Abstract
Multiple voltage-gated calcium channels (VGCCs) contribute to the processing of nociceptive signals in primary afferent fibers. In addition, alteration of calcium channel activity is associated with a number of chronic pain conditions. Therefore, VGCCs have emerged as prime target for the management of either neuropathic or inflammatory pain, and selective calcium channel blockers have been shown to have efficacy in animal models and in the clinic. However, considering that multiple calcium channels contribute pain afferent signaling, broad-spectrum inhibitors of several channel isoforms may offer a net advantage in modulating pain. Here, we have analyzed the ability of the compound surfen to modulate calcium channels, and assessed its analgesic potential. We show that surfen is an equipotent blocker of both low- and high-voltage-activated calcium channels. Furthermore, spinal (intrathecal) delivery of surfen to mice produces sustained analgesia against both acute and chronic pain. Collectively, our data establish surfen as a broad-spectrum calcium channel inhibitor with analgesic potential, and raise the possibility of using surfen-derived compounds for the development of new pain-relieving drugs.
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Introduction
Voltage-gated calcium channels (VGCCs) are essential contributors to the processing of peripheral nociceptive information within neurons of the dorsal root ganglion (DRG) [4, 60]. Among the various VGCCs expressed in DRG neurons [33, 47, 57, 67], the high-voltage-activated (HVA) Cav2.2 (N-type) and low-voltage-activated (LVA) Cav3.2 (T-type) channels are the main calcium channels isoforms that mediate processing of the pain signals. For instance, Cav2.2 channels are predominantly expressed in presynaptic terminals of afferent nerve fibers where they support evoked release of pronociceptive neurotransmitters such as glutamate, substance P and calcitonin gene-related peptide (CGRP) [7, 29, 45, 49]. In contrast, Cav3.2 channels are expressed along axons where they possibly regulate the excitability of afferent fibers via their electrogenic function that may facilitate the opening of voltage-gated sodium channels [16]. In addition, Cav3.2 channels expressed in nerve endings in skin hair follicles [42] are essential for mechanotransduction [8, 15], and contribute to mechanical allodynia [35]. Finally, Cav3.2 channels also contribute to excitatory synaptic transmission in the dorsal horn of the spinal cord [19], possibly by supporting low-threshold release of neurotransmitters by virtue of their interaction with the synaptic vesicle release machinery [61, 62]. Consequently, Cav2.2 and Cav3.2 channels play a major role in the development and maintenance of neuropathic pain, and have thus emerged as prime targets for its treatment [38, 68]. In addition, there is also evidence for a role of other VGCC members. For instance, Cav1.2 and Cav1.3 channels (L-type) are present in neurons of the dorsal horn of the spinal cord [6, 52] where they contribute to sensitization to pain [41]. Moreover, a role for Cav2.3 channels (R-type) in the spinal transmission of the pain signal was also reported [31, 55], along with a role for Cav3.3 channels [64]. Given that multiple calcium channels contribute to the processing of peripheral pain signaling, broad-spectrum inhibitors of VGCCs may represent an effective mean of mediating analgesia.
Surfen (bis-2-methyl-4-amino-quinolyl-6-carbamide) was first described in the late thirties as a byproduct in the production of depot insulin [58], and was later reported to block C5a receptor binding [24] and to inhibit anthrax lethal factor [36]. More recently, surfen was shown to inhibit heparan sulfate [46, 63]. Here, we report that surfen is a potent, broad-spectrum inhibitor of VGCCs. An electrophysiological analysis indicates that surfen effectively inhibits recombinant and native VGCC channels in DRG neurons. In addition, our results reveal that surfen produces sustained analgesia when delivered intrathecally in mouse models of acute and chronic inflammatory pain.
Materials and methods
Cell culture and heterologous expression
Human embryonic kidney tsA-201 cells were gown in DMEM medium supplemented with 10% fetal bovine serum (FBS) and 1% streptomycin/penicillin (all media from Invitrogen), and maintained under standard conditions at 37 °C in a humidified atmosphere containing 5% CO2. Cells were plated out onto 60 mm dishes and transfected using the calcium/phosphate method with cDNAs encoding human Cav1.2 or Cav2.1 channels along with β1b and α2δ-1. Human Cav3.2 and Cav3.3 channels were expressed alone as previously described [25]. The CHO cell line stably transfected with rat Cav2.2-EGFP/α2δ-1/β was previously described [30] and grown in MEM alpha medium supplemented with 10% FBS, 200 mM L-glutamine, 0.7 mg/ml G418, 0.25 mg/ml hygromycin B and 0.005 mg/ml blasticidin.
