Distinct Subtypes of Metabotropic Glutamate Receptors Mediate Differential Actions on Excitability of Spinal Respiratory Motoneurons

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The Journal of Neuroscience, July 1, 1999, 19(13):5173-5184

Distinct Subtypes of Metabotropic Glutamate Receptors Mediate Differential Actions on Excitability of Spinal Respiratory Motoneurons
Xiao-Wei Dong and Jack L. Feldman
Systems Neurobiology Laboratory, Departments of Neurobiology and Physiological Science, University of California, Los Angeles, Los Angeles, California 90095-1763

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Metabotropic glutamate receptors (mGluRs) modulate neuronal function by affecting excitability and altering synaptic transmission.We have shown that the mGluR agonist (1S,3R)-1-amino-1,3-cyclopentanedicarboxylicacid (1S,3R-ACPD) has multiple actions on phrenic motoneurons(PMNs), including reduction of inspiratory-modulated synapticcurrents and an increase of neuronal excitability. We hypothesizedthat these actions were mediated by different mGluR subtypes.We have now identified the involvement of mGluR subtypes and theirroles in modulating the excitability of PMNs and the consequentinspiratory motor output in an in vitro neonatal rat brainstem-spinalcord preparation. Activation of postsynaptic group-I mGluRs increasesPMN excitability, associated with the production of an inwardcurrent and a decrease in membrane conductance, whereas activationof group-II or group-III mGluRs decreases PMN inspiratory-modulatedsynaptic current, probably via a presynaptic mechanism. To confirmfurther the distinction and the involvement of group-I and group-II/-IIIreceptor subtypes affecting PMN excitability, we used the membranepermeable cAMP analog 8-bromo-cAMP (8-Br-cAMP) to elevate intracellularcAMP concentration to mask or occlude any effects mediated viathe cAMP cascade. 8-Br-cAMP attenuated the reduction of the inspiratory-modulatedactivity of PMNs by both (S)-4-carboxy-3-hydroxyphenylglycine(4C3HPG) and L-(+)-2-amino-4-phosphonobutyric acid (L-AP4), agonistsfor group-II and group-III mGluRs, respectively, but did not affectthe actions of 3,5-dihydroxyphenylglycine (DHPG), an agonist forgroup-I mGluRs. These three groups of mGluRs are all endogenouslyactivated during the inspiratory phase. We conclude that threegroups of mGluRs are functionally expressed in the phrenic nucleusand that their activation modulates PMN excitability via distinctmechanisms, with group-I acting at postsynaptic sites and group-IIand group-III acting at presynapticsites.

Key words: metabotropic glutamate receptors; group-I subtype; group-II; group-III; synaptic transmission; presynaptic; postsynaptic; excitability; potassium channels; brainstem; spinal cord; phrenic motoneurons; respiration

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Metabotropic glutamate receptors (mGluRs) modulate neuronal function via affecting excitability and altering synaptic transmission(Schoepp and Conn, 1993; Gallagher et al., 1994; Pin and Duvoisin,1995). The diversity of mGluR actions can be primarily attributedto different receptor subtypes [mGluR1-8 (Pin and Bockaert, 1995)]and their cellular localizations. Group-I mGluRs (mGluR1 and mGluR5)are coupled to phospholipase C and increase the synthesis of inositol1,4,5-trisphosphate (Masu et al., 1991; Abe et al., 1992; Aramoriand Nakanishi, 1992); they can be selectively activated by 3,5-dihydroxyphenylglycine(DHPG) (Schoepp et al., 1994). Group-I mGluRs appear to be localizedpostsynaptically (Martin et al., 1992; Baude et al., 1993; Lujanet al., 1996; Shigemoto et al., 1997) where they act to increaseneuronal excitability (Davies et al., 1995; Netzeband et al.,1997; Schoppa and Westbrook, 1997; Schrader and Tasker, 1997).Group-II (mGluR2 and mGluR3) and group-III (mGluR4 and mGluR6-8)mGluRs are negatively coupled to adenylyl cyclase and inhibitthe formation of cAMP (Tanabe et al., 1992, 1993; Nakajima etal., 1993; Okamoto et al., 1994; Saugstad et al., 1994; Duvoisinet al., 1995). Group-II and group-III receptors are predominantlylocalized in presynaptic terminals (Shigemoto et al., 1995, 1996,1997) where they inhibit transmitter release (Forsythe and Clements,1990; Baskys and Malenka, 1991; Trombley and Westbrook, 1992;Gereau and Conn, 1995; Salt and Eaton, 1995; Vignes et al., 1995;Macek et al., 1996; Schrader and Tasker, 1997).

The physiological roles of mGluR subtypes in identified neurons with measurable behaviors warrant investigation. Althoughthe effects of different mGluRs in single neurons have been extensivelyreported (Poncer et al., 1995; Salt and Eaton, 1995; Macek etal., 1996; Libri et al., 1997; Schoppa and Westbrook, 1997; Schraderand Tasker, 1997), their roles in regulating integrative functionsor in behavior are poorly understood. In this study, we examinethe actions of different mGluRs affecting respiratory motor output,in particular, on phrenic motoneurons (PMNs) that receive inspiratorydrive from the brainstem and control the diaphragm, the principalinspiratory muscle. We performed this study in an in vitro brainstem-spinalcord preparation, in which the transmission of endogenous inspiratorydrive to PMNs is mediated by glutamate acting primarily at non-NMDAreceptors (McCrimmon et al., 1989; Liu et al., 1990; Feldman andSmith, 1994). Thus, we can study mGluR actions at an identified,endogenously driven glutamatergic synapse onto a functionallyidentified neuron participating in a meaningful and measurablebehavior. A broad spectrum mGluR agonist (1S,3R)-1-amino-1,3-cyclopentanedicarboxylicacid (1S,3R-ACPD) reduces inspiratory-modulated synaptic currentsand increases the excitability of PMNs (Dong et al., 1996). Theseactions are mediated by distinct mechanisms at pre- and postsynapticsites. We have now identified the mGluR subtypes underlying theseeffects by examining the actions of specific agonists on endogenousinspiratory-modulated synaptic current, baseline membrane current,and action potential patterns in PMNs. We then examined the effectsof perturbing second messenger pathways associated with group-Iand group-II/-III receptor subtypes. We analyzed the effects ofthese various perturbations on postsynaptic membrane propertiesof PMNs and on the frequency and amplitude of miniature EPSCs(mEPSCs).

Parts of this paper have been published previously (Dong and Feldman, 1995b, 1996).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

En bloc preparation. Experiments were performed on in vitro preparations of brainstem and spinal cord from 0- to 4-d-old neonatalrats. Details of the preparation have been described elsewhere(Smith and Feldman, 1987; Liu et al., 1990; Dong and Feldman,1995a). In brief, the brainstem and cervical spinal cord wereisolated from 0- to 4-d-old Sprague Dawley rats anesthetized withether or hypothermia. The en bloc neuraxis was then pinned downwith the ventral surface upward on Sylgard resin in a recordingchamber and continuously superfused with normal artificial CSF(aCSF) (in mM): 128 NaCl, 3 KCl, 1.5 CaCl₂, 1 MgSO₄, 21 NaHCO₃,0.5 NaH₂PO₄, and 30 D-glucose, equilibrated with 95% O₂/5% CO₂.The bath temperature was gradually raised from 10-15°C (for isolation)to 25-26°C beforerecording.

