Respiratory changes induced by kainic acid lesions in rostral ventral respiratory group of rabbits

doi:10.1152/ajpregu.00579.2001

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Respiratory changes induced by kainic acid lesions in rostral ventral respiratory group of rabbits

Donatella Mutolo, Fulvia Bongianni, Marco Carfì, and Tito Pantaleo

Dipartimento di Scienze Fisiologiche, Università degli Studi di Firenze, I-50134 Firenze, Italy

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

The role played by the Bötzinger complex (BötC), the pre-Bötzinger complex (pre-BötC), and the more rostral extent ofthe inspiratory portion of the ventral respiratory group (iVRG)in the genesis of the eupneic pattern of breathing was investigatedin anesthetized, vagotomized, paralyzed, and artificially ventilatedrabbits by means of kainic acid (KA, 4.7 mM) microinjections (20-30nl). Unilateral KA microinjections into all of the investigatedVRG subregions caused increases in respiratory frequency associatedwith moderate decreases in peak phrenic amplitude in the BötCand pre-BötC regions. Bilateral KA microinjections into eitherthe BötC or pre-BötC transiently eliminated respiratory rhythmicityand caused the appearance of tonic phrenic activity ("tonic apnea"),whereas injections into the rostral iVRG completely suppressedinspiratory activity. Rhythmic activity resumed as low-amplitude,high-frequency oscillations and displayed a progressive, althoughincomplete, recovery. Combined bilateral KA microinjections (BötCand pre-BötC) caused persistent (>3 h) tonic apnea. Results showthat all of the investigated VRG subregions exert a potent controlon both the intensity and frequency of inspiratory activity, thussuggesting that these areas play a major role in the genesis ofthe eupneic pattern ofbreathing.

Bötzinger complex; breathing control; respiratory neurons

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

BREATHING IN MAMMALS IS RELIANT on a neuronal network located in the lower brain stem. Neuronal mechanisms responsible forgenerating the eupneic pattern of breathing are localized withinthe pons and the medulla oblongata (for reviews, see Refs. 5,57, 62). In the pons, respiratory neurons are mainly concentratedin a region encompassing the nucleus parabrachialis medialis andthe Kölliker-Fuse nucleus, which corresponds to the "pneumotaxiccenter" that controls the inspiratory off switch and, more generally,the timing of the respiratory phases (5, 31, 62). Thispontine region has also been termed the pontine respiratory group,although other populations of respiration-modulated neurons havebeen encountered at scattered locations in the pons (5, 57,62). Evidence has been provided that the pons plays an importantrole in respiratory-rhythm generation and eupneic pattern formation,as only gasping can be generated at the medullary level aftercomplete removal of the pons (see, e.g., Ref. 57 also for furtherreferences). However, the results of several studies (for reviews,see Refs. 5, 41, 43, 47, 62, 63) have led to theproposal that the basic mechanism responsible for rhythm generation,the so-called central pattern generator (CPG), may be locatedwithin the medulla oblongata, where medullary respiratory neuronsare concentrated in two distinct regions: the dorsal (DRG) andventral (VRG) respiratorygroups.

Extensive multiple electrolytic lesions placed in the DRG and VRG of anesthetized or decerebrated cats have caused a gradualdecline in the amplitude of inspiratory activity without affectingthe respiratory rhythm (54, 55). These studies suggest thatthese medullary areas are not crucial for respiratory-rhythm generation.In fact, gradual declines in the magnitude of inspiratory activity,but not in respiratory frequency, are usually considered to reflectblockade of tonic drive and not an impairment of rhythm generation(12, 39, 55, 62). Unilateral focal cold blocks of structureslocated in the rostral ventrolateral medulla (10) caused strongdepression of respiratory rhythmicity or apnea, the latter beingcharacterized by the complete absence of inspiratory activityor by low levels of tonic phrenic discharges ("tonic apnea").A prominent feature of focal cold blocks in the rostral ventrolateralmedulla was an increase in respiratory rate accompanying depressanteffects on inspiratory activity. This "apnea region" extends inthe ventrolateral aspects of the rostral medulla from ~2 mm rostralto the obex to the level of the facial nucleus and overlaps (atleast in part) the inspiratory portion of the VRG, the retrofacialregion (Bötzinger complex; BötC), and the more superficiallylocated chemoceptive regions (10). The neural structures correspondingto the apnea region were not interpreted as possible sites forrespiratory-rhythm generation but, with great caution, were suggestedto be important for chemoceptive and other drive inputs necessaryfor respiratory rhythmogenesis (10). These experiments focusedattention also on structures located outside the DRG and VRG aspossible sites for respiratory-rhythm generation or sources oftonic inputs necessary for the maintenance of eupneic breathing.Other neuronal groups that may constitute components of the apnearegion have been subsequently identified; they include, for example,the retrotrapezoid nucleus and the so-called subretrofacial region(for reviews, see Refs. 5, 57).

The conclusion that both the DRG and VRG were not critical for eupneic breathing has more recently been reevaluated. Severalstudies have led to the identification of a small subregion ofthe rostral VRG that may be crucial for respiratory-rhythm generation.This region was at first identified in an in vitro brain stem-spinalcord preparation of the neonatal rat (48; for reviews, see Refs.5, 41) and subsequently also in adult animals in vivo (13,40, 45, 50, 56 60; for reviews, see Refs. 5, 41). This subregion,named the pre-Bötzinger complex (pre-BötC), corresponds to thetransition zone between the rostral expiratory neurons of theBötC and the inspiratory portion of the VRG (iVRG), which isoften reported in the literature as the rostral VRG (5, 62).The rostral and caudal boundaries of the pre-BötC are not definedwith absolute precision, but in the adult this region of the VRGcan be characterized by the presence of a mix of different typesof inspiratory and expiratory neurons, which are for the mostpart propriobulbar neurons (13, 41, 45, 56, 60). Resultsobtained with electrolytic, radio-frequency, and kainic acid (KA)lesions (29, 53, 58) have suggested that the BötC and rostraliVRG may be crucial in the generation and/or maintenance of therespiratory rhythm. All of these VRG subregions (see also Refs.41 and 57) may be components of the apnea region describedby Budzinska et al. (10).

However, considering the studies performed with different types of lesions and blockades of neuronal activity in the rostralportions of the VRG, including the BötC (29, 53, 58) andthe pre-BötC (2, 10, 18, 21-24, 40, 56; for review, see Ref.57), discrepancies in the results are obvious. Thus the roleplayed by these different VRG subregions in the control of respirationis far from being definitely settled. Most of the above-mentionedstudies have been carried out in cats and rats. The rabbit iswidely used as an experimental model in the study of the neuralcontrol of breathing (e.g., Refs. 5, 8, 32, 62); however,very little information is available on the respiratory functionof the rostral VRG subregions in this animalspecies.

The present study was undertaken in an attempt to get further insights into the role played by the BötC, the pre-BötC, andthe immediately adjacent rostral part of the iVRG in the genesisof the eupneic pattern of breathing of anesthetized, vagotomized,paralyzed, and artificially ventilated rabbits. For this purpose,we have made use of microinjections of the neurotoxin KA (14)to produce lesions systematically placed in different subregionsof the rostral VRG. Preliminary accounts of the present work havealready been presented in abstract form (30).

