Synergistic Enhancement of Glutamate-Mediated Responses by Serotonin and Forskolin in Adult Mouse Spinal Dorsal Horn Neurons

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Synergistic Enhancement of Glutamate-Mediated Responses by Serotonin and Forskolin in Adult Mouse Spinal Dorsal Horn Neurons

Guo-Du Wang and Min Zhuo

Washington University Pain Center, Departments of Anesthesiology, Anatomy and Neurobiology, and Psychiatry, Washington University, St. Louis, Missouri 63110

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Wang, Guo-Du and Min Zhuo. Synergistic Enhancement of Glutamate-Mediated Responses by Serotonin and Forskolin in Adult Mouse Spinal Dorsal Horn Neurons. J. Neurophysiol. 87: 732-739, 2002. Glutamate is the major excitatory amino acid neurotransmitter in the CNS, including the neocortex, hippocampus, and spinalcord. Normal synaptic transmission is mainly mediated by glutamateAMPA and/or kainate receptors. Glutamate N-methyl-D-aspartate(NMDA) receptors are normally inactive and only activated whena sufficient postsynaptic depolarization is induced by the activity.Here we show that in sensory synapses of adult mouse, some synapticresponses (26.3% of a total of 38 experiments) between primaryafferent fibers and dorsal horn neurons are almost completelymediated by NMDA receptors. Dorsal root stimulation did not elicitany detectable AMPA/kainate receptor-mediated responses in thesesynapses. Unlike young spinal cord, serotonin alone did not produceany long-lasting synaptic enhancement in adult spinal dorsal hornneurons. However, co-application of the adenylyl cyclase activatorforskolin and serotonin (5-HT) produced long-lasting enhancement,including the recruitment of functional AMPA receptor-mediatedresponses. Calcium-sensitive, calmodulin-regulated adenylyl cyclases(AC1, AC8) are required for the enhancement. Furthermore the thresholdsfor generating action potential responses were decreased, and,in many cases, co-application of forskolin and 5-HT led to thegeneration of action potentials by previously subthreshold stimulationof primary afferent fibers in the presence of the NMDA receptorblocker 2-amino-5-phosphonovaleric acid. Our results suggest thatpure NMDA synapses exist on sensory neurons in adult spinal cordand that they may contribute to functional sensory transmission.The synergistic recruitment of functional AMPA responses by 5-HTand forskolin provides a new cellular mechanism for glutamatergicsynapses in mammalian spinalcord.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Glutamate is the major excitatory amino acid transmitter in the CNS (Bliss and Collingridge 1993; Hollmann and Heinemann 1994;Seeburg 1993). Glutamate mediates synaptic transmission by bindingto postsynaptic $alpha$ -amino-3-hydroxy-5-methyl-isoxozole propionicacid (AMPA), N-methyl-D-aspartate (NMDA), and kainate receptors.In most cases, synaptic responses are primarily mediated throughpostsynaptic AMPA and kainate receptors as NMDA receptors areblocked by magnesium at resting membrane potential. However, thereare reports that NMDA receptors contribute to synaptic transmissionand modulation in brain slice preparations including the cortex,hippocampal, olfactory bulb, and spinal cord (Bardoni et al. 2000;Gil and Amitai 1996; Sah et al. 1989; Schiller et al. 2000; Schoppaet al. 1998; Yoshimura and Jessell 1990). For example, in spinalslices of young rats, it has been recently shown that high-intensityroot stimulation evoked D-APV-sensitive slow synaptic activityin lamina II neurons that drove action potential firing (Bardoniet al. 2000). In thalamocortical slices, both NMDA and non-NMDAreceptors contribute to excitatory synaptic transmission (Giland Amitai 1996).

