Background
Complex regional pain syndrome type I (CRPS) is an often chronic pain condition characteristically disproportionate to the inciting event. The syndrome develops after a range of injuries including fractures, soft tissue trauma to the extremities, or as a consequence of a separate disease process like stroke or myocardial infarction [
1]. In most cases, CRPS has three stages, but CRPS does not always follow this pattern. In many patients, the early symptoms are of a warm, erythematous, swollen, painful limb, the so-called “warm phase” thought to be supported by neurogenic inflammation [
2‐
4]. In the acute phase, cutaneous immunological mechanisms underlying CRPS have been discovered, including autoimmunity [
5], keratinocyte activation, proliferation, and expression of inflammatory mediators such as tumor necrosis factor alpha (TNFα), interleukin-1 beta (IL-1β) and interleukin-6 (IL-6), nerve growth factor (NGF), and mast cell activation [
6,
7]. Substance P (SP), acting through up-regulated neurokinin 1 (NK1) receptors expressed in the peripheral tissues of the involved limb, appears to be a key signaling molecule supporting the signs and symptoms of CRPS [
8,
9]. Over time, however, this acute picture gives way to a cold, dystrophic but still painful limb. Changes with origins clearly within the central nervous system (CNS) such as emotional problems, cognitive changes, and movement disorders can be observed in some patients [
10,
11]. Prospective studies have observed a gradual spontaneous resolution of CRPS symptoms and signs in distal limb fracture cases, with 66 to 80 % of cases completely resolving by 6 months after injury [
12‐
15]. The mechanisms supporting the chronic phases of CRPS are still very poorly understood.
The fracture/cast immobilization rodent model of CRPS displays the principal signs of CRPS including warmth, edema, enhanced neurogenic extravasation, epidermal hypertrophy, bone loss, and nociceptive changes [
16‐
19]. These animals also show an evolution of signs over time to resemble the more chronic phases of CRPS in humans [
17]. Using this model, it has been shown that neuropeptide signaling is particularly important for nociceptive sensitization and cytokine generation in the affected limb 4 weeks after fracture when acute phase changes are present. However, it is unclear whether these peripheral mechanisms continue to contribute to the persistent signs of CRPS in the chronic phases of the model, or whether central changes become the predominant mechanistic factors. Some evidence from CRPS patients suggests that peripheral inflammatory mechanisms may fade with time including levels of skin cytokines and mast cell abundance in skin [
6,
20].
Therefore, in the present study, we hypothesized that the enhanced vascular permeability, edema, warmth, and nociceptive sensitization observed in the rodent CRPS model could be attributed to enhanced peripheral neuropeptide and cytokine signaling in the acute phase, whereas the persistent allodynia observable 16 weeks post fracture would be attributable to NK1 receptor activation and neuroinflammation in the spinal cord. Such findings might enhance our understanding of the evolution of CRPS over time and may suggest approaches to tailoring CRPS treatment to its duration and clinical features.
Methods
These experiments were approved by our institute’s Subcommittee on Animal Studies and followed the guidelines of the International Association for the Study of Pain (IASP) [
21]. Adult (9 months old) male Sprague Dawley rats (Simonsen Laboratories, Gilroy, CA, USA) were used in all experiments. The animals were housed individually in isolator cages with solid floors covered with 3 cm of soft bedding and were fed and watered ad libitum. During the experimental period, the animals were fed Teklad Global 18 % Protein Rodent Diet (
www.Envigo.com, Madison, WI.) and were kept under standard conditions with a 12-h light–dark cycle. For all experiments, animals were randomly assigned to study groups, and observers were blinded to treatment conditions such as drug injections.