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Animal preparation. Experiments were carried out on 58 male New Zealand White rabbits (2.8-3.6 kg) anesthetized with a mixture of $alpha$ -chloralose(40 mg/kg iv; Sigma Chemical, St. Louis, MO) and urethane (800mg/kg iv; Sigma Chemical) supplemented when necessary (4 and 80mg/kg, respectively). The adequacy of anesthesia was assessedby the absence of reflex withdrawal of the hindlimb in responseto noxious pinching of the hindpaw. All animal care and experimentalprocedures were conducted in accordance with the Italian legislationand the official regulations of the European Communities Councilon the use of laboratory animals (directive 86/609/EEC). The experimentalprotocol was approved by the Animal Care and Use Committee ofthe University ofFlorence.

After cannulation of the trachea, polyethylene catheters were inserted into a femoral artery and vein for the measurementof arterial blood pressure and systemic administration of drugs,respectively. Both C₅ phrenic roots were dissected free, cut distally,and prepared for recordings. Both cervical vagus nerves were separatedfrom the sympathetic trunks for subsequent vagotomy. The animalwas placed in a prone position and fixed by a stereotaxic headholder and vertebral clamps; the head was ventroflexed to facilitaterecordings from the medulla. The dorsal surface of the medullawas widely exposed by occipital craniotomy, and the dura and arachnoidmembranes were removed. The posterior part of the cerebellum wasremoved by gentle suction to provide access to the rostral partof the medulla. All exposed tissues were covered with warm paraffinoil (37-38°C). Body temperature was maintained within the rangeof 38.5-39.5°C by a heating blanket controlled by a rectal thermistorprobe. The animals were vagotomized, paralyzed with gallaminetriethiodide (4 mg/kg iv, supplemented with 2 mg/kg every 30 min;Sigma Chemical), and artificially ventilated. End-tidal CO₂ partialpressure (PCO₂) was maintained approximately at the level of spontaneousbreathing (28.5-36.5 mmHg) by adjusting the frequency and strokevolume of the respiratory pump. In paralyzed animals, the depthof anesthesia was assessed by monitoring a stable and regularpattern of phrenic activity as well as the absence of fluctuationsin arterial blood pressure, whether spontaneous or in responseto somatic nociceptivestimulation.

Recording procedures. Efferent phrenic nerve activity was recorded with bipolar platinum electrodes from desheathed C₅ phrenic roots, amplified,full-wave rectified, and passed through a leaky integrator (low-passresistor capacitor filter, time constant 100 ms) to obtain a "movingaverage" of the activity usually referred to in the literatureas integrated activity. Extracellular recordings from medullaryneurons were made with tungsten microelectrodes (5-10 M $Omega$ impedanceas tested at 1 kHz). We defined the obex at the most rostral extentof the area postrema for use as a standard point of anatomic reference.Neuronal activity was recorded from rostral expiratory neuronsof the BötC (3.0-4.5 mm rostral to the obex, 2.4-3.4 mm lateralto the midline, and 3.5-4.6 mm below the dorsal medullary surface),from the iVRG (from 0.7 caudal to 2.0 mm rostral to the obex,2.3-3.2 mm lateral to the midline, and 3.0-3.5 mm below the dorsalmedullary surface), and from the transition zone between the BötCand the iVRG where a mix of inspiratory and expiratory neuronsis present (2.1-2.9 mm rostral to the obex, 2.4-3.3 mm lateralto the midline, and 3.5-4.2 mm below the dorsal medullary surface).The latter region has already been studied in the rabbit (32)and may correspond to the so-called pre-BötC described in theadult cat and rat (see, e.g., Refs. 13, 41, 45, 56, 60).Recordings were also performed from the expiratory neurons ofthe caudal VRG (cVRG; 0.8-2.6 mm caudal to the obex, 2.0-2.6 mmlateral to the midline, and 2.0-3.0 mm below the dorsal medullarysurface). Stereotaxic coordinates of the different VRG subregionshave been provided, taking into account animal variability; ineach individual preparation, the rostrocaudal extent of each investigatedregion was smaller than that defined by the above-reported coordinates(see RESULTS). A schematic representation of medullary respiration-relatedregions in the rabbit is provided in Fig. 5A. Strain-gauge manometerswere used for monitoring intratracheal pressure and arterial bloodpressure. PCO₂ was monitored by an infrared CO₂ analyzer (DatexCD-102, Normocap, Helsinki,Finland).

Integrated phrenic nerve activity as well as the signals of the other variables studied were recorded on an eight-channelrectilinearly writing chart recorder (model 8K20, NEC San-ei,Tokyo, Japan). In some experiments, phrenic neurogram and neuronalactivity were also acquired and analyzed by using a personal computerequipped with an analog-to-digital interface (Digidata 1200, AxonInstruments, Forster City, CA) and software (Axoscope, AxonInstruments).

Microinjection procedures and experimental protocol. To ablate neurons while largely sparing fibers of passage, the neurotoxin KA was microinjected (14). This method has widelybeen used to study respiratory network properties in vivo (see,e.g., Refs. 4, 18, 21, 22, 29, 56, 64). Microinjectionsof 4.7 mM KA (Sigma Chemical) were performed via a glass micropipette(tip diameter 10-25 µm) by applying pressure with an air-filledsyringe connected to the micropipette by polyethylene tubing.The drug was dissolved in 0.9% NaCl solution containing 0.1-0.2%Pontamine sky blue dye to mark the injection site and to evaluatethe spread of the injectate. The pH was adjusted to 7.4 with 0.1N NaOH. The volume of the injectate (20-30 nl) was measured directlyby monitoring the movement of the fluid meniscus in the pipettebarrel with a dissecting microscope equipped with a fine reticule.The time taken to inject the solution ranged from 5 to 10 s. Inmost cases, the micropipette was glued to a tungsten microelectrodewith a tip that protruded 100-150 µm from the pipette tip. Therefore,it was possible to perform KA microinjections into the exact samearea from which neuronal activity wasrecorded.

