Neurokinin-1 Receptor-Expressing Cells of the Ventral Respiratory Group Are Functionally Heterogeneous and Predominantly Glutamatergic

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The Journal of Neuroscience, May 1, 2002, 22(9):3806-3816

Neurokinin-1 Receptor-Expressing Cells of the Ventral Respiratory Group Are Functionally Heterogeneous and Predominantly Glutamatergic
Patrice G. Guyenet, Charles P. Sevigny, Matthew C. Weston, and Ruth L. Stornetta
Department of Pharmacology, University of Virginia, Charlottesville, Virginia 22908

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

According to a recent theory (Gray et al., 1999) the neurokinin-1 receptor (NK1R)-immunoreactive (ir) neurons of the ventralrespiratory group (VRG) are confined to the pre-Bötzinger complex(pre-BötC) and might be glutamatergic interneurons that driverespiratory rhythmogenesis. In this study we tested whether theNK1R-ir neurons of the VRG are glutamatergic. We also examinedwhether different groups of NK1R-ir neurons coexist in the VRGon the basis of whether these cells contain preproenkephalin (PPE)mRNA or project to the spinalcord.
NK1R immunoreactivity was found in two populations of VRG neurons that are both predominantly glutamatergic because most ofthem contained vesicular glutamate transporter 2 mRNA (77 ± 9%;n = 3). A group of small fusiform neurons (somatic cross section:91 ± 3.6 µm²) that has neither PPE mRNA nor spinal projections is primarilyrestricted to the pre-BötC. These cells may be the interneuronsthe destruction of which produces massive disruptions of the respiratoryrhythm (Gray et al., 2001). The rest of the NK1R-ir neurons ofthe VRG are multipolar, are larger (somatic cross section: 252± 15 µm²), and express high levels of PPE mRNA. Some of these cells locatedin the rostral half of the rostral VRG project to the spinal cord(C4 or T3). Using electrophysiological methods, we showed thatthese bulbospinal NK1R-ir neurons are slowly discharging inspiratory-augmentingneurons, suggesting that they may control phrenic or intercostalmotorneurons.
In summary, NK1R-expressing cells of the VRG are a heterogeneous group of predominantly glutamatergic neurons that includesubpopulations of respiratory premotorneurons.

Key words: pre-Bötzinger complex; respiration; respiratory rhythm generation; vesicular glutamate transporters; VGLUT2; substance P; opioid peptides; preproenkephalin; premotor neurons

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The pre-Bötzinger complex (pre-BötC) contains a distinctive mix of propriomedullary neurons with respiratory discharges(Ellenberger and Feldman, 1990; Connelly et al., 1992; Dobbinsand Feldman, 1994; Schwarzacher et al., 1995). Acidification orchemical activation of the pre-BötC greatly increases respiratoryrate, indicating that this restricted region of the ventral respiratorygroup (VRG) regulates or perhaps generates the respiratory rhythm(Chitravanshi and Sapru, 1999; Solomon et al., 1999, 2000). Inneonate preparations in vitro, the pre-BötC is the source ofa respiratory-like rhythm that is transmitted polysynapticallyto hypoglossal or phrenic motor neurons (Smith et al., 1991; Feldmanand McCrimmon, 1999). This periodic activity is driven by a kernelof glutamatergic neurons that includes cells with intrinsic burstingproperties (Johnson et al., 1994; Butera et al., 1999a,b; Lieskeet al., 2000; Rekling et al., 2000). The recently proposed hybrid-pacemakernetwork theory of respiration (Feldman and McCrimmon, 1999; Smithet al., 2000) postulates that rhythm generation in vivo mightalso be driven by this kernel of pre-BötC excitatory interneuronsrather than by reciprocal interactions between sets of inhibitoryneurons (Duffin et al., 1995).

The adult characteristics of the glutamatergic neurons that drive the respiratory-like rhythm of neonate brainstem preparationsare unknown, although several lines of evidence suggest that thesecells might be identifiable by their high level of expressionof neurokinin-1 receptors (NK1Rs) (Gray et al., 1999, 2001). However,this theory is based on three basically undemonstrated assumptions:namely, the NK1R-immunoreactive (ir) cells of the adult VRG areglutamatergic neurons and confined to the pre-BötC, they arepropriomedullary, and they are functionallyhomogeneous.

NK1R immunoreactivity is detectable in a subset of VRG neurons that are neither cholinergic nor catecholaminergic and generallylack markers of inhibitory transmission [glutamic acid decarboxylase67 (GAD 67) and glycine transporter-2] (Liu et al., 2001; Pilowskyand Feldman, 2001; H. Wang et al., 2001). A major alternativeleft by elimination is that the NK1R-ir cells of the VRG are glutamatergic(H. Wang et al., 2001). To address this question directly we testedin the present study whether the NK1R-ir cells of the VRG containthe mRNA that encodes vesicular glutamate transporter 2 (VGLUT2)(Aihara et al., 2000; Bai et al., 2001; Fremeau et al., 2001).VGLUT2 is a diagnostic marker of glutamatergic neurons (Fremeauet al., 2001), especially in the cardiorespiratory portion ofthe brainstem reticular formation (Stornetta et al., 2002a).

To determine whether VRG NK1R-ir cells are a functionally homogeneous population, we analyzed the pattern of expression ofanother marker, preproenkephalin (PPE) mRNA and found that thismarker is associated with two morphologically different typesof VRG NK1R-ir neurons. To test whether the NK1R-expressing cellsare confined to the Pre-BötC and exclusively propriomedullary,we examined whether any of them project to the cervical and thoraciccord. Having confirmed that some of them are bulbospinal (H. Wanget al., 2001), we tested whether these bulbospinal NK1R-ir neuronscould be some form of respiratory premotorneuron.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

All experiments were performed on male Sprague Dawley rats (250-350 gm; Hilltop Laboratories, Scotsdale, PA) in accordancewith National Institutes of Health and institutional animal careand use guidelines. All procedures and protocols were approvedby the University of Virginia's Animal ResearchCommittee.

Recording and juxtacellular labeling of rostral VRG bulbospinal inspiratory neurons. Anesthesia was induced with 5% halothanein 100% oxygen. During surgery, the rats (n = 9) were artificiallyventilated with 1.6-1.8% halothane in 100% oxygen via a trachealcannula (50-60 cycles/min; 1-1.2 ml/100 gm). End-expiratory CO₂was maintained between 4.5 and 5% during surgery, and rectal temperaturewas kept between 37.5 and 38.5°C. A femoral artery and a veinwere catheterized to record arterial blood pressure (AP) and toadminister drugs, respectively. The rats were placed in a stereotaxicframe, and the right phrenic nerve was isolated as described previously(Guyenet and Wang, 2001). A concentric bipolar stimulating electrode(Rhodes Medical Instruments, Woodland, CA; diameter 250 µm; tipseparation 500 µm) was placed in the fascia surrounding the mandibularbranch of the left facial nerve to elicit antidromic field potentialsin the facial motor nucleus (Schreihofer and Guyenet, 1997). Asecond bipolar electrode was inserted into the left lower quadrantof spinal segment C4 and used to test for spinal axonal projectionsof neurons recorded in the rostral VRG (monophasic square pulses;100 µsec duration; 50-400 µAintensity).