Recent studies indicate that glutamatergic synapses are not functionally homogenous; at some synapses, only functional NMDAreceptors are available to respond to glutamate released frompresynaptic terminals during a synaptic event (Baba et al. 2000;Bardoni et al. 1998; Durand et al. 1996; Gomperts et al. 1998;Isaac et al. 1995, 1997; Li and Zhuo 1998; Liao et al. 1995; Rumpelet al. 1998; Wu et al. 1996; see Malenka and Nicoll 1997; Malinowet al. 2000 for reviews). Assuming that dendritic resting membranepotentials are in the same range as those that can typically beobserved at the soma, one would predict that in the absence ofany prior postsynaptic depolarization, pure NMDA synapses wouldnot respond to glutamate release, and thus appear functionally"silent." What makes pure NMDA synapses important is their involvementin central synaptic plasticity. These synapses can be convertedinto AMPA and NMDA mixed synapses, at least functionally (Durandet al. 1996; Hayashi et al. 2000; Isaac et al. 1995; Li and Zhuo1998; Liao et al. 1995, 1999). In the hippocampus and somatosensorycortex, long-term potentiation may involve the unsilencing ofsynapses (Durand et al. 1996; Issac et al. 1997; Liao et al. 1995).

Sensory transmission in the spinal cord dorsal horn receives biphasic descending modulation from supraspinal structures includingthe rostroventral medulla (RVM) (Fields et al. 1991; Zhuo andGebhart 1992, 1997). Serotonin-containing neurons in the RVM senddescending projecting terminals to the spinal cord, and serotoninreleased from descending projecting fibers regulates spinal sensorytransmission in a dose-related, biphasic manner (Li and Zhuo 1998).In the young rat spinal cord, serotonin at a low dose or a selective5-HT₂ receptor agonist induced long-lasting synaptic enhancement,and activation of silent synapses at least in part contributesto the enhancement (Li and Zhuo 1998; Li et al. 1999). No similarstudy has been carried out in adult spinalslices.

Several studies clearly indicate that pure NMDA synapses may be involved in development-related synaptic plasticity (Isaacet al. 1997; Liao et al. 1999; Petralia et al. 1999). What aboutthe role of pure NMDA synapses in adult animal physiology? Lessinformation is available related to this question. We wanted todetermine if pure NMDA synapses contribute to sensory plasticityin adult neurons. Considering potential advantages of geneticallymanipulated mice, we selected adult mice (greater than 8 wk) inthis study. We demonstrate here that there are pure NMDA receptor-mediatedresponses in these sensory synapses and reveal a signaling synergisticpathway for recruiting functional AMPA receptor-mediatedresponses.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Slice preparation

Adult male 8-14 wk-old mice (C57/6J; Jackson Laboratory) were used. AC1, AC8 and AC1, and AC8 double knockout and littermatewild-type mice were generously provided by Dr. Louis Muglia. Micewere anesthetized with urethan. Transverse lumbar spinal cordslices, 450-500 µm with 7-12 mm of attached dorsal root, wereobtained from male adult mice. Slices were kept in a plastic chambercontaining oxygenated saline [which was composed of (in mM) 124NaCl, 4 KCl, 26 NaHCO₃, 2 NaH₂PO₃, 2 CaCl₂, 1 MgSO₄, and 10 D-glucose]at 32°C for at least 2-3 h. Experimental protocols were approvedby the Animal Studies Committee at WashingtonUniversity.

Intracellular recordings

Intracellular recordings of synaptic responses were performed from neurons located in the dorsal horn Lamina I and II witha 3 M potassium chloride-filled glass microelectrode (DC impedance,75-200 M $Omega$ ). The synaptic responses were activated by electricalstimulation of dorsal roots with a bipolar electrode or a suctionelectrode. We did not find any obvious difference in responsesto stimulation using a bipolar electrode or a suction electrode.Postsynaptic excitatory postsynaptic potentials (EPSPs) were evokedat 0.01-0.02 Hz. Monosynaptic EPSPs were identified using twocriteria: the response latency did not change with increasingintensities of electrical stimulation and repetitive stimulationdid not change response latency. EPSPs of the neurons were evokedwith electrical stimulation at different intensities (0.2 ms,1-30 V) and recorded through a high-input impedance bridge circuitof amplifier (Intracellular Electrometer IE-210, Warner Instrument,or Axonclamp 2B, Axon Instruments) and stored in PClamp (AxonInstruments) files. The perfusion medium [containing (in mM) 124NaCl, 4 KCl, 26 NaHCO₃, 1 NaH₂PO₄, 1 MgSO₄, 2 CaCl₂, and 10 glucose]was oxygenated with 95% O₂-5% CO₂. The temperature and perfusionrate of recording were kept at 34°C and 2-5 ml/min, respectively.All drugs were purchased from RBI-Sigma. In all experiments, bicucullinemethiodide (10 µM) and strychnine hydrochloride (1 µM) were addedto the perfusion solution to block inhibitorytransmission.

