1Division of Pulmonary and Critical Care Medicine, Department of Medicine, University of Medicine and Dentistry of New Jersey, Robert Wood Johnson Medical School, New Brunswick, New Jersey 08903-0019; and 2Department of Physiology and Biophysics, State University of New York at Stony Brook, Stony Brook, New York 11794-8661
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ABSTRACT |
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Solomon, Irene C., Norman H. Edelman, and Judith A. Neubauer. Pre-Bötzinger Complex Functions as a Central Hypoxia Chemosensor for Respiration In Vivo. J. Neurophysiol. 83: 2854-2868, 2000. Recently, we identified a region located in the pre-Bötzinger complex (pre-BötC; the proposed locus of respiratory rhythm generation) in which activation of ionotropic excitatory amino acid receptors using DL-homocysteic acid (DLH) elicits a variety of excitatory responses in the phrenic neurogram, ranging from tonic firing to a rapid series of high-amplitude, rapid rate of rise, short-duration inspiratory bursts that are indistinguishable from gasps produced by severe systemic hypoxia. Therefore we hypothesized that this unique region is chemosensitive to hypoxia. To test this hypothesis, we examined the response to unilateral microinjection of sodium cyanide (NaCN) into the pre-BötC in chloralose- or chloralose/urethan-anesthetized vagotomized, paralyzed, mechanically ventilated cats. In all experiments, sites in the pre-BötC were functionally identified using DLH (10 mM, 21 nl) as we have previously described. All sites were histologically confirmed to be in the pre-BötC after completion of the experiment. Unilateral microinjection of NaCN (1 mM, 21 nl) into the pre-BötC produced excitation of phrenic nerve discharge in 49 of the 81 sites examined. This augmentation of inspiratory output exhibited one of the following changes in cycle timing and/or pattern: 1) a series of high-amplitude, short-duration bursts in the phrenic neurogram (a discharge similar to a gasp), 2) a tonic excitation of phrenic neurogram output, 3) augmented bursts in the phrenic neurogram (i.e., eupneic breath ending with a gasplike burst), or 4) an increase in frequency of phrenic bursts accompanied by small increases or decreases in the amplitude of integrated phrenic nerve discharge. Our findings identify a locus in the brain stem in which focal hypoxia augments respiratory output. We propose that the respiratory rhythm generator in the pre-BötC has intrinsic hypoxic chemosensitivity that may play a role in hypoxia-induced gasping.
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INTRODUCTION |
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Pflüger (1868) established
that mammalian ventilation is stimulated by hypoxia. A CNS site for
chemosensitivity to the lack of oxygen was assumed, but only by
inference from indirect data. Accordingly, the discovery of the hypoxia
sensing function of the carotid bodies by Heymans and colleagues
(1930)
focused full attention on arterial chemoreceptors as the
only hypoxia sensors involved in ventilatory control. Over the last 15 to 20 yr, however, many observations have been made that are not wholly
consistent with this idea. Among them is the stimulation of breathing
in unanesthetized (i.e., awake or decerebrate) deafferented animals (Gautier and Bonora 1980
; Miller and Tenney
1975
; Tenney and Ou 1976
), which is thought to
be supramedullary in origin and the demonstration of gasping in
response to severe hypoxia in anesthetized deafferented animals
(Guntheroth and Kawabori 1975
; Oyer-Chae et al.
1993
; St. John and Knuth 1981
), which is likely
to originate in the medulla. Further, some studies in anesthetized
deafferented cats have demonstrated a biphasic respiratory response
that consists of an initial increase in the frequency and amplitude of
ventilation (augmentation) followed by a decrease (depression) that can
lead to cessation of breathing (apnea) (Richter et al.
1991
).
The sites and mechanisms responsible for centrally mediated hypoxic
respiratory excitation (i.e., augmentation and gasping) remain unclear.
Recent work from our laboratory (Solomon et al. 1999)
investigating the role of the pre-Bötzinger complex
[pre-BötC; which is the proposed origin of respiratory
rhythmogenesis (Smith et al. 1991
)] in the generation
and modulation of inspiratory motor output in vivo has demonstrated
that activation of ionotropic excitatory amino acid (EAA) receptors
elicits a variety of excitatory responses in the phrenic neurogram,
ranging from tonic firing to a rapid series of high-amplitude, rapid
rate of rise, short-duration inspiratory bursts that are
indistinguishable from gasps produced by severe brain hypoxia.
Additionally, studies by Ramirez et al. (1997a
,
1998a
) from the in vitro transverse brain stem slice
preparation that contains the pre-BötC demonstrate a biphasic
response (i.e., augmentation followed by depression) of rhythmic
discharges in both pre-BötC neurons and the hypoglossal nerve,
suggesting that the medulla contains the necessary elements required
for the production of centrally mediated hypoxic respiratory excitation.
Previous studies have established that a unique population of neurons
located in the rostral ventrolateral medulla (RVLM), namely the
reticulospinal sympathoexcitatory neurons, many of which exhibit
pacemaker-like activity, are intrinsically hypoxia chemosensitive
(Sun and Reis 1994). Because these neurons have been
previously shown to be essential for the tonic generation of vasomotor
tone and the reflex regulation of arterial blood pressure (Ross
et al. 1984
), it is tempting to speculate that a similar
population of respiratory rhythm-generating neurons may be hypoxia
chemosensitive as well.
Thus the current studies were designed to test the hypothesis that the pre-BötC is hypoxia chemosensitive and may serve as a locus for CNS hypoxic modulation of respiratory output.
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METHODS |
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General
Experiments were conducted in 41 adult cats, weighing 2.8-5.0
kg. Twenty cats were anesthetized initially with ketamine hydrochloride (15 mg/kg im) and acepromazine maleate (1.1 mg/kg im). The right brachial vein was cannulated and -chloralose (10-20 mg/kg iv) was
administered intravenously. Supplemental
-chloralose was given as
needed (3-5 mg/kg iv). The remaining 21 cats were anesthetized initially by placing them inside a sealed, plastic induction chamber into which a gaseous mixture of halothane (5%) and oxygen was introduced. After the cats were anesthetized, they were removed from
the chamber, and anesthesia was maintained by delivering halothane
(1.5-3%) and oxygen through a face mask placed over the cat's nose
and mouth. The right brachial vein was cannulated, and
-chloralose
and urethan (35 and 210 mg/kg iv, respectively) were administered. The
gaseous anesthesia was then removed. Supplemental
-chloralose and
urethan (5 and 10 mg/kg iv, respectively) were given as needed. The
adequacy of anesthesia was regularly verified by firmly pinching a toe.
If an increase in blood pressure was evoked or, during the absence of
paralysis (see Experimental protocol), if the cat withdrew
its limb, additional anesthesia was given. Dexamethasone (2 mg iv) was
administered to minimize brain swelling. In all cats, both brachial
arteries were cannulated. The left brachial cannula was connected to a
Statham transducer (P23Db) for measurement of arterial blood pressure;
the right brachial cannula was used for sampling arterial blood.