After completion of surgery, halothane was turned off and replaced by urethane administered intravenously to a final doseof 1 gm/kg. This dose was sufficient to maintain anesthesia ata level at which a strong pinch of the tail or hindpaw producedno retraction and no change in arterial pressure or phrenic nervedischarge (PND). After 45 min, the muscle relaxant pancuroniumwas administered (1 mg/kg, i.v., with 0.3-0.5 mg/kg supplementsas required), ventilation was adjusted so that end-expiratoryCO₂ was ~1% above the threshold of the phrenic discharge (~5.5%),and electrophysiological recordings were initiated. Under paralysis,the adequacy of the anesthesia was gauged by the lack of effectof the above-mentioned nociceptive stimuli on AP and PND rateor amplitude. Additional urethane (0.2 gm/kg) was administeredas needed. During the recording period, the mean AP of the ratswas between 125 and 140mmHg.

PND (bipolar recordings, 200-3000 Hz) was full-wave rectified and filtered (Guyenet and Wang, 2001). Unit activity was recordedwith glass electrodes filled with 0.5 M sodium acetate containing1.5% biotinamide (MW 367.3; Molecular Probes, Eugene, OR), pH4.5, using an intracellular amplifier in bridge mode (Axoclamp2A), and the signal was further processed through an AC amplifier(100× gain; 0.2-3 kHz bandpass; 60 Hz notchfilter).

The region of the rostral VRG (rVRG) was determined in each rat with reference to the location of the caudal pole of the facialmotor nucleus. Our previous experiments have suggested that thepre-BötC is centered ~0.8 mm behind the facial motor nucleus(0.6-1.1 mm) (Guyenet and Wang, 2001; H. Wang et al., 2001). Inspiratoryaugmenting neurons beyond 1.2 mm caudal to the facial motor nucleuspredominate, suggesting that this region corresponds to the rVRG.The latter region (1.2-1.5 mm caudal to the facial motor nucleus)was selectively targeted in the present study to record from putativebulbospinal inspiratory premotor neurons. The classification ofrespiratory neurons was based on the timing of their dischargein relation to that of the phrenic nerve using accepted nomenclature(Schwarzacher et al., 1995; Feldman and McCrimmon, 1999).

Recorded neurons were individually filled with biotinamide using the juxtacellular labeling method (Pinault, 1996; Schreihoferand Guyenet, 1997; Schreihofer et al., 1999). The activity ofthe unit was monitored during the entire labeling procedure (30sec to 2 min) to insure that only one recorded cell was beingentrained.

All physiological variables (AP, end-expiration CO₂, PND, integrated PND, and unit activity) were monitored and stored ona PC with a Power 1401 interface and version 3 of the Spike2 software(both from Cambridge Electronics Design Ltd., Cambridge, UK).Analog signals were sampled at 11,120 Hz for spikes, 4600 Hz forPND, and 100 Hz for AP, integrated PND, and end-expiratory CO₂.Action potential frequency was measured by binning spikes into50 msec intervals. To make the final illustrations, representativeexcerpts of the Spike2 data files were exported into a drawingprogram (Canvas 6, Deneba, Miami,FL).

After juxtacellular labeling of two to four rVRG inspiratory neurons, the rats were deeply anesthetized with 4% halothanein 100% O₂. They were then perfused through the ascending aortawith 250 ml of PBS, pH 7.4, followed by 4% phosphate-buffered(0.1 M), pH 7.35) paraformaldehyde (Electron Microscopy Sciences,Fort Washington, PA). The brainstem was removed and stored inthe same fixative overnight at 4°C. Series of coronal sections(30 µm) were cut through the medulla using a vibrating microtomeand stored in cryoprotectant solution at 20° C for up to 2 weeks(20% glycerol plus 30% ethylene glycol in 50 mM phosphate buffer,pH 7.4) until histologicalprocessing.

Injections of retrograde markers. In three rats anesthetized with a mixture of ketamine (75 mg/kg), xylazine (5 mg/kg), andacepromazine (1 mg/kg) administered intramuscularly, the retrogrademarker Fluoro-Gold (FG; Fluorochrome, Inc., Englewood, CO) (Schmuedand Fallon, 1986) was injected iontophoretically into the leftventral horn of spinal segment C4. Two to four penetrations witha recording electrode were used to identify the phrenic motornucleus, and then the recording electrode was withdrawn and amicropipette filled with 3% FG in 0.9% NaCl was inserted in itsplace. Fluoro-Gold was ejected by iontophoresis (5 sec pulses;50% duty cycle; 5 µA positive current; 20 min) using a constantcurrent source. Two more rats received pressure injections ofFG into segment C4 (six sites, three on each side; 40 nl per site;2% FG in normal saline). These injections were targeted at theventral horn (1 mm from midline, 1.6 mm below dorsal surface)and separated by 1 mm in the rostrocaudal direction. Finally,two more rats received pressure injections of FG into segmentT3 (same volume), also targeted at the ventral horn (lateral 0.7mm; depth 1.3 mm). In the four rats subjected to pressure injectionsof FG, a 2- to 3-mm-long necrotic center was observed at the injectionsite, and intense FG fluorescence extended over approximatelytwo spinal segments. At the end of surgery, all rats were treatedwith the antibiotic ampicillin (100 mg/kg) and the analgesic ketorolac(0.6 mg/kg, s.c.). None of the injections produced obvious behavioralor motor deficits after 24 hr. All rats with spinal injectionsof FG were allowed to survive for 8 d, and then they were anesthetizedwith urethane (1.8 gm/kg, i.p.) and perfused with formaldehydeas describedabove.

