Concurrent Inhibition and Excitation of Phrenic Motoneurons during Inspiration: Phase-Specific Control of Excitability

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The Journal of Neuroscience, March 15, 1999, 19(6):2368-2380

Concurrent Inhibition and Excitation of Phrenic Motoneurons during Inspiration: Phase-Specific Control of Excitability
M. A. Parkis¹, X.-W. Dong², J. L. Feldman³, and G. D. Funk¹
¹ Department of Physiology, Faculty of Medicine and Health Sciences, University of Auckland, Auckland, New Zealand, ² Schering-Plow Research Institute, CNS/CV Research, Kenilworth, New Jersey 07033, and ³ Systems Neurobiology Laboratory, Departments of Neurobiology and Physiological Science, University of California Los Angeles, Los Angeles, California 90095-1763

  ABSTRACT

Top
Abstract
Introduction
References

The movements that define behavior are controlled by motoneuron output, which depends on the excitability of motoneurons andthe synaptic inputs they receive. Modulation of motoneuron excitabilitytakes place over many time scales. To determine whether motoneuronexcitability is specifically modulated during the active versusthe quiescent phase of rhythmic behavior, we compared the input-outputproperties of phrenic motoneurons (PMNs) during inspiratory andexpiratory phases ofrespiration.
In neonatal rat brainstem-spinal cord preparations that generate rhythmic respiratory motor outflow, we blocked excitatoryinspiratory synaptic drive to PMNs and then examined their phase-dependentresponses to superthreshold current pulses. Pulses during inspirationelicited fewer action potentials compared with identical pulsesduring expiration. This reduced excitability arose from an inspiratory-phaseinhibitory input that hyperpolarized PMNs in the absence of excitatoryinspiratory inputs. Local application of bicuculline blocked thisinhibition as well as the difference between inspiratory and expiratoryfiring. Correspondingly, bicuculline locally applied to the midcervicalspinal cord enhanced fourth cervical nerve (C4) inspiratory burstamplitude. Strychnine had no effect on C4 output. Nicotinic receptorantagonists neither potentiated C4 output nor blocked its potentiationby bicuculline, further indicating that the inhibition is notfrom recurrent inhibitory pathways. We conclude that it is bulbospinalinorigin.
These data demonstrate that rapid changes in motoneuron excitability occur during behavior and suggest that integration ofoverlapping, opposing synaptic inputs to motoneurons is importantin controlling motor outflow. Modulation of phasic inhibitionmay represent a means for regulating the transfer function ofPMNs to suit behavioraldemands.

Key words: phrenic motoneuron; brainstem; spinal cord; respiration; GABA; neonatal rat

  INTRODUCTION

Top
Abstract
Introduction
References

Motoneurons shape motor patterns by transforming inputs into appropriate outputs controlling muscle contraction. This transformationof input into output, excitability, is determined by an interactionbetween synaptic inputs and the expression and modulation of intrinsicvoltage- and ligand-gated conductances (Hultborn and Kiehn, 1992).Excitability is not static. It changes over multiple time scales(Feldman et al., 1990), such as during development (Berger etal., 1996) and in transitions between sleep states (Soja et al.,1991; Kubin et al., 1993). Because the output of multiple motoneuronpools must be coordinated to optimize movements for various behaviors,motoneuron properties may also change over faster time scalesto achieve changes in excitability specific to a given behavior(Dickinson, 1995; Krawitz et al., 1997) or to a particular phaseof behavior (Brownstone et al., 1992).

Various mechanisms could underlie such rapid changes in motoneuron excitability. (1) Coactivation of neuromodulatory pathwaysto motoneurons during behaviors is suggested by reductions inaction potential threshold during fictive locomotion (Krawitzet al., 1997) and by monoamine-induced plateau potentials (Hounsgaardet al., 1988; Hounsgaard and Kiehn, 1989; Hultborn and Kiehn,1992). (2) The strength of recurrent inhibitory pathways can bemodulated (Hultborn et al., 1979; Hilaire et al., 1986). (3) Thebalance of concurrent excitatory and inhibitory synaptic inputsmay be adjusted. Indirect evidence for such opposing inputs tohypoglossal motoneurons during inspiration (Withington-Wray etal., 1988; Woch and Kubin, 1995), and evidence for GABAergic gainmodulation of respiratory premotoneurons (McCrimmon et al., 1997),led us to test whether concurrent inhibition and excitation underliephase-specific modulation of motoneuronexcitability.

Determining whether motoneuron excitability is differentially modulated between phases of a behavior requires preparationsexhibiting behavior. Moreover, investigating motoneuron excitabilityduring the active phase of behavior presents a challenge, becausechanges in membrane potential and input resistance produced byexcitatory synaptic drive can mask underlying modulatory effects.For example, increased excitability of lumbar motoneurons duringthe active versus quiescent phase of the fictive locomotor cycle(Brownstone et al., 1992) suggests that activation of centralrhythmic behavioral circuits changes the input-output functionof motoneurons. However, interpretation of these results is confoundedby the presence of ongoing rhythmic locomotor drive potentialsand the associated changes in membrane conductance. In most rhythmicbehaviors, block of these postsynaptic drive potentials to motoneuronswill disrupt generation of behavioral rhythm, due to proximityof the motoneurons to the rhythm-generating circuitry (Robertsonand Stein, 1988; Brownstone et al., 1992).

To address these problems and test for rapid, phase-specific modulation of motoneuron excitability, we used a neonatal ratbrainstem-spinal cord preparation that generates rhythmic inspiratorydrive to motoneurons (Smith and Feldman, 1987). This preparationwas chosen because phrenic motoneurons (PMNs), which drive thediaphragm, are spatially segregated from the rhythm-generatingnetworks that produce their primary behavioral (inspiratory) input,thereby facilitating pharmacological manipulation of fast excitatoryinputs at the motoneuron level without disruption of respiratoryrhythm. In addition, in vitro conditions allow complete blockof excitatory postsynaptic rhythmic drivecurrents.

  MATERIALS AND METHODS

Brainstem-spinal cord preparations. Experiments were performed on brainstem-spinal cord preparations (n = 74) from neonatalWistar rats ranging in age from 0 to 3 d postnatal (P0-P3). Preparationswere isolated using methods previously described for Sprague Dawleyrats (Smith and Feldman, 1987; Dong and Feldman, 1995). Briefly,an animal was anesthetized with diethyl ether and decerebrated,then the brainstem-spinal cord isolated in a dissection chambercontaining artificial CSF (aCSF) containing (in mM): 128 NaCl,3 KCl, 1.5 CaCl₂, 1 MgSO₄, 21 NaHCO₃, 0.5 NaH₂PO₄, 30 D-glucose,pH 7.4, at 20-22°C, oxygenated with 95%O₂/5%CO₂. Preparationsextended from the midpontine level rostrally to the seventh cervicalsegmentcaudally.