Surgery and recovery
Tibial fracture was performed under isoflurane anesthesia as we have previously described [
17]. The right hindlimb was wrapped in stockinet (2.5 cm wide), and the distal tibia was fractured using pliers with an adjustable stop that had been modified with a 3-point jaw. The hindlimb was wrapped in casting tape so the hip, knee, and ankle were flexed. The cast extended from the metatarsals of the hindpaw up to a spica formed around the abdomen. To prevent the animals from chewing at their casts, the cast material was wrapped in galvanized wire mesh. The rats were given subcutaneous saline and buprenorphine (0.03 mg/kg) immediately after the procedure and on the next day after fracture for postoperative hydration and analgesia. At 4 weeks, the rats were anesthetized with isoflurane, and the cast removed with a vibrating cast saw. All rats used in this study had mechanical union at the fracture site after 4 weeks of casting. To study changes in the chronic phase, after cast was removed at 4 weeks, fracture rats were allowed to recover in cages until 16 weeks after fracture prior to behavioral and biochemical testing.
Drugs
The NK1 receptor antagonist LY303870 was a generous gift from Dr. L. Phebus (Eli Lily Company, Indianapolis, IN, USA). This compound has nanomolar affinity for the rat NK1 receptor, has no affinity for 65 other receptors and ion channels, has no sedative, cardiovascular or core body temperature effects in rats at systemic doses up to 30 mg/kg, and is physiologically active for 24 h after a single systemic dose of 10 mg/kg [
22‐
24]. The doses of systemic and intrathecal LY303870 used in the study were based on our prior studies demonstrating analgesic efficacy with these doses in the 4-week post-fracture rat model [
17,
25]. LY303870 (30 mg/kg/day, i.p.) was administered daily for 7 days and one final dose at 1 h prior to testing [
24] or via intrathecal injection (10 μl at 20 μg/μl, 30 min prior to testing). All testing was carried out at 4 and 16 weeks after tibia fracture.
A naturally occurring IL-1-receptor antagonist (IL-1ra) modulates the activity of IL-1β in vivo. Anakinra, a recombinant met-human IL-1ra (r-metHuIL-1ra, Kineret, Amgen) that binds to the IL-1 type I receptor (IL-1 RI), effectively inhibits IL-1β signal transduction [
26]. To test the hypothesis that IL-1β signaling mediates the vascular and nociceptive changes observed after tibia fracture in rats, osmotic pumps (model 2ML4, Alzet) were used for delivering anakinra IL-1ra. The pumps were inserted subcutaneously over the rat’s back. Based on previous studies using IL-1ra in rodents [
27‐
29] and based on discussions with lead scientists from Amgen, it was previously decided to administer 10 mg/kg/day of anakinra via subcutaneous pump for 28 days prior to testing at 4 weeks post fracture. During the present study, we discovered that, at 16 weeks, systemic treatments with LY303870 and anti-NGF lost more than 50 % of their anti-nociceptive effects observed at 4 weeks post fracture. In addition, skin cytokines at 16 weeks, including IL-1β, declined from 4 weeks post fracture, but spinal cord cytokine concentrations at 16 weeks remained high and close to the peak concentration at 4 weeks post fracture. These data suggested that SP signaling and inflammation in the spinal cord at the central level might contribute to nociceptive abnormalities at 16 weeks. To demonstrate the effects of anakinra on fracture-induced nociceptive abnormalities at the spinal cord level, anakinra was administered via a single intrathecal injection (10 μl at 10 μg/μl) at 1 h prior to testing at 4 and 16 weeks post fracture. As a comparison at the systemic level, 100 mg anakinra/kg, one dose i.p. was injected 1 h prior to testing at 16 weeks post fracture. All testing was carried out at 4 and 16 weeks after tibia fracture.
The anti-NGF antibody muMab 911 (Rinat Laboratories, Pfizer Inc.) is a TrkA immunoglobulin G (TrkA-IGG) fusion molecule that binds to the NGF molecule, thus blocking the binding of NGF to the TrkA and p75 NGF receptors and inhibiting TrkA autophosphorylation [
30]. Pharmacokinetic and behavioral experiments in rodents indicate that muMab 911 has a terminal half-life of 5 to 6 days in plasma and that a 10 mg/kg dose administered every 5 or 6 days reduces nociceptive behavior in a variety of rodent chronic pain models [
31‐
34]. Based on these data and discussions with lead scientists at Rinat, it was determined to administer muMab 911 via a single subcutaneous injection (10 mg/kg) 7 days prior to testing or via a single intrathecal injection (10 μl at 1.24 μg/μl) 1 h prior to testing. All testing was carried out at 4 and 16 weeks after tibia fracture.
