Role of Inspiratory Pacemaker Neurons in Mediating the Hypoxic Response of the Respiratory Network In Vitro

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The Journal of Neuroscience, August 1, 2000, 20(15):5858-5866

Role of Inspiratory Pacemaker Neurons in Mediating the Hypoxic Response of the Respiratory Network In Vitro
Muriel Thoby-Brisson and Jan-Marino Ramirez
Department of Organismal Biology and Anatomy, Committee on Neurobiology, The University of Chicago, Chicago, Illinois 60637

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In severe hypoxia the breathing frequency is modulated in a biphasic manner: an initial increase (augmentation) is followedby a depression and cessation of breathing (apnea). Using a mouseslice preparation that contains the functional respiratory network,we aimed at identifying the neurons responsible for this frequencymodulation. Whole-cell patch recordings revealed that expiratoryneurons become tonically active during anoxia, indicating thatthese neurons cannot be responsible for the respiratory frequencymodulation. Inspiratory neurons tended to depolarize (by 6.9 mV;n = 9), and the frequency of rhythmic activity was significantlyincreased during anoxia (from 0.16 to 0.4 Hz; n = 9). After theblockade of network activity with 6-cyano-7-nitroquinoxaline-2,3-dione,most inspiratory neurons became tonically active (72%; n = 25,non-pacemaker). In anoxia, the membrane potential of these non-pacemakerneurons did not change ( $-$ 0.26 mV; n = 6), and their tonic activityceased. Only a subpopulation of inspiratory neurons remained rhythmicallyactive in the absence of network activity (pacemaker neurons,28%, 7 of 25 inspiratory neurons). In anoxia two subgroups ofpacemaker neurons were differentiated; one group showed a transientincrease in the bursting activity, followed by a decrease andcessation of rhythmic activity. These neurons tended to depolarize(by 10.3 mV) during anoxia. The second group remained rhythmicduring the entire anoxic exposure and exhibited no depolarization.The time course of the frequency modulation in all pacemaker neuronsresembled that of the intact network. We conclude that pacemakerneurons are primarily responsible for the frequency modulationin anoxia and that in the respiratory network there is a strictseparation between rhythm- and pattern-generatingmechanisms.

Key words: pacemaker neurons; hypoxic response; respiratory; apnea; augmentation; anoxia

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The mammalian respiratory system responds to severe hypoxia (anoxia) in a biphasic manner (Lawson and Long, 1983; Bureau etal., 1984; St. John and Bianchi, 1985; Richter et al., 1991; Haddadand Jiang, 1993). An initial increase in the breathing frequency(augmentation) is followed by a frequency decline (depression)and a complete cessation of respiratory activity (apnea). Thecharacterization of the activity of respiratory neurons withinthe medulla revealed an unexpected finding. Despite the pronouncedfrequency increase, a significant proportion of bulbospinal neuronsshowed no change or even a decline in their spiking activity duringhypoxia. Only a few neurons in the ventral respiratory group (VRG)increased their activity (St. John and Wang, 1977; St. John andBianchi, 1985). Similarly, in chemodeafferented animals, as wellas in the brainstem-spinal cord preparation, many inspiratoryand expiratory VRG neurons ceased their activity during augmentation(Richter et al., 1991; Ballanyi et al., 1994; England et al.,1995). This was surprising because it is generally believed thatthe VRG contains the rhythm-generating neural network. These findingssuggest that the initial frequency augmentation is not causedby a general excitation of the entire respiratory network. However,the mechanisms underlying the frequency increase remainunresolved.

