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The Journal of Neuroscience, September 28, 2005, 25(39):8825-8832; doi:10.1523/JNEUROSCI.0160-05.2005
Previous Article | Next Article
Cellular/Molecular
Bradykinin-Induced Functional Competence and Trafficking of the-Opioid Receptor in Trigeminal Nociceptors
Amol M. Patwardhan,1 Kelly A. Berg,1 Armen N. Akopain,2 Nathaniel A. Jeske,2 Nikita Gamper,3 William P. Clarke,1 andKenneth M. Hargreaves1,2 Departments of 1Pharmacology, 2Endodontics, and 3Physiology, University of Texas Health Science Center at San Antonio, San Antonio, Texas 78229
Abstract
Top
Abstract
Introduction
Peripheral opioid analgesia is increased substantially after inflammation. We evaluated the hypothesis that an inflammatory mediator, bradykinin (BK), evokes functional competence of the-opioid receptor (DOR) for inhibiting trigeminal ganglia (TG) sensory neurons. We also evaluated whether BK evokes trafficking of the DOR to the plasma membrane. Rat TG cultures were pretreated with BK (10 µM) or vehicle, and the effects of DOR agonists ([D-Pen2,5]-enkephalin or [D-Ala2, D-Leu5]-enkephalin) on BK (10µM)/prostagladin E2 (PGE2; 1 µM)-stimulated immunoreactive calcitonin gene-related peptide (iCGRP) release or PGE2 (1 µM)-stimulated cAMP accumulation were measured. The effect of BK treatment on opioid receptor trafficking was evaluated by DOR immunohistochemistry, cell-surface DOR biotinylation, and live imaging of neurons transfected with mDOR–green fluorescent protein. BK pretreatment rapidly and significantly increased DOR agonist inhibition of evoked iCGRP release and cAMP accumulation. These effects of BK pretreatment were blocked by a B2 receptor antagonist (HOE-140; 10µM) or a protein kinase C (PKC) inhibitor [bisindolymaleimide (BIS); 1µM]. Moreover, BK treatment rapidly and significantly increased the accumulation of DOR in the plasma membrane. However, BK-induced trafficking of DOR was not reversed by pretreatment with BIS, nor was trafficking evoked by application of a PKC activator PMA (200 nM). These data suggest that BK, in a PKC-dependent manner, induces rapid functional competence of DOR for inhibiting TG nociceptors and in a PKC-independent manner rapidly induces trafficking of DOR to the plasma membrane. These findings indicate that exposure to certain inflammatory mediators rapidly alters the signaling properties and neuronal localization of DOR, possibly contributing to peripheral opioid analgesia.
Key words: bradykinin;
Introduction
Peripherally administered opioids have higher efficacy for inhibiting hyperalgesia in inflammatory conditions compared with uninjured tissue (Joris et al., 1987; Stein et al., 1989
The
In the present study, we addressed three major hypotheses: first, that application of BK rapidly induces functional DOR competence as measured by inhibition of evoked neuropeptide exocytosis and by inhibition of stimulated adenylyl cyclase activity; second, that application of BK induces DOR competence by insertion of receptor into the plasma membrane; and third, that these actions of BK are mediated by protein kinase C (PKC)-dependent signaling pathways.
Materials and Methods
Animals. Adult male Sprague Dawley (Charles River Laboratories, Wilmington, MA) rats weighing 250–300 g were used in this study. All animal study protocols were approved by the Institutional Animal Care and Use Committee of the University of Texas Health Science Center at San Antonio and conformed to the International Association for the Study of Pain and federal guidelines. Animals were housed for 1 week before the experiment with food and water available ad libitum.Compounds. [D-Pen2,5]-enkephalin (DPDPE), [D-Ala2, D-Leu5]-enkephalin (DADLE), naltrindole, BK, HOE-140 (all from Sigma, St. Louis, MO), and deltorphin (Bachem California, Torrance, CA) were all made up in stock solutions of double-distilled H2O on the day of the experiment. Bisindolylmaleimide (BIS) and phorbol-12-myristate-13-acetate (PMA; Calbiochem, La Jolla, CA) were dissolved in DMSO and diluted in buffer (final, 0.05% DMSO). Prostagladin E2 (PGE2) (Cayman Chemical, Ann Arbor, MI) was made in stock solutions with ethanol (EtOH) and diluted by buffer on the day of the experiment (final, 0.01% EtOH).
