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First published online March 2, 2006
Journal of Experimental Biology 209, 1135-1146 (2006)
Published by The Company of Biologists 2006
doi: 10.1242/jeb.02106
Chronic hypercapnia modulates respiratory-related central pH/CO2 chemoreception in an amphibian, Bufo marinus
The Centre for the Neurobiology of Stress, Department of Life Sciences, University of Toronto at Scarborough, 1265 Military Trail, Toronto, Ontario, M1C 1A4, Canada
* Author for correspondence (e-mail: sgreid{at}utsc.utoronto.ca)
Accepted 24 January 2006
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Key words: brainstem–spinal cord, central pH/CO2 chemoreceptors, chronic hypercapnia, hypercapnic ventilatory response, olfactory CO2 chemoreceptor, cane toad, Bufo marinus
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; Taylor et al.,
2003b). The peripheral chemoreceptors in the aortic body and
carotid labyrinth (Macintyre and Toews,
1976; West et al.,
1987) are stimulated by changes in arterial pH/CO2,
contributing approximately 25% of the increase in respiratory drive during
acute hypercapnia (Smatresk and Smits,
1991; Van Vliet and West,
1992). Olfactory CO2 chemoreceptors, located in the
nasal epithelium, reduce breathing frequency when stimulated by increased
levels of inspired CO2 (Kinkead
and Milsom, 1996; Coates,
2001; Milsom,
2002). Furthermore, pulmonary stretch receptor (PSR) discharge in
anurans is CO2 sensitive with increasing levels of CO2
inhibiting PSR activity (Milsom and Jones,
1977; Kuhlman and Fedde,
1979). The effect of PSR feedback on breathing in anurans is
complex in itself and depends upon whether or not the pattern of feedback is
phasic or tonic and also on the state of lung inflation at the time of PSR
feedback (Kinkead et al.,
1994; Kinkead and Milsom,
1996; Wang et al.,
1999; Wang et al.,
2004; Reid et al.,
2000b; Saunders and Milsom,
2001; Reid and West,
2004). Pulmonary vagotomy, which eliminates PSR feedback to the
brain, abolishes the acute hypercapnic ventilatory response
(Reid et al., 2000b).
Air-breathing animals are rarely faced with exposure to acute or chronic
hypercapnia (CHC). Exceptions to this generalisation include those animals
that live in underground burrows (Boggs et
al., 1984; Kuhnen,
1986). Burrowing animals that live underground and breathe
relatively high levels of CO2 have, for the most part, a reduced
ventilatory response to acute hypercapnia compared to non-burrowing species
(Boggs et al., 1984). In
temperate climates during the winter months, many terrestrial amphibians
burrow into the soil (Pinder et al.,
1992) or occupy burrows made by mammals. For example, the adult
plains spadefoot toad (Scaphiopus bombifrons)
(Russell and Bauer, 1993), the
Manitoba toad (Bufo hemiophrys)
(Breckenridge and Tester, 1961)
and the Canadian toad (Bufo hemiophrys) will bury between 0.5 and 1.3
m during the winter while the Boreal toad (Bufo boreas) and the Great
Plains toad (Bufo cognatus) may also over-winter in rodent burrows.
Although measurements of O2 and CO2 levels in these
temperate microhabitats have not been reported, it is possible that these
burrows also become hypoxic and hypercapnic.
Boutilier et al. (Boutilier et al.,
1979b) reported elevated arterial PCO2 levels
(approximately 15 mmHg) in burrowing cane toads whose nares were open to the
air while the skin was surrounded by sand at 25°C for 6 days. Boutilier et
al. (Boutilier et al., 1979a)
state that it is not uncommon for cane toads to encounter hypercapnic
conditions in their environment, including hypercapnic waters in the tropics
(Toews and Macintyre, 1978).
Whereas the cardiorespiratory responses to acute hypercapnia in amphibians
have been well studied, the effects of prolonged exposure to hypercapnia have
not been addressed. A recent study, on cane toads, from this laboratory
(McAneney et al., in press)
demonstrated that exposure to chronic hypoxia blunts the acute hypoxic
ventilatory response but does not alter resting levels of ventilation.
The goal of this study was to address the hypothesis that CHC would alter
respiratory-related CO2 chemoreceptor function and reduce the
overall hypercapnic ventilatory response to a subsequent bout of acute
hypercapnia. Cane toads (Bufo marinus; a species in which respiratory
physiology has been well studied) were exposed to CHC for 9 days, following
which central pH/CO2 chemosensitivity was assessed using in
vitro brainstem–spinal cord preparations and whole animal
hypercapnic ventilatory responses were measured in vivo. A midbrain
transection slightly caudal to the optic chiasma was previously demonstrated
to reduce the clustering of breaths into episodes and cause an increase in
fictive breathing frequency in vitro
(Reid et al., 2000a). We
hypothesised that a change in descending inputs, from the level of the optic
chiasma, would alter CO2 chemosensitivity following CHC.