Data and statistical analysis

Data are presented as means ± SE. Statistical comparisons were made with the use of one-way ANOVAs (Dunnett test for posthoc comparison) or Student's t-test. P < 0.05 was consideredsignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Pure NMDA receptor-mediated sensory responses

To examine if pure NMDA receptor synapses may exist in adult sensory synapses between primary afferent fibers and dorsal hornneurons, we recorded EPSPs from neurons in the superficial dorsalhorn of the spinal cord, which receive afferent inputs from peripheralsensory neurons. EPSPs were induced by electrical stimulationdelivered to the dorsal root, and the selective NMDA receptorantagonist inhibitor 2-amino-5-phosphonovaleric acid (AP5, 50or 100 µM) was used to identify the NMDA receptor-mediated componentof an EPSP. In a total of 38 dorsal horn neurons tested, 10 ofthem were completely blocked by bath application of AP5 (26.3%of the total population; Fig. 1A). The blockade was reversible,as the EPSP recovered after washout of AP5. The resting membranepotentials were not significantly affected throughout the experiments.The mean stimulation intensity (0.2-ms duration) was 19.0 ± 2.1V (n = 10, ranged from 10.0 to 30.0 V). In the other 28 neurons,AP5 only partially blocked the synaptic responses, and subsequentco-application of CNQX and AP5 completely blocked the response(Fig. 1, B and D). Dorsal horn neurons containing only NMDA receptor-mediatedEPSPs had the similar resting membrane potential (mean $-$ 74.7 ±2.1 mV, n = 10) as neurons exhibiting mixed AMPA/NMDA responses( $-$ 71.0 ± 2.0 mV, n = 28), indicating that pure NMDA receptor-mediatedEPSPs did not require depolarization at the soma.

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Fig. 1. Pure N-methyl-D-aspartate (NMDA) receptor and mixed NMDA/AMPA receptor-mediated sensory synaptic transmission in adult neurons. A: examples of pure NMDA receptor-mediated excitatory postsynaptic potentials (EPSPs) showing synaptic responses before, during, and after treatment with 50 µM 2-amino-5-phosphonovaleric acid (AP5). EPSPs recovered during the washout of AP5. Resting membrane potentials (V_m) of neurons are given at top. B: examples of mixed NMDA/AMPA receptor-mediated EPSPs showing synaptic responses before and during perfusion of 50 µM AP5 or 50 µM AP5 plus 20 µM 6-cyano-7-nitroquinoxalene-2,3-dione (CNQX). Data shown in A and B were collected from 2 different neurons. C: the effect of AP5 on the EPSP slopes in the experiment shown in A. D: the effects of AP5 and CNQX on the EPSP slopes in the experiment shown in B.

We also tested if pure NMDA receptor-mediated EPSPs may be affected by changing extracellular Mg²⁺ concentrations. After obtaining pure NMDA EPSPs in normal Mg²⁺ (1 mM), we then perfused the slices with the solution with lessMg²⁺ (0.2 mM). In a total of eight neurons tested, no significantdifference in the slopes of NMDA receptor-mediated EPSPs werefound (the ratio of EPSP slopes at 1 vs. 0.2 mM Mg²⁺: 0.9 ± 0.1, n = 8), indicating that these NMDA receptors areless sensitive to the Mg²⁺ blockade than the normal NMDAreceptors.

Pure NMDA receptor-triggered action potentials

Can pure NMDA receptor-mediated EPSPs generate action potentials in adult dorsal horn neurons in response to stimulation ofthe dorsal root? Bardoni et al. (2000) reported that in youngrat dorsal horn neurons, repetitive stimulation could generateaction potentials in neurons with pure NMDA synapses. We thuswanted to see if action potentials can be induced at pure NMDAsynapses in adult dorsal horn neurons. As shown in Fig. 2, adultdorsal horn neurons containing pure NMDA receptor-mediated synapsesgenerated spike responses in respond to stimulation of the dorsalroot. Bath application of the NMDA receptor antagonist AP5 completelyblocked the EPSP and action potentials. These results indicatethat at adult sensory synapses (between primary afferent fibersand dorsal horn neurons), pure NMDA receptor-mediated EPSPs canmediate sensory transmission. The results also provide directevidence that pure NMDA receptor synapses can drive action potentialsin adult dorsal horn neurons.

