Regulation of Intrinsic and Synaptic Properties of Neonatal Rat Trigeminal Motoneurons by Metabotropic Glutamate Receptors

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The Journal of Neuroscience, November 15, 1998, 18(22):9216-9226

Regulation of Intrinsic and Synaptic Properties of Neonatal Rat Trigeminal Motoneurons by Metabotropic Glutamate Receptors
Christopher A. Del Negro and Scott H. Chandler
Department of Physiological Science, University of California at Los Angeles, Los Angeles, California 90095-1586

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We studied how metabotropic glutamate receptor (mGluR) activation modifies the synaptic and intrinsic membrane propertiesof neonatal rat trigeminal motoneurons using the broad-spectrummGluR agonist (1S,3R)-1-amino-1,3-cyclopentane-dicarboxylic acid[(1S,3R)-ACPD], group I/II antagonist (±)- $alpha$ -methyl-4-carboxy-phenylglycine(MCPG), and group III agonist L-2-amino-4-phosphonobutanoate (L-AP4).(1S,3R)-ACPD depressed excitatory transmission to trigeminal motoneuronspresynaptically and postsynaptically via presynaptic inhibitionand by reducing the currents carried by ionotropic glutamate receptorsselective for AMPA. (1S,3R)-ACPD also depolarized trigeminal motoneuronsand increased input resistance by suppressing a Ba²⁺-sensitive leakage K⁺ current. These effects were not mimicked by L-AP4 (100-200 µM).High-threshold Ca²⁺ currents were also suppressed by (1S,3R)-ACPD. Repetitive stimulationof excitatory premotoneurons mimicked the postsynaptic effectsof (1S,3R)-ACPD. The postsynaptic effects of (1S,3R)-ACPD andrepetitive stimulation were both antagonized by MCPG, suggestingthat mGluRs were similarly activated in both experiments. We concludethat mGluRs can be recruited endogenously by glutamatergic premotoneuronsand that mGluR-mediated depression of excitatory transmission,combined with increased postsynaptic excitability, enhances thesignal-to-noise ratio of oral-related synaptic input to trigeminalmotoneurons during rhythmical jawmovements.

Key words: (1S,3R)-ACPD; MCPG; leakage K⁺ currents; Ca²⁺ currents; mEPSCs; mGluR

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

To understand how the brain generates jaw movements, we must characterize the electrophysiological properties of oral-relatedbrain stem trigeminal neurons and their synaptic connections anddetermine whether these properties are modulated by endogenousneuromessengers. The anatomy and electrophysiology of the trigeminalmotoneurons, which innervate jaw musculature, have been studied(Moore and Appenteng, 1990, 1991; Curtis and Appenteng, 1993;Chandler et al., 1994; Turman and Chandler, 1994; Appenteng etal., 1995). However, neuromodulation of these properties has onlybeen examined for serotonin (Trueblood et al., 1996; Hsiao etal., 1997, 1998).

The endogenous excitatory transmitter glutamate, acting at metabotropic receptors, can modulate neuronal systems by regulatingthe intrinsic and synaptic properties of constituent neurons (forreview, see Gerber and Gähwiler, 1994; Glaum and Miller, 1994;Pin and Duvoisin, 1995). The neurons controlling jaw movementsmight also be influenced by metabotropic glutamate receptor (mGluR)activation. First, trigeminal motoneurons express mGluRs (Turmanet al., 1997) and receive glutamatergic input (Turman and Chandler,1994; Appenteng et al., 1995) from rhythmically active premotoneuronsduring masticatory activity (Katakura and Chandler, 1990). Also,continuous high-frequency stimulation of the masticatory cortexis the most effective method to evoke rhythmical jaw movementsin vivo (Lund, 1976; Nakamura, 1980; Goldberg et al., 1982). Suchrepetitive, high-frequency recruitment of excitatory synapsesactivates mGluRs endogenously (Scanziani et al., 1997).

In specific brain and spinal systems, the diverse effects of mGluR activation modify neuronal function. For instance, in thehippocampus, mGluR activation presynaptically inhibits transmissionto the dentate gyrus and CA1 region and enhances pyramidal cellexcitability. These effects may amplify the signal-to-noise ratioof transmission through the hippocampus (Conn et al., 1994). Inbrain stem-spinal networks that generate respiratory rhythms (Smithand Feldman, 1987), (1S,3R)-1-amino-1,3-cyclopentane-dicarboxylicacid [(1S,3R)-ACPD] reduces inspiratory motor output at low agonistconcentrations yet enhances inspiratory motor output at high agonistconcentrations. These paradoxical effects of mGluR activationwere attributed, in part, to differential effects of (1S,3R)-ACPDon the synaptic and intrinsic properties of diaphragmatic motoneurons(Dong et al., 1996).

Unfortunately, the same level of understanding has not been established for the neurons controlling jaw movements. Therefore,we tested the hypothesis that mGluR activation influences thesynaptic and intrinsic properties of trigeminal motoneurons invitro. We examined the regulation of excitatory synaptic transmissionto trigeminal motoneurons at presynaptic and postsynaptic sitesof action and the modulation of intrinsic membrane propertiesby mGluR activation. Finally, we provide evidence for the endogenousactivation of mGluRs by excitatory trigeminalpremotoneurons.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Whole-cell patch-clamp experiments were performed using a neonatal rat brain stem slice preparation. Rats (0-7 d) were anesthetizedby halothane inhalation (Halocarbon Laboratories, River Edge,NJ) and dissected in oxygenated ice-cold cutting solution (seebelow). Coronal slices (300 µm) were cut (DSK Microslicer, TedPella, Redding, CA) and placed into incubation solution (see below)at 37°C for 40min.

Cutting solution contained (in mM): 126 NaCl, 3 KCl, 1.25 NaH₂PO₄, 26 NaHCO₃, 10 glucose, 1 CaCl₂, 5 MgCl₂, and 4 lactic acid(Schurr et al., 1988). Recording solution contained (in mM): 124NaCl, 3 KCl, 1.25 NaH₂PO₄, 26 NaHCO₃, 10 glucose, 2 CaCl₂, and2 MgCl₂. Incubation solution was identical to recording solutionwith additional 4 mM lactic acid. Solutions were bubbled with95% O₂-5% CO₂ and maintained at pH $congruent$ 7.3 (22-24°C). When recordingCa²⁺ currents we used a phosphate-free solution containing (in mM):105.25 NaCl, 3 KCl, 26 NaHCO₃, 10 glucose, 2 CaCl₂, 20 tetraethylammoniumchloride (TEA-Cl), and 3CsCl.