Furthermore, given that CHC would continually stimulate olfactory
CO2 chemoreceptors, we hypothesised that an increase in central
pH/CO2 chemosensitivity would occur to counter an increase in
inhibitory input from olfactory chemoreceptors during CHC. Midbrain
transection (in vivo and in vitro) and olfactory denervation
(in vivo) experiments addressed these two hypotheses.
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Exposure to chronic hypercapnia
Toads were placed, for a 9 day period, into a Plexiglas chamber (35
cmx25 cm) within which the inspired CO2 level was maintained
at 3.5% using a Pro-CO2 control unit (Biospherix, NY, USA). A
CO2 electrode, within the chamber, monitored the level of
CO2. When the CO2 concentration fell below 3.5%, the
Pro-CO2 delivered a small amount of CO2 to raise the
level back to 3.5%. In this manner, the amount of CO2 was
maintained at a constant level within the chamber at all times. A level of
3.5% CO2 was selected as it approximates the average CO2
concentration found in mammalian burrows based on a study of 15 different
species (Kuhnen, 1986).
Routine measurements of O2 (S-3A O2 analyser, AEI,
Pittsburgh, PA, USA) confirmed that inspired O2 levels remained at
approximately 20.2%. The chamber was maintained at room temperature and
exposed to a 12 h:12 h light:dark cycle.
In vitro experiments
The in vitro brainstem-spinal cord preparation
Toads were anaesthetised by emersion in a solution of 3-aminobenzoic acid
ethyl ester (MS222, 1.0 g l–1; Sigma) neutralised with sodium
bicarbonate. Animals were kept in the anaesthetic until the eye-blink and
toe-pinch reflexes were eliminated. Using a Dremmel Tool, a longitudinal
incision was made in the skull rostral to the optic lobes and the cranial case
was removed with Rongeurs and bone shears, and placed onto a Sylgard-coated
dissecting dish. The brain was exposed and superfusion with ice-cold
oxygenated artificial cerebrospinal fluid (aCSF) was initiated; the rostral
forebrain was then removed. The remaining brain tissue was continually
superfused with the aCSF (in mmol l–1; NaCl, 103; KCl, 4.05;
MgCl2, 1.38; glucose, 10; NaHCO3, 29.2;
CaCl2, 2.45; pH 7.8) (Taylor et
al., 2003a; Taylor et al.,
2003b).
Cranial nerves were cut close to their exit to the skull and the spinal
cord was severed at the level of the third spinal nerve. The preparation was
transferred from the brain case and immobilised with insect pins in a
Sylgard-coated dissecting dish continually superfused with oxygenated aCSF.
The meninges surrounding the brain were removed in order to free the cranial
nerve roots, and the nerve tips were cut to provide a clean surface for
recording. The preparation was then pinned, ventral side up, onto a fine
stainless steel mesh within a superfused recording chamber. The mesh divided
the chamber into upper and lower compartments, which ensured simultaneous
superfusion of both surfaces of the preparation
(McLean et al., 1995). The
preparation was continuously superfused with oxygenated aCSF, at a rate of 10
ml min–1, using peristaltic pumps that delivered and removed
the aCSF from the chamber. The aCSF was recycled. The preparations were
maintained at pH 7.8 and room temperature for 60 min before commencing the
experiment.
Suction electrodes of various diameters were made from thin-walled
capillary glass (1 mm diameter) pulled to a fine tip using a vertical pipette
puller (Kopf model 720, Tujunga, CA, USA). The tips were polished using a
grinding stone and flame to provide a smooth surface. Using a
micro-manipulator, an appropriately sized suction electrode was positioned
near the end of the vagus nerve root and the nerve was carefully aspired into
the electrode such that a tight seal was obtained between the nerve and the
electrode. In all preparations, recordings were taken of whole nerve discharge
from the vagus nerve. In the intact animal, a branch of the vagus nerve
innervates the glottis, which opens and closes with each breath. Since these
preparations are devoid of any afferent input and breathing is an inherently
rhythmic process generated in the brainstem, all rhythmic activity (in
vitro motor output) recorded from the vagus nerve was assumed to
represent motor output to the respiratory muscles (glottis) and is therefore
an index of breathing termed fictive breathing
(Sakakibara, 1984a;
Sakakibara, 1984b;
Kinkead et al., 1994;
McLean et al., 1995;
Reid and Milsom, 1998;
Reid et al., 2000a;
Reid et al., 2000b;
Morales and Hedrick, 2002;
Taylor et al., 2003a;
Taylor et al., 2003b).