The trachea was cannulated low in the neck and the lungs ventilated with room air enriched with O2. The chest was opened bilaterally through the sixth intercostal spaces, and the expiratory outlet of the ventilator was placed under 1-2 cm H2O to prevent collapse of the lungs during expiration. End-tidal CO2 was monitored continuously through a side port in the tracheal cannula and maintained between 4.0 and 5.5% by adjusting the tidal volume and frequency of the ventilator. Arterial PO2, PCO2, and pH were measured at hourly intervals (Radiometer ABL-30), and when necessary, blood gas values were corrected by either adjusting the ventilator or intravenous infusion of sodium bicarbonate (8.5%). At the start of the experimental protocol (see Experimental protocol), arterial PO2, PCO2, and pH averaged (means ± SE) 226 ± 15 mmHg, 40 ± 1 mmHg, and 7.40 ± 0.01, respectively. Body temperature was measured and maintained at 36-38°C with the use of a heating pad and a heat lamp.
Both cervical vagus nerves were exposed and cut bilaterally. In 19 cats, the carotid sinus nerves were also exposed and cut bilaterally. The cat's head was then placed in a Kopf stereotaxic instrument and the dorsal surface of the medulla exposed by separating the nuchal musculature along the midline, removing the basioccipital bone, and opening the atlantooccipital membrane. The dorsal surface of the brain stem was covered with warm mineral oil to prevent drying.
The C5 rootlet of one or both phrenic nerves was isolated in the neck via a lateral approach, cut, and desheathed, and the central end was placed on a bipolar hook electrode. The nerve was then covered with a mixture of mineral oil and petroleum jelly. Phrenic nerve discharge was amplified (×1,000-10,000) and filtered (1-10,000 Hz), and a moving average was obtained using a third-order Paynter filter with a 100-ms time constant. Both the raw and averaged nerve outputs were recorded on digital tape (A. R. Vetter, Model 4000A) and on a chart recorder.
Experimental protocol
We examined the effects of focal hypoxia in the pre-BötC
on phrenic nerve discharge and arterial blood pressure. Focal hypoxia was produced using sodium cyanide (NaCN) which is a powerful stimulant of chemoreceptors (Choi 1988; Eyzaguirre and
Zapata 1984
) and is often used as a model for producing tissue
hypoxia (DiRodriguez and Bazan 1983
; Goldberg et
al. 1987
). Responses from a total of 81 sites in the
pre-BötC were recorded. Responses from an additional 23 sites
adjacent (within 200-500 µm) to the pre-BötC, including the
rVRG and the Böt complex, were also recorded. Sites in the
pre-BötC were initially localized using predetermined stereotaxic
coordinates relative to the calamus scriptorius (3.4-4.0 mm rostral),
midline (3.8-4.2 mm lateral), and dorsal surface (4.2-4.5 mm
ventral). The range in values for the coordinates used to find the
pre-BötC reflects the variability in the dimensions of the brain
stems in cats of different sizes. All sites were functionally verified
to be in the pre-BötC as previously described (Solomon et
al. 1999
) using the glutamate analogue
DL-homocysteic acid (DLH) and histologically confirmed (see
Location of responsive and nonresponsive sites). For
functional identification, unilateral microinjection of DLH produced
either 1) a series of high-amplitude, short inspiratory
duration (i.e., gasplike) bursts, 2) tonic excitation of
phrenic nerve discharge, or 3) augmented bursts (i.e.,
eupneic breath ending with a high-amplitude, short-duration burst).
Many of these DLH data have been reported previously (Solomon et
al. 1999
).
All microinjections into the medulla were made with the use of a
multibarreled glass pipette (20-40 µm tip diameter) attached to a
pressure injection device (General Valve Picospritzer II). One barrel
of the pipette contained NaCN (1 mM). The remaining barrels contained
DLH (10 mM), saline, and Fast Green dye (2%) which was used to mark
the injection sites (105 nl). All microinjected chemicals were
dissolved in a saline solution, and the pH was adjusted to 7.36-7.44.
Microinjection volumes of NaCN, DLH, and saline were 21 nl, and
microinjection typically required 1-2 s to complete. The volume of
each injection was monitored by observing the displacement of the fluid
meniscus using a microscope equipped with an eyepiece reticule. To
control for nonspecific effects, equivalent volumes of saline were
microinjected into all sites in which NaCN elicited changes in phrenic
nerve discharge and/or arterial blood pressure. In all experiments, the
order of microinjection of NaCN and DLH into the pre-BötC was
random, with the remaining chemical being microinjected after a 10-15
min recovery period.
In 38 of the 41 cats, responses to microinjection of NaCN into 1-3 sites in the pre-BötC were examined; 4 sites each were examined in the remaining cats. Our first site was identified using the stereotaxic coordinates defined above, and subsequent microinjections were made after movement of the pipette in 100- to 300-µm increments in the rostral-caudal, medial-lateral, or dorsal-ventral direction. Most often, the pipette was moved in a rostral-caudal direction. In 11 of the 41 cats, we also examined the response to microinjection of NaCN into 1-3 sites adjacent (within 200-500 µm) to the pre-BötC. No more than 4 microinjection sites (including adjacent sites) were examined on one side of the brain stem, and bilateral microinjections were made in 13 animals.
Baseline phrenic neurogram amplitude was initially set at 40-60% of the maximum amplitude evoked in response to ventilating the lungs, through a rebreathing circuit, with 95% O2-5% CO2 until end-tidal CO2 was increased to 8.0%. By setting the baseline amplitude this way, we were able to record increases or decreases in phrenic neurogram amplitude evoked by microinjection of NaCN into the medulla. Before stimulation of sites in the medulla, the cats were paralyzed with gallamine triethiodide (2 mg/kg iv). The effect of the paralytic agent was always allowed to dissipate so that the level of anesthesia could be assessed. Supplemental doses of the paralytic agent were administered as needed.
Histology
At the conclusion of the experiment, the cat was killed under deep anesthesia by an injection of saturated KCl solution. The brain stem was removed and placed in 4% Formalin for at least 48 h. The brain stem was then frozen, sectioned coronally (40 µm), mounted on slides, and stained for cell bodies using 1% Neutral Red dye. With the use of a microprojector, we made drawings of tissue sections containing sites marked with Fast Green dye.
Data analysis
Amplitude of integrated phrenic nerve discharge, inspiratory time (Ti), expiratory time (Te), frequency of phrenic bursts, and rate of rise were determined from the phrenic neurogram off-line (AT CODAS; DATAQ Instruments). Amplitude of integrated phrenic nerve discharge is reported as a percentage of the maximal amplitude recorded in each cat. This maximal amplitude occurred either in response to ventilating the lungs with CO2 (see Experimental protocol) or in response to microinjection of NaCN or DLH into the pre-BötC. Rate of rise was determined over the linear phase of activity and is reported as a percentage of the maximal rate of rise recorded in each cat. Baseline values for all of these variables were determined by averaging the values obtained for the 60-s period immediately preceding microinjection of NaCN into the pre-BötC. Peak response values for these variables were determined by averaging the first five consecutive breathing cycles that displayed the greatest change from baseline values. Baseline values for mean arterial pressure were taken as the steady-state values. Peak responses were taken as the highest or lowest value reached after microinjection of NaCN.