Normally, patch electrode solution contained (in mM): 9 NaCl, 140 KCl, 1 MgCl₂, 10 HEPES buffer, 0.2 EGTA, 10 phosphocreatine,0.1 leupeptin, 5 K₂-ATP, 1 Na₃-GTP, pH $congruent$ 7.25 (osmolarity 280-290mM). When recording synaptic or Ca²⁺ currents we used a modified patch solution to block K⁺ currents containing (in mM): 125 cesium methanesulfonate (CsMeSO₄),4 NaCl, 3 KCl, 1 MgCl₂, 8 HEPES, 9 EGTA, 10 phosphocreatine, 0.1leupeptin, 5 K₂-ATP, 1 Na₃-GTP, pH $congruent$ 7.25. Lucifer yellow (0.1%)was added to patch solutions for fluorescentviewing.

Drugs were bath-applied at the following concentrations: (1S,3R)-ACPD (10-100 µM; RBI, Natick, MA), MCPG (1 mM; RBI), L-AP4(0.1-0.2 mM), bicuculline methiodide [20 µM; Sigma (St. Louis,MO)], strychnine (5 µM; Sigma), 6-cyano-7-nitroquinoxaline-2,3-dionedisodium (CNQX) (10 µM; RBI), D,L-2-amino-5-phosphonovaleric acid(APV) (10 µM; Sigma), 6-chloro-3,4-dihydro-3-[2-norbornen-5-y]-2H-1,2-4-benzothiadiazine-7-sulfonamide1,1-dioxide (cyclothiazide) (10 µM; Sigma), glycine (2 µM; Sigma),and tetrodotoxin (TTX) (0.5 µM; Sigma). AMPA (0.5 mM; RBI) andNMDA (1 mM; RBI) were applied by micropressure ejection. Ba²⁺ (2 mM) and Cd²⁺ (50-200 µM) were added directly to the bath in some experimentsto reduce leakage K⁺ and Ca²⁺ currents,respectively.

Slices were perfused by oxygenated recording solution at room temperature and visualized by differential interference contrastmicroscopy (Edwards et al., 1989; Stuart et al., 1993). The trigeminalmotor nucleus was identified bilaterally in the coronal sliceunder low magnification (5×) as an ellipsoid region, equidistantfrom the midline and lateral border, ventral to the mesencephalictrigeminal sensory nucleus. The trigeminal motor nucleus couldalso be distinguished at 40× for visual selection of motoneurons.In some experiments, the trigeminal motor and sensory nuclei wereretrogradely and anterogradely labeled, respectively, using Texasred (10%, Molecular Probes, Eugene, OR) for fluorescent viewing.Microinjections of Texas red into the masseter and temporalisjaw closer muscles were performed at least 24 hr before theexperiment.

We fabricated patch electrodes from capillary glass (3-7 M $Omega$ ; Sutter Instruments P-97, Novato, CA), and recorded using an Axopatch-1Damplifier and pCLAMP software (Axon Instruments, Burlingame, CA).Signals were grounded (Ag/AgCl wire) using a 3 M KCl agar bridge;a 1 mV junction potential was notcompensated.

Cell capacitance (C_M) for each trigeminal motoneuron recorded in voltage clamp was determined from the integral of capacitycurrent in response to 15 msec hyperpolarizing commands. Uncompensatedseries resistance (R_S) was calculated from the decay time constant( $tau$ ) of the transient ( $tau$ $congruent$ R_SC_M). It averaged 17.1 ± 0.9 M $Omega$ andwas routinely compensated to 5.3 ± 0.3 M $Omega$ (n = 66) through theamplifier.

We recorded excitatory synaptic currents in the presence of bicuculline and strychnine to block inhibitory ionotropic receptorsand used patch solution containing intracellular Cs⁺ to block K⁺ currents and improve space clamp. Motoneuronal membrane propertieswere examined in the presence of bicuculline, strychnine, CNQX,APV, and usually TTX to block inhibitory and excitatory ionotropicreceptors and Na⁺ channels, respectively. During these experiments we used normalpatch solution because motoneuronal K⁺ channels were ofinterest.

To measure miniature EPSCs (mEPSCs), cells were held at $-$ 60 mV in the presence of TTX, and spontaneous synaptic events wererecorded at 5 kHz and analog-filtered at 2 kHz for a durationof 2 min. A noise histogram was generated from the baseline currentduring periods containing no synaptic events (>16,000 points),and a Gaussian distribution was fitted to the histogram to determinethe SD of baseline noise. Synaptic events were selected automaticallyby a threshold-crossing algorithm, with detection level set at,or greater than, two times the SD of baseline noise (Datapac III,Run Technologies, Irvine, CA). To test whether (1S,3R)-ACPD modifiedthe amplitude or frequency of miniature synaptic currents, weused cumulative probability histograms, for amplitude (bin size0.1-0.5 pA) and interevent interval (minimum bin size 10 msec),and the Kolmogorov-Smirnov statistic (SYSTAT 7.0, SPSS, Chicago,IL). Significance was assessed at p < 0.05.

To evoke excitatory synaptic responses, individual interneurons (0.1-15 µA) or clusters of interneurons (10-150 µA) surroundingthe trigeminal motor nucleus were stimulated extracellularly (GrassInstruments, Quincy, MA) using saline-filled pipettes. Ionotropicglutamate receptor currents were measured in trigeminal motoneuronsusing intracellular Cs⁺ patch solution in the presence of bicuculline, strychnine, andTTX. Glutamate agonists were pressure-applied locally by a PicospritzerII ejection system (General Valve, Fairfield, NJ) using patch-likepipettes (diameter = 10 µM) and ejection times of 300-750 msec.Differences in the means of evoked synaptic currents and theirnumber of failures and ionotropic glutamate receptor agonist-evokedcurrents were tested using Student's t statistic (SYSTAT); significancewas assessed at p < 0.05. Means are expressed ± SE of the mean(except for Fig. 1A; seelegend).