An important step toward a more rigorous cellular analysis of the hypoxic response was the demonstration that the respiratorynetwork isolated in a medullary slice preparation still respondsto anoxia with an initial augmentation of respiratory frequencyfollowed by a depression and apnea (Ramirez et al., 1997, 1998;Telgkamp and Ramirez, 1999). This slice preparation contains thepre-Bötzinger complex (PBC), a VRG region that is essential forrespiratory rhythm generation (Smith et al., 1991; Schwarzacheret al., 1995; Koshiya and Guyenet, 1998; Ramirez et al., 1998).Neurons that are activated in phase with XII and VRG populationactivity are inspiratory neurons. Neurons that are inhibited duringVRG activity are expiratory neurons. In the absence of synapticinhibition, expiratory neurons discharged tonically or in phasewith inspiratory activity (Ramirez and Richter, 1996; Ramirezet al., 1997; Shao and Feldman, 1997). These findings suggestthat respiratory rhythm generation originates from rhythmic inspiratoryactivity, which is derived from a subpopulation of inspiratoryneurons with pacemaker properties (Smith et al., 1995). Pacemakerneurons that could contribute to this activity have been identifiedin the respiratory network (Smith et al., 1991; Johnson et al.,1994; Koshiya and Smith, 1999). It has been proposed that theendogenous rhythmicity in pacemaker neurons is synchronized viaglutamatergic [6-cyano-7-nitroquinoxaline-2,3-dione (CNQX)-sensitive]mechanisms and transformed in the presence of synaptic inhibitioninto the respiratory rhythm, which consists of inspiration andexpiration (Johnson et al., 1994; Smith et al., 1995; Reklingand Feldman, 1998; Butera et al., 1999a,b; Koshiya and Smith,1999).

In this study we examined the hypothesis that the anoxia-induced frequency increase is attributable to a specific activationof pacemaker neurons. To test this hypothesis, we compared theanoxic effect on the activity of respiratory neurons in the presenceand absence of network activity. We demonstrate that after isolationfrom the network all pacemaker neurons exhibited an increase inbursting frequency. In contrast, pharmacologically isolated non-pacemakerneurons became rapidly inactive in anoxia. We conclude that pacemakerneurons are primarily responsible for the generation of the anoxicaugmentation in respiratoryactivity.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of slices. Experiments were performed on male and female mice (6-13 d old) that were deeply anesthetized withether and decapitated at the C3-C4 level. The procedure will besummarized only briefly here (for details, see Ramirez et al.,1996). The brainstem was isolated in an ice-cold artificial CSF(ACSF) bubbled with carbogen (95% oxygen and 5% CO₂). The ACSFcontained (in mM): 128 NaCl, 3 KCl, 1.5 CaCl₂, 1 MgSO₄, 24 NaHCO,0.5 NaH₂PO₄, and 30 D-glucose, pH of 7.4. The brainstem was thenglued onto an agar block with its rostral end up and mounted intoa vibratome. Thin slices were serially sectioned from rostralto caudal until the rostral boundary of the PBC became visible.This area was recognized by specific landmarks such as the inferiorolive, the nucleus ambiguus, and the hypoglossal nucleus (XII)(Fig. 1). Slices that contained the PBC (500-600 µm thick) wereimmediately transferred into a recording chamber and maintainedat a temperature of 29°C. After 30 min the potassium concentrationwas raised from 3 to 8 mM over another 30 min to obtain spontaneousrhythmic activity. Anoxia was induced by switching the gas usedto bubble the incoming ACSF from carbogen to nitrogen (95% N₂-5%CO₂). In all of the experiments, anoxic conditions were maintainedfor 4 min.

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Figure 1. Experimental model and cellular recordings of respiratory neurons. Left panel, Schematic representation of a brainstem slice preparation obtained from mice. This slice contains the pre-Bötzinger complex (PBC), the hypoglossal nucleus (XII), the inferior olive (IO), the nucleus ambiguus (NA), the nucleus tractus solitarius (NTS), and the spinal trigeminal nucleus (Sp5). Extracellular population recordings of respiratory activity from the PBC (PBC int: integrated trace) were obtained simultaneously with intracellular recordings from an expiratory neuron (middle panel) or inspiratory neuron (right panel).

Recordings. Extracellular recordings were obtained with suction electrodes placed on the surface of the PBC. The signal thatwas collected was amplified 2000 times, filtered (low-pass 1.5kHz, high-pass 250 Hz), rectified, and integrated using an electronicfilter (time constant 30-50 msec). Integrated population activityfrom the PBC is in phase with integrated XII activity (Telgkampand Ramirez, 1999). Therefore, we will use this extracellularlyrecorded PBC activity as a marker for inspiratory population activity(Fig. 1).

