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Previous Article | Next Article
The Journal of Neuroscience, February 1, 2003, 23(3):1026
Spinal Glia and Proinflammatory Cytokines Mediate Mirror-Image Neuropathic Pain in Rats
Erin D. Milligan1, Carin Twining1, Marucia Chacur2, Joseph Biedenkapp1, Kevin O'Connor1, Stephen Poole3, Kevin Tracey4, David Martin5, Steven F. Maier1, and Linda R. Watkins1 1 Department of Psychology and the Center for Neuroscience, University of Colorado at Boulder, Boulder, Colorado 80309-0345, 2 Laboratory of Pathophysiology, Butantan Institute, 05503-900, San Paulo, SP, Brazil,3 Division of Endocrinology, National Institute for Biological Standards and Control, South Mimms, Potters Bar, Herts EN6 3QG, United Kingdom, 4 Laboratory of Biomedical Science, North Shore-LIJ Research Institute, Manhasset, New York 11030, and 5 Department of Pharmacology, Amgen, Thousand Oaks, California 91320
ABSTRACT
TOP
ABSTRACT
Introduction
Mirror-image allodynia is a mysterious phenomenon that occurs in association with many clinical pain syndromes. Allodynia refers to pain in response to light touch/pressure stimuli, which normally are perceived as innocuous. Mirror-image allodynia arises from the healthy body region contralateral to the actual site of trauma/inflammation. Virtually nothing is known about the mechanisms underlying such pain. A recently developed animal model of inflammatory neuropathy reliably produces mirror-image allodynia, thus allowing this pain phenomenon to be analyzed. In this sciatic inflammatory neuropathy (SIN) model, decreased response threshold to tactile stimuli (mechanical allodynia) develops in rats after microinjection of immune activators around one healthy sciatic nerve at mid-thigh level. Low level immune activation produces unilateral allodynia ipsilateral to the site of sciatic inflammation; more intense immune activation produces bilateral (ipsilateral + mirror image) allodynia. The present studies demonstrate that both ipsilateral and mirror-image SIN-induced allodynias are (1) reversed by intrathecal (peri-spinal) delivery of fluorocitrate, a glial metabolic inhibitor; (2) prevented and reversed by intrathecal CNI-1493, an inhibitor of p38 mitogen-activated kinases implicated in proinflammatory cytokine production and signaling; and (3) prevented or reversed by intrathecal proinflammatory cytokine antagonists specific for interleukin-1, tumor necrosis factor, or interleukin-6. Reversal of ipsilateral and mirror-image allodynias was rapid and complete even when SIN was maintained constantly for 2 weeks before proinflammatory cytokine antagonist administration. These results provide the first evidence that ipsilateral and mirror-image inflammatory neuropathy pain are created both acutely and chronically through glial and proinflammatory cytokine actions.
Key words: microglia; astrocyte; interleukin-1; tumor necrosis factor; interleukin-6; allodynia; p38 MAP kinase
Introduction
Trauma and inflammation of peripheral nerves induce pathological pain, referred to as neuropathic pain (Zimmermann, 2001
). Although neuropathic pain is perceived to arise from the skin innervated by the damaged/inflamed nerve, pathological pain can also arise from sites contralateral to (the mirror image of) the site of pathology (Watkins and Maier, 2002
How mirror-image pain is created is unknown. Although neuropathic pain from the area of nerve trauma can be accounted for, in part, by ectopic action potentials and hyperexcitability (Woolf and Salter, 2000
The ability to study mirror-image allodynia has recently been facilitated by the development of the sciatic inflammatory neuropathy (SIN) model (Chacur et al., 2001
The purpose of the present series of experiments is to provide an initial investigation of spinal cord mechanisms underlying mirror-image allodynia. It also provides the first investigation of spinal mediators of inflammatory neuropathy pain. In contrast to the wealth of studies focused on the spinal neurochemistry of pain from traumatic neuropathy (Zimmermann, 2001
Materials and Methods
Subjects
Pathogen-free adult male Sprague Dawley rats (300-450 gm; Harlan Labs, Madison, WI) were used in all experiments. Rats were housed in temperature-controlled (23 ± 3°C) and light-controlled (12 hr light/dark; lights on at 7:00 A.M.) rooms with standard rodent chow and water available ad libitum. Behavioral testing was performed during the light cycle. There were five to six rats per in every experiment. All procedures were approved by the Institutional Animal Care and Use Committee of the University of Colorado at Boulder.Drugs
Zymosan (yeast cell walls; Sigma, St. Louis, MO) was made fresh daily by suspension in a vehicle of incomplete Freund's adjuvant (Sigma) to final concentrations of 0.08 µg/µl and 3.2 µg/µl. The glial metabolic inhibitor fluorocitrate (Sigma) (Paulsen et al., 198770°C. The vehicle (0.3% 2 M HCl in PBS, pH 6.0) was aliquoted and stored at 4°C. The p38 mitogen-activated protein (MAP) kinase inhibitor CNI-1493 (Denham et al., 2000
Behavioral measures
The von Frey test (Chaplan et al., 1994Surgery and microinjections
Chronic intrathecal catheters. Lumbosacral intrathecal catheters were constructed and implanted by lumbar approach as described previously in detail (Milligan et al., 1999Data analysis
