Abstract
Behavioral, electrophysiological, and autoradiographic experiments were done to study the second nociceptive phase in the formalin test. In initial experiments, this second phase was attenuated by 1–10 mg of the NK-1 receptor antagonist CP-99,994, given subcutaneously 10, 30, or 60 min before formalin (n = 8–10) and by 20 μg given intrathecally 20 min after formalin (n = 13); the inactive isomer CP-100,263 was ineffective. In electrophysiological experiments on single dorsal horn neurons in vivo, the excitatory responses to subcutaneous formalin injection (50 μl, 2.5%) were attenuated by subsequent intravenously administration of the NK-1 receptor antagonist CP-96,345 (0.5 mg/kg;n = 8), given 35–40 min after formalin, but not by the inactive enantiomer CP-96,344 (0.5 mg/kg;n = 9). Finally, autoradiographic binding of exogenous [125I]BH-substance P in the lumbar cord was reduced at 5 and 25 min after formalin (50 μl, 1 or 5%), with an intermediate level of reduction at 12 min. These data are interpreted as evidence that the second phase of nociceptive scores in the formalin test is attributable at least partially to tonic activation of NK-1 receptors at the spinal level, whether because of a temporally limited release of substance P, for example only during the first phase, but a slow removal or breakdown of substance P, or, more likely, because of tonic release from primary afferents throughout the second phase. Irrespective of the mechanism, it can be concluded that at least some of the persistent nociceptive effects associated with peripheral inflammation, or at least those provoked by subcutaneous injection of formalin, are mediated via continuous activation of NK-1 receptors at the level of the spinal dorsal horn; this may relate directly to mechanisms underlying prolonged nociceptive pains in humans.
- substance P
- substance P receptor
- NK-1 receptor
- tachykinin
- substance P antagonist
- CP-96,345
- CP-99,994
- nociception
- formalin test
- wide dynamic range neuron
- dorsal horn
- spinal cord
- intrathecal
- binding
- autoradiography
The formalin test is commonly used as a model of acute and tonic pain, and sometimes even of inflammatory or chronic pain, or hyperalgesia. The nociceptive response to injection of dilute formalin into the plantar surface, usually of the hindpaw, consists of an early favoring, biting and licking of the injected paw, then a period of reduced nociceptive responses, and finally a second period of favoring and licking. More attention has been paid to mechanisms eliciting the second nociceptive phase, perhaps because some pharmacological manipulations that block the first phase tend also to block the second phase, and it has been argued that the second phase must be influenced by central changes induced during the first phase. Thus, the second nociceptive phase has been presented as a form of central sensitization. In view of evidence that lidocaine-induced block of the thoracic spinal cord fails to alter nociceptive responses in the formalin test (Coderre et al., 1994), it appears that at least some of the mechanisms giving rise to the second phase responses lie below the thoracic cord. This conclusion is strengthened by the further observation that in rats chronically spinalized at the midthoracic level, nociceptive responses to formalin could still be elicited (Coderre et al., 1994).
At the spinal level, various chemical messengers have been implicated in mediating or otherwise bringing about the second nociceptive phase, including substance P (Ohkubo et al., 1990), which we have been studying for some time. Consistent with a role for substance P in mediating these nociceptive responses, subcutaneous injection of formalin induces the release of substance P in the superficial dorsal horn (McCarson and Goldstein, 1991) and an increase in the number of spinal dorsal horn neurons expressing c-fos, and this increase is reduced by an NK-1 receptor antagonist (Chapman et al., 1996; Tao et al., 1997). In vivo, dorsal horn neurons show similar increases in excitability in response to formalin injection, but both the first and second excitatory phases have been reported to be inhibited by pretreatment with an NK-1 receptor antagonist (Chapman and Dickenson, 1993). Intrathecal administration of substance P increases the nociceptive scores during the second nociceptive phase (Ohkubo et al., 1990; Coderre and Yashpal, 1994; although see Mjellem-Joly et al., 1992; Sakurada et al., 1993a). This second phase is reduced by administration of a substance P (NK-1) receptor antagonist (Yamamoto and Yaksh, 1991; Yashpal et al., 1993). Importantly, the antagonism of the second phase response by NK-1 receptor antagonists has been reported to occur only when these antagonists are administered before the formalin is injected (Yamamoto and Yaksh, 1991; Traub, 1996), prompting the suggestion that substance P is involved in the generation but not the maintenance of the hyperalgesia (Yamamoto and Yaksh, 1991;Traub, 1996).