After isolation, the brainstem-spinal cord was pinned, ventral surface up, on Sylgard resin in a recording chamber (2 ml volume)perfused with oxygenated aCSF at a flow rate of 2-2.5 ml/min.The pia mater was then removed from the ventral surface of thespinal cord just lateral to midline at the level of the C4 nerveroot to allow introduction of whole-cell recording electrodesinto the PMN column and facilitate drug diffusion. Bath temperaturewas gradually increased to 26-27°C beforerecording.

Extracellular recording of whole-nerve inspiratory activity. Inspiratory motoneuron activity was recorded from the severedends of C1 or C4 cervical roots using suction electrodes (80-100µm internal diameter). In experiments requiring block of glutamatergicdrive to individual PMNs, C4 nerve output was also abolished.Thus C1 nerve output was recorded as an index of respiratory cycletiming. In experiments designed to determine the effect of drugson PMN population output, we recorded from the C4 nerve. Nerverecordings were amplified (50,000 times), bandpass-filtered (0.1-3kHz), full wave-rectified, and integrated using a leaky integrator( $tau$ = 50msec).

Whole-cell recording. Intracellular recordings from PMNs (n = 54) were made using "blind" whole-cell patch-clamp recordingtechniques (Blanton et al., 1989). Patch electrodes (resistance4.0-5.5 M $Omega$ ; 1.5-2 µm tip size) were pulled on a horizontal puller(Sutter Model P-97) from 1.2 mm outer diameter, filamented borosilicateglass (Clark/WPI) and filled with solution containing (in mM):K⁺-gluconate 125, NaCl 5, CaCl₂ 1, HEPES 10, BAPTA 10, ATP (Mg²⁺ salt) 2. Intracellular solution pH was adjusted to 7.2-7.3 with5 M KOH. Signals were amplified and filtered with a patch-clampamplifier (5 kHz Bessel filter, Axopatch 1D; Axon Instruments,Foster City,CA).

Series resistance and whole-cell capacitance were estimated under voltage-clamp conditions by using short voltage pulses (100Hz, $-$ 10 mV, 3.0 msec). Series resistance ranged from 10 to 32M $Omega$ , (mean, 17 ± 6 M $Omega$ ) and was monitored throughout experiments.Data were discarded if series resistance changed between controland test conditions. Voltage-current (V-I) relationships wereobtained in current clamp by applying a series of current steps(500 msec, +50 to $-$ 300 pA). In voltage clamp, current-voltage(I-V) relationships were obtained by applying a series of voltagesteps (+24 to $-$ 36 mV from resting membrane potential). Cell inputresistance (R_N) was calculated from the slope or the inverse ofthe slope of a least squares regression line fitted to V-I orI-V curves, respectively. Rheobase was estimated by increasingthe amplitude of depolarizing square-wave current steps (400-600msec duration) until a single spike waselicited.

Neurons included in the database satisfied criteria described previously for PMNs (Liu et al., 1990; Dong and Feldman, 1995).Briefly, they had resting membrane potentials of $-$ 60 mV or morehyperpolarized, received rhythmic synaptic drive currents/potentialsin phase with inspiratory burst activity on C1 ventral nerve roots,produced action potentials that overshot 0 mV, and were locatedat intermediate laterality 110-260 µm deep from the ventral surfaceat the level ofC4.

Pharmacological substances and application. Drugs that were used included bicuculline methbromide [Research Biochemicals (RBI),Natick, MA; 0.1-1.0 mM], 6-cyano-7-nitroquinoxaline-2,3-dionedisodium (CNQX) (RBI; 0.25-0.5 mM), GABA (Sigma, St. Louis, MO;1 mM), hexamethonium bromide (Serva Feinbiochemica, Heidelberg,Germany; 0.1-0.5 mM), 3-[2-methylphenoxy]-1,2-propanediol (mephenesin)(Sigma; 1 mM), mecamylamine hydrochloride (RBI; 50 µM), (+)-MK-801hydrogen maleate (MK801) (RBI; 0.5-1.0 mM), 5-aminomethyl-3-hydroxyisoxazole(muscimol) (Sigma; 10-100 mM), 1,2,3,4-tetrahydro-6-nitro-2,3-dioxo-benzo[f]quinoxaline-7-sulfonamidedisodium (NBQX) (RBI; 0.375-0.5 mM), strychnine hydrochloride(Sigma; 1 mM), and tetrodotoxin (TTX) (RBI; 0.5-1.0 µM). All drugswere made up in aCSF and stored as frozen aliquots, with the exceptionof hexamethonium, which was made fresh before eachuse.

Drugs were either applied locally over the ventral surface of the C4 spinal cord over the region containing the PMN pool,or added to the bath. Local application of drugs from triple-barreledpipettes (6 µm per barrel outside diameter at the tip) was viatimed pressure injection controlled by solenoidvalves.

Drugs were bath-applied when multisegmental action of a given drug was required (e.g., when we wanted to block recurrent inhibitionthroughout the cervical cord rather than at C4 alone). The recordingchamber was divided into two compartments (split-bath configuration)by construction of a petroleum jelly barrier at the spinomedullaryjunction. This allowed selective application of drugs to the spinalcord aCSF without affecting processes in the brainstem where respiratoryrhythm originates. A minimum of 10 min was allowed for drug equilibration.The split-bath configuration involved analysis of C4 populationoutput only, because the petroleum jelly used for the partitioninterferes with formation of G $Omega$ seals required for whole-cellrecording. The integrity of the partition was tested at the startand the end of each experiment by removing all solution from onecompartment and verifying that no solution leakedthrough.

Neuronal properties during inspiratory and expiratory periods: repetitive firing protocol. The paradigm used to compare repetitivefiring elicited during inspiration with firing elicited betweeninspiratory bursts, which we refer to as expiration, is illustratedin Figure 1. First, C1 ventral root population inspiratory activityand whole-cell recording of PMN inspiratory synaptic inputs wereestablished (see Fig. 1Bi). After inspiratory synaptic inputswere characterized under voltage- and current-clamp conditions,they were blocked via continuous local application of a glutamatereceptor antagonist mixture over the C4 PMN pool until no depolarizationof PMNs was observed concurrent with inspiratory bursts on theC1 nerve (see Fig. 1Bii). The antagonist mixture comprised 0.25-0.5mM CNQX and 0.5 mM MK801, or 0.375 mM NBQX and 0.5 mM MK801, or0.5 mM CNQX, 0.375 mM NBQX, and 0.5 mM MK801. C1 nerve inspiratoryactivity remained unblocked by the glutamate antagonist cocktailbecause of its spatial separation from the site of drug injectionand therefore was used as an index of cycle phase. The risingphase of C1-integrated inspiratory activity elicited a TTL pulsefrom a window discriminator that initiated an eight-cycle seriesof injected current pulse triplets. The first pulse was deliveredduring inspiration; the second and third pulses of equal magnitudewere delivered during the expiratory period (between inspiratorybursts) at 2-4 sec intervals (see Fig. 1Biii). The third pulsewas applied to control for the possibility that accommodativeproperties may have produced different PMN responses to the secondof a pair of identical current pulses independent of any phasicalteration of neuron properties. Temporal characteristics of thesquare-wave pulses were controlled with a Master-8 Stimulator(A.M.P.I., Jerusalem, Israel) and Axodata software. Duration ofthe pulses was varied from 400 to 600 msec to match the durationof the inspiratory phase of the preparation. Injected currentamplitude incremented or decremented with each respiratory cycle(i.e., after one inspiratory and two expiratory pulses), witha total of eight equal steps chosen empirically to produce a rangeof firing frequencies comparable betweenPMNs.

