Central respiratory activity of the tadpole in vitro brain stem is modulated diversely by nitric oxide

doi:10.1152/ajpregu.00513.2001

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Central respiratory activity of the tadpole in vitro brain stem is modulated diversely by nitric oxide

Michael B. Harris¹, Richard J. A. Wilson², Konstantinon Vasilakos², Barbara E. Taylor¹, and John E. Remmers²

¹ Department of Physiology, Dartmouth Hitchcock Medical Center, Dartmouth College, Lebanon, New Hampshire 03756; and ² Department of Medical Physiology and Biophysics, University of Calgary, Calgary, Alberta, Canada T2N 4N1

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Nitric oxide (NO) is a potent central neuromodulator of respiration, yet its scope and site of action are unclear. We used7-nitroindazole (7-NI), a selective inhibitor of endogenous neuronalNO synthesis, to investigate the neurogenesis of respiration inlarval bullfrog (Rana catesbeiana) isolated brain stems. 7-NItreatment (0.0625-0.75 mM) increased the specific frequency ofbuccal ventilation (BV) events, indicating influence on BV centralrhythm generators (CRGs). The drug reduced occurrence, alteredburst shape, and disrupted clustering of lung ventilation (LV)events, without altering their specific frequency. LV burst occurrenceand clustering also differed between pH conditions. We concludethat NO has diverse effects on respiratory rhythmogenesis, beingnecessary for the expression of respiratory rhythms, inhibitingthe frequency of BV CRG, and affecting both shape and clusteringof LV bursts through conditional modulation of LV CRG. We confirmcentral chemosensitivity in these preparations and demonstratechemomodulation of LV burst clustering and occurrence but notspecific frequency. Results support distinct oscillators underlyingLV and BVCRGs.

nitric oxide synthase; neuronal nitric oxide synthase; nitric oxide synthase-1; breathing; central pattern generation; central chemoreception; carbon dioxide; 7-nitroindazole; L-arginine; amphibian; tadpole; Rana catesbeiana; episodic periodic discontinuous clustered breathing

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

NITRIC OXIDE (NO) is a potent chemical messenger in the central nervous system. It is synthesized in neurons via a constitutiveand calcium-sensitive isoform of the enzyme NO synthase [NOS-1or neuronal NOS (nNOS); for review, see Refs. 11, 18]. NeuronalNO synthesis is induced, in part, by the synaptic activation ofN-methyl-D-aspartate-type glutamatergic receptors as well as byGABA and $beta$ -endorphins. The glutamatergic neuromodulatory cascadeis intimately involved in the genesis and regulation of breathingin vertebrates, and a growing body of evidence suggests that NOis an extremely important neuromodulator of central respiratorycontrol (3, 10, 12, 15-17, 19, 20, 29, 64). Thespecific respiratory action of NO, however, remains largelyunexplored.

In vitro brain stem preparations are used extensively to examine the central mechanisms responsible for the generation andmodulation of respiratory rhythm in vertebrates (37, 44, 48,49, 58). Such preparations derived from ectothermic vertebratesbenefit from their small dimension, relative hypoxia tolerance,and low metabolic demand (22, 28, 34, 44, 53, 54,68). In vitro brain stem preparations derived from larval amphibians,being well oxygenated and relatively nonacidic, are particularlywell suited to investigations of vertebrate central respiratoryrhythmogenesis and pattern formation (32, 44, 61, 69).

Semiterrestrial (postmetamorphic) tadpoles and adult frogs such as Rana catesbeiana exhibit prolonged periods of rhythmicventilation of the buccal cavity, termed buccal oscillations,interspersed by tidal lung ventilation (LV), which occurs as eithersingle events or periodic multibreath clusters (6, 7, 9,13, 24, 26, 51, 67). Motor patterns indicative of bothbuccal ventilation (BV) and LV persist in the amphibian in vitrobrain stem preparation, indicating that the capacity for theirgeneration resides within the brain itself (28, 34, 53,54). The neuronal elements that generate these ventilatory patternsand the factors that modulate the period and expression of thesebehaviors are poorlyunderstood.

Hedrick and co-workers (19, 20), using an in vitro preparation derived from adult bullfrogs, have recently demonstratedthat NO stimulates the occurrence of LV and propose that NO maybe a necessary messenger for neurotransmission and/or modulationof central respiratory drive. Indeed, these authors suggest thatthe general incidence of such robust fictive breathing among invitro preparations may result from an excitatory influence ofNO (19). The influence of NO on ventilatory pattern formation,and the levels at which it acts, however, are unclear. In thepresent study, we used in vitro brain stem preparations derivedfrom larval bullfrogs to further investigate the role of NO, synthesizedvia nNOS, in the genesis and modulation of respiratory rhythm.Specifically, we address the role of NO beyond the modulationof lung ventilatory occurrence. We examine the specific frequency(the inverse of the interval between successive events) of respiratoryburst discharge, taken to represent the activity of respiratorycentral rhythm generators (CRGs), as well as the overall occurrencerate (events per unit time) of this discharge and the shape andtendency of these LV bursts to occur in periodic clusters, reflectingthe conditional modulation of CRG activity. We postulate thatendogenously synthesized NO, arising from nNOS, influences theinherent frequency as well as the conditional expression of centralrespiratoryactivity.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

A total of 19 postmetamorphic R. catesbeiana tadpoles (stages 23-25, Taylor-Kollros scheme, Ref. 60) were used in this investigation.Animals were purchased from a commercial supplier and maintainedat room temperature in filtered dechlorinated water. This researchwas approved by the institutional animal care and use committee,and animal care and experimental protocols conformed to localand national standards of ethics. The work fully conforms withthe Guiding Principles for Research Involving Animals and HumanBeings specified by the American PhysiologicalSociety.