Our main interest was focused on the respiratory effects evoked by KA microinjections performed into the rostral part of theVRG, from ~1.0 to ~4.5 mm rostral to the obex, i.e., in the BötC,in the pre-BötC, as well as in the closely adjacent portion ofthe iVRG. Nevertheless, KA microinjections were also executedinto the other regions of the VRG for comparison (i.e., into theremaining portion of the iVRG as well as into the cVRG). Duringeach experiment, extracellular recordings were first performedto localize the different neuronal aggregates of the VRG. Thedistance between tracks was usually 0.5 mm, but it was reducedto 0.3 mm to more accurately localize some VRG regions, such asthe transition zone (pre-BötC) between the condensed populationof rostral expiratory neurons (BötC) and the almost purely inspiratoryportion of the iVRG. Single-unit recordings of neuronal activitywere also performed to further characterize the pre-BötC region.Unilateral and bilateral KA microinjections were made into themedullary respiratory regions previously defined by extracellularrecordings; we paid maximum attention to place the micropipettetip as far as possible just in the middle of the encountered populationsof respiratory neurons to avoid the spread of the injectate toadjacent regions. Bilateral KA microinjections were executed insome instances with two micropipettes driven by separate micromanipulatorsplaced bilaterally in the medulla; the injections were performedin succession (interval of 20-30 s). In most cases, a single micropipettewas used; it was withdrawn after the first injection and was reintroducedin the corresponding contralateral site to make the second injection.In this case, the interval between the two injections was ~60-120s. Respiratory effects evoked by bilateral KA microinjectionswere followed for at least 120-130 min. Combined bilateral KAmicroinjections were also performed into the BötC and pre-BötCof the same animal. Bilateral microinjections in the second regionwere performed 60-70 min after the completion of the first injections.In some experiments, respiratory changes in response to unilateralKA microinjections were also studied; they were evaluated for~60 min. At that time, a second KA microinjection was executedin the corresponding contralateral site. Control injections ofequal volumes of the vehicle solution were also performed. Insome experiments, bilateral microinjections (20-30 nl) of 4.7mM KA or 160 mM D,L-homocysteic acid (DLH), a broad-spectrum excitatoryamino acid agonist, were made at the same sites previously chemicallylesioned by KA to test neuronal responsiveness and, therefore,indirectly provide an estimate of the extent of the inactivatedarea. Theoretical calculations by Nicholson (35) suggest thatvolumes of 20-30 nl should spread <350 µm in any direction fromthe injection site. In addition, recordings of neuronal activitywithin the injected area and in close vicinity to it were performed60 min or more after the injections to estimate the extent ofKA-inducedlesions.

To evaluate chemical sensitivity during KA-induced respiratory responses, hypercapnic and hypoxic stimuli were employed. Hypercapniawas produced by allowing the animal to inspire an appropriatemixture of CO₂ and O₂ from a large (150 liter) bag; PCO₂ was adjustedat ~30 mmHg higher than the level of spontaneous breathing (rangeof 55-65 mmHg). After a stable PCO₂ level was achieved, hypercapnicstimulation was maintained for at least 3 min. Hypoxia was inducedby allowing the animal to inspire a gas mixture containing 6%O₂ in N₂ for ~2min.

Histology. At the end of the experiment, the brain was perfused with 0.9% NaCl solution and then with 10% formalin solution via a carotidartery. After at least a 48-h immersion in 10% formalin solution,the brain was placed in a hypertonic sucrose solution, frozen,and cut to obtain coronal sections (20 µm thick). Unstained sectionswere used to evaluate the spread of the Pontamine sky blue dye.Sections stained with cresyl violet were used for the histologicalcontrol of pipette tracks and injection sites. The atlas of Sheket al. (46) was used forcomparison.

Data collection and analysis. Measurements were made on paper recordings (paper speed was usually 5-10 mm/s and less frequently 25 mm/s). From the traceof integrated phrenic nerve activity, we derived respiratory frequency(breaths/min), inspiratory time (TI), expiratory time (TE), andpeak amplitude (arbitrary units). When a level of tonic phrenicnerve activity developed in response to KA microinjection (seeRESULTS), it was included in the measurement of peak phrenic amplitude.The rate of rise of integrated phrenic nerve activity was evaluatedwith accuracy on higher speed recordings (paper speed of 25 mm/s).The slope of the straight line drawn from the onset to 90% ofthe maximum level of the phrenic ramp was considered a reliableestimate of the inspiratory rate of rise (see, e.g., Refs. 6,8). Respiratory variables were measured for 10 s both in theperiod immediately preceding each trial (control period) and atscheduled times during KA-induced effects. After the completionof KA unilateral and bilateral microinjections, 30 min were takenbefore changes in respiratory activity were considered to be reliableand were, therefore, evaluated. This time was necessary to allowcomplete inactivation of neurons in the injected area (14, 16)and to avoid confounding effects on respiration due to changesin blood pressure (see RESULTS). In the same periods, systolicand diastolic blood pressure were assessed at 2-s intervals. Meanarterial pressure (MAP) was calculated as the diastolic pressureplus one-third of the pulse pressure. Owing to the small variationsin respiratory variables and MAP within a measurement period,average values for each period were taken as single measurementsfor the purpose of analysis. Statistical analysis of data obtainedfor each VRG subregion was performed by using Wilcoxon signed-ranktests. Kruskal-Wallis nonparametric analysis of variance, followedby Dunn's multiple comparison test, was used in the comparisonsof the effects observed in response to KA microinjections intothe different VRG subregions. Changes in respiratory variableswere expressed as percent variations of control values. All valuesare presented as means ± SE; P < 0.05 was considered assignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Neuronal recordings. The distribution of respiratory neurons showed a consistent rostrocaudal organization. In the most rostral medulla, the BötCcould be easily identified by recordings of almost purely multiunitexpiratory activities with prevailing augmenting discharge patterns(see Ref. 8). This region had an extent $<=$ 1.2 mm in each individualanimal. Immediately caudal to the BötC, a mix of inspiratoryand expiratory neuronal activities was recorded (Fig. 1A). A totalof 72 single units was recorded from this area in 24 preparations.We encountered different types of respiratory neurons, i.e., expiratoryneurons with augmenting discharge patterns (17/72, 23.6%), expiratoryneurons with decrementing discharge patterns or postinspiratoryneurons (13/72, 18.1%), inspiratory neurons with augmenting dischargepatterns (22/72, 30.5%), and phase-spanning neurons (20/72, 27.8%).Some phase-spanning neurons started firing during the expiratoryphase (expiratory-inspiratory; n = 13, 18.1%) and attained a maximumrate during inspiration [in most cases (n = 10) at or close tothe transition from expiration to inspiration]. Other phase-spanningneurons started firing during inspiration (inspiratory-expiratory;n = 7, 9.7%) and reached a firing peak at the transition frominspiration to expiration; these could extend firing into midexpiration(n = 4) or late expiration (n = 3). The patterns of dischargeof these different types of neurons are shown in Fig. 1, B-F.This transition zone, which extends $<=$ 0.7 mm in individual preparations,appears to correspond to the pre-BötC region as defined by neuronalrecordings in the cat and the rat (see, e.g., Refs. 13, 41,45, 56, 60). Caudal to this region, a high concentrationof inspiratory neurons with prevailing augmenting discharge patternswas encountered (multiunit recordings); this area, which correspondsto the iVRG, extended $<=$ 2.5 mm in each preparation. In the mostcaudal part of the VRG, expiratory neurons with prevailing augmentingdischarge patterns were encountered for a rostrocaudal extent $<=$ 1.6 mm (cVRG).

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Fig. 1. Discharge patterns of respiratory neurons encountered in the pre-Bötzinger complex. Each record shows phrenic neurogram (PN) and extracellular neuronal activity (NA). A: mix of inspiratory and expiratory neuronal activities. B: expiratory augmenting discharge pattern. C: expiratory decrementing discharge pattern. D: inspiratory augmenting discharge pattern. E: discharge pattern of an expiratory-inspiratory phase-spanning neuron beginning to fire during expiration with maximum firing rate at the transition between expiration and inspiration. F: discharge pattern of an inspiratory-expiratory phase-spanning neuron starting firing during inspiration with firing peak at the transition between inspiration and expiration and extending its firing into late expiration.