Although this evidence ties substance P to processes in the spinal cord referred to generally as central sensitization, other evidence suggests a peripheral contribution to nociceptive responses in the second phase of the formalin test, raising the possibility of continuous release of substance P during this second phase. Nerve block of the first phase did not influence the second phase response (Dallel et al., 1995). Systemic (Abbadie et al., 1997) or hindpaw (Coderre et al., 1990) administration of a local anesthetic after formalin injection depresses the second phase response. Recordings from primary afferents indicate that injection of formalin into the receptive field produces a biphasic activation of A and C fibers with a time course parallel to the behavioral response to formalin injection (McCall et al., 1996; Puig and Sorkin, 1996). A conclusion from these studies is that the second phase cannot be entirely caused by central sensitization (Dallel et al., 1995).
Thus, to determine whether tonic activation of NK-1 receptors contributes to the second phase of the formalin test, an NK-1 receptor antagonist was given after the onset of the second phase in both behavioral and electrophysiological studies and by measuring the binding of exogenous substance P in the dorsal horn at different times after injection of formalin (Yashpal et al., 1994).
Some of the results have been presented in abstract form (Yashpal et al., 1996).
MATERIALS AND METHODS
In all cases, the guidelines described in The Care and Use of Experimental Animals of the Canadian Council of Animal Care, Vols. 1 and 2, were strictly followed. In addition, all animal protocols were examined and approved by the Animal Care Committees of McGill University and of the Clinical Research Institute of Montreal.
Behavioral studies
Male Sprague Dawley rats (300–400 gm) were used.
Formalin test. In this paradigm, each rat was given a subcutaneous injection of 50 μl of 2.5% formalin into the plantar surface of one hindpaw using a 27 gauge syringe needle. Each rat was then immediately placed in a Plexiglas box (30 × 30 × 30 cm) positioned over a mirror angled at 45° to allow an unobstructed view of the paws by the observer. Observations to determine nociceptive responses began after placing the rat into the box and continued for the next 60 min. A nociceptive score was determined for each 5 min block during that period by measuring the amount of time spent in each of four behavioral categories: 0, treatment of the injected hindpaw is indistinguishable from that of the contralateral paw; 1, the injected paw has little or no weight placed on it; 2, the injected paw is elevated and is not in contact with any surface; 3, the injected paw is licked, bitten, or shaken. Then, a weighted nociceptive score, ranging from 0 to 3 was calculated by multiplying the time spent in each category by the category weight, summing these products, and dividing by the total time for each 5 min block of time.
Subcutaneous administration of CP-99,994 before formalin injection. Eight groups of rats were used to determine the optimal dose and the optimal time of administration of (+)-(2S,3S)-3-(2-methoxybenzylamino)-2-phenylpiperidine (CP-99,994) in the formalin test. Information on the synthesis, properties, and bioavailability of this antagonist has been reported (McLean et al., 1993). CP-99,994 was injected subcutaneously in doses of 1, 5, and 10 mg/kg in a volume of 0.1 ml/100 gm of body weight. In the first series of experiments, CP-99,994 was given subcutaneously 30 min before formalin injection. Control rats were given a subcutaneous injection of saline (0.9% NaCl). Nociceptive scores were measured from the time of formalin injection for 50 min.
In a second series, 5 mg/kg of CP-99,994 was given 10 or 60 min before formalin injection (as compared with 30 min in the previous experiment), and nociceptive scores were measured for 50 min following the formalin injection. Rats were otherwise treated the same as in the previous groups.
Intrathecal administration of CP-99,994 and CP-100,263 before formalin injection. CP-99–994 was administered intrathecally 20 min after formalin injection, with the rationale to determine whether the second phase could be blocked once the response had started. In this experiment each rat was implanted with a chronic indwelling intrathecal catheter (Intramedic PE-10) under chloral hydrate anesthesia (300 mg/kg, i.p.). This catheter was inserted through an incision in the dura at the atlanto-occipital junction and was positioned so that the inner tip lay at the lower lumbar vertebral level. Spinous processes were used as landmarks for this positioning (Yashpal et al., 1985). The outer end of the catheter was fixed with dental cement to a screw embedded in the skull. The exact location of the inner tip of the catheter was verified routinely during postmortem examination. Results were included only if the tip of the catheter was confirmed to lie at the lumbar level. In addition, the viability of the intrathecal catheter was checked by injecting 20 μl of lidocaine (a 1% aqueous solution) the day before testing; implantation was considered to have been successful in rats showing motor and sensory loss within 2 min of administration of lidocaine and a reversal of these effects within 5–10 min. The rats were allowed to recover for 4–6 d after implantation of the catheter, and only those animals that were free of any neurological deficit were used in the experiments. CP-99,994 or its inactive isomer CP-100,263 was given intrathecally in a single dose of 20 μg in 10 μl of artificial CSF [an aqueous solution of (in mm) 128.6 NaCl, 2.6 KCl, 1.0 MgCl2, and 1.4 CaCl2, phosphate buffered to pH 7.33]. This was followed by an additional 10 μl of CSF to flush the catheter (approximate internal volume was 8 μl). CSF replaced the drug solution in control rats.