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Depression of excitatory synaptic transmission

We identified unitary connections between excitatory trigeminal premotoneurons and trigeminal motoneurons by stimulating visuallyidentified, putative premotoneurons (0.1-15 µA). If a synapticconnection existed with the target motoneuron, an evoked EPSCwas observed only when the stimulus intensity was increased beyondthreshold (Fig. 1A, 3 µA). Retracting the stimulating pipette2-5 µm from the cell soma elevated the threshold. Suprathresholdstimulus intensities did not induce graded responses in evokedEPSC amplitude (Fig. 1A). These data indicate that trigeminalpremotoneuron-motoneuron synaptic connections were unitary, thatis, the result of stimulation of a single presynaptic neuron (Sternet al., 1992).

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Figure 1. The effects of (1S,3R)-ACPD on unitary evoked synaptic transmission. A, A plot of the relationship between evoked EPSC amplitude (mean ± SD) and stimulus intensity. B, Evoked EPSCs from the cell in A during control (top), 100 µM (1S,3R)-ACPD (middle), and washout (bottom) conditions. Trigeminal motoneurons were recorded with patch solution containing intracellular Cs⁺ in the presence of bicuculline and strychnine. Holding potential was $-$ 60 mV; time and current calibrations are shown. The stimulus artifact is partially deleted. C, D, A summary of the effects of 20 and 100 µM (1S,3R)-ACPD on evoked EPSC amplitude (C) and proportion of synaptic failures relative to control (D). Both ordinate axes reflect percentage of control; bars reflect the mean of all cells tested (± SE).

To test the effects of mGluR activation on evoked synaptic transmission, 20-50 suprathreshold stimuli were applied at 0.3Hz during control, (1S,3R)-ACPD, and washout conditions. The meanamplitude of the evoked EPSC was calculated from the average ofall traces containing a synaptic event, and the number of synapticfailures was noted. (1S,3R)-ACPD reversibly reduced the mean amplitudeof the evoked EPSC and increased the number of synaptic failures(Fig. 1B, same cell as A). In general, 100 µM (1S,3R)-ACPD significantlydecreased the mean amplitude of the evoked EPSC from 59.1 ± 16.0pA to 24.1 ± 5.0 pA (n = 6). Evoked EPSC amplitude was also significantlyreduced by 20 µM (1S,3R)-ACPD from 43.0 ± 9.8 pA to 28.9 ± 4.6pA (n = 9) (Fig. 1C). The extent to which 20 and 100 µM (1S,3R)-ACPDsuppressed the evoked EPSC also differedsignificantly.

The effect of (1S,3R)-ACPD on synaptic failures was evaluated by the ratio of the number of failures in (1S,3R)-ACPD to thenumber of failures in control. Failures increased significantlyby 472 ± 90% in the presence of 100 µM (1S,3R)-ACPD (n = 6) andby 397 ± 95% in the presence of 20 µM (1S,3R)-ACPD (n = 9) (Fig.1D). The elevation in synaptic failures suggests that mGluR activationlowered the probability of presynaptic release. However, thesedata could not establish whether the (1S,3R)-ACPD-induced reductionin evoked EPSC amplitude resulted from inhibition of presynapticrelease or from postsynaptic modification of excitatory aminoacid receptors, orboth.

To distinguish presynaptic and postsynaptic effects of mGluR activation, we recorded mEPSCs in trigeminal motoneurons usingTTX (Figs. 2, 3). (1S,3R)-ACPD (100 µM) reversibly and significantlydecreased mEPSC frequency by 2.6 ± 0.9 Hz (57 ± 16% of control)in four of five cells tested; in one cell mEPSC frequency increasedby 2.3 Hz. (1S,3R)-ACPD (20 µM) significantly decreased mEPSCfrequency by 2.3 ± 1.2 Hz (60 ± 8% of control) in all cells tested(n = 3). The (1S,3R)-ACPD-mediated reduction in mEPSC frequencyis shown in sample traces (Fig. 2A) and mEPSC amplitude histogramsfrom the same cell (Fig. 2B). These data also suggest that (1S,3R)-ACPDcaused presynaptic inhibition.

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Figure 2. The effects of (1S,3R)-ACPD on miniature synaptic currents. A, Sample traces from a representative TMN in control (top), 100 µM (1S,3R)-ACPD (middle), and washout (bottom) conditions. Trigeminal motoneurons were recorded using patch solution containing intracellular Cs⁺ in the presence of bicuculline, strychnine, and TTX. Holding potential was $-$ 60 mV; time and current calibrations are shown. B, mEPSC amplitude histograms from the cell in A. Histograms for control (open bars) and (1S,3R)-ACPD (closed bars) conditions are superimposed (left). The histogram for washout is shown at right. The ordinate axis (left) applies to both histograms.

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Figure 3. The effects of (1S,3R)-ACPD on cumulative probability mEPSC amplitude histograms. A, In the same cell as Figure 2, 100 µM (1S,3R)-ACPD caused a leftward shift of the cumulative probability histogram. B, An example of a TMN whose cumulative probability histograms superimposed for control and 20 µM (1S,3R)-ACPD conditions. For both A and B, control and (1S,3R)-ACPD conditions are distinguished by $open circle$ and $bullet$ , respectively. Bin size was adjusted to 1 pA for display purposes.