Block of primary excitatory inspiratory synaptic drive was essential for these experiments. (1) It prevented changes in motoneuroninput conductance associated with activation of the ligand-gatedglutamate receptor channels that mediate inspiratory drive (Liuet al., 1990); (2) it removed rapid membrane potential fluctuationsassociated with inspiratory synaptic drive (see Fig. 1Bi), facilitatinganalysis of repetitive firing behavior; and most importantly,(3) it ensured that inspiratory-phase responses were not evokedfrom more depolarized membrane potentials than expiratory-phaseresponses. If excitatory synaptic inputs were not blocked, inspiratory-phaseresponses would be from the summed action of synaptic and injectedcurrents, whereas expiratory-phase responses would represent responsesto injected current only. Thus PMNs were not subjected to therepetitive firing protocol if inspiratory-phase depolarizationswere stillobserved.

Tests for phase-dependent changes in R_N. PMN R_N during inspiratory and expiratory periods was compared, after blockof glutamatergic inputs, from the slope of least squares regressionline fitted through voltage-current relationships generated byplotting the steady-state voltage responses to incrementing ordecrementing current pulses (50 pA steps; $-$ 200 to +50 pA) deliveredduring the inspiratory and expiratory periods. As above, the risingphase of C1 inspiratory activity was used as the index of inspiratoryonset.

Data acquisition and analysis. Signals were displayed on line on a chart recorder and oscilloscope and were recorded on videotapevia pulse code modulation (Vetter 402 or 3000A; A. R. Vetter,Rebersberg, PA) (sampled at 10-40 kHz/channel) for storage andoff-line analysis. Selected portions of data were digitized at1-20 kHz using AxoData software and a National Instruments NBMIO-16A/D board and stored on computer for subsequent analysis. Peaksof EPSPs and IPSPs and of integrated nerve activity were calculatedusing the peak detection analysis in AxoGraph software (version3.0). The effects of bath-applied and locally applied drugs onfrequency and peak amplitude of C4 inspiratory bursts were assessedusing a custom-written LabVIEW acquisition and analysisprogram.

PMNs exhibited a wide range of rheobase, R_N, and maximum firing frequency values. Thus, the absolute magnitude of the eightcurrent pulses injected to examine repetitive firing varied betweenPMNs. Therefore to pool data on firing frequency versus injectedcurrent from different PMNs for statistical analysis, firing frequencywas plotted against the current step number rather than absolutecurrent. Each of the eight steps produced a similar incrementin PMN output relative to maximum firing for thatcell.

Data are reported as mean ± SE. Means of data on C4 burst amplitude and PMN subthreshold properties were compared using atwo-tailed Student's paired t test. An arc sine transform wasperformed to normalize all percentage data before statisticalcomparison. Comparison of PMN firing behavior during the inspiratoryand expiratory phase was made with Statistical Analysis Softwareusing an 8 × 3 or 3 × 3 univariate one-way ANOVA for unbalanceddata sets. Linear contrast coefficients were used to partitionthe sum of squares to determine whether firing was significantlydifferent between inspiration and expiration or between the twoexpiratory pulses. Values of p < 0.05 were assumed to besignificant.

  RESULTS

Behavior of brainstem-spinal cord preparations isolated from P0-P3 Wistar rats was indistinguishable from that of similarpreparations isolated from Sprague Dawley rats [Smith and Feldman(1987); Lin et al. (1990); Dong and Feldman (1995); also see Connellyet al. (1992)]. Preparations produced spontaneous inspiratory-relatedbursts of activity (5-12/min) on ventral cervical nerve roots.Burst envelopes were rapidly incrementing and slowly decrementing(Fig. 1).

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Figure 1. Experimental set-up and protocol for comparison of PMN firing behavior during inspiratory and expiratory phases. A, Schematic of the rhythmically active brainstem-spinal cord preparation showing the configuration of the suction electrode for recording first cervical nerve (C1) activity, the whole-cell recording electrode at the level of the fourth cervical nerve for recording PMN activity, and the triple-barrel drug ejection pipette. B, Rectified, integrated recording of C1 output ( $int$ C₁, top trace) showing population inspiratory activity and whole-cell current-clamp record of a PMN (V_M, middle trace) (i) under control conditions with inspiratory synaptic potential present, (ii) after complete blockade of the PMN excitatory inspiratory input with NBQX and MK801, and (iii) during the repetitive firing protocol in the continued presence of NBQX and MK801. After block of excitatory inspiratory drive to the PMN (Bii), population inspiratory activity on $int$ C₁ was used to trigger injection of square-wave current pulses during inspiration (Biii). Responses of PMNs to current pulses injected during inspiratory and expiratory periods were then compared. C, Expanded versions of voltage traces (V_M) in B, showing the firing responses of the PMN to (i) endogenous inspiratory synaptic input, (ii) a 380 pA pulse delivered during inspiration, and (iii) the same amplitude current pulse delivered during expiration.

PMN properties were also similar to those described previously (Liu et al., 1990; Dong and Feldman, 1995). PMNs received rhythmicsynaptic input (200-1500 pA) in phase with C1 inspiratory nerveactivity, had resting membrane potentials of $-$ 64 ± 1 mV, R_N of79 ± 5 M $Omega$ in control solution (n = 41), and fired repetitivelyin response to square-wave depolarizing current pulses (rheobase,370 ± 210pA).

Repetitive firing is reduced during inspiration versus expiration

To facilitate comparison of repetitive firing behavior of PMNs during inspiration and expiration, excitatory synaptic inputsmediating the inspiratory drive were blocked with local applicationof NBQX or CNQX + MK801 or both. Drugs were applied continuouslyto ensure continued block of excitatory synaptic drive until protocolswere completed. Although 95% of the inspiratory synaptic inputsto PMNs can be blocked by 5-50 µM CNQX (Liu et al., 1990), completeblock of excitatory input required up to 500 µM CNQX or NBQX.MK-801 was included in the antagonist solution to ensure thatall ionotropic glutamatergic receptors were blocked (Greer etal., 1991). Complete block of excitatory drive was determinedby the absence of inspiratory-phase depolarizing inputs to therecorded PMN. Although recent observations suggest a possiblemetabotropic glutamate receptor contribution to the inspiratorydrive to PMNs (Dong and Feldman, 1996), our ability to completelyblock inspiratory-phase depolarization in 32 of 37 PMNs suggeststhat a metabotropic component is not present in all cells, orthat, where present, it was blocked by the high concentrationsof antagonists. Complete block typically took 5-15 min. The antagonistmixture was associated with a 22 ± 4% increase in R_N (to 97 ±6 M $Omega$ ; n =26).