Intracellular patch-clamp recordings were obtained from PBC neurons with the blind-patch technique. Respiratory neurons wereidentified according to their anatomical location (Fig. 1) andwith respect to their discharge characteristics in relation tothe population respiratory activity. Inspiratory neurons wereactivated in phase with population activity (Fig. 1, right panel).Expiratory neurons were activated out of phase with populationactivity (Fig. 1, middle panel). The recordings were obtainedusing patch electrodes manufactured from borosilicate glass tubescontaining a filament (Clarke GC 150TF) filled with a solutioncontaining (in mM): 140 K-gluconic acid, 1 CaCl₂*6H₂O, 10 EGTA,2 MgCl₂*6H₂O, 4 Na₂ATP, 10 HEPES. The recorded membrane potentialswere corrected for junctional potentials as described by Neher(1992). All recordings were stored with a personal computer onAxotape (Version 2.0, Axon Instruments). All substances were obtainedfrom Sigma (St. Louis, MO), except for CNQX (Tocris, Ballwin,MO). CNQX was diluted in ACSF and bath-applied at the final concentrationof 20 µM.

Graphs containing population data were obtained by measuring in individual slices for each experiment the mean values forinspiratory frequency, action potential (AP) frequency, and/orthe amplitude of phasic synaptic inhibition. The mean values wereobtained by averaging each parameter during consecutive respiratorycycles over a period of 10 sec. The mean values obtained fromdifferent individual slices for any given experiment were averagedand used for the finalgraph.

Statistical values are given as mean value ± SEM. Significance was assessed with the one-way ANOVA test; values were assumedto be significant at p < 0.05.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Anoxic response of expiratory neurons in the intact network

As described previously (Ramirez et al., 1998; Telgkamp and Ramirez, 1999), anoxia caused an initial increase in the frequencyof rhythmic population activity (augmentation) (Figs. 2A, toptrace, 3A). This frequency increase was accompanied by a gradualcessation of spiking activity of expiratory neurons (Figs. 2A,bottom trace, B, 3B) and a gradual suppression of synaptic inhibitionreceived by expiratory neurons (Figs. 2A, bottom trace, B, 3C).During the depression period there was no tonic activity in threeof nine expiratory neurons.

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Figure 2. Anoxic response of an expiratory neuron in the intact network. A, Simultaneous recording of integrated population activity from the PBC (top trace) and an expiratory neuron during anoxia (bottom trace). The top gray bar represents the time of the anoxic exposure. Action potentials have been truncated to better illustrate the anoxic suppression of phasic synaptic inhibition (fast downward deflections). The large inspiratory burst generated during anoxia represents a sigh burst, which is followed by a brief burst of apnea. This activity has been characterized by Lieske et al. (2000). B, The three examples were obtained at the times indicated by 1, 2, and 3 in A. The examples shown in an extended time scale represent control conditions obtained at time 20 sec (1), the anoxic augmentation obtained at time 90 sec (2), and the depression period obtained at time 150 sec (3). The action potentials were not truncated in these recordings. Recordings were obtained from an 8-d-old animal.

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Figure 3. Graphs representing the changes induced by anoxia in respiratory frequency (A), action potential frequency in expiratory neurons (B), and the amplitude of the phasic inhibition of expiratory neurons (C) over time. The left panels represent measurements obtained from the same neuron illustrated in Figure 2. The right panels represent pooled data obtained from six different experiments. Time 0 was set at the onset of anoxia exposure. Data were obtained from 7- to 13-d-old animals.

A quantitative analysis of nine expiratory neurons revealed a slight depolarization during anoxia (by 1.5 ± 0.9 mV); however,the average membrane potential measured for nine expiratory cellsdid not significantly change from $-$ 62 ± 1.6 mV under control conditionsto $-$ 60 ± 1.9 mV (p > 0.05) during the anoxic augmentation andthen to $-$ 61.1 ± 1.8 mV (p > 0.05) during depression. These membranepotential values were determined during the expiratory periodsat the time of the maximal augmentation and the maximal depression,as was evident in the maximal and minimal frequency of respiratoryrhythmic activity. The anoxia-induced depolarization was not accompaniedby an increase in spiking frequency. Instead, expiratory neuronsshowed a significant decrease in the rate of AP generation from10.44 ± 1.53 Hz under control conditions to 7.22 ± 0.7 Hz (p >0.05) during the anoxic augmentation, and to 1.46 ± 0.6 Hz (p< 0.01) during the depression period. The AP frequency was measuredduring four consecutive expiratory periods in control conditionsand during the anoxic augmentation and depression. The amplitudeof the phasic inhibition decreased from $-$ 6.9 ± 1 mV in controlconditions to $-$ 5.2 ± 1.5 mV (p > 0.05) during the maximal augmentationand to $-$ 0.5 ± 0.3 (p < 0.01) during the maximal depression. Tobetter illustrate the time course of these changes, we obtainedthe mean respiratory frequency (Fig. 3A, right panel), the meanAP frequency (Fig. 3B, right panel), and the mean amplitude ofphasic inhibition (Fig. 3C, right panel) for consecutive intervalsof 10 sec. Figure 3, left panels, shows the time course obtainedfrom one individual expiratory neuron (the same neuron as illustratedin Fig. 2); the right panels show the time course averaged fromsix recordings of expiratoryneurons.