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Fig. 2. Pure NMDA receptor-driven action potentials by stimulation of primary afferent fibers. Stimulation of primary afferent fibers at synapses containing pure NMDA EPSPs elicited action potentials and the blockade after the perfusion of 50 µM AP5.

Serotonin predominantly inhibited sensory synaptic responses in adult spinal cord slices

5-HT is a key transmitter of descending pain modulatory systems (Fields et al. 1991; Willis 1982). 5-HT biphasically regulatesspinal sensory synaptic transmission in young spinal cord slices,causing facilitation of responses at lower doses and inhibitionat higher doses by acting on different 5-HT receptor subtypes(Hori et al. 1996; Li and Zhuo 1998; Li et al. 1999). To exploreif similar modulatory effects can be observed in adult spinalcord slices, we applied 5-HT through the bath solution duringrecordings of EPSPs in which AMPA and NMDA components were notdistinguished. In contrast to spinal slices from young animals,all doses of 5-HT used (5, 10, and 100 µM; n = 5-8) produced predominantlyinhibitory effects on EPSPs (Fig. 3) in 18 of 20 experiments.In the other two experiments, 5-HT produced slight increases inthe EPSPs (5 µM 5-HT, 114% of control; 10 µM 5-HT, 136% of control),and the EPSPs returned to the baseline after the washout of 5-HT.Resting membrane potentials were not significantly affected inthese neurons by 5-HT application.

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Fig. 3. Serotonin produced predominantly inhibitory modulation in adult neurons. A: examples of EPSPs showing synaptic responses before, during, and after perfusion of 5 µM serotonin (5-HT). B: examples of EPSPs showing synaptic responses before, during, and after treatment with 100 µM 5-HT. Data shown in A and B were collected from 2 different neurons. C: summarized data of the effects of 5-HT are plotted at 3 different doses (5, 10, and 100 µM;

). For comparison, previously published results of biphasic modulation by 5-HT (5, 50, and 100 µM) (Li and Zhuo 1998

) in young sensory synapses are also plotted (···).

Synergistic effects between 5-HT and forskolin

Adult in vivo electrophysiological, pharmacological, and behavioral studies have consistently demonstrated that the spinalserotonergic system mediates descending facilitation as well asinhibition from the raphe nuclei and adjacent nuclei (Zhuo andGebhart 1992, 1997). Intrathecal administration of 5-HT or 5-HTreceptor subtype-selective agonists facilitates spinal nociceptivereflexes in adult awake animals (see Millan 1999 for a review).What could be the cellular mechanism explaining the differencebetween in vivo physiological findings and our in vitro spinalcord slice electrophysiology? We hypothesized that the facilitatoryeffect of 5-HT in adult animals may depend on the cAMP signalpathway. Evidence from several different studies suggests cAMPmay serve as a bifunctional signal transduction molecule in centralglutamatergic synapses and contribute to synaptic potentiationand depression (Blitzer et al. 1995; Brandon et al. 1995; Leeet al. 2000; Lisman 1989; Qi et al. 1996). In the spinal dorsalhorn, sensory transmitters such as glutamate and neuropeptidescan increase postsynaptic calcium and may raise the cAMP levelthrough calcium-sensitive adenylyl cyclases (Gu et al. 1996; Parsonsand Seybold 1997).

To test this hypothesis, we examined the effect of an activator of adenylyl cyclase, forskolin (10 µM), on sensory synaptictransmission. Unlike at hippocampal synapses (Chavez-Noreiegaand Stevens 1992; Weisskorf et al. 1994), 10 µM forskolin didnot significantly affect synaptic responses (n = 6, 96.2 ± 6.5%of control; Fig. 4B). Co-application of 5 µM 5-HT with 10 µM forskolinproduced significant enhancement of EPSPs (mean 263.8 ± 40.1%of control; P < 0.05, n = 6; Fig. 4A). The duration of EPSPs werealso increased after the application. This enhancement sustainedafter washout. Resting membrane potentials were not significantlyaffected by 5 µM 5-HT and forskolin co-application in the sameneurons ( $-$ 74.5 ± 1.8 mV before and $-$ 75.8 ± 2.2 mV after). Thesynergistic effect of 5-HT and forskolin depended on the doseof 5-HT. Co-application of 10 µM forskolin with 100 µM 5-HT producedsignificant inhibition of synaptic responses (25.5 ± 9.5% of control;n = 4) and synaptic responses recovered during washout.