The repetitive firing protocol was completed in 20 of the PMNs in which all inspiratory-phase depolarization was blocked.Visual inspection of the responses revealed a clear reductionin inspiratory-phase firing in 14 PMNs, as shown for one PMN inFigure 2A. In the remaining six PMNs, differences between inspiratoryand expiratory firing responses were not obvious. We comparedfiring frequencies between inspiration and expiration on datapooled from all 20 PMNs and on data from the 14 cells showingobvious reductions in inspiratory-phase firing. Inspiratory-phasefiring was significantly lower than expiratory firing regardlessof whether 20 or 14 cells were used for analysis (see below).Because the 14 PMNs with obvious phase differences in firing mayrepresent a subpopulation of PMNs that receive inspiratory modulation,we report only the quantitative results from analysis of thosecells. Firing frequencies were calculated in two ways. (1) Toquantify the overall response to a current pulse, the number ofaction potentials produced was divided by pulse duration. Thisgave a value for average firing frequency that enabled comparisonof firing between inspiration and expiration at current levelsthat did not produce enough action potentials to calculate a representativeinstantaneous firing frequency. (2) Instantaneous firing frequency,the inverse of the interspike interval duration, was also averagedat the fourth, sixth, and eighth current steps to ensure thataverage and instantaneous firing frequencies responded similarlyto inspiratory and expiratory input.

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Figure 2. PMN excitability is reduced in inspiration relative to expiration. A, Responses of one PMN to four levels of current steps presented during inspiration and at two times during expiration after block of excitatory inspiratory synaptic input. Responses to pulses presented during the inspiratory phase are shown in the left-hand traces (INSPIRATION); responses to pulses presented during the expiratory phase are shown in the middle (EXPIRATION, Pulse 1) and right-hand traces (EXPIRATION, Pulse 2). Pulse amplitude is indicated to the left of each triplet. B, Plot of total pulse firing frequency versus current step number calculated from responses to pulses presented during inspiration (Insp) and at two times during expiration (Exp 1, Exp 2) (n = 14). C, Plot of instantaneous firing frequency versus current step number calculated from responses to the fourth, sixth, and eighth current steps during inspiration (Insp) and at two times during expiration (Exp 1, Exp 2) (n = 14). D, Plot of percentage reduction in inspiratory-phase action potential (AP) output (number of APs relative to expiratory phase discharge) as a function of current step number. E, Plots of interspike interval (ISI) duration versus interval number for repetitive firing in one PMN. Firing was elicited by the sixth (left-hand trace) and eighth (right-hand trace) current steps delivered during inspiration () and by the same current levels at two times during the expiratory phase (Exp 1, $black-triangle$ ; Exp 2, ). Compare with Figure 4C.

The relationship of firing frequency to injected current step was shifted to the right during inspiration (i.e., more currentwas needed to produce a given firing frequency). Thus the overallmean spike frequency during inspiration (15.4 ± 1.1 Hz) was significantlylower than during expiration (17.4 ± 1.1 Hz; n = 14; p < 0.001)(Fig. 2B). Similarly, instantaneous firing frequency was significantlylower during inspiration than during expiration. At the fourth,sixth, and eighth steps, average instantaneous firing frequenciesduring inspiration were 13 ± 1, 22 ± 1, and 28 ± 2 Hz, respectively,versus 16 ± 1, 25 ± 1, and 30 ± 2 Hz during expiration (p < 0.001)(Fig. 2C). Firing frequency responses to pulses delivered earlyand late in expiration were not different at any level of current(p > 0.5) regardless of whether average or instantaneous firingfrequencies were compared (Fig. 2B,C). The reduction in firingwas manifest as one or two fewer action potentials per 400-600msec current pulse, independent of current level. Thus, when expressedin terms of relative change in action potential output, the reductionin inspiratory versus expiratory discharge was greater at thelower firing levels (Fig. 2D). Relative to the expiratory phase,inspiratory firing was reduced by 49 ± 15% and 7 ± 3% for steps1 and 8, respectively (n =14).

Plots of interspike interval duration against time, calculated from the firing responses to square-wave pulses, revealed thatinterspike interval durations increased during inspiration relativeto expiration (Fig. 2E), indicating that excitability is reducedduring the inspiratoryphase.

The reduction in inspiratory firing is caused by phasic inspiratory inhibition

The increase in duration of interspike intervals during evoked repetitive firing in the inspiratory phase indicated that PMNexcitability was decreased during inspiration. Examination ofmembrane potential during the inspiratory phase (after block ofexcitatory synaptic input) revealed that in 16 of the 32 PMNsin which the inspiratory-phase depolarization was completely blocked,a small hyperpolarizing input arrived coincident with inspiratorybursts on the C1 nerve. Ten of the PMNs exhibiting this hyperpolarizationwere among those subjected to the repetitive firing protocol.Of these 10 PMNs, nine showed a clear reduction in inspiratoryfiring. Failure to observe a hyperpolarization in ~50% of thePMNs may reflect that not all PMNs are phasically inhibited orthat where unobserved, the hyperpolarization was masked by incompletelyblocked excitatory drive. The latter possibility was supportedby the finding that blocking the hyperpolarization with bicuculline(100-200 µM) in 10 cells revealed a small (<2 mV) remaining inspiratory-phasedepolarization in four of them (data notshown).

An example of the inspiratory hyperpolarization in one PMN in current clamp is shown in Figure 3A. Hyperpolarizations hadan average duration of 580 ± 97 msec at a membrane potential of $-$ 55 mV. Peak magnitude was dependent on membrane potential, increasingfrom $-$ 0.7 ± 0.1 mV at resting membrane potential ( $-$ 62 mV), to $-$ 1.1 ± 0.4 mV and $-$ 1.5 ± 0.5 mV at $-$ 55 and $-$ 50 mV, respectively(n = 4). The hyperpolarization reversed between $-$ 65 and $-$ 75 mV(Fig. 3A).

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Figure 3. PMNs receive hyperpolarizing input during inspiration. A, Current-clamp recordings from one PMN illustrating the magnitude of the inspiratory hyperpolarization at five different membrane potentials (shown at left of traces). Traces represent averages of five inspiratory cycles. B, Time course of the excitatory (top trace) and inhibitory inspiratory potentials (middle trace) relative to the inspiratory burst recorded from C1 (bottom trace). Traces represent averages of 10 inspiratory cycles. C, The high degree of overlap between these inspiratory excitatory and inhibitory synaptic inputs is demonstrated by inverting and amplifying (8.7 times) the inhibitory input (gray trace) and superimposing it on the excitatory input (thin black trace).

Durations of the inhibitory (580 ± 97 msec) and excitatory (690 ± 66 msec) inputs to PMNs were similar (n = 6), and a rapidlyincrementing, slowly decrementing envelope was common to both.The temporal relationship between excitatory and inhibitory inspiratorysynaptic inputs could not be established directly because theinhibitory input was only visible during block of the excitatoryinput. Instead, the timing of the peak of the excitation, measuredbefore application of glutamate antagonists, and the peak of theinspiratory inhibition, measured after glutamate receptor block,were compared relative to the peak of the C1 ventral root inspiratoryburst. Peaks of the inspiratory synaptic excitation and inhibitionwere thus determined to be nearly coincident, arriving 10 ± 10msec and 34 ± 22 msec (n = 5), respectively, after the peak ofthe C1 nerve inspiratory burst (Fig. 3B).