Electrophysiology. Respiratory activity was recorded with suction electrodes from the C4 ventral root, which contains phrenicmotoneuronal axons, and sometimes simultaneously from cranialnerves (X and XII). Signals were amplified (Grass P511K; GrassInstrument, Quincy, MA), rectified, and low-pass filtered (Paynterfilter; $tau$ = 15msec).

Electrodes for whole-cell patch-clamp recordings were pulled from aluminosilicate glass (A-M Systems, Everett, WA) with atip size of ~2 µm and a resistance of 3.5-5 M $Omega$ when filled withsolution containing (in mM): 120 K⁺-gluconate, 1 CaCl₂, 5 NaCl, 10 HEPES, 2 ATP (magnesium salt),and 10 1,2-bis-(2-aminophenoxy)ethane-N,N,N',N'-tetra-acetic acid(tetrapotassium salt), at pH 7.3 adjusted by KOH. Successful whole-cellrecording was ensured by the initial formation of a gigaohm seal(2-10 G $Omega$ ) and low series resistance (R_S; 8-15 M $Omega$ ). R_S was estimatedusing 100 Hz, $-$ 10 mV, 5 msec voltage pulses. When in voltage-clampmode, a 60-80% R_S compensation was used. During experiments, R_Swas frequently checked, and data were discarded if large increasesoccurred during the course of the recording. PMNs were voltage-clampedat the end-expiratory potentials of $-$ 60 to $-$ 75 mV. Data obtainedfrom PMNs displaying fast Na⁺ currents during inspiration (indicative of poor space clamp)were not included in the analysis. Signals were amplified witha patch-clamp amplifier (AXOPATCH 1D or AXOPATCH 200; Axon Instruments,Foster City, CA) and filtered at 2-5 kHz (Besselfilter).

Current-voltage (I-V) relations were obtained by applying a series of command voltage step pulses (step size, 2-5 mV; width,100-200 msec; frequency, 2 Hz) controlled by software (Axodataor Axoscope; Axon Instruments). I-V curves were obtained by plottingcurrent change (averaged steady-state current values at 5-10 msecbefore offset of voltage step) against membrane potential. Becausemost PMNs did not exhibit slow time-dependent membrane propertiesover the testing voltage range and the membrane current reachedsteady state at 50 msec after the onset of a voltage pulse (Donget al., 1996), steady-state current could be obtained using voltagepulses with widths $>=$ 100 msec. Membrane potentials (V_m)were adjusted for liquid junction potentials ( $-$ 10 mV). Neuroninput conductance (G_N) was calculated at the holding potential( $-$ 60 to $-$ 75 mV) from the slope of a least-squares regression linefitted to thedata.

Neurons subjected to experimental measurements and data analysis satisfied various criteria described previously (Liu et al.,1990; Lindsay and Feldman, 1993). Briefly, these neurons had restingmembrane potentials of at least $-$ 60 mV and displayed rhythmicsynaptic drive currents in synchrony with the inspiratory burstactivity on the C4 ventral root. These neurons were located atintermediate laterality and 130-300 µm below the ventral surfaceat the C4 segment, consistent with the location of the PMN poolin neonatal rats (Lindsay et al., 1991). Axons of these neuronswere contained in the C4 ventral root, indicated by antidromicactivation by stimulating the C4 nerve through the suction electrode.Moreover, their other intrinsic properties, such as input resistance,were consistent with the measurements made in neurons identifiedas PMNs (Smith et al., 1988).

Pharmacological substances and application. The drugs used included (RS)-DHPG (Tocris Cookson, Ballwin, MO; 30-200 µM), (S)-4-carboxy-3-hydroxyphenylglycine(4C3HPG; Tocris Cookson; 30-500 µM), L-(+)-2-amino-4-phosphonobutyricacid (L-AP4; Tocris Cookson; 3-50 µM), (RS)-1-aminoindan-1,5-dicarboxylicacid (AIDCA; Tocris Cookson; 2 mM), (2S)- $alpha$ -ethylglutamic acid(EGLU; Tocris Cookson; 2 mM), (RS)- $alpha$ -methylserine-O-phosphate(MSOP; Tocris Cookson; 1-2 mM), 8-bromo-cAMP (8-Br-cAMP; ResearchBiochemicals, Natick, MA; 0.8-1.2 mM), 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX; Tocris Cookson; 100 µM), (+)-5-methyl-10,11-dihydro-5H-dibenzo[a,d] cyclohepten-5,10-iminemaleate (MK-801; Research Biochemicals;250 µM), and tetrodotoxin (TTX; Sigma, St. Louis, MO; 1 µM).

Experiments were performed while preparations were perfused with normal aCSF solution as described above. Drugs were addedto the spinal cord bath and/or applied locally via a glass pipetteplaced over the midcervical spinal cord region containing thePMN pool. Bath application was used to determine the minimum concentrationsrequired for drug action. With bath application of drugs, thechamber was partitioned into two compartments at the level ofthe spinomedullary junction by a transverse barrier of petroleumjelly (Vaseline) across the neuraxis (Liu et al., 1990). Thisallows selective drug application to the spinal cord to affectsynaptic transmission at the spinal level without disturbing processesat the brainstem level, where the descending inspiratory motordrive originates. Drugs were added to the spinal compartment atconcentrations starting from the minimum necessary to induce aclear change in C4 root activity, and 6-8 min was allowed forequilibrium.

Vaseline often caused difficulty in obtaining good seals for patch recording. Thus, when such recordings were desired, testagents were applied locally in an unpartitioned chamber via pressureejection from single- or multibarrel pipettes positioned closeto the ventral surface of the midcervical spinal cord over thePMN pool (Liu et al., 1990). Each barrel had an orifice of 8-10µm and was filled with a drug solution, saline, or aCSF. Applicationof drugs was controlled by brief air pressure pulses to the appropriatedrug barrel. Control injections were made by ejecting saline oraCSF. The observed change caused by a test drug acting at a spinalsite rather than at a supraspinal site was indicated by unchangedrespiratory rate recorded from the C4 root and unchanged amplituderecorded from cranial nerves (X andXII).

In experiments examining the effect of changing intracellular cAMP concentration on drug action with C4 root recording, bathapplication of 8-Br-cAMP was combined with local application ofan agonist. Thus, after the effect of a locally applied agonistwas examined, 8-Br-cAMP was added to the spinal compartment, andthen the agonist was tested again. The application of 8-Br-cAMPbegan at least 8-10 min before agonist application and continuedduring the agonisttest.

Data acquisition and analysis. Data were recorded on videotape via pulse code modulation (Vetter model 3000; A. R. Vetter,Rebersburg, PA; sampled at 10-40 kHz per channel) for off-lineanalysis. Selected segments of records were digitized at 5-25kHz using an analog-to-digital converter and were stored on aVaxstation 3200 computer disk (Digital Equipment Corporation,Maynard, MA) or on a Pentium computer disk for subsequent computer-aidedanalysis.