DRG neuron culture
DRG neurons from 5- to 6-week-old mice were dissociated enzymatically with 0.7 mg/ml collagenase (Sigma-Aldrich) and 5 mg/mL trypsin-EDTA (Thermo-Fisher) in HBSS for 1 h at 37 °C, followed by mechanical trituration with fire-polished Paster pipette. Cells were seeded in 35 mm dishes coated with Poly-L-Lysine (Sigma-Aldrich) in DMEM medium supplemented with 10% FBS and penicillin-streptomycin (Thermo-Fisher).
Patch-clamp electrophysiology
Recording of barium currents in the whole-cell configuration of the patch-clamp technique in tsA-201 cells expressing various calcium channels was performed 72 h after transfection in a bath solution containing (in millimolar): 5 BaCl2, 5 KCl, 1 MgCl2, 128 NaCl, 10 TEA-Cl, 10 D-glucose, 10 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid (HEPES) (pH 7.2 with NaOH). Patch pipettes had a resistance of 2–4 MΩ when filled with a solution containing (in millimolar): 110 CsCl, 3 Mg-ATP, 0.5 Na-GTP, 2.5 MgCl2, 5 D-glucose, 10 EGTA, and 10 HEPES (pH 7.4 with CsOH). Whole-cell patch-clamp recordings were performed using an Axopatch 200B amplifier (Axon Instruments). Acquisition and analysis were performed using pClamp 10 and Clampfit 10 software, respectively (Axon Instruments). Ba2+ currents were recorded in response to depolarizing steps to various potentials applied every 5 or 10 s from a holding potential of −100 or −80 mV for LVA and HVA channels, respectively. The linear leak component of the current was corrected online and current traces were digitized at 10 kHz, and filtered at 2 kHz. The voltage dependence of the peak Ba2+ current density was fitted with the following modified Boltzmann equation:
with I(V) being the peak current amplitude at the command potential V, Gmax the maximum conductance, Vrev the reversal potential, V 0.5 the half-activation potential, and k the slope factor.
The steady-state voltage dependence of inactivation of the Ba2+ current was determined by measuring the peak current amplitude in response to a 150 ms-long depolarizing step to +10 mV (Cav2.2) or −20 mV (Cav3.2) applied after a 5-s-long conditioning prepulse at various voltages. The current amplitude obtained during each test pulse was normalized to the maximum at −80 mV (Cav2.2) or −100 mV (Cav3.2) and plotted as a function of the prepulse potential. The voltage dependence of the steady-state inactivation was fitted with the following two-state Boltzmann function:
with I max corresponding to the maximal peak current amplitude and V 0.5 to the half-inactivation voltage.
Recording of calcium currents in primary DRG neurons was performed after 24 h in culture and elicited with a ramp command (0.5 V/s) from a holding potential of −90 mV as previously described [5]. For recording of Nav currents, the bath solution contained (in millimolar): 35 NaCl, 30 TEA-Cl, 65 choline-Cl, 5 MgCl2, 10 HEPES, 10 D-glucose, and 0.05 CdCl2 (pH 7.2). The pipette solution contained (in millimolar): 100 CsCl, 40 TEA-Cl, 5 NaCl, 1 CaCl2, 2 MgCl2, 11 EGTA, 10 HEPES, 2 Mg-ATP, and 1 Li2GTP (pH 7.2). For recording of K v currents, the bath solution contained (in millimolar): 140 choline-Cl, 4 KCl, 1 MgCl2, 1.8 CaCl2, 0.1 CdCl2, 10 D-glucose, and 10 HEPES (pH 7.2). The pipette solution contained (in millimolar): 140 KCl, 4 NaCl, 1 MgCl2, 10 EGTA, 2 Na2-ATP, and 10 HEPES (pH 7.2). All experiments were performed at room temperature (22–24 °C).
Animals and surfen treatment
All experiments were approved by the Institutional Care and Use Committee and carried out according the guidelines of the Internal Association for the Study of Pain. Efforts were made to minimize animal suffering and distress. Adult (7–9 weeks old) male C57BL/6 J mice were kept on a 12 h light/dark cycle at a maximum of five per cage in a room maintained at 23 ± 1 °C with ad libitum access to food and water. To verify if surfen produces antinociception when delivered spinally to mice, intrathecal (i.t.) injections were performed using volumes of 10 μl and according the method described by Hilden and Wilcox [18] and as routinely performed in our laboratory [10, 11]. Control groups were assessed simultaneously. Surfen was dissolved in 1% or less DMSO, whereas control animals received PBS +1% DMSO (which was the concentration of DMSO in the highest dose delivered to mice in the formalin test). Each mouse was tested only once.