Surgical Preparation

Animals were initially anesthetized by immersion in an ice-cold 0.2 mM solution of tricaine methanesulfonate (MS222; Sigma)in dechlorinated water, buffered with NaHCO₃ to pH 7.4, untilunresponsive to tail or leg pinch (30-60 s). A block of tissuespanning a region between the orbits and forelimbs dorsal to themouth was removed and placed in a dissection chamber, where thedorsal cranium was removed and the forebrain rostral to the opticlobes was resected. This decerebration was achieved within 2 minof initiating dissection. During subsequent dissection, brainstems were superfused with ice-cold oxygenated artificial cerebrospinalfluid (aCSF) composed of (in mM) 104 NaCl, 4 KCl, 1.4 MgCl₂, 10D-glucose, 25 NaHCO₃, and 2.4 CaCl₂, equilibrated with 100% O₂.

Surgical procedures for preparing the in vitro brain stem have been described previously (61, 62). Briefly, the brainwas transected midtectum, at the level of the third cranial nerve(CN III) and 2 to 4 mm caudal to the second spinal nerve (SN II).The choroid plexus, dura, and portions of the arachnoid membraneon the ventral medulla were removed. Brain stems were then transferredto a low-volume (0.5 ml) flow-through recording chamber (61,62). Preparations were supported ventral side up between coarsenylon mesh such that all sides were bathed with aCSF flowing fromrostral to caudal over the tissue at a rate of 5-10 ml/min, resultingin 15-30 dish volume changes per minute. The aCSF solution, notedabove, closely matches the ionic composition reported for postmetamorphictadpole and adult frog plasma (6, 24, 57). In particular,the aCSF bicarbonate concentration is equal to that of plasma,so that equilibration of aCSF with a normal CO₂ produced a normalpH. Preparations maintained in this solution produce easily identifiablerespiratory discharge patterns that are consistent and stablefor many hours and that closely resemble those associated withspontaneous ventilatory behavior in vivo (13). A supply of aCSFflowed to the chamber from perfusion reservoirs through glasstubing and a bubble trap. The reservoirs served as tonometerswhere aCSF was equilibrated with O₂-CO₂ gas mixtures to producethe desired pH. The fractional concentration of O₂ and CO₂ (FO₂and FCO₂, respectively) in the equilibration gas was regulatedwith precision needle-valve flow meters on the inlet lines, andFCO₂ was monitored with an infrared medical gas analyzer (SensorMedics,LB-2). The pH of the solution in the tonometer was monitored (Corning140) and maintained between 7.6 and 8.0 by adjusting FCO₂ in theequilibration gas. Solutions were equilibrated with approximately3.5, 2.2, and 1.4% CO₂, balance O₂, to produce aCSF pH of 7.6,7.8, and 8.0, respectively. The resulting aCSF CO₂ partial pressureswere approximately 25, 16, and 10 mmHg, respectively. Pilot studiesdemonstrated that the pH of the tonometers and recording chamberwere identical and stabilized in 2 to 3 min after a change inequilibration gas FCO₂.

Nerve Recording

Roots of CN VII and SN II were drawn into glass suction electrodes fabricated from 1-mm-diameter capillary glass (A-M Systems,Everett, WA) pulled to tip diameters of ~40 µm. Whole nerve dischargewas amplified (×1,000) and filtered [100-300 Hz (low pass) to1 kHz (high pass)] using a differential AC amplifier (model 1700,A-M Systems) and fed to a modified Bessel filter (time constant50 ms; SagaTech, Calgary, Alberta, Canada; see Ref. 45). Bothraw (amplified) and Bessel-filtered signals were digitized at2,000 Hz/ channel and archived as computer files (AT-CODAS, DATAQInstruments, Akron, OH) for subsequent analysis (ADVPOST and WINDAQ,DATAQInstruments).