For analysis of changes of respiratory drive, the average values of peak amplitude and area of inspiratory-modulated synapticcurrent (charge transfer) or integrated C4 ventral root dischargeswere computed from respiratory cycles before and after drug application.Statistical values are reported as means ± SEM. Differences betweenmeans were assessed by Student's t test, and a value of p < 0.05was consideredsignificant.

For analysis of perturbations of frequency and amplitude of mEPSCs, the data were first filtered using a Wiener (optimal)filter (Press et al., 1989; Barkat, 1991), which greatly attenuatesbackground noise without significantly affecting the characteristicsof the original signal (Liu and Feldman, 1992). Events were detectedusing a threshold detector. Then under visual inspection, eventsabove noise level were collected for data analysis. The reliabilityof detection of unitary events was ensured by a high signal-to-noiseratio (>2.2) (Liu and Feldman, 1992); the amplitudes of mEPSCswere well above noise level in each cell tested. We did not observeany presumptive mEPSCs of size below 2.2 × the mean noise level.We therefore assume that we detected almost all spontaneous EPSCs.To ensure identical voltage control before and after drug treatmentso that the error in amplitude measurement because of inadequatespace clamp would be similar under these two conditions, we monitoredthe series resistance and discarded data if significant increasesoccurred during the course of the recording. All collected EPSCswere then subject to analysis. For each condition, cumulativeprobability distribution histograms for interval and amplitudewere constructed. Statistical significance for the differencebetween distributions was assessed by the Kolmogorov-Smirnov test(Van der Kloot, 1991), and a value of p < 0.05 was consideredsignificant.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Phrenic motoneurons receive rhythmic excitatory inspiratory inputs from bulbospinal inspiratory neurons. Under voltage-clampconditions in the brainstem-spinal cord preparation, PMNs exhibitlarge, fast-rising, and slow-declining EPSCs during the inspiratoryphase of the respiratory cycle (Fig. 1) (Liu et al., 1990; Donget al., 1996). C4 ventral roots, which contain PMN axons, displayspontaneous periodic bursts of discharges representing PMN populationactivity during the inspiratory phase (Fig. 1).

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Figure 1. Effects of the group-I mGluR agonist DHPG on membrane currents of a PMN and the activity in C4 ventral roots. A, Raw traces of simultaneously recorded C4 ventral root activity (C4; top) and membrane current (I_m; bottom) of a PMN showing responses to locally applied DHPG (200 µM; period of DHPG application indicated by the horizontal line). At this concentration, DHPG caused tonic activity in C4 roots. Concurrently, DHPG induced an inward current in the PMN, which was voltage-clamped at the end-expiratory potential (V_h) of $-$ 64 mV. Note that the inspiratory drive current was not significantly affected. B, Superimposed inspiratory drive currents (I_m) and integrated C4 root activity ( $int$ C4) before and during the treatment with a lower concentration (100 µM, local) of DHPG. Inspiratory drive currents were not significantly affected by DHPG. The inspiratory discharges of C4 roots were increased. Traces are averages from six consecutive inspiratory phases in control conditions and during the period of peak effect on C4 activity after drug application. C, Summary of effects of DHPG (100 µM, local) on peak inspiratory drive currents and C4 discharges. Vertical bars are averages from six successive inspiratory phases of peak inspiratory drive currents (left) and integrated inspiratory discharges of C4 ( $int$ C4; right) during peak effect of the drug pooled from eight and six preparations, respectively. Error bars indicate SEM. An asterisk indicates a significant difference (p < 0.05; t test) from control values. Insp, Inspiratory. D, Raw trace showing the persistence of DHPG-induced inward current in a PMN after the bath application of a cocktail containing TTX (1 µM) and ionotropic glutamate receptor antagonists CNQX (100 µM) and MK-801 (250 µM).

Enhancement of excitability of PMNs by group-I mGluRs

To determine the role of group-I mGluRs in affecting PMN excitability, we examined the effect of an agonist for group-I mGluRs,DHPG (Schoepp et al., 1994), on membrane currents of PMNs andon C4 ventral root activity. DHPG (50-200 µM, local) producedan inward current (I_DHPG; 50-200 pA) in all PMNs examined (n =8) when the membrane potentials were clamped at end-expiratorypotentials ( $-$ 60 to $-$ 75 mV; Fig. 1). The inspiratory-modulatedsynaptic currents, however, were not significantly affected (96± 6%; n = 8; Fig. 1A-C). Inspiratory discharges in C4 ventralroots increased at low concentrations of DHPG ( $<=$ 150 µM, local;n = 12; Fig. 1B,C). At 100 µM DHPG (local), the integrated C4root discharge increased to 123 ± 8% of control (n = 6; Fig. 1C).At high concentrations (>150 µM, local), DHPG induced tonic dischargesin the C4 roots (n = 6; Fig. 1A). No changes in respiratory frequency(Fig. 1A) or in inspiratory activity of cranial nerves (X andXII) (data not shown) were observed after local application ofDHPG to the midcervical spinalcord.

The current induced by DHPG could result from actions of DHPG in addition to its presumed effect on postsynaptic group-I mGluRs,including (1) increased activity of spinal interneurons projectingto PMNs and (2) actions mediated by ionotropic GluRs. To elucidatethe mechanisms underlying I_DHPG, we examined the effects of DHPGafter treatment with TTX (1 µM) to block voltage-dependent Na⁺ action potentials and associated synaptic transmission and withMK-801 (250 µM) and CNQX (100 µM), NMDA and non-NMDA receptorantagonists, respectively, to block currents mediated by ionotropicglutamate receptors. Under these conditions, DHPG continued toproduce inward currents (six of six neurons; Fig. 1D), indicatinga direct action on postsynaptic mGluRs ofPMNs.

Suppression of synaptic transmission to PMNs by group-II and group-III

We showed previously (Dong et al., 1996) that simultaneous activation of different mGluR subtypes by 1S,3R-ACPD, a broad-spectrumagonist, affected several currents in PMNs, including the inductionof an inward current and the decrease of inspiratory drive current.Because the above results indicate that group-I mGluRs inducean inward current but do not affect inspiratory drive current,receptors in other groups were candidates for mediating the suppressionof inspiratory drive current. We therefore examined the role ofgroup-II mGluRs by testing the effect of an agonist, 4C3HPG (Birseet al., 1993; Kingston et al., 1995), on PMN membrane currentsand C4 ventral root activity. 4C3HPG decreased inspiratory drivecurrent and spontaneous EPSCs during the expiratory phase (n =7), with no detectable effects on baseline membrane current (Fig.2B). The reductions of peak and total charge transfer of inspiratorydrive current by locally applied 4C3HPG (500 µM) were 53 ± 8 and58 ± 7% of control (n = 7), respectively (Fig. 2C). The effectof 4C3HPG began within one respiratory cycle (<10 sec) after drugapplication and reached peak within 1 min. After washout, theinspiratory drive current returned to the control level within5-8 min (Fig. 2D). Concurrent with the reduction of inspiratorydrive current, a decrease in inspiratory discharges in C4 ventralroots occurred (Fig. 2A). The effect of 4C3HPG on C4 roots hada time course similar to that of the effect on inspiratory currentof PMNs (Fig. 2A).