We examined postsynaptic contributions to (1S,3R)-ACPD-mediated synaptic depression using cumulative probability mEPSC amplitudehistograms (Fig. 3). These distributions are obtained by integratingthe mEPSC amplitude histogram (e.g., Fig. 2B) and normalizingthe ordinate range to the interval zero to one. In the majorityof trigeminal motoneurons tested, (1S,3R)-ACPD caused a significantleftward shift of the cumulative probability amplitude histogram,indicating a postsynaptic reduction in mEPSC amplitude (Fig. 3A;same cell as Fig. 2). This result was observed in four of fivecells tested at 100 µM (1S,3R)-ACPD and in one of three cellstested at 20 µM (1S,3R)-ACPD. In all other cells tested, at 20or 100 µM (1S,3R)-ACPD, the cumulative probability histogramssuperimposed for control and (1S,3R)-ACPD conditions, and theKolmogorov-Smirnov statistic was not significant, suggesting nopostsynaptic modification of mEPSC amplitude (Fig. 3B). All motoneuronswhose cumulative probability histograms superimposed in controland (1S,3R)-ACPD conditions also exhibited an (1S,3R)-ACPD-inducedreduction in mEPSC frequency. Therefore, it is unlikely that thereduction in mEPSC frequency could have been an artifact of areduction in mEPSC amplitude caused by mEPSCs falling below detectionlevels.

The leftward shift of the cumulative probability histogram could be caused by postsynaptic modulation of excitatory aminoacid receptors. To test this possibility, specific excitatoryamino acid receptor agonists were locally applied to trigeminalmotoneurons in control, (1S,3R)-ACPD (20 or 100 µM), and washoutconditions. We used AMPA to activate non-NMDA receptors, whiletrigeminal motoneurons were held at $-$ 60 mV in the presence ofthe NMDA receptor antagonist APV and cyclothiazide to preventAMPA receptor desensitization (Hall et al., 1993; Partin et al.,1993; Sharp et al., 1994). (1S,3R)-ACPD (100 µM) significantlyand reversibly reduced the peak AMPA-induced current from 2.7± 0.5 nA to 1.8 ± 0.3 nA (n = 5) (Fig. 4A). (1S,3R)-ACPD (20 µM)reduced the AMPA current from 1.5 ± 0.5 nA to 1.2 ± 0.2 nA (n= 4 of 5), although this was not statistically significant.

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Figure 4. (1S,3R)-ACPD modulation of ionotropic glutamate receptors. A, Current responses of trigeminal motoneurons to specific excitatory amino acid receptor agonists: NMDA (top) and AMPA (bottom). Agonists were applied at the time indicated by the large arrow (duration 300-750 msec). All trigeminal motoneurons were recorded using a patch solution containing intracellular Cs⁺ in the presence of bicuculline and strychnine and other drugs needed to isolate ionotropic glutamate receptor subtypes (see Materials and Methods). Holding potentials and current calibrations are shown. The 2.5 sec time calibration applies to the NMDA traces; the 5 sec time calibration applies to the AMPA traces. Sample NMDA responses during control, 100 µM (1S,3R)-ACPD, and washout conditions are superimposed (top). AMPA responses during control, 100 µM (1S,3R)-ACPD, and washout conditions are differentiated by traces labeled a, b, and c, respectively (bottom). B, A summary of the effects of 20 and 100 µM (1S,3R)-ACPD on ionotropic glutamate receptor currents. A statistically significant change relative to control is indicated by an asterisk.

The potential for modulation of NMDA receptors was tested with NMDA in the presence of glycine and the AMPA receptor antagonistCNQX. Trigeminal motoneurons were held at +40 mV to relieve voltage-dependentblock of NMDA channels by Mg²⁺. Postsynaptic NMDA currents were unaffected by either 20 or 100µM (1S,3R)-ACPD in all cells tested (n = 3 and 7, respectively)(Fig. 4A, top). The effects of (1S,3R)-ACPD on peak excitatoryamino acid agonist responses are summarized in Figure 4B.

To test whether the output of excitatory premotoneurons was affected by mGluR activation, we recorded spontaneous EPSCs intrigeminal motoneurons in the absence of TTX. The recording protocoland statistical tests were identical for spontaneous EPSCs andmEPSCs. In five motoneurons, 100 µM (1S,3R)-ACPD reversibly andsignificantly increased spontaneous EPSC frequency by 10.4 ± 0.9Hz (277% of control) (Fig. 5A). Because (1S,3R)-ACPD caused presynapticinhibition (Figs. 1-3), the enhancement of spontaneous EPSC frequency,in the absence of TTX, suggests that the soma-dendritic membranesof premotoneurons were excited by (1S,3R)-ACPD to produce morespikes and augment synaptic output. In contrast, in two of sevencells tested, 100 µM (1S,3R)-ACPD reversibly and significantlydecreased spontaneous EPSC frequency by 3.4 Hz (52% of control)(Fig. 5B), suggesting either presynaptic inhibition or disfacilitationof excitatory input to trigeminal motoneurons (TMNs).

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Figure 5. The effects of (1S,3R)-ACPD on spontaneous synaptic currents. Trigeminal motoneurons were recorded with intracellular Cs⁺ patch solution and held at $-$ 60 mV, in the presence of bicuculline and strychnine. Sample traces during control (top), 100 µM (1S,3R)-ACPD (middle), and washout (bottom) are shown. A, (1S,3R)-ACPD (100 µM) increased spontaneous EPSC frequency. B, Spontaneous EPSC frequency was reversibly reduced by (1S,3R)-ACPD in this cell. Time and current calibrations apply to A and B.

Modulation of TMN excitability

In current clamp, using TTX to prevent excitation of premotoneurons by (1S,3R)-ACPD (e.g., Fig. 5A), 100 µM (1S,3R)-ACPD reversiblydepolarized trigeminal motoneurons and increased input resistance(Fig. 6A) (n = 3). At a lower dose (20 µM), (1S,3R)-ACPD depolarizedthe majority of trigeminal motoneurons tested (n = 5 of 7); at10 µM, (1S,3R)-ACPD was ineffective (n = 3; data not shown). Therefore,20 µM approximated the minimum dose required to depolarize trigeminalmotoneurons. To examine the effects of (1S,3R)-ACPD in more detail,we measured the input resistance of motoneurons from the slopeof the steady-state voltage-current (V-I) relationship constructedfrom membrane potential responses to 600 msec current step commands.(1S,3R)-ACPD (100 µM) reversibly increased input resistance, mostlikely by decreasing a tonic K⁺ conductance, because the steady-state V-I curves intersectedat $-$ 90 mV (close to the Nernst potential for K⁺, $-$ 97 mV) (Fig. 6B, same cell as A).