All values are reported as means ± SE. Responses before and after stimulation are presented as paired data. A Student's paired t-test or ANOVA was used to determine statistical significance, for which the criterion level was set at P < 0.05.
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RESULTS |
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General effects of microinjection of NaCN into the pre-BötC
We identified 81 histologically confirmed sites in the
pre-BötC in which unilateral microinjection of DLH (10 mM, 21 nl) produced either a series of high-amplitude, rapid rate of rise, short
inspiratory duration bursts, a tonic excitatory discharge, or an
augmented pattern (i.e., eupneic breath ending with a high-amplitude, short-duration burst) of phrenic nerve discharge. Unilateral
microinjection of NaCN (1 mM, 21 nl) into these sites produced
excitation of phrenic nerve discharge in 49 of the 81 sites examined.
This augmentation of inspiratory motor output exhibited one of the
following changes in cycle timing and/or pattern: 1) a rapid
series of high-amplitude, short-duration bursts in the phrenic
neurogram (a discharge similar to a gasp), 2) a tonic
excitation of phrenic neurogram output (with or without respiratory
oscillations), 3) augmented bursts in the phrenic neurogram
(i.e., eupneic breath ending with a high-amplitude, short-duration
burst), or 4) an increase in frequency of phrenic bursts
accompanied by small increases or decreases in the amplitude of
integrated phrenic nerve discharge. These responses will be described
in more detail below. In 18 sites, the phrenic neurogram response was
accompanied by a marked (25 mmHg) increase or decrease in arterial
blood pressure; however, changes in arterial blood pressure (
10 mmHg)
accompanied phrenic neurogram responses in 30 of the sites examined. In
general, the onset of the respiratory effects preceded the blood
pressure response.
Responses to microinjection of NaCN were rapid and reproducible. In each of the sites examined, repeated microinjection of NaCN produced a repeatable and consistent response. In general, we waited at least 10 min before attempting to demonstrate repeatability of the phrenic neurogram and blood pressure responses to microinjection of NaCN. Movement of the pipette tip by as little as 100-200 µm, however, resulted in marked differences in the phrenic neurogram response evoked by unilateral microinjection of NaCN. In 12 cats in which multiple microinjection sites in the pre-BötC were examined on one side of the brain stem, we were able to elicit at least 2 of the different patterns of augmentation of inspiratory output described above. All responses to microinjection of NaCN were completely reversible. Microinjections of equivalent volumes of saline into all responsive sites were ineffective in producing any changes in phrenic nerve discharge or blood pressure.
Similar phrenic neurogram and blood pressure responses were observed in cats under both anesthetic paradigms. Additionally, similar phrenic neurogram and blood pressure responses were observed in cats with carotid sinus nerves intact or cut. Therefore these data will not be considered separately.
Rapid series of high-amplitude, short-duration bursts
Unilateral microinjection of NaCN into nine sites in the pre-BötC produced a rapid series of high-amplitude, short-duration bursts in the phrenic neurogram (Fig. 1). This response typically occurred within 1-2 s from the beginning of microinjection of NaCN and had durations ranging from 27 to 248 s. Bilateral recordings were obtained in response to microinjection of NaCN into five of these nine sites in the pre-BötC, and the effects on phrenic nerve discharge were bilaterally symmetrical in those animals with bilateral recordings. On average, microinjection of NaCN into these sites decreased Ti from 1.75 ± 0.18 to 0.31 ± 0.02 s (mean ± SE, P < 0.01), decreased Te from 2.43 ± 0.27 to 0.80 ± 0.41 s (P < 0.01), increased the amplitude of integrated phrenic nerve discharge from 30.5 ± 7.6 to 79.6 ± 2.3% (P < 0.01) of maximal amplitude, and increased the rate of rise of phrenic nerve activity from 4.5 ± 0.8 to 81.9 ± 1.8% (P < 0.01) of the maximal rate of rise (Fig. 2). In addition, microinjection of NaCN increased the frequency of phrenic bursts from 14 ± 2 to 45 ± 5 bursts/min (P < 0.01).
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In five of these sites, the rapid series of high-amplitude, short-duration bursts in the phrenic neurogram was accompanied by an increase in mean arterial pressure from 109 ± 11 to 134 ± 8 mmHg (P < 0.05). In the remaining sites, the rapid series of bursts was accompanied by either a decrease (n = 2) or no change (n = 2) in mean arterial pressure.
Tonic excitation
Unilateral microinjection of NaCN into 21 sites in the pre-BötC produced a tonic excitation of phrenic nerve discharge. Bilateral recordings were obtained in response to microinjection of NaCN into 12 of these 21 sites in the pre-BötC, and the effects on phrenic nerve discharge were bilaterally symmetrical in those animals with bilateral recordings. The tonic excitation was characterized by either an abrupt rise in phrenic nerve discharge to a plateau level (nonrhythmic; Fig. 3) or respiratory rhythmic oscillations superimposed on varying levels of tonic discharge (rhythmic). In general, the peak amplitude of integrated phrenic nerve discharge at the onset of the response was higher or the same as that seen during baseline breaths; however, in a few cases, peak amplitude was slightly reduced. Despite the variable effects on the peak amplitude of integrated phrenic nerve discharge, at the onset of the response an increase in the rate of rise of phrenic activity was usually present. The response occurred within 1-3 s from the beginning of microinjection of NaCN and had durations ranging from 36 to 324 s. In addition, this type of tonic excitation exhibited a gradual recovery (n = 8 sites) or an increase in the frequency of phrenic bursts as the tonic discharge declined (n = 5 sites; Fig. 3), or was followed by a transient postexcitatory depression of phrenic nerve discharge that lasted 90-310 s (n = 8 sites).
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In 12 of these sites, the tonic excitation of phrenic nerve discharge was accompanied by a marked increase in mean arterial pressure from 103 ± 7 to 141 ± 14 mmHg (P < 0.01). In five of these sites, the tonic excitation of phrenic nerve discharge was accompanied by a marked decrease in mean arterial pressure from 102 ± 10 to 60 ± 8 mmHg (P < 0.01). No change in mean arterial pressure was seen in the remaining four sites.
Augmented bursts
Unilateral microinjection of NaCN into nine sites in the pre-BötC produced augmented bursts in the phrenic neurogram (i.e., eupneic breath ending with a high-amplitude, short-duration burst; Fig. 4). Bilateral recordings were obtained in response to microinjection of NaCN into eight of these nine sites in the pre-BötC, and the effects on phrenic nerve discharge were bilaterally symmetrical in those animals with bilateral recordings. These augmented bursts appeared as either a series of augmented breaths or were interspersed between eupneic breaths. In some cases, the onset of these augmented bursts was preceded by either an apneustic burst or a high-amplitude, short-duration burst of phrenic nerve discharge. In addition, the peak amplitude of integrated phrenic nerve discharge of the eupneic portion of the augmented burst was often increased above that seen during baseline breaths. The onset of augmented bursts occurred within 1-3 s from the beginning of microinjection of NaCN unless preceded by an apneustic burst. In all cases, the duration of the response with augmented bursts ranged from 40 to 472 s.