Nerve activity from the suction electrode was amplified (10x) and filtered (30 Hz, high pass; 3 kHz, low pass) using a DAM50 AC amplifier [World Precision Instruments (WPI), Sarasota, FL, USA]. The output from the DAM50 was sent to a second AC amplifier (ISO8A, WPI) and amplified a further 100x. The amplified nerve signal from the ISO8A was sent to a moving averager (CWE MA821/RSP) for integration (time constant=200 ms) and to an audio monitor (AM Systems Model 3300, Carlsborg, WA, USA). The amplified/filtered nerve signal and integrated trace were monitored and stored using a data acquisition system (Biopac Systems, MP150, Goleta, CA, USA). The sampling rate of the analogue to digital conversion was 2000 Hz.
Gassing the aCSF with varying levels of CO2 (0–5%; balance O2) altered the aCSF pH. The levels of CO2 and O2 gassing the aCSF were set using digital mass flow controllers (Smart-Trak 100, Sierra Instruments, Monterey, CA, USA). The pH level of the aCSF was monitored using a pH electrode placed within the aCSF reservoir.
Series 1: effects of CHC on pH-sensitive fictive breathing
Following the 1 h stabilisation period and the observation of stable levels
of neural discharge (fictive breathing), the pH of the aCSF was lowered from
7.8 to 7.4. The pH was then raised by 0.2 units every 30 min until a pH of 8.2
was achieved. This pH range approximates that used in previous studies on
amphibian brainstem–spinal cord preparations (e.g.
McLean et al., 1995;
Reid and Milsom, 1998). All
experiments were performed at room temperature (approximately 22°C). This
is within the temperature range (15–25°C) reported
(Morales and Hedrick, 2002) in
which fictive breathing is consistently active from in vitro adult
bullfrog preparations. This protocol was performed on brains taken from
control (N=6) and chronically hypercapnic (N=6) toads.
Series 2: effects of CHC and midbrain transection on pH-sensitive fictive breathing
This series used separate groups of toads from those used in series 1. The
preparation was prepared as described above. Following the 1 h stabilisation
period, the pH of the aCSF was increased to 8.0 and then lowered to 7.8 and
7.5 in 30 min intervals. Following this, the brain was transected slightly
caudal to the optic chiasma at a level previously demonstrated to
significantly attenuate (and almost abolish) episodic (clustered) fictive
breathing (Reid et al., 2000a)
as well as alter the pH sensitivity of fictive breathing in brains taken from
chronically hypoxic toads (J. McAneney and S. Reid, unpublished data).
Following a second 1 h stabilisation period, the pH changes (8.0, 7.8 and 7.5)
were repeated. This protocol was performed on brains taken from control
(N=8) and chronically hypercapnic (N=9) toads.
In vivo experiments
Series 3: breathing during the 9 days of CHC
In these experiments, breathing was measured by impedance as the per breath
movement of the body wall. Toads were anaesthetised with MS222 as described
above. Impedance leads, fabricated from thin insulated copper wire, were
sutured to the flanks of the animal at the site of maximal displacement during
lung inflation and deflation. We have previously validated impedance
measurements as an appropriate measure of breathing in this species
(McAneney et al., in press).
Following a 48 h recovery period, toads were placed into the chronically
hypercapnic chamber (described above) for 9 days. On each day of exposure to
3.5% CO2, in vivo, breathing was recorded for 1 h and 15
min while the animals remained in the CHC chamber. To measure breathing, the
impedance leads were connected to extensions which, in turn, input into an
impedance converter (UFI, Morro Bay, CA, USA; model 2991). The signal from the
impedance converter was recorded using a digital data acquisition system (DI
194; DataQ Systems, Akron, OH, USA) at a sampling rate of 120 Hz.
Series 4: effects of CHC and midbrain transection on the hypercapnic ventilatory response
Four groups of animals were studied in this series: (1) control, midbrain
intact (N=9); (2) control, midbrain transected (N=8); (3)
CHC, midbrain intact (N=8) and (4) CHC, midbrain transected
(N=7).