All statistical comparisons were computed using Statview 5.0.1 for the Macintosh. Data from the von Frey test were analyzed as the interpolated 50% threshold (absolute threshold) in log base 10 of stimulus intensity (monofilament stiffness in milligrams × 10). Pre-drug baseline measures were analyzed by one-way ANOVA. Post-drug time course measures were analyzed by repeated measures ANOVAs followed by Fisher's protected least significant difference post hoc comparisons, where appropriate.Experiment 1: effect of intrathecal fluorocitrate on sciatic inflammatory neuropathy-induced allodynia: blockade of allodynia
Fluorocitrate selectively inhibits aconitase, an enzyme that is in the Krebs' energy cycle of glia, but not neurons (Paulsen et al., 1987Experiment 2: effect of intrathecal CNI-1493 on sciatic inflammatory neuropathy-induced allodynia: prevention of allodynia
CNI-1493 is a p38 MAP kinase inhibitor (Denham et al., 2000Experiment 3: effect of intrathecal CNI-1493 on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia
After baseline behavioral assessments, perisciatic microinjections of 0, 4, or 160 µg zymosan were performed as above. Behavior was reassessed 13 hr later to confirm the effectiveness of the perisciatic injections before intrathecal drug delivery. At 14.5 hr after perisciatic injection, each rat received an intrathecal injection of either CNI-1493 (9 µg) or equivolume saline (1 µl). Behavior was then assessed 0.5, 2.5, and 4.5 hr later (that is, 15, 17, and 19 hr after the perisciatic injection).Experiment 4: effect of intrathecal tumor necrosis factor binding protein on sciatic inflammatory neuropathy-induced allodynia: blockade of allodynia
It should be noted here that CNI-1493 has recently been demonstrated to be capable of crossing the blood-brain barrier into spinal cord after systemic administration (Milligan et al., 2001aExperiment 5: effect of intrathecal anti-rat interleukin-6 on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia 1 d later
After baseline behavioral assessments, perisciatic microinjections of 0, 4, or 160 µg zymosan were performed as above. Behavior was reassessed 13 hr later to confirm the effectiveness of the perisciatic injections before intrathecal drug delivery. At 14.5 hr after perisciatic injection, each rat received an intrathecal injection of either affinity-purified sheep anti-rat IL6 IgG (0.065 µg in 5 µl) or affinity-purified normal sheep IgG (0.065 µg in 5 µl). Behavior was then assessed 0.5, 2.5, and 4.5 hr later (that is, 15, 17, and 19 hr after the perisciatic injection).Experiment 6: effect of intrathecal interleukin-1 receptor antagonist on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia 1 d later
After baseline behavioral assessments, perisciatic microinjections of 0, 4, or 160 µg zymosan were performed as above. Behavior was reassessed 13 hr later to confirm the effectiveness of the perisciatic injections before intrathecal drug delivery. At 14.5 hr after perisciatic injection, each rat received an intrathecal injection of either IL1ra (100 µg) or equivolume vehicle (1 µl). Behavior was then assessed 0.5, 2.5, and 4.5 hr later (that is, 15, 17, and 19 hr after the perisciatic injection).Experiment 7: effect of intrathecal interleukin-1 receptor antagonist on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia 2 weeks later
Behavioral assessments were recorded before (baseline) and at 1, 4, 8, 10, 12, and 14 d after baseline. In half of the animals, a perisciatic microinjection of 160 µg zymosan was delivered immediately after baseline (day 0) and 3, 5, 7, 9, 11, and 13 d later. This injection schedule was based on pilot studies aimed at maintaining robust allodynia across days. The remaining animals were identically implanted with indwelling perisciatic catheters and injected with equivolume saline on corresponding days. On day 14, after an initial behavioral assessment (day 14 baseline), all animals received either IL1ra (100 µg) or equivolume (1 µl) vehicle intrathecally. Behavior was reassessed 0.5, 1, 1.5, 2 and 2.5 hr later.
Results
Experiment 1: effect of intrathecal fluorocitrate on sciatic inflammatory neuropathy-induced allodynia: blockade of allodynia
Immunohistochemical evidence of bilateral astrocyte and microglial activation has been observed after traumatic neuropathies (Colburn et al., 1999
As in our previous studies (Chacur et al., 2001
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Figure 1. Blockade of perisciatic SIN-induced mechanical allodynias by intrathecal fluorocitrate, a glial metabolic inhibitor. Rats were assessed for low-threshold mechanical sensitivity (von Frey test) both before (baseline) and 1, 2, and 3 hr after completion of intrathecal drug administration. Replicating our earlier studies (Chacur et al., 2001
These observations were supported by statistical analyses. ANOVA revealed reliable main effects of zymosan dose (F(2,210) = 214.125; p < 0.0001), intrathecal fluorocitrate (F(2,62) = 182.756; p < 0.0001), laterality (F(1,62 = 88.069; p < 0.0001), and time (F(2,124) = 33.601; p < 0.0001), and interactions between intrathecal fluorocitrate and zymosan dose (F(2,62) = 70.867; p < 0.0001), zymosan dose and laterality (F(2,62) = 31.775; p < 0.0001), intrathecal fluorocitrate, zymosan dose, and laterality (F(2,62) = 12.070; p < 0.0001) and time, intrathecal fluorocitrate, zymosan dose, and laterality (F(4,124) = 2.692; p < 0.05).
