the heat-induced DNICs was tested by administering the DOPR-selective antagonist naltrindole. For all the tested neurons, systemic administration of naltrindole (intravenous injection 4 mg/kg) antagonized the effect of Dlt II, indicating that it was DOPR-mediated (Fig. 4G,H).
As for thermal stimulation, intrathecal DAMGO and Dlt II have comparable inhibitory effects on mechanically induced DNICs (p = 0.1654, F = 2.13, two-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test).
Interestingly, when the effects of intrathecal injection of DAMGO on the DNICs triggered by either noxious heat or mechanical stimulation were compared, no significant difference was found (p = 0.643, F = 0.2244, two-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test). Similarly, Dlt II was found to inhibit DNICs triggered by either noxious heat or mechanical stimulation with comparable potencies (p = 0.499, F = 0.48, two-way ANOVA for repeated measures followed by Bonferroni's multiple-comparison test).
The effects of intrathecal DAMGO and Dlt II injection on mechanically induced NK1 receptor internalization
As seen for noxious heat stimulation, application of a 300 g pressure induced a strong NK1 receptor internalization (Fig. 5B; 66 ± 5% of ipsilateral lamina I neurons). Only discrete NK1 receptor internalization was observed in the contralateral side of the lumbar spinal cord (Fig. 5A). In animals pretreated with intrathecal DAMGO (Fig. 5C) or Dlt II (Fig. 5D), a significant decrease in the proportion of neurons showing NK1 receptor internalization was observed (Fig. 5E; 33 ± 7% and 38 ± 4%, respectively, for DAMGO and Dlt II, of ipsilateral laminae I neurons have internalized NK1 receptors). This result corresponds to a reduction of ∼50% and 42% of laminae I neurons with internalized NK1 receptors. In addition, there is no significant difference between the effects of DAMGO and Dlt II on inhibition of mechanically induced NK1 receptor internalization (Fig. 5E; p = 0.0002, F = 13.82, one-way ANOVA followed by Bonferroni's multiple-comparison test).
Heat-induced and mechanically induced NK1 receptor internalization in mice
We then studied the effects of noxious heat and mechanical stimuli on the internalization of NK1 receptors in mice. We observed the localization of NK1 receptors after either immersion of the right hindpaw of mice in a 49°C waterbath or application of a 200 g pressure with calibrated forceps for 38 s. As shown in Figure 6, in control mice the NK1 receptor labeling was mostly found at the cell surface (Fig. 6A,D; 14 ± 1% of lamina I neurons had internalized NK1 receptors). Immersion of the hindpaw in the 49°C waterbath induced a strong proportion of internalized NK1 receptors (Fig. 6B,D; 71 ± 2% of neurons). Application of the mechanical pressure also induced a significant internalization of NK1 receptors (Fig. 6C,D; 53 ± 4% of lamina I neurons have internalized NK1 receptors).
Discussion
In the present study, we investigated the role of spinal MOPRs and DOPRs in heat and mechanical pain regulation using electrophysiological and immunohistochemical approaches. By measuring the firing of WDR neurons of the spinal trigeminal subnucleus oralis (Sp5O), we demonstrated that intrathecal administration of either DAMGO or Dlt II, respectively, MOPR- and DOPR-selective agonists, was able to inhibit the activation of DNICs triggered by heat and mechanical noxious stimuli. We further observed that both spinal MOPR and DOPR activation blocks substance P release and inhibits NK1 receptor internalization induced by thermal and mechanical stimuli.
The existence of polymodal nociceptors implies that discrimination of pain modalities occurs at the higher spinal cord level and in the brain (Melzack and Wall, 1962; Perl, 2007). This dogma was, however, recently challenged. Indeed, using pharmacological ablation of mouse sensory neurons expressing the sodium channel Nav1.8 or genetic ablation of Mrgprd-expressing sensory neurons, others revealed that specific pain modalities are encoded by distinct subpopulations of nociceptors (Abrahamsen et al., 2008; Cavanaugh et al., 2009). These findings were further supported by the fact that, in mice, nonpeptidergic IB4-positive DRG neurons were found to specifically mediate the responses to mechanical pain, whereas a subpopulation of IB4-negative neurons mediates thermal pain (Scherrer et al., 2009).