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Figure 2. Activation of group-II mGluRs depresses synaptic transmission to and output from PMNs. A, B, Local application of the agonist 4C3HPG (500 µM) simultaneously decreased the activity of C4 ventral roots (A) and the inspiratory drive current of a PMN that was voltage-clamped at the end-expiratory potential of $-$ 60 mV (B). Inset, The superimposed traces are averages of six consecutive inspiratory drive currents of a PMN (I_m) and integrated inspiratory discharges of C4 roots ( $int$ C4) in control conditions and during the period of peak effect after drug application. C, Summary of effects of 4C3HPG (500 µM, local) on peak amplitude (Amp) and charge transfer of inspiratory drive currents is shown. Vertical bars are averages of six successive inspiratory drive currents during peak effect of the drug pooled from seven preparations. Error bars indicate SEM. An asterisk indicates a significant difference (p < 0.05; t test) from control values. D, Time course of peak inspiratory drive currents in response to 4C3HPG (500 µM, local) is shown. Each data point is the average of three consecutive peak inspiratory drive currents expressed as the percentage of the control value.

The role of group-III mGluRs was also examined. L-AP4, an agonist for group-III mGluRs (Bushell et al., 1995; Tones et al.,1995), inhibits synaptic transmission to PMNs (Liu et al., 1990).L-AP4 potently reduced the inspiratory current of PMNs (Fig. 3)without any effect on the baseline current. The peak inspiratorycurrent was reduced to 51 ± 6% (n = 6) of control by 50 µM L-AP4.Concurrent with the reduction of inspiratory current of PMNs,a decrease in inspiratory discharges in C4 ventral roots occurredin response to L-AP4 (data not shown). In the presence of MSOP(1 mM, local), an antagonist for group-III mGluRs (Thomas et al.,1996), the effect of L-AP4 was diminished; 50 µM L-AP4 reducedinspiratory current only to 88 ± 7% (n = 6; Fig. 3).

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Figure 3. Activation of group-III mGluRs reduces PMN inspiratory drive currents. A, Locally applied L-AP4 (50 µM) potently reduced inspiratory drive currents. This effect was effectively blocked by the antagonist MSOP. Local application of MSOP (1 mM) began 5 min before L-AP4 (50 µM, local) application and continued during the course of the L-AP4 test. Traces are the averages of six consecutive inspiratory drive currents in each condition. B, Summary of the L-AP4 (50 µM, local) effect on peak inspiratory drive currents with and without concurrent application of MSOP (1 mM, local) is shown. Error bars indicate SEM. An asterisk indicates a significant difference (p < 0.05; t test) from control values. A pound symbol indicates a significant difference (p < 0.05; t test) from values obtained from the L-AP4 condition.

There were no changes in respiratory frequency with either 4C3HPG (Fig. 2) or AP-4 (data not shown) applied locally to thespinalcord.

Effects of elevation of intracellular cAMP on mGluR-mediated actions

The various mGluRs are coupled to different second messenger cascades (Masu et al., 1991; Abe et al., 1992; Aramori and Nakanishi,1992). To confirm further the distinction of the effects on PMNexcitability of group-I and group-II/-III receptor subtypes, weexamined the involvement of specific second messenger pathways.The membrane-permeable cAMP analog 8-Br-cAMP was used to elevateintracellular cAMP concentration so that any effects mediatedvia the cAMP cascade would be masked oroccluded.

In the presence of 8-Br-cAMP (0.8-1.2 mM) in the spinal bath of a partitioned chamber, the ability of both 4C3HPG and L-AP4to reduce inspiratory-modulated activity in the C4 roots was greatlyattenuated (Fig. 4). Thus, 4C3HPG (500 µM) could only reduce C4root discharges to 87 ± 6% (n = 6) of control, compared with 40± 7% before 8-Br-cAMP treatment (Fig. 4A,B), and L-AP4 (50 µM)could only reduce C4 root discharges to 77 ± 7% (n = 6) of control,compared with 42 ± 9% before 8-Br-cAMP treatment (Fig. 4C,D).In contrast, the effect of DHPG was unaffected by 8-Br-cAMP (n= 4), i.e., it continued to elicit tonic discharges in C4 ventralroots (Fig. 5).

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Figure 4. Elevation of intracellular cAMP attenuates the effects mediated by group-II and group-III mGluRs. A, C, Time courses of changes of C4 root inspiratory discharges in response to local application of 4C3HPG (500 µM; A) and L-AP4 (50 µM; C) with and without 8-Br-cAMP (1 mM, bath) treatment. Effects of both 4C3HPG and L-AP4 on inspiratory discharges were significantly attenuated by 8-Br-cAMP. Bath application of 8-Br-cAMP began 8 min before 4C3HPG or L-AP4 application and continued during the course of each agonist's application. Each data point is the average of three consecutive integrated inspiratory discharges expressed as the percentage of the control value. B, D, Pooled data from six preparations showing attenuated effects of 4C3HPG (B) and L-AP4 (D) on C4 root inspiratory activity by 8-Br-cAMP. Error bars indicate SEM. An asterisk indicates a significant difference (p < 0.05; t test) from control values. A pound symbol indicates a significant difference (p < 0.05; t test) from values obtained from the 4C3HPG or L-AP4 condition. CTRL, Control.

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Figure 5. Lack of effect of intracellular cAMP elevation on the effect of group-I mGluR activation. A, Local application of DHPG (200 µM) caused tonic discharges in C4 ventral roots. B, This effect was unaltered by treatment with 8-Br-cAMP. C4, Raw trace of C4 root activity is shown. $int$ C4, Integrated trace of C4 root activity is shown. Protocols described in Figure 4 were used for the 8-Br-cAMP treatment. The horizontal dashed line in B indicates the period of 8-Br-cAMP treatment.

Differential effects of distinct mGluR subtypes on postsynaptic membrane properties

To elucidate the ionic mechanisms underlying the effects on baseline membrane current and inspiratory drive current mediatedby the various mGluR subtypes, we examined the PMN current-voltage(I-V) relationship before and after drug treatment after synapticisolation by TTX (1 µM, bath; Fig. 6).

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Figure 6. Differential effects of distinct mGluR subtypes on postsynaptic membrane properties. A, Membrane I-V relationship before and after application of DHPG (30 µM, bath). The I-V curve was obtained by plotting current changes (averaged steady-state current values at 5-10 msec before offset of voltage step) against membrane potentials. Currents were generated by a series of command voltage pulses. Pulse step size was 5 mV; pulse width was 100 msec; and pulse frequency was 2 Hz. Note that the membrane input resistance increased in the DHPG condition as indicated by the reduced slope of the I-V plot. B, I-V relationship, obtained by subtracting the I-V relationship during DHPG treatment from that in the control condition, for the DHPG-induced inward current (I_DHPG). These experiments were performed in the presence of TTX (1 µM, bath). C, D, Membrane I-V relationships before and after applications of 4C3HPG (50 µM, bath; C) and L-AP4 (5 µM, bath; D).

