Abstract
Bradykinin, an inflammatory mediator, sensitizes nociceptor peripheral terminals reducing pain threshold. We now show that the B2 kinin receptor is expressed in rat dorsal horn neurons and that bradykinin, a B2-specific agonist, augments AMPA- and NMDA-induced, and primary afferent-evoked EPSCs, and increases the frequency and amplitude of miniature EPSCs in superficial dorsal horn neurons in vitro. Administration of bradykinin to the spinal cord in vivo produces, moreover, an NMDA-dependent hyperalgesia. We also demonstrate that nociceptive inputs result in the production of bradykinin in the spinal cord and that an intrathecal B2-selective antagonist suppresses behavioral manifestations of central sensitization, an activity-dependent increase in glutamatergic synaptic efficacy. Primary afferent-evoked central sensitization is, in addition, reduced in B2 receptor knock-out mice. We conclude that bradykinin is released in the spinal cord in response to nociceptor inputs and acts as a synaptic neuromodulator, potentiating glutamatergic synaptic transmission to produce pain hypersensitivity.
Introduction
Acute nociceptive pain is the consequence of the activation of the peripheral terminals of high-threshold primary afferent nociceptor neurons by intense mechanical, chemical, or thermal stimuli (Julius and Basbaum, 2001). If a noxious peripheral stimulus damages tissue, however, an increase in pain sensitivity follows, with a reduction in pain threshold both at the immediate site of the injury (primary hyperalgesia) and in neighboring noninjured tissue (secondary hyperalgesia) (Woolf and Salter, 2000). Postinjury pain hypersensitivity results from changes both in the peripheral nervous system and the CNS. At the site of tissue damage, injured cells and recruited inflammatory cells release multiple inflammatory mediators including cytokines, growth factors, chemokines, prostanoids, amines, purines, protons, and kinins (Mizimura and Kumazawa, 1996; Levine and Reichling, 1999). These mediators reduce the threshold of nociceptor peripheral terminals, a phenomenon known as peripheral sensitization (Mizimura and Kumazawa, 1996; Levine and Reichling, 1999). Peripheral sensitization is the consequence of posttranslational changes in transducer proteins, including the noxious heat-sensitive transient receptor potential vanilloid 1 (TRPV1) channel (Chuang et al., 2001) and TTX-resistant voltage-gated sodium channels (Gold et al., 1998). Kinin peptides, in particular bradykinin, are released from kininogen precursors at the site of tissue injury and inflammation by protease kallikreins and kininases and act on constitutively expressed B2 and injury-induced B1 G-protein-coupled receptors (GPCRs) expressed on primary sensory neuron peripheral terminals (Couture and Lindsey, 2000; Prado et al., 2002), to contribute to peripheral sensitization (Rueff and Dray, 1993; Couture et al., 2001).
Sensory inflow carried by nociceptors into the spinal cord induces an activity-dependent increase in synaptic efficacy in dorsal horn neurons, a phenomenon known as central sensitization (Woolf, 1983; Cook et al., 1987; Simone et al., 1991). Central sensitization results from alterations in the responsiveness of ionotropic NMDA and AMPA glutamate receptors, attributable both to the trafficking of intracytoplasmic receptors to the membrane and phosphorylation-mediated alterations in receptor/ion channel functional properties (Woolf and Salter, 2000) and is responsible for secondary hyperalgesia and allodynia, pain elicited in response to normally innocuous low-threshold afferent input (Torebjork et al., 1992). Multiple factors can induce central sensitization, notably glutamate acting on NMDA, mGluR (metabotropic glutamate receptor), and AMPA receptors, substance P on NK1 (neurokinin 1) receptors, BDNF on TrkB (tyrosine receptor kinase B) receptors, and PGE2 (prostaglandin E2) on EP (prostaglandin E) receptors (Ji et al., 2003; Hartmann et al., 2004). These diverse ligand-gated ion channels, GPCRs, and receptor tyrosine kinases activate intracellular signaling pathways that ultimately increase glutamatergic synaptic efficacy by altering both glutamate release and responsiveness (Ji et al., 2003).
Bradykinin, although considered essentially a peripherally acting inflammatory mediator, has several effects that support a possible role in central pain transmission; intrathecal B2 agonists induce thermal hyperalgesia and B2 antagonists reduce the second phase of the intraplantar formalin test, a model of acute inflammatory pain hypersensitivity (Chapman and Dickenson, 1992; Ferreira et al., 2002). The site, mechanism, and functional significance of these actions are not known. We have now examined whether, and how, bradykinin alters synaptic function in the spinal cord and whether this contributes to activity-dependent central sensitization.