Formalin test
Formalin-induced acute pain was performed as originally described [17]. After a period of at least 60 min acclimation, mice were injected intraplantarily (i.pl.) in the ventral surface of the right hindpaw with 20 μL of a formalin solution (1.25%) prepared in PBS. Immediately after intraplantarily injection of formalin, mice were placed individually into observation chambers and monitored for the time spent licking of biting the injected paw as a mean to assess nocifensive response. Animals were observed from 0 to 5 min and 15 to 30 min to assess acute nociceptive and inflammatory phases, respectively. Surfen was delivered intrathecally (i.t.) 20 min prior injection of formalin and its effect against both nociceptive and inflammatory phases was evaluated.
Persistent inflammatory pain induced by CFA
To induce thermal hyperalgesia caused by peripheral inflammation, animals received 20 μl of CFA injected i.pl. in the right hind paw as performed previously [10]. Sham groups received 20 μl of PBS in the ipsilateral paw. Animals were treated with either surfen (10 μg/i.t.) or vehicle (10 μl/i.t.) 2 days following CFA injection and their thermal withdrawal threshold was subsequently tested.
Measurement of thermal hyperalgesia
Immediately before receiving CFA (baselines) and 2 days after CFA injection (time-course testing day), animals were accessed on a plantar test apparatus (Hargreaves, UgoBasile, Varese, Italy) and the latency to withdrawal the right hindpaws from an infra-red radiant heat (IR = 30%) was scored. Mice were kept individually in enclosed testing chambers (10 cm × 10 cm × 13 cm, length × width × height) placed on top of a glass floor and were allowed to acclimate before testing for at least 120 min. The infra-red heat source was placed underneath the right hind paw and three measurements were taken for each mouse. The cut-off time was set at 30 s to avoid tissue damage.
Chemicals
All chemicals were purchased from Sigma-Aldrich. Surfen (Sigma S6951) was dissolved in DMSO to prepare a stock solution of 10 mM, and was diluted in the external recording solution prior to the experiments so that the final concentration of DMSO was 0.1% or less. Pertussis toxin (PTX) was dissolved in distilled water and applied to the cell at 1 μg/ml for 24 h. The PLC inhibitor U73122 was dissolved in DMSO to prepare a stock solution of 5 mM and applied to the cells at 10 μM for 30 min.
Statistical analysis
Statistical significance for electrophysiology data was determined using a paired or unpaired Student’s t test. For behavioral analysis, data were evaluated by one-way or two-way ANOVA followed by Tukey’s test. All data are presented as mean ± standard error. Value of p ≤ 0.05 was considered to be significant (*p ≤ 0.05; **p ≤ 0.01; ***p ≤ 0.001).
Results
Surfen is an effective inhibitor of voltage-gated calcium channels
We performed whole-cell patch-clamp recordings to assess the ability of surfen to mediate tonic block of various recombinant VGCCs involved in pain transmission. Representative current traces recorded for HVA channels (Cav1.2, Cav2.1, and Cav2.2) and LVA channels (Cav3.2 and Cav3.3) are shown in Fig. 1b before (black traces) and after (gray traces) application of 10 μM surfen. Application of surfen produced robust current inhibition of all calcium channels tested (ranging from 69 ± 2% for Cav2.2 to 84 ± 2% for Cav3.2) (Fig. 1c). We next further analyzed the blocking properties of surfen on the two main calcium channel isoforms (Cav2.2 and Cav3.2) involved in the processing of peripheral nociceptive information. The dose-response relation for block of Cav2.2 and Cav3.2 channels is shown in Fig. 2a, b, respectively. The IC50 values obtained from the fit of the dose-response curves were 1.3 and 2.7 μM for Cav2.2 and Cav3.2 channels, respectively, and did not significantly differ (p = 0.2564). The Hill coefficients were 0.6 and 0.4 for Cav2.2 and Cav3.2 (p = 0.5796), respectively, and in both cases (and in particular for Cav2.2) block appeared to be incomplete at a saturating concentration. The effect of surfen on the voltage dependence of Cav2.2 and Cav3.2 is shown in Fig. 2c, d, respectively. At a concentration of 10 μM, surfen blocked Cav2.2 and Cav3.2 channels at all test potentials, but did not significantly alter the mean half-activation potential (−6.5 ± 0.5 mV versus 0.9 ± 1.6 mV, n = 10 for Cav2.2 channels, and −47.1 ± 1.9 mV versus − 45.6 ± 6.5 mV, n = 9 for Cav3.2 channels). Similarly, there was no significant difference in the mean half-steady-state inactivation potential (−26.3 ± 0.5 mV versus − 26.5 ± 1.0 mV, n = 7 for Cav2.2 channels, and −71.7 ± 0.8 mV versus − 70.7 ± 0.9 mV, n = 10 for Cav3.2 channels) (Fig. 2e, f, respectively). The time course of inhibition at 10 μM for both Cav2.2 and Cav3.2 channels is presented in Fig. 2g, h, respectively, and required approximately 3–4 min to reach a steady-state block. The inhibition was irreversible and we did not observe obvious differences in the time course of inhibition at lower concentrations of surfen (data not shown).