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In six of these sites, no change in mean arterial pressure accompanied the phrenic neurogram response. A marked increase in mean arterial pressure was seen in one of these sites, and a decrease in mean arterial pressure was seen in the remaining site.
Increased frequency of phrenic bursts
Unilateral microinjection of NaCN into 10 sites in the pre-BötC produced an increase in frequency of phrenic bursts accompanied by small increases or decreases in the amplitude of integrated phrenic nerve discharge (Fig. 5). Bilateral recordings were obtained in response to microinjection of NaCN into 3 of these 10 sites in the pre-BötC, and the effects on phrenic nerve discharge were bilaterally symmetrical in those animals with bilateral recordings. In some cases, this increase in the frequency of phrenic bursts was superimposed on a small tonic discharge (n = 3). In addition, in two sites, the appearance of augmented bursts occurred on some breaths. The onset of this frequency response occurred within 1-4 s from the beginning of microinjection of NaCN and had durations ranging from 18 to 118 s. On average, microinjection of NaCN into these sites increased the frequency of phrenic bursts by 29.5 ± 6.0% (P < 0.05) above baseline frequency. In nine of these sites, the increase in frequency resulted from a decrease in Te (from 3.0 ± 0.2 s to 2.1 ± 0.1 s; P < 0.05), whereas Ti remained constant or increased slightly. In addition to the increase in frequency of phrenic bursts, there was a small but significant increase (P < 0.05) in the rate of rise of phrenic nerve activity in 6 of the 10 sites examined (not shown).
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In two of these sites, the phrenic neurogram response was accompanied
by an increase (15-20 mmHg) in mean arterial pressure. In the
remaining eight of these sites, the phrenic neurogram response was
accompanied by small (10 mmHg) increases or decreases or no change in
mean arterial pressure.
NaCN- versus DLH-induced responses in the pre-BötC
Unilateral microinjection of NaCN into discrete sites in the pre-BötC produced excitation of phrenic nerve discharge in 49 of the 81 sites examined. The responses evoked by NaCN and DLH into 27 of these sites in the pre-BötC were similar. In the remaining 22 sites, however, the responses evoked by NaCN and DLH were not always identical. The distribution of these inspiratory motor output excitations based on response types to unilateral microinjection of both NaCN and DLH are described in Table 1.
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In the nine sites in which unilateral microinjection of NaCN into the pre-BötC produced a series of high-amplitude, short-duration bursts, unilateral microinjection of DLH produced either a rapid series of high-amplitude, short-duration bursts (n = 5), a tonic excitatory response (n = 1), or a series of high-amplitude, short-duration bursts superimposed on a tonic excitatory response (n = 3). Further, unilateral microinjection of DLH increased mean arterial pressure in seven of these sites and decreased it in the remaining two sites (not shown).
In all sites in which microinjection of NaCN into the pre-BötC evoked a tonic excitatory response in the phrenic neurogram, unilateral microinjection of DLH similarly produced a tonic excitatory response. Further, unilateral microinjection of DLH increased mean arterial pressure in 13 of these sites and decreased it in the remaining 8 sites (not shown).
In the nine sites in which microinjection of NaCN into the pre-BötC evoked augmented bursts in the phrenic neurogram, unilateral microinjection of DLH into these sites produced either a rapid series of high-amplitude, short-duration bursts (n = 2), a tonic excitatory response (n = 6), or augmented bursts (n = 1). In addition, unilateral microinjection of DLH increased mean arterial pressure in four of these sites, decreased mean arterial pressure in four sites, and was ineffective in altering mean arterial pressure in the remaining site (not shown).
Of the 10 sites in which microinjection of NaCN into the pre-BötC elicited a transient increase in the frequency of phrenic bursts, unilateral microinjection of DLH into these sites produced either a rapid series of high-amplitude, short-duration bursts (n = 1), a tonic excitatory response (n = 6), or a series of high-amplitude, short-duration bursts superimposed on a tonic excitatory response (n = 3). In addition, unilateral microinjection of DLH increased mean arterial pressure in four of these sites, decreased mean arterial pressure in four sites, and was ineffective in altering mean arterial pressure in the remaining two sites (not shown).
In 32 sites in the pre-BötC in which unilateral microinjection of NaCN was ineffective in eliciting a change in phrenic nerve discharge or mean arterial pressure, unilateral microinjection of DLH produced either a rapid series of high-amplitude, short-duration bursts (n = 5), a tonic excitatory response (n = 22), a series of high-amplitude, short-duration bursts superimposed on a tonic excitatory response (n = 3), or augmented bursts (n = 2) in the phrenic neurogram. Further, unilateral microinjection of DLH increased mean arterial pressure in 13 of these sites and decreased it in the remaining 19 sites (not shown).
Microinjection of NaCN and DLH into sites adjacent to the pre-BötC
We also examined the effects of unilateral microinjection of NaCN and DLH into 23 sites adjacent to the pre-BötC as a control for the spread of injectate. These microinjections were made into sites in the rVRG, Böt complex, and 200-500 µm dorsomedial, dorsolateral, or lateral to the pre-BötC.
Unilateral microinjection of DLH into the rVRG (n = 10) produced site-specific transient increases or decreases in the peak amplitude of integrated phrenic nerve discharge. In eight of these sites, unilateral microinjection of NaCN was ineffective in producing any changes in phrenic nerve discharge or blood pressure. In the remaining two sites, unilateral microinjection of NaCN produced a small transient decrease in the peak amplitude of integrated phrenic nerve discharge; the response to DLH in these sites was excitatory on phrenic motor output.
Unilateral microinjection of DLH into the Böt complex (n = 3) produced apnea. In these sites, unilateral microinjection of NaCN was ineffective in producing any changes in phrenic nerve discharge; however, a pressor response was seen in one of these sites.
In the 10 sites located dorsomedial, dorsolateral, or lateral to the pre-BötC, unilateral microinjection of both NaCN and DLH elicited no effect on phrenic nerve discharge or blood pressure.
Location of responsive and nonresponsive sites
The distribution of sites in which NaCN was microinjected into the medulla is shown in Fig. 6. As landmarks for identifying the rostrocaudal level of the pre-BötC, we identified the caudal pole of the retrofacial nucleus, nucleus ambiguus, the rostral pole of the lateral reticular nucleus, and the rostral pole of the hypoglossal nucleus. Examining our data from the level of obex produced considerable overlap in the types of responses seen, and placed over 90% of our sites in the same coronal section. Therefore in our analyses, all sites in the pre-BötC were identified with reference to the caudal pole of the retrofacial nucleus, not the obex. We found that mapping our sites in this way was consistent with the difference in the types of responses obtained based on movement of the pipette using stereotaxic coordinates in our experiments.