Hindpaw nociception
To measure mechanical allodynia in the rats, an up-down von Frey testing paradigm was used as we have previously described [
17,
35,
36]. Rats were placed in a clear plastic cylinder (20 cm in diameter) with a wire mesh bottom and allowed to acclimate for 15 min. The paw was tested with one of a series of eight von Frey hairs ranging in stiffness from 0.41 to 15.14 g. The von Frey hair was applied against the hindpaw plantar skin at approximately midsole, taking care to avoid the tori pads. The fiber was pushed until it slightly bowed. Hindpaw withdrawal from the fiber was considered a positive response. The initial fiber presentation was 2.1 g, and the fibers were presented according to the up-down method of Dixon to generate six responses in the immediate vicinity of the 50 % threshold. Stimuli were presented at an interval of several seconds. In addition, to measure hindpaw unweighting, an incapacitance device (IITC Inc. Life Science, Woodland, CA, USA) was used. The rats were manually held in a vertical position over the apparatus with the hindpaws resting on separate metal scale plates, and the entire weight of the rat was supported on the hindpaws. The duration of each measurement was 6 s, and ten consecutive measurements were taken at 60-s intervals. Eight readings (excluding the highest and lowest ones) were averaged to calculate the bilateral hindpaw weight-bearing values.
Hindpaw temperature
The room temperature was maintained at 23 °C, and humidity ranged between 25 and 45 %. The temperature of the hindpaw was measured using a fine wire thermocouple (Omega, Stanford, CT, USA) applied to the paw skin, as previously described [
17,
35,
36]. The investigator held the thermistor wire using an insulating Styrofoam block. Three sites were tested over the dorsum of the hindpaw; the space between the first and second metatarsals (medial), the second and third metatarsals (central), and the fourth and fifth metatarsals (lateral). After a site was tested in one hindpaw, the same site was immediately tested in the contralateral hindpaw. The testing protocol was medial dorsum right then left, central dorsum right then left, lateral dorsum right then left, medial dorsum left then right, central dorsum left then right, and lateral dorsum left then right. The six measurements for each hindpaw were averaged for the mean temperature.
Hindpaw thickness
A laser sensor technique was used to determine the dorsal-ventral thickness of the hindpaw, as we have previously described [
35]. For laser measurements, each rat was briefly anesthetized with isoflurane and then held vertically so the hindpaw rested on a table top below the laser. The paw was gently held flat on the table with a small metal rod applied to the top of the ankle joint. Using optical triangulation, a laser with a distance measuring sensor was used to determine the distance to the table top and to the top of the hindpaw at a spot on the dorsal skin over the midpoint of the third metatarsal, and the difference was used to calculate the dorsal-ventral paw thickness. The measurement sensor device used in these experiments (4381 Precicura, Limab, Goteborg, Sweden) has a measurement range of 200 mm with a 0.01-mm resolution.
Epidermal thickness
This experiment determined whether fracture chronically increases epidermal thickness. four and sixteen-week post-fracture rats were anesthetized with isoflurane and then transcardially perfused with 4 % paraformaldehyde in phosphate-buffered saline (PBS, pH 7.4); the dorsal hindpaw skin including sub-dermal layers was immediately removed and post-fixed in 4 % paraformaldehyde (PFA) for 2 h; then, the tissues were treated with 30 % sucrose in PBS at 4 °C before embedding in OCT. Following embedding, 20-μm slices were made using a cryostat and mounted onto Superfrost microscope slides (Fisher scientific, Pittsburgh, PA). All sections were stored at −70 °C until use for immunohistochemistry. Frozen sections were permeabilized and blocked with PBS containing 10 % donkey serum and 0.3 % Triton X-100 prior to primary antibody incubation. Sections were incubated with a pan-keratinocyte marker recognizing both the acidic and basic (types I and II) subfamilies of cytokeratins for keratinocyte labeling, and fluorescent immunohistochemistry and confocal microscopy were performed as previously described [
19]. Epidermal thickness measurements were made using LSM Image Browser from Zeiss LSM Data Server. A blinded observer selected four to eight sections from each skin specimen, and four to eight thickness measurements were made in each section to derive a mean score for that sample. The individual mean scores were then used to calculate the mean thickness and standard error of the mean for the control limbs and the fracture limbs at 4 and 16 weeks post injury.