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Fig. 4. Forskolin and serotonin synergistically facilitate sensory synaptic transmission. A: examples of EPSPs showing synaptic responses before, during, and after co-application of 5 µM 5-HT and 10 µM forskolin. Note that stimulation of primary afferent fibers at the same intensity induced action potentials from the same neuron during the washout. B: forskolin (10 µM) alone did not produce any facilitation in a separate experiment. C: summarized results for different treatments with forskolin and/or 5-HT. Data are shown as percentages in EPSP slopes during the drug application. While forskolin (10 µM) alone did not induce significant changes in synaptic responses, co-application of 5-HT (5 µM) and forskolin (10 µM) induced long-lasting enhancement of synaptic responses. However, co-application of 5-HT at a high dose (100 µM) with forskolin (10 µM) produced inhibition of synaptic responses during the drug application. Synaptic responses recovered after 10 min washout with normal solution. *P < 0.05 indicates significant difference from control.

Two major forms of calcium-calmodulin-sensitive adenylyl cyclases type 1 and 8 (AC1 and AC8) are found in the CNS (Xia andStorm 1997). To examine if the effects of forskolin depends onactivation of AC8 or AC1, we performed experiments in wild-typemice and mutant mice lacking AC1, AC8, and AC1 and AC8. Consistently,co-application of 5-HT (5 µM) and forskolin (10 µM) produced significantenhancement of synaptic responses in wild-type mice (n = 6, 221.1± 59.9% of control, P < 0.05). However, the enhancement of 5-HTand forskolin was absent in mice lacking AC1 (n = 9, 92.5 ± 7.7%of control) and AC8 (n = 7; 88.2 ± 8.0% of control) or mice lackingboth AC1 and AC8 (n = 2, 100.2 and 95.4% of control, respectively;Fig. 5). These findings indicate that forskolin acts through AC1and AC8.

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Fig. 5. Adenylyl cyclases type 1 and 8 (AC1 and AC8) are required for the enhancement induced by 5-HT and forskolin. A: examples of EPSPs showing synaptic responses before and during co-application of 5 µM 5-HT and 10 µM forskolin in slices of AC1 and AC8 knockout mice. Co-application of 5-HT and forskolin did not produce any significant increase in synaptic responses in slices of AC1 or AC8 knockout mice. B: summary data of 5-HT and forskolin in wild-type, AC1, AC8, and AC1 and AC8 knockout mice. *P < 0.05 indicates significant difference from wild type.

Due to enhanced EPSP amplitudes after the application of 5-HT and forskolin, dorsal horn neurons showed enhanced spike responsesto the dorsal root stimulation. In three of six experiments, followingtreatment with 5-HT plus forskolin, dorsal horn neurons demonstratedspike responses to stimulation at an intensity that did not induceany spike response before drug application (Fig. 4A). Spike responsesto stimulation of primary afferent fibers had a late onset andoften appeared during washout. In the other three cells, synapticresponses were enhanced without any spikeresponse.

Recruitment of AMPA/kainate receptor-mediated responses at pure NMDA synapses

We tested if the synergistic interaction between 5-HT and forskolin recruits AMPA receptors to pure NMDA synapses. We pickedrecordings where 100 µM AP5 blocked EPSPs completely (Fig. 6A).We then perfused both 5-HT (5 µM) and forskolin (10 µM) in thecontinuous presence of AP5. Interestingly, in all three experiments,co-application of 5-HT and forskolin caused AMPA/kainate receptor-mediatedEPSPs to appear (Fig. 6A). The effect was long-lasting and persistedduring the washout (in the continuous presence of AP5). Spikeresponses were also observed after the treatment. Both newly recruitedEPSPs and spike responses were completely blocked by bath applicationof 20 µM CNQX in the continuous presence of 100 µM AP5 (Fig. 6).These results indicate that recruited AMPA receptor-mediated EPSPswere large enough to excite the neurons and generate spike responsesto primary afferent fiber stimulation at intensities that werepreviously unable to activate action potentials. Our results arein agreement with previous studies in young animals that the recruitmentof AMPA responses in dorsal horn neurons are NMDA receptor-independent(Li and Zhuo 1998; Li et al. 1999), a different form of plasticityfrom that reported in the hippocampus (Durand et al. 1996; Isaacet al. 1995; Liao et al. 1995).