To analyze the pharmacological properties of surfen under more physiological conditions, we assessed the ability of surfen to block native calcium channels in adult mouse DRG neurons. Patch-clamp recordings were performed on small DRG neurons (15–30 μm diameter) corresponding to unmyelinated nociceptive C fibers [65]. Representative current traces elicited by a ramp command (0.5 V/s) from a holding potential of −90 mV are shown in Fig. 3a before (black traces) and after application of 10 μM surfen (gray traces). Consistent with previous studies [3], we observed different electrophysiological profiles of small DRG neurons. A subset of cells displayed a combination of LVA and HVA currents (Fig. 3a, left panel), and application of surfen potently blocked both current components by 58 ± 4% (n = 7) and 69 ± 7% (n = 7), respectively (Fig. 3b, left side). The remaining cells exclusively expressed HVA currents (Fig. 3a, right panel) that were blocked by 64 ± 3% (n = 9) (Fig. 3b, right side). In contrast, we observed only a moderate block of voltage-gated sodium currents (Nav) by 20 ± 5% (n = 5) (Fig. 3c, left panel, and Fig. 3d) and of voltage-gated potassium currents (Kv) by 11 ± 4% (n = 5) (Fig. 3c, right panel, and Fig. 3d).
Altogether, these results indicate that surfen is a preferential broad-spectrum inhibitor of recombinant and native voltage-gated calcium channels in nociceptive neurons, with comparatively moderate effects on voltage-gated sodium and potassium channels.
Surfen-mediated inhibition of calcium channels does not rely on G-protein signaling
We next conducted a series of analysis in order to investigate the mechanisms behind surfen-induced imbibition of calcium channels. It was previously reported that surfen triggers Gβγ- and phospholipase C (PLC)-depend signaling by releasing Gβγ dimers from Gα-bound GDP without activating either G-protein coupled receptors (GPCRs) or Gα subunits and their downstream pathways [53]. Considering that one of the main mechanisms by which GPCRs modulate neuronal Cav2 calcium channels involves the activation of Gβγ [39], we explored the possibility that this regulation could support surfen-mediated inhibition of the channels. Direct inhibition of neuronal calcium channels by Gβγ dimers is typically assessed with a double pulse protocol where a conditioning prepulse to depolarized potentials relieves most of the inhibition (facilitation) [39]. Hence, we recorded Cav2.2 currents before (P1) and after (P2) application of a depolarizing prepulse (PP) to +100 mV to assess the implication of Gβγ in surfen-mediated inhibition of the channel. Representative current traces before (black trace) and after application of 10 μM surfen (gray trace) are shown in Fig. 4a. In control condition, application of a depolarizing prepulse produced a small current facilitation suggesting the existence of a slight tonic blockade of the channel likely caused by basal G-protein activity (Fig. 4a black trace and Fig. 4b). However, we did not observe any prepulse facilitation under surfen inhibition indicating that surfen-induced inhibition of Cav2.2 is voltage-independent ruling out a direct G-protein βγ-mediated inhibition of the channel (Fig. 4a gray trace and Fig. 4b). Consistent with this notion, pre-treatment of cells with pertussis toxin (PTX) for 24 h did not alter the ability of surfen to block Cav2.2 channels (Fig. 4c, d), indicating that Gi/o-coupled receptor signaling is not involved in surfen-mediated inhibition of the channels. Furthermore, pre-treatment of cells with the PLC inhibitor U73122 for 30 min had no effect on surfen-mediated inhibition of Cav2.2 channels (Fig. 4c, d).