DHPG increased input resistance, as indicated by the reduced slope of the I-V curve (Fig. 6A). The membrane input resistanceat the resting potential ( $-$ 60 to $-$ 75 mV) increased to 159 ± 8%of control (n = 6) after DHPG treatment (30 µM, bath). The I-Vrelationship for I_DHPG (Fig. 6B) was obtained by subtracting theI-V relationship during DHPG treatment from that obtained undercontrol conditions (Fig. 6A). I_DHPG decreased linearly with hyperpolarizingpotentials (Fig. 6B). A reversal potential of $-$ 102 ± 6 mV forI_DHPG was seen in four of six PMNs within the testing voltagerange ( $-$ 50 to $-$ 120mV).

To examine the possible postsynaptic actions of group-II and group-III mGluRs on PMNs, we also examined the effects of 4C3HPG(n = 5) and L-AP4 (n = 4). In contrast to the group-I agonistDHPG, neither 4C3HPG nor L-AP4 had a significant effect on theI-V relationship over the test voltage range ( $-$ 50 to $-$ 120 mV)(Fig. 6C,D). There was no detectable change in membrane inputresistance after 4C3HPG or L-AP4 (Fig. 6C,D).

Site of mGluR actions affecting inspiratory drive currents

The reduction of the inspiratory drive current of PMNs caused by group-II and group-III mGluR agonists could result from actionseither at presynaptic sites to decrease glutamate release or atpostsynaptic sites to affect the responsiveness of ionotropicglutamate receptors to released glutamate. To investigate theunderlying mechanism(s), we examined the effects of these agonistson the amplitude and frequency of mEPSCs. After treatment withTTX (1 µM, bath), PMNs exhibit spontaneous mEPSCs (Fig. 7A) (Liuand Feldman, 1992; Dong and Feldman, 1995a). These events werecollected from a 20-25 min control period (Fig. 7B, top) and subsequently25-30 min during drug application (Fig. 7B, bottom). The timeinterval between successive mEPSCs and their peak amplitude wereused to construct cumulative interval and amplitude histograms(see Fig. 7C,D).

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Figure 7. Effect of group-II and group-III agonists on mEPSCs in PMNs. A, Raw trace with higher temporal resolution showing typical mEPSCs after bath application of TTX (1 µM). B, Top, Raw trace showing mEPSCs before drug treatment. Bottom, Decrease of mEPSC frequency after 4C3HPG (30 µM, bath) treatment. C, Cumulative (Cum) interval (Intvl) histograms of mEPSCs from the cell represented in B before (1012 events; gray curve) and after (810 events; black curve) bath application of 4C3HPG, which induced a significant (p < 0.01) rightward shift in the cumulative distribution of mEPSC intervals (i.e., a decrease in mean EPSC frequency). D, Cumulative amplitude (Amp) histograms of mEPSCs from the same data sets shown in C. Note that there was no significant (p > 0.05) difference in the amplitude distributions between control and 4C3HPG conditions. Statistical significance for the difference between distributions was assessed by the Kolmogorov-Smirnov test. E, F, Summary of 4C3HPG (E) and L-AP4 (F) effects on the amplitude (Amp) and frequency (Freq) of mEPSCs. Each value (mean ± SEM) was obtained by averaging the percentage changes of mean amplitude or interval (as the reciprocal of frequency) from cells tested with 4C3HPG (30 µM, bath; n = 5) or L-AP4 (5 µM, bath; n = 4). An asterisk indicates a significant difference (p < 0.05; t test) from control values.

The group-II agonist 4C3HPG caused a significant decrease in the frequency of mEPSCs (Fig. 7C). The decrease is indicatedby the shift toward longer values of the interval histogram for4C3HPG compared with the control histogram. In contrast, the amplitudeof mEPSCs was not significantly altered by 4C3HPG, as indicatedby overlapping cumulative amplitude histograms (Fig. 7D). Themean frequency of mEPSCs was 74 ± 11% of control (n = 5) after4C3HPG (30 µM, bath) treatment (Fig. 7E), whereas the mean amplitudeof mEPSCs was not significantly altered (97 ± 9%; n = 5) by 4C3HPG(Fig. 7E).

Similarly, the group-III agonist L-AP4 significantly decreased the frequency of mEPSCs while not affecting their amplitude.The mean frequency of mEPSCs after L-AP4 (5 µM, bath) was reducedto 69 ± 10% (n = 4), whereas the mean amplitude was not significantlyaltered (96 ± 11%; n = 4; Fig. 7F).

Endogenous activation of mGluRs shapes the inspiratory drive to PMNs

To determine the endogenous activation of mGluRs and their physiological roles in synaptic transmission of inspiratory driveto PMNs, we examined the effects of their antagonists. The group-ImGluR antagonist AIDCA, applied locally over the PMN pool (2 mM),significantly (p < 0.01) reduced the peak inspiratory drive current(Fig. 8A,D) to 84 ± 6% (n = 5) of control. Concurrent with thedecrease of PMN inspiratory drive currents, a reduction of C4root activity by AIDCA occurred (data not shown). The effect ofAIDCA began 25-30 sec after the onset of drug application andtook 4-5 min to peak (Fig. 8D). After washout, inspiratory activityreturned to the control level within 10-15 min.

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Figure 8. Endogenous activation of mGluRs during the inspiratory phase revealed by antagonists for different subgroups of mGluRs. A, Attenuation of inspiratory drive current of a PMN by the group-I mGluR antagonist AIDCA (2 mM, local). B, Enhancement of inspiratory drive current of a PMN by the group-II mGluR antagonist EGLU (2 mM, local). C, Increase of inspiratory activity in C4 ventral roots by the group-III antagonist MSOP (2 mM, local). Traces are the averages of six consecutive inspiratory drive currents (I_m; A, B) or six integrated inspiratory discharges in C4 roots ( $int$ C4; C) before and after drug application. D, E, Time courses of changes of inspiratory currents in response to locally applied AIDCA (D) and EGLU (E). Each data point is the average of three consecutive peak inspiratory currents expressed as the percentage of the control value.

In contrast, antagonists for group-II and group-III mGluRs enhanced the inspiratory activity of PMNs. EGLU, an antagonistfor group-II mGluRs, increased inspiratory current in PMNs (Fig.8B,E) and in C4 root activity (data not shown). Locally appliedEGLU (2 mM) increased inspiratory current by 31 ± 7% (n = 5) abovecontrol. The time course of the effect was similar to that ofAIDCA (Fig. 8E). An antagonist for group-III, MSOP, also increasedinspiratory drive current of PMNs (data not shown) and their outputas C4 root activity (Fig. 8C).

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study demonstrates that inspiratory-modulated release of glutamate can activate various subtypes of mGluRs to affectdifferentially the excitability of PMNs. Using specific agonists,we identified mGluR subtypes mediating different effects. We proposethat group-I mGluRs mediate the increase of excitability and thatgroup-II and group-III mGluRs are responsible for the decreaseof synaptictransmission.

Postsynaptic group-I mGluRs mediate an increase in PMN excitability

Activation of group-I mGluRs results in an increase in PMN excitability characterized by enhanced firing in response to inspiratorydrive input. We found that the associated cellular responses,such as the production of an inward current and the increase ininput resistance, persisted when synaptic transmission was blocked;these responses were not associated with any change in synapticcurrent. In addition, these effects were induced only by the agonistfor group-I mGluRs and not by the agonists for the other groups.Taken together, our data suggest that postsynaptic group-I mGluRsmediate the increase of PMNexcitability.