Burst Classification

The burst discharge patterns of various cranial and spinal nerves associated with the normal activation of respiratory musclesduring spontaneous LV, and either gill ventilation or buccal oscillations,have been previously characterized in both frogs and tadpoles(13, 25, 30, 51, 52). Burst activity patterns recordedfrom CN VII and SN II are indicative of the activation of musclesthat contract in phase with movements of the buccal cavity duringspontaneous ventilation, such as the depressor mandibulae, subhyoideus,sternohyoid, hyoglossus, and omohyoid muscles (51). Burst activitypatterns were classified as described by Torgerson et al. (62)and Gdovin et al. (13) as corresponding to buccal ventilation(BV) and LV. BV bursts were identified as rhythmic bursts of activityin CN VII recordings, of <1 s in duration and having a generallymonophasic gradual incrementing onset and decrementing offsetprofile. The relative amplitude of BV bursts in the Bessel-filteredsignal was generally 3 to 5 times that of tonic baseline activity.BV bursts were apparent, frequently but not always, in the SNII neurogram. LV bursts were identified as rhythmic bursts ofactivity that were always coincident in CN VII and SN II recordings.Such bursts were also of <1 s in duration, were either monophasicor biphasic, and also had incrementing onset and decrementingoffset profiles. The relative amplitude of LV bursts in the Bessel-filteredsignal was generally 3 to 5 times that of BV bursts. Patternsof activity that did not meet the criterion for BV or LV burstswere classified as "nonrespiratory" (see Ref. 47 for examples).These bursts have long durations, large amplitudes, or shapesinconsistent with those normally associated with ventilation,and they may represent neural activity associated with such behaviorsas vocalization, feeding, swallowing, coughing, regurgitation,or gasping (8, 32, 46, 47, 52, 53). Alternately,this discharge may not relate to naturally occurring phenomenain vivo and may be an artificial construct of some in vitro preparations(4). Such nonrespiratory bursts occurred uncommonly in ourpreparations.

Protocol

Disruption of endogenous NO synthesis. After the 1-h period of stabilization, FCO₂ of the gas equilibrating the tonometer of aCSF was adjusted to produce an aCSFpH of either 7.6 (n = 5), 7.8 (n = 5), or 8.0 (n = 7), and burstactivity was monitored for a 60-min baseline period. Pilot studiesindicated that burst activity stabilized within ~10 min of a pHchange. Preparations were then exposed to drug solutions containingvarious concentrations (0.06-1.0 mM) of a selective noncompetitiveinhibitor of nNOS, 7-nitroindazole (7-NI), in aCSF. Drug solutionswere prepared in identical tonometers, equilibrated with the samegas, and had the same pH as the baseline aCSF. Each preparationwas exposed to at least four concentrations of 7-NI. The maximum7-NI concentration was that which all but abolished LV burst activityduring pilot investigations. As preparations produced differentlevels of activity at the three pH levels, the tested range of7-NI concentrations differed between pH conditions. All preparationstested at a given pH were exposed to the same range of 7-NI concentrations.Treatment 7-NI concentrations were administered randomly, andeach 30-min period of exposure was followed by at least a 30-min"washout" period of exposure to drug-free aCSF. Although levelsand patterns of activity during washout periods returned towardthose observed during initial conditions, most of the values obtainedfrom such periods were different from initial values, indicatingthat residual effects of 7-NI exposure were long-lasting. Hedrickand Morales (19) also observed a long latency to incompleterecovery after exposure to 7-NI.

Data analysis. Data were analyzed from 15-min "observation" periods taken from the end of both the 60-min baseline and 30-min drug exposureperiods. Values obtained from "washout" periods have not beenincluded in the presentanalysis.

Burst occurrence rate and specific frequency. Total burst occurrence was the sum of all BV and LV bursts within the observation period. Burst occurrence rate was calculatedas the ratio of total burst occurrence to observation period durationto yield an overall frequency (bursts/min). The specific frequencyof bursts was calculated from the period of successive BV or LVbursts. Only pairs of sequential and alike bursts not separatedby any other burst type were included in this analysis. The inverseof this period was multiplied by 60 and expressed as a frequency(bursts/min).

Burst duration and shape. The duration of BV and LV bursts was determined from the Bessel-filtered record of CN VII whole nerve discharge, as the timebetween burst onset, i.e., where the signal deviated from tonicbackground activity, to the point where the signal returned tothis baseline. The shape of LV bursts in the Bessel-filtered CNVII discharge was assessed subjectively as being either biphasicor monophasic. The influences of NOS inhibition were demonstratedby generating event-triggered average tracings from individualpreparations. Recordings of Bessel-filtered CN VII discharge surroundingsingle breaths or clusters were compiled from initial and treatmentconditions. Tracings from 25 consecutive events from initial andtreatment conditions were averaged and expressed as the mean levelof activity ± 1 SD of the mean for eachcondition.

Burst clustering. In all cases, LV bursts occurred intermittently, with LV bursts occurring as periodic events (episodes) with otherwise relativelyrhythmic and continuous BV burst activity. An episode of LV burstswas defined as either a single or an uninterrupted cluster ofLV bursts separated from subsequent LV bursts by one or more BVbursts or, in cases where BV activity was absent, by a periodexceeding twice the control LV-LV burst period. The clusteringof LV bursts was assessed by determining the average number ofbursts occurring in each episode, expressed as bursts/cluster,with single isolated bursts counted as a "cluster" of one burstfor the purpose of analysis. The duration of burst episodes (theperiod from the onset of the first to the end of the last burstin an episode) and the number of episodes occurring during theobservation period, expressed as episodes per minute, were alsodetermined.