Unilateral KA microinjections. The main purpose of the present study was to investigate the respiratory responses induced by bilateral KA microinjections.Nevertheless, on some occasions, respiratory changes induced byunilateral KA microinjections (performed as a first step) wereevaluated for ~60 min; at that time, the corresponding contralateralmicroinjection was executed. Unilateral KA microinjections intoeither the BötC (n = 6) or the transition zone, where a mix ofinspiratory and expiratory neurons was encountered (i.e., thepre-BötC region; n = 5), produced similar effects. Respiratorychanges observed 30 min after KA microinjections (Table 1) werecharacterized mainly by increases in respiratory frequency accompaniedby moderate decreases in peak phrenic amplitude without significantchanges in the inspiratory rate of rise. The increases in respiratoryfrequency were largely due to reductions in TE associated withsmall decreases in TI (Fig. 2); they were accompanied by the developmentof variable but relatively low levels of tonic phrenic activity.Respiratory effects decreased over time but were still significant60 min after the injection (Table 1). Similar unilateral KA microinjections(n = 5) performed into the rostral part of the iVRG (~1.5 mm rostralto the obex) induced moderate increases in respiratory frequencywithin 30 min that were mainly due to reductions in TE and, toa lesser extent, in TI (Fig. 2); small, not significant decreasesin peak phrenic amplitude and inconsistent changes in the inspiratoryrate of rise were also observed. Significant increases in respiratoryfrequency were still present 60 min after the injection (Table1).

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Table 1. Changes in respiratory variables after unilateral 4.7 mM kainic acid microinjections

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Fig. 2. Respiratory changes induced by unilateral microinjections (30 nl) of 4.7 mM kainic acid (KA) into different subregions of the ventral respiratory group (VRG). Recordings are of integrated phrenic nerve activity (Phr) under control conditions and at different times after the completion of the microinjections performed into the Bötzinger complex (BötC), pre-Bötzinger complex (pre-BötC), and rostral inspiratory portion of the VRG (iVRG).

Bilateral KA microinjections. Bilateral KA microinjections caused similar results independently of the interval scheduled between them. As shown in Fig.3, bilateral KA microinjections into the BötC (n = 15) and thepre-BötC (n = 12) caused loss of respiratory rhythmicity within30 min and the progressive development of a relatively intensetonic phrenic nerve activity (tonic apnea). The level of tonicphrenic nerve activity was significantly higher after KA microinjectionsinto the BötC; the mean amplitudes of tonic phrenic nerve activitywere 39.3 ± 3.1 and 23.5 ± 2.5% of the peak phrenic amplitudein control breaths after bilateral KA microinjections into theBötC and the pre-BötC, respectively (P < 0.05). In both cases,rhythmic activity resumed within 50 min after the injections (Fig.3) as low-amplitude, high-frequency irregular oscillations superimposedon tonic activity and then displayed a progressive recovery. Owingto the presence of tonic activity and the irregular pattern ofbreathing, it was possible to provide an accurate evaluation ofrespiratory variables only ~60 min after KA microinjections. Atthat time, significant increases in respiratory frequency andthe rate of rise of inspiratory activity, which are associatedwith marked reductions in peak phrenic amplitude, were observed.The increases in respiratory frequency were due to marked reductionsin TE combined with less-pronounced decreases in TI. An evaluationof changes in some respiratory variables 60 and 120 min afterKA microinjections is provided in Table 2.

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Fig. 3. Respiratory responses induced by bilateral microinjections (30 nl) of 4.7 mM KA into different subregions of the VRG. Recordings are of integrated Phr under control conditions and at different times after the completion of the microinjections performed into the BötC, pre-BötC, and iVRG.

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Table 2. Changes in respiratory variables after bilateral 4.7 mM kainic acid microinjections

Bilateral KA microinjections (n = 12) into the iVRG from ~1.0-2.0 mm (usually 1.5 mm) rostral to the obex (Fig. 3) inducedapnea without any appearance of tonic phrenic activity within30 min. However, 35-50 min after the injections, low-intensity,high-frequency phrenic bursts progressively appeared. Also inthis case, a reliable evaluation of respiratory variables couldbe performed only 60 min after KA microinjections (Table 2).Respiratory frequency showed marked increases (mainly due to reductionsin TE) accompanied by strong decreases in the peak amplitude ofphrenic nerve activity and no significant changes in the inspiratoryrate of rise. Respiratory activity displayed a progressive andrelatively slow recovery (Table 2); comparisons between changesin respiratory variables observed after KA microinjections intoeach of these three VRG subregions revealed on some occasionsthe presence of small but significant differences (Table 2).

Control injections of equal volumes of the vehicle solution performed at the same locations were without significant effects.Bilateral KA microinjections (n = 12) at sites >0.5 mm away fromthese responsive sites of the BötC, pre-BötC, and iVRG, whereintense multiunit respiratory neuronal activity was encountered,failed to induce the characteristic respiratory responses reportedabove and caused either no change or only transient (<5-min duration),inconsistent changes in respiratory activity. For comparison,bilateral KA microinjections were performed also in more caudalregions of the VRG. Changes in respiratory variables in responseto bilateral KA microinjections (n = 6) from ~0.5 mm rostral to0.7 mm caudal to the obex were less consistent and did not reachthe level of statistical significance. Respiratory responses couldbe completely absent. When present, they were similar to thosedescribed for the more rostral portion of the iVRG but characterizedby much shorter durations; complete recovery occurred within <15min. No appreciable variations in respiratory activity were observedin response to bilateral KA microinjections (n = 5) into the cVRGextending from ~0.8 to 2.6 mm caudal to theobex.

An attempt was also made to evaluate CO₂ and O₂ sensitivity after bilateral KA microinjections into either the BötC (n =3) or the pre-BötC (n = 2) regions. The complete absence of responsivenessto hypercapnic or hypoxic stimuli was observed during tonic apnea;i.e., neither the tonic level of phrenic nerve activity changed,nor did rhythmic activity resume during chemical stimulations.However, both types of chemical sensitivity were present as soonas some rhythmic phrenic nerve activity resumed. Examples of respiratoryresponses to chemical stimuli after KA lesion in the BötC regionare illustrated in Fig. 4. Similarly, after KA lesions in theiVRG, rhythmic respiratory patterns but not apnea turned out tobe affected by hypercapnic or hypoxic stimuli (n = 2).

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Fig. 4. Respiratory responses to hypercapnia and hypoxia before and after bilateral microinjections (30 nl) of 4.7 mM KA into the BötC. Recordings are of integrated Phr under control conditions and at different times after the bilateral microinjections. A: effects of hypercapnic stimulation (from eucapnic values of ~30 to ~58 mmHg). B: effects of hypoxic stimulation (after 2 min of 6% O₂ in N₂).

Combined bilateral KA microinjections were performed into the BötC and the pre-BötC in the same preparation. The injectionswere performed either at first into the BötC and subsequentlyinto the pre-BötC (n = 3) or vice versa (n = 2); they were madejust in the middle of each region so that the distance betweenthem was $>=$ 0.8 mm. Bilateral microinjections into the first regioncaused respiratory changes similar to those already described.Bilateral microinjections in the second region caused loss ofrespiratory rhythmicity and the appearance of tonic phrenic nerveactivity, which, however, did not show any tendency to changeover time (Fig. 5). The absence of recovery of rhythmic respiratoryactivity was ascertained at least for 3 h.