Anoxic response of inspiratory neurons in the intact network

We also examined the anoxic response of inspiratory neurons. Nine inspiratory neurons were analyzed using the same procedureas described for the expiratory neurons. During the anoxic augmentation,inspiratory neurons tended to depolarize but remained rhythmicallyactive (Fig. 4A,B2). During the depression phase, inspiratoryneurons discharged sporadically with weak (amplitude of the oscillation<20% of the control bursts) and rare bursts (Fig. 4B3). Six ofnine inspiratory neurons became inactive during this phase. Figure4C illustrates the time course of the instantaneous inspiratorybursting frequency for the same neuron shown in Figure 4A. Thetime course averaged from seven neurons is illustrated on Figure4D; C and D were obtained as described for the expiratory neuronsand demonstrate a biphasic frequency modulation in response toanoxia.

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Figure 4. Anoxic response of inspiratory neurons in the intact network. A, Simultaneous recording of integrated population activity from the PBC (top trace) and an inspiratory neuron during anoxia (bottom trace). The top gray bar represents the time of the anoxic exposure. B, The three examples were obtained at the times indicated by 1, 2, and 3 in A. The examples shown in an extended time scale represent control conditions at time 20 sec (1), the anoxic augmentation at time 90 sec (2), and the anoxic depression at time 150 sec (3). As in Figure 2, the large inspiratory bursts represent in vitro sighs. C, Instantaneous inspiratory frequency plotted against time obtained from the recording illustrated in A. Time 0 is set at the onset of anoxia. The filled squares represent strong inspiratory bursts; open squares represent weak inspiratory bursts. Recordings obtained from a postnatal day 8 (P8) animal. D, Mean plot of the instantaneous inspiratory frequency versus time obtained from seven neurons. Data were obtained from 6- to 13-d-old animals.

The anoxic response was quantified for nine inspiratory neurons. The most hyperpolarized membrane potential values that weregenerated after each inspiratory burst were measured both in controland under anoxic conditions. The average amplitude of the anoxia-induceddepolarization was 6.8 ± 1.7 mV. The membrane potential mean valuetended to depolarize from $-$ 62.5 ± $-$ 1.7 mV in control to $-$ 55.6± 3 mV (p > 0.05) during the maximal augmentation and to $-$ 57.6± 1.5 mV (p > 0.05) during the maximal depression phase. Bothburst duration and intraburst AP frequency were altered duringanoxia. The burst duration decreased from 0.82 ± 0.04 sec undercontrol conditions to 0.74 ± 0.04 sec (p > 0.05) during the maximalaugmentation and to 0.23 ± 0.04 sec (p < 0.01) during the maximaldepression. The intraburst frequency of AP decreased from 38.1± 2.4 Hz under control conditions to 33.09 ± 2.5 Hz (p > 0.05)during the maximal augmentation and to 11.96 ± 2.2 Hz (p < 0.01)during the maximaldepression.

Blockade of respiratory network activity reveals pacemaker and non-pacemaker inspiratory neurons

To assess more directly the anoxic effect on individual respiratory neurons, we blocked glutamatergic synaptic activity withCNQX, which eliminated rhythmic population activity. In the absenceof respiratory network activity, 18 of 25 inspiratory neuronsceased to discharge rhythmically and became tonically active.These neurons are referred to as non-pacemaker neurons (Fig. 5A).In contrast, seven inspiratory neurons remained rhythmically activein the absence of respiratory network activity. These neuronsare referred to as pacemaker neurons according to Koshiya andSmith (1999) (Fig. 5B).