Homogenization procedure and enzyme immunoassay for TNFα, IL-1β, IL-6, and NGF
Rat hindpaw dorsal skin and ipsilateral spinal cord of lumbar enlargement section were collected after behavioral testing or at time points as indicated and frozen immediately on dry ice. Skin and spinal cord tissues were cut into fine pieces in ice-cold phosphate-buffered saline (PBS), pH 7.4, containing protease inhibitors (aprotinin [2 μg/ml], leupeptin [5 μg/ml], pepstatin [0.7 μg/ml], and PMSF [100 μg/ml]; Sigma, St. Louis, MO, USA) followed by homogenization using a rotor/stator homogenizer. Homogenates were centrifuged for 5 min at 14,000 g, and at 4 °C. Supernatants were transferred to fresh pre-cooled Eppendorf tubes. Triton X-100 (Boehringer Mannheim, Germany) was added at a final concentration 0.01 %. The samples were centrifuged again for 5 min at 14,000 g at 4 °C. The supernatants were aliquoted and stored at −80 °C. TNFα, IL-1β, and IL-6 protein levels were determined using EIA kits (R&D Systems, Minneapolis, MN, USA). The NGF concentrations were determined using the NGF Emax® ImmunoAssay System kit (Promega, Madison, WI, USA) according to the manufacturer’s instructions. The optical density (OD) of the reaction product was read on a microplate reader at 450 nm. The concentrations of TNFα, IL-1β, IL-6, and NGF proteins were calculated from the standard curve at each assay. Positive and negative controls were included in each assay. Each protein concentration was expressed as picogram per milligram total protein. Total protein contents in all tissue extracts were measured by the Coomassie Blue Protein Assay Kit (Bio-Rad, Hercules, CA).
Enzyme immunoassay procedure for sciatic nerve SP
The aim of this experiment was to determine whether fracture induced up-regulated SP protein expression in the sciatic nerve at 4 and 16 weeks post fracture. The right sciatic nerve was collected under isoflurane anesthesia, immediately frozen, and weighed. Nerve samples were minced in 1 ml of 3:1 ethanol/0.7 M HCl and homogenized for 20 s. The homogenates were shaken for 2 h at 4 °C and centrifuged at 3000 g for 20 min at 4 °C. The supernatant was frozen and lyophilized, and the lyophilized product was stored at −80 °C. All nerve samples were assayed in duplicate using an EIA kit to determine SP levels (Assay Designs, Ann Arbor, MI) following the manufacturer’s protocols.
This experiment tested the hypothesis that tibia fracture facilitates SP-evoked extravasation responses in the injured hindlimb at 4 and 16 weeks after injury, when compared with the normal controls. Five minutes after injection of Evans blue dye (50 mg/kg in Ringers, Sigma), SP (10 μg/kg, Sigma) was injected intravenously into the internal jugular vein. Five minutes after SP injection, the rats were anesthetized with isoflurane, transcardially perfused as previously described, and the plantar and dorsal skin on each hindpaw was collected for dye content determination [
16].