Post hoc means comparison revealed several important points. After 4 µg zymosan (Fig. 1A), mechanical allodynia was observed in the left (ipsilateral) hindpaw compared with the right (contralateral) hindpaw (p < 0.0001). Mechanical responses of the right hindpaw after 4 µg zymosan did not differ from that after perisciatic vehicle (Fig. 1A), supporting the conclusion that 4 µg zymosan induced only a unilateral allodynia ipsilateral to the site of injection. Fluorocitrate greatly reduced the allodynic effects of 4 µg zymosan (p < 0.0001 comparing the ipsilateral paw of rats receiving 4 µg zymosan with versus without intrathecal fluorocitrate) (Fig. 1A), because mild allodynia was observed only at 1 hr after perisciatic zymosan (p < 0.001). Intrathecal fluorocitrate, in the absence of perisciatic zymosan, had no effect on paw withdrawal thresholds, compared with intrathecal vehicle controls (p > 0.5) (Fig. 1A). Post hoc means comparison also revealed that bilateral mechanical allodynia occurred in response to 160 µg zymosan. That is, the thresholds of the left and right hindpaws did not differ (p > 0.05 comparing the ipsilateral and contralateral paws of rats receiving 160 µg zymosan but no fluorocitrate) (Fig. 1B), but the thresholds for both the left and right paws for all of these groups were reliably different from those of the vehicle controls (p < 0.0001 and p < 0.0001, respectively) (Fig. 1A). Fluorocitrate greatly reduced the perisciatic allodynia in both the ipsilateral (p < 0.0001) and contralateral (p < 0.0001) paws, compared with 160 µg zymosan-injected rats receiving vehicle intrathecally (Fig. 1B). Indeed, only mild, transient allodynia was observed in the fluorocitrate-treated animals at 1 hr after perisciatic zymosan (p < 0.05).
Experiment 2: effect of intrathecal CNI-1493 on sciatic inflammatory neuropathy-induced allodynia: prevention of allodynia
Experiment 1 provided initial evidence that spinal cord glia may be involved in the mediation of both ipsilateral and mirror-image SIN-induced allodynias. This is the first evidence that pain induced by inflammation around healthy peripheral nerves likely involves spinal cord glia. This suggests that SIN-induced pain changes would be mediated by pain-enhancing substances known to be released by activated glia. Although various substances are released by activated glia, proinflammatory cytokines have recently been implicated as mediators of diverse exaggerated pain states (Watkins et al., 2001
As in our previous studies (Chacur et al., 2001
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Figure 2. Blockade of perisciatic SIN-induced mechanical allodynias by intrathecal CNI-1493, a p38 mitogen-activated kinase inhibitor. Rats were assessed for low-threshold mechanical sensitivity (von Frey test) both before (baseline) and 1, 1.5, 2, 3, and 24 hr after completion of intrathecal drug administration. Replicating our earlier studies (Chacur et al., 2001
These observations were supported by statistical analyses. ANOVA revealed reliable main effects of zymosan dose (F(2,120) = 30.742; p < 0.0001), intrathecal CNI-1493 (F(1,120) = 132.044; p < 0.0001), and laterality (F(1,120) = 46.807; p < 0.0001), and interactions between intrathecal CNI-1493 and zymosan dose (F(2,60) = 28.656; p < 0.0001), zymosan dose and laterality(F(2,60) = 7.481; p < 0.01), and intrathecal CNI-1493, zymosan dose, and laterality (F(2,60) = 11.843; p < 0.0001). Allodynia recovered by 24 hr. Both ipsilateral allodynia (Fig. 2A) and bilateral allodynia (Fig. 2B) were fully restored by this time. At 24 hr, ANOVA revealed reliable main effects of zymosan dose (F(1,60) = 13.925; p < 0.0001) and laterality (F(1,60) = 21.370; p < 0.0001), and interactions between zymosan dose and laterality (F(1,60) = 9.864; p < 0.001). As in experiment 1, 4 µg zymosan (Fig. 2A) produced mechanical allodynia in the left (ipsilateral) hindpaw compared with the right (contralateral) hindpaw (p < 0.0001). Also as in experiment 1, mechanical responses of the right hindpaw after 4 µg zymosan did not differ from that after perisciatic vehicle (p > 0.2) (Fig. 2A), indicating that 4 µg zymosan induced only a unilateral allodynia ipsilateral to the site of injection. CNI-1493 abolished the allodynic effects of 4 µg zymosan through 3 hr (p < 0.0001) comparing the ipsilateral paw of rats receiving 4 µg zymosan + intrathecal CNI-1493 with the ipsilateral paw of rats receiving no zymosan + intrathecal CNI-1493 (Fig. 2A). Intrathecal CNI-1493, in the absence of perisciatic zymosan, had no effect on paw withdrawal thresholds, compared with intrathecal vehicle controls (p > 0.5) (Fig. 2A).