In primary afferents, MOPR are mainly expressed by small IB4-negative peptidergic neurons (Ji et al., 1995; Minami et al., 1995; Zhang et al., 1998b; Wang and Wessendorf, 2001; Rau et al., 2005), whereas DOPR was found to be expressed in large- and small-diameter neurons (Mansour et al., 1994; Wang and Wessendorf, 2001). Although the presence of DOPR in substance P- and calcitonin gene-related peptide-containing neurons has been shown (Ji et al., 1995; Zhang et al., 1998a; Riedl et al., 2009; Wang et al., 2010), enhanced green fluorescent protein-tagged DOPR is confined to nonpeptidergic fibers in knockin mice (Scherrer et al., 2009). In agreement with the hypothesis that specific pain modalities are encoded by distinct subpopulations of nociceptors, it was observed that spinal DAMGO specifically inhibited heat-induced pain whereas activation of spinal DOPR specifically attenuated mechanical stimuli-induced behaviors (Scherrer et al., 2009).
In the current study, we measured the effects of heat and mechanical noxious stimuli applied to the hindpaws of rats on the firing of trigeminal WDR neurons and confirmed previous studies showing the existence of DNIC acting on these trigeminal neurons (Le Bars, 2002; Lapirot et al., 2011). As opposed to stimulus-induced reflex or withdrawal responses studied in most behavioral tests, DNICs can only be triggered by noxious stimuli (Le Bars et al., 1979) and therefore represent an efficient and unbiased strategy to evaluate the analgesic properties of drugs applied intrathecally. Here, we demonstrated that activation of both MOPR and DOPR at the spinal level resulted in a profound decrease in the effects of the DNIC on the firing of WDR neurons. Indeed, intrathecal DAMGO and Dlt II were able to similarly reduce the effects of the DNIC induced by heat or mechanical noxious stimulation of the hindpaw. The fact that intrathecal administration of DAMGO or Dlt II alone had no effect on C-fiber-evoked responses of trigeminal WDR neurons in the absence of heterotopic conditioning stimuli suggests that the reduction of DNIC-induced analgesia does not result from direct action of MOPR or DOPR agonists in the trigeminal nucleus.
The efficacy of MOPR agonists to inhibit mechanical pain in rodents has also been shown by others (Nakazawa et al., 1985; Chaki et al., 1988; Nichols et al., 1995; Kondo et al., 2005; Back et al., 2006; Iwai et al., 2012; Lee et al., 2012). Similarly, a number of studies demonstrated that intrathecal DOPR agonists efficiently alleviate noxious heat-induced behaviors in rats and in mice (Stewart and Hammond, 1994; Tseng et al., 1997; Qiu et al., 2000; Cahill et al., 2001, 2003; Morinville et al., 2003; Gendron et al., 2007a, b; Beaudry et al., 2009, 2011; Overland et al., 2009; Dubois and Gendron, 2010). Lessons from knock-out mice also provided evidence supporting a role for MOPR and DOPR in the modulation of diverse pain modalities. Indeed, both MOPR and DOPR knock-out mice were found to have increased sensitivity to thermal (Sora et al., 1997; Matthes et al., 1998; Qiu et al., 2000; Martin et al., 2003) and mechanical pain (Martin et al., 2003).
In accordance with the polymodal nature of nociceptors, peripheral thermal (Zachariou and Goldstein, 1996; Abbadie et al., 1997; Allen et al., 1997; King et al., 2005), mechanical (McCarson and Goldstein, 1991; Zachariou and Goldstein, 1996; Abbadie et al., 1997; King et al., 2005; Kondo et al., 2005), and chemical (Marvizon et al., 2003; Nazarian et al., 2008; Beaudry et al., 2011) noxious stimulations were shown to evoke the release of substance P in the superficial layers of the rat spinal cord. Interestingly, the blockade of NK1 receptors expressed by spinoparabrachial neurons was previously shown to inhibit DNICs triggered by intraplantar formalin (Lapirot et al., 2009). To determine whether DAMGO and Dlt II can inhibit the release of substance P induced by heat and mechanical noxious stimulation of the hindpaw in rats, we measured NK1 receptor internalization in the superficial laminae of the lumbar spinal cord. As shown previously (Kondo et al., 2005; Zhang et al., 2010), we observed that DAMGO blocked the NK1 receptor internalization induced by noxious mechanical stimulation. We also showed, for the first time, that intrathecal DAMGO decreased the NK1 receptor internalization evoked by noxious heat stimulation of the paw. Similarly, intrathecal Dlt II blocked NK1 receptor internalization induced by heat and mechanical noxious stimuli. The fact that intrathecally injected Dlt II has an effect on NK1 receptor internalization confirms previous reports showing that a subpopulation of substance P-containing nociceptors expresses DOPRs (Ji et al., 1995; Zhang et al., 1998a; Riedl et al., 2009; Wang et al., 2010; Beaudry et al., 2011). Our results also reveal that peptidergic primary afferents are involved in DNICs triggered by noxious heat and mechanical stimulations and that these fibers are regulated by both MOPRs and DOPRs.