High levels of mGluR1 and mGluR5 mRNA expression are present in rat spinal cord (Valerio et al., 1997). Although there isa lack of information regarding the cellular localization of mGluRsin the phrenic nucleus, in many other brain areas group-I mGluRsare mainly localized postsynaptically (Martin et al., 1992; Baudeet al., 1993; Lujan et al., 1996; Shigemoto et al., 1997), wherethey increase neuronal excitability (Davies et al., 1995; Batcheloret al., 1997; Schoppa and Westbrook, 1997; Schrader and Tasker,1997) consistent with our conclusion that postsynaptic group-ImGluRs increase PMN excitability. Our finding is in agreementwith studies in other brain regions. Activation of postsynapticgroup-I mGluRs increases firing of hypothalamic neurons (Schraderand Tasker, 1997) and induces a depolarization or an inward currentand an associated increase in input resistance in hippocampalCA1 pyramidal neurons (Davies et al., 1995) and olfactory bulbmitral cells (Schoppa and Westbrook, 1997).

The effect of DHPG on PMNs resembles that elicited by 1S,3R-ACPD (Dong et al., 1996), including the production of an inwardcurrent that reverses at a potential close to the estimated E_K⁺ ( $-$ 95 mV) and an associated decrease in membrane conductance.Elevation of extracellular [K⁺] shifts the reversal potential of the 1S,3R-ACPD-induced inwardcurrent (I_ACPD) in the same direction as the E_K⁺ change. In addition, the K⁺ channel blocker Ba²⁺ occludes the effects of 1S,3R-ACPD. We concluded that I_ACPD resultsprincipally from the blockade of a Ba²⁺-sensitive K⁺ conductance (Dong et al., 1996). This mechanism may also underlieDHPG effects because the action of 1S,3R-ACPD and DHPG on thepostsynaptic membrane of PMNs is very likely mediated by the samemGluR group, i.e., group-I, according to the following evidence.(1) The effects produced by 1S,3R-ACPD and DHPG on the postsynapticmembrane of PMNs are quite similar, suggesting that the same signaltransduction mechanisms are involved. (2) DHPG is highly selectivefor group-I over group-II and group-III mGluRs. (3) Although 1S,3R-ACPDcan interact with group-II and/or group-III mGluRs, their agonistsdid not affect postsynaptic membrane properties of PMNs. We concludethat the postsynaptic component of 1S,3R-ACPD actions describedpreviously was mediated via group-I mGluRs. Therefore, we suggestthat blockage of a Ba⁺-sensitive K⁺ conductance mediates the increase in PMN excitability by group-ImGluRs. In addition, changes in some other conductance(s) maybe also involved in group-I mGluR-mediated action [see Dong etal. (1996), their Discussion].

Presynaptic group-II and group-III mGluRs mediate a decrease of synaptic current

Activation of group-II or group-III mGluRs decreased inspiratory drive current in PMNs. This effect was not observed whenthe agonist for group-I mGluRs was applied. To confirm furtherthe involvement of group-II or group-III mGluRs, their secondmessenger pathways were examined. Group-II and group-III mGluRsare linked to cAMP (Tanabe et al., 1992, 1993; Nakajima et al.,1993; Okamoto et al., 1994; Saugstad et al., 1994; Duvoisin etal., 1995), whereas group-I mGluRs are coupled to phospholipaseC (Masu et al., 1991; Abe et al., 1992; Aramori and Nakanishi,1992). Elevation of intracellular cAMP concentration would maskor occlude an effect mediated via cAMP cascades. Pretreatmentwith the membrane-permeable cAMP analog 8-Br-cAMP occluded thereduction of inspiratory drive by agonists for group-II and group-III,confirming that group-II and group-III mGluRs mediate the decreaseof synaptic transmission of inspiratorydrive.

The reduction of inspiratory drive current appears to result from a decrease of transmitter release because of activationof mGluR autoreceptors located at presynaptic terminals of bulbospinalinspiratory neurons onto PMNs. First, our mEPSC analysis showedthat the frequency of mEPSCs was significantly reduced by bothgroup-II and group-III agonists, whereas the mEPSC amplitude wasunaffected. Because mEPSC frequency is dependent on transmitterrelease probability (Fatt and Katz, 1952; Redman, 1990), we assumethat its reduction is a presynaptic action of a group-II or group-IIIagonist to decrease transmitter release from bulbospinal terminalsonto PMNs. On the other hand, changes in mEPSC amplitude couldresult from a postsynaptic action of test drugs to affect thepostsynaptic sensitivity to the endogenously released transmitter(Fatt and Katz, 1952; Redman, 1990; Kullmann and Siegelbaum, 1995).The fact that mEPSC amplitude was unaffected by either group-IIor group-III agonists suggests a lack of their postsynaptic action.Although the origin of these mEPSCs was not identified, it islikely that the presynaptic terminals producing the mEPSCs includethose of bulbospinal inspiratory neurons. Therefore, we extendour conclusion drawn from the mEPSCs to unitary EPSCs comprisingthe endogenous excitatory inspiratory drive current. However,caution must be taken when extrapolating the conclusions frommEPSC analysis of PMNs to inspiratory drive current. One importantdifference between spontaneous mEPSCs and evoked synaptic currentsis that mEPSCs do not require Ca²⁺ influx (Scanziani et al., 1992; Scholz and Miller, 1992), whichmust be considered because activation of presynaptic mGluRs hasbeen postulated to reduce Ca²⁺ influx (Stefani et al., 1994; Glaum and Miller, 1995; Yoshinoand Kamiya, 1995). The reduction in mEPSC frequency we observedindicates that a Ca²⁺-independent mechanism, such as interference with the secretioncascade (Hayashi et al., 1993; Gereau and Conn, 1995; Scanzianiet al., 1995; Tyler and Lovinger, 1995; Schoppa and Westbrook,1997), is involved. Such a mechanism could also attribute, ifnot exclusively, to the inhibition of evoked transmitter release.Regardless of the precise mechanism, the decrease in transmitterrelease from bulbospinal presynaptic terminals by presynapticgroup-II and group-III mGluRs leads to the reduction of inspiratorydrivecurrent.

Second, no alterations in steady-state membrane current or the input resistance of PMNs were produced by the agonist for group-IIor group-III mGluRs, indicating that the decrease of inspiratorydrive current by activation of these receptors is not caused bythe shunting of postsynapticcurrents.

Third, the decrease in synaptic current is most likely caused by direct action of drugs on the synapses of bulbospinal inspiratoryterminals to PMNs rather than by an action on putative spinalinterneurons relaying the descending inspiratory drive to PMNs.Bulbospinal transmission of inspiratory drive to PMNs seems tobe mediated primarily by a monosynaptic pathway (Ellenberger andFeldman, 1988; Berger et al., 1989; Ellenberger et al., 1990;Lipski et al., 1994) and not by spinal interneurons (Davies etal., 1985; Lipski and Duffin, 1986; Palisses et al., 1989; Bellinghamand Lipski, 1990; Grelot et al., 1993) (X.-W. Dong and J. L. Feldman,unpublished observations). In addition, when PMNs were isolatedby TTX, group-II or group-III mGluR agonist continued to affectthe frequency of mEPSCs. Therefore, drug effects seem to be attributableto direct action on impinging presynapticterminals.