Statistical assessment. Statistical analyses were performed with the aid of a computer and statistical software (SigmaStat v. 2.03, Jandel Scientific).Influences of pH on burst discharge parameters under initial conditionswere determined by a series of one-way (non-repeated) analysesof variance (ANOVA). The influence of 7-NI treatment was assessedthrough a series of one-way repeated-measures ANOVA for each pHcondition. The specific frequency of BV and LV bursts was comparedbetween pH conditions by a series of two-way (non-repeated) ANOVAmade at each concentration of 7-NI. In these cases, additionalpairwise multiple comparison procedures were done using the Student-Newman-Keulsmethod. Data illustrating the influence of pH on burst clusteringunder initial conditions were not normally distributed, and theparametric ANOVA assessing this influence did not achieve thedesired power. As such, an additional analysis was made usinga Kruskal-Wallis one-way ANOVA on ranks with Dunn's method ofpairwise multiple comparisons. In addition, a parametric t-testwas used to assess the normally distributed subset of these data(between pH 7.8 and 8.0), as noted in the text. Data illustratingthe influence of 7-NI on burst clustering at pH 7.6 were alsonot normally distributed, and parametric ANOVA assessing thisinfluence did not achieve the desired power. Additional analysiswas made using a Friedman repeated-measures ANOVA on ranks. Alltests employed an $alpha$ -value of 0.05; thus normality, equality ofvariance, and significance of differences were attributed to P< 0.05.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

LV and BV Burst Discharge

For the most part, patterns of whole nerve burst discharge recorded from CN VII and SN II matched the criterion for classificationas either LV or BV bursts. Under initial conditions, burst dischargepattern and shape were remarkably consistent both over time withina given preparation, and between preparations. At most, one ortwo nonrespiratory bursts occurred in any given 15-min period.As such, events were overshadowed by the far more prevalent LVand BV and were not analyzed. BV bursts were most prevalent, appearingto occur rhythmically and relatively continuously, interruptedby intermittent periods of LV burst activity (Fig. 1, top tracing).

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Fig. 1. Recordings of the moving average of whole nerve discharge in cranial nerve VII (CN VII) illustrating ventilatory motor patterns from an isolated tadpole brain stem bathed in pH 7.6 mock cerebral spinal fluid with various concentrations of 7-nitroindazole ([7-NI], in mM). Two distinct motor patterns are apparent: large and small amplitude bursts, indicative of lung and buccal ventilation, respectively.

Influence of NOS Disruption

Specific frequency. The specific frequency of LV bursts within a cluster was constant regardless of pH or the concentration of 7-NI (Fig. 2).The specific frequency of BV bursts, however, increased with 7-NItreatment (F_4,19 = 4.2, P = 0.03; F_4,17 = 3.8, P = 0.04; F_4,25= 6.3, P = 0.04, at pH 7.6, 7.8, and 8.0 respectively). Underno circumstance did the specific frequency of BV bursts exceedthat of LV bursts.

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Fig. 2. Histograms illustrating the effect of 7-NI on the specific frequencies (means + SE, expressed as bursts/min) of lung and buccal respiratory events, during exposure to various concentrations of 7-NI in superfusates with pH 7.6 (A), 7.8 (B), and 8.0 (C). * Significant difference from values observed during initial exposure to drug-free superfusate (P < 0.05).

Burst occurrence. Under all three pH conditions (7.6, 7.8, and 8.0), NOS inhibition influenced both LV and BV bursts. This treatment reducedthe occurrence of LV bursts (F_4,24 = 5.6, P = 0.05; F_5,20 = 22.6,P < 0.001; F_4,29 = 11.6, P < 0.001, respectively) and increasedthe occurrence of BV bursts (F_4,24 = 23.4, P < 0.001; F_5,19 =5.1, P = 0.014; F_4,25 = 11.3, P <0.001, respectively, Fig. 3).

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Fig. 3. Histograms illustrating the effect of 7-NI on the occurrence (means + SE, expressed as bursts/min) of lung and buccal respiratory events, during exposure to various concentrations of 7-NI in superfusates with pH 7.6 (A), 7.8 (B), and 8.0 (C). * Significant difference from values observed during initial exposure to drug-free superfusate (P < 0.05).

NOS inhibition tended to reduce the occurrence of LV bursts at all levels of perfusate acidity. However, LV bursts were moreresilient to the effects of 7-NI at low pH. Thus, at the lowestlevel of pH (7.6), LV bursts were eliminated only at 7-NI concentrationsof 1.0 mM. For pH values of 7.8 and 8.0, LV bursts were abolishedwith 7-NI concentrations above 0.75 and 0.5 mM, respectively.BV bursts were generally not discernable at 1.0 mM 7-NI. BV burstactivity was robust below this level, and such bursts routinelypersisted despite the relative absence of LVburst.

Burst shape. 7-NI treatment decreased LV burst duration only at pH 7.6 (F_4,24 = 6.3, P = 0.003), while this treatment decreased BV burstduration at pH 7.6 and 8.0 (F_4,20 = 6.3, P = 0.006; F_4,27 = 3.4,P = 0.033, respectively, Fig. 4).

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Fig. 4. Histograms illustrating the effect of 7-NI on the duration (means + SE, expressed in s) of lung and buccal respiratory events, during exposure to various concentrations of 7-NI in superfusates with pH 7.6 (A), 7.8 (B), and 8.0 (C). * Significant difference from values observed during initial exposure to drug-free superfusate (P < 0.05).

The shapes of LV bursts recorded from CN VII were generally biphasic, although a minority of isolated single bursts and occasionallythe first bursts in a multiburst cluster were monophasic. NOSinhibition had an obvious influence on this shape by causing adose-dependent reduction in the magnitude of the initial phaseof the biphasic burst and a smoothing of the initial peak (Figs.5 and 6). This resulted in a more gradual and smaller initialwave, which resembled the rising phase of a BV burst, followedby a monophasic peak.