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Fig. 5. Respiratory changes induced by combined bilateral microinjections (30 nl) of 4.7 mM KA performed into the BötC and pre-BötC in the same preparation. A: dorsal view of the medulla oblongata of the rabbit indicating the regions where multiple KA microinjections (

) have been performed. AP, area postrema; cVRG, caudal ventral respiratory group; DRG, dorsal respiratory group. B: integrated Phr under control conditions, 60 min after bilateral KA microinjections into the BötC, and 120 min after subsequent bilateral KA microinjections into the pre-BötC region.

Histological examination of coronal sections of the medulla oblongata revealed the bilateral presence of the Pontamine skyblue marking dye in the injected areas. Each dye spot coveredan approximately spherical area with a diameter that ranged from0.6 to ~0.75 mm. Bilateral microinjections (20-30 nl) of 160 mMDLH (see Ref. 8) into the BötC region (n = 5) or in the regionimmediately caudal to it (n = 3), performed 60 min after KA microinjections,were completely ineffective. Similar DLH microinjections intothese two regions have been proven to cause depressant and excitatoryrespiratory responses, respectively (8, 50). These findingsconfirmed the presence of inactivated or lesioned areas with diameterscomparable to those of the dye spots (see Ref. 35). Similarly,bilateral KA microinjections (20-30 nl) performed into each ofthe investigated VRG subregions 60 min after the completion ofsimilar injections at the same sites did not affect the ongoingrespiratory activity or the recovery process. Finally, recordingsof neuronal activity performed in 15 experiments within KA-injectedareas 60 min or more after the completion of the injections approximatelyalong the injection track and along tracks located in close vicinityto it ( $<=$ 0.4 mm) revealed either the complete absence of neuronalactivity or the presence of very sparse, low-frequency, nonrespiration-relateddischarges. Recordings at different depths along each track enableda determination of the dorsoventral extent of the silent area;the dorsoventral extent showed a maximum range from ~0.6 to ~0.8mm at the level of the injection track and decreased at progressivelyincreasing distances from it. Neuronal activities similar to thoseencountered in control trials were recorded along tracks performedat rostrocaudal distances $>=$ 0.5 mm from the injection site. Anexample of these recordings has been reported in Fig. 6. Takentogether, the results of these trials indicate that the inactivatedregions have diameters ranging from 0.6 to 0.8 mm; i.e., verysimilar to those revealed by the marking dye or expected on thebasis of theoretical calculations (35).

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Fig. 6. Extracellular recordings of neuronal activity performed 70 min after bilateral microinjections (30 nl) of 4.7 mM KA into the pre-BötC. Recordings were made approximately along the injection track at 2.6 mm rostral to the obex and 2.7 mm lateral to the midline (A), as well as along tracks located 2.9 mm (B) and 3.2 mm (C) rostral to the obex (same lateral coordinates). KA microinjections were performed at 3.8 mm below the dorsal surface of medulla. Depth from the dorsal medullary surface is indicated. Neuronal recordings performed at the upper and lower limit of the inactivated area are reported in A (3.4-4.1 mm) and B (3.6-4.0 mm), which show the virtually complete absence of neuronal discharges. Tonic neuronal activity was recorded above and below these depths. Note that the dorsoventral extent of the silent area is ~0.7 mm at the level of the injection track (A) and that it is smaller along the more rostral track (B), thus suggesting the presence of an approximately spherical damaged area. Recordings within a region 0.6 mm rostral to the injection site (C) show patterns of neuronal activity commonly encountered at different depths along control tracks aiming at the BötC. Assuming that the lesioned area is approximately spherical, its maximal rostrocaudal extent can be inferred to be <0.8 mm.

Examples of typical placements of the micropipette within three different medullary regions are shown in Fig. 7. Series ofrepresentative coronal sections of the medulla oblongata of therabbit, showing the distribution of sites where bilateral KA microinjectionsinduced changes in respiratory activity, are represented in Fig.8.

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Fig. 7. Photomicrographs of coronal sections through the medulla oblongata showing examples of typical placements of the micropipette within three different medullary regions. A: coronal section at ~4.0 mm rostral to the obex showing the location of a track (horizontal arrows) along which a microinjection was performed into the BötC. Intense multiunit expiratory activity was recorded at this injection site located just medial to the retrofacial nucleus. B: coronal section at ~2.6 mm rostral to the obex showing the location of a track (horizontal arrows) along which a microinjection was performed into the pre-BötC. A mix of inspiratory and expiratory neurons was encountered at this injection site, which was located in the vicinity of the rostral portion of the nucleus ambiguus. C: coronal section at ~1.2 mm rostral to the obex, showing the location of a track (horizontal arrows) along which a microinjection was performed into the rostral inspiratory portion of the VRG. This injection site was in close vicinity of the intermediate portion of the nucleus ambiguus, where intense multiunit inspiratory activity was recorded. NA, nucleus ambiguus; NOI, nucleus olivaris inferior; NRF, nucleus retrofacialis; NTS, nucleus tractus solitarii; NV, nucleus tractus spinalis nervi trigemini; NXII, nucleus nervi hypoglossi; P, tractus pyramidalis.

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Fig. 8. Series of representative coronal sections of the medulla oblongata of the rabbit showing the distribution of responsive sites where bilateral microinjections of 4.7 mM KA were performed. For simplicity, injection sites (

) are projected on the nearest of the reported sections. Outlines of the maps derive from selected sections of one histological preparation (camera lucida redrawing). The atlas of Shek et al. (46) was used for comparison. Distance in millimeters from the rostral margin of the area postrema (taken as obex level) is indicated at left of each section.

Cardiovascular effects. Although our interest was mainly focused on respiratory effects, we will briefly deal with changes in MAP observed in ourexperiments. Both unilateral and bilateral KA microinjectionsinto rostral sites of the VRG, which correspond to the BötC andpre-BötC, caused similar marked increases in MAP ranging from21 to 90 mmHg. These pressor responses occurred immediately afterthe injections and reached a maximum within ~10 min. Maximum pressorresponses were 27.6 ± 3.3 and 44.4 ± 4.1 mmHg after unilateraland bilateral KA microinjections, respectively (P always < 0.001).Arterial blood pressure progressively decreased and completelyrecovered within <30 min. Transient decreases in MAP, which reacheda maximum (20.3 ± 4.5 mmHg; P < 0.005) within ~10 min, were observedafter bilateral KA microinjections into the iVRG. Transient andinconsistent decreases in MAP were also seen after unilateralKA microinjections into the same area (13.8 ± 4.7 mmHg; P > 0.05).In all instances, blood pressure displayed stable values quitesimilar to those observed during control periods when evaluationof respiratory effects was commenced, i.e., 30 min after KA injections.No obvious or consistent changes in MAP were observed with KAmicroinjections into more caudal sites of theVRG.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The results of this study indicate that important components of the neural network underlying respiratory-rhythm generationare located in the rostral ventrolateral medulla. However, theydo not allow us to ascribe to any lesioned area of the VRG anexclusive role in the generation of the eupneic pattern of breathing.In fact, present data suggest that the BötC, the pre-BötC, andthe rostral portion of the iVRG have similar and potent influenceson the respiratory frequency and intensity of the inspiratorymotoroutput.