Data analysis. Nociceptive scores over the 5 min time blocks were analyzed using repeated measures ANOVA, with comparisons between experimental groups and the control group at each time interval using Dunnett’s post hoc t test and between experimental groups using Newman–Keuls’ post hoctest.
Electrophysiological studies
Experiments were done on adult, male Sprague Dawley rats from Charles River (St. Constant, Quebec, Canada).
Animal preparation. Male Sprague Dawley rats (350–375 gm) were anesthetized with sodium pentobarbital (50 mg/kg, i.v.; Abbott Laboratories, Montreal, Quebec, Canada). The right common carotid artery and jugular vein were catheterized for continuous monitoring of arterial pressure and for injection of drugs, respectively. Spinal cord segments L1 to L3were exposed for recording. The spinal cord was transected at the T9 vertebral level to eliminate supraspinal influences on the activity of lumbar dorsal horn neurons. Just before transection, lidocaine (0.05 ml of 1%; Astra Pharma, Mississauga, Ontario, Canada) was injected into the spinal cord at the level of transection to minimize spinal shock. The rats normally breathed spontaneously, and if the breathing pattern became irregular or if respiratory arrest occurred, the animal was paralyzed with pancuronium bromide (Pavulon; Organon, Scarborough, Ontario, Canada; 1 mg/kg i.v., supplemented as necessary) and ventilated mechanically according to standard parameters (Kleinman and Radford, 1964). The spinal cord was covered with mineral oil (Marcol 72; Imperial Oil Limited, Montreal, Quebec, Canada) at 37.5°C to prevent drying. The temperature of the rat was maintained at ∼37.5°C using a heating lamp.
Electrical recording and data acquisition. Single-unit spikes were recorded extracellularly using seven-barrelled (overall tip diameter, 2–4 μm) and single-barrelled (1–2 μm) micropipettes. A solution of 2.7 m NaCl was placed in the recording barrel (impedance 2–4 MΩ measured at 1 kHz with the tip submerged in saline). Single-unit recordings were made at depths ranging from 250 to 1300 μm in the dorsal horn, representing all laminae of the dorsal horn; effects were without any clear differentiation as to sensitivities depending on depth. The raw data were amplified 10,000 times (DP-301 Differential Amplifier; Warner Instrument Corporation), displayed on an oscilloscope (Tektronix 5111), and stored on video cassette tapes using a digital data recorder that incorporated a digital pulse code modulation technique (VR-100A; Instrutech Corporation) and a conventional video cassette recorder. The signals were also relayed to a frequency counter/gating unit, which discriminated single units, based on spike amplitude, and counted the number of spikes per unit time (bin widths were 1 sec). All recordings were from single units. Sampling of extracellular recordings was done using the electrophysiological data acquisition program Spike 2 (version 2.02; Cambridge Electronic Design, Cambridge, UK) on an IBM Pentium computer. The rate of discharge (the output of the gating unit) was displayed continuously on a Grass 79D polygraph.
Functional classification of dorsal horn neurons. Functional classification of neurons was based on the responses to stimulation of their receptive fields in the ipsilateral hind limb by both noxious and innocuous stimuli. The following natural peripheral stimuli were used: (1) an air stream passed over the receptive field at a strength only sufficient to move the hairs, (2) light touch, (3) moderate pressure, (4) noxious mechanical stimulation using a calibrated clip (21 N), and (5) noxious thermal stimulation (measured to be 50°C) using radiant heat. During experimentation, classification of the identified neurons was in three categories (Henry, 1976): (1) non-nociceptive neurons that responded only to non-noxious stimuli such as hair deflection, touch, and/or pressure (some receptive fields on the rat hindlimb did not have hair), (2) wide dynamic range neurons that responded to both noxious and innocuous stimuli, and (3) nociceptive-specific neurons that responded only to noxious mechanical and/or thermal stimulation. In addition, all the units that responded to the “noxious” range of mechanical and/or thermal stimulation showed a characteristic afterdischarge, as described previously (Henry, 1976). Non-nociceptive neurons were not used in this study; thus only wide dynamic range and nociceptive specific neurons were tested with formalin injection into the cutaneous receptive field. The sites of injection of formalin are represented schematically in the figures.
Formalin injection. Once stable ongoing activity of a wide dynamic range or nociceptive specific neuron was obtained, the receptive field of the ipsilateral hindpaw was injected with 50 μl of 2.5% formalin subcutaneously using a 27 gauge syringe needle. Only one such injection was made in each experiment.