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Fig. 5. Event-triggered averages (solid line) ± SE (dashed lines) of CN VII activity, demonstrating the influence of various concentrations of 7-NI (in superfusate with pH 7.8) on ventilatory burst shape and pattern. Tracings were triggered from the largest peak of Bessel-filtered CN VII activity and averaged over 25 consecutive episodes of lung burst activity (either the 1st burst of a cluster or a single burst).

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Fig. 6. Event-triggered averages (solid line) ± SE (dashed lines) of CN VII activity, demonstrating the influence of various concentrations of 7-NI (in superfusate with pH 8.0) on ventilatory burst shape and pattern. Tracings were triggered from either 1) the largest peak of Bessel-filtered CN VII activity and averaged over 25 consecutive episodes of lung burst activity (either the 1st burst of a cluster or a single burst) or 2) in the absence of lung burst activity, from the characteristic "trough" after a buccal burst and averaged over 25 consecutive 10-s periods.

Clustering LV bursts into multiburst episodes. 7-NI treatment altered the number of LV bursts occurring in each episode (Fig. 7). At pH 7.6, 7-NI treatment caused a marginalreduction in the number of bursts per cluster (Fig. 7B; F_4,24= 2.9, P = 0.051). However, the power of this assessment (0.457at $alpha$ = 0.05) was less than the 0.800 desired, and data were notnormally distributed. The trend for a decrease in the number ofbursts per cluster with 7-NI was demonstrated by a Friedman repeated-measuresANOVA on ranks (Chi-square = 17.053 with 4 degrees of freedom;P = 0.002). At pH 7.8, 7-NI treatment reduced the number of burstsper cluster and converted multiburst episodes to single bursts(F_5,20 = 15.0, P < 0.001; Fig. 7C). LV bursts at pH 8.0 generallyoccurred as single or paired bursts per episode. NOS inhibitionaltered burst clustering at pH 8.0 (F_4,22 = 4.9, P = 0.014), atlow doses by enhancing the number of bursts per cluster (P = 0.018and 0.036 by multiple comparison at 0.06 and 0.12 mM, respectively)and at higher doses by reducing them (Fig. 7D).

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Fig. 7. Histograms illustrating the occurrence of lung bursts and the clustering of bursts (means ± SE). A: the influence of superfusate pH and the relationship between burst occurrence and burst clustering. B-D: the influences of exposure to various concentrations of 7-NI (in superfusates with pH 7.6, 7.8, and 8.0, respectively) on burst occurrence, clustering, and the relationship between the two. Significant differences are noted in the text.

Importantly, 7-NI treatment could independently alter clustering without changing burst occurrence (Fig. 7). At pH 7.8, 0.12mM 7-NI reduced the number of bursts per cluster without changingoverall LV burst occurrence. Figure 1 illustrates a particularcase where 7-NI treatment clearly converts burst pattern frommultiburst episodes to single unclustered bursts, without alteringoverall burst occurrence (between 0 and 0.5 mM 7-NI). The apparentreductions in overall LV burst occurrence caused by 0.25 mM 7-NIat pH 8.0 with no change in clustering (Fig. 7D) reflects simplythe fact that in these cases bursts generally occurred as singleevents rather than multiburstclusters.

NOS inhibition did not alter the frequency of LV burst episodes. The duration of such episodes at pH 7.6 and 7.8 was reducedby 7-NI treatment (F_4,24 = 3.407, P = 0.034; F_5,21 = 6.55, P =0.004), although no similar effects were noted at pH 8.0 (F_4,22=1.375, P = 0.30; power at $alpha$ = 0.050: 0.107 < 0.800).

Influence of CO₂/H+ in Drug-Free Superfusate

Specific frequency. LV burst specific frequency (within a cluster of breaths) was insensitive to changes in pH, while the specific frequency ofBV bursts was influenced by pH (F_2,16 = 7.5, P = 0.006, Fig. 2),being higher at pH 7.8 than either 7.6 or 8.0 (P = 0.05 and 0.038).Regardless of pH, however, BV burst specific frequency was alwayslower than that of LV bursts (F_2,33 = 19.0, P < 0.001). The durationof LV bursts increased with elevations in pH (F_2,16 = 4.8, P =0.027), with longer bursts occurring at pH 8.0 than pH 7.6 (P= 0.026), while pH did not influence the duration of BV bursts(Fig. 4).

Burst occurrence. There was a significant influence of pH on the occurrence of lung and buccal bursts (F_2,16 = 7.1, P = 0.008; F_2,16 = 5.0,P = 0.024, respectively, Fig. 3). Fewer LV bursts occurred atpH 8.0 than at either pH 7.8 or 7.6 (P = 0.024 and 0.008, respectively),while the values at pH 7.8 and 7.6 did not differ significantly.Fewer BV bursts occurred at pH 7.6 than at either pH 7.8 or 8.0(P = 0.031 and 0.02) with no differences between pH 7.8 and 8.0(P = 0.637; power at $alpha$ = 0.050: 0.609 < 0.800).