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Figure 5. Blockade of respiratory network activity reveals non-pacemaker and pacemaker inspiratory neurons. A1, B1, Two examples of inspiratory neurons recorded simultaneously with integrated population activity from the PBC in control conditions. A2, B2, After elimination of network activity by blocking glutamatergic synaptic transmission with CNQX (20 µM), the non-pacemaker neuron became tonically active (A2), whereas pacemaker neuron remained rhythmically active (B2). Recordings were obtained from P9 and P7 animals, respectively.

Anoxic response of non-pacemaker inspiratory neurons

Six of 18 non-pacemaker neurons were tested for their sensitivity to anoxia. On application of anoxic conditions, none ofthe inspiratory non-pacemaker neurons showed a significant increasein their discharge frequency. One recording is illustrated inFigure 6A. Ninety seconds after the onset of anoxia, which isequivalent to the augmentation phase in the intact network, theneuron continued to generate some action potentials. However,the example in Figure 6B2 shows at an extended time scale a significantdecrease in the AP frequency compared with control (Fig. 6B1).The AP activity ceased completely during prolonged anoxia (Fig.6B3). The instantaneous AP frequency of this neuron was plottedagainst time (Fig. 6C). The mean plot obtained for six neuronsrecorded in six different slices is illustrated in Figure 6D.The biphasic character of the anoxic response, as was evidentin the intact network (Figs. 3A, 4D), was abolished in the pharmacologicallyisolated non-pacemaker neurons. Instead these neurons exhibitedonly a rapid depression in their AP frequency.

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Figure 6. Anoxic response of isolated non-pacemaker inspiratory neurons. A, Recording of integrated population activity indicating the absence of rhythmic activity in the PBC (top trace) and a non-pacemaker neuron (bottom trace) in the presence of CNQX (20 µM). The top gray bar represents the time of the anoxic exposure. B, The three examples were obtained at the times indicated by 1, 2, and 3 in A. The examples shown in an extended time scale represent control conditions at time 20 sec (1), the anoxic augmentation at time 90 sec (2), and the depression period at time 150 sec (3). C, Instantaneous inspiratory frequency plotted against time obtained from the recording illustrated in A. Time 0 is set at the onset of anoxia. Recordings were obtained from a P9 animal. D, Mean plot of the instantaneous inspiratory frequency versus time obtained from six neurons. Note the absence of a significant excitation. Data were obtained from 7- to 9-d-old animals.

Anoxia did not alter the membrane potential of non-pacemaker neurons. The membrane potential values for six neurons were $-$ 56.6± 1.2 mV under control conditions, $-$ 56.3 ± 1.4 mV during the timecorresponding to the maximal augmentation in the intact network,and $-$ 57.3 ± 1.4 mV during the time corresponding to the maximaldepression. During the initial time of the anoxic exposure (90sec), there was no significant change in the AP frequency (from3.6 ± 0.7 Hz under control conditions to 3.3 ± 0.7 Hz in anoxia;p > 0.05); however, the AP frequency decreased significantly to1.3 ± 0.6 Hz during prolonged anoxia (110 sec; p < 0.01). Thesevalues were obtained during intervals of 15 sec at 90 and 110sec,respectively.

Anoxic response of pacemaker inspiratory neurons

Seven pacemaker neurons that were rhythmically active in phase with inspiration under control conditions and remained rhythmicallyactive after perfusion of CNQX were exposed to anoxic conditions.As in the intact network they responded in a biphasic manner;however, we found two different types of responses. For threepacemaker neurons, application of anoxic conditions led firstto an increase in bursting frequency corresponding in time tothe augmentation phase of the intact network (Fig. 7A,B2). Duringprolonged anoxia, bursting became irregular and not as pronouncedcompared with the control conditions, and these neurons generatedonly weak bursts after 3 min in anoxia (Fig. 7B3). Figure 7C showsthe instantaneous bursting frequency of the same neuron shownin Figure 7A. The mean histogram obtained for the three pacemakerneurons with this type of response is illustrated in Figure 7D.Both graphs show response properties resembling the biphasic responseof the intact network. This is better illustrated by superimposingthe response of the pacemaker neurons (Fig. 7D, filled squares)on the response of the intact network (Fig. 7D, open circles).Like the intact network, these neurons became inactive after 3min in anoxia. Because our recordings were obtained with the conventionalwhole-cell patch-clamp technique, the anoxia-induced suppressionof pacemaker bursts after 3 min in anoxia could be caused by awashout of bursting properties. However, this is unlikely becausebursting properties reappeared 10 min after the return to normoxicconditions (Fig. 7A, right panel).