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Fig. 6. Synergistic recruitment of AMPA/kainate receptor-mediated responses at pure NMDA synapses. A: examples of EPSPs showing synaptic responses before, during, and after co-application of 5 µM 5-HT and 10 µM forskolin in the presence of 100 µM AP5. B: the effect of 5-HT and forskolin on the EPSP slopes in the experiment shown in A. Spike responses to stimulation of the dorsal root nerves at the subthreshold intensity were observed during the washout (indicated by arrows). C: in a separate experiment, 20 µM CNQX completely blocked both EPSPs and action potentials induced by 5 µM 5-HT and 10 µM forskolin in the presence of AP5. D: summary data of 5 µM 5-HT and 10 µM forskolin. Data contain 2 sets of experiments: pure NMDA synapses (n = 3) and mixed AMPA/kainate and NMDA synapses (n = 6). In both cases, significant enhancement was observed, and data were pooled together.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We provide strong evidence that pure NMDA receptor-mediated synapses exist on adult dorsal horn sensory neurons. More importantly,we show here that these synapses can indeed mediate somatosensorysynaptic transmission between primary afferent fibers and dorsalhorn neurons. Because dorsal horn neurons containing pure NMDAsynapses have normal resting membrane potentials, we believe thatpure NMDA receptors contribute to normal sensory synaptic transmissionin adult mammalian spinal cord. Due to the fact that the sensitivityof intracellular recording is lower than that of patch clamping,it is quite possible that there may be some AMPA receptor-mediatedresponses below the detectable level in these synapses. Baba etal. (2000) reported that in adult rat dorsal horn there are afew pure NMDA synapses by using the whole cell patch-clamp recordingtechnique. One obvious difference is that adult mice were usedin the present study. We think that our studies will allow usto investigate the contribution of different subtypes of NMDAreceptors to sensory synaptic EPSPs in the spinal cord using geneticallymanipulated mice in future. Our current results do not excludethe possible presynaptic effects of serotonin and forskolin andfuture studies are needed to determine the pre- versus postsynapticcontribution to the enhancement. It is also important to determinewhat serotonin receptor subtypes are involved in the present experimentsby using both pharmacological and geneticapproaches.

Pure NMDA receptor-mediated synaptic responses

The existence of pure NMDA synapses has been reported in many different regions of the CNS, including the neocortex, hippocampus,and spinal cord (see INTRODUCTION). Studies from brain slicesfrom young rats as well as neuronal cultures indicate that therecruitment of AMPA receptors into pure NMDA synapses occurs duringdevelopment and may contribute to development-related synapticplasticity. In some areas of the brain, pure NMDA synapses disappearin late developmental stages with the loss of ability to undergosynaptic potentiation (or long-term potentiation). However, inother regions of the brain, long-term potentiation or long-lastingsynaptic enhancement of synaptic transmission happen in adultanimals and are thought to contribute to different functions ofthe brain, such as learning, memory in physiological conditionsand persistent pain after tissue injury (see Bliss and Collingridge1993; Malenka and Nicoll 2000; Sandkühler 2000). One criticalquestion is whether pure NMDA synapses are still present in adultneurons and, if so, whether the functional recruitment of AMPAreceptors into these synapses also occurs under certain circumstances.Indeed, early studies by Bardoni et al. (1998) and Li and Zhuo(1998) in the spinal cord were able to detect pure NMDA synapsesin slices from postnatal 21-day-old rats; this is different fromwhat is observed in the neocortex. Our present studies providestrong evidence that indeed pure NMDA synapses exist in adultspinal cord dorsal horn neurons. About 26% of synaptic responsesbetween primary afferent fibers and dorsal horn neurons are mediatedpurely by NMDA receptors. The stimulation paradigm used in thecurrent study is sufficient to activate A and even C fibersin some cases (see Yoshimura and Jessell 1989). This is in consistentwith the fact that neurons in superficial dorsal horn of adultanimals primarily receive nociceptive A and C fiber inputs(Light et al. 1979). Our results suggest that some of pure NMDAsynapses exit between nociceptive primary afferent fibers anddorsal hornneurons.