Drug administration. The nonpeptide NK-1 receptor antagonist, (2S,3S)-cis-2-(diphenylmethyl)-N-[(2-methoxyphenyl)methyl]-1-azabicyclo[2.2.2]octan-3-amine (CP-96,345) was administered intravenously 35–40 min after subcutaneous injection of formalin into the plantar receptive field of the hindpaw; information on the synthesis, properties, and bioavailability of this antagonist has been reported (McLean et al., 1991; Lowe et al., 1992). This time was considered appropriate as it was generally shortly after onset of the second phase of the excitatory response to subcutaneous injection of formalin. The rationale was to determine whether the second phase could be reversed once it had begun. CP-96,345 was administered intravenously in a single dose of 0.5 mg/kg in saline. The inactive isomer CP-96,344 was given at the same dose in a similar manner in another group of rats. The results of both groups of rats were compared with responses of a control group that received no pharmacological manipulation beyond the formalin injection.
Data analysis. The total number of spikes was counted for 5 min periods, beginning 5 min before formalin injection; this prestimulus period thus represented the baseline level of activity. The mean of these counts for each period was calculated for each group of animals.
To calculate the effects of drug administration, neuronal activity in the 5 min period ending when formalin was injected was normalized to 100%. Thus, the effects of CP-96,345, CP-96,344, or no pharmacological manipulation on neuronal activity subsequent to the injection were determined relative to the neuronal activity at that time.
To calculate significance, the mean ± SEM percent values of the 5 min periods throughout the testing period of the formalin response of each of the three groups were compared with each other. Statistical analysis of the data was done using one-way ANOVA and Student–Newman–Keuls test. A difference in responses between groups was considered significant with a p value < 0.05.
Autoradiographic studies
Long–Evans hooded male rats, weighing 300–350 gm, were used in these experiments.
Behavioral studies. The methods followed for the formalin test were the same as those described above, with the exception that the concentration of formalin was 1 or 5%.
Autoradiography. Following injection of either 1 or 5% formalin, the rats were decapitated at 5, 12, 25, or 60 min. Control rats were not given the formalin injection. Each group consisted of 3 or 4 animals. After decapitation, the spinal cords were rapidly removed and snap frozen in 2-methylbutane at −40°C. Blocks of lumbar cord were mounted on cryostat chucks and cut into 20 μm sections at −18°C. Sections were mounted on slides, dried overnight in a desiccator at 4°C, and stored at −80°C. For the binding procedures, tissue sections were incubated for 90 min at room temperature in a buffer containing 50 mm Tris–HCl, pH 7.4, 3 mm MnCl2, 0.02% BSA, 40 μg/ml bacitracin, 2 μg/ml chymostatin, 4 μg/ml leupeptin, and 50 pm [125I]BH-substance P (2200 Ci/mmol; New England Nuclear, Boston, MA) for binding to NK-1 receptor sites. Nonspecific binding was assessed in the presence of 1 μmsubstance P (Peninsula Laboratories, Belmont, CA). At the end of the incubation period, slides were washed four times (1 min each) in Tris–HCl buffer, rinsed in cold distilled water, air-dried, and apposed to Hyperfilms for 7 d. Hyperfilms were developed, and autoradiograms were quantified densitometrically using an MCID (Imaging Research, St. Catharines, Ontario, Canada) image analysis system. The optical densities from laminae I and II of the dorsal horn of the lumbar spinal cord were converted into semiquantitative values expressed in femtomoles per milligram of tissue wet weight using appropriate radioactive microscales that were coexposed with the radiolabeled sections. All the data are expressed as mean ± SEM, and each value represents the mean of 5–12 sections from three rats.
RESULTS
Behavioral studies
Effects of different doses of CP-99,994 given before formalin injection
Figure 1 illustrates the results obtained from administration of different systemic doses of CP-99,994 on nociceptive scores in the formalin test when the antagonist was given 30 min before formalin injection. In general, there was no effect of any dose on the first phase of the response to injection, measured within the first 5 min. However, the second phase was depressed variably, depending on the dose. The maximum effective dose was 5 mg/kg (n = 10), a dose of 10 mg/kg (n = 8) having no further effect. When 1 mg/kg of CP-99,994 was given (n = 10), only a minor effect was seen. The ANOVA indicated a main effect of dose (F(3,34) = 8.33; p < 0.001) and a main effect of time (F(9,306) = 17.2; p < 0.001). There was also a dose × time interaction (F(27,306) = 2.17; p < 0.001). Post hoc comparisons indicated differences at levels of p < 0.05 and 0.01 at different test times for the different dose groups, as indicated in Figure 1.