Materials and Methods
In situ hybridization. Animals were perfused with saline followed by 4% paraformaldehyde in 0.1 m phosphate buffer, pH 7.4 (4°C), the L4–L5 spinal cord and dorsal root ganglion (DRG) were removed, postfixed for 2 h, and then placed in 20% sucrose. An 1100 bp B2 PCR fragment was subcloned into pCRII vector (Invitrogen, Carlsbad, CA), and DIG–UTP-labeled sense or antisense cRNA probes were generated using T7 RNA polymerase. Sections (10 μm) were acetylated (0.25% acetic anhydride, 10 min), prehybridized for 1 h at room temperature, incubated in hybridization buffer overnight at 55°C, washed in SSC (5, 0.2, and 0.1×), blocked with 2% goat serum, and incubated at 4°C with alkaline phosphatase (1:1000; for enzymatic reaction) or peroxidase [1:50; for tyramide signal amplification (TSA) reaction] conjugated anti-DIG antibodies (Roche Diagnostics, Indianapolis, IN). Sections were visualized using 75 μg/ml nitroblue–tetrazolium and 50 μg/ml 5-bromo-4-chlorindolyl-phosphate or the TSA biotin system (PerkinElmer, Wellesley, MA).
Immunohistochemistry and cell counting. After visualization of TSA signals, sections were incubated with monoclonal anti-neurofilament 200 (NF200) (1:500; Sigma, St. Louis, MO), anti-peripherin (1:100; Chemicon, Temecula, CA), anti-GFAP (1:1000; Chemicon), anti-NMDA receptor subunit NR1 (1:1000; Chemicon), and anti-mouse rhodamine (1:100, Chemicon). Images for NR1–B2 and GFAP–B2 double staining were acquired by confocal laser-scanning microscopy (MRC 600; Bio-Rad, Hercules, CA), and all other images were acquired by fluorescence microscope with a digital camera system (Nikon, Tokyo, Japan). For profile counting, four sections, at least 100 μm apart, were chosen. Profile area was measured for neurons with visible nuclei using the Scion (Frederick, MD) image software.
ELISA. Levels of bradykinin in the lumbar enlargement of the spinal cord were measured by ELISA. Animals were deeply anesthetized with isoflurane, and bilateral intraplantar capsaicin (20 μg, 20 μl; Sigma) was administrated 20 min before decapitation. The lumbar vertebral column was removed, and the spinal cord was extruded by injecting cold lactated Ringer's solution through a 16 gauge needle into the lumbar spinal canal. The lumbar enlargement was collected and immediately frozen on dry ice. The total procedure took <1 min. The tissue was weighed, homogenized in 500 μl of PBS containing a protease inhibitor mixture (Sigma), and then centrifuged for 30 min at 4°C and 10,000 rpm. The supernatant was then collected and assayed for levels of bradykinin using a competitive ELISA kit (Bachem, Bubendorf, Switzerland). Duplicates of both samples and standards were used.
Spinal cord slice preparation and whole-cell patch-clamp recording. Transverse lumbar spinal cord slices (∼600 μm) with an attached dorsal root from adult (5–8 weeks) Sprague Dawley rats (Charles River Laboratories, Wilmington, MA) were prepared with a vibrating microslicer (DTK 1500; Dosaka, Kyoto, Japan) and perfused in oxygen-bubbled Krebs' solution (in mm: 117 NaCl, 3.6 KCl, 2.5 CaCl2, 1.2 MgCl2, 1.2 NaH2PO4, 25 NaHCO3, and 11.5 d-glucose) at 35°C for blind whole-cell patch-clamp recordings. Resistance of patch pipettes were typically 4∼10 MΩ. The pipette solution contained the following (in mm): 135 K-gluconate, 0.5 CaCl2, 2 MgCl2, 5 KCl, 5 EGTA, 5 HEPES, 5 d-glucose, and 5 QX-314 (lidocaine N-ethyl bromide). Currents were filtered at 2 kHz and digitized at 5 kHz using the Axopatch 200A (Molecular Devices, Union City, CA) and analyzed by pCLAMP8.1 (Molecular Devices). Holding potential was –70 mV for AMPA and –40 mV for NMDA currents. TTX (0.5 μm) was presented in the bath solution, except for recording evoked EPSCs (eEPSCs). Dorsal root stimulation, sufficient to recruit Aδ and C-fiber, was delivered with a suction electrode (Kohno et al., 2003) linked to a constant-current stimulator (Digitimer, Welwyn Garden City, UK). Monosynaptic evoked EPSCs were studied in the presence of 20 μm bicuculline, 2 μm strychnine, and 50 μm APV. Miniature EPSC (mEPSC) frequency and amplitude were analyzed with Axograph (Molecular Devices). All drugs were purchased from Sigma.