Surfen mediates analgesia in acute and chronic inflammatory pain models
To evaluate the analgesic potential of surfen, we assessed the effect of the molecule against both nociceptive (phase 1) and inflammatory (phase 2) responses after formalin injection. Intrathecal (i.t.) injection of surfen produced effective and dose-dependent inhibition of nocifensive responses in both phases of the formalin test, such that injection of 10 μg/i.t. of surfen, 20 min before the injection of formalin, caused significant inhibition of the first phase by 55 ± 5% (Fig. 5a), and second phase by 77 ± 6% (Fig. 5b). Considering that surfen was highly effective in inhibiting the acute nocifensive response in the inflammatory phase of the formalin test, we further analyzed the analgesic potential of surfen on CFA-induced persistent inflammatory nociception. The ability of surfen to modulate CFA-induced hypersensitivity was assessed by thermal paw withdrawal latency (in seconds) in response to thermal stimulation. As shown in Fig. 6a, intrathecal injection of 10 μg/i.t of surfen produced a significant and long-lasting attenuation of CFA-induced thermal hyperalgesia (open circle) when compared with control animals who received intrathecal injection of PBS + 1% DMSO (dark circles). Notably, this effect was apparent as early as 20 min after the injection of surfen (p < 0.05), and remained sustainable up to over 180 min (p < 0.01).
Altogether, these data demonstrate the analgesic potential of surfen when injected intrathecally in mouse models of acute and chronic inflammatory pain.
Discussion
Initially described in the late thirties as a byproduct in the production of depot insulin [58], the therapeutic potential of surfen in the treatment of various chronic disorders has gained increasing attention. For instance, surfen and derivatives have been proposed as potential antibacterial agents (patent US20070112048) [2], and more recently for the treatment of tauopathies including Alzheimer’s disease (patent WO2013020909) [1]. Here, we report new pharmacological properties of surfen and demonstrate its analgesic potential in mouse models of acute and chronic inflammatory pain.
A number of voltage-gated calcium channels have been implicated in the processing of the pain signal with specific subcellular expression patterns and function [4]. Among them, Cav2.2 and Cav3.2 channels are validated drug targets for the management of pain in the clinic [37, 56, 59, 60, 68]. For instance, inhibition of Cav2.2 channels by opioid receptors represents one of the mechanisms by which morphine mediates analgesia [20]. In addition, the gabapentinoid drugs gabapentin (Neurontin™) and pregabaline (Lyrica™) that target the Cavα2δ-1 ancillary subunit to modulate Cav2.2 channels have shown clinical efficacy in patients with neuropathic pain [23]. Small peptide inhibitors of Cav2.2 channels isolated from cone snails toxins have also shown analgesic potential in animal pain models, and the ω-conotoxin MVIIA (Prialt™) was approved for the management of refractory chronic pain in patients [44, 51]. More recently, Cav3.2 channels have emerged as clinically relevant drug targets for the management of neuropathic pain. For instance, inhibition of Cav3.2 channels by intrathecal delivery of ethosuximide (Zarontin™) has shown clinical efficacy [21]. Furthermore, the T-type channel inhibitor Z944 is currently assessed in Phase II clinical trials for pain [26]. In addition to Cav2.2 and Cav3.2 channels that are validated clinical targets, there is evidence that spinal modulation other calcium channel members, including Cav1.2/Cav1.3 [66], Cav2.1 [9, 28, 34], Cav2.3 [31, 55], and Cav3.3 [64], can produce analgesia in animal pain models. Considering that a variety of calcium channels participate in the transmission and processing of pain signals, targeting multiple channels with broad-spectrum inhibitors may represent an effective avenue to mediate analgesia.
Here, we showed that surfen effectively blocks multiple voltage-gated calcium channels including L-type (Cav1.2), P/Q-type (Cav2.1), N-type (Cav2.2), and T-type (Cav3.2 and Cav3.3) channels, without apparent selectivity. Furthermore, surfen was also effective in blocking native LVA and HVA channels in small DRG neurons in culture, with only minimal blocking activity on Nav and K v channels. The ability of surfen to block LVA currents in small DRG neurons implies that this compound acts on native Cav3.2 channels as it is the only channel isoform to carry T-type currents in these neurons [3]. In contrast, our observation that surfen blocked up to 65% of the HVA current suggests that multiple HVA channel isoforms were blocked as none of the HVA channels expressed in small DRG neurons account for more than 30% of the whole HVA current [33].