Clustering bursts. LV bursts occurred intermittently as episodes of either single or clustered LV bursts, each separated by BV bursts. CO₂/H⁺ did not consistently influence the tendency to cluster burstsover the full range of pH levels (F_2,16 = 2.16, P = 0.152, byone-way ANOVA), although the statistical power of this assessment(0.208 at $alpha$ = 0.050) was well below that desired (0.800), anddata were not normally distributed. The trend for an increasein the number of bursts per cluster with a decrease in pH wasdemonstrated by a nonparametric Kruskal-Wallis one-way ANOVA onranks (H = 6.633 with 2 degrees of freedom, P = 0.036). The greaterpredominance of single LV bursts and fewer LV bursts occurringper cluster at pH 8.0 than at pH 7.8 was demonstrated by Dunn'spairwise multiple comparison procedure (difference on ranks =7.243; Q = 2.45; P < 0.05) or by parametric t-test (t = 5.159with 10 degrees of freedom, P < 0.001; power at $alpha$ = 0.050: 0.997;Fig. 7A). Changes in burst occurrence were generally associatedwith corresponding changes in clustering. No influence of pH onthe number of LV burst episodes per minute was detected, althoughthe duration of these episodes was marginally influenced by pH(F_2,16 = 3.5, P = 0.058; power at $alpha$ = 0.050: 0.584 < 0.800; Fig.4).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

General

LV bursts in the amphibian brain stem preparation occur in clusters separated by periods of BV. We have attempted to elucidatethe effects of 7-NI and of changes in PCO₂/pH by examining overallrate of burst occurrence, the number of LV bursts per episode,and the specific frequency of LV and BV bursts. The specific frequenciesof sequential ventilatory events represent the period or oscillatoryfrequency of the CRG(s) controlling these events. This variableindicates the endogenous rhythm of intermittent events (28).While changes in the apparent frequency of bursts can occur throughskipped beats, changes in specific frequency, in the absence ofskipped beats, can result only from direct modulation of mechanismsresponsible for rhythmogenesis. In contrast, overall burst occurrenceis more indicative of the degree to which the conditional oscillatoris active. Changes in the occurrence of cranial nerve bursts canresult from changes in the frequency of a central oscillator,but can also result from upstream modulation of the conditionaloscillator, which alters the probability of its activation orquiescence, as well as downstream modulation of the transductionof oscillator output at the level of premotor and motor neuronpools.

Sensitivity of In Vitro Ventilatory Pattern to NOS Disruption

Specific frequency of ventilatory bursts. The specific frequency of LV bursts within clusters was invariant over the range of 7-NI treatment, indicating that endogenousNO does not regulate the frequency of the oscillator producingthis burst pattern. In contrast, the elevation of BV specificfrequency with 7-NI treatment suggests that the oscillator responsiblefor BV burst generation is frequency modulated by NO. These resultssuggest that the period of the BV oscillator is normally depressedby endogenous NO synthesis and that different circuits generatethese two types ofrhythm.

The genesis of buccal oscillations appears to require postsynaptic inhibition, while lung oscillations do not, suggestingthat the buccal oscillator requires network interaction whilethe lung oscillator possesses pacemaker properties (8). NOdoes not appear to influence the pacemaker properties of the lungoscillator. As disruption of endogenous NO synthesis increasedthe specific frequency of BV bursts, our present results suggestthat endogenous NO lengthens the period of the buccal oscillator,possibly by modulating synaptic strength within the buccal oscillatornetwork or modulating some other drive to thisoscillator.

Occurrence of ventilatory bursts. Treatment with 7-NI produced a dose-dependent reduction in the occurrence of LV bursts. Thus, although endogenous NO synthesisdoes not regulate the intrinsic frequency of the oscillator producingthis burst pattern, the expression of this oscillator appearsto be dependent on the endogenous production of the neuromodulator.This observation is consistent with the lung CRG being a conditionaloscillator, having the capacity to oscillate but requiring anexcitatory input to induce this oscillation (49). Hedrick andco-workers (19, 20) have also demonstrated that treatmentwith 7-NI decreases the occurrence of LV in a similar in vitropreparation derived from adult frogs. The authors conclude thatNO was somehow necessary for the expression of this dischargeand may, thus, be a necessary messenger for neurotransmissionand/or modulation of central respiratory drive. Our results agreewith this conclusion and indicate that NO synthesis influencesthe expression of LV bursts upstream and/or downstream of theoscillator, rather than by influencing the properties of the oscillatoritself. Endogenously produced NO does appear to contribute totonic excitation of the lung oscillator. Thus this influence facilitatesand may be necessary for the expression (occurrence) of LV bursts.Robust BV bursts generally persist while LV bursts become lesscommon as endogenous NO synthesis is disrupted. This suggeststhat motor output itself is not compromised by 7-NI treatment.An exception, however, may be occurring in the current study atpH 7.6 during exposure to 1.0 mM 7-NI. Under these conditionsthe expression of both BV and LV bursts appears to be disrupted.A significance to the effect of this relatively high 7-NI doseisunknown.