KA produces profound metabolic alterations of cell bodies within 30 min while sparing axons of passage; affected neurons havebeen reported to cease firing within 10 min after the injections(14). However, we waited 30 min before evaluating the effectsof KA microinjections (see, e.g., Refs. 16, 58). The effectsobserved in the period immediately after the injections may alsoreflect transient activation of adjacent neuronal systems, assubtoxic levels of KA could diffuse beyond the lesion site (14).Accordingly, KA-induced changes in blood pressure are conceivablydue to the transitory activation of neighboring medullary neuronalpools implicated in cardiovascular regulation, such as the rostraland caudal vasomotor areas (15, 28); these faded out within<30 min from the injection. Therefore, the role of baroceptivereflexes in the genesis of the KA-induced responses can be ruledout (15).

Respiratory responses induced by KA microinjections in the three rostral VRG subregions are rather similar; the main differencesconcern the presence and the level of tonic inspiratory activityduring KA-induced loss of respiratory rhythmicity as well as theintensity of changes in some respiratory variables during therecovery period (see Table 2). Owing to the close proximity ofthese subregions, the spread of the injectate could have playeda role in determining these similarities. However, we are confidentthat the respiratory effects were confined to circumscribed areaslocalized within the VRG. Injection sites were selected by usingstereotaxic coordinates and especially extracellular recordingsof respiratory neurons that are well known to be concentratedaccording to type in rather well-defined subregions of the VRG(5, 41, 62). Our extracellular recordings of neuronal activitiesallowed us to define accurately not only the BötC and the iVRG(5, 62), but also the pre-BötC region (see Fig. 1), wherewe encountered patterns of neuronal activities similar to thosedescribed in other animal species (see, e.g., Refs. 13, 41,45, 56, 60). Furthermore, the localization of the injectionsites was confirmed by the histological control (Fig. 7). Microinjectionswere performed, as far as possible, just in the middle of eachselected subregion to avoid the spread of the injectate to adjacentstructures. To restrict the spread of the injectate and therebythe number of neurons affected, relatively small volumes (20-30nl) of KA solutions were injected. Theoretical calculations (35)suggest that volumes of 30 nl should spread <350 µm in any directionfrom the injection site. Accordingly, KA injections into neighboringregions >0.5 mm away from responsive sites, where intense multiunitrespiratory activity was recorded, failed to induce the characteristicrespiratory effects reported above. Our histological observationson the spread of the marking dye are in keeping with theoreticalsuggestions and provide evidence that we have lesioned circumscribedareas (35). Furthermore, the results of DLH or subsequent KAmicroinjections into KA-lesioned areas, and especially those ofextracellular recordings performed within or close to the injectedregions (see Fig. 6), indicate the presence of lesions with anextent comparable to that expected on the basis of the spreadof the injectate. As already mentioned, subtoxic levels of KAcould diffuse beyond the injection site and cause transient activationof adjacent neurons (14); only the respiratory responses observedimmediately after the injections may reflect these excitatoryphenomena, as also suggested by the time course of KA-inducedchanges in blood pressure observed in the present study. However,we started to evaluate changes in respiratory activity only 30min after the completion of theinjections.

The technique of KA microinjections has widely been used as a useful and reliable tool in the study of the respiratory networkin in vivo preparations (4, 18, 21, 22, 29, 56, 64).KA-induced respiratory effects were specific because control injectionsof equal volumes of the vehicle solution performed at the sameresponsive site did not alter respiratory activity. In addition,specificity is strengthened by the above-mentioned absence ofsignificant respiratory responses to KA injections into neighboringregions >0.5 mm away from the three investigated VRG subregions,as well as by the lack of responsive sites in the cVRG. In fact,although some studies have shown that strong activation of caudalexpiratory neurons may cause respiratory depression and alterthe pattern of breathing (e.g., Ref. 6), the bulk of data fromelectrophysiological, morphological, and lesion studies indicatethat neurons of this region are not involved in the respiratoryrhythmogenesis (see, e.g., Ref. 54; for reviews, see Refs. 5,62). Nevertheless, each injected area could lead to respiratoryresponses via synaptic interactions with the adjacent VRG subregions(for reviews, see Refs. 5, 57, 62). If these responseswere due to the ablations of neurons in the circumscribed injectedsubregion, then they would exactly reflect the results that wewere aiming for and, therefore, would be specific. Furthermore,neurons within the injected area are at first strongly activatedand subsequently cease firing within 10 min after the injection(14). Thus respiratory effects could also be due to synapticinteractions of activated neurons with neighboring regions, whereeither inhibitory or excitatory short-lasting phenomena mightbe produced. In particular, excitatory phenomena in adjacent regionsmay produce local depolarization blocks of neurons. The durationof these blocks cannot be long lasting, because even depolarizationblocks caused by microinjections of large volumes of excitatoryamino acids at high concentrations have relatively short durations(26). We believe that respiratory responses induced by thesesynaptic interactions, if present, should have faded out wellbefore the time at which the evaluation of KA-induced respiratoryeffects wascommenced.

Lesions produced by KA microinjections have been reported to be irreversible (4, 14, 16). However, a progressive albeitpartial recovery of eupneic patterns of breathing was observedin our experiments. At present, the mechanisms underlying thisbehavior are not clear. The hypothesis can be advanced that readjustments,compensation, or plasticity phenomena in the respiratory networkmay subserve the recovery process of respiratory activity. Inagreement with St. John (57), a general aspect of blockadesor lesions of medullary regions leading to respiratory depressionor apnea is that the magnitude of respiratory effects is greatestimmediately after these experimental maneuvers (Ref. 56 alsofor further reference). Furthermore, because KA lesions were relativelysmall, they could have affected only part of each investigatedsubregion; the remaining neurons may have contributed to the recoveryprocess. However, taking into account the relative extent of eachinvestigated area, it seems conceivable that this may be relevant,especially to the iVRG and the BötC, but rather unlikely to thepre-BötC, owing to its very small size. We cannot at presentexclude that an irreversible cessation of rhythmic respiratoryactivity could be induced by completely lesioning each of theinvestigated medullarysubregions.