One may argue that the apparent discrepancies between our observations and those made by others could be explained by interspecies differences. Indeed, as previously mentioned, a dichotomy between C-fiber subpopulations and pain modalities was observed in mice (Abrahamsen et al., 2008; Cavanaugh et al., 2009; Scherrer et al., 2009). Thus, transient receptor potential vanilloid 1, an important but not unique transducer of thermal nociception (Caterina et al., 2000; Davis et al., 2000; Woodbury et al., 2004), is almost exclusively found in heat-specific peptidergic sensory neurons in mice (Zwick et al., 2002; Woodbury et al., 2004; Lawson et al., 2008; Cavanaugh et al., 2011) while it is found in both peptidergic and nonpeptidergic C-fibers in rats (Gold et al., 1996; Tominaga et al., 1998; Guo et al., 1999; Michael and Priestley, 1999; Woodbury et al., 2004; Yu et al., 2008). Others hypothesized that the observed dichotomy between C-fiber populations and nociceptive modalities; thus, the effects of intrathecal MOPR and DOPR agonists may not apply to rats or higher-order primates (Saeed and Ribeiro-da-Silva, 2012; Taylor et al., 2012). For instance, we observed here that both noxious thermal and mechanical stimuli can induce NK1 receptor internalization in both rats and mice, confirming that peptidergic primary afferents participate in thermal and mechanical nociception in both species.
Alternatively, it is possible that the mechanical stimuli used by Scherrer et al. (2009), namely, von Frey filaments, were not noxious and therefore that paw withdrawals were the consequence of stimulation of non-nociceptive Aδ and/or Aβ-fibers shown to express DOPR. von Frey filaments are indeed commonly used to measure allodynia, that is, pain induced by a non-noxious stimulus (e.g., light touch), in injured or sensitized subjects. As a noxious mechanical stimulus, we rather used a 200 g (mice) or 300 g (rats) pressure applied for 38 s to the hindpaw with calibrated forceps and show that it efficiently recruits mechanical nociceptors, induces the release of substance P by primary afferents and, most importantly, activates DNICs, which are only triggered by noxious stimuli.
In conclusion, our results reveal that the activation of either MOPR or DOPR can equally relieve both pain modalities (i.e., thermal and mechanical), possibly via direct action on peptidergic C-fibers. Admittedly, although we found that spinal DAMGO and Dlt II similarly inhibited the DNIC triggered by heat and mechanical noxious stimuli applied to the hindpaws, other MOPR and DOPR agonists may not be equally potent at inhibiting all pain modalities. As an example, neuropathic pain is often found to be less sensitive than inflammatory pain to MOPR agonists (Arner and Meyerson, 1988; Obara et al., 2009). Despite the fact that we cannot exclude that spinal DAMGO and Dlt II could inhibit multiple subpopulations of selective heat-sensitive and mechanosensitive nociceptors, the current study revealed that peptidergic C-fibers are involved in heat and mechanical pain processing in rodents, a hypothesis recently challenged by others (Cavanaugh et al., 2009; Scherrer et al., 2009).
Footnotes
This work was supported by the Natural Sciences and Engineering Research Council of Canada and the Canadian Institutes of Health Research grants to L.G. and a Laboratory exchange program opportunity grant from the Fonds de Recherche Québec-Santé (FRQ-S)-funded Quebec Pain Research Network to L.G. and R.D. L.G. is the recipient of a FRQ-S Junior 2 salary support. A.N. was the recipient of the Frederick Banting and Charles Best Canada Graduate Scholarships-Master's Award awarded by the Canadian Institutes of Health Research and a Master scholarship from the FRQ-S. This work was also supported by the Institut National de la Santé et de la Recherche Médicale, Université d'Auvergne-Clermont 1 (France) and Région Auvergne. We thank Hélène Beaudry for technical assistance and Robert Dumaine and Philippe Sarret (Université de Sherbrooke) for granting access to the Olympus confocal microscope funded by the Canadian Foundation for Innovation.
The authors declare no competing financial interests.
- Correspondence should be addressed to either of the following: Dr. Louis Gendron, Département de physiologie et biophysique, Université de Sherbrooke, Faculté de médecine et des sciences de la santé, 3001 12th Avenue North, Sherbrooke, QC J1H 5N4, Canada, Louis.Gendron{at}USherbrooke.ca; or Pr. Radhouane Dallel, INSERM UMR 1107, Neuro-Dol, Douleur Trigéminale et Migraine, Faculté de Chirurgie Dentaire, 11 boulevard Charles de Gaulle, 63000 Clermont-Ferrand, France, Radhouane.dallel{at}udamail.fr