Post hoc means comparison also revealed that bilateral mechanical allodynia occurred in response to 160 µg zymosan. That is, the thresholds of the left and right hindpaws did not differ, except at the 1 hr time point (p < 0.001) (Fig. 2B). The thresholds for both the left and right paws for all of these groups were reliably different from those of the appropriate vehicle controls (p < 0.0001) (Fig. 2A). CNI-1493 greatly reduced the perisciatic allodynia in both the ipsilateral (p < 0.0001) and contralateral (p < 0.0001) paws through 3 hr, compared with 160 µg zymosan-injected rats receiving vehicle intrathecally (Fig. 2A,B).
Experiment 3: effect of intrathecal CNI-1493 on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia
Experiment 2 provided initial evidence that p38 MAP kinase pathways are involved in the initiation of both ipsilateral and mirror-image SIN-induced allodynias. The present experiment tests whether p38 MAP kinases may be involved in the maintenance of these ipsilateral and mirror-image allodynias as well. This is a key issue for pathological pain states, because drug manipulations can often prevent but not reverse pathological pain once it develops (Traub, 1996
Compared with vehicle controls (Fig. 3A), low-dose perisciatic zymosan induced a unilateral allodynia (Fig. 3A), whereas higher dose perisciatic zymosan induced a bilateral allodynia (Fig. 3B), measured 13 hr later. CNI-1493 injected intrathecally at 14.5 hr abolished these SIN-induced pain changes within 2.5-4.5 hr (that is, 17-19 hr after perisciatic injection) (Fig. 3B).
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Figure 3. Reversal of perisciatic SIN-induced mechanical allodynias by intrathecal CNI-1493, a p38 mitogen-activated kinase inhibitor. Rats were assessed for low-threshold mechanical sensitivity (von Frey test) both before (baseline) and 13, 15, 17, and 19 hr after completion of perisciatic drug administration. Replicating and extending our earlier studies (Chacur et al., 2001
These observations were supported by statistical analyses. ANOVA revealed reliable main effects of zymosan dose (F(2,66) = 125.279; p < 0.0001) and laterality (F(1,66) = 80.804; p < 0.0001), and interactions between zymosan dose and laterality (F(2,66) = 30.638; p < 0.0001). Post hoc means comparison revealed that 4 µg zymosan (Fig. 3A) induced mechanical allodynia in the left (ipsilateral) hindpaw compared with the right (contralateral) hindpaw (p < 0.0001). Mechanical responses of the right hindpaw after 4 µg perisciatic zymosan did not differ from that after perisciatic vehicle (Fig. 3A), showing that 4 µg zymosan induced only a unilateral allodynia ipsilateral to the site of injection. In addition, post hoc analyses showed that bilateral mechanical allodynia occurred in response to 160 µg perisciatic zymosan. That is, the thresholds of the left and right hindpaws did not differ (Fig. 3B). The thresholds for both the left and right paws for all of these groups were reliably different from those of the vehicle controls (p < 0.0001) (Fig. 3A). At 14.5 hr, either CNI-1493 or vehicle was injected intrathecally. Behavior was recorded 0.5, 2.5, and 4.5 hr later (that is, 15, 17, and 19 hr after perisciatic drug administration). Although CNI-1493 had no effect in the absence of perisciatic zymosan (Fig. 3A), it reversed both unilateral (Fig. 3A) and bilateral (Fig. 3B) allodynias induced by perisciatic zymosan. ANOVA revealed reliable main effects of zymosan dose (F(2,60) = 111.593; p < 0.0001), intrathecal CNI-1493 (F(1,60) = 162.991; p < 0.0001), and laterality (F(1,60) = 61.422; p < 0.0001), and interactions between intrathecal CNI-1493 and zymosan dose (F(2,60) = 84.320; p < 0.0001), and intrathecal CNI-1493, zymosan dose, and laterality (F(2,60) = 15.675; p < 0.0001).