Not only was its time course similar: the inspiratory inhibition corresponded closely in shape to the inverted excitatorydrive. This is shown for one PMN in Figure 3C where the inhibitorypotential envelope averaged from 10 inspiratory cycles was inverted,scaled (in this case amplified 8.7 times), and superimposed onthe averaged excitatory inspiratory input (before it was blocked)from the same cell. The close correspondence of the relationshipsbetween inhibitory and excitatory synaptic inputs (Fig. 3C) isconsistent with the possibility that inhibitory and excitatorydrives areproportional.

To test whether the inspiratory hyperpolarization was mediated via GABA receptors, we examined the effects of locally appliedbicuculline (GABA_A receptor antagonist; 100-200 µM) on the inspiratory-relatedhyperpolarization. Bicuculline blocked the hyperpolarization inall PMNs tested (n = 11) (Fig. 4A). It also eliminated the differencebetween inspiratory and expiratory firing (Fig. 4B) (n = 3) andblocked the differences between inspiratory and expiratory firingbehavior evident in the plots of interspike interval versus time(Fig. 4C). These data support our hypothesis that the inspiratory-phasehyperpolarization was responsible for reduced firing during theinspiratory relative to the expiratory phase.

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Figure 4. The hyperpolarizing inspiratory inhibition of PMNs and the reduction in PMN firing during inspiration are blocked by bicuculline. A, The same cell as in Figure 3A at $-$ 56 mV. The membrane potential of a PMN during the inspiratory phase, before (CONTROL) and after local application of 200 µM bicuculline (BICUCULLINE). Traces are averages of eight inspiratory cycles. B, Bicuculline (200 µM) blocked the reduction in spike output during inspiration relative to expiration (same cell as in Fig. 2A). C, Bicuculline also blocked the increases in inspiratory interspike interval (same cell and current steps as in Fig. 2E).

GABA receptor activation inhibits PMN excitability

We tested the effects of GABA and muscimol (GABA_A receptor agonist) on PMN properties and repetitive firing behavior to determinewhether their actions supported our hypothesis that the reductionsin inspiratory firing were caused by endogenous activation ofGABA_Areceptors.

GABA (1 mM, applied locally) rapidly (within one inspiratory cycle) and reversibly reduced the number of spikes produced duringthe inspiratory phase (Fig. 5A), completely blocking inspiratory-phasefiring in six of six cells. Similarly, GABA greatly reduced repetitivefiring elicited by current injection (n = 6) (Fig. 5B). This wasnot due to block of cells' ability to fire action potentials,because higher amplitude current pulses still elicited repetitivefiring (data not shown). The associated increase in rheobase didnot appear to be attributable to a change in spike threshold butto a reduction in cell R_N by GABA to 33 ± 8% of control (n = 10)(Fig. 5C,D). The GABA-induced decrease in R_N persisted in TTX(n = 3) (Fig. 5D), suggesting that it is mediated at least inpart by postsynaptic receptors. The effects of GABA were mimickedby the GABA_A receptor agonist muscimol (0.01-1.0 mM), which similarlydecreased R_N to 48 ± 12% of control (n = 4) (Fig. 5C). No consistenteffects on membrane potential were observed in response to GABAor muscimol at resting membrane potential ( $-$ 63 ± 5 mV).

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Figure 5. GABA reduces PMN excitability. A, Current-clamp recording from a PMN before (CONTROL), during (GABA), and after (WASH) local application of GABA (1 mM) over the C4 phrenic motoneuron pool. During GABA application, endogenous excitatory synaptic drive did not elicit action potentials. B, The same PMN as in A, showing that injected current pulses that elicited firing in control did not bring the cell to threshold during GABA application. C, Plot of membrane potential versus injected current for one PMN, showing a decrease in slope of the V-I relationship in the presence of GABA (1 mM, ) or muscimol (0.01 mM, $triangle$ ) relative to control (), indicating a reduction in cell R_N. D, Application of GABA (1 mM) also reduced R_N after block of synaptic transmission with 0.8 µM TTX (different cell than in C).

In keeping with its observed effects on PMN activity, local application of 1 mM GABA over the C4 spinal cord for 10, 30, and60 sec significantly reduced C4 nerve burst amplitude to 40 ±7, 25 ± 7, and 21 ± 7% of control (Fig. 6) (n = 5).

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Figure 6. A, Sixty second application of GABA (1 mM) over the PMN pool nearly abolished $int$ C4 population inspiratory activity in a P1 rat. B, Pooled data showing the dose-dependent reduction in $int$ C4 burst amplitude (expressed as percentage of control amplitude) produced by 10, 30, and 60 sec applications of 1 mM GABA over the C4 motoneuron pool (n = 5; mean ± SE).

Bicuculline potentiates C4 inspiratory activity

To assess the impact of the bicuculline-sensitive inspiratory inhibition of PMNs on inspiratory input to the diaphragm, wemeasured changes in C4 nerve burst activity after locally applyingbicuculline (1 mM) over the C4 PMN pool. Bicuculline (1 mM; 30-60sec) significantly increased C4 nerve burst amplitude by 33 ±9% (Fig. 6) (n = 14; p < 0.05). The bicuculline-induced potentiationpeaked at 1-2 min and returned to control levels 10-15 min afterapplication.

A bicuculline-induced potentiation of C4 burst amplitude could result from block of tonic rather than inspiratory-phase GABA-mediatedinhibition of PMN activity. We therefore examined the effectsof bicuculline on PMN membrane properties and repetitive firingbehavior during expiration. Consistent with a phase-dependent(inspiratory) inhibition, bicuculline (0.2 or 1.0 mM) did notincrease R_N during the expiration (n = 9) (Fig. 7C), nor did italter the relationship between injected current and firing frequency(n = 4) (Fig. 7D,E). Establishing that the potentiation of C4burst amplitude by bicuculline results from block of an inspiratory-phaseinhibition enabled us to later use bicuculline-induced potentiationas an indirect measure of the magnitude of the inspiratory inhibition(Figs. 7, 9, 10).

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Figure 7. Bicuculline increases C4 inspiratory output without changing R_N or firing responsiveness of PMNs during expiration. A, Rectified, integrated C4 nerve recording from a P1 rat showing increased burst amplitude in response to a 60 sec application of bicuculline (1 mM) over the PMN pool (bar under trace). B, Time course of the effects of bicuculline on C4 inspiratory burst amplitude expressed as a percentage of control (n = 5; mean ± SE). C, Bicuculline (0.2-1.0 mM) had no significant effect on R_N of PMNs measured during expiration (n = 10). D, Current-clamp recording from a PMN showing repetitive firing during expiration elicited by current steps injected under control conditions and during local application of bicuculline (1 mM) over the C4 motoneuron pool. E, Plot of firing frequency versus injected current during expiration for a PMN in control () and bicuculline (1 mM, ).