Western blotting
These experiments tested the hypothesis that tibia fracture with cast immobilization can induce chronic increases in the NK1-receptor protein in the hindpaw skin and spinal cord of lumbar enlargement. At 4 or 16 weeks after fracture, the ipsilateral hindpaw dorsum skin was collected under isoflurane anesthesia and was homogenized in modified RIPA buffer (50 mM Tris–HCl, 150 mM NaCl, 1 mM EDTA, 1 % Igepal CA-630, 0.1 % SDS, 50 mM NaF, and 1 mM NaVO3) containing protease inhibitors (aprotinin [2 μg/ml], leupeptin [5 μg/ml], pepstatin [0.7 μg/ml], and PMSF [2 mM]; Sigma, St. Louis, MO, USA). The homogenate was centrifuged at 13,000
g for 30 min at 4 °C. Total protein concentration of the homogenate was measured using a Coomassie Blue Protein Assay (Bio-Rad, Hercules, CA) and normalized against BSA protein standards (Pierce, Rockford, IL). The supernatant was subjected to Western blot analysis using our previously described methods [
16] to elucidate changes in NK1-receptor protein expression in the skin or spinal cord. Equal amounts of protein (30 μg) were subjected to SDS-PAGE (12 % Tris–HCl acrylamide gel, Bio-Rad, Hercules, CA) and electrotransferred onto a polyvinylidene difluorided membrane (Millipore). The blots were blocked with 5 % non-fat dry milk in Tris-buffered saline, incubated with goat anti-rat NK1R primary antibody overnight at 4 °C and further incubated with HRP-conjugated secondary antibody (Santa Cruz Biotechnology, Santa Cruz, CA) for 1 h at room temperature. After washing in TBST three times, the blot was then incubated in ECL plus chemoluminescence reagents (Amersham, Piscataway, NJ) and scanned by PhosphoImager (Typhoon, GE Healthcare), and the band intensity was analyzed using ImageQuant 5.2 software (Molecular Dynamics, Piscataway, NJ) and normalized with the corresponding internal loading control band, β-actin. The specific protein/actin band intensity ratio represents the change of the specific protein.
Study design
To study the acute and chronic changes in nociceptive behavior, vascular signs, and inflammatory responses, rats were randomly assigned to four primary experimental cohorts: 4-week controls, 4-week post fracture, 16-week controls, and 16-week post fracture. Control rats received no fracture or other treatments. At the designated time point, all cohorts were tested for bilateral hindpaw mechanical nociceptive withdrawal thresholds to von Frey fibers, weighting, hindpaw temperature, and hindpaw thickness as well as intravenous SP-induced hindpaw extravasation. Ipsilateral to the fracture, the hindpaw skin, as well as sciatic nerve and lumbar spinal cord was collected and stored for determination of TNFα, IL-1β, IL-6, and NGF protein, as well as SP and NK1 receptor levels, respectively.
Separate cohorts of fracture rats at the 4- and 16-week time points were treated systemically with vehicle (i.p. or s.c.), LY303870 (i.p.), anakinra (s.c. pump or i.p. injection), or anti-NGF (s.c. injection). Anakinra and anti-NGF are large molecules with poor CNS penetration; thus, we assumed that these treatments inhibited peripheral inflammatory mechanisms in the injured limb without affecting CNS inflammatory changes. Additional fracture rats at the 4- and 16-week time points were treated intrathecally with either vehicle, LY303870, anakinra, or anti-NGF to test the hypothesis that spinal cord SP signaling, IL-1β, and NGF contribute to pathological signs of CRPS in the acute and chronic phases. Each cohort was tested for bilateral hindpaw mechanical nociceptive withdrawal thresholds to von Frey fibers, unweighting, warmth, and edema.
Statistical analysis
Statistical analysis was accomplished using a one-way analysis of variance (ANOVA) followed by Neuman-Keuls multiple comparison test to compare among all cohorts. All data are presented as the mean ± standard error (SE) of the mean, and differences are considered significant at a P value less than 0.05 (Prism 5, GraphPad Software, San Diego, CA, USA).
Hindpaw temperature, thickness, and mechanical nociceptive threshold data were analyzed as the difference between the fracture side (right, R) and the contralateral untreated side (left, L). Right hindpaw weight-bearing data were analyzed as a ratio between twice the right hindpaw weighting and the sum of the right (R) and left (L) hindpaw values ([2R/(R + L)] × 100 %).