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Figure 6. The effects of (1S,3R)-ACPD on membrane properties of trigeminal motoneurons. All cells were recorded with a normal patch solution. A, (1S,3R)-ACPD (100 µM) caused reversible depolarization and increase in input resistance. Current steps command of 300 msec, $-$ 350 pA were delivered at 0.1 Hz; inset shows membrane potential deflections before, during, and after (1S,3R)-ACPD application. B, Steady-state V-I curves for the cell in A before, during, and after a subsequent application of 100 µM (1S,3R)-ACPD. Steady-state voltage deflections were measured at the end of 600 msec current step commands. Control ( $open circle$ ), (1S,3R)-ACPD ( $bullet$ ), and washout ( $black-square$ ) are shown with regression lines. C, Membrane potential responses to 20 µM (1S,3R)-ACPD in the presence of TTX. The duration of (1S,3R)-ACPD application is shown by bars overlying the voltage trace. Bath application of MCPG is also illustrated by a bar overlying the voltage trace. Time breaks in the record are indicated; time and voltage calibrations apply only to C. D, E, Steady-state I-V curves obtained from slow voltage ramp protocols (8 mV/sec) were used to calculate the current induced by (1S,3R)-ACPD (I_ACPD). Cells were bathed in bicuculline, strychnine, CNQX, APV, and TTX. The abscissa and ordinate apply to both D and E. I_ACPD ( $open circle$ ) is shown during control (D) and 1 mM MCPG conditions (E). The reversibility of (1S,3R)-ACPD is indicated by the subtracted current (washout $-$ control; D, $bullet$ ). The inset in E shows I_ACPD on an expanded ordinate axis; the abscissa is identical to the main plot (below).

The postsynaptic depolarizing effects of (1S,3R)-ACPD were significantly and reversibly antagonized by preapplication (>6min) of the group I/II mGluR antagonist MCPG (n = 5) (Eaton etal., 1993; Jane et al., 1993). (1S,3R)-ACPD (20 µM) normally depolarizedtrigeminal motoneurons by 7.8 ± 1.2 mV. The (1S,3R)-ACPD-induceddepolarization decreased significantly and reversibly to 1.0 ±0.6 mV in the presence of MCPG (Fig. 6C), suggesting that (1S,3R)-ACPDdepolarized trigeminal motoneurons by recruiting a group I orII mGluR to directly modulate postsynaptic membraneproperties.

To further examine the effects of (1S,3R)-ACPD, we measured the steady-state V-I relationship of trigeminal motoneurons involtage clamp in the presence of bicuculline, strychnine, CNQX,APV, and TTX to synaptically isolate cells and block spikes. Weused slow voltage ramps (8 mV/sec) to obtain quasi-steady-stateI-V data. To justify the use of ramps, which approximate steadystate, the I-V curve was obtained using a series of 2 sec voltage-stepcommands; this curve superimposed with the I-V relationship obtainedfrom the slow voltage ramp (verified in five trigeminal motoneurons;data not shown). The ramp protocol was preferable because it couldcollect I-V data more rapidly, thereby minimizing the periodsof drugapplication.

The current induced by 20 µM (1S,3R)-ACPD (I_ACPD) was obtained by subtracting the current obtained in control from that obtainedduring (1S,3R)-ACPD application (Fig. 6D, $open circle$ ). I_ACPD, when plottedversus membrane potential, was U-shaped in all cells tested at20 or 100 µM (1S,3R)-ACPD (n = 13 and n = 8, respectively). Thesedata suggested that (1S,3R)-ACPD induced a voltage-dependent inwardcurrent in the range $-$ 100 to $-$ 30 mV, which appeared to reverseat a membrane potential less than $-$ 65 mV, and another voltage-dependentcurrent from $-$ 30 mV to more depolarized levels, which reversedat a potential greater than $-$ 20 mV. The effects of (1S,3R)-ACPDwere largely reversible, as shown by the difference current obtainedfrom subtracting control from the washout conditions (Fig. 6D, $bullet$ ).

In separate cells, we measured I_ACPD in the presence of the group I/II mGluR antagonist MCPG (Fig. 6E). Normally, the peakinward I_ACPD, measured near $-$ 30 mV was $-$ 210 ± 31 pA (n = 13).Pre-incubation (>6 min) in MCPG significantly reduced the peakI_ACPD to $-$ 27 ± 14 pA (n = 8) (Fig. 6E). The inset of Figure 6Eshows that I_ACPD, plotted versus membrane potential, was stillU-shaped, but the magnitude of I_ACPD was greatly reduced becauseof MCPG antagonism. Because I_ACPD was negligible in the presenceof MCPG (Fig. 6E), the data are consistent with the current-clampexperiments in which MCPG antagonized the (1S,3R)-ACPD-induceddepolarization (Fig. 6C).

To test whether a group III mGluR could also be involved in modulation of motoneuronal membrane properties, we applied thegroup III agonist L-AP4 at 100 and 200 µM (n = 5 and 3, respectively)in the presence of bicuculline, strychnine, CNQX, APV, and TTX.In current clamp, neither dose of L-AP4 depolarized trigeminalmotoneurons or had any affect on the steady-state V-I relationship,suggesting no involvement of group III mGluRs (Fig. 7).

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Figure 7. The effect of 200 µM L-AP on membrane properties. Trigeminal motoneurons were recorded with normal patch solution in the presence of bicuculline, strychnine, CNQX, APV, and TTX. Steady-state V-I curves, obtained from 600 msec current pulses, are superimposed for control ( $open circle$ ), L-AP4 ( $bullet$ ), and washout ( $triangle$ ) conditions.