Pure NMDA synapses in adult neurons are functional. At normal soma resting membrane potentials, we detected pure NMDA receptor-mediatedEPSPs. Our results are thus unlikely due to tonic soma depolarization,which removes the magnesium blockade of the NMDA receptor channel.One likely possibility is that the magnesium blockade is reducedat NMDA receptors at distal synapses sites. There are at leasttwo mechanisms for reduced magnesium blockade: first, pure NMDAsynapses may be primarily situated in distal dendrites and localpostsynaptic potentials may be depolarized. Therefore the magnesiumblockade of NMDA receptors at these sites may be reduced. Second,they may represent a subpopulation of NMDA subtype receptors suchas NMDA2C and NMDA2D that are less sensitive to the magnesiumblockade (Burnashev et al. 1992; Momiyama 2000; Momiyama et al.1996; Seeburg 1993). Our results using a low concentration ofmagnesium support the second possibility. Consistent with thisfinding, in young spinal dorsal horn neurons, Bardoni et al. (2000)observed a slow, NMDA receptor-mediated excitatory postsynapticcurrent (EPSC) at $-$ 70 mV evoked by stimulation, implying thatnot all current through NMDA receptors is blocked by magnesiumat negative membrane potentials. Furthermore, these NMDA receptor-mediatedEPSCs can generate action potentials during repetitive stimulationin young animals (Bardoni et al. 2000) and after chemical treatmentsin adult dorsal horn neurons in the present study. This suggeststhat pure NMDA synapses can indeed contribute to sensory transmissionin the spinal cord. It is worthy to mention that indeed NMDA receptor-mediatedspikes has been reported in cortical pyramidal neuronal dendrites(Schiller et al. 2000). In their experiments using fluorescenceconfocal microscopy and mimicking EPSPs by ultraviolet laser glutamateuncaging, Schiller et al. (2000) showed that NMDA receptors onfine basal dendrites can be activated by glutamate and contributeto initiating local dendriticspikes.

Effects of serotonin on sensory synaptic transmission and nociception

Pharmacological and electrophysiological studies have provided evidence for spinal 5-HT system exerts biphasic effects onspinal nociceptive transmission. 5-HT or 5-HT receptor agonistsproduced both inhibitory and excitatory effects on spinal dorsalhorn neurons including ascending spinothalamic tract cells (seeMillan 1999 for a review). In behavioral tests, biphasic modulatoryeffects of 5-HT are also reported, and different subtypes of 5-HTreceptors are thought to contribute to biphasic modulation (Aliet al. 1994, 1996; Solomon and Gebhart 1988; Zelman et al. 1983).One major source of spinal 5-HT is from descending projectionfibers from the raphe nucleus and adjacent nuclei in the brainstem (Bowker and Abbott 1990; Fields et al. 1991), and stimulationat high intensities in these areas or indirectly in the periaqueductalgray released 5-HT in the lumbar spinal cord (Cui et al. 1999;Sorkins et al. 1993). Indeed, electrical or chemical stimulationin brain stem areas produces biphasic modulation in spinal nociceptivetransmission and the tail-flick reflex (Haber et al. 1980; Lightet al. 1986; McCreery et al. 1979; Zhuo and Gebhart 1990-1992,1997). Descending facilitation and descending inhibition are mediatedby different spinal 5-HT subtype receptors (Zhuo and Gebhart 1991).

Synaptic mechanisms for 5-HT-produced inhibition and facilitation have been studied in spinal cord slices from young animals(Hori et al. 1996; Khasabov et al. 1999; Li and Zhuo 1998; Lopes-Garziaand King 1996). 5-HT at high doses produced inhibition of synapticEPSCs or EPSPs by acting through postsynaptic and/or presynaptic5-HT receptors (see Grudt et al. 1996; Hori et al. 1996; Khasabovet al. 1999; Li and Zhuo 1998, 2001; Lopes-Garzia and King 1996).For 5-HT-induced excitatory or facilitatory effects, the recruitmentof postsynaptic silent synapses is critical for the facilitation(Li and Zhuo 1998; Li et al. 1999). Furthermore, the interactionbetween AMPA receptor and PDZ-domain-containing proteins are importantfor the effects of 5-HT (Li et al. 1999).