Preparation of digoxigenin-labeled RNA probes for histological detection of VGLUT2 mRNA and PPE mRNA by in situ hybridization.Both digoxigenin-labeled cRNA probes were prepared as describedpreviously (Stornetta et al., 2001, 2002a). The antisense cRNAriboprobe for rat PPE was transcribed from a 1132 bp DNA templateinserted into the EcoRI site of Bluescript SK+ (Stratagene, LaJolla, CA) (Stornetta et al., 2001). The PPE construct was kindlysupplied and previously characterized by R. Howells (Universityof Medicine and Dentistry of New Jersey-NJ Medical School) (Raoand Howells, 1992). The antisense cRNA riboprobe for rat VGLUT2was transcribed from a 1119 bp DNA template inserted into theTOPO cloning site of pCRII-TOPO (Invitrogen, Carlsbad, CA) (Stornettaet al., 2002a). Both PPE and VGLUT2 antisense riboprobes weresynthesized in an in vitro polymerization reaction using appropriateRNA polymerases (VGLUT2: SP6; PPE: T3; Promega, Madison, WI) inthe presence of digoxigenin-11-UTP (Roche Molecular Biochemicals).The efficiency of digoxigenin-11-UTP incorporation was estimatedby direct immunological detection on dot blots using a sheep polyclonalanti-digoxigenin antibody (Roche MolecularBiochemicals).

Histochemistry. All histochemical procedures were done using free-floating sections removed from the cryoprotectant mixtureand rinsed three times in 1× Dulbecco's sterile PBS, pH 7.4. Hybridizationhistochemistry was performed as described previously (Stornettaet al., 2001, 2002a). Briefly, digoxigenin was revealed with asheep polyclonal anti-digoxigenin antibody conjugated to alkalinephosphatase (Roche Molecular Biochemicals), and alkaline phosphatasewas reacted with nitro-blue tetrazolium (NBT) and 5-bromo-4-chloro-3-indolyl-phosphate,4-toluidine salt (BCIP). Previous testing has established thespecificity of our probes (Stornetta et al., 2001, 2002a). Absenceof labeling in facial, hypoglossal, and ambigual motor neuronswas taken as quality standard because these cells are the mostprone to exhibit nonspecific NBT/BCIP reaction product under suboptimalconditions. The in situ hybridization protocol was always performedbefore any immunohistochemistry, i.e., before detection of NK1R,biotinamide, or FG (Schreihofer and Guyenet, 1997; H. Wang etal., 2001). Briefly, NK1R immunoreactivity was detected usinga guinea-pig polyclonal antibody (1:1000 dilution; Chemicon International,Temecula, CA), followed by a goat anti-guinea pig IgG conjugatedto Cy3 (1:200 dilution; Jackson ImmunoResearch Laboratories, WestGrove, PA). FG was detected using a rabbit polyclonal antibody(1:10,000 dilution; Chemicon) followed by anti-rabbit IgG conjugatedto Alexa 488 (Molecular Probes). Biotinamide (juxtacellular labeling)was revealed with streptavidin Alexa 488 (1:200 dilution; MolecularProbes). The sections were mounted in sequential rostrocaudalorder onto slides, dried, and covered with Vectashield (Vector,Burlingame, CA). No label was observed in the absence of any ofthe primary antibodies. In one experiment, NK1R immunoreactivitywas detected using the NK1R antibody that was originally usedto define the distribution of this receptor (Nakaya et al., 1994).This reagent was kindly provided by Dr. Ryuichi Shigemoto (NationalInstitute for Physiological Sciences, Myodaiji, Okazaki, Japan).In this experiment the avidin-biotin method was used to detectNK1R immunoreactivity as described previously (H. Wang et al.,2001). The NK1R antibodies used in the present study, like thoseused by other investigators previously, are directed against theC-terminal end of the classic long form of the NK1 receptor (Nakayaet al., 1994; Brown et al., 1995; Gray et al., 1999). These antibodiesshould not be able to detect the alternatively spliced form ofthe NK1 receptor, which lacks the C terminus (Fong et al., 1992;Li et al., 1997).

Mapping and imaging. The sections were examined under dark-field illumination to identify the two sections that containedour chosen diagnostic landmarks. The first landmark was the verycaudal end of the facial motor nucleus, which was assigned thelevel 11.6 mm caudal to bregma according to the atlas of Paxinosand Watson (1998). The second landmark was the rostral end ofthe lateral reticular nucleus, where this structure displays alateral and a medial portion as opposed to a single outline. Thesection corresponding to that landmark was assigned the level13.0 mm caudal to bregma according to the nomenclature of Paxinosand Watson (1998). The theoretical distance between the two landmarksections (1.4 mm) closely matched the actual distance representedby the product of the number of intervening sections times thesection thickness (30 µm). Therefore the bregma level of the interveningsections was determined arithmetically by their location relativeto the two landmarksections.

The outlines and major landmarks of the sections of interest were drawn under dark-field illumination using a motor-drivenmicroscope stage controlled by the Neurolucida software as describedpreviously (Stornetta and Guyenet, 1999). This system was alsoused to map the location of the neurons of interest using a 40×or 25× objective and to draw the outline of cell somata undera 100× objective. The Neurolucida files were exported to the NeuroExplorersoftware (MicroBrightfield, Colchester, VT) to count the varioustypes of neurons within a defined area of the reticular formationor to obtain measurements of soma size, including circumference,area, and ferets. The Neurolucida files were exported to the Canvas6software drawing program for final modifications. Photographswere taken with a 12-bit color CCD camera (CoolSnap, Roper Scientific,Tucson, AZ; resolution 1392 × 1042 pixels) (Stornetta et al.,2002a). The neuroanatomical nomenclature is after Paxinos andWatson (1998).

Statistics. The average linkage method of cluster analysis (SAS v. 8.2; procedure: cluster) was applied to the coordinatedata of Figure 7 (spikes per burst vs conduction velocity). Beforethe technique was applied, the variables were first standardizedto variables with mean 0 and SD 1. The cubic clustering criterionand the pseudo F statistic identified two clusters as the optimalnumber of clusters. Other methods of cluster analysis were alsoapplied and yielded the same results. Group data are expressedas means ± SEM and were compared by ttest.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

VGLUT2 mRNA is present in most of the NK1R-ir neurons of the ventral respiratory group

To test whether NK1R-ir neurons of the VRG are glutamatergic, we determined whether these neurons express the mRNA encodingthe vesicular glutamate transporter VGLUT2, the predominant vesiculartransporter subtype found in the brainstem. To also test whethersome of these cells project to the spinal cord, these experimentswere performed in three rats that had received an iontophoreticinjection of FG into the ventral horn of spinal segment C4. Theresulting injection sites were spherical, confined to the leftventral horn with variable encroachment on lamina 6, and sparedthe white matter. The ensuing pattern of retrograde labeling inthe VRG was used to pinpoint the location of the rVRG/pre-BötCtransition because this level is characterized by an abrupt reductionin the density of bulbospinal neurons with projections to thephrenic motor nucleus (Ellenberger and Feldman, 1990; Dobbinsand Feldman, 1994; Feldman and McCrimmon, 1999).