As we have stated above, we are confident that in most cases the whole pre-BötC region was ablated by our KA microinjections.This is in obvious conflict with the view that the pre-BötC iscrucial for respiratory-rhythm generation in in vivo preparationsof adult mammals (41). However, this contrast seems to be stronglyattenuated by the fact that even authors who support the hypothesisthat pre-BötC pacemaker neurons constitute the kernel for respiratory-rhythmgeneration (47) have recently proposed that purely reciprocalinhibitory interactions could generate a stable respiratory rhythmin the absence of active pacemaker cells; under these circumstances,rhythmogenesis has been suggested (47) to occur as originallyproposed by Richter et al. (42) and demonstrated by a numberof computational models (see, e.g., Refs. 3, 5, 36, 44).Recently it has been suggested that the normal breathing rhythmin mammals is generated within the pre-BötC by neurokinin 1 receptor(NK1R)-expressing neurons, which have been estimated to represent<10% of all pre-BötC neurons (20). Bilateral destructions of>80% of NK1R neurons within the pre-BötC and possibly other neighboringregions of unrestrained awake adult rats did not result in fatalapnea, but in an "ataxic" breathing pattern generally characterizedby increases in frequency associated with an irregular sequenceof inspiratory efforts of near normal amplitude interspersed withapnea or very low-amplitude inspiratory activity (20). Lesionedrats displayed altered blood gases and pH as well as abnormalresponses to hyperoxia, hypercapnia, and hypoxia. Interestingly,no gasping was observed in response to severe hypoxia (for a discussionon the neurogenesis of gasping, see, e.g., Refs. 25, 40, 56,57). On the basis of these results, Gray et al. (20) havesuggested that normal breathing in mammals requires the presenceof NK1R-expressing neurons of the pre-BötC. In the absence ofthese neurons, an irregular rhythm sufficient to maintain lifecan still be produced in awake rats by undetermined structures,which may include, for example, non-NK1R-expressing neurons inthe pre-BötC as well as the VRG or other brain stem respiratorystructures. Thus in agreement with the suggestions of Smith etal. (47), these conclusions seem to imply the possibility thata respiratory rhythm can be generated by interactions within theneuronal network in which kernel neurons are embedded, even whenthese neurons have been silenced or destroyed. The reasons ofthe discrepancies between present results and those of Gray etal. (20) are obscure but are unlikely due to differences inthe animal species employed, because bilateral ablations of thepre-BötC in decerebrate rats (56) proved to cause results consistentwith those observed in the present study. The discrepancies maybe at least partially accounted for by the great differences inthe type of preparation employed and by the very selective lesionsof NK1R neurons within the pre-BötC and possibly neighboringregions performed by means of relatively large-volume microinjections(100-150 nl) in the study by Gray et al. (20). However, howthese differences may have contributed to produce contrastingresults is only a matter ofspeculation.

The finding of apneic responses, albeit transient, in all of the investigated subregions of the rostral VRG may indicate thatwe have operated on important components of the neuronal networksubserving eupneic breathing (see Fig. 3). As far as the BötCregion is concerned, present results are in general agreementwith those previously obtained in the cat with different typesof lesions (53, 58) or focal cold blocks (10). However,the medullary areas involved in some of these studies extendedwell beyond the boundaries of the BötC (10, 58). Persistentor transient apnea was induced by blockades or ablations of neuronalactivities within the pre-BötC or possibly corresponding medullaryregions of cats and rats in some previous studies (10, 21-24,29, 40, 56; see also Ref. 41), but contrasting results wereobtained in other investigations (2, 18). The reasons forthese discrepancies are not clear; they are probably related tothe differences in the preparations and the experimental techniquesused, as well as in the localization and extent of the lesionedor inactivated area. We believe that our results could contributeto disclose the role of these rostral VRG subregions because theyhave been obtained in the same animal species, with the same typeof preparation, and the same technique. Apnea observed in responseto KA injections into the iVRG may be due to the involvement notonly of propriobulbar neurons of the medullary respiratory networkbut also of bulbospinal premotor inspiratory neurons (5, 62).

Despite the similarities in the results obtained in the different subregions, the arrest of the respiratory rhythm was combinedwith the appearance of relatively intense tonic phrenic nerveactivity after KA lesions in the BötC and pre-BötC (see Fig.3). The development of tonic activity has been reported to occurin the cat in response to focal cold blocks in the rostral regionsof the ventrolateral medulla, including the BötC (10). Althoughnot specifically described, tonic inspiratory activity after KAor electrolytic lesions in these subregions can be recognizedin the results of some other studies (see, e.g., Ref. 29, Fig.4; Ref. 53, Fig. 3; Ref. 58, Fig. 4). A plausible interpretationof these findings is that the development of tonic inspiratoryactivity is due to the lack of the potent inhibitory influenceson inspiratory activity arising from rostral expiratory neurons(7, 8; for a review see Ref. 5) that are mainly concentratedin the BötC but are also encountered in the pre-BötC as shownin the present results (see Fig. 1) and described in previousreports (13, 41, 45, 56, 60). Accordingly, it has beenshown that blockade of inhibitory synaptic activity within thepre-BötC of the cat causes the cessation of rhythmic respiratoryactivity and the appearance of tonic phrenic discharges (39).In agreement with the interpretation provided for these latterfindings (39), we can also advance the hypothesis of a prominentrole of pontine influences on the BötC and the pre-BötC in thegenesis of tonic apnea that recalls very closely apneusis inducedby the ablation of the pneumotaxic center (for a review, see Ref.57). Pontine influences on respiration seem to be rather complexand involve both excitatory and inhibitory pathways (5, 11,31, 39, 62); these influences can be mediated at least inpart by afferent projections from parabrachial and Kölliker-Fusenuclei to these two subregions of the VRG (see, e.g., Refs. 5,11, 17, 19, 49, 57). Furthermore, we propose that pontineinhibitory effects on inspiratory activity can be exerted viasynaptic actions on neurons located in the BötC and the pre-BötC(possibly involved in the inspiratory off switch) or in the inhibitionof inspiratory neurons during the expiratory phase (see, e.g.,Ref. 5). Removal of the target neurons may partly correspondto the ablation of the pontine pneumotaxic mechanisms and leadto tonic apnea orapneusis.

An important problem concerning the generation of eupnea (56, 57) is whether apneic regions are critical for rhythm generationor provide a tonic input necessary for eupnea to be expressed.First of all, the neuronal populations encountered in the injectionsites did not display tonic discharge patterns, but rhythmic respiratoryactivities. In addition, KA-induced cessation of rhythmic respiratoryactivity was not reverted by increasing the tonic chemical driveby hypercapnia or hypoxia (see Fig. 4). These considerations suggestthat we provoked lesions of rhythmic populations of respiratoryneurons, which may constitute important elements of the respiratoryCPG. Apnea or respiratory depression insensitive to increasinglevels of arterial PCO₂ has already been reported to occur withcold blocks or lesions in the BötC and pre-BötC regions of catsand rats (10, 56, 58). However, a eupneic rhythm recoveredin response to the activation of peripheral chemoreceptors duringapnea induced by KA in the pre-BötC of the rat (56). We cannotrule out that apnea ensued because KA-lesioned areas are involvedin CO₂ and O₂ chemoreception or in the transmission and integrationof chemical drive inputs (see, e.g., Refs. 10, 34, 38, 51,52, 59; for a review see Ref. 33). However, because lesionedareas were relatively small, whereas multiple sites for centralchemoreception are widely distributed in the brain stem (33),a resumption of rhythmic activity could be expected in responseto both hypoxic and hypercapnic stimulation. In the absence ofsuch recovery, a disruption of important connections in the neuralnetwork subserving respiratory-rhythm generation seems plausible.The question of the neurogenesis of gasping (see, e.g., Refs.25, 40, 56, 57) was not addressed in this research; moreover,our hypoxic stimulations probably were not sufficiently long toinduce gasping in therabbit.