Next we identified the intrinsic conductances modulated by (1S,3R)-ACPD. I_ACPD in the range of $-$ 100 to $-$ 30 mV reversed near $-$ 90 mV (Fig. 6D). Because the reversal potential for K⁺ is $-$ 97 mV (in our conditions) and (1S,3R)-ACPD caused depolarizationand increased input resistance, we hypothesized that (1S,3R)-ACPDreduced a leakage K⁺ current. To test this, Ba²⁺ was added to the bath before (1S,3R)-ACPD in an attempt to occludemodulation of leakage currents. For these and all subsequent experiments,3 mM Cs⁺ was used to block the hyperpolarization-activated, mixed cationic,inwardly rectifying current I_h, which is active at potentialsmore negative than rest in trigeminal (Chandler et al., 1994)and other motoneurons (Takahashi, 1990; Bayliss et al., 1994).The current induced by Ba²⁺ (I_Ba) was obtained by subtraction: the difference between Ba²⁺ conditions and control. I_Ba was a linear inward current at potentialsgreater than $-$ 100 mV and appeared to reverse at $-$ 100 mV (n = 5)(Fig. 8, $open circle$ ). This is consistent with the blockade of leakage K⁺ channels (Hsiao et al., 1997). We then applied 100 µM (1S,3R)-ACPD.In the voltage range $-$ 100 to $-$ 30 mV, Ba²⁺ occluded the effects of (1S,3R)-ACPD (I_ACPD is negligible atpotentials more negative than $-$ 30 mV) (Fig. 8, $bullet$ ).

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Figure 8. The effect of extracellular Ba²⁺ on I_ACPD. Trigeminal motoneurons recorded with normal patch solution in the presence of extracellular Cs⁺, bicuculline, strychnine, CNQX, APV, and TTX. The current induced by Ba²⁺ (I_Ba) was obtained by subtraction ( $open circle$ ). I_ACPD (100 µM) in the presence of Ba²⁺ is also shown ( $bullet$ ).

In the presence of Ba²⁺, 100 µM (1S,3R)-ACPD still induced outward current at potentials greater than $-$ 30 mV (Fig. 8, $bullet$ ). Theoutwardly rectifying current induced by (1S,3R)-ACPD could beexplained by enhancement of a voltage-dependent K⁺ current, reduction of a voltage-dependent, noninactivating inwardcurrent, or both. To test this, 20 mM TEA-Cl was substituted forNaCl (in normal recording solution containing ionotropic receptorantagonists, TTX, Ba²⁺, and Cs⁺) in an attempt to occlude the (1S,3R)-ACPD-induced outward current.The block of TEA-sensitive outward currents exposed a prominentregion of inward current (presumably attributable to Ca²⁺ channels) in the steady-state I-V relationship. I_ACPD (Fig. 9A,bottom) was not occluded by TEA, because under these conditions(1S,3R)-ACPD reversibly reduced the region of inward current atpotentials more positive than $-$ 30 mV (Fig. 9A, top) (n = 5). However,the outward current induced by (1S,3R)-ACPD was blocked by previousapplication of 100 µM Cd²⁺ (n = 3) (Fig. 9B). These data suggested that (1S,3R)-ACPD reduceda Cd²⁺-sensitive, noninactivating, high-threshold Ca²⁺ current (I_Ca).

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Figure 9. The effects of (1S,3R)-ACPD on high-threshold Ca²⁺ currents. A, Steady-state I-V curves (not subtracted currents) from a representative cell during control ( $open circle$ ), 100 µM (1S,3R)-ACPD ( $bullet$ ), and washout conditions (line) are displayed in the top plot. The bottom plot shows the subtracted current, I_ACPD (ACPD $-$ control). B, The top plot shows raw membrane current. Preapplication of 100 µM Cd²⁺ ( $bullet$ ) blocked the effects of 100 µM (1S,3R)-ACPD (gray circles). The subtracted current, I_ACPD, is shown in the bottom plot. Motoneurons in A and B were recorded with normal patch solution in the presence of TEA, Ba²⁺, extracellular Cs⁺, bicuculline, strychnine, CNQX, APV, and TTX. C, The sequence of a typical experiment using intracellular Cs⁺ patch solution and phosphate-free recording solution with TEA to test mGluR modulation of Ca²⁺ currents. The results are qualitatively identical to A and B but were obtained in a continuous experiment in one cell.

Modulation of I_Ca by (1S,3R)-ACPD was further examined under conditions that isolate Ca²⁺ currents (Fig. 9C). Normal patch electrode solution was replacedby patch solution containing intracellular Cs⁺, and recording solution was replaced by phosphate-free solution.Under these conditions, intracellular Cs⁺ minimizes the leakage K⁺ current (and I_h), and Ca²⁺ was the only charge carrier for Ca²⁺ channels. The recording solution also contained TEA to blockactive K⁺ currents, including Ca²⁺-dependent K⁺ currents (Chandler et al., 1994; Kobayashi et al., 1997). Figure9C illustrates a typical experiment in one cell. (1S,3R)-ACPD(100 µM) reversibly reduced I_Ca. After recovery, 50 µM Cd²⁺ was applied to block I_Ca. In the presence of Cd²⁺, (1S,3R)-ACPD reapplication was ineffective; I_ACPD was nearlyzero over the range of potentials tested (n = 3). These effectswere reversible (Fig. 9C).

Endogenous activation of mGluRs

On the basis of the sensitivity of trigeminal motoneurons to (1S,3R)-ACPD, we hypothesized that mGluRs would be activatedendogenously during repetitive stimulation of excitatory premotoneurons.To test this, we identified a compound excitatory synaptic connectionbetween several trigeminal premotoneurons and a motoneuron. Thecompound synaptic connection was more advantageous than a unitaryconnection because it provided a larger amplitude, more consistentsynaptic response. Therefore, it was more likely to activate alarger proportion of postsynaptic glutamate receptors. Trigeminalmotoneurons were recorded using normal intracellular patch solutionin the presence of bicuculline and strychnine. Groups of cells,visually identified outside the borders of the trigeminal motornucleus, were stimulated extracellularly. Evoked compound EPSCswere observed at all stimulus intensities. The amplitude of thecompound EPSC was graded (until the maximal response), and nosynaptic failures were observed (Fig. 10A), demonstrating thatthe synaptic connection was compound, as opposed to unitary (compareFig. 1A).

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Figure 10. Endogenous activation of mGluRs by high-frequency activity in excitatory synapses onto trigeminal motoneurons. A, Compound excitatory synaptic currents in a motoneuron held at $-$ 60 mV. Stimulus intensity is indicated by each sample trace (left). Time and current calibrations apply to all traces in A. Stimulus artifacts were partially deleted. B, Schematic diagram of a typical experiment. Pharmacological conditions are indicated by the bars overlying the protocol. Time breaks are shown. Ramp icons represent the acquisition of a steady-state I-V curve via slow voltage ramp commands (8 mV/sec). The inverted comb icon represents 30 Hz stimulation (40 µA intensity) of premotoneurons for 1 min (as labeled). C, Subtracted currents from the protocols illustrated in B. Abscissa and ordinate axes are identical for all three plots.