The histological appearance of neurons containing VGLUT2 mRNA is shown in Figure 1A-D,F. Examples of neurons that containedboth VGLUT2 mRNA and NK1R immunoreactivity are also shown in Figure1E,F. VGLUT2 mRNA was absent from fiber tracts (e.g., pyramidaltract) (Fig. 1A) and from cholinergic neurons that were assumednot to use glutamate as transmitter, such as hypoglossal (Fig.1B) or ambigual motor neurons (Fig. 1C). VGLUT2 mRNA was foundin vast numbers of inferior olivary neurons as expected (Fremeauet al., 2001; Stornetta et al., 2002a) (Fig. 1A). Neurons expressingVGLUT2 were abundant in the VRG at the level of the pre-BötC(Fig. 1C). The rVRG, identified by the large number of cells retrogradelylabeled from the C4 ventral horn, also contained many VGLUT2-positiveneurons (Fig. 1D).

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Figure 1. VGLUT2 mRNA in the NK1R-ir neurons of the VRG. A, VGLUT2 mRNA is present in the inferior olive (IO) but absent from the pyramidal tract (pyr). B, VGLUT2 mRNA is absent from the hypoglossal motor nucleus (XII). C, VGLUT2 mRNA is present in the pre-BötC (bregma $-$ 12.4 mm) but absent from nucleus ambiguus (NA). D, VGLUT2 mRNA is present in the rVRG (bregma $-$ 13.0 mm). NK1R-ir neurons shown under fluorescence illumination in E contain VGLUT2 mRNA as seen under bright-field in F (arrows show two double-labeled neurons). Scale bars (shown in A): A-D, 100 µm; (shown in F): E, F, 20 µm.

Five classes of cells could be distinguished on the basis of the presence of one or more of the three markers (VGLUT2, FG,NK1R). Computer-assisted mapping of these cells was done at sixmedullary levels (11.7, 12.06, 12.42, 12.78, 13.16, and 13.52mm behind bregma). Mapping was done only in the ventrolateralmedulla on the side ipsilateral to the spinal injection, althoughthe number of bulbospinal projections from the VRG appeared similaron both sides. This symmetry was expected because most VRG inspiratorypremotor neurons have bilateral projections in the rat (Duffinet al., 2000). Cells were counted within a 750 × 500 µm box delineatingthe VRG (Fig. 2). The box was positioned so that the middle ofits upper side coincided with the bottom of the compact portionof nucleus ambiguus. This nucleus is easily identifiable rostrally(bregma $-$ 11.7 to $-$ 12.7 mm) in tissue stained for NK1R becauseof its very high level of immunoreactivity. Caudal to this levelthe nucleus ambiguus is ill-defined, and the counting box wascentered in the VRG around a well defined, roughly circular clusterof FG-labeled neurons presumed to consist primarily of inspiratorypremotor neurons (Fig. 2) (bregma level $-$ 13.0 mm).

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Figure 2. Rostrocaudal distribution of five cell types at four levels of the VRG. Five categories of cells are shown in four sections from a single representative brain. Neurons that contained only VGLUT2 mRNA are not represented. The 750 × 500 µm box outlines the region of the medulla where cell counts were made. Numbers on each section refer to location relative to bregma (in millimeters). FG, Cells immunoreactive for Fluoro-Gold retrogradely transported from spinal cord C4; NA, nucleus ambiguus pars compacta; IO, inferior olive; pyr, pyramidal tract.

The example shown in Figure 2 illustrates that at the level of the pre-BötC (12.42 mm behind bregma), the vast majority ofthe NK1R-ir neurons contained VGLUT2 mRNA (filled triangles).At more caudal levels (12.78 and 13.0 mm behind bregma), thiswas still the case, but, in addition, a fraction of the NK1R-irneurons also projected to C4 (stars). Large NK1R-ir neurons devoidof VGLUT2 mRNA were frequently encountered outside the VRG alongthe ventral surface of the medulla (Fig. 2, all levels). Theseneurons may be GABAergic (H. Wang et al., 2001). Smaller NK1R-irneurons devoid of VGLUT2 mRNA were found more frequently in theBötzinger region (Fig. 2) (bregma $-$ 12.06 mm). At this very rostrallevel, a few of these cells may be cholinergic neurons (H. Wanget al., 2001).

The average cell counts from three rats are shown in Figure 3. Figure 3A represents the rostrocaudal distribution of bulbospinalneurons within the VRG on the side ipsilateral to the spinal injection.The largest concentration of bulbospinal cells was found caudalto bregma $-$ 12.7 mm, identifying this level as the rostral tipof the rVRG. Within the rVRG, >90% of the bulbospinal neuronscontained VGLUT2 mRNA (Fig. 3A), consistent with the known presenceof large numbers of bulbospinal inspiratory glutamatergic premotorneurons at this level (Dong and Feldman, 1995; Dong et al., 1996).The rostral half of the rVRG contained bulbospinal neurons thatexpressed both VGLUT2 mRNA and NK1R immunoreactivity (Fig. 3A).Strikingly, 100% of the NK1R-ir neurons identified as bulbospinalalso contained VGLUT2 mRNA.

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Figure 3. Most NK1R-ir neurons of the VRG contain VGLUT2 mRNA. A, Rostrocaudal distribution of bulbospinal neurons within the 750 × 500 µm box defined in Figure 2. Spinally projecting (FG⁺) NK1R-ir neurons were concentrated at the rostral end of the rVRG. B, Rostrocaudal distribution of NK1R-ir neurons. The vast majority of NK1R-ir neurons, including 100% of the bulbospinal ones, contained VGLUT2 mRNA. Ordinate indicates mean ± SE number of neurons counted per section on the side ipsilateral to the FG injection (n = 3 rats). FG was iontophoretically injected into the ventral horn at C4. The bars above the graphs indicate our best estimate of the minimum probable rostrocaudal extent of the Bötzinger, pre-BötC, and rVRG based on this study and previous electrophysiological work (Guyenet and Wang; 2001; H. Wang et al., 2001).

Figure 3B shows that a large majority of the NK1R-ir neurons (bulbospinal plus others) expressed detectable levels of VGLUT2mRNA. The proportion varied from 67% at the rostral end of theVRG (Bötzinger region) to 100% at the caudal end (rVRG). Theaverage for the entire VRG (all five levels pooled) was 76.6%,although this figure varied between animals (60, 80, and 89.8%).This intersubject variability probably reflects differences inthe detection of the VGLUT2 mRNA NBT/BCIP reaction product, andthus the highest figure (89.8%) may be closest to the truth (seeDiscussion for methodologicalconsiderations).