Behavior. PE-10 catheters were placed in the lumbar subarachnoid space while animals were under isoflurane anesthesia. Either Icatibant (HOE 140) (10/100 μg; 10 μl) or vehicle was administrated intrathecally 20 min before intraplantar injections. Formalin (1.5%; 50 μl) was injected in the left hindpaw and time spent paw lifting and licking was counted in 5 min blocks for 60 min. Capsaicin (20 μg; 20 μl) was injected in the rat left heel, and mechanical sensitivity was assessed with von Frey filaments applied to the plantar surface distal to the injection site. For the hotplate test, (+)-5-methyl-10,11-dihydro-5H-dibenzo[a,d]-cyclohepten-5,10-imine maleate (MK-801) (0.1 mg/kg) was injected intraperitoneally 15 min before bradykinin (2 μg; 10 μl) intrathecal administration. Rat paw withdrawal latency was measured at 52°C. B2 receptor knock-out mice were obtained from The Jackson Laboratory (Bar Harbor, ME), and capsaicin (2.5 μg; 10 μl) was injected into the heel on one side. Mechanical sensitivity was compared before and 25 min after capsaicin injection. The observer was always blind to the treatment.
Data analysis. Data are expressed as mean ± SEM. Peak AMPA and NMDA currents were measured before and after each treatment and expressed as follows: (posttreatment/pretreatment –1) × 100%. Student's t test, one-way ANOVA, two-way ANOVA repeated measurement followed by post hoc test [SigmaStat (Systat Software, Point Richmond, CA) and SAS (SAS Institute, Cary, NC)], and Kolmogorov–Smirnov test were used where appropriate.
Results
B2 receptor mRNA is expressed in dorsal root ganglion and dorsal horn neurons
Although B2 receptor protein expression is reported in DRG (Steranka et al., 1988) and dorsal horn neurons (Lopes et al., 1995), we found that the staining in these two tissues produced by three different anti-B2 antibodies was identical in wild-type and B2 knock-out mice (data not shown). We therefore used in situ hybridization for B2 mRNA to identify the distribution and cellular localization of this receptor in adult rats. In the DRG, B2 was expressed by both small and medium-sized sensory neurons (Fig. 1A) with a size-frequency distribution of 200–1200 μm2 (Fig. 1B). Forty-five percent of small-diameter peripherin-positive DRG neurons with unmyelinated axons were B2 mRNA positive, with a smaller proportion (25%) of NF200-expressing DRG neurons with myelinated axons expressing the receptor transcript (Fig. 1C,D). In the superficial dorsal horn, ∼70% of NMDA (NR1) receptor subtype immunostained neurons also expressed B2 mRNA, whereas no GFAP-positive glial cells did (Fig. 2B,C). B2 is expressed then by primary sensory and second-order dorsal horn neurons, providing an opportunity in the dorsal horn for a presynaptic and postsynaptic action of bradykinin, its endogenous ligand.
Intraplantar capsaicin induces bradykinin production in spinal cord
To test whether bradykinin is produced in the dorsal horn in response to nociceptor input, we measured bradykinin levels in the spinal cord after activation of TRPV1 receptors by intraplantar injection of capsaicin. Capsaicin was injected (20 μg; 20 μl) in each hindpaw of deeply anesthetized rats. This produces a short-lasting nociceptor afferent input into the spinal cord. The lumbar enlargement of the spinal cord was rapidly removed 20 min after the capsaicin injection, and bradykinin levels were measured by ELISA. In the naive spinal cord, bradykinin levels were below the ELISA detection threshold (0.03 ng/ml), and this was also true for the majority of animals after intraplantar vehicle injection (0.07 ± 0.07 pg of bradykinin per milligram of tissue; n = 7). Bradykinin was detectable in the spinal cord, however, after capsaicin injection (0.37 ± 0.07 pg of bradykinin per milligram of tissue; n = 7) (Fig. 2D). These levels are likely an underestimate, because bradykinin is broken down very rapidly (Cyr et al., 2001). Because B2 is expressed in both presynaptic and postsynaptic elements in the dorsal horn and bradykinin, a B2-selective agonist, is induced after noxious stimulation, we next investigated whether activation of B2 by bradykinin modulates synaptic activity in the dorsal horn.