Previous studies have suggested that surfen modulates neutrophil chemotaxis via a Gβγ- and PLC-dependent signaling pathway [53]. Here, we did not observe any evidence for the implication of Gβγ or PLC in surfen-mediated inhibition of the calcium channels. On the other hand, the observation that inhibition of Cav2.2 and Cav3.2 channels plateaued at 80% inhibition with similar pharmacological properties (IC50 values and Hill coefficients) may be consistent with a diffuse, but common effect by which surfen indirectly modulates the calcium channels rather than a direct block of the channel itself, although we cannot rule out the latter mechanism. Along these lines, surfen was recently reported as an antagonist of cell-surface heparan sulfate with the potential to prevent glycosaminoglycan (GAG)-protein interaction [46, 63]. Although not studied here, it is a possibility that surfen could modulate calcium channels by altering GAG-channel interactions. Consistent with this idea, reduced calcium influx in pyramidal hippocampal neurons after enzymatic removal of heparan sulfate was recently documented [32]. Consistent with this notion, direct binding of heparin to exofacial Cav1.2 channel regions such as the pore-forming loop connecting transmembrane segments S5 and S6 of the first domain was reported to modulate channel activity [12]. It is possible that binding of surfen to heparan sulfate could disrupt this interaction and alter channel activity. Further studies will be needed to uncover the role of heparan sulfate in functioning of calcium channels.
Regardless of the mechanism behind surfen-induced inhibition of calcium channels, our in vivo data revealed that inthrathecal delivery of surfen results in long-lasting analgesic effects in rodent models of acute and persistent inflammatory pain. These data are consistent with previous studies reporting analgesic effects of calcium channel blockers on inflammatory hyperalgesia. For instance, and consistent with the notion that Cav2.2 channels are up-regulated in CFA-induced inflammatory pain model [27], inhibition of Cav2.2 by aminopiperidine sulfonamide reduced inflammatory hyperalgesia [48]. Reduced inflammatory pain was also documented in mice lacking Cav2.2 channels [43]. Along these lines, inhibition of T-type channel activity using pharmacological blockers [40, 54] or small interfering peptides to reduce surface expression of the channel [13, 14] also produced marked analgesic effect on mouse models of inflammatory pain. Hence, it is reasonable to propose that reduced inflammatory hyperalgesia observed during the second phase of the formalin test and in CFA-induced inflammatory pain model was at least partly mediated by the ability of surfen to block calcium channels. It is worth noting that surfen was also reported to have anti-inflammatory activity [24] that could have contributed to the analgesic effect in the CFA model. In addition, and although our data indicate that surfen has only a minor blocking activity on Nav and K v channels that is unlikely to have had a major contribution to its analgesic properties (the slight blockade of K v channels would actually have a pronociceptive effect), we cannot rule out the possibility that surfen may have affected the functioning of other channels and receptors by virtue of its pharmacological activity on heparan sulfate which in turn may have contributed to the observed analgesic effect. For instance, modulation of angiotensin II-mediated signaling by heparan sulfate glycosaminoglycans has been reported [22] and the angiotensin II type 2 receptor is a potential target to modulate pain [50]. Yet, our pain data are consistent with numerous reports showing that blockade of calcium channels in vivo supports analgesia in various animal pain models.
Although selective inhibitors are usually preferred in order to limit the risk of side effects, broad-spectrum blockers may have an advantage especially for disorders like neuropathic pain where multiple channels are implicated. Hence, our data raise the possibility of using surfen-type compounds for the development of new analgesic drugs.
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Work in the Weiss laboratory is supported by the Czech Science Foundation (grant 15-13556S), the Czech Ministry of Education Youth and Sports (grant 7AMB15FR015), and the Institute of Organic Chemistry and Biochemistry (IOCB). GWZ is a Canada Research Chair and supported by the Canadian Institutes of Health Research.
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Rivas-Ramirez, P., Gadotti, V.M., Zamponi, G.W. et al. Surfen is a broad-spectrum calcium channel inhibitor with analgesic properties in mouse models of acute and chronic inflammatory pain. Pflugers Arch - Eur J Physiol 469, 1325–1334 (2017). https://doi.org/10.1007/s00424-017-2017-8
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DOI: https://doi.org/10.1007/s00424-017-2017-8