Apneic effects, although dramatic, were reversible; an interesting finding was the increase in respiratory frequency and thedecrease of peak phrenic amplitude observed during the recoveryprocess (see Fig. 3 and Table 2). These changes in respiratoryactivity are consistent with the results of unilateral KA microinjectionsand with those of some previous studies performed on other animalspecies. Increases in respiratory frequency and reductions inpeak phrenic amplitude have been reported to occur during unilateralfocal cold blocks in the rostral ventrolateral medulla (10),as well as after unilateral or bilateral KA or electrolytic lesionsof the BötC or the rostral VRG (29, 58, 64) and after unilateraltetrodotoxin microinjections into the pre-BötC (40). Recentresults obtained in decerebrate cats using excitatory amino acidreceptor antagonists (1) suggest that the VRG contains varioussubregions that differentially affect timing and intensity componentsof the breathing pattern. Although excitatory amino acid receptorblockades do not appear to be directly comparable with KA lesions,it seems relevant to the present discussion that microinjectionsof a specific non-N-methyl-D-aspartate (NMDA) receptor antagonistinto the iVRG induced transient apnea, followed by increases inrespiratory frequency associated with reductions in peak phrenicamplitude. Furthermore, NMDA-receptor antagonism within the samearea caused only increases in respiratory frequency. This subregionmay correspond at least partially to the portion of the iVRG lesionedby means of KA microinjections in the presentstudy.

The recovery of a eupneic pattern of breathing could suggest that the neural structures affected by KA injections do not havea crucial role in the respiratory rhythmogenesis. However, itcould be worth recalling that KA lesions could have affected onlypartially each investigated region. We did not perform injectionsof larger volumes to avoid confounding effects due to the involvementof neighboring areas, especially those located in adjacent subregionsof the VRG. Nevertheless, combined KA lesions in two adjacentsubregions produced apneic responses of much longer duration thatwere possibly irreversible (see Fig. 5). On the other hand, itdoes not seem surprising that the extent of the lesioned VRG areamay be of importance in determining the arrest of the respiratoryrhythm and its duration. Present findings could also suggest thepossibility that multiple brain stem regions and, in particular,pontine structures play a role in the generation of the eupneicpattern of breathing (56, 57). Independent respiratory rhythmscan be recorded on each side of the brain stem after completemidsagittal transections (e.g., Refs. 5, 62). In addition,caudal-to-rostral brain stem transections have demonstrated thattrigeminal motoneurons continue to discharge rhythmic bursts aftera separation of the medulla from the pons; these results suggestthat pontine mechanisms might have an important role in the genesisof the respiratory rhythm (for a review, see Ref. 57). However,the relationships of pontine rhythms to eupnea are unknown. Presentresults more strictly suggest that the different subregions ofthe rostral VRG are part of the respiratory CPG. In fact, therostral VRG subregions appear to control not only the amplitudebut also the frequency of inspiratory bursts (12, 39, 55,62). Respiratory responses to unilateral KA microinjectionsare in agreement with this interpretation (see Fig. 2 and Table1). It is also worth noting that VRG subregions more rostrallylocated have a more prominent role in this control (Table 2).

An attempt can be made to explain the genesis of the rather similar respiratory changes in response to KA lesions in the BötC,pre-BötC, and more rostral portion of the iVRG on the basis ofcurrent models of respiratory rhythmogenesis (see, e.g., Refs.3, 5, 36, 42-44, 47). These models are based on reciprocalinhibitory interactions between different types of propriobulbarneurons and, as more recently suggested (see, e.g., Refs. 43,47), on a combination of a network of inhibitory interneuronsand excitatory pacemaker-like neurons with intrinsic oscillatorybursting properties (hybrid pacemaker-network model). However,these models do not display a high level of anatomic specificity:in most cases, they concern functionally differing groups of neuronswithout taking into account an exact localization within VRG subregions.In addition, the models do not include in the respiratory networkthe pons, which (as already mentioned) has been suggested to havean important role in the genesis of eupnea (57). Thus it israther hard to explain present results in the light of these models.Nevertheless, some general considerations can be of some helpfor this purpose. Interneurons involved in the respiratory rhythmogenesisare inhibitory (GABAergic or glycinergic) and receive inhibitoryinputs (see, e.g., Refs. 5, 37, 43, 47); they are distributedprevailingly in the BötC and pre-BötC but have been also encounteredin the adjacent iVRG (e.g., Refs. 5, 13, 37, 45, 47,60 also for further references). The importance of inhibitoryinteractions in the respiratory-rhythm generation is well documented,especially in adult animals (e.g., Refs. 43, 47); networkrhythmicity may depend on reciprocal inhibition and postinhibitoryrebound that shape the final alternating pattern (e.g., Refs.27, 47). In addition, as already mentioned, even in the hybridpacemaker-network model, purely reciprocal inhibitory interactionscould generate a respiratory rhythm in the absence of activityin the kernel pacemaker cells (47). Inhibitory interactionsand postinhibitory rebound are involved in the synchronizationof neuronal systems (e.g., Refs. 9, 61 also for further references);on the other hand, desynchronization of neuronal oscillating networksby blockade of inhibitory synapses leads to reductions in theintensity of output bursts and increases in frequency (e.g., Ref.9 also for further references). On the basis of these arguments,we can speculate that removal of inhibitory interneurons, whichare mainly concentrated in the BötC, pre-BötC, and adjacentiVRG (5, 37, 39, 47), may produce at first the arrestof respiratory rhythm and subsequently after readjustments andcompensation phenomena in the respiratory network, a resumptionof breathing patterns characterized by decreases in peak phrenicamplitude and increases in respiratory frequency. These patternsof breathing are possibly due to the loss of part of inhibitoryinterneurons and reduced strength of inhibitory synapses (seealso Ref. 44), which cause desynchronization of the respiratorynetwork. We have already provided some comments on the KA-inducedapneic responses; in accordance with the above-mentioned considerations,they are probably due to the sudden deficit of inhibitory mechanismsand might represent a level of network desynchronization beyondwhich the respiratory rhythm cannot begenerated.

In conclusion, present findings show that all of the investigated rostral subregions of the VRG exert a potent control onthe respiratory frequency and intensity of the inspiratory motoroutput, thus suggesting that they are important components ofthe neural network responsible for the generation of the eupneicpattern of breathing. We believe that it is unlikely that a vitalfunction such as respiration would rely on a CPG confined to asmall medullary area. Rather, we agree with the view that therespiratory CPG is a distributed neural system characterized bya great deal of redundancy (63).

	ACKNOWLEDGEMENTS

The authors thank Salvatore Cammarata, Alessandro Aiazzi, and Mario Dolfi for technical assistance, and Adrio Vannucchi forpreparation of theillustrations.

	FOOTNOTES

This study was supported by grants from the Ministero dell'Università e della Ricerca Scientifica e Tecnologica ofItaly.

Address for reprint requests and other correspondence: T. Pantaleo, Dipartimento di Scienze Fisiologiche, Università degliStudi di Firenze, Viale G.B. Morgagni 63, I-50134 Firenze, Italy(E-mail: tito.pantaleo{at}unifi.it).

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.

First published February 28, 2002;10.1152/ajpregu.00579.2001

Received 20 September 2001; accepted in final form 26 February 2002.

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