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We often found that movement of the pipette tip, using stereotaxic
coordinates, by as little as 100-200 µm resulted in marked differences in the phrenic neurogram and blood pressure responses evoked by unilateral microinjection of NaCN. An example may be seen in
Fig. 7. In this example (Fig.
7A), unilateral microinjection of NaCN into the
pre-BötC initially produced a transient rapid series of
high-amplitude, rapid rate of rise, short-duration inspiratory bursts
superimposed on a small tonic discharge. This series of bursts was
followed by three eupneic-like breaths that were coupled to a rapid
rate of rise, short-duration burst, which then recovered to a eupneic
pattern. In addition, no change in blood pressure was noted in response
to microinjection of NaCN into this site. Movement of the pipette tip
stereotaxically (and histologically confirmed) 200 µm rostral to the
initial site elicited a response that consisted predominantly of an
increase in frequency, although some small augmented bursts were seen
(Fig. 7B). In this site, microinjection of NaCN also
elicited a decrease in blood pressure. Although a frequency response
was evoked from both regions, the effects on timing and patterning of
phrenic nerve discharge are quite different. With reference to
histological identification (see Fig. 6 and explanation below), both
injection sites were identified in the coronal section labeled 0.4
mm.
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Our histological analyses (Fig. 6) revealed that all microinjection
sites identified functionally as pre-BötC were located within the
anatomic boundaries described for the pre-BötC in adult cat
(Connelly et al. 1992; Ramirez et al.
1998
; Schwarzacher et al. 1995
; Solomon
et al. 1999
). As can be noted from our histological analyses,
microinjection of NaCN into the pre-BötC produced a series of
high-amplitude, short inspiratory duration bursts in a fairly
restricted region. Also included within this region are the sites in
which microinjection of NaCN produced augmented bursts (i.e., eupneic
breath ending with a high-amplitude, short-duration burst). In fact,
all but 2 of the 18 sites that included high-amplitude, short
inspiratory duration bursts were located in this region of the
pre-BötC. Additionally, the majority (~90%) of sites in which
microinjection of NaCN elicited a modulation of phrenic burst frequency
(i.e., rapid series of high-amplitude, short inspiratory duration
bursts; increased frequency of phrenic bursts) are located within this
region of the pre-BötC. Encompassing a much larger area of the
pre-BötC are the sites in which microinjection of NaCN produced a
tonic excitation of phrenic neurogram output. In these sites, we could
not distinguish nonrhythmic from rhythmic tonic excitatory responses
based on their histological distribution.
We encountered 32 sites in the pre-BötC in which DLH but not NaCN elicited an excitatory pattern of inspiratory output. We could not differentiate these NaCN-responsive (Fig. 6, A-C) from NaCN-unresponsive (Fig. 6D) sites in the pre-BötC based on our histological analyses. In addition, we could not distinguish pressor and depressor responses based on their histological distribution.
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DISCUSSION |
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In the present study, we have demonstrated that NaCN-induced focal
hypoxia in discrete regions of the pre-BötC alters both respiratory rhythm and pattern in an excitatory manner. This excitation of inspiratory motor output appears to be specific to the
pre-BötC because focal hypoxia in the rVRG and Böt complex
was ineffective in producing excitation of inspiratory motor output.
Previous studies using NaCN have shown depression, but not excitation
of respiratory output. For example, in cats, perfusion of the fourth ventricle with NaCN decreases tidal volume or produces apnea
(Loeschcke and Koepchen 1958), and topical application
of NaCN to the intermediate area of the ventral medullary surface (VMS)
rapidly and reversibly decreases both inspiratory and expiratory
related respiratory activities (Haxhiu et al. 1993
).
Additionally, microinjection of NaCN into the RVLM of cats and rats,
including the intermediate area of the VMS, depresses phrenic nerve
activity (Mitra et al. 1993
; Sun et al.
1992
). Thus this study shows for the first time that focal
brain stem hypoxia produced by NaCN acting in a known respiratory
modulatory region augments inspiratory motor output. Based on these
findings, we suggest that the pre-BötC contains a hypoxia
chemosensitive element that when stimulated is capable of producing
excitation of inspiratory motor output.
Limitations of pressure injection
The response to NaCN was induced rapidly on microinjection locally in the region of the pre-BötC. Although the neural substrate responsible for initiating this response is unknown, it is most likely to be neurons located in this region or neuronal structures close to pre-BötC neurons. We believe that the transient bilateral increases in phrenic nerve discharge evoked by unilateral microinjection of NaCN into the pre-BötC resulted from hypoxic excitation of neurons in the immediate vicinity of the pipette tip. It is unlikely that microinjection of NaCN elicited its effects by inhibiting neurons in this region because microinjection of the excitatory amino acid DLH into the same sites produced similar types of responses in phrenic nerve discharge and arterial blood pressure. Further, it is unlikely that these responses resulted from nonspecific effects of pressure or volume of the injectate, because they were not produced by equal volumes of saline or larger volumes of Fast Green dye from adjacent barrels of the same pipette.
The effective spread of injectate is difficult to gauge without direct
measurement. Nevertheless, the dose of NaCN used in our experiments was
relatively small and probably did not spread far from the injection
site. Theoretical calculations by Nicholson (1985)
demonstrate that based on a 10-nl injection into brain tissue, the
concentration of injectate 300 µm from the injection site never
exceeds 20% of the initial injectate concentration. Additionally,
Lipski et al. (1988)
estimated that microinjection of a
30-nl volume had a radius spread of 325 µm. In contrast, Mitra
et al. (1993)
reported that the distribution of
[14C]cyanide based on a 100-nl (20 mM)
microinjection was larger than those estimated by Nicholson
(1985)
and Lipski et al. (1988)
; however, they
suggest that the physiological response to their injections was
restricted to a spread within 1 mm from the injection site. The volume
and concentration used by Mitra et al. (1993)
is much
larger than that used in our experiments. Our findings, however, appear
to be consistent with the estimations by Nicholson (1985)
and Lipski et al. (1988)
in that in our
experiments, movement of the pipette tip by as little as 100-200 µm
produced marked differences in the phrenic neurogram and blood pressure
responses to microinjection of NaCN (see Fig. 7). Additionally, we
often found that movement of the pipette tip by
500 µm
distinguished responsive from unresponsive sites. We cannot exclude the
possibility, however, that microinjection of NaCN had an effect on
dendrites whose cell bodies were distant from the site of injection.
Effects of brain hypoxia on respiratory and sympathetic output
To our knowledge, our data are the first to demonstrate in vivo a hypoxia chemosensitive region in the medulla that plays a role in the generation and modulation of respiratory rhythm and pattern. In our experiments, we found that unilateral microinjection of NaCN into the pre-BötC elicits a variety of excitatory responses in the phrenic neurogram, ranging from a rapid series of high-amplitude, rapid rate of rise, short-duration bursts to tonic firing.