Next, the compound EPSC was eliminated by CNQX and APV application (Fig. 10A, bottom). In the presence of ionotropic glutamatereceptor antagonists, the effects of mGluR activation are unlikelyto be obscured by temporal summation of fast synaptic currents.Figure 10B shows the protocol. The steady-state I-V relationshipwas obtained as a control (Fig. 10Ba). Premotoneurons were thenstimulated at 30 Hz for 1 min to induce glutamate accumulationand mGluR activation (Scanziani et al., 1997). The I-V relationshipwas acquired immediately after termination of the 30 Hz protocol(Fig. 10Bb) to assess whether the protocol modified postsynapticmembrane properties. The current induced by 30 Hz stimulation(I_30Hz) was obtained by subtraction (post-30 Hz $-$ control) andis illustrated in Figure 10C (b-a). I_30Hz was U-shaped, similarto I_ACPD (e.g., Fig. 6D). The I-V relationship was then obtained1 min after the stimulation protocol to assess the reversibilityof these effects (Fig. 10Bc). These effects were partially reversible,with some rundown [60 sec post-30 Hz $-$ control; Fig. 10C (c-a)].

This experiment was then repeated in the presence of MCPG (Fig. 10B). Here, the effects of 30 Hz stimulation were antagonizedover the entire voltage range, although I_30Hz was still slightlyU-shaped (Fig. 10C, e-d). These data resemble the MCPG antagonismof I_ACPD (Fig. 6E). The stimulation protocol mimicked (1S,3R)-ACPDapplication, and I_30Hz was antagonized by MCPG (n = 6 of 8). Thissuggests that high-frequency activation of excitatory synapsesrecruited mGluRsendogenously.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In trigeminal motoneurons, mGluR activation depresses excitatory transmission via presynaptic inhibition and postsynapticdepression of ionotropic glutamate receptors selective for AMPA.Also, mGluRs enhance postsynaptic excitability by reducing leakageK⁺ currents and high-threshold Ca²⁺ currents. How can these seemingly disparate effects influencethe neurophysiology of jawmovements?

We propose that mGluR activation enhances the signal-to-noise ratio of oral-related motor commands. The presynaptic and postsynapticeffects of mGluRs inhibit asynchronous sources of synaptic "noise"and accentuate rhythmical oral-related signals composed of slowand synchronous synaptic potentials. Finally, motoneuronal outputis augmented via mGluR enhancement of postsynaptic excitability.We elaborate on this hypothesis in our discussion of thedata.

According to our hypothesis, mGluRs are activated endogenously by high-frequency recruitment of excitatory synapses. mGluRactivation will decrease the amplitude and frequency of fast excitatorysynaptic inputs to trigeminal motoneurons. However, excitatorytransmission using non-NMDA receptors will be more strongly depressedthan transmission mediated by NMDA receptors, because NMDA receptorsare not modulated by mGluRs postsynaptically (Fig. 4). Therefore,this favors slow and synchronous sources of synaptic input that,through temporal summation, depolarize trigeminal motoneuronsaway from the resting potential ( $-$ 65 mV) and recruit NMDA receptors,to a greater extent, by relieving the voltage-dependent Mg²⁺ blockade (Mayer et al., 1984; Nowak et al., 1984; Mayer and Westbrook,1985). The relative effectiveness of fast and asynchronous sourcesof excitatory input, which are mediated primarily by AMPA receptorsnear resting potential, will decrease in comparison. This mayrepresent a mechanism to depress sporadic and asynchronous synaptic"noise" and favor rhythmical signals composed of the sum of slowand synchronous synapticpotentials.

The postsynaptic effectiveness of "favored," synchronous synaptic signals will be amplified by the effects of mGluRs on theintrinsic properties of trigeminal motoneurons. The reductionin leakage K⁺ current by mGluR activation causes depolarization and increasesinput resistance. Depolarization brings the cell closer to spikethreshold and the threshold for activation of NMDA receptors.Increased input resistance amplifies the gain between synapticcurrent and membrane voltage response. Therefore, the synapticcurrents received by trigeminal motoneurons will cause greaterdepolarization, leading to NMDA receptor activation and spikedischarge. The reduction of high-threshold Ca²⁺ currents may further augment the frequency-current relationshipin trigeminal motoneurons by suppressing Ca²⁺-dependent K⁺currents.

Depression of excitatory transmission

The reversible reduction of mEPSC frequency by (1S,3R)-ACPD indicated presynaptic inhibition. Presynaptic inhibition was alsoindicated by the reversible increase in the number of evoked EPSCfailures during (1S,3R)-ACPD application. We believe that thislatter effect represents a reduction in presynaptic release probability,as opposed to a failure to excite premotoneurons. Our conclusionis based on indirect evidence, shown in Figure 5A, that excitabilitywas enhanced by (1S,3R)-ACPD in the majority of excitatorypremotoneurons.

The mean amplitude of unitary evoked EPSCs in trigeminal motoneurons was consistently depressed by (1S,3R)-ACPD. We attributethis depression to presynaptic and postsynaptic effects, becausepresynaptic inhibition reduces the quantal content of evoked synapticevents and AMPA receptor depression reduces the postsynaptic effectivenessof the releasedtransmitter.

In contrast to other reports of solely presynaptic mechanisms for (1S,3R)-ACPD-induced depression of excitatory transmission(Gereau and Conn, 1995; Dong et al., 1996; Zorumski et al., 1996),mGluR activation in trigeminal motoneurons also regulates transmissionpostsynaptically by modulating AMPA receptors. This conclusionis based on the (1S,3R)-ACPD-induced leftward shift of the cumulativeprobability amplitude histogram and the reversible reduction ofAMPA-evoked currents. mGluR-mediated presynaptic inhibition andpostsynaptic regulation of AMPA receptors has been reported, butin contrast to trigeminal motoneurons, AMPA receptor currentswere enhanced in these cells (Glaum and Miller, 1992, 1993; Glaumet al., 1992, 1993). In these neurons, the differential effectsof mGluR activation may sustain the level of excitatory driveby enhancing AMPA receptor currents during presynapticinhibition.