PPE mRNA defines two classes of VRG NK1R-ir neurons

PPE mRNA is expressed by many neurons within the cardiorespiratory region of the rostral ventrolateral medulla (Stornettaet al., 2001b). The following experiments performed in six ratswere designed to determine whether PPE mRNA is expressed by someof the NK1R-ir neurons of the VRG. Two animals received largebilateral FG injections in cervical segment C4, and two othersreceived similarly large bilateral injections into spinal thoracicsegment T3. The ensuing pattern of retrograde labeling in theVRG was used to identify the location of the rVRG/pre-BötC transition(see above). The larger pressure injections were designed to maximizethe number of retrogradely labeled bulbospinal neurons in theVRG. We also used tissue from two of the three rats that had receivedsmall iontophoretic injections of FG into the phrenic motor nucleus.A one in six series of sections (180 µm apart) from each of thesix rats was processed for the simultaneous detection of PPE mRNA,NK1R-ir, and FG immunoreactivity. Mapping was done only in theventrolateral medulla on the left side of thebrain.

The presence or absence of PPE mRNA defined two classes of VRG NK1R-ir neurons with differing somatic sizes but equally intenseimmunoreactivity (Fig. 4). The NK1R-ir neurons devoid of PPE mRNAhad small fusiform cell bodies from which one or usually two primarydendrites emerged in the coronal plane (Fig. 4A,C). The NK1R-irneurons that expressed PPE mRNA were larger and generally multipolar(Fig. 4B,E,F). The difference in size and cell body morphologybetween these neurons is further illustrated by high-magnificationconfocal photomicrographs in Figure 4, A and B. Computer-aidedmeasurements of somatic size (perimeter, cross-sectional area,largest width, and length) were made in neurons of each classselected at random in the VRG between bregma $-$ 12.2 and $-$ 12.9 mm.These measurements revealed a striking 2.5-fold difference inaverage cross-sectional area between the PPE mRNA expressing NK1R-ircells and the rest of the NK1R-ir cells, with very little overlapbetween the two populations (Table 1). The absence of PPE mRNAsignal in the small NK1R-ir neurons of the VRG was not causedby a lack of sensitivity of the hybridization method, becauseequally small or smaller neurons within the nucleus of the solitarytract routinely expressed high levels of PPE mRNA reaction product(result not illustrated).

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Figure 4. Cell size and presence of PPE mRNA define two types of NK1R-ir neurons in the VRG. A, B, Confocal images of a cluster of small NK1R-ir neurons within the pre-BötC (A) and of a large isolated NK1R-ir neuron of the rVRG (B, arrow). The inside of the cell shown in B is especially dark because Cy3 fluorescence is quenched by dense VGLUT2 mRNA reaction product. C, D, Light microscopic images of a cluster of small neurons of the pre-BötC under fluorescence (C) and bright-field illumination (D). The NK1R-ir cells (C, arrows) are devoid of PPE mRNA (D) but are surrounded by neurons lacking NK1R immunoreactivity that express high levels of PPE mRNA. E, F, Light microscopic images of a large NK1R-ir neuron of the rVRG under fluorescence (E) and bright-field illumination (F). The dendrites of this cell display intense NK1R immunofluorescence (E), whereas in the cell body, NK1R immunofluorescence is quenched by the very high level of PPE mRNA reaction product (F). Scale bars (shown in B): A, B, 20 µm; (shown in F): C-F, 50 µm.


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Table 1. Cross-sectional area of NK1R-ir neurons with or without PPE mRNA

The rostrocaudal distribution of the two classes of NK1R-ir neurons (with and without PPE mRNA) was also different (Fig. 5).This figure describes the location of five classes of neuronsdefined by the presence or absence of the three histological markers(NK1R, FG, PPE mRNA) within the 750 × 500 µm box defined in Figure2. On the basis of the pattern of retrograde labeling from thecord, the rVRG/pre-BötC transition point was found again at Bregma $-$ 12.7 mm (Fig. 6A). The same transition point was identified regardlessof whether FG was injected in C5 or T3 or by pressure injectionor iontophoresis. The distribution of bulbospinal neurons shownin Figure 5A is therefore an average of the six animals. In agreementwith our previous results, NK1R-ir neurons were broadly distributedwithin the VRG, with a peak located just rostral to rVRG (Fig.5A). The small NK1R-ir neurons devoid of PPE mRNA were concentratedaround bregma $-$ 12.3 mm, and their number decreased abruptly inthe rVRG (caudal to bregma $-$ 12.7 mm), a structure identified byits large number of bulbospinal neurons (Fig. 5B). Thus the bulkof the small fusiform NK1R-ir neurons is located in the pre-BötC,although cells with apparently similar characteristics are alsopresent in the Bötzinger region. A very rough estimate of thenumber of fusiform NK1R-ir and PPE-negative cells present perside in the area defined at pre-BötC (Fig. 2, box) over a rostrocaudalspan of 500 µm (bregma $-$ 12.1-12.6 mm) is 220 (16.6 sections withan average of 13 cells per section), but it should be emphasizedthat the present method was not designed to produce accurate countsof the total number of cells present in a given three-dimensionalarea. The larger NK1R-ir neurons that express high levels of PPEmessage had a broad distribution with a peak at the rostral endof the rVRG (Fig. 5B). As expected, we found that some of theintensely fluorescent NK1R-ir neurons of the VRG contained FG,indicating that these cells have spinal projections. BulbospinalNK1R-ir cells were detected in all six rats, although their numberwas higher in the four animals that had received larger pressureinjections of FG (C4 or T3) than in the two rats that had receivediontophoretic injections of FG at C4. Without exception, all ofthe FG-labeled NK1R-ir neurons of the VRG were of the large multipolartype, and they contained PPE mRNA. The rostrocaudal distributionof these cells was the same in the rats that had received pressureinjections into the cervical cord as in those with thoracic levelinjections. The pooled results from these four rats are shownin Figure 5B. This figure indicates that all bulbospinal NK1R-irneurons were located in the rostral half of the rVRG. At thislevel, these cells constituted <20% of all the retrogradely labeledrVRG neurons.

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Figure 5. Distribution of NK1R-ir neurons that contain PPE mRNA. The plots represent the number of neurons (mean ± SE) per hemisection found within the 750 × 500 µm box outlined in Figure 2 (n = 6 rats). A, Rostrocaudal distribution of all NK1R-ir neurons and all bulbospinal neurons. The dip in the curve representing the bulbospinal neurons (FG⁺ total) identifies the location of the pre-BötC. B, Distribution of three classes of VRG NK1R-ir neurons based on the presence or absence of PPE mRNA and spinal projections to C4 or T3. All of the bulbospinal NK1R-ir neurons contained PPE mRNA.

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Figure 6. Low- and high-threshold inspiratory augmenting neurons of the rVRG: characterization and labeling. A1-A3, Low-threshold unit; B1-B3, high-threshold unit. A1, Resting discharge of a typical low-threshold neuron. Note the incrementing discharge of the cell (fourth trace from top: rate; fifth trace from top: original unit recording), which resembles the discharge pattern of the phrenic nerve (iPND, integrated discharge; PND, original nerve discharge). A2, Collision test demonstrating that the cell has an axonal projection to spinal level C4 (s, spontaneous spike; arrowhead, stimulus artifact; a, antidromic spike; asterisks indicate sweeps when collisions occurred). Antidromic latency of this unit was 1.2 msec. A3, Juxtacellular labeling by entrainment of the cell discharge with intermittent pulses of depolarizing current. B1, Resting discharge of high-threshold neuron. B2, Same unit during brief interruption of ventilation. B3, Collision test. The antidromic latency of this unit was 17.9 msec.

In one experiment, NK1R immunoreactivity was detected using the NK1R antibody that was used to provide the original map ofCNS NK1 receptors (Nakaya et al., 1994). The pattern of NK1R stainingin the VRG could not be distinguished from that obtained withthe commercial antibody, and the selective association betweenlarge NK1R-ir neurons and PPE mRNA was verified (results notshown).

Bulbospinal NK1R-ir neurons of the rVRG include a subtype of the inspiratory-augmenting neuron

It has been hypothesized that NK1R immunoreactivity might be a diagnostic marker for a group of respiratory rhythmogenic interneuronsof the VRG (Gray et al., 1999). However, the existence of NK1R-irwith spinal projections and the location of these cells (rostralpart of the rVRG) suggested to us that NK1 receptors may alsobe expressed by inspiratory bulbospinal premotor neurons (Duffinet al., 1995). The next experiments were designed to test whetherthe bulbospinal NK1R-ir neurons of the rVRG could indeed be inspiratorypremotor neurons and whether all or only a fraction of the inspiratorypremotor neurons express this receptor. To do so we recorded fromrVRG bulbospinal inspiratory-augmenting (I-AUG) neurons, and welabeled them juxtacellularly with biotinamide. The tissue wasprocessed for detection of NK1R immunoreactivity to determinewhether the recorded cells expressed NK1receptors.

In nine rats, the VRG was explored between 1.1 and 1.6 mm caudal to the caudal end of the facial motor nucleus because thisregion (bregma $-$ 12.8 to $-$ 13.3 mm) contains the highest densityof cells with projections to the phrenic motor nucleus (Fig. 3).In contrast to the rostrally located pre-BötC (0.6-1.0 mm behindfacial motor nucleus), this region of the VRG contained largenumbers of inspiratory neurons with incrementing discharge (I-AUG).These cells could be divided into two types. The most commonlyfound I-AUG neurons discharged at a very high rate during inspiration.Their discharge onset corresponded closely to that of the phrenicnerve (Fig. 6A1), and they exhibited an incremental rate of dischargethat could reach >200 spikes per second (Fig. 6A1, 205 Hz). Thishigh discharge rate typically caused a slight decrement in spikeheight at the end of the burst (Fig. 6A1). In virtually everycase, spikes with constant and very short latency could be observedin these fast-discharging I-AUG cells after spinal cord stimulation(Fig. 6A2, 1.2 msec). The collision test (Lipski, 1981) illustratedin Figure 6A2 was used to demonstrate that these constant latencyspikes were antidromic. The constant latency action potentials(a) evoked by spinal cord stimulation (arrow) were not evoked(sweeps denoted by an asterisk) when the stimulus was deliveredwithin a critical interval (1.1 msec in this example) after aspontaneously occurring spike (s). The discharge of the cellswas eliminated by hyperventilation, and it maintained the sametemporal relationship to the PND when ventilation was interrupted,indicating that the discharge of the cell did not require lungafferent input (data notshown).

A second class of I-AUG cells was also encountered (Fig. 6B1). At rest, these neurons had a much lower rate of discharge andthus much smaller numbers of spikes per phrenic burst (from <1to 20). An extreme case is shown in Figure 6B1. The dischargerate of the slow I-AUG cells was increased along with the inspiratorydrive (PND amplitude), when ventilation was interrupted for briefperiods (10-20 sec). During these episodes the cells remainedphase-locked with the PND (Fig. 6B2), but they fired earlier andearlier during the phrenic burst. This firing pattern suggeststhat they are indeed high-threshold I-AUGs and not late inspiratorycells. These cells could also be antidromically activated fromC5 but their antidromic latency was typically much longer thanthat of the fast-conducting neurons (5-55 msec; a typical exampleis shown in Fig. 6B3).

Figure 7 illustrates the relationship between discharge rate (spikes per phrenic burst) and conduction velocity (two-pointdetermination based on an estimated straight-line distance of25 mm) for all the I-AUG cells analyzed (n = 49). The cubic clusteringcriterion and the pseudo F statistic identified two clusters asthe optimal number (see Materials and Methods). Thus, I-AUG neuronsmay belong to two groups: one with low discharge rate and slowconduction velocity (high-threshold I-AUG cells, n = 21; cluster1) and the other with high discharge rate and fast conductionvelocity (low-threshold I-AUG cells, n = 28; cluster 2). The distancefrom the origin was calculated for each data point. The distributionof distance measures for cluster 1 did not overlap with that forcluster 2; hence this numerical value may have diagnostic value.The two clusters were also well differentiated by the number ofspikes per burst (9.6 ± 1.5 vs 51.5 ± 2.5; p < 0.001) and conductionvelocity (4.5 ± 0.7 vs 16.4 vs 0.9; p < 0.001), with only minoroverlap. A sparse section in the center of each of the distributionsfor distance, spikes per burst, and conduction velocity (metersper second) reinforced the impression of two populations of data.

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Figure 7. Relationship between discharge rate and axonal conduction velocity of inspiratory augmenting neurons. Mean number of spikes per burst under resting condition (averaged over 20 consecutive bursts) plotted against the conduction velocity of the spinal axon (25 mm estimated straight-line distance between stimulating and recording points divided by antidromic latency). n = 49 cells. The two cell clusters delineated by the average linkage method (see Materials and Methods) are identified by (high-threshold cells) and $open circle$ (low-threshold neurons).

The end-expiratory CO₂ was 5.85 ± 0.1% for the 29 neurons firing above 20 spikes per respiratory burst and 6.23 ± 0.16% forthe 20 I-AUG cells with 0-20 spikes per burst. Thus the slowerdischarge rate of the slow-conducting neurons was clearly notcaused by a difference in the CO₂ level and, presumably, in centralinspiratory drive. In fact, because many of these cells were dischargingso slowly, ventilation was deliberately reduced to permit theircharacterization, which accounts for the slightly higher baselineCO₂ level registered during analysis of their discharge rate.Both types of neurons (slow and fast discharging) could be reliablyentrained by the extracellular pulses of positive current (2.5-8nA; 5.2 nA in Fig. 6A3) procedure, which resulted in their labelingwith biotinamide. Note that during the entrainment, the cell maintainedits normal respiratory pattern of discharge, but the stimuluswas strong enough to activate the cell during the normally silentexpiratoryphase.

Most of the I-AUG cells labeled with biotinamide were not NK1R-ir (38 of 42). This general case is illustrated in Figure 8A,B.Note that the biotinamide-labeled cell lies in immediate proximityto another neuron that did express very high levels of NK1R immunoreactivity.In the first six rats in which only fast-firing I-AUG cells werelabeled, we did not find a single NK1R-ir cell (of 28). The locationof these 28 neurons is shown in Figure 9A. In the three remainingrats, we labeled preferentially I-AUG cells with slow axonal conductionvelocity (11 neurons of 14 with an antidromic latency of >5 msec).Four of the labeled cells were NK1R-ir (Fig. 8C,D), suggestingthat NK1R-ir cells may be a subtype of the high-threshold I-AUGcells. The location of the 14 predominantly slow I-AUG cells recoveredin these last experiments is shown in Figure 9B. The anatomicaldistribution of the low- and high-threshold bulbospinal I-AUGneurons was similar (Fig. 9, compare A, B), although the NK1R-irneurons appear to lie at the lower edge of the column of I-AUGneurons (Fig. 9B).

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Figure 8. Examples of inspiratory augmenting neurons labeled with biotinamide. A, B, Biotinamide-filled I-AUG neuron (A, arrow) with fast discharge rate and fast axonal conduction velocity that lacks NK1R-immunoreactivity (B, arrow). Note presence of NK1R immunoreactivity in an adjacent cell (B, arrowhead). C, D, Biotinamide-labeled I-AUG neuron (C) with low discharge rate and slow axonal conduction velocity that contained NK1R-immunoreactivity (D). Scale bar, 25 µm.

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Figure 9. Location and phenotype of labeled inspiratory augmenting neurons. A, Location of 28 biotinamide-labeled I-AUG neurons with fast discharge rate and fast axonal conduction velocity (low-threshold cells) recorded in six rats. B, Location of 14 biotinamide-labeled I-AUG, predominantly high-threshold (11 of 14) neurons recorded in three rats. , Neurons without NK1R immunoreactivity. $open circle$ , NK1R-ir neurons. All cells were plotted on the same coronal plane (bregma $-$ 13.0 mm). NTS, Nucleus of the solitary tract; IO, inferior olive; pyr, pyramidal tract; XII, hypoglossal nucleus.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

According to this study, the NK1R-expressing neurons of the VRG are functionally heterogeneous but predominantly glutamatergic.A group of small fusiform neurons that lack PPE mRNA is primarilyrestricted to the pre-BötC and may be the interneurons the destructionof which produces massive disruptions of the respiratory rhythm(Gray et al., 2001). The remaining VRG NK1R-ir neurons, includingthe bulbospinal ones of the rVRG, are larger multipolar cellsthat express PPE mRNA and include premotorneurons.

Technical considerations

The recent identification of two rat vesicular glutamate transporters, VGLUT1 and VGLUT2, now provides diagnostic tools toidentify glutamatergic neurons (Takamori et al., 2000; Bai etal., 2001; Fremeau et al., 2001). Only VGLUT2 is expressed inthe VRG (Stornetta et al., 2002a). Under our experimental conditions,VGLUT2 is absent from GABAergic or cholinergic neurons (Stornettaet al., 2002a), but it is present in known glutamatergic cellssuch as the inferior olive (Auger and Atwell, 2000; Ito, 2001)or the bulbospinal neurons of the rVRG (Dong et al., 1996; Feldmanand McCrimmon, 1999). Thus our histological method appears tocorrectly identify glutamatergic neurons; however, the VGLUT2mRNA reaction product was light, and some of the cells that expressthis transporter may not have been identified. In contrast, thePPE cRNA probe produced an extremely dense reaction product (Fig.4), suggesting that absence of labeling was truly indicative ofvery low mRNAlevels.

Most NK1R-ir neurons of the VRG are glutamatergic

The presence of VGLUT2 mRNA in 77 ± 9% of VRG NK1R-ir cells demonstrates that most of these neurons are glutamatergic andconfirms a previous tentative phenotyping based on glutamate immunoreactivity(Liu and Wong-Riley, 2001). In agreement, GAD67 mRNA is rarelydetectable in VRG NK1R-ir cells (<10%), and they are not glycinergic,cholinergic, or catecholaminergic (Gray et al., 1999; H. Wanget al., 2001). Because the hybridization method may not be sensitiveenough to detect all of the cells that contain VGLUT2 mRNA, wemay have underestimated the proportion of VRG NK1R-ir cells thatare glutamatergic. However, we also cannot exclude the possibilitythat that up to 23% of the NK1R-ir cells of the VRG might be otherthanglutamatergic.

Absence of PPE mRNA defines a class of NK1R-ir neurons that could be the hypothesized kernel of the pre-BötC respiratory rhythm generator

Respiratory rhythm generation has long been attributed to reciprocal interactions between inhibitory neurons (Rybak et al.,1997; for review, see Feldman and McCrimmon, 1999). Accordingto these models, the excitatory drive to this set of mutuallyinhibitory neurons is tonic (e.g., from chemoreceptors, state-dependentinputs) or caused by inward currents (e.g., I_h, I_CaT,) reactivatedby GABAergic or glycinergic hyperpolarization (Richter and Spyer,2001). The central role of glutamatergic neurons in respiratoryrhythmogenesis has only recently come to the fore. According tothe pacemaker-driven network theory (Feldman and McCrimmon, 1999;Smith et al., 2000), glutamatergic interneurons, including a coreof cells with intrinsic bursting properties, constitute the kernelof the respiratory rhythm generating circuit (Onimaru et al.,1995; Rekling and Feldman, 1998; Ballanyi et al., 1999; Del Negroet al., 2001; Johnson et al., 2001). The theory that NK1R immunoreactivityis a selective marker for the rhythmogenic neurons is based onthe high level of these receptors in the pre-BötC, the excitatoryeffect of substance P on some inspiratory pre-BötC neurons invitro, and the disruption of breathing caused by selective lesionof NK1R-ir cells (Gray et al., 1999, 2001). The present data addtwo pieces of evidence to the theory. First, VRG NK1R-ir cellsare indeed predominantly glutamatergic, whereas most GABAergicand glycinergic VRG neurons are not NK1R-ir (H. Wang et al., 2001).Second, we found a subtype of NK1R-ir glutamatergic neuron withoutspinal projections that is present almost exclusively in the pre-BötC.These small fusiform neurons are likely to be functionally differentfrom the large PPE mRNA-expressing NK1R-ir neurons because theirsomatic size and morphology are so different. Because of theirlocation, the small fusiform NK1R-ir neurons that do not expressPPE mRNA may be the adult version of the inspiratory substanceP-sensitive neurons recorded in vitro (Gray et al., 1999). Thesecells are believed to be rhythmogenic and may have pacemaker properties(Feldman and McCrimmon, 1999; Pilowsky and Feldman, 2001). Thedischarge pattern of these NK1R-ir cells in vivo needs to be identifieddefinitively. Candidates include some form of excitatory I-constantneurons that are sometimes viewed as antecedent to VRG I-AUG neurons(Duffin et al., 1995, 2000) or the pre-inspiratory cells of thepre-BötC shown by us previously to be NK1R-ir (Guyenet and Wang,2001). However, further work is needed to determine whether thelatter neurons are the small fusiformones.

The rVRG contains NK1R-ir neurons that are both glutamatergic and enkephalinergic and may be inspiratory premotor neurons

The retrograde labeling experiments (Figs. 2, 3, 5) confirmed the presence of bulbospinal NK1R-ir neurons in the rVRG region,which is defined by its large concentration of neurons projectingto the C4 ventral horn. These NK1R-ir cells were shown to projectto thoracic and cervical levels. All bulbospinal NK1R-ir neuronscontained VGLUT2 mRNA in one experiment and PPE mRNA in the other;thus they are both glutamatergic and enkephalinergic. Severalprecedents for this unusual combination of transmitters existin the pontomedullary region (Van Bockstaele et al., 2000; Stornettaet al., 2001, 2002b).

The combination of a glutamatergic phenotype, location in the rVRG, and projection to the phrenic motor nucleus suggestedto us that some of the bulbospinal NK1R-ir cells might be inspiratoryneurons. Accordingly, some of the I-AUG bulbospinal neurons exhibitedhigh levels of NK1R immunoreactivity (Fig. 8C,D). In agreementwith the retrograde labeling experiments (Figs. 2, 3, 5), mostbulbospinal I-AUG neurons of the rVRG did not express NK1R (Figs.8A,B, 9). This observation agrees with the fact that many inspiratorypremotor neurons survive after lesion of VRG NK1R-ir neurons (Grayet al., 2001).

The NK1R-ir I-AUG neurons required a high level of respiratory drive to be activated (Fig. 6B1,B2). Most of these high-thresholdcells could be silent at rest, which may account for the smallnumber of NK1R-ir cells encountered in our initial experiments.The physiological role of the NK1R-ir high-threshold I-AUG neuronsremains to be clarified. Judging from their firing pattern, location,and spinal projections, these cells could be inspiratory premotorneurons that innervate both phrenic and inspiratory intercostalmotor neurons, but their projections to the thoracic spinal cordcould also suggest a role in controlling vasomotor sympatheticefferents.

Putative role of the enkephalinergic NK1R-ir neurons without spinal projections

Although large injections of FG into a single spinal segment cannot possibly label all bulbospinal neurons, the present experimentsclearly demonstrate that most of the large enkephalinergic NK1R-irneurons of the VRG are not bulbospinal. Indeed, regardless ofthe site of injection (thoracic or cervical), FG-labeled NK1R-irneurons were found exclusively caudal to bregma level $-$ 12.6 mm.The NK1R-ir neurons located rostral to that point therefore cannotbe bulbospinal, and they clearly reside within the pre-BötC.Because the spinally projecting enkephalinergic NK1R-ir cellsappear to be a form of inspiratory premotor neuron, we propose,by analogy, that those without spinal projections may be otherforms of respiratory glutamatergic premotor neurons. Candidatescould be the NK1R-ir pre-I/I-DEC of the pre-BötC (Guyenet andWang, 2001) that do not project to the cord (Sun et al., 1998;P. Guyenet and H. Wang, unpublished results) and have a dischargepattern that is theoretically consistent with a role as laryngealpremotorneurons.

Because only a fraction of the bulbospinal I-AUG neurons express NK1R, it is possible that the presence of this receptor doesnot provide diagnostic identification of functionally homogeneousclasses of respiratory cells. Instead, NK1R immunoreactivity maybe expressed by restricted subpopulations of neurons that belongto different functional groups. If this is true, the differentialexpression of NK1R in the VRG may exist to produce a specificrespiratory response pattern to substance Prelease.

Conclusion and physiological significance

The respiratory stimulant effect of substance P is mediated in part by NK1 receptors (Chen et al., 1990; Monteau et al., 1996)and is observed in medullary slices and individual respiratory-relatedneurons of the pre-BötC (Johnson et al., 1996; Monteau et al.,1996; Gray et al., 1999). The association of NK1 receptors withglutamatergic neurons explains satisfactorily the respiratorystimulation produced by substance P administered in the ventrolateralmedulla. The increase in respiratory rate and amplitude (Grayet al., 1999) may be achieved by simultaneous activation of severaltypes of NK1R-ir neurons, including rhythmogenic cells and selectedsubpopulations of excitatory premotorneurons.

The pre-BötC, like the neighboring C1 area, probably receives substance P-containing inputs from serotonergic neurons thatare activated by acidification (Milner et al., 1996; W. G. Wanget al., 2001). Central hypercapnia could thus stimulate respirationby depolarizing pre-BötC glutamatergic neurons via substanceP released from raphe neurons. Nociceptive or muscle metabotropicafferents may also trigger the release of substance P into theVRG from spinoreticular neurons (Potts et al., 1999; Gamboa-Esteveset al., 2001).

  FOOTNOTES

Received Dec. 26, 2001; revised Feb. 7, 2002; accepted Feb. 12, 2002.

This work was supported by National Institutes of Health Grants HL28785 and HL 60003 to P.G.G. We also thank Dr. Ryuichi Shigemoto(National Institute for Physiological Sciences, Myodaiji, Okazaki,Japan) for providing a sample of their antibody against the NK1receptor.

Correspondence should be addressed to Dr. Patrice G. Guyenet, University of Virginia Health System, P.O. Box 800735, 1300Jefferson Park Avenue, Charlottesville, VA 22908-0735. E-mail:pgg{at}virginia.edu.

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