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Figure 7. Anoxic response of isolated pacemaker inspiratory neurons. A, Simultaneous recording of integrated population activity from the PBC (top trace) and an inspiratory pacemaker neuron (bottom trace) during anoxia in the presence of CNQX (20 µM) obtained from a P6 animal. The top gray bar represents the time of the anoxic exposure. The right part of the recording illustrates the bursting activity 10 min after a return to normoxic conditions. B, Samples from A presented in an extended time scale and representing control conditions at time 20 sec (1), anoxic augmentation at time 90 sec (2), and the depression period at time 150 sec (3). C, Instantaneous inspiratory frequency plotted against time. Time 0 was set at the onset of anoxia. The filled squares represent strong inspiratory bursts; open squares represent weak inspiratory bursts. D, Mean plot of the instantaneous inspiratory frequency versus time obtained from three neurons (filled squares). The mean plot obtained from seven neurons in an intact network has been added in this graph for comparison (open circles). The pacemaker neurons showed an anoxic response, which is qualitatively similar to the network response, despite the fact that the increase in the bursting frequency is more pronounced for pacemaker neurons. Data were obtained from 6- to 11-d-old animals.

The three pacemaker neurons tended to depolarize from $-$ 59.6 ± 5.8 mV under control conditions to $-$ 49.3 ± 8 mV during the maximalaugmentation (p > 0.05). The membrane potential returned to $-$ 60± 4.9 mV during the maximal depression (p > 0.05). The burst durationchanged insignificantly from 0.70 ± 0.23 sec in control conditionsto 0.45 ± 0.29 sec during the maximal augmentation (p > 0.05)and significantly to 0.04 ± 0.15 sec during the maximal depression(p < 0.01). The intraburst AP frequency changed significantlyfrom 53.2 ± 2.8 Hz in control conditions to 21.36 ± 13.1 Hz duringthe maximal augmentation (p < 0.05) and to 6.7 ± 3.6 Hz duringthe maximal depression (p < 0.01). Measurements were performedfor six consecutive bursts in control conditions, maximal augmentation,and maximaldepression.

In contrast to these neurons, four pacemaker neurons remained rhythmically active during the entire time of anoxic exposure(Fig. 8A,B) and exhibited a transient increase in bursting frequency(Fig. 8B2). The two graphs representing the time course of thebursting frequency for one neuron (Fig. 8C) and for a group offour cells (Fig. 8D) show a typical biphasic response to anoxiawithout a cessation of rhythmic activity. The bursting activitypersisted after returning to normoxic conditions, as illustratedon Figure 8A (right panel).

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Figure 8. Anoxic response of isolated pacemaker inspiratory neurons. A, Simultaneous recording of integrated population activity from the PBC (top trace) and an inspiratory pacemaker neuron (bottom trace) during anoxia in the presence of CNQX (20 µM) obtained from a P10 animal. The top gray bar represents the time of the anoxic exposure. The right part of the recording illustrates the bursting activity 10 min after a return to normoxic conditions. B, Samples from A presented in an extended time scale and representing control conditions at time 20 sec (1), anoxic augmentation at time 90 sec (2), and the depression period at time 150 sec (3). C, Instantaneous inspiratory frequency plotted against time. Time 0 was set at the onset of the anoxic exposure. D, Mean plot of the instantaneous inspiratory frequency versus time obtained from four neurons (filled squares). The mean plot obtained from seven neurons in an intact network has been added in this graph for comparison (open circles). Note that these pacemaker neurons remained rhythmically active for a longer time than the network. Data were obtained from 7- to 13-d-old animals.