Bradykinin enhances excitatory synaptic transmission in dorsal horn
Bath administration of AMPA (10 μm for 30sat –70 mV) or NMDA (50 μm at –40 mV) induced inward currents (30–200 pA) in lamina II neurons recorded by whole-cell patch clamp in isolated adult rat spinal cord slices. Both of these currents were potentiated (∼40%), in ∼80% of the neurons tested, by preapplication for 3 min of bradykinin (10 μm) with full recovery by 10 min (Fig. 3A,B,D,F). The enhancement by bradykinin was dose dependent (n = 9) (Fig. 3D). Pretreatment with the B1-selective agonist des-Arg9-bradykinin (10 μm) did not modify either AMPA or NMDA currents (Fig. 3C,D). To confirm that the observed effect of bradykinin was mediated directly by B2 expressed on the recorded neuron, GDP-β-S, a G-protein inhibitor, was added to the pipette solution. Intrapipette GDP-β-S (2 mm) blocked the potentiation by bradykinin of both AMPA (n = 5) and NMDA (n = 7) currents (Fig. 3E,F). To test whether bradykinin potentiates primary afferent-evoked synaptic currents, we next examined its effects on monosynaptic AMPA receptor-mediated EP-SCs (eEPSCs) evoked by stimulating Aδ- and C-fibers in the attached dorsal root. Both Aδ-fiber (n = 6) (Fig. 4A–C) and C-fiber (n = 7) (Fig. 4A,C) eEPSCs in superficial dorsal horn neurons were reversibly enhanced by bath application of bradykinin (Fig. 4B).
To determine whether the B2-mediated augmentation of glutamatergic transmission occurs presynaptically and/or postsynaptically, the effect of bradykinin on the frequency and amplitude of AMPA-mediated mEPSCs was measured at a –70 mV holding potential. The frequency (Fig. 5A–C) and amplitude (Fig. 5A–C) of mEPSCs increased (215 ± 39 and 53 ± 9%, respectively; n = 10; p < 0.001; paired t test) after bath administration of bradykinin with a leftward shift of the interevent interval plot and a rightward shift of the cumulative amplitude plot (Fig. 5B) (p < 0.01; Kolmogorov–Smirnov test). Des-Arg9-bradykinin had no detectable effect (Fig. 5A, right). To selectively target the postsynaptic neuron and leave GPCRs on presynaptic terminals intact, we delivered GDP-β-S through the recording pipette. GDP-β-S (2 mm; n = 6) in the pipette eliminated the potentiation of the amplitude (Fig. 5D, right) (p < 0.01) but not the frequency of mEPSCs by bradykinin (Fig. 5D, left) (p = 0.45). We conclude that bradykinin acts via B2 presynaptically to increase glutamate release and postsynaptically to increase the sensitivity of glutamate ionotropic receptors. This raises the question of whether this occurs in vivo and, if so, what is its functional significance?
Intrathecal bradykinin causes an NMDA-dependent hyperalgesia
Intrathecal bradykinin injection (10 and 2 μg, respectively) produced mechanical (von Frey threshold, 60 min after treatment, 9 ± 2.8 g vs control, 15.3 ± 3 g; n = 7; p < 0.05) and thermal hyperalgesia (hot plate, 52°C, n = 12), with a decrease in thermal response latency that peaks at 75 min and slowly recovers over 4 h (Fig. 6A) (n = 5; p < 0.01 vs vehicle). To test whether the bradykinin-induced pain hypersensitivity involves the NMDA receptor, rats were pretreated with the NMDA receptor antagonist MK-801 (0.1 mg/kg, i.p.) immediately before the intrathecal bradykinin injection. MK-801 pretreatment abolished the bradykinin-induced thermal hyperalgesia (Fig. 6A) (n = 6; p < 0.01 vs bradykinin only). This dose of MK-801 produced no effect on basal thermal sensitivity when given without bradykinin (Fig. 6A) (n = 6; p > 0.05). Bradykinin then acts in vitro to potentiate NMDA receptor action and in vivo to produce an NMDA receptor-dependent pain hypersensitivity.