Rat trigeminal ganglia primary culture. Trigeminal ganglia (TG) were removed quickly after decapitation, placed in ice-cold calcium- and magnesium-free HBSS (Invitrogen, San Diego, CA), and washed twice with HBBS. Ganglia were then treated with 5 mg/ml collagenase (Sigma) for 30 min and 0.1% trypsin (Sigma) for 15 min before homogenization. The TG were then treated with 10 U of DNase I (Roche, Indianapolis, IN), centrifuged at 2000 rpm for 2 min, and resuspended in DMEM (Invitrogen), which also contained 1x penicillin–streptomycin (Invitrogen), 1x glutamine (Invitrogen), 3 µg/ml 5-fluoro-2-deoxyuridine, 7 µg/ml uridine (Sigma), 10% fetal calf serum (Invitrogen), and 100 ng/ml nerve growth factor (NGF; Harlan, Indianapolis, IN). The tissue was triturated gently, and cells from six ganglia were plated on one 48-well poly-D-lysine-coated plate (BD Biosciences, Bedford, MA), yielding
4000 cells per well. For the immunohistochemical and cell-surface biotinylation experiments, cells were plated on poly-D-lysine-coated coverslips or 10 cm plates, respectively. The media were replaced at the end of 24 h and then 48 h later.
CGRP release assay. All culture experiments were performed on days 5–7, at 37°C, using modified HBSS (Invitrogen) (10.9 mM HEPES, 4.2 mM sodium bicarbonate, 10 mM dextrose, and 0.1% bovine serum albumin were added to 1x HBSS). After two initial washes, a 15 min baseline sample was collected. The cells then were exposed to either vehicle or BK (10 µM) for 15 min; samples were collected, and cells were exposed to either vehicle or test opioid (15 min) and stimulated with the combination of BK (10 µM)/PGE2 (1 µM) for 15 min. In experiments using B2 antagonist or PKC inhibitor, the cells were pre-exposed to HOE-140 (10 µM) or BIS (1 µM) for 15 min before BK application. In experiments using the DOR antagonist, the cells were pre-exposed to naltrindole (2 µM) before the opioid application. All the supernatants were collected for analysis of immunoreactive calcitonin gene-related peptide (iCGRP) content by radioimmunoassay (RIA). The basal release was typically 4–6 fmol per well.
cAMP accumulation. The experimental protocol was identical to that of the CGRP release assay except for the fact that all these experiments included the phosphodiesterase inhibitor rolipram (10 µM). At the end of the experiments, neurons were exposed to 500 µl of ice-cold ethanol to extract cAMP. The EtOH-treated cells were kept at –20°C overnight. The day after evaporation and resuspension in RIA buffer in RIA tubes, cAMP levels were measured using RIA, as described previously (Berg et al., 1994
Superfusion of acutely isolated rat TG. As described previously (Ulrich-Lai et al., 2001
iCGRP RIA. A previously used (Garry et al., 1994
In situ hybridization and immunohistochemistry. In studies with combined in situ hybridization (ISH)/immunohistochemistry (IHC) analysis, cryosections of TG or coverslips containing cultured TG neurons were fixed with 4% formaldehyde, permeabilized with 0.5% Triton X-100, acylated in acetic anhydride, dehydrated in alcohol, and delipidated in chloroform. In situ hybridizations (55°C) were performed using DIG-cRNA (containing digoxigenin-UTP) probe against bradykinin receptor 2 (position 102–500; GenBank accession number NM 173100). After RNase treatment, slides/coverslips were washed with decreasing concentration of SSC buffer (final wash, 0.1x SSC at 55°C), and hybridization was detected using standard alkaline phosphate-based reaction (substrates BCIP-NBT; Roche). Slides/coverslips were then incubated with already characterized (Cahill et al., 2001b
(1:1000; Molecular Probes) to identify BK-responsive neurons (Cesare et al., 1999
Plasma membrane DOR labeling. Cultured TG neurons were treated with BK or BIS followed by BK and then biotinylated with EZ-Link Sulfo-NHS-LC-Biotin (0.5 mg/ml; Pierce, Rockford, IL) in PBS for 30 min at 4°C. Cells were rinsed three times with 50 mM glycine in PBS, two times with PBS, and lysed in general lysis buffer by 20 passes through a 25 ga needle. Lysates were clarified by centrifugation, and equal aliquots were retained for either immunoprecipitation with the above-mentioned antibody specific to DOR (1:1000; Chemicon) or precipitation with streptavidin-bound agarose beads. Precipitates were resolved by 12.5% SDS-PAGE, transferred to polyvinylidene difluoride, and visualized by Western blot analysis with antibodies specific to DOR. Results were quantified using NIH Image 1.62, with streptavidin-pecipitated bands normalized to respective immunoprecipitated bands. The specificity of the DOR antibody was confirmed by preincubating the antibody with the appropriate blocking peptide.