Post hoc means comparisons showed that CNI-1493 reversed the allodynic effects of 4 µg zymosan by 17-19 hr (p < 00001 comparing the ipsilateral paw of rats receiving 4 µg zymosan with vs without intrathecal CNI-1493) (Fig. 3A). Indeed, the response thresholds of rats receiving 4 µg zymosan + CNI-1493 were not different from vehicle controls at this time (p > 0.3) (Fig. 3A). This drug reversed the bilateral allodynic effects of 160 µg perisciatic zymosan by 17-19 hr as well (p < 0.0001 comparing the ipsilateral paw of rats receiving 160 µg zymosan with vs without intrathecal CNI-1493; p < 0.0001 comparing the contralateral paw of rats receiving 160 µg zymosan with vs without intrathecal CNI-1493) (Fig. 3A,B). Again, the response thresholds of rats receiving 160 µg zymosan + CNI-1493 were not different from vehicle controls at this time (p > 0.1) (Fig. 3A). Intrathecal CNI-1493, in the absence of perisciatic zymosan, had no effect on paw withdrawal thresholds, compared with intrathecal vehicle controls (Fig. 3A).
Experiment 4: effect of intrathecal tumor necrosis factor binding protein (soluble receptors) on sciatic inflammatory neuropathy-induced allodynia: blockade of allodynia
Experiments 2 and 3 demonstrate that p38 MAP kinase is a key mediator in the intracellular signaling leading to SIN-induced allodynias. Given that p38 MAP kinases are strongly associated with proinflammatory cytokine production and signaling (Lee et al., 2000
As before, low-dose zymosan again induced a unilateral allodynia (Fig. 4A), whereas higher dose zymosan induced a bilateral allodynia (Fig. 4B) through 24 hr, compared with vehicle controls (Fig. 4A). Pretreatment with intrathecal TNFbp prevented these SIN-induced pain changes through 24 hr, in keeping with the prolonged half-life of this compound relative to IL1ra (Bendele et al., 1998
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Figure 4. Blockade of perisciatic SIN-induced mechanical allodynias by intrathecal TNFbp (TNF-soluble receptors), a TNF antagonist. Rats were assessed for low-threshold mechanical sensitivity (von Frey test) both before (baseline) and 1, 3, and 24 hr after completion of intrathecal drug administration. Replicating our earlier studies (Chacur et al., 2001
These observations were supported by statistical analyses. ANOVA revealed reliable main effects of intrathecal TNFbp (F(1,58) = 35.604; p < 0.0001) and laterality (F(1,58) = 23.061; p < 0.0001) and time (F(2,116) = 6.141; p < 0.005), and interactions between intrathecal TNFbp and zymosan dose (F(2,58) = 11.509; p < 0.0001), zymosan dose and laterality (F(2,58) = 6.736; p < 0.01), intrathecal TNFbp and zymosan dose and laterality (F(2,58) = 7.331; p < 0.005), time, and zymosan dose (F(4,116) = 3.739; p < 0.01), and time, intrathecal TNFbp, zymosan dose, and laterality (F(4,116) = 3.681; p < 0.01). Post hoc means comparison revealed that 4 µg zymosan induced a unilateral mechanical allodynia observed in the left (ipsilateral) hindpaw compared with the right (contralateral) hindpaw (p < 0.0001) (Fig. 4A). Mechanical responses of the right hindpaw after 4 µg zymosan did not differ from that after perisciatic vehicle (p > 0.05) (Fig. 4A), showing that 4 µg zymosan induced only a unilateral allodynia ipsilateral to the site of injection. TNFbp prevented the allodynic effects of 4 µg zymosan (p < 0.0001 comparing the ipsilateral paw of rats receiving 4 µg zymosan with vs without intrathecal TNFbp; p > 0.25 comparing the ipsilateral paw of rats receiving 4 µg zymosan + intrathecal TNFbp vs control groups receiving perisciatic vehicle) (Fig. 4A). Intrathecal TNFbp, in the absence of perisciatic zymosan, had no effect on paw withdrawal thresholds, compared with intrathecal vehicle controls (p > 0.05) (Fig. 4A).
Post hoc means comparison also revealed that bilateral mechanical allodynia occurred in response to 160 µg zymosan. That is, the thresholds of the left and right hindpaws did not differ (p > 0.05) (Fig. 4B), but the thresholds for both the left and right paws for all of these groups were reliably different from those of the vehicle controls (p < 0.0001 and p < 0.0001 for ipsilateral and contralateral comparisons, respectively) (Fig. 4A). TNFbp prevented the perisciatic 160 µg zymosan-induced allodynia in both the ipsilateral and contralateral paws compared with 160 µg zymosan-injected rats receiving vehicle intrathecally (p < 0.0001 and p < 0.0001 for ipsilateral and contralateral comparisons, respectively) and compared with control groups receiving perisciatic vehicle (p > 0.05 and p > 0.05 for ipsilateral and contralateral comparisons, respectively) (Fig. 4A,B).
Experiment 5: effect of intrathecal anti-rat interleukin-6 on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia 1 d later
Experiment 4 provided evidence that the proinflammatory cytokine TNF is a key mediator of SIN-induced allodynias. Because TNF can both induce the release of IL6 (Benveniste et al., 1990
As before, low-dose perisciatic zymosan induced a unilateral allodynia (Fig. 5A), whereas higher dose perisciatic zymosan induced a bilateral allodynia (Fig. 5B), measured 13 hr later. Anti-IL6 injected intrathecally at 14.5 hr reversed these SIN-induced pain changes within 2.5-4.5 hr (that is, 17-19 hr after perisciatic injection) (Fig. 5A,B).