AB2 antagonist blocks central sensitization
Intraplantar injection of formalin (1.5%; 50 μl) induces two behavioral responses in rodents: an immediate foot lifting and paw licking that lasts ∼5 min and is attributable to the direct irritant action of formalin on nociceptors (phase 1) and a second phase that peaks at ∼40 min and reflects the action of low-level ongoing nociceptor input on a spinal cord sensitized by the earlier input (phase 2) (Fig. 6B) (Coderre and Melzack, 1992; Puig and Sorkin, 1995). The second, but not the first, phase of the formalin response is sensitive to spinal administration of NMDA receptor antagonists (Coderre and Melzack, 1992) and a conditional knock-out of the NR1 NMDA receptor subunit in the dorsal horn (South et al., 2003) and is, therefore, a behavioral model of NMDA-dependent central sensitization. Intrathecal administration of HOE 140, a B2-selective antagonist, eliminated the second phase of the formalin test, leaving the first unaffected (Fig. 6B) (100 μg; n = 5; p < 0.01), implying that this kinin receptor contributes significantly to the expression of activity-dependent central sensitization.
The most characteristic feature of central sensitization is pain sensitivity to low-intensity mechanical stimuli outside the area of injury (secondary tactile allodynia) (Woolf and Salter, 2000). This can be modeled behaviorally by a subcutaneous injection of capsaicin that directly activates TRPV1-expressing nociceptors, leading to activity-dependent central sensitization and mechanical allodynia beyond the area of injection (Gilchrist et al., 1996). The mechanical hypersensitivity that manifested in the distal plantar foot after injection of capsaicin (20 μg) into the proximal heel was significantly suppressed by intrathecal HOE 140 (100 μg; n = 8; p < 0.05) (Fig. 6C), a dose that did not itself alter basal mechanosensitivity (Fig. 6C). Capsaicin-evoked nociceptor input induces bradykinin release in the spinal cord and B2-dependent central sensitization.
Capsaicin-induced tactile allodynia is reduced in B2 receptor knock-out mice
To complement the pharmacological demonstration of a B2-dependent component to capsaicin-induced central sensitization, we tested whether a B2 receptor knock-out (Rupniak et al., 1997) has a similar effect. To address this, we first investigated the immediate pain response (the first 5 min) evoked by subcutaneous injection of capsaicin (2.5 μg; 10 μl). B2 receptor knock-out (n = 9) and wild-type (n = 6) mice showed no difference in this nociceptor-activated behavior (Fig. 6D, inset) (p = 0.4). This suggests that capsaicin produces a comparable level of nociceptive inputs in both the B2 receptor knock-out and wild-type mice. Basal mechanical sensitivity was also similar in both mice (Fig. 6D) (p = 1). However, the mechanical allodynia normally present 25 min after intraplantar capsaicin injection was significantly less in B2 receptor knock-out mice (Fig. 6D) (p < 0.05), indicating that these mice develop less central sensitization than wild types.
Discussion
B2 receptor activation with bradykinin augments primary afferent-evoked glutamatergic synaptic currents, the frequency and amplitude of spontaneous mEPSCs, and the currents evoked directly by AMPA and NMDA in lamina II spinal cord neurons. We conclude that bradykinin is a modulator of glutamatergic synaptic transmission in the spinal cord with presynaptic and postsynaptic actions, which is compatible with the cellular localization of B2 receptor mRNA in small-caliber DRGs and in NR1-expressing superficial dorsal horn neurons. We did not find any B2 receptor expression in glial cells, and the blockade by GDP-β-S of the potentiating actions of bradykinin on glutamatergic ionotropic receptors indicates a direct postsynaptic neuronal action. The more robust potentiating effect of bradykinin that we found on mEPSCs than on bath-applied AMPA/NMDA and eEPSCs may reflect a “ceiling effect” in the latter two situations in which the scope for an increase in currents is likely to be limited by the greater amount of agonist available for the binding to the receptors. In addition, the finding that the vesicle pools available for mEPSCs are distinct from those of eEPSCs (Sara et al., 2005) may contribute to the disparity.