Anoxia induced also no significant change in the membrane potential of these four pacemaker neurons. Membrane potential valueswere $-$ 60 ± 3.9 mV during control conditions, $-$ 56.5 ± 2.6 mV duringthe maximal augmentation (p > 0.05), and $-$ 59 ± 3.4 mV during themaximal depression (p > 0.05). The burst duration was not significantlyaltered from 0.49 ± 0.06 sec under control conditions to 0.44± 0.04 sec during the maximal augmentation (p > 0.05) and to 0.37± 0.05 sec during the maximal depression (p > 0.05). The intraburstAP frequency remained constant during the augmentation phase (from28 ± 2.9 Hz in control conditions to 26.4 ± 1.9 Hz during themaximal augmentation; p > 0.05) and during the maximal depression(to 34.7 ± 2.4 Hz; p > 0.05). Measurements were obtained for sixconsecutive bursts in control conditions, maximal augmentation,and maximaldepression.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study intended to identify the neurons responsible for the generation of the increased respiratory frequency in anoxia.Therefore, we compared the anoxic effects on different types ofrespiratory neurons: expiratory, inspiratory non-pacemaker, andinspiratory pacemaker. Expiratory neurons were slightly depolarizedduring anoxia and became tonically active during augmentation.This suggests that expiratory neurons are not responsible forgenerating the increased respiratory frequency. This is consistentwith previous in vitro studies, which have demonstrated that anoxiasuppresses synaptic inhibition in expiratory neurons (Ballanyiet al., 1994; Ramirez et al., 1998).

In contrast to the expiratory neurons, rhythmic activity persisted in inspiratory neurons during the augmentation phase. Duringthis time their bursting frequency was increased, which is alsoconsistent with previous in vitro experiments (Ramirez et al.,1998). Here we showed that most inspiratory non-pacemaker neuronscannot contribute to this frequency increase. In the absence ofrhythmic population activity, the non-pacemaker neurons ceasedto discharge rhythmically, they were not depolarized, and thetonic activity present in the absence of network activity didnot increase during the augmentationphase.

Only a few neurons remained rhythmically active in the absence of network activity. These neurons are referred to as pacemakerneurons. The increase in bursting frequency exhibited by thesepacemaker neurons resembled the frequency increase as observedin the intact network. Therefore we conclude that the anoxia-inducedincrease in respiratory activity is caused by a direct modulationof pacemaker activity. This will drive the remaining respiratorynetwork at a higher frequency. To our knowledge, this is the firstdemonstration that anoxic effects on the respiratory frequencyare mediated by pacemaker inspiratoryneurons.

We found two types of pacemaker neurons: those that generated bursts of activity during the entire exposure to anoxia andthose that lost their bursting activity during prolonged anoxia.It is known that the amplitude of some membrane conductances showsan irreversible rundown when the conventional patch-clamp techniqueis used. This raises the possibility that during prolonged anoxiathe loss of bursting properties in one group of pacemaker neuronscould be caused by an anoxia-induced washout of pacemaker properties.However, this is unlikely to be the case because pacemaker burstingproperties recovered on return to normoxicconditions.

The role of synaptic inhibition in modulating the anoxic response of the respiratory system

As described previously in vivo (Richter et al., 1991; England et al., 1995; Schmidt et al., 1995) and in vitro (Ballanyiet al., 1994; Ramirez et al., 1998), synaptic inhibition is significantlysuppressed during anoxia. This suppression was most evident inthe pattern of expiratory neuronal activity. Because of the declinein synaptic inhibition, expiratory neurons became initially tonicand then inactive during anoxia. It is possible that expiratoryneurons influence tonically the respiratory network and that adecreased tonic activation of these neurons could lead to theanoxic augmentation; however, there is no experimental evidencefor this possibility. Furthermore, if these neurons provide aninhibitory input on the remainder of the respiratory network,other mechanisms have to be considered to explain the depressionof respiratory activity during prolonged anoxia, because theseneurons are inactive during thisphase.

Although the suppression of expiratory activity may not be responsible for the generation of the increased respiratory frequency,it may be important for reconfiguring the respiratory network.During severe hypoxia, normal respiratory activity is transformedinto gasping. This transformation is associated with a cessationof rhythmic expiratory activity (St. John, 1998) and a suppressionof synaptic inhibition (Lieske et al., 2000).