Effects of time of preadministration of CP-99,994
Regardless of the time between administration of the antagonist and formalin injection, there was no effect of systemic administration of 5 mg/kg of CP-99,994 on the first phase of the nociceptive response. However, the second phase was depressed, with the greater effect occurring when administration preceded formalin injection by 30 min (n = 10), rather than by 10 (n = 8) or 60 (n = 8) min. The results obtained are illustrated in Figure 2, with the data from the group given 5 mg/kg 30 min before formalin injection taken from Figure 1 for comparison. The ANOVA indicated a main effect of injection time (F(3,30) = 8.19; p < 0.001) and a main effect of test time (F(9,270) = 19.5; p < 0.001). There was also an injection treatment × test time interaction (F(27,270) = 2.36;p < 0.001). Post hoc comparisons indicated differences at levels of p < 0.05 and 0.01 at different test times in the different injection time groups, as indicated in Figure 2.
Effects of intrathecal administration of CP-99,994 or CP-100,263 after formalin injection
At ∼10 min after the second phase had begun, that is 20 min after formalin injection, the intrathecal administration of 20 μg of CP-99,994 (n = 13) induced a rapid decrease in the amplitude of this second phase. When CP-100,263 was given in a similar manner (n = 6), behavioral scores showed the typical pattern. The data are illustrated in Figure3, along with similar data from the control group given CSF (n = 6). There was no significant difference between the three groups up to 20 min after formalin injection. However, in the group treated with CP-99,994 an immediate decrease in nociceptive scores was seen at 25 min, and this group remained lower than the other two groups for the remainder of the testing period. The ANOVA indicated a main effect of treatment (F(1,17) = 10.33; p < 0.001) and a main effect of test time (F(9,153) = 10.06; p < 0.001). There was also a time × test time injection effect (F(9,153) = 3.97]; p < 0.001). Post hoc comparison indicated a difference ofp < 0.05 and 0.01 for the group given CP-99,994 at the times indicated in Figure 3.
Electrophysiological studies
Effects of subcutaneous injection of formalin into the cutaneous receptive field
Subcutaneous injection of 2.5% formalin (50 μl) into the plantar surface of one hindpaw of the rat induced a biphasic excitatory effect on the firing frequency in all nine of the neurons tested (Figs.4A,5A). The first phase began immediately after injection of formalin and persisted for ∼5 min. This was followed by a decrease in neuronal activity that lasted for ∼25–30 min. At this time a second phase of increased activity began. This second excitatory phase was longer-lasting, remaining up to ∼100 min after formalin injection. Figure 4A shows the effect of injection of formalin into the cutaneous receptive field on the firing frequency of a wide dynamic range neuron. The immediate increase in firing rate of wide dynamic range neurons before the first phase response to formalin injection into the receptive field is the excitatory response of the neuron to mechanical pressure of the cutaneous receptive field by the experimenter lightly holding the paw while injecting formalin. This is not a response to formalin because this effect did not occur in nociceptive-specific neurons tested with injection of formalin in the cutaneous receptive field. The biphasic nature and duration of the increased activity following formalin injection was observed in one nociceptive specific neuron and eight wide dynamic range neurons. The firing frequency during the inhibitory period (between the two excitatory phases) was generally greater than the ongoing baseline activity before formalin injection. This was seen consistently in recordings of most neurons (Figs.4A–C, 5A).
Effects of intravenous administration of CP-96,345 or CP-96,344 after formalin injection
Figure 4B illustrates the effect of intravenous administration of 0.5 mg/kg CP-96,345 on the response of a wide dynamic range neuron to subcutaneous formalin injection. CP-96,345 was given at 35–40 min after formalin injection, during the initial part of the increase in neuronal activity of the second phase. CP-96,345 depressed any subsequent increase in neuronal activity. The inhibitory effect of CP-96,345 on the second phase of the formalin response was observed in 9 of the 10 wide dynamic range neurons tested.
Figure 5A reveals a significant depressant effect of CP-96,345 on the second period of excitation in the response to formalin injection. Figure 5B shows the time course of the second phase of the formalin response beginning 40 min after formalin injection, the time of intravenous administration of CP-96,345 or CP-96,344. Each value represents the normalized mean number of spikes for each 5 min period expressed as a percent of the mean number of spikes at 40 min after injection. Comparison of the groups reveals a significant difference in the percent response of neurons between rats given CP-96,345 and those given the inactive isomer CP-96,344 (p < 0.01 at 45, 50, 55, and 60 min). Comparison of the group that received CP-96,345 and the group that received no pharmacological manipulation reveals a significant difference (p < 0.001 at 45 and 50 min;p < 0.01 at 55 and 60 min).
Administration of 0.5 mg/kg CP-96,344 in a similar manner was without effect on the second excitatory phase in any of the eight wide dynamic range neurons tested (Figs. 4C, 5A). The amplitude and duration of the second phase of the formalin response of these neurons in rats given CP-96,344 were no different from the responses of neurons in rats that received no pharmacological manipulation (compare Fig. 4A,C, with Fig.5A,B ).