GABA-mediated gain modulation of PMN excitability

The shapes of IPSPs and EPSPs appear similar (Fig. 3). This raises the possibility that the GABA-mediated inhibition providesa means for gain control over PMN output. Gain control is definedas a process whereby the output discharge frequency of a neuron,F_o(t), is the product of its discharge frequency in the absenceof modulation, F_i(t), and a modulation coefficient (1 $-$ $alpha$ ) (McCrimmonet al., 1997). If endogenous GABAergic inhibition decreases gainof the PMN to inspiratory inputs, it would reduce the peak outputof the PMN, reduce the slope of the relation between F_o(t) andF_i(t) below identity, and cause minimal change in burst duration,such that F_o(t) = (1 $-$ $alpha$ ) F_i(t). Blocking this inhibition wouldhave the oppositeeffect.

To test for gain modulation, we examined the effect of bicuculline applied over the PMN pool on C4 nerve inspiratory bursts.We examined C4 output rather than individual PMN output because(1) C4 output provides a reliable estimate of PMN activity, asevident in the close correspondence between the shape of the inspiratorysynaptic drive potential and C4 burst envelope (Fig. 8), and (2)firing of individual PMNs during inspiration was often low, makingit difficult to establish a reliable relationship between dischargeF_o(t) and F_i(t). Thus, we compared voltage of the integrated C4nerve recording during bicuculline (V_(bic)) versus control (V_(con)).Voltage was measured at 25 msec intervals during the decrementingphase of the cycle (Fig. 8A, boxed region). Figure 8A shows thevoltage profile of the integrated C4 nerve burst (averaged from10 cycles) for one preparation before and after bicuculline application.Bicuculline increased the peak C4 burst amplitude (also apparentin Fig. 7). Linear regression indicated that the slope of therelationship between V_(bic) and V_(con) was greater than unity(control) (Fig. 8B). The slope and intercept were 1.47 ± 0.10and 0.20 ± 0.04, respectively (n = 3). Burst duration was notsignificantly affected by bicuculline (673 ± 72 msec in control;714 ± 113 msec in bicuculline). These data suggest that phasicGABAergic input modulates PMN gain during inspiration. Althoughthis may appear inconsistent with the lack of a change in slopein the relationship between firing and injected current step inFigure 2B, a change in slope would not be expected in that relationshipbecause the square-wave pulses used to elicit the firing did notmatch the waveform of the inspiratory inhibition. The proposedgain control arises from the proportionality of the excitatoryand inhibitory inputs.

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Figure 8. GABA-mediated gain modulation of PMN inspiratory activity. A, Superimposed voltage profiles of the integrated C4 nerve inspiratory burst envelopes (averaged from 10 cycles) for one preparation before (Control) and after local application of bicuculline (1 mM) over the C4 PMN pool. Bicuculline increased C4 burst amplitude and the slope of dV/dt, but did not change burst duration. B, Measurements of voltage, taken at 25 msec intervals through the decrementing phase (region enclosed in box) of the control and bicuculline C4 burst envelopes shown in A were used to generate a plot of voltage in bicuculline (V_(bic)) versus control (V_(con)). Linear regression provided estimates of the slope (1.55) and intercept of this relationship and indicated a 1.55-fold increase in gain of the population PMN inspiratory input-output relationship. The line of identity was produced by plotting V_(con) versus V_(con).

Source of inspiratory inhibition

The endogenous GABA-mediated inspiratory inhibition to PMNs had two potential sources: (1) recurrent (feedback) inhibitionarising from PMN activation of Renshaw cells or (2) concurrent(feedforward) inhibition from the brainstem via either directmonosynaptic inhibition of PMNs from bulbospinal inspiratory inhibitoryneurons, or polysynaptic inhibition through activation of GABAergicinterneurons in the spinal cord by bulbospinal inspiratory excitatoryneurons.

Recurrent Inhibition

Recurrent inhibition sometimes has a GABAergic component (Curtis et al., 1976; Cullheim and Kellerth, 1981; Schneider andFyffe, 1992); however, there are no reports of recurrent inhibitionin which glycine does not play a major role. Thus, if recurrentinhibition were the source of the inspiratory hyperpolarization,block of glycine receptors should potentiate C4 inspiratory burstamplitude. Strychnine (1 mM), a glycinergic antagonist, had nosignificant effect on C4 output when applied for up to 2 min (n= 6) (Fig. 9A,B) over the C4 motoneuron pool at the same sitewhere GABA inhibited (Fig. 6), and bicuculline potentiated (Fig.7A,B), C4 inspiratory burst amplitude.

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Figure 9. Renshaw cells do not mediate the bicuculline-sensitive inspiratory inhibition. A, Rectified, integrated record of C4 inspiratory activity from a P1 rat brainstem-spinal cord showing no change in nerve burst amplitude after a 60 sec application of 1 mM strychnine (bar under trace) to the C4 PMN pool. B, Pooled data confirm that strychnine applied to the C4 PMN pool (60 sec starting at t = 0, indicated by bar) had no effect on C4 inspiratory output (n = 6; mean ± SE). C, Addition of mecamylamine (50 µM) to the medium perfusing the spinal cord (split-bath configuration) did not block the potentiation of $int$ C4 inspiratory burst amplitude induced by local application of bicuculline (1 mM, 60 sec) (n = 4; error bars indicate SE). D, Potentiation of C4 burst amplitude induced by local application of bicuculline (60 sec, 1 mM) over the PMN pool (Control) was not affected by addition of mephenesin (1 mM) to the spinal cord bath (n = 5; error bars indicate SE).

Motoneuronal excitation of Renshaw cells, which mediate recurrent inhibition, is largely via nicotinic acetylcholine receptors(nAChRs) (Curtis and Ryall, 1966; Noga et al., 1987). Thus, weused the split-bath configuration to further test for involvementof recurrent inhibitory pathways in producing the inspiratoryinhibition. The nAChR antagonists hexamethonium and mecamylaminewere applied in the spinal bath to determine whether they wouldincrease C4 inspiratory burst amplitude and occlude the bicuculline-mediatedresponse. Hexamethonium (500 µM) had no effect on C4 burst amplitude,nor did it block potentiation of C4 nerve burst amplitude inducedby locally applied bicuculline (1 mM) (n = 2; data not shown).Similarly, C4 burst amplitude was unaffected by application ofmecamylamine (50 µM) to the spinal cord bath. The bicuculline-mediatedpotentiation of C4 burst amplitude was reduced slightly in mecamylamine,from 42 ± 5 to 35 ± 4% (n = 5), but was never abolished (Fig.9C).