Role of pacemaker activity in regulating the frequency of respiratory activity during anoxia

We have demonstrated that pacemaker neurons exhibited an increased bursting frequency in anoxia. The frequency changes observedin the pharmacologically isolated pacemaker neurons were qualitativelysimilar to those observed in the intact respiratory network. Incontrast, non-pacemaker neurons exhibited no intrinsic excitationduring anoxia. The absence of an anoxia-induced excitation isvery interesting, because it indicates that anoxia could not causean increased transmitter release from these neurons. It is thereforevery unlikely that the non-pacemaker neurons could contributeto the increased frequency of the intact network. This leads tothe conclusion that the anoxia-induced frequency modulation isentirely dependent on the anoxic modulation of pacemaker neurons.During anoxia, these pacemaker neurons would provide a fasterrhythmic drive to the non-pacemaker neurons. Like the expiratoryneurons, non-pacemaker neurons therefore may play no role in thefrequency modulation but rather may play a role in the transformationof the respiratory motor pattern from normal respiration intogasping. It has been proposed that during normal respiration,concurrent inhibition and excitation in inspiratory neurons isresponsible for the augmenting activity that characterizes eupneicinspiratory activity (Ramirez et al., 1997; Lieske et al., 2000).In severe anoxia, the suppression of inhibition in inspiratoryneurons results in a decrementing activation, which is typicalfor gasping (Lieske et al., 2000).

Our findings therefore suggest that there is a strict separation into neurons associated with rhythm generation (pacemakerneurons) and those associated with pattern generation (expiratoryand non-pacemaker inspiratory neurons). A further functional separationof the pattern-generating mechanisms seems to occur at the motoroutput. The anoxic augmentation is characterized by a dramaticincrease in the amplitude of XII motor activity, which was notcaused by an increased synaptic drive from the pre-Bötzingercomplex (Telgkamp and Ramirez, 1999). Instead, the motor outputwas modulated by a mechanism that was functionally separate fromthe modulation of the frequency and shape of respiratory activitywithin the pre-Bötzinger complex. A separation into rhythm- andpattern-generating mechanisms has been proposed previously byFeldman and co-workers (1990). Our conclusions are also remarkablyconsistent with the model by Smith et al. (1995), who proposedthat pacemaker neurons provide rhythmic drive to the remainderof the network, which is primarily responsible for the generationof the respiratory motorpattern.

Ionic mechanisms leading to the frequency modulation of pacemaker neurons

To understand the anoxic effect on the respiratory rhythm, it will be essential to investigate the conductances that characterizepacemaker activity in respiratory neurons. However, so far onlyone study has experimentally investigated the conductances underlyingrespiratory pacemaker activity (Thoby-Brisson et al., 2000). Thisstudy demonstrated that pacemaker inspiratory neurons expressthe hyperpolarization-activated current (I_h) and that this currentplays a crucial role in determining their bursting frequency.It is well established that the I_h current is modulated by anoxia(Erdemli and Crunelli, 1998). Therefore, a modulation of thiscurrent may indeed play an important role in the anoxia-inducedincrease in the respiratory frequency. In fact, the absence ofan increase in intraburst frequency during anoxia suggests thatanoxia affects primarily the interval between two bursts. Thisinterval is highly affected by the I_h current; however, additionalexperiments will be necessary to examine whether this is thecase.

Are the pacemaker neurons the chemosensors for oxygen?

Our data have demonstrated that in response to anoxia the bursting frequency of pacemaker neurons is altered in the absenceof respiratory network activity. Although these neurons may wellbe the chemosensors of the respiratory network, the synaptic isolationdoes not provide sufficient evidence for this. It is conceivablethat under these conditions anoxia still caused the release ofneuromodulators, such as serotonin (Richter et al., 1999), adenosine(Schmidt et al., 1995), or substance P (Gray et al., 1999). Theseneuromodulators could then alter pacemaker activity even in theabsence of respiratory network activity. The resulting mechanismmay be complicated further, because these neuromodulators arenot released simultaneously and therefore may modulate pacemakeractivity in a differential and time-dependent manner (Richteret al., 1999). Thus, it is likely that the modulation of pacemakeractivity is caused by a combination of direct and indirect anoxiceffects. Examination of these possibilities will be an importantnext step in understanding the cellular mechanisms that lead tothe frequency modulation duringanoxia.

  FOOTNOTES

Received March 7, 2000; revised May 2, 2000; accepted May 11, 2000.

This study was supported by National Institutes of Health Grant HL60120 (J.M.R.).
Correspondence should be addressed to Dr. Jan-Marino Ramirez, Department of Organismal Biology and Anatomy, Committee on Neurobiology,The University of Chicago, 1027 East 57th Street, Chicago, IL60637. E-mail: Jramire{at}midway.uchicago.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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