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Figure 5. Reversal of perisciatic SIN-induced mechanical allodynias by intrathecal anti-rat IL6, 1 d later. Rats were assessed for low-threshold mechanical sensitivity (von Frey test) both before (baseline) and 13, 15, 17, and 19 hr after completion of perisciatic drug administration. Replicating experiment 3 and extending our earlier studies (Chacur et al., 2001
These observations were supported by statistical analyses. Before intrathecal anti-IL6 administration, ANOVA revealed reliable main effects of zymosan dose (F(2,60) = 94.296; p < 0.0001) and laterality (F(1,60) = 23.977; p < 0.0001), and interactions between zymosan dose and laterality (F(2,60) = 21.085; p < 0.0001). Post hoc means comparison revealed that 4 µg zymosan (Fig. 5A) induced mechanical allodynia in the left (ipsilateral) hindpaw compared with the right (contralateral) hindpaw (p < 0.0001). Mechanical responses of the right hindpaw after 4 µg perisciatic zymosan did not differ from that after perisciatic vehicle (p > 0.5) (Fig. 5A), showing that 4 µg zymosan induced only a unilateral allodynia ipsilateral to the site of injection. In addition, post hoc analyses showed that bilateral mechanical allodynia occurred in response to 160 µg perisciatic zymosan. That is, the thresholds of the left and right hindpaws did not differ (p > 0.5) (Fig. 5B). The thresholds for both the left and right paws for all of these groups were reliably different from those of the vehicle controls (p < 0.0001) (Fig. 5A). At 14.5 hr, either affinity-purified sheep anti-rat IL6 IgG or affinity-purified normal sheep IgG (control) was injected intrathecally. Behavior was recorded 0.5, 2.5, and 4.5 hr later (that is, 15, 17, and 19 hr after perisciatic drug administration). Although anti-IL6 had no effect in the absence of perisciatic zymosan (Fig. 5A), it completely reversed unilateral allodynia (Fig. 5A) and greatly reduced bilateral allodynia (Fig. 5B) induced by perisciatic zymosan. ANOVA revealed reliable main effects of zymosan dose (F(2,60) = 40.371; p < 0.0001), intrathecal anti-IL6 (F(1,60) = 29.745; p < 0.0001), and laterality (F(1,60) = 16.992; p < 0.0001), and interactions between zymosan dose and intrathecal anti-IL6 (F(2,60) = 18.022; p < 0.0001), zymosan dose and laterality (F(2,60) = 5.186; p < 0.01), and zymosan dose and intrathecal anti-IL6 and laterality (F(2,60) = 5.849; p < 0.005).
Post hoc means comparisons showed that anti-IL6 reversed the allodynic effects of 4 µg zymosan by 17-19 hr (p < 0.0001 comparing the ipsilateral paw of rats receiving 4 µg zymosan with vs without intrathecal anti-IL6; p > 0.2 comparing the ipsilateral paw of rats receiving 4 µg zymosan + intrathecal anti-IL6 versus perisciatic vehicle controls) (Fig. 5A). This antiserum reversed the bilateral allodynic effects of 160 µg perisciatic zymosan by 17-19 hr as well (p < 0.001 comparing the ipsilateral paw of rats receiving 160 µg zymosan with vs without intrathecal anti-IL6; p < 0.001 comparing the contralateral paw of rats receiving 160 µg zymosan with vs without intrathecal anti-IL6; p > 0.1 and p > 0.1 comparing the ipsilateral and contralateral paw of rats receiving 160 µg zymosan + intrathecal anti-IL6 vs perisciatic vehicle controls) (Fig. 5A). Intrathecal anti-IL6, in the absence of perisciatic zymosan, had no effect on paw withdrawal thresholds, compared with intrathecal IgG controls (p > 0.09) (Fig. 5A).
Experiment 6: effect of intrathecal interleukin-1 receptor antagonist on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia 1 d later
Experiments 4 and 5 provided evidence that the proinflammatory cytokines TNF and IL6 are key mediators of SIN-induced allodynias. Because TNF and IL6 can both (1) induce the release of IL1 (Watkins et al., 1999
As before, low-dose perisciatic zymosan induced a unilateral allodynia (Fig. 6A), whereas higher dose perisciatic zymosan induced a bilateral allodynia (Fig. 6B), measured 13 hr later. IL1ra injected intrathecally at 14.5 hr greatly reduced these SIN-induced pain changes within 2.5-4.5 hr (that is, 17-19 hr after perisciatic injection) (Fig. 6A,B).