Discussion
Complex regional pain syndrome (CRPS) is a pain syndrome of modest prevalence in the overall population but has a relatively high incidence after injuries and surgeries to the limbs. Fracture of an extremity followed by immobilization is a particularly common set of circumstances leading to CRPS. The acute phase of the syndrome frequently involves an erythematous, warm, swollen, painful limb, all signs of acute neurogenic inflammation [
38]. While some patients retain these signs of inflammation, it is more common for the warmth and swelling to resolve over the course of months with a normal or even cool atrophic but still painful limb in the chronic phases of the condition [
39]. Thus CRPS is often thought to have an acute or “warm” phase followed by a more chronic “cold” phase. This difference is seldom considered when providing therapeutic interventions, though the mechanisms supporting the condition appear to be changing. Our earlier studies showed that gene transcription patterns within the CNS change as fracture mice progress from the acute to the chronic stages of the syndrome [
40]. Moreover, centrally mediated signs and symptoms become more common in the chronic phases of the condition such as cognitive changes, mood alterations, and motor function disturbances. Thus, we hypothesized that we would observe a shift in the location of mediators driving the CRPS-like changes of our model from the periphery to the spinal cord over time. The fundamental observations of our studies were: (1) cytokines and NGF are elevated in skin at relatively acute time points after tibia fracture and immobilization, but these normalize over time; (2) hindpaw edema, keratinocyte proliferation, and increase in peripheral SP and NK1-receptor expression resolve as the condition becomes more chronic; (3) spinal cord cytokines, NGF, SP, and NK1-receptor levels are increased in the early post-fracture period, and most of these spinal inflammatory changes persist in the chronic post fracture period; (4) spinal cord SP, cytokine, and NGF signaling support nociceptive sensitization at both acute and chronic time points; and (5) mechanical allodynia is the most durable of the CRPS-like changes exhibited by our model over time.
A great deal of attention has been paid to the presence of pain and inflammation-related mediators in the skin of patients with CRPS. Some of the most compelling studies have involved the analysis of fluid from suction blisters made on the skin of CRPS patients. Numerous cytokines including TNFα, IL-6, and others have been discovered at elevated levels [
41,
42]. While the relationship of mediator abundance to CRPS duration has not been firmly established, it does appear that cytokine levels may decline over time in some patients [
42]. Our study using human hand surgery patients discovered elevated levels of skin cytokines and NGF 3–5 weeks after surgery at the point of cast-removal [
43]. Mechanical allodynia, warmth, and edema were all present in these patients suggesting that tissue trauma followed by immobilization may commonly evoke this type of peripheral inflammatory response, though not all patients go on to develop chronic CRPS. Additional studies using a radiolabeled anti-TNF molecule found greatly enhanced TNF activity in the limbs of CRPS patients [
44]. On the other hand, results from small human trials using biologic anti-TNF agents are less clear, though encouraging results were noted in some patients [
45,
46].
The present study monitored the pathological changes accompanying CRPS-like changes in early (4 weeks) and later (16 weeks) stages of a rat model. By 16 weeks post fracture, vasculature abnormalities, including warmth and edema, recovered as inflammation subsided in skin. Our data indicate that the processes supporting persistent sensitization in the late stage animals are likely spinal. This has implications concerning the tailoring of treatments for early versus late stage disease. Future experiments might exploit the individual patterns of recovery both of humans and laboratory animals to gain insight into the mechanisms contributing to each of the features of CRPS.