Live imaging of DOR–green fluorescent protein trafficking. mDOR–green fluorescent protein (GFP) fusion protein was constructed by subcloning of the entire coding sequence of mDOR (apart from start codon) into pEGFP-N1 vector (BD Biosciences) between EcoRI and BamHI restriction sites. Cultured TG neurons (density, 50–75 cells per coverslip) were transfected using the PDS-1000/He Biolistic particle delivery system (Bio-Rad, Hercules, CA) according to the manufacturer's protocols. Twenty-four hours after transfection, we typically observed one or two cells per coverslip demonstrating successful transfection. Fluorescent microscopy was performed with an oil-immersion 40x/1.30 numerical aperture objective and Polychrome IV monochromator (TILL Photonics, Pittsfield, MA). Drugs were prepared in standard external solution [containing the following (in mM): 140 NaCl, 5 KCl, 2 CaCl2, 1 MgCl2,10 D-glucose, and 10 HEPES, pH 7.4] and applied (37°C) through a recording chamber inlet. Images were collected every 5 s with equal exposure time of 50 ms and stored/analyzed with TILLvisION 4.0 software (TILL Photonics). The experiment was repeated nine independent times on independently transfected cultures, and a total of 20 transfected cells were observed. The statistical calculations were done using change in initial versus post-BK application fluorescence intensity in membrane and cytosolic areas of the tested cells.
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Figure 1. Bradykinin pretreatment rapidly evokes competence in DOR to inhibit TG nociceptors. A, Cultured TG neurons were treated with either vehicle (no BK pretreatment; squares; n = 6–8) or BK (10µM; triangles; n = 6–8) for 15 min and aspirated, and DPDPE (10 nM to 10 µM) modulation of BK (10 µM)/PGE2 (1 µM)-evoked iCGRP release was observed. Data are presented as mean ± SEM. ANOVA with Bonferroni's post hoc test (*p < 0.05). B, In a similar paradigm, BK pretreatment concentration varied from 10 nM to 10 µM with DPDPE (1 µM) (**p < 0.01). C, After vehicle or BK pretreatment, an effect of naltrindole (2 µM) pretreatment on DPDPE (1 µM) modulation of BK/PGE2-evoked iCGRP release was observed (n = 8; **p < 0.01). D, After appropriate pretreatments (15 min vehicle or BK, followed by vehicle or naltrindole), DPDPE (1 µM) modulation of PGE2-(1 µM) evoked cAMP accumulation was observed (n = 8; *p < 0.05). E, After BK (10 µM) pretreatment, DPDPE (100 pM to 1 µM) modulation of PGE2-evoked cAMP accumulation was observed in the presence (squares; solid line) or absence (triangles; dotted line) of naltrindole (20 nM). Veh, Vehicle; BL, baseline.