In many brain regions, group-II and group-III mGluRs appear predominantly localized in presynaptic terminals (Shigemoto etal., 1995, 1996, 1997). The presynaptic distribution is consistentwith their physiological roles in modulating synaptic transmission.These mGluRs can inhibit transmitter release in areas such asthe hippocampus (Forsythe and Clements, 1990; Baskys and Malenka,1991; Gereau and Conn, 1995; Schrader and Tasker, 1997), thalamus(Salt and Eaton, 1995), hypothalamus (Schrader and Tasker, 1997),olfactory bulb (Trombley and Westbrook, 1992; Schoppa and Westbrook,1997), and trigeminal motor nucleus (Del Negro and Chandler, 1998).We conclude that this is also the case for bulbospinal transmissionof inspiratory drive toPMNs.

Endogenous activity and functional significance of mGluRs

We observed significant changes in the inspiratory-modulated activity of PMNs by antagonists for each of three groups of mGluRs,suggesting endogenous activation of all groups. The reductionof inspiratory drive current by the mGluR1 antagonist AIDCA suggeststhat mGluR1s, in addition to various ionotropic receptors (Liuet al., 1990; Greer et al., 1991), are activated by endogenouslyreleased glutamate during the inspiratory phase and the resultantcurrent contributes to the total inspiratory drive current. ThemGluR1-mediated inward current will produce an incremental increasein the inspiratory-modulated depolarization. The concurrent increasein membrane resistance should also increase this depolarization.Our finding that the EPSCs of PMNs are mediated by glutamate actingat both ionotropic and group-I mGluRs is consistent with observationsin other brain areas. In hippocampal CA3 pyramidal cells, whenthe fast ionotropic response is blocked pharmacologically, stimulationof mossy fibers produces a depolarizing postsynaptic potentialassociated with a decrease in membrane conductance (Charpak andGähwiler, 1991; Gerber et al., 1993). This EPSP is greatly reducedby a mGluR antagonist methyl-4-carboxyphenylglycine (Gerber etal., 1993). mGluR1s also mediate responses of thalamic neuronsto noxious thermal somatosensory stimuli (Salt and Turner, 1998)and EPSPs at parallel fiber-Purkinje cell synapses in the cerebellum(Batchelor et al., 1997).

The enhancement of inspiratory drive current or discharges of PMNs by antagonists for group-II and group-III mGluRs is presumablycaused by the blockade of presynaptic receptors. This findingsuggests that, at least in this in vitro preparation, bulbospinaltransmission is attenuated by endogenous activation of presynapticgroup-II and group-III mGluRs. Such a presynaptic action may providea rapid negative (autoregulatory) feedback to reduce further glutamaterelease under physiologicalconditions.

In summary, three groups of mGluRs are all functionally expressed in the synapses of bulbospinal inspiratory neuron terminalsto PMNs. These receptors are activated during endogenous inspiratorydrive transmission to modulate this process. Along with othermodulatory systems, such as 5-HT (Lindsay and Feldman, 1993) andadenosine (Dong and Feldman, 1995a), different groups of mGluRsfunction to ensure that the synaptic transmission of inspiratorydrive to spinal respiratory motoneurons is well adjusted to producethe appropriate respiratory motor output under widely varyingphysiological conditions with different ventilatorydemands.

  FOOTNOTES

Received Nov. 5, 1998; revised April 2, 1999; accepted April 12, 1999.

This work was supported by the National Institutes of Health Grant NS24742. We thank Dr. Didier Morin for participating inthe early experimentalstudies.
Correspondence should be addressed to Dr. Jack L. Feldman, Department of Neurobiology, University of California, Los Angeles,Box 951763, Los Angeles, CA 90095-1763.