Shape of ventilatory bursts. In adult and larval frogs, inspiration is initiated by depression of the buccal floor and acquisition of air through opennares into the buccal cavity (constituting buccal acquisitionor the loading phase of the buccal force pump). Lung inflationoccurs with the elevation of the buccal floor, with closed naresand an open glottis. Expiration immediately precedes lung inflationduring tidal ventilation and occurs when the glottis and naresare opened between buccal acquisition and lung inflation (7,9, 13, 30, 31, 51, 64, 67). Although the removalof peripheral inputs does alter respiratory motor pattern, biphasicLV bursts recorded in vitro correspond to the burst dischargepattern of respiratory muscles during the ventilatory cycle invivo, with the first and second waves corresponding to activationof buccal depression and elevation, respectively (13, 25,30, 31, 51).

7-NI treatment abolishes the first element of the biphasic burst in CN VII without any apparent alteration of either the secondphase of these bursts or the BV burst (Figs. 5 and 6). This indicatesthat NO plays an important role in the modulation of LV burstshape, particularly the buccal depression wave or loading phase.The dose-dependent abolishment of the initial phase of normallybiphasic LV bursts by NOS inhibition results in a monophasic bursts.This transition suggests that endogenous NO production is essentialfor the genesis of biphasic ventilatory bursts and may indicatea role of NO in the determination of biphasic (tidal) ventilatoryevents vs. monophasic (deflationary) events (66).

Despite contributing to a distinct biphasic to monophasic transition in LV burst shape, 7-NI had no effect on the durationof these bursts. The occurrence of what resembled a BV-like risingphase in place of the initial phase of a biphasic burst resultedin a monophasic burst having the same duration as the biphasicbursts that occurred in the absence of NOS inhibition. The significanceof such an alteration of burst shape with a preservation of burstduration isunknown.

Clustering bursts into multiburst episodes. During periodic breathing, the tendency to cluster breaths into multibreath episodes is an important element of ventilatorycontrol and specifically regulated by the central nervous system(35, 36). The present results illustrate that NOS inhibitiongenerally reduces the number of putative lung breaths per clusterand prompts the occurrence of single breaths rather than clusters.Such a transition can occur without a reduction in the overalloccurrence of breaths, indicating that the regulation of burstclustering can occur independent of overall ventilatory occurrence.Abundant evidence indicates that supramedullary influences contributeto the production of multibreath breathing episodes (23, 27, 39,40, 42, 43, 46; for reviews, see Refs. 35, 36). The neuralelements and mechanistic basis for the production of multibreathepisodes are, however, unknown. Our data demonstrate that endogenousNO synthesis is strongly involved in, if not necessary for, clusteringbreaths into multibreath episodes. Recently Straus et al. (59)have suggested that a pathway dependent on GABA B-type receptorscould also regulate such clustering. Given these results, it ispossible that several neuromodulators may influence breathclustering.

The site of action for such modulation is uncertain. A number of investigations have suggested that multibreath clusters arethe result of specific supramedullary modulatory influences (23,27, 39, 40, 42, 43, 46; for reviews, see Refs. 35, 36). Weroutinely observe multiburst clusters of LV activity in isolatedbrain stem preparations after midtectal transection at the levelof the CN III (Ref. 57 and present investigation), but not afterisolation of the medulla from the tectum (63). These observationssuggest that elements necessary for the generation of multiburstclusters could reside in the tectum caudal to CN III. NOS-containingneurons have been identified in a number of amphibian brain stemregions (2, 5, 14). High concentrations occur in the midto caudal tectum proximal to the nucleus isthmi, an area involvedin the genesis of multibreath clusters as well as modulating ventilatorysensitivity to respiratory stimuli (10, 27). This distributionidentifies a potential mechanism through which the isthmic regionmodulates this clustering. Without discounting a supramedullaryinfluence, we reserve the opinion that the genesis of multibreathbreathing episodes may not require a specific, distinct, and necessaryneural element such as an episode center. Modulatory inputs ofmany sorts and sources appear to alter the probability that breathswill occur in clusters (23, 26-28, 35, 36, 59; present investigation).Thus clustered breaths may result from more general propertiesof the central pattern generator for ventilation itself, ratherthan from the influence of an episode center perse.

Sensitivity of In Vitro Ventilatory Pattern to pH/CO₂

Specific frequency. Regardless of pH, the specific frequency of LV bursts within clusters was invariant, suggesting that central chemosensoryinputs do not modulate the frequency of the LV oscillator. Althoughstatistically significant, we cannot determine the biologicalrelevance of a BV burst specific frequency higher at pH 7.8 thaneither 7.6 or 8.0. The presence of this difference, however, suggeststhat the oscillator responsible for BV burst generation is frequencymodulated by chemosensory inputs, while that underlying LV burstgeneration is not, as we have recently suggested (50). Again,CO₂/pH would appear to influence network properties of the buccaloscillator but not pacemaker properties of the lungoscillator.

Occurrence. The occurrence of LV bursts was stimulated by a reduction in pH, confirming the presence of CO₂/H⁺ chemosensitivity within the in vitro brain stem preparation.Thus, although the frequency of the LV oscillator is insensitiveto CO₂/H⁺, the expression of this oscillator appears to be conditionallydependent on such input. The degree of this sensitivity is comparablewith that previously observed in similar in vitro preparationsand in adult frogs in vivo after vagotomy (26, 62). Thesefindings differ from other reports of amphibian in vitro preparationsdisplaying little or no sensitivity to hypercapnia (46, 50).Fewer BV bursts occurred at lower pH. As BV bursts occur rhythmicallyand relatively continuously in the absence of LV bursts, the reducedoccurrence of BV bursts likely reflects the lower opportunityfor such bursts to occur under conditions which stimulate LVbursts.