Data analysis. All experiments were conducted with n = 8 or more wells to determine the experimental observation and then repeated at least three times to conduct the statistical analysis. The CGRP data are presented as percentage of basal release (mean ± SEM), and cAMP accumulation data are presented as percentage of stimulus (PGE2; mean ± SEM). Data were analyzed using GraphPad (San Diego, CA) Prism software version 4. The DPDPE-treated groups (with or without BK pretreatment) were compared with respective (with or without BK pretreatment) control BK/PGE2 groups. Multifactorial experimental data were analyzed using single-factor, two-way-ANOVA, multiple treatment data were analyzed using one-way-ANOVA, and individual groups were compared using a Bonferroni's post hoc test, whereas experiments examining the difference between two groups were analyzed by using a two-tailed t test. The statistical significance was tested at 0.05.
Results
Bradykinin pretreatment rapidly evokes competence in DOR to inhibit TG nociceptors
To test our hypothesis of BK modulation of DOR function, we exposed cultured TG neurons to either vehicle or BK (10 µM) for 15 min and then determined DPDPE (10 nM to 10 µM) modulation of BK (10 µM)/PGE2 (1 µM)-evoked iCGRP release (Fig. 1A). In the absence of BK (i.e., vehicle pretreatment), DPDPE did not inhibit BK/PGE2-evoked iCGRP release at any of the concentrations tested; indeed, a trend toward potentiation was observed. However, after BK pretreatment, DPDPE significantly inhibited BK/PGE2-evoked iCGRP release in a concentration-dependent manner with a maximal inhibition of 49% (p < 0.05). We next evaluated the concentration dependence of BK for altering DPDPE (1 µM) inhibition of BK/PGE2-evoked iCGRP release (Fig. 1B). The results demonstrated that BK pretreatment (10 nM to 10 µM) initiates DOR competence in a concentration-dependent manner (p < 0.01). The post-BK pretreatment inhibitory effect of DPDPE (1 µM) on BK/PGE2-evoked iCGRP release was completely blocked by treatment with the DOR antagonist naltrindole (2 µM) (Fig. 1C).We then tested our hypothesis by evaluating the effect of BK pretreatment on DOR inhibition of stimulated adenylyl cyclase activity (Fig. 1D). Pretreatment with BK (10 µM), but not vehicle, resulted in the rapid development of a significant DPDPE (1 µM) inhibition of PGE2 (1 µM)-stimulated cAMP accumulation by 67% (p < 0.01). This effect was blocked by treatment with naltrindole (2 µM). After BK pretreatment, the application of DPDPE (100 pM to 1 µM) produced a concentration-dependent inhibition of PGE2-stimulated cAMP accumulation (Fig. 1E). This DPDPE concentration–response curve was right-shifted in cultures treated with the DOR antagonist naltrindole (20 nM).
BK pretreatment produces DOR competence regardless of the DOR agonist used
Because agonist-specific signaling of GPCRs has been proposed (Berg et al., 1998BK pretreatment is necessary for the inhibitory effect of DPDPE in acutely isolated and superfused rat TG
To verify that the BK pretreatment effect is not an artifact of culturing conditions, we next evaluated the requirement for BK pretreatment on DPDPE modulation of BK/PGE2-evoked iCGRP release using acutely isolated and superfused rat TG slices (Ulrich-Lai et al., 2001BK-evoked DOR inhibitory competence is mediated by activation of bradykinin B2 receptor that is coexpressed with DOR in rat TG
Because many actions of BK on NGF treated sensory neurons are mediated via B2 receptor (Vellani et al., 2004BK evoked DOR competence is mediated via activation of PKC
BK-induced activation of the B2 receptor leads to PKC signaling in many sensory neurons (Cesare et al., 1999
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Figure 2. BK pretreatment produces DOR competence regardless of the DOR agonist used. A, The effect of pretreatment with vehicle (Veh) or BK (10µM) on DADLE (100 nM) modulation of BK/PGE2-evoked iCGRP release was determined using the paradigm of Figure 1C (n = 8; *p < 0.05). B, The effect of BK pretreatment on DADLE (100 nM) modulation of PGE2-evoked cAMP accumulation was determined using the paradigm of Figure 1 D (n = 8; *p < 0.05). BL, Baseline. Error bars represent SEM.