Feedforward inhibition from inspiratory-modulated brainstem areas

The minimal change in the C4 inspiratory output after disruption of recurrent inhibitory spinal networks suggested that theinspiratory inhibition originates supraspinally. To test whetherthe inspiratory inhibition of PMN activity was monosynaptic orpolysynaptic (see above), mephenesin was applied to the solutionperfusing the spinal cord (split-bath configuration) to selectivelyblock transmission in polysynaptic versus monosynaptic pathwayswithin the spinal cord (Farkas et al., 1989). Mephenesin (1 mM)reduced C4 output by 30-40% but did not alter the bicuculline-mediatedincrease in C4 burst amplitude (n = 4), which was 28 ± 3% in controland 29 ± 3% in mephenesin (Fig. 9D).

We next tested the hypothesis that the inspiratory inhibition of PMNs originated within the Bötzinger Complex, a region inthe rostral medulla that has widespread inhibitory inputs to manybrainstem and spinal respiratory neurons (Fedorko and Merrill,1984; Merrill and Fedorko, 1984). The brainstem-spinal cord preparationwas pinned onto a paraffin-coated chuck in a vibratome bath, andserial sections (60-100 µm) were removed in the rostrocaudal directionstarting at the caudal pons. The response of C4 inspiratory burstamplitude to local application of bicuculline (1 mM) over C4 wasrecorded after each section. Sections were fixed in 4% paraformaldehydein 0.1 M phosphate buffer and stained with cresyl violet to identifystructures. In the three preparations tested, complete removalof the Bötzinger Complex up to the rostral border of the pre-BötzingerComplex had no effect on the bicuculline-mediated potentiationof C4 burst amplitude. Amplitude potentiation was 51% before and56% after removal of the Bötzinger Complex. Tests of bicucullineresponses after removal of more caudal structures were not performedbecause sectioning of the pre-Bötzinger Complex substantiallyreduced burst amplitude and disrupted respiratory rhythm (Fig.10Biii) (Smith et al., 1991).

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Figure 10. The inspiratory-related inhibition does not arise from structures rostral to the pre-Bötzinger Complex. A, Sagittal view of the brainstem showing levels of transection (dashed lines labeled 1 through 6) taken serially, in relation to organization of ventrolateral brainstem respiratory nuclei. B, Time course of the effects on $int$ C4 inspiratory burst amplitude (in volts) and burst frequency (F) of locally applying bicuculline (60 sec, 1 mM) over the C4 PMN pool after transection of the brainstem at levels 1 (Bi) and 5 (Bii). Individual data points represent amplitude and frequency of single inspiratory cycles. The line in the top panel of Bi represents the moving average of the C4 burst amplitude response to bicuculline applied after transection at level 1. This moving average is included in Bii to illustrate that the effects of bicuculline were unaffected with progressively more caudal transections up to level 5. Removal of the rostral component of the pre-Bötzinger Complex with transection at level 6 disrupted both respiratory rhythm and C4 burst amplitude (Biii), precluding further analysis of responses to bicuculline. BötC, Bötzinger Complex; VII, facial nucleus; XII, hypoglossal nucleus; cNA, compact division of nucleus ambiguus; LRN, lateral reticular nucleus; NA, nucleus ambiguus; Pre-BötC, pre-Bötzinger Complex; rVRG, rostral-ventral respiratory group).

  DISCUSSION

We describe an inspiratory-phase inhibitory input to PMNs that (1) reduces inspiratory output of the C4 nerve, (2) reducesPMN excitability during inspiration relative to expiration, (3)is mediated via GABA_A receptors, (4) is unlikely to arise fromrecurrent inhibitory pathways or from descending inputs from theBötzinger Complex, and (5) is synchronous with, and of similarshape to, the inspiratory excitatory drive to PMNs. We proposethat this concurrent inhibition allows for rapid modulation ofPMNexcitability.

Mechanism of inspiratory inhibition

GABAergic inhibition
Complete block of the inspiratory inhibition by bicuculline in all PMNs tested and reduction of PMN R_N and action potentialdischarge by GABA and muscimol indicate that the inhibition ismediated by GABA_A receptors. Potentiation of C4 inspiratory outputby bicuculline, but not strychnine, further supports the conclusionthat the inhibition is GABA-mediated, with minimal contributionof glycine receptors. The possibility that bicuculline producedits actions through direct effects (i.e., non-receptor-mediated),as reported in cultured mouse neurons (Heyer et al., 1982), isunlikely because bicuculline had no effect on subthreshold propertiesor firing behavior of PMNs during expiration. Our studies didnot establish whether the GABAergic inhibition is presynapticor postsynaptic; however, GABA receptors are present on PMNs (Zhanet al., 1989), and reduction in PMN R_N by GABA [and muscimol (Suand Chai, 1998)] after block of synaptic transmission with TTXis consistent with postsynaptic GABA receptorinvolvement.

Recurrent inhibition
Innervation of Renshaw cells by PMNs and the demonstration of recurrent inhibition of PMNs (Hilaire et al., 1983, 1986; Lipskiet al., 1985) raise the possibility that the inspiratory inhibitionarises from a recurrent inhibitory pathway. However, several linesof evidence argue against this. (1) Glycine is an important transmitterin recurrent inhibitory pathways (Curtis et al., 1976; Cullheimand Kellerth, 1981; Schneider and Fyffe, 1992), yet strychninehad no effect on C4 inspiratory output. (2) Motoneurons activateRenshaw cells primarily via nAChRs (Curtis and Ryall, 1966; Nogaet al., 1987); however, nAChR antagonists neither potentiatedC4 inspiratory burst output nor occluded its potentiation by bicuculline.(3) The inspiratory inhibition was present during prolonged applicationof glutamate receptor antagonists over the C4 motoneuron pool,which would have greatly reduced the number of PMNs capable ofactivating recurrentpathways.