Dr. Dong's present address: Schering-Plough Research Institute, 2015 Galloping Hill Road, Kenilworth, NJ07033.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Abe T, Sugihara H, Nawa H, Shigemoto R, Mizuno N, Nakanishi S (1992) Molecular characterization of a novel metabotropic glutamate receptor mGluR 5 coupled to inositol phosphate/Ca2+ signal transduction. J Biol Chem 267:13361-13368[Abstract/Free Full Text].
Aramori I, Nakanishi S (1992) Signal transduction and pharmacological characteristics of a metabotropic glutamate receptor, mGluR1, in transfected CHO cells. Neuron 8:757-765[ISI][Medline].
Barkat M (1991) In: Signal detection and estimation. Boston: Artech.
Baskys A, Malenka RC (1991) Agonists at metabotropic glutamate receptors presynaptically inhibit EPSCs in neonatal rat hippocampus. J Physiol (Lond) 444:687-701[Abstract/Free Full Text].
Batchelor AM, Knöpfel T, Gasparini F, Garthwaite J (1997) Pharmacological characterization of synaptic transmission through mGluRs in rat cerebellar slices. Neuropharmacology 36:401-403[ISI][Medline].
Baude A, Nusser Z, Roberts JDB, Mulvihill E, Mcilhinney RAJ, Somogyi P (1993) The metabotropic glutamate receptor (mGluR1 $alpha$ ) is concentrated at perisynaptic membrane of neuronal subpopulations as detected by immunogold reaction. Neuron 11:771-787[ISI][Medline].
Bellingham MC, Lipski J (1990) Respiratory interneurons in the C5 segment of the spinal cord of the cat. Brain Res 533:141-146[ISI][Medline].
Berger AJ, Dick TE, Jodkowski JS, Viana F (1989) Phrenic motoneurons: descending inputs, electrical properties, and recruitment. In: Chemoreceptors and reflexes in breathing, cellular and molecular aspects (Lahiri S, Forster II RE, Davies R, Pack A, eds), pp 343-350..
Birse EF, Eaton SA, Jane DE, Jones PL, Porter RH, Pook PC, Sunter DC, Udvarhelyi PM, Wharton B, Roberts PJ (1993) Phenylglycine derivatives as new pharmacological tools for investigating the role of metabotropic glutamate receptors in the central nervous system. Neuroscience 52:481-488[ISI][Medline].
Bushell TJ, Jane DE, Tse HW, Watkins JC, Davies CH, Garthwaite J, Collingridge GL (1995) Antagonism of the synaptic depressant actions of L-AP4 in the lateral perforant path by MAP4. Neuropharmacology 34:239-241[ISI][Medline].
Charpak S, Gähwiler BH (1991) Glutamate mediates a slow synaptic response in hippocampal slice cultures. Proc R Soc Lond [Biol] 243:221-226[Medline].
Davies CH, Clarke VR, Jane DE, Collingridge GL (1995) Pharmacology of postsynaptic metabotropic glutamate receptors in rat hippocampal CA1 pyramidal neurones. Br J Pharmacol 116:1859-1869[ISI][Medline].
Davies JG, Kirkwood PA, Sears TA (1985) The distribution of monosynaptic connexions from inspiratory bulbospinal neurones to inspiratory motoneurones in the cat. J Physiol (Lond) 368:63-87[Abstract/Free Full Text].
Del Negro CA, Chandler SH (1998) Regulation of intrinsic and synaptic properties of neonatal rat trigeminal motoneurons by metabotropic glutamate receptors. J Neurosci 18:9216-9226[Abstract/Free Full Text].
Dong XW, Feldman JL (1995a) Modulation of inspiratory drive to phrenic motoneurons by presynaptic adenosine A1 receptors. J Neurosci 15:3458-3467[Abstract].
Dong XW, Feldman JL (1995b) Differential modulation of synaptic transmission to phrenic motoneurons by metabotropic glutamate receptor subtypes. Soc Neurosci Abstr 21:765.
Dong XW, Feldman JL (1996) Role and mechanism of endogenously activated mGluR1 in modulating synaptic transmission to phrenic motoneurons. Soc Neurosci Abstr 22:598.
Dong XW, Morin D, Feldman JL (1996) Multiple actions of 1S,3R-ACPD in modulating endogenous synaptic transmission to spinal respiratory motoneurons. J Neurosci 16:4971-4982[Abstract/Free Full Text].
Duvoisin RM, Zhang C, Ramonell K (1995) A novel metabotropic glutamate receptor expressed in the retina and olfactory bulb. J Neurosci 15:3075-3083[Abstract].
Ellenberger HH, Feldman JL (1988) Monosynaptic transmission of respiratory drive to phrenic motoneurons from brainstem bulbospinal neurons in rats. J Comp Neurol 269:47-57[ISI][Medline].
Ellenberger HH, Feldman JL, Goshgarian HG (1990) Ventral respiratory group projections to phrenic motoneurons: electron microscopic evidence for monosynaptic connections. J Comp Neurol 302:707-714[ISI][Medline].
Fatt P, Katz B (1952) Spontaneous subthreshold activity at motor nerve endings. J Physiol (Lond) 117:109-128.
Feldman JL, Smith JC (1994) Neural control of respiratory pattern in mammals: an overview. In: Lung biology in health and disease: regulation of breathing (Dempsey J, Pack A, eds), pp 39-69. New York: Dekker.
Forsythe ID, Clements JD (1990) Presynaptic glutamate receptors depress excitatory monosynaptic transmission between mouse hippocampal neurones. J Physiol (Lond) 429:1-16[Abstract/Free Full Text].
Gallagher JP, Zheng F, Shinnick-Gallhager P (1994) Long-lasting modulation of synaptic transmission by metabotropic glutamate receptors. In: The metabotropic glutamate receptors, pp 173-193. Totowa, NJ: Humana.
Gerber U, Lüthi A, Gähwiler BH (1993) Inhibition of a slow synaptic response by a metabotropic glutamate receptor antagonist in hippocampal CA3 pyramidal cells. Proc R Soc Lond [Biol] 254:169-172[Medline].
Gereau IV RW, Conn PJ (1995) Multiple presynaptic metabotropic glutamate receptors modulate excitatory and inhibitory synaptic transmission in hippocampal area CA1. J Neurosci 15:6879-6889[Abstract/Free Full Text].
Glaum SR, Miller RJ (1995) Presynaptic metabotropic glutamate receptors modulate omega-conotoxin-GVIA-insensitive calcium channels in the rat medulla. Neuropharmacology 34:953-964[ISI][Medline].
Greer JJ, Smith JC, Feldman JL (1991) Role of excitatory amino acids in the generation and transmission of respiratory drive in neonatal rat. J Physiol (Lond) 437:727-749[Abstract/Free Full Text].
Grelot L, Milano S, Portillo F, Miller AD (1993) Respiratory interneurons of the lower cervical (C4-C5) cord: membrane potential changes during fictive coughing, vomiting, and swallowing in the decerebrate cat. Pflügers Arch 425:313-320[ISI][Medline].
Hayashi Y, Momiyama A, Takahashi T, Ohishi H, Ogawa-Meguro R, Shigemoto R, Mizuno N, Nakanishi S (1993) Role of a metabotropic glutamate receptor in synaptic modulation in the accessory olfactory bulb. Nature 366:687-690[Medline].
Kingston AE, Burnett JP, Mayne NG, Lodge D (1995) Pharmacological analysis of 4-carboxyphenylglycine derivatives: comparison of effects on mGluR1 alpha and mGluR5a subtypes. Neuropharmacology 34:887-894[ISI][Medline].
Kullmann DM, Siegelbaum SA (1995) The site of expression of NMDA receptor-dependent LTP: new fuel for an old fire. Neuron 15:997-1002[ISI][Medline].
Libri V, Constanti A, Zibetti M, Postlethwaite M (1997) Metabotropic glutamate receptor subtypes mediating slow inward tail current (IADP) induction and inhibition of synaptic transmission in olfactory cortical neurones. Br J Pharmacol 120:1083-1095[ISI][Medline].
Lindsay AD, Feldman JL (1993) Modulation of respiratory activity of neonatal rat phrenic motoneurones by serotonin. J Physiol (Lond) 461:213-233[Abstract/Free Full Text].
Lindsay AD, Greer JJ, Feldman JL (1991) Phrenic motoneuron morphology in the neonatal rat. J Comp Neurol 308:69-79.
Lipski J, Duffin J (1986) An electrophysiological investigation of propriospinal inspiratory neurons in the upper cervical cord of the cat. Exp Brain Res 61:625-637[Medline].
Lipski J, Zhang X, Kruszewska B, Kanjhan R (1994) Morphological study of long axonal projections of ventral medullary inspiratory neurons in the rat. Brain Res 640:171-184[ISI][Medline].
Liu G, Feldman JL (1992) Quantal synaptic transmission in phrenic motor nucleus. J Neurophysiol 68:1468-1471[Abstract/Free Full Text].
Liu G, Feldman JL, Smith JC (1990) Excitatory amino acid-mediated transmission of inspiratory drive to phrenic motoneurons. J Neurophysiol 64:423-436[Abstract/Free Full Text].
Lujan R, Nusser Z, Roberts JD, Shigemoto R, Somogyi P (1996) Perisynaptic location of metabotropic glutamate receptors mGluR1 and mGluR5 on dendrites and dendritic spines in the rat hippocampus. Eur J Neurosci 8:1488-1500[ISI][Medline].
Macek TA, Winder DG, Gereau IV RW, Ladd CO, Conn PJ (1996) Differential involvement of group II and group III mGluRs as autoreceptors at lateral and medial perforant path synapses. J Neurophysiol 76:3798-3806[Abstract/Free Full Text].
Martin LJ, Blackstone CD, Huganir RL, Price DL (1992) Cellular localization of a metabotropic glutamate receptor in rat brain. Neuron 9:259-270[ISI][Medline].
Masu M, Tanabe Y, Tsuchida K, Shigemoto R, Nakanishi S (1991) Sequence and expression of a metabotropic glutamate receptor. Nature 349:760-765[Medline].
McCrimmon DR, Smith JC, Feldman JL (1989) Involvement of excitatory amino acids in neurotransmission of inspiratory drive to spinal respiratory motoneurons. J Neurosci 9:1910-1921[Abstract].
Nakajima Y, Iwakabe H, Akazawa C, Nawa H, Shigemoto R, Mizuno N, Nakanishi S (1993) Molecular characterization of a novel retinal metabotropic glutamate receptor mGluR6 with a high agonist selectivity for