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Figure 3. BK pretreatment is necessary for the inhibitory effect of DPDPE in acutely isolated and superfused rat TG. In acutely dissociated rat TG, after a washout time and collection of three fractions for basal release of iCGRP, tissue was superfused with BK (10 µM) or vehicle for two 7 min fractions, and DPDPE (1µM) modulation of BK (10µM)/PGE2 (1µM)-evoked iCGRP release was observed (n = 8; *p < 0.05). BL, Baseline. Error bars represent SEM.
BK evokes trafficking of DOR to the plasma membrane in a PKC-independent manner
Because inflammation induces axonal trafficking of DOR toward inflamed tissue (Hassan et al., 1993
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Figure 4. BK-evoked DOR inhibitory competence is mediated by activation of bradykinin B2 receptor that is coexpressed with DOR in rat TG. A, Effect of pretreatment with B2 antagonist HOE-140 (10 µM) on BK-evoked DPDPE modulation of PGE2-stimulated cAMP accumulation (n = 8; *p < 0.05). Error bars represent SEM. B, Coexpression of B2 mRNA (left) and DOR immunoreactivity (right) in cultured TG neurons. Pictures were taken at 60x. The horizontal arrows denote examples of coexpressing cells. The vertical arrows denote examples of B2-expressing cells that do not express DOR. C, Coexpression of B2 mRNA (left) and DOR immunoreactivity (right) in native TG neurons. Pictures were taken at 20x. Arrows denote examples of coexpressing cells. D, Coexpression of B2 immunoreactivity (left) and DOR immunoreactivity (right) in cultured TG neurons. Pictures were taken at 60x. E, Coexpression of B2 immunoreactivity (left) and CGRP immunoreactivity (right) in cultured TG neurons. Pictures were taken at 60x (picture shows example of 1 cell coexpressing both or another cell coexpressing neither). Veh, Vehicle; -ir, immunoreactivity.
Live imaging of sensory neurons expressing DOR–GFP fusion protein confirms BK-induced trafficking of DOR
We evaluated BK-evoked trafficking of DOR using a third independent method. We transfected cultured TG neurons with a DOR–GFP-containing vector and observed changes in green fluorescence intensity after BK treatment. Because in rat TGs, B2 receptor is predominantly expressed in small- to medium-sized neurons, we evaluated BK-induced trafficking of DOR only in cells in that diameter range. We observed two types of neurons in these cultures. One group of cells did not show any change in fluorescence intensity in plasma membrane or cytosol after either vehicle treatment or BK treatment (Fig. 7A). However, another group of cells responded to BK application with a gradual increase in fluorescent signal in the plasma membrane accompanied with a gradual decrease in intensity in the cytosol (Fig. 7B). Of the total 20 cells tested, eight cells showed DOR trafficking to the plasma membrane. In a digitally magnified image of the plasma membrane of a BK-responsive cell, the membrane fluorescence becomes well defined only after application of BK suggestive of insertion of additional DOR to the plasma membrane (Fig. 7C). Additional quantification of change in cytosolic and membrane fluorescence in BK-responsive cells showed that BK application resulted in a significant (17.6%; p < 0.01) increase in plasma membrane intensity accompanied by a 7.2% decrease in cytosolic intensity.
Discussion
The results from this study demonstrate that signaling events occurring via activation of the B2 receptor rapidly lead to a functional competence in the DOR for inhibition of TG nociceptors. This BK-evoked DOR inhibitory competence was concentration dependent and was observed regardless of the DOR agonist used, dependent measure (iCGRP and cAMP) used, or cellular model (cultured and acutely dissociated TG) studied. Moreover, using three independent methods, we demonstrate that BK induces rapid trafficking of DOR to the plasma membrane. Although the priming effect of BK on DOR competence is PKC dependent, BK-induced DOR trafficking effect is independent of PKC signaling.