The bradykinin precursor kininogen is expressed in spinal cord neurons, glia, and endothelial cells (Li et al., 1999). After administration of the kallikrein activator melittin, bradykinin-like immunoreactivity becomes prominent in the dorsal horn (Lopes and Couture, 1997). We find that nociceptor afferent input increases bradykinin levels in the spinal cord from undetectable levels in the naive state. The activity-dependent increase in bradykinin in the spinal cord represents a source of endogenous ligand for B2 receptors enabling them to modulate glutamatergic transmission in the dorsal horn. How and where nociceptor afferent inputs activate kallikrein, to convert kininogen to bradykinin, now need to be established. Is bradykinin produced in presynaptic terminals and released as a synaptic neuromodulator, is it produced in postsynaptic neurons, and does it act as an autocrine or retrograde signal, or is it produced by non-neuronal cells?
The reduction in the behavioral manifestations of activity-dependent central sensitization in the spinal cord, which we find both on antagonizing the B2 receptor and in B2 null mutants, reinforces the conclusion that this kinin is a centrally acting synaptic modulator that has a particular role in producing acute injury-induced pain hypersensitivity. Angiotensin-converting enzyme inhibitors, which are widely used to treat hypertension and cardiac failure, prevent the degradation of bradykinin because angiotensin-converting enzyme (ACE) acts on bradykinin as well as angiotensin I. This is responsible for the most prominent side effect of this class of drugs: coughing. Interestingly, another spontaneously reported side effect is pain involving any part of the body, including the chest, abdomen, limbs, joints, back, shoulder, and head (http://www.whvc.org/Treatment/AceInhibitors.htm). No study has, however, specifically examined whether a reduction in pain threshold occurs in these patients; however, interestingly, the level of pain in human volunteers in response to sustained isometric contraction after administration of ACE inhibitors positively correlates with the concentration of bradykinin in the tested muscle (Boix et al., 2005).
What downstream signaling mechanism underlies the B2 receptor-mediated potentiating effects on NMDA and AMPA currents in the spinal cord? The B2 receptor couples to phospholipase Cβ, which increases intracellular calcium and activates protein kinase C. The B2 receptor also couples to phospholipase A2, which converts membrane lipids to arachidonic acid that can be converted into E prostanoids. Additional study is required to establish the nature of the link between B2 and ionotropic glutamatergic receptors and whether it involves recruitment of the NMDA and AMPA receptors to the membrane (Carroll and Zukin, 2002) or phosphorylation-dependent changes in channel kinetics (Yu et al., 1997; Esteban et al., 2003). The major form of therapy targeted at acute central sensitization clinically has been NMDA receptor antagonists. These antagonists are certainly effective in reducing central sensitization-mediated pain in laboratory animals (Woolf and Thompson, 1991), but their use in patients is severely limited by their psychotomimetic side effects (Stubhaug et al., 1997). A better target, based on our present findings, may well be bradykinin, because we show that it is an initiator of both NMDA and AMPA use-dependent synaptic potentiation. Several other sensitizing agents, including substance P and BDNF, also play a role in central sensitization. They may act in either series with the production or action of bradykinin on B2 receptors or may share common intracellular signaling pathways, providing opportunity for cross talk and synergistic interactions. The relationships and relative contributions of the different sensitizing agents will need to be worked out, but bradykinin is likely to play a prominent role.
The dual actions of bradykinin, producing peripheral sensitization in the peripheral nervous system and central sensitization in the CNS, imply that preventing its production (using kallikrein inhibitors) or action (with B2 receptor antagonists) will provide a particularly useful means of controlling acute inflammatory pain hypersensitivity.
Footnotes
This work was supported by National Institutes of Health Grant NS039518 (C.J.W.). We thank Drs. Z. Y. Zhuang, D. Broom, C.-R. Lin, T. Samad, D.-H. Youn, and R. Griffin for technical assistance and advice.
Correspondence should be addressed to Dr. Clifford J. Woolf, Neural Plasticity Research Group, Department of Anesthesia and Critical Care, Massachusetts General Hospital and Harvard Medical School, Charlestown, MA 02129. E-mail: cwoolf{at}partners.org.
T. Kohno's present address: Division of Anesthesiology, Niigata University Graduate School of Medical and Dental Sciences, Niigata 951-8510, Japan.
DOI:10.1523/JNEUROSCI.2393-05.2005
Copyright © 2005 Society for Neuroscience 0270-6474/05/257986-07$15.00/0
↵* H.W. and T.K. contributed equally to this work.