In contrast, in neostriatal cells and trigeminal motoneurons, presynaptic inhibition is coupled with depression of ionotropicglutamate receptors (Lovinger, 1991; Lovinger et al., 1993; Colwelland Levine, 1994; Lovinger and Tyler, 1996). However, in neostriatalneurons, the NMDA receptor is the postsynaptic target of mGluRregulation, as opposed to the AMPA receptor in trigeminal motoneurons.Therefore, mGluR activation in neostriatal neurons (Colwell andLevine, 1994) and trigeminal motoneurons suppresses excitatorytransmission presynaptically and postsynaptically, but by actingat different ionotropicreceptors.

We believe that differential regulation of ionotropic glutamate receptors influences the production of rhythmical jaw movements.In trigeminal motoneurons, non-NMDA receptors primarily mediatefast synaptic potentials evoked in vivo by brief cortical stimulation(Katakura and Chandler, 1990) or reflex activation (Chandler,1989). However, non-NMDA and NMDA receptors are used during corticallyinduced, sustained rhythmical masticatory activity (Katakura andChandler, 1990). This cyclical masticatory drive, recorded invivo in trigeminal motoneurons (Chandler and Goldberg, 1982; Goldberget al., 1982), closely resembles our proposed favored synapticsignal. This, we argue, is a rhythmical signal, composed of manyslow and synchronous synaptic potentials, that recruits both non-NMDAas well as NMDA receptors. Therefore, mGluR activation may helpdiscriminate synaptic noise from fundamental masticatory, or oral-related,motor patterns based on the temporal characteristics of synapticinputs and the ionotropic receptors they preferentially activate.This signal/noise discrimination is achieved postsynapticallyby differentially modulating the ionotropic glutamatereceptors.

When synaptic transmission from trigeminal premotoneurons to motoneurons occurred spontaneously in the absence of TTX, (1S,3R)-ACPDincreased synaptic activity (spontaneous EPSCs) in the majorityof cells. These results imply that the soma-dendritic membranesof most premotoneurons are excited by (1S,3R)-ACPD and overcomepresynaptic inhibition through enhanced spike output. In anothersubset of premotoneurons, spontaneous synaptic activity was reducedby (1S,3R)-ACPD, which we attribute, in part, to presynaptic inhibition.If premotoneuronal mGluRs are endogenously activated during theproduction of jaw movements, then a subset of cells will be excited.Their elevated spike output could be an additional mechanism forsculpting excitatory input to trigeminal motoneurons, favoringinputs with strong modulation (excitation) bymGluRs.

Modulation of intrinsic properties

The final integration of synaptic input is controlled by the intrinsic membrane properties of trigeminal motoneurons. (1S,3R)-ACPDreduced a Ba²⁺-sensitive leakage K⁺ current. Reduction in the leakage current causes depolarizationand increased input resistance in trigeminal motoneurons and otherneurons (McCormick and von Krosigk, 1992; Crépel et al., 1994;Guérineau et al., 1994; Dong et al., 1996; Mercuri et al., 1996).(1S,3R)-ACPD also reversibly induced a sustained outward current,which activated near $-$ 30 mV and was blocked by Cd²⁺. We conclude that mGluR activation caused a transient reductionin a noninactivating high-threshold Ca²⁺ current (Sayer et al., 1992; Swartz and Bean, 1992; Trombleyand Westbrook, 1992; Sahara and Westbrook, 1993; Stefani et al.,1994). The depression of high-threshold Ca²⁺ currents could indirectly suppress Ca²⁺-dependent K⁺ currents in trigeminal motoneurons (Kobayashi et al., 1997).This would increase the excitability of trigeminal motoneuronsby reducing spike afterhyperpolarizations and elevating the frequency-currentrelationship.

These postsynaptic effects of mGluR activation were mediated by a group I or II mGluR because the effects of (1S,3R)-ACPDwere antagonized by the group I/II antagonist MCPG, and the postsynapticeffects of (1S,3R)-ACPD were not mimicked by the selective groupIII agonist L-AP4, even at 200 µM (Fig. 7).

Endogenous activation of mGluRs during jaw movements

Our hypothesis regarding the role of mGluRs in jaw movements requires endogenous activation of the metabotropic receptorsduring oral-motor activity. The evidence suggests that this probablyoccurs. First, trigeminal motoneurons express mGluRs (Turman etal., 1997) and receive glutamatergic input (Turman and Chandler,1994; Appenteng et al., 1995) from rhythmically active premotoneuronsduring masticatory activity (Katakura and Chandler, 1990). Second,high-frequency activity in excitatory synapses causes glutamateaccumulation and endogenous mGluR activation (Scanziani et al.,1997), and the most effective method to evoke rhythmical jaw movementsin vivo is continuous high-frequency stimulation of the masticatorycortex (Dellow and Lund, 1971; Lund, 1976; Nakamura, 1980; Goldberget al., 1982). Last, in vitro, high-frequency activity in excitatorypremotoneurons mimicked exogenous mGluR activation and was antagonizedbyMCPG.

During periods of endogenous mGluR activation, we propose that the presynaptic and postsynaptic regulatory effects of mGluRswork together to discriminate the favored, synchronous synapticsignal from asynchronous synaptic noise and amplify its postsynapticeffectiveness via increased motoneuronal excitability. Thus, mGluRshelp sculpt the final oral-related motor output of trigeminalmotoneurons.

  FOOTNOTES

Received April 3, 1998; revised Aug. 14, 1998; accepted Sept. 9, 1998.

This work was supported by National Institute of Dental Research Grant RO1 DE-06193. We thank Dr. M. Levine for critical readingof this manuscript and Marvin Z. Castillo for technicalcontributions.
Correspondence should be addressed to Dr. Scott H. Chandler, Department of Physiological Science, 2851 Slichter Hall, Universityof California at Los Angeles, Los Angeles, CA 90095-1568.

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