Clustering. LV bursts generally occurred in multiburst clusters, with fewer bursts occurring per cluster at pH 8.0 than at a lower pH.This trend appears to match our finding of a lower LV occurrencerate at higher pH and illustrates a consistent relationship betweenventilatory drive (the occurrence of bursts) and the tendencyto cluster bursts into multibreath episodes. This distinct influenceof pH on LV burst clustering also emphasized the hypercapnic sensitivityof thispreparation.

While the specific frequency of LV bursts occurring in episodes is unrelated to pH, we note a marginal influence of pH onthe duration of these episodes. In other words, with a constantspecific frequency of LV bursts, a tendency toward single breathsat pH 8.0 should also be reflected in a tendency toward shorterepisode durations at this pH. The strength of this relationship,however, appears to beminimal.

Possible role of NO modulation of breathing pattern. The core of the tadpole in vitro brain stem preparation is hyperoxic and mildly acidotic, resulting from a respiratory acidosisand restricted CO₂/H⁺ diffusion from the nonperfused tissues (61, 69). Undoubtedly,LV burst activity in these preparations is sensitive to PCO₂/pHand will be facilitated by the core tissue acidosis. Yet, in theabsence of other peripheral inputs, stimulation from these levelsof CO₂/H⁺ in vivo may not result in such robust respiratory patterns (28,55, 56). As NO synthesis is enhanced by hyperoxia (1),we agree with the contention of Hedrick and Morales (19) thattissue NO may be elevated and that this elevated NO stimulatesthe production of LVbursts.

The PO₂ of our hyperoxic in vitro preparations is within the range (0-150 Torr) over which NOS activity is exquisitely sensitiveto O₂ (1). We propose that tissue PO₂ normally modulates NOSactivity over this range and, thus, regulates endogenous NO synthesis.Hypoxia could then result in a reduction of tissue NO, which isof primary importance to the modulation of a number of physiologicalfactors that underscore such phenomena as hypoxic ventilatoryand metabolic depression (12, 38). Recently, Gargaglioni andBranco (10) have reported that disrupting NO synthesis withinthe nucleus isthmi of toads enhances their ventilatory responsesto hypoxia or hypercarbia. These results indicate that reductionsin NO synthesis within specific brain stem areas can augment ventilatorysensitivity to respiratory stimuli and suggest that NO synthesiscould be involved in the transduction or integration of chemosensoryinformation. We further postulate that endogenous tissue NO synthesisprovides central oxygen sensitivity to some if not all neuraltissues, allowing such tissues to arrest their function and metabolismin the face of hypoxia, thereby shielding themselves from hypoxicdamage. The NOS enzyme is found in organisms ranging from bacteriato vertebrates and in most energetically active tissues proneto damage by hypoxia (21, 41). Given the relatively universalnature of NO and its potent role as a modulator, a mechanism ofNO-mediated hypoxia-induced hypometabolism may be highly significant,and both ancient and highlyconserved.

Oscillatory mechanisms for BV and LV. Amphibians exhibit BV and LV oscillations, two rhythmic patterns that could result from the same or distinct neuronal oscillators(28). In the present investigation, the specific frequency ofLV bursts within a cluster was constant regardless of pH or theconcentration of 7-NI. In contrast, the specific frequency ofBV bursts 1) was lower than that of LV bursts under initial conditions,2) was influenced by pH, and 3) increased with 7-NI treatment.The oscillator generating BV bursts, therefore, appears to havea different endogenous period and be differentially modulatedthan that which generates LV bursts. These differences lend furthersupport to the hypothesis that LV and BV bursts are generatedby functionally distinctoscillators.

Conclusion

Endogenous NO synthesis has a diverse influence on respiratory burst activity. It modulates the period of a BV oscillatorand the conditional expression of a functionally distinct LV oscillator.It influences the shape, and perhaps function, of LV bursts andthe tendency for such bursts to cluster into multiburst episodes.These influences could explain the presence of robust ventilatoryrhythms in hyperoxic in vitro preparations that lack other modulatoryinputs, and they may be highly significant in mediating adaptiveresponses to hypoxia invivo.

	ACKNOWLEDGEMENTS

We thank M. Hedrick for assisting on the formulation of thisinvestigation.

	FOOTNOTES

Research was funded by an operating grant to J. E. Remmers from the Medical Research Council of Canada and by fellowshipsfrom the Alberta Heritage Foundation for Medical Research (R.J. A. Wilson and K. Vasilakos), the Medical Research Council ofCanada (K. Vasilakos), the Natural Science and Engineering ResearchCouncil of Canada (M. B. Harris), and the Parker B. Francis Foundationfor Pulmonary Research (R. J. A.Wilson).

Address for reprint requests and other correspondence: M. B. Harris, Dept. of Physiology, Dartmouth College, Borwell Bldg.,Dartmouth Hitchcock Medical Center, One Medical Center Drive,Lebanon, New Hampshire 03756 (E-mail address: michael.b.harris{at}.dartmouth.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

May 6, 2002;10.1152/ajpregu.00513.2001

Received 22 August 2001; accepted in final form 2 May 2002.

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