Binding studies
Behavioral studies
Nociceptive scores following injection of either 1 or 5% formalin to Long-Evans hooded rats are shown in Figure6, A and B, respectively. Both concentrations of formalin induced the typical biphasic nociceptive behavior. The early phase occurred at 5 min and was followed by a period of relatively low nociceptive scores and a subsequent nociceptive phase starting at ∼20 min after formalin injection and continuing beyond the completion of testing at 60 min.
As expected, the response was concentration-dependent. In the group injected with 1% formalin (Fig. 6A), the mean maximum nociceptive score in the first excitatory phase was 1.3, and in the second excitatory phase it was ∼1.5. In the group given 5% formalin (Fig. 6B), the maximum response in the first excitatory phase was 2.2, whereas in the second it was 2.4. There was a significant difference in nociceptive scores between rats given 1 and 5% formalin at 5 min and then from 30 min onward, through the rest of the testing period. Thus, in general, the nociceptive scores after injection of 5% formalin were higher than those after 1%.
Quantification of autoradiograms
Examples of the quantitated images of autoradiograms used for analysis of binding are shown in Figure7. Samples are from an untreated rat from the control group and from individual rats killed at 5, 12, and 25 min after intraplantar injection of 1 or 5% formalin. The image from the control cord shows that binding extended throughout the dorsal horn. The changes in binding are seen in both the superficial and the deep laminae at all time points after formalin injection.
Figure 6, C and D, illustrates the combined data. The histograms show that compared with controls there is less [125I]BH-substance P binding in the dorsal horn of the spinal cords of the groups given 1 or 5% formalin injections. No significant difference was found at any time between these two groups. Quantification of the data show that for both test groups binding of [125I]BH-substance P was significantly lower than in untreated controls at all time periods sampled. ANOVA revealed a significant effect of time after formalin injection for both 1% (F(4,37) = 19.8; p < 0.001) and 5% (F(4,36) = 19.6;p < 0.001) groups.
In the case of 1% formalin, there was no significant difference in binding between 5 and 12 min samples (p > 0.05). However, at 25 and 60 min, binding of [125I]BH-substance P was significantly lower than that at 12 min (p < 0.05). In the case of 5% formalin, the binding at all other times, i.e., at 5, 25, and 60 min, was significantly lower than at 12 min (p < 0.05). Thus, in the 5% group, there was more binding of the exogenous ligand at 12 min than at the other times after formalin injection.
DISCUSSION
Formalin test
The results of this study indicate that when the nonpeptide NK-1 receptor antagonist CP-99,994 is given subcutaneously it has a dose-related depressant effect on the second phase, but not the first phase, of the nociceptive response in the formalin test. The dose–response curve indicates that the maximum effect is reached with 5 mg/kg subcutaneously and that the effect is greatest when the antagonist is given 30 min before formalin is injected into the paw, i.e., 50 min before the second phase begins. These data thus support the earlier suggestion that when NK-1 receptor antagonists are given before formalin injection, they block the second phase but not the first phase of the formalin test (Yamamoto and Yaksh, 1991; Yashpal et al., 1993). The data also indicate, though, that the time of onset of the effects of systemic administration of CP-99,994 is too slow for studies in which NK-1 receptor block is to be attempted after formalin injection.
When CP-99,994, but not the inactive isomer, was given intrathecally after formalin injection, in fact during the second phase, the subsequent second phase nociceptive scores were significantly attenuated. This observation, that the second phase can be reversed by an NK-1 receptor antagonist, differs from that of an earlier study (Yamamoto and Yaksh, 1991), which reported that intrathecal administration of CP-96,345, 5 min after formalin injection, had no effect on the nociceptive scores during the second excitatory phase. This difference regarding reversal of the nociceptive response during the second phase is important. It raises the issue of the mechanisms bringing about the second phase of the nociceptive response to formalin injection, which has variously been attributed to central sensitization and to sustained afferent input. Some investigators have suggested that the second phase is caused in part by short-term input during the first phase (Coderre et al., 1990; Yamamoto and Yaksh, 1992), which causes a so-called central sensitization (Coderre and Melzack, 1992; Yamamoto et al., 1993; Abram et al., 1994; Goto et al., 1994). This central sensitization is sometimes thought to have been produced by glutamate (Coderre and Melzack, 1992; Yamamoto and Yaksh, 1992; Malmberg and Yaksh, 1993; Vaccarino et al., 1993) and/or substance P (Yamamoto and Yaksh, 1991; Traub, 1996) released during the first phase. This concept is inconsistent with the time course of the effects of substance P when applied by iontophoresis onto single neurons in vivo (Henry, 1976) and on the tail flick reflex when given intrathecally (Yashpal et al., 1982; Cridland and Henry, 1986). In both paradigms the effects peak at ∼1 min, rather than at 20–60 min as this interpretation would suggest. Nonetheless, our data are supported by a recent publication reporting that administration of CP-99,994 after intra-articular injection of inflammatory agents blocks the ensuing decrease in paw withdrawal latency and the pain-related behaviors (Sluka et al., 1997).