Previous studies have reported that the generalized effect of brain
stem hypoxia is primarily a depression of respiratory output that is
accompanied by an increase in sympathetic output. In anesthetized,
peripherally chemodenervated animals, mild to moderate brain hypoxia
produces a depression of respiratory output and an increase in tonic
sympathetic nerve activity (Wasicko et al. 1990).
Similarly, intravertebral artery injection of hypoxic saline or NaCN
results in depression of phrenic nerve activity and an increase in
sympathetic nerve activity and arterial blood pressure (Arita et
al. 1989
; Mitra et al. 1992
).
The increase in sympathetic nerve activity in response to CNS hypoxic
hypoxia or cyanide appears to be mediated by direct hypoxic stimulation
of reticulospinal sympathoexcitatory neurons located in the RVLM
(Sun and Reis 1994; Sun et al. 1992
).
These neurons have been previously shown to be essential for the tonic generation of vasomotor tone and the reflex regulation of arterial blood pressure (Ross et al. 1984
). The most convincing
evidence for direct hypoxic excitation comes from the work of
Sun et al. (1992)
in which they have demonstrated that
microinjection of cyanide into the RVLM of rats evokes a pressor
response and a transient depression of phrenic nerve discharge.
Additionally, they have shown that iontophoretic application of NaCN
into the RVLM selectively and reversibly excites reticulospinal
sympathoexcitatory neurons, many of which exhibit pacemaker-like activity.
Centrally mediated hypoxic respiratory excitation: augmentation and gasping
Although hypoxic respiratory depression has been reported in both
anesthetized and awake peripherally chemodenervated animals, stimulation of breathing in these animal preparations has also been
demonstrated (Gautier and Bonora 1980; Miller and
Tenney 1975
; Richter et al. 1991
; Tenney
and Ou 1976
). For example, in anesthetized deafferented cats,
Richter et al. (1991)
have reported a biphasic
respiratory response that consists of an initial increase in the
frequency and amplitude of ventilation (augmentation) followed by a
decrease (depression) that can lead to cessation of breathing (apnea).
Further, in unanesthetized (i.e., awake or decerebrate) deafferented
cats, Tenney and colleagues have reported an increase in respiratory
frequency (i.e., tachypnea) (Miller and Tenney 1975
;
Tenney and Ou 1976
). It has been suggested that the
stimulation of respiratory frequency in response to global CNS hypoxia
originates from suprapontine regions (Tenney and Ou
1976
).
In addition to these initial stimulatory effects on breathing, severe
brain hypoxia results in a shift from respiratory depression to
respiratory excitation. In this case, respiratory excitation takes the
form of gasping that is characterized by an abrupt onset (i.e., rapid
rate of rise), short-duration burst of inspiratory activity
(Fung et al. 1994; St. John and Knuth
1981
; Zhou et al. 1991
). Further, in the cat,
gasping is also characterized by a significant increase in the peak
amplitude of integrated phrenic nerve discharge (St. John and
Knuth 1981
). This form of respiratory excitation (i.e.,
gasping) in response to severe brain hypoxia has been suggested to
originate in the medulla (this study; Solomon et al.
1996
; St. John 1996
; St. John et al.
1984
, 1985
); however, the specific medullary
sites and mechanisms have been unclear.
Previous work from St. John and colleagues in cats (St. John et
al. 1984, 1985
) and rats (Fung et al.
1994
) has identified a region in the lateral tegmental field
(LTF) of the medulla that they propose is critical for the expression
of gasping. They have shown that electrical stimulation in this region
during gasping evokes premature gasps and that lesioning this region
eliminates gasping, although neither maneuver alters the eupneic
breathing pattern. Two recent studies have examined the role of the
pre-BötC in the production and/or expression of both eupnea and
gasping in vivo (Huang et al. 1997
; Ramirez et
al. 1998b
). Huang et al. (1997)
have
demonstrated that lesioning a region of the ventrolateral medulla that
includes the pre-BötC and pre-I region (which is located rostral
to the pre-BötC) in decerebrate neonatal rats using kainic acid
abolished gasping in response to severe hypoxia but was ineffective in
altering the eupneic pattern of breathing. In contrast, Ramirez
et al. (1998b)
have demonstrated that bilateral synaptic
blockade of the pre-BötC in anesthetized cats using tetrodotoxin
(TTX) abolished the eupneic pattern of breathing without eliminating
gasping in response to asphyxia or severe hypoxia. It is possible,
however, that gasping may result from TTX-insensitive mechanisms and
may be independent of synaptic transmission [i.e., similar to the
hypoxic excitation of reticulospinal sympathoexcitatory neurons of the
RVLM (Sun and Reis 1993
, 1994a
,b
)].
In our experiments, we found that both types of respiratory stimulation
(i.e., augmentation of frequency and amplitude of eupneic bursts and
production of gasplike bursts) could be produced by unilateral
microinjection of NaCN into the pre-BötC. Our current findings
suggest that direct hypoxic stimulation of a discrete region located in
the pre-BötC can modify both inspiratory timing and patterning to
produce either an increase in frequency of phrenic bursts or a gasplike
inspiratory output. It should be noted, however, that these
high-amplitude, short-duration (gasplike) bursts produced by focal
hypoxia in the pre-BötC, were rapid with a short Te, whereas
gasps produced by severe brain hypoxia usually exhibit a prolonged Te.
However, in our experiments, our cats were maintained hyperoxic
(arterial PO2 200 mmHg) throughout the
experimental protocol. Thus the typical low frequency of gasps with
global brain hypoxia may reflect the depressant effect of hypoxia
at sites other than the pre-BötC, whereas the response manifest by focal NaCN may reflect the intrinsic response of the neurons that
initiate the gasp.
In our experiments, unilateral microinjection of NaCN into the
pre-BötC produces phase resetting of the respiratory rhythm (indicated by our increases in respiratory burst frequency). Thus our findings do not drive the conclusion that the pre-BötC is a
pattern generator for gasping and not eupnea because a variety of
responses, including increased frequency of eupneic bursts, were
observed. Because this region is proposed to represent the primary
locus of respiratory rhythm generation (Smith et al.
1991; for a recent review see Rekling and Feldman
1998
), our findings are consistent with the idea that the
principal respiratory rhythm generator or a subset of neurons embedded
within are hypoxia chemosensitive albeit, the physiological range of
hypoxic chemosensitivity remains to be determined.
Hypoxic chemosensitivity in the pre-BötC
Recently, Ramirez et al. (1998a) examined the
hypoxic responses of pre-BötC neurons from in vitro transverse
brain stem slices obtained from neonatal mice (postnatal days
0-22). Thirty minutes of exposure to hypoxic artificial
cerebrospinal fluid (95% N2 and 5%
CO2) elicited a biphasic response of inspiratory
motor output (i.e., augmentation followed by depression) as previously reported (Ramirez et al. 1997a
). During the initial
phase of the hypoxic exposure, augmentation of inspiratory motor output
was characterized by an increase in the frequency of rhythmic
discharges in pre-BötC inspiratory neurons and an increase in
frequency of burst discharges on the hypoglossal nerve. In addition, in ~50% of pre-BötC inspiratory neurons examined, the initial
augmentation was accompanied by an increase in the amplitude of
excitatory synaptic drive potentials.