Unlike slices from young animals, a few reports were performed in slices of adult animals. Both postsynaptic excitatory andinhibitory effects on dorsal horn neurons have been reported inadult frog spinal cord, although synaptic responses to stimulationof afferent fibers had not been examined (Tan and Miletic 1990).In adult rats spinal cord, 5-HT produced inhibition or no effectson primary afferent-evoked synaptic responses (Ito et al. 2000).Consistent with this report in adult rats, we showed here that5-HT produced predominant inhibition of synaptic responses indorsal horn neurons of adult mice. Furthermore, we provided anew synergistic mechanism between 5-HT and cAMP for explainingthe facilitatory effect of spinal 5-HTsystem.

Synergistic effect between cAMP and serotonin

cAMP signal pathways haven been implicated in the function of spinal dorsal horn neurons. Activation of several receptorsfor sensory transmitters such as glutamate and CGRP has been reportedto raise cAMP levels. In slices or isolated cells from young animals,cAMP analogue enhanced glutamate receptor-mediated synaptic responses(Cerne et al. 1992, 1993) or no effect on AMPA/kainate receptor-mediatedsynaptic responses (Hori et al. 1996). In the present studies,application of forskolin did not significantly affect synapticresponses induced by dorsal root stimulation in slices of adultmice. However, co-application of 5-HT and forskolin produced long-lastingfacilitation of synaptic responses. Possible contributors to theincreases in the cAMP levels are the calcium-sensitive adenylylcyclases. We found that the facilitatory effect induced by 5-HTand forskolin was completely blocked in mice lacking AC1or AC8,indicating that calcium-sensitive adenylyl cyclases are important.Our results demonstrate that in adult sensory synapses, cAMP-signalingpathways determine whether activation of 5-HT receptors causesfacilitatory or inhibitory effects on synaptic responses. Unlikesynapses from young animals, 5-HT alone did not induce reliableand long-lasting facilitation of synaptic responses (see Li andZhuo 1998). Instead, 5-HT at the same low dose induced no effects,short-lasting increases or inhibition (see RESULTS) in adult neurons.However, co-application of the same dose of 5-HT with forskolinproduced significant long-lasting enhancement of synaptic responses.This finding provides a possible scenario for regulation of twodifferent signaling pathways under physiological or pathologicalconditions. Postsynaptic increases in cAMP levels by sensory transmittersmay favor 5-HT-induced facilitation. The interaction between cAMPand 5-HT may provide an associative heterosynaptic form of centralplasticity in the spinal dorsal horn to allow sensory inputs fromthe periphery to act synergistically with central descending modulatoryinfluences. We think that it is unlikely that cAMP acts additionallyto 5-HT signal pathways. First, 5-HT at a higher dose produceopposite effects, that is inhibition of synaptic responses. Forskolinalone did not produce any facilitation. Second, in young neurons,it has been reported that PKC is required for the effects of 5-HT(Li et al. 1999).

Physiological implications

Our results may provide a synaptic mechanism for the recruitment of ineffective synapses in adult animals after tissue ornerve injury (Wall 1977, 1988; Zhuo 2000). Recruitment of functionalAMPA responses may allow subthreshold stimulation of primary afferentfibers, which alone were not sufficiently strong to raise thecells above their firing threshold, to fire action potentials.A recent study revealed that AMPA receptor-PDZ domain interactionsare important for the 5-HT induced facilitation in young sensoryneurons (Li et al. 1999). Considering rapid developments in researchon glutamate receptors and advanced mouse genetics (Garner etal. 2000; Hollmann and Heinemann 1994; Seeburg 1993), we believethat this mouse study will facilitate future dissection of molecularmechanisms for plasticity of sensory glutamatergic synapses inthe spinalcord.

	ACKNOWLEDGMENTS

We thank Drs. Jim Huettner and Liang-Gang Wu for reading the manuscript and for suggestions. We also thank Dr. Louis Mugliafor providing AC1 and AC8 knockout mice for control experimentsand all members of the Zhuo laboratory for helpfulsuggestions.

This work was supported in part by National Institutes of Health Grants DA-10833 and NS-38680.

	FOOTNOTES

Address for reprint requests: M. Zhuo, Dept. of Anesthesiology, Washington University, Campus Box 8054, St. Louis, MO 63110(E-mail: zhuom{at}morpheus.wustl.edu).

Received 22 May 2001; accepted in final form 22 October 2001.

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