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Figure 5. BK-evoked DOR competence is mediated via activation of PKC. A, Effect of pretreatment with BIS (1 µM) on BK-evoked DPDPE inhibition of BK/PGE2-evoked iCGRP release (n = 8; **p < 0.01). B, Effect of pretreatment with BIS (1 µM) on BK-evoked DPDPE inhibition of PGE2-evoked cAMP accumulation (n = 8; **p < 0.01). Separate cultures were exposed to pretreatment with PMA (200 nM) to evaluate DPDPE modulation of PGE2-evoked cAMP accumulation (n = 8; **p < 0.01). BL, Baseline; Veh, vehicle. Error bars represent SEM.
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Figure 6. BK evokes trafficking of DOR to the plasma membrane in a PKC-independent manner. A, Cultured TG cells were treated with vehicle (Veh)/BIS (1µM), followed by Veh/BK (10µM). Cells were biotinylated and lysed.Streptavidin-precipitated(Precip)bands normalized to respective immunoprecipitated bands(Western blot shown at the top with the blocking peptide control). Finally, data were presented as a percentage of vehicle-treated cells (n = 3; **p < 0.01). B, Cultured TG cells were treated with vehicle (VEH)/BK (10µM)/PMA (200 nM) for 15 min. Cells were then fixed, and double immunohistochemistry was performed for DOR-ir (green; top) and PKC
Peripherally administered opioid agonists display increased efficacy after inflammation. Several studies suggest multiple mechanisms could account for this phenomenon, and they include release of endogenous opioid ligands, increased opioid receptor expression, and axonal trafficking, sensory nerve sprouting, disruption of perineural barrier, and alternation in agonist efficacy (Cahill et al., 2003The present study demonstrates that activation of B2 signaling via the PKC pathway leads to rapid functional competence of DOR for inhibiting TG nociceptors. In the absence of BK pretreatment, we observed either no or slight excitatory effects of DOR activation in agreement with other groups (Bao et al., 2003
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Figure 7. Live imaging of sensory neurons expressing DOR–GFP fusion protein confirms BK induced trafficking of DOR. A, A representative cell showing change in green fluorescence (DOR–GFP) in cytoplasm (black) and plasma membrane (red) over time after BK (10µM) application (blue line shows time point of BK application). B, A representative cell expressing DOR–GFP fusion protein is shown at top. Changes in green fluorescence (DOR–GFP) in cytoplasm (black) and plasma membrane (red) over time after BK (10 µM) application (blue line shows time point of BK application). C, Membrane close-up of a representative cell showing that after BK (10 µM) application, membrane DOR–GFP fluorescence becomes more defined (arrow). D, Quantification of change in fluorescence in plasma membrane and cytosol after BK (10 µM) application (n = 8; **p < 0.01). Error bars represent SEM.
Inflammation leads to increased axonal trafficking of DOR toward terminals innervating inflamed tissue (Hassan et al., 1993-opioid receptors in pituitary (Shuster et al., 1999
In summary, the present study is consistent with the hypothesis that the inflammatory mediator BK rapidly evokes functional DOR competence to inhibit nociceptor function. Moreover, BK evokes DOR trafficking in a PKC-independent manner. The findings of this study might help in developing a better analgesic strategy in conditions such as neuropathic pain in which peripheral opioid administration is less efficacious.
Footnotes
Received Jan 12, 2005; revised August 4, 2005; accepted August 5, 2005.This work was supported by National Institute on Drug Abuse P01 Grant DA 016179 (K.M.H.) and by National Institute of Dental and Craniofacial Research Grant DE016500 (N.A.J.). We thank Teresa Sanchez, Gaby Helesic, Amanda Trott, and Jaime Cerecero for technical assistance.
Correspondence should be addressed to Dr. Ken M. Hargreaves, University of Texas Health Science Center at San Antonio, 7703 Floyd Curl Drive, San Antonio, TX 78229-3900. E-mail: Hargreaves{at}UTHSCSA.edu.
DOI:10.1523/JNEUROSCI.0160-05.2005
Copyright © 2005 Society for Neuroscience 0270-6474/05/258825-08$15.00/0
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