Descending inhibition from the brainstem: concurrent inhibition
Given that recurrent inhibition appears minimal, we propose that the inspiratory inhibition arises from inspiratory-modulatedneurons within thebrainstem.
Direct bulbospinal pathways. Respiratory-modulated bulbospinal inputs to PMNs originate primarily from the Bötzinger Complex,the rostral-ventral respiratory group (rVRG), the dorsal respiratorygroup (DRG) and the raphe obscuris and pallidus (Fedorko and Merrill,1984; Ellenberger et al., 1990a,b; Dobbins and Feldman, 1994).The Bötzinger Complex is unlikely to be the source of the inspiratoryinhibition. Bötzinger Complex neurons provide expiratory- ratherthan inspiratory-phase inhibition to PMNs (Merrill and Fedorko,1984; Milano et al., 1992), and in our study, removal of the BötzingerComplex by serial sectioning was without effect on the bicuculline-mediatedpotentiation of C4 inspiratory burstamplitude.
In rat, the predominant direct inspiratory bulbospinal projection to PMNs originates from the rVRG (Ellenberger and Feldman,1988; Ellenberger et al., 1990b; Saji and Miura, 1990; Dobbinsand Feldman, 1994), with minimal contributions from the DRG (Onaiet al., 1987; Dobbins and Feldman, 1994). Although data indicatethat these projections are primarily excitatory (Ellenberger etal., 1990a; Tian and Duffin, 1996b), they may not be exclusivelyso. Some inspiratory neurons in the rVRG inhibit other respiratoryneurons (Segers et al., 1987; Ezure et al., 1989; Schmid et al.,1996; Ramirez et al., 1997), and a population of inspiratory rVRGneurons may provide inhibitory inputs to PMNs, as suggested bythe presence of a small proportion of symmetrical densities atrVRG-PMN synapses (Ellenberger et al., 1990a). Coactivation ofbulbospinal inhibitory and excitatory premotoneuron pools wouldaccount for the similar time course of inhibitory and excitatorysynaptic inputs we observed inPMNs.
Medullary raphe neurons may also provide the inspiratory inhibition of PMNs. Neurons in the raphe obscuris and pallidus projectto the region of the phrenic nucleus (Holtman et al., 1984; Onaiet al., 1987; Dobbins and Feldman, 1994) and show GAD immunoreactivity(Jones et al., 1991; Holmes et al., 1994) and respiratory-modulatedactivity (Lindsey et al., 1987; Hosagai et al., 1993; Gilbey etal., 1995).
Propriospinal pathways. Inspiratory phase inhibition with a profile similar to the excitatory input could arise polysynaptically.In cat spinal cord, agonist motoneurons and Ia inhibitory interneuronsthat inhibit antagonist motoneurons receive parallel descendingsynaptic drive (Baldissera et al., 1981).
Inspiratory and expiratory interneurons with unknown connectivity are located proximal to the phrenic nucleus in cat (Bellinghamand Lipski, 1990; Grelot et al., 1993) and rabbit (Palisses etal., 1989). A group of interneurons 200 µm from PMNs may be interposedbetween bulbospinal neurons and PMNs (Dobbins and Feldman, 1994).However, a role for either group in mediating the inspiratoryinhibition that we observed is doubtful. Their proximity to thephrenic nucleus means that their inspiratory activation wouldhave been greatly reduced, if not blocked, by local applicationof glutamatergicantagonists.
Contributions from more distant propriospinal inspiratory neurons in the upper cervical cord (Nakazono and Aoki, 1994; Tianand Duffin, 1996a) cannot be ruled out. However, mephenesin, whichpreferentially blocks polysynaptic versus monosynaptic transmission(Farkas et al., 1989), failed to block the bicuculline-inducedpotentiation of C4 burst amplitude when applied to the spinalcord bath, arguing against a propriospinal-mediated inhibitionof PMNactivity.
In summary, we conclude that the inspiratory-phase inhibition of PMNs does not originate from recurrent inhibition at thelevel of the spinal cord or from descending Bötzinger projections.Its proposed bulbospinal origin remains to beverified.

Functional significance of concurrent inhibitory and excitatory inputs

The physiological relevance of the inspiratory inhibition of PMNs is apparent in that blocking it with bicuculline producesan ~30% increase in C4 inspiratory output. This inhibition mayserve a number of functions, as describedbelow.

Competing synaptic drives in the control of motoneuron excitability
Integration of simultaneous excitatory and inhibitory synaptic inputs is important in shaping neuronal discharge patternsat the interneuronal/premotoneuronal level in various motor systems,including respiration (Ballantyne and Richter, 1984; Schmid etal., 1996; Ramirez et al., 1997). GABA receptor-mediated inhibitionof medullary inspiratory neuron discharge during inspiration iswell documented (Wang et al., 1982; Paton and Richter, 1995; Schmidet al., 1996; McCrimmon et al., 1997; Ramirez et al., 1997). Incontrast, at the level of the motoneuron, it is generally heldthat excitatory and inhibitory synaptic inputs arrive alternately,not simultaneously, and thus underlie rhythmic alternation betweenactive and quiescent phases in behaviors including scratching,locomotion, and respiration (Perret, 1983; Merrill and Fedorko,1984; Shefchyk and Jordan, 1985; Robertson and Stein, 1988). Periodsof overlap between inhibitory and excitatory synaptic inputs aretypically brief and presumed to bring about phase transitions.In inspiratory-modulated hypoglossal motoneurons, however, IPSPsarrive concurrently with excitatory inspiratory drive (Withington-Wrayet al., 1988), and R_N is reduced during inspiration (Woch andKubin, 1995). These findings, in conjunction with our observationof simultaneous excitation and inhibition of PMNs during inspirationand observations of large periods of overlap between excitatoryand inhibitory inputs in cat motoneurons during fictive locomotion(Perret, 1986) and in turtle motoneurons during some forms offictive scratch (Robertson and Stein, 1988), suggest that integrationof overlapping opposing synaptic inputs at the level of the motoneuronmay play multiple roles in controlling motor output. It may controlgain, shape discharge pattern, establish recruitment order, orsmooth force production and provide greater flexibility of control(Robertson and Stein, 1998; Feldman and Smith, 1995).

Phase-specific control of motoneuron excitability
Evidence for behavioral- or phase-specific modulation of motoneuron properties is limited. Krawitz et al. (1997) showed thatfiring of lumbar motoneurons is enhanced during all phases offictive locomotion. They suggest that this may result from a locomotion-relatedmodulation of motoneuron excitability, perhaps via a mechanismsimilar to that which underlies bistable behavior [i.e., "plateaupotentials" (see Hultborn and Kiehn, 1992)]. Brownstone et al.(1992) found that motoneuron excitability increases specificallyduring the active phase of the locomotor cycle and attributedthis to a phase-specific reduction in afterhyperpolarization.In our study, block of rhythmic excitatory drive revealed a GABA-mediatedinhibition of PMNs during the inspiratory phase. Relative to othermotoneuron systems with partially overlapping inhibitory and excitatoryinputs (Perret, 1983; Orsal et al., 1986; Robertson and Stein,1988), the unique aspect of the inspiratory-phase inhibition ofPMNs is that its shape and time course match those of the excitatoryinput (Fig. 3). It therefore provides a means for inspiratory-specificgain control of PMN output. Gain control via GABAergic inhibitionmay play a role in controlling the excitability of respiratorypremotoneurons (McCrimmon et al., 1997), where it is proposedto contribute to the optimization of respiratory and nonrespiratorybehaviors. A similar mechanism may operate at the motoneuron level.Inspiratory inhibition may arise from neurons that provide theinterface between respiratory and nonrespiratory behavior (Orem,1989), and modulation of its amplitude may adjust PMN output fromthat optimal for respiration to that suited to other behaviorssuch as apnea, gasping, coughing, vocalization, or defecation(Chang, 1992; Grelot et al., 1992; Gestreau et al., 1996).

  FOOTNOTES

Received Oct. 20, 1998; revised Dec. 28, 1998; accepted Jan. 7, 1999.

This research was supported by grants from the Marsden Fund, the New Zealand Lottery Grants Board, the Health Research Councilof New Zealand, and National Institutes of Health (Grant NS-24742).We thank Ms. C. Walsh, Dr. D. Robinson, and Mr. A. Frankcom-Burgessfor excellent technicalassistance.
Correspondence should be addressed to to Dr. M. A. Parkis, Department of Physiology, Faculty of Medicine and Health Science,University of Auckland, Private Bag 92019, Auckland, NewZealand.

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