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Figure 6. Reversal of perisciatic SIN-induced mechanical allodynias by intrathecal IL1ra, an IL1 receptor antagonist, 1 d later. Rats were assessed for low-threshold mechanical sensitivity (von Frey test) both before (baseline) and 13, 15, 17, and 19 hr after completion of perisciatic drug administration. Replicating experiments 3 and 5 and extending our earlier studies (Chacur et al., 2001
These observations were supported by statistical analyses. ANOVA revealed reliable main effects of zymosan dose (F(2,68) = 39.635; p < 0.0001) and laterality (F(1,68) = 28.972; p < 0.0001), and interactions between zymosan dose and laterality (F(2,68) = 12.846; p < 0.0001). Post hoc means comparison revealed that 4 µg zymosan (Fig. 6A) induced mechanical allodynia in the left (ipsilateral) hindpaw compared with the right (contralateral) hindpaw (p < 0.0001). Mechanical responses of the right hindpaw after 4 µg perisciatic zymosan did not differ from that after perisciatic vehicle (p > 0.30) (Fig. 6A), showing that 4 µg zymosan induced only a unilateral allodynia ipsilateral to the site of injection. In addition, post hoc analyses showed that bilateral mechanical allodynia occurred in response to 160 µg perisciatic zymosan, that is, the thresholds of the left and right hindpaws did not differ (p > 0.4) (Fig. 6B). The thresholds for both the left and right paws for all of these groups were reliably different from those of the vehicle controls (p < 0.0001) (Fig. 6A). At 14.5 hr, either IL1ra or vehicle was injected intrathecally. Behavior was recorded 0.5, 2.5, and 4.5 hr later (that is, 15, 17, and 19 hr after perisciatic drug administration). Although IL1ra had no effect in the absence of perisciatic zymosan (Fig. 6A), it completely reversed unilateral allodynia (Fig. 6A) and greatly reduced bilateral allodynia (Fig. 6B) induced by perisciatic zymosan. ANOVA revealed reliable main effects of zymosan dose (F(2,68) = 33.459; p < 0.0001), intrathecal IL1ra (F(1,68) = 24.257; p < 0.0001), and laterality (F(1,68) = 7.489; p < 0.01), and time (F(1,68) = 4.543; p< 0.05), and interactions between zymosan dose and intrathecal IL1ra (F(2,68) = 26.404; p < 0.0001), zymosan dose and laterality (F(2,68) = 5.114; p < 0.01), and time, intrathecal IL1ra, and zymosan dose (F(2,68) = 7.412; p < 0.01).
Post hoc means comparisons showed that IL1ra reversed the allodynic effects of 4 µg zymosan by 19 hr (p < 0.0001 at 19 hr, comparing the ipsilateral paw of rats receiving 4 µg zymosan with or without intrathecal IL1ra; p > 0.9 at 19 hr, comparing the ipsilateral paw of rats receiving 0 or 4 µg zymosan with intrathecal IL1ra) (Fig. 6A). This drug greatly reduced the bilateral allodynic effects of 160 µg perisciatic zymosan by 19 hr as well (p < 0.0001 at 19 hr, comparing the ipsilateral paw of rats receiving 160 µg zymosan with or without intrathecal IL1ra; p < 0.0001 at 19 hr, comparing the contralateral paw of rats receiving 160 µg zymosan with vs without intrathecal IL1ra) (Fig. 6B). Intrathecal IL1ra in the absence of perisciatic zymosan had no effect on paw withdrawal thresholds, compared with intrathecal vehicle controls (p > 0.05) (Fig. 6A).
Experiment 7: effect of intrathecal interleukin-1 receptor antagonist on sciatic inflammatory neuropathy-induced allodynia: reversal of allodynia 2 weeks later
Experiment 6 provided evidence that the proinflammatory cytokine IL1 is a key mediator of SIN-induced allodynias and is involved in the maintenance of allodynia. Because chronic pain can persist for long periods of time, it was of interest to determine whether IL1 would still be a key mediator of allodynia once pain enhancement was maintained for weeks. If so, this would support the idea that IL1 in particular, and proinflammatory cytokines in general, may be clinically relevant targets for pain control. Thus, this last experiment tested whether IL1ra would still be able to reverse long-standing (2 weeks) SIN-induced allodynias.
Figure 7, A and B (left panels), presents the behavioral results of chronic perisciatic injections, with no intrathecal injections made at any time. That is, all rats in any given left panel are identical in terms of the drugs administered to them through the day 14 time point. Thus the small differences between groups within any given left panel reflect random variability. On day 14, the group designations within each panel of Figure 7 become meaningful because it is on day 14 that the single intrathecal injection of IL1ra or vehicle was administered. The day 14 data shown in the left panels simultaneously serve as the baseline measure for the intrathecal IL1ra versus vehicle test presented in the right panels.