In our experiments, we found that unilateral microinjection of NaCN
elicited responses in ~60% of the sites examined in the pre-BötC. There are at least two possible explanations for this finding that are not mutually exclusive. First, the dose of NaCN used
in our experiments was low and therefore may have been inadequate to
elicit effects in all of the sites examined. Consistent with this idea
are the findings of Mitra et al. (1992) and Sun
et al. (1992)
, who have demonstrated that cyanide increases
sympathetic nerve discharge and reticulospinal sympathoexcitatory
neuronal activity in a dose-dependent manner. We only used one dose of NaCN in the pre-BötC, based on our pilot experiments conducted in
other regions of the medullary respiratory network (Solomon et
al. 1995
). In these pilot experiments, we found that this 1-mM dose produced transient, repeatable responses in phrenic nerve discharge and that lower doses ranging from 200 to 500 µM were ineffective in consistently altering respiratory motor output, whereas
the higher doses ranging from 2 to 20 mM were not repeatable and
resulted in irreversible apnea.
Alternatively, only a subpopulation of neurons located in the
pre-BötC may be selectively hypoxia chemosensitive. In support of
this idea, previous studies have demonstrated that reticulospinal sympathoexcitatory neurons of the RVLM, many of which exhibit pacemaker-like activity, are intrinsically hypoxia chemosensitive (Sun and Reis 1993, 1994a
; Sun et al.
1992
). These neurons are directly and reversibly excited by
hypoxia, whereas adjacent neurons in this region are inhibited or
unaffected (Sun and Reis 1993
, 1994b
; Sun et al.
1992
). We suggest that the pre-BötC contains a
hypoxia chemosensitive element that is similarly selectively and
directly excited by hypoxia, and that this chemosensitive element is
part of the respiratory rhythm-generating network located in this
region. From our experiments, we cannot determine which neuronal
elements were responsible for the excitation of inspiratory motor
output. We speculate that the hypoxia chemosensitive element contains,
but is not limited to, the voltage-dependent pacemaker cells that are
believed, at least in the neonate, to provide rhythmic drive to the
rest of the respiratory network during the inspiratory phase of network
activity (Butera et al. 1999b
; Feldman and Smith 1995
; Koshiya and Smith 1999
; Rekling and
Feldman 1998
; Smith et al. 1991
,
1995
). Additionally, the preinspiratory (pre-I)
(Connelly et al. 1992
; Schwarzacher et al.
1995
; Smith et al. 1990
) or inspiratory-driver (I-driver) (Segers et al. 1987
) neurons proposed to be
key elements in respiratory phase transition (Smith et al.
1990
, 1995
) are likely candidates to be hypoxia chemosensitive.
It should also be noted that unilateral microinjection of NaCN into the
pre-BötC produced modulation of respiratory rhythm and pattern
that exhibited different forms of augmentation of inspiratory motor
output (i.e., rapid series of high-amplitude, rapid rate of rise,
short-duration bursts; tonic firing; increased frequency of eupneic
bursts). These differences in the cycle timing (i.e., rhythm) and
pattern may reflect a continuum of excitatory responses evoked by
stimulation of the respiratory rhythm generator located in the
pre-BötC. As such, our findings could be explained by either the
hybrid model or network models of respiratory rhythm generation
(Balis et al. 1994; Butera et al.
1999a
,b
; Feldman and Smith 1995
; Koshiya
and Smith 1999
; Ogilvie et al. 1992
;
Ramirez et al. 1997b
; Rekling and Feldman
1998
; Richter et al. 1986
; Smith et al.
1991
, 1995
). The hybrid model postulates that
respiratory rhythm generation arises from a population of
voltage-dependent pacemaker neurons, with intrinsic oscillatory
bursting capabilities (i.e., conditional pacemaker neurons), which
provide rhythmic drive to the rest of the respiratory network during
the inspiratory phase of network activity (Butera et al.
1999b
; Feldman and Smith 1995
; Koshiya
and Smith 1999
; Rekling and Feldman 1998
;
Smith et al. 1991
, 1995
). In this model,
synaptic interactions synchronize and modify the basic rhythm generator
by affecting the intrinsic membrane conductances of these
voltage-dependent pacemaker neurons; thus the pacemaker neurons have
multiple functional states ranging from quiescence (hyperpolarized
levels) to oscillatory bursting to tonic action potential generation
(beating) (Smith et al. 1995
). Recent computer
simulations examining the ionic basis of oscillatory bursting of
respiratory pacemaker neurons in the pre-BötC suggest that these
voltage-dependent oscillatory bursting properties may be important in
the control of baseline membrane potential and modulation of bursting
frequency, such that the dynamic interactions of intrinsic cellular
properties and excitatory synaptic mechanisms underlie rhythm
generation (Butera et al. 1999a
,b
). Because this pacemaker cell population would be expected to be a distribution of
cells in the different functional states, excitatory synaptic coupling
would produce synchronous oscillatory bursting, resulting in a more
robust respiratory oscillator (Butera et al. 1999b
). Based on the hybrid "pacemaker-network" model of respiratory rhythm generation, our findings may represent a shift in the functional state
of the voltage-dependent pacemaker cells. As such, we suggest that in
some of our sites in the pre-BötC, stimulation by NaCN could have
depolarized quiescent pacemaker neurons to an oscillatory bursting
state that resulted in an increase of respiratory burst frequency
(i.e., a rapid series of high-amplitude, short-duration bursts or
increased frequency of eupneic bursts). In other sites in the
pre-BötC, stimulation by NaCN could have depolarized either quiescent or bursting pacemaker neurons to a tonic state of action potential generation that resulted in a tonic excitation of inspiratory output. Finally, in some sites in the pre-BötC, stimulation by NaCN could have depolarized pacemaker neurons such that a both oscillatory bursting behavior and tonic action potential generation coexist resulting in excitation of inspiratory motor output that exhibits both frequency and tonic excitatory modulations.
Although our findings are consistent with the hybrid model for
respiratory rhythm generation, voltage-dependent bursting pacemaker neurons have not yet been demonstrated in vivo; therefore our findings
are also consistent with network models of respiratory rhythm
generation that do not include conditional bursting pacemaker neurons
(Balis et al. 1994; Ogilvie et al. 1992
;
Ramirez et al. 1997b
; Richter et al.
1986
). These models postulate that respiratory rhythm
generation arises from the interaction of inhibitory synaptic influences with intrinsic membrane properties of specific classes of
respiratory-modulated neurons (for a review see Ramirez et al.
1997b
). Because network models rely on respiratory
phase-dependent synaptic interactions among the various types of
respiratory-modulated neurons (Balis et al. 1994
;
Ogilvie et al. 1992
; Ramirez et al. 1997b
; Richter et al. 1986
), changes in the
strength of these synaptic interactions and/or changes in activity of a
population of respiratory neurons can modify respiratory rhythm and
pattern (Balis et al. 1994
; Ogilvie et al.