Other investigators have suggested that the second phase may be caused by continued afferent fiber input throughout the period of the second phase. This suggestion came because subcutaneous injection of formalin causes C-fiber primary afferents to discharge in two phases, which correspond temporally to the two phases of the behavioral responses to formalin injection (Dallel et al., 1995; McCall et al., 1996; Puig and Sorkin, 1996). This suggestion is strengthened by the observation that in the formalin test in the gerbil, systemic administration of an NK-1 receptor antagonist which crosses the blood–brain barrier inhibits the second phase, whereas an antagonist that does not have access to the CNS is without effect in this test (Rupniak et al., 1996).
Although these two possible mechanisms are not necessarily mutually exclusive, the attenuation of the nociceptive response by the NK-1 receptor antagonist in the present study indicates that the second phase is at least partially caused by tonic actions of substance P or a related ligand at the NK-1 receptor. This may be caused by continuous release of the ligand, to persistence of the ligand in the synaptic cleft or possibly to other mechanisms. Irrespective of this, though, on the basis of the results presented in this study, we propose that the nociceptive scores in the second phase of the formalin test are caused at least in part by continuous activation of NK-1 receptors.
Electrophysiological study
Data from the electrophysiological study confirm that subcutaneous injection of dilute formalin into the cutaneous receptive field gives rise to a three-phase response in dorsal horn wide dynamic range neurons. This response consists of (1) an initial excitatory component lasting only a few minutes, followed by (2) a period of reduced activity lasting 25–30 min, and finally (3) a second excitatory response lasting >70 min. The second excitatory response seen here is longer than that reported from other electrophysiological studies (Chapman and Dickenson, 1993; Diaz and Dickenson, 1997). It is also longer than the second phase in the formalin test (Dubuisson and Dennis, 1977), possibly because descending controls were interrupted by the spinal transection in the electrophysiological part of the present study.
More importantly, the results indicate that when CP-96,345 is given during the second excitatory phase, this phase is attenuated. As this effect is not shared by the inactive enantiomer, CP-96,344, the data support the earlier suggestion that activation of NK-1 receptors contributes to this second excitatory phase of the response of dorsal horn nociceptive neurons to subcutaneous injection of formalin in the rat (Chapman and Dickenson, 1993).
Although the earlier study has already implicated NK-1 receptors in the second excitatory phase of the response to injection of formalin on the basis of preadministration of an NK-1 receptor antagonist, the important part of the present electrophysiological study is that it indicates that when CP-96,345 is given after formalin injection, during the onset of the second excitatory phase, this phase is attenuated. Thus, the effects of the antagonist on the second excitatory phase could not have included mechanisms altered during the first excitatory phase. These data therefore parallel the results obtained from the behavioral paradigm of this report. Both series of experiments show a reversal of the second excitatory response to formalin injection when an NK-1 receptor antagonist is given, not before or just after formalin injection, but during the onset of the second phase. This evidence suggests clearly not only the activation of NK-1 receptors following the noxious peripheral stimulus, but it also indicates the continuous presence of a ligand at these receptors throughout the period of recording electrophysiologically or testing behaviorally. Accordingly, the data support the proposal presented above that the second phase is at least partially caused by tonic actions of substance P or a related ligand at the NK-1 receptor, whether this is caused by continuous release, persistence of the ligand in the synaptic cleft, or other mechanisms.
Autoradiographic study
The autoradiographic data indicate an inverse relation between nociceptive scores and binding of exogenous substance P following intraplantar injection of formalin into a rat hindpaw. In view of our previous report that binding of exogenous substance P was decreased by noxious thermal stimulation of a hindlimb (Yashpal et al., 1994), we suggest that this binding is also decreased in the present experiments by noxious chemical stimulation of a hindpaw. Both stimuli provoke a physiological response mediated at the spinal cord level by activation of NK-1 receptors (Yamamoto and Yaksh, 1991; Birch et al., 1992;Yashpal et al., 1993, 1995; Traub, 1996). Thus, the decrease in density of [125I]BH-substance P receptor binding can be presumed to correlate with the release of an endogenous ligand for the NK-1 receptor, such as substance P. Such a proposal is not without precedent. A similar occupation of receptors by an endogenous ligand has been reported for opiate receptors in the brain of the rat (Seeger et al., 1984; Wagner et al., 1990; Ruiz-Gayo et al., 1992).