Using mouse and rat tibia fracture/cast immobilization models, the effects of peripherally restricted anti-cytokine and anti-NGF have been reported. For example, the administration of the same anti-IL-1ra agent used in these studies (anakinra), the anti-TNF agent etanercept, and an anti-NGF antibody all effectively reduced nociceptive changes [
28,
34,
47]. Importantly, all of those studies involved measurements made during the acute phase of the model. Correspondingly, elevated levels of these cytokines and NGF were identified in the skin of the affected limbs. The present group of studies demonstrates that anti-IL-1β and anti-NGF were effective at 4 weeks post fracture, but these agents lost effect at 16 weeks after fracture, despite ongoing nociceptive changes. This corresponded to the resolution of elevated levels of these mediators in the peripheral tissues. On the other hand, our data showed both chronic elevations of IL-1β and NGF in spinal cord tissue, as well as the persistent efficacy of spinally administered IL-1β and NGF inhibitors in reversing nociceptive changes. Thus, the relevant pool of these mediators appears to be located within the CNS in the more chronic phases of the syndrome. We previously demonstrated that keratinocytes are the chief peripheral cell-type producing cytokines and NGF in this model and in CRPS patients [
6,
19], though the central sources of these mediators have not been identified. Furthermore, as LY303870, anakinra, and anti-NGF exerted potent anti-nociceptive effects at 4 weeks in the CRPS rat model, an important question is whether these treatments can prevent the development of CRPS when these drugs are administered immediately or very early on after fracture.
Neurogenic inflammation has well-established roles in the peripheral manifestations of CRPS. Substance P (SP) released peripherally from afferent/efferent nerves has been shown to alter capillary permeability in humans, an effect that is exaggerated in CRPS-affected limbs [
9] and in animal models of CRPS [
16]. These effects are believed to be mediated through increased NK1-receptor expression on endothelial cells in the affected limb [
8,
16]. In addition, SP containing fibers penetrate the epidermis. Activation of the NK1 receptors expressed by keratinocytes stimulate these cells to produce cytokines, NGF, and other mediators capable in turn of interacting with receptors on afferent neurons to support nociception [
48]. Earlier work demonstrated that administration of the selective NK1 antagonist LY303870 during the early weeks after fracture inhibited nociceptive sensitization, edema, warmth, keratinocyte proliferation, and the up-regulation of cytokines in the skin [
17,
18,
25].
Because the fracture/cast rats showed a reduction in hindpaw edema, warmth, keratinocyte proliferation, and skin cytokine levels over time, we hypothesized peripheral SP/NK1 signaling might also diminish over time. Indeed, at 4 weeks post fracture, SP levels in sciatic nerve and NK1-receptor levels in the skin were both elevated. Correspondingly, SP-evoked plasma extravasation was augmented. Both the expression and plasma extravasation responses were similar to those of the control animals by week 16, however. This is additional evidence for a normalization of peripheral neural function and response over time, in spite of persistent nociceptive changes.
In contrast to the expression and functional responses of peripheral tissues, NK1-receptor levels remained elevated in ipsilateral lumbar spinal cord tissue throughout the course of study. Likewise, intrathecal injection of the NK1-receptor antagonist LY303870 reduced nociceptive sensitization at both the 4- and 16-week time points to approximately the same degree (but systemically administered LY303870 appeared to lose analgesic efficacy over time). The NK1 receptor is densely expressed on spinal cord nociceptive projection neurons. Using both pharmacological and neuroablative techniques, it has been shown that spinal NK1-expressing neurons are critical components of nociceptive signaling in many pain models [
24,
49,
50]. Though there is some evidence for the local spinal production of SP, spinal NK1 receptors are generally felt to respond to SP released from the central terminals of primary afferent nerves. Thus, central NK1-mediated signaling may be at least partially responsible for the persistent nociceptive sensitization seen in this model. It should be mentioned that NK1-receptor antagonists with good CNS penetrance have not been proven to be effective analgesics in humans, though they do have potent antiemetic properties [
51]. We are unaware of a trial of an NK1-receptor antagonist in human CRPS patients, however.
Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
TW carried out the immunoassays and NK1 analyses, performed the statistical analyses, and drafted the manuscript. TG performed the behavioral studies. WL carried out the immunostaining of keratin and epidermal thickness determination. WK conceived of and coordinated the study, participated in its design, and helped to draft the manuscript. JC helped to design the study and to draft the manuscript. All authors read and approved the final manuscript.