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Figure 7. Reversal of perisciatic SIN-induced mechanical allodynias by intrathecal IL1ra, an IL1 receptor antagonist, 2 weeks later. Rats were assessed for low-threshold mechanical sensitivity (von Frey test) both before (baseline) and across 2 weeks after completion of perisciatic drug administration. Extending our earlier studies (Chacur et al., 2001
Low dose perisciatic zymosan induced a unilateral allodynia by 1 d and was stably maintained across the 2 week observation period (Fig. 7A, left panel). There was a trend toward mild allodynia developing in the contralateral paw with chronic zymosan, but there was still clearly a marked allodynia in the ipsilateral paw compared with the contralateral paw (Fig. 7A, left panel). Higher dose perisciatic zymosan also induced a bilateral allodynia by 1 d and was also stably maintained across the 2 week observation period (Fig. 7B, left panel). This is the first demonstration that stable allodynias can be chronically produced by this SIN model. IL1ra injected intrathecally on day 14 reversed these SIN-induced pain changes within 2.5 hr (Fig. 7A,B, right panels).
These observations were supported by statistical analyses. ANOVA revealed reliable main effects of zymosan dose (F(2,36) = 46.844; p < 0.0001) and laterality (F(1,36) = 18.455; p < 0.0001), and interactions between sciatic treatment and laterality (F(2,36) = 8.550; p < 0.0001). Post hoc means comparison revealed that 4 µg zymosan (Fig. 7A) induced mechanical allodynia in the left (ipsilateral) hindpaw compared with the right (contralateral) hindpaw (p < 0.0001). Mechanical responses of the right hindpaw after 4 µg perisciatic zymosan did not differ from that after perisciatic vehicle, showing that 4 µg zymosan induced only a unilateral allodynia ipsilateral to the site of injection. In addition, post hoc analyses showed that bilateral mechanical allodynia occurred in response to 160 µg perisciatic zymosan (Fig. 7B). The thresholds for both the left and right paws for all of these groups were reliably different from those of the vehicle controls (p < 0.0001). At 14 d, either IL1ra or vehicle was injected intrathecally. Behavior was then recorded for 2.5 hr. Although IL1ra had no effect in the absence of perisciatic zymosan, it completely reversed unilateral allodynia (Fig. 7A, right) and greatly reduced bilateral allodynia (Fig. 7B, right) induced by perisciatic zymosan. ANOVA revealed reliable main effects of intrathecal IL1ra (F(4,42) = 91.950; p < 0.0001), and laterality (F(1,42) = 53.390; p < 0.0001), and time (F(4,168) = 48.251; p < 0.0001), and interactions between intrathecal IL1ra and laterality (F(4,42) = 22.964; p < 0.0001) and time and intrathecal IL1ra (F(16,168) = 8.799; p < 0.0001).
Post hoc means comparisons showed that IL1ra abolished the allodynic effects of 4 µg zymosan by 2.5 hr on day 14 (p < 0.0001 comparing the ipsilateral paw of rats receiving 0 or 4 µg zymosan with intrathecal IL1ra) (Fig. 7A, right). This drug greatly reduced the bilateral allodynic effects of 160 µg perisciatic zymosan by 2.5 hr on day 14 as well (p < 0.0001 comparing the ipsilateral paw of rats receiving 160 µg zymosan with or without intrathecal anti-IL6; p < 0.0001 comparing the contralateral paw of rats receiving 160 µg zymosan with vs without intrathecal IL1ra) (Fig. 7B, right). Intrathecal IL1ra, in the absence of perisciatic zymosan, had no effect on paw withdrawal thresholds, compared with intrathecal vehicle controls.
Discussion
These experiments provide the first identification of spinal mediators of mirror-image low-threshold mechanical allodynia. They also provide the first identification of neurochemical bases of inflammatory neuropathy-induced pain. These data support the conclusion that spinal cord glia and proinflammatory cytokines (TNF, IL1, IL6) are key mediators of these pathological pain phenomena. These experiments thus support and extend the recent report that spinal proinflammatory cytokines (IL1) induce allodynia and hyperexcitability of pain transmission neurons (Reeve et al., 2000
SIN is not alone in creating mirror-image effects. As noted above, numerous clinical pain syndromes are associated with mirror-image pain, primarily allodynic in nature. Mirror-image thermal hyperalgesia and mechanical allodynia have also been observed in diverse animal models of pathological pain (Seltzer et al., 1990
The involvement of glia in creating mirror-image effects is intriguing. Glia are well suited for creating expansions of the body region from which pain is perceived, for two reasons. First, proinflammatory cytokines act in a paracrine manner to excite distant cells (Watkins et al., 1999
Although the present data support a role for glial activation in mediating the allodynic effects of sciatic nerve inflammation, they do not indicate how nerve inflammation leads to glial activation. There are three obvious possibilities. The first is that glia are directly activated by neurotransmitters released in the dorsal horn by the inflamed sensory neurons. Indeed astrocytes and microglia may be activated by "pain" neurotransmitters, including substance P, ATP, calcitonin gene-related peptide (CGRP), and glutamate. Spinal cord astrocytes are activated by substance P-binding neurokinin-1 (NK-1) receptors (Palma et al., 1997
The second possibility is that sciatic inflammation activates spinal glia indirectly. Dorsal horn neurons are strongly activated in response to SIN, and strong neuronal activation can release fractalkine from the neuronal external surface (Chapman et al., 2000