An interesting difference exists in the time course of the displaced binding between the previous study with noxious thermal stimulation and the present study with noxious chemical stimulation. The noxious thermal stimulus produced a transient response lasting <5 min, and the binding displacement was depressed most at 1 min after the stimulus, with a partial return at 10 min and a full return at 60 min. In the present experiments, the binding displacement also followed the time course of the nociceptive response, in that the nociceptive scores were still elevated 60 min after formalin injection, and displacement of binding continued at ∼40% of control at 60 min. Thus, in each case, the displacement of binding correlated temporally with the physiological response.
The prolonged time course of the decrease in binding in this study suggests that the second phase of the formalin test may be associated with sustained occupation of NK-1 receptors and thus that the second phase may be caused at least in part by continued activation of NK-1 receptors. Although this possibility is at odds with previous reports that administration of the NK-1 receptor antagonist CP-96,345 after injection of formalin into the hindpaw fails to alter the second phase of the nociceptive response (Yamamoto and Yaksh, 1991; Sakurada et al., 1993b; Traub, 1996), the binding data are consistent with our observations in this study that intrathecal administration of CP-99,994 reverses the nociceptive response in the second phase of the formalin test and that systemic administration of CP-96,345 reverses the second excitatory phase of the response of spinal nociceptive neurons to subcutaneous injection of formalin. Therefore, our binding data support the proposal above that the second phase may be caused at least in part by continuous activation of NK-1 receptors.
The present results may also be interpreted to support the concept of tonic input from primary afferents during the second phase because binding displacement, which the previous study showed was not prolonged >10 min (Yashpal et al., 1994), was still occurring in the present study 25 min after formalin injection.
The bilateral decrease in binding is difficult to explain. However, it is consistent with previous reports of bilateral changes in [125I]BH–substance P binding after noxious thermal stimulation (Yashpal et al., 1994), in 2-deoxyglucose metabolic activity following formalin injection (Aloisi et al., 1993), and in a rat model of peripheral mononeuropathy (Mao et al., 1992), as well as c-fos expression after formalin injection (Herdegen et al., 1991) and noxious thermal stimulation (Williams et al., 1990).
General conclusions
Evidence is presented that indicates that the second phase of the responses to subcutaneous injection of formalin is caused at least partially by tonic activation of NK-1 receptors. This is an important consideration as it contradicts the previous suggestion that intrathecal administration of an NK-1 receptor antagonist after formalin injection does not alter the second phase in the formalin test (Yamamoto and Yaksh, 1991; Traub, 1996).
Our data do not allow us to comment directly on whether the tonic activation of NK-1 receptors is caused by tonic release from primary afferents throughout the second phase, to a temporally limited release of substance P, for example only during the first phase, but a slow removal or breakdown of substance P, or to any other mechanism. However, in view of evidence from other laboratories that after injection of formalin into the paw (Puig and Sorkin, 1996) or into the peripheral receptive field (McCall et al., 1996) C-fiber afferent activity shows a biphasic excitation similar in time course to the two phases of the formalin test. In addition, when lidocaine was given into the formalin injection site just before formalin was given, the first phase was blocked, yet the second phase still occurred (Dallel et al., 1995). Thus, tonic activation from primary afferent fibers throughout the second phase seems to be at least one mechanism to account for the second excitatory phase. If this is indeed the case, then it can be concluded that at least some of the persistent nociceptive effects associated with inflammatory inputs, or at least those provoked by subcutaneous injection of formalin, are mediated via continuous activation of NK-1 receptors at the level of the spinal dorsal horn by continuous or tonic primary afferent input. As we indicate in the introductory remarks, the formalin test is often used as a model of acute and tonic pain. The present data support a role of continuous activation of NK-1 receptors in maintenance of tonic pain. Thus, we suggest that the hyperexcitability that characterizes tonic pain (Lautenbacher et al., 1995; Rossi and Decchi, 1997; Bakke et al., 1998) may be at least partly caused by continuous activation of NK-1 receptors (Svensson et al., 1998).
Footnotes
This study was supported by grants from the Canadian Medical Research Council to J.L.H., T.J.C., and J.-G.C. G.M.P. was a student supported by the Royal Victoria Hospital Research Institute, McGill Faculty of Medicine, and the Fonds pour la formation de chercheurs et l’aide à la recherche (Province of Quebec). CP-96,345, CP-96,344, CP-99,994, and CP-100,263 were generously provided by Pfizer Central Research, Groton, CT.
Correspondence should be addressed to Dr. J. L. Henry, Department of Physiology, McGill University, 3655 Drummond Street, Montreal, Quebec, H3G 1Y6 Canada.