Toads were anaesthetised and fitted with impedance leads as described above. In the midbrain-transected toads, following attachment of the impedance leads, a narrow opening was drilled in the skull slightly caudal to the optic chiasma. The brain was then transected using a sharp blade. The small hole was packed with cotton and covered with dental dam held in place by superglue. Following a 48 h recovery period the animals were placed into control or chronically hypercapnic conditions for 9 days. The surgical procedure used to open the skull in order to perform the in vivo brain transection is relatively minor and was performed at the same time as the impedance leads were sutured to the toads. As such, the control animals also underwent anaesthesia although non-transected control animals did not undergo any sham treatment (a hole drilled in the skull without transecting the brain) because this is not a very invasive procedure.
Following 9 days of CHC (or control conditions) acute breathing trials were performed within a small (15 cmx15 cmx9 cm) plastic chamber in which the animals were exposed to increasing concentrations of inspired CO2. Toads were placed into the experimental chamber for 1 h prior to commencing the breathing trials. During this period, the chamber was ventilated (1 l min–1) with room air. The chamber was then gassed with increasing concentrations of CO2 (2.5%, 3.5%, 4.5% and 5.5%; 20 min per level). These CO2 levels were achieved by mixing CO2 with air using Aalborg (Georgetown, NY, USA; model GFC 171) and Sierra (Smart Trak 100) digital mass flow controllers. The levels of CO2 and O2 within the experimental chamber were continuously monitored using CO2 (CD-3A, AEI Technologies) and O2 (S-3A/I, AEI Technologies) analysers.
Series 5: effects of CHC and olfactory denervation on the hypercapnic ventilatory response
Toads were anaesthetised, as described above, and fitted with impedance
leads. In the olfactory-denervated groups, a thin slit was drilled in the
skull above the border between the olfactory lobes and the forebrain. A sharp
blade was inserted through the hole to cut the olfactory nerves. The hole was
then packed with cotton and covered with dental dam. Sham experiments were not
performed for reasons described above. The animals were allowed to recover for
48 h before being divided into the following four groups: (1) normocapnic
controls (olfactory nerves intact; N=9); (2) normocapnic controls
(olfactory denervated; N=6); (3) chronically hypercapnic (olfactory
nerves intact; N=8); and (4) chronically hypercapnic
(olfactory-denervated; N=7). Each group subsequently underwent acute
breathing trials.
Before beginning the acute breathing trials, animals were exposed to room air for 60 min. At the end of this period, the animals were exposed to acute hypercapnia (21% O2; 5% CO2) for 20 min and then returned to room air for 20 min.Throughout these trials, the O2 and CO2 levels within the chamber were monitored with the O2 and CO2 analysers, respectively. Olfactory denervation was confirmed, post mortem, by autopsy.
Data analysis
In vitro: in series 1 and 2, the final 10 min of data at each pH
level was analysed to determine mean values for fictive breathing frequency
(fictive breaths min–1), the number of fictive breaths per
episode, the number of fictive episodes per minute and fictive breath duration
(s). Fictive breaths in a given episode were defined as occurring within 2 s
of each other, according to general practices in the literature
(Kinkead et al., 1997;
Reid and Milsom, 1998). The
area under the integrated (moving average) trace may be taken as an index of
fictive breath amplitude. However, given that respiratory-related motor output
from the vagus is primarily related to glottal opening and closing [laryngeal
branch of the vagus (Sakakibara,
1984a)] rather than buccal pumping [pharyngeal posterior superior
branch of the vagus (Sakakibara,
1984a; Sakakibara,
1984b)], integrated vagal activity may not be the ideal index of
breath amplitude or tidal volume. A larger breath would, presumably, require
that the glottis remain open for a longer period of time.
To further examine whether the output/sensitivity of central respiratory-related chemoreceptors was altered by CHC in series 1 and 2 (prior to transection) the slopes of the pH-fictive breathing dose–response curves (first order regression) were determined for each animal and a mean value was obtained.
In vivo: in series 3 and 4, the final 10–15 min of each experimental period was analysed to determine breathing frequency, breaths per episode, episodes per minute and breath duration. To determine breath amplitude, any DC offset was mathematically subtracted from the impedance trace and the resulting trace was integrated using the DI194 analysis software. The integrated area of the breath was taken as a measure of breath amplitude or tidal volume. The product of breathing frequency and breath amplitude gave an index of total ventilation.
In series 5, values for breathing frequency were determined for the last 10
min of each 20 min period during exposure to room air and 5% CO2.
Following the return to air, this value was determined for the first 5 min
following the CO2 to air transition in order to examine the
CO2-off response (Kinkead and
Milsom, 1996). Since the olfactory chemoreceptors affect breathing
frequency, other variables were not analysed.
Statistical analysis
In vitro: in all in vitro experiments, the values