1992
). Previous studies have demonstrated that the
pre-BötC contains a high concentration of pre-I neurons
(Connelly et al. 1992
; Schwarzacher et al.
1995
) that appear to be necessary for phase transition
(Schwarzacher et al. 1995
; Smith et al.
1990
). As such, the modulations of respiratory rhythm and
pattern reported in our study could have resulted from hypoxic
stimulation of pre-I (I-driver) neurons, which are known to provide
excitatory drive to inspiratory neurons exhibiting augmenting (I-AUG)
and decrementing (I-DEC) patterns of discharge (Segers et al.
1987
). In computer simulations inferred from spike train
cross-correlation data (Balis et al. 1994
) and the
mathematical model of a network oscillator by Ogilvie et al.
(1992)
, increasing excitation of I-AUG neurons decreases Ti and
increases the slope of the inspiratory ramp (i.e., produces a "square
wave" discharge), whereas increasing excitation of I-DEC neurons
lengthens Ti (i.e., produces apneusis). Thus it is possible that focal
hypoxia in the pre-BötC stimulated this population of pre-I
(I-driver) neurons that in turn synaptically altered the activity of
other inspiratory-modulated neurons (i.e., I-AUG and/or I-DEC) to
produce the differences in the cycle timing (i.e., rhythm) and pattern
seen in our experiments.
Mechanisms of hypoxic excitation
The cellular mechanisms by which focal hypoxia in the
pre-BötC produced excitation of inspiratory motor output in our
current study are not known. It is unlikely that the excitation
resulted from pathological consequences of O2
lack associated with impairment in cell functions because the responses
to microinjection were rapid, completely reversible, and reproducible
over many trials (even before recovery to eupnea). More likely, the
excitation represents a direct cellular signaling process comparable
perhaps to those of the carotid bodies, in which application of cyanide in doses comparable with those used here similarly results in rapid
vigorous stimulation (Biscoe et al. 1988).
Within a neural network, however, other possibilities must be
considered. For example, hypoxia may elicit excitatory transynaptic mechanisms via activation of glutamate receptors or indirect
facilitation mediated by withdrawal of a tonic GABAergic input. Hypoxia
has been shown to increase release of glutamate in some regions of the
brain (Hagberg et al. 1985; Rothman and Olney
1986
), which may potently excite
N-methyl-D-aspartate receptors (Goldberg
et al. 1987
; Rothman 1984
). It is unlikely that
the excitation of phrenic motor output reported in our study resulted
simply from hypoxic release of glutamate because hypoxic excitation of
phrenic nerve discharge was only seen in a portion of the sites in
which the glutamate analogue DLH elicited excitatory effects. In
addition, preliminary evidence from our laboratory suggests that
microinjection of NaCN into the pre-BötC following focal
administration of the broad spectrum ionotropic EAA receptor antagonist
kynurenic acid (Collingridge and Lester 1989
), in a dose
that blocks the DLH-induced excitation, is ineffective in abolishing
the NaCN-induced response (unpublished observation).
Activation of GABAA receptors requires
ATP-dependent phosphorylation to maintain functional integrity
(Chen et al. 1990; Shirasaki et al. 1992
;
Stelzer et al. 1988
). During severe hypoxia, reduced ATP
availability may limit phosphorylation, resulting in disinhibition. In
our experiments, the responses to NaCN occurred within seconds, so it
is unlikely that ATP levels would have decreased significantly. In
fact, previous studies have shown that ATP levels change very little in
carotid body after brief periods of hypoxia (Verna et al.
1990
) or exposure to cyanide (Obesö et al.
1989
), and that the responses to cyanide occur in both the
presence and absence of intracellular ATP (Biscoe and Duchen
1989
).
Effects of focal hypoxia in the pre-Böt complex on arterial blood pressure
In most of our sites, the augmentation of inspiratory output was
accompanied by a pressor or depressor response; however, we did
encounter sites in which no blood pressure changes were observed.
Although focal hypoxia in the RVLM is known to increase sympathetic
nerve discharge and arterial blood pressure (Mitra et al.
1993; Sun et al. 1992
), it is unlikely that the
increases in blood pressure reported here resulted from direct hypoxic
stimulation of sympathoexcitatory vasomotor neurons located in the
RVLM. In this region of the RVLM, focal hypoxia has been shown to not
only increase arterial blood pressure but also depress phrenic nerve activity (Mitra et al. 1993
; Sun et al.
1992
). In addition, the RVLM region containing the C1 neuronal
population (McAllen and Dampney 1989
) is located rostral
and ventral to the pre-BötC. It seems more likely that the
increases in blood pressure observed in our study resulted from
enhanced respiratory modulation of sympathetic activity (Bachoo
and Polosa 1987
; Darnall and Guyenet 1990
;
Solomon et al. 1997
). This proposal is supported by
neuroanatomic studies using intracellular biocytin injections
demonstrating that inspiratory neurons originating in the rostral rVRG
(some in the vicinity of the pre-BötC) project directly onto
tyrosine hydroxylase immunoreactive neurons located in the RVLM
(Pilowsky et al. 1994
), suggesting that these
respiratory neurons may provide direct synaptic input to RVLM
sympathoexcitatory neurons.
Our data provide no insight into the mechanism responsible for the production of the depressor responses reported here. Whether respiratory neurons originating in this region provide inhibitory synaptic inputs to sympathoexcitatory neurons of the RVLM or project directly to depressor regions of the caudal ventrolateral medulla remains to be determined.
Conclusion
Our experiments have identified a locus in the brain stem in which focal hypoxia augments respiratory output. Using discrete focal hypoxic stimulation, our data provide strong evidence to suggest that the respiratory rhythm generator in the pre-BötC has intrinsic hypoxic chemosensitivity resulting in modulation of phrenic motor output. It should be noted that in the in vitro transverse medullary slice model, rendering the entire slice hypoxic has been shown to result in excitation of pre-BötC neurons and hypoglossal nerve activity. In our experiments, we have demonstrated that focal hypoxia in discrete regions of the pre-BötC produces increases in respiratory burst frequency and tonic discharge of inspiratory output, as well as modulation of burst pattern in vivo. This hypoxic excitation of inspiratory motor output appears at this time to be specific to the pre-BötC. The findings establish the potential for hypoxic chemosensitivity in the brain stem for the respiratory control system.
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ACKNOWLEDGMENTS |
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The authors thank T. Le Hoang and J. Cooper for technical assistance.
This work was supported by a grant from the National Heart, Lung, and Blood Institute (HL-16022). I. C. Solomon was supported by a postdoctoral fellowship from the American Heart Association, New Jersey Affiliate.
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FOOTNOTES |
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Address for reprint requests: I. C. Solomon, Dept. of Physiology and Biophysics, Health Sciences Center, Basic Science Tower, Level 6, Rm. 140, State University of New York at Stony Brook, Stony Brook, NY 11794-8661.
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 27 August 1999; accepted in final form 26 January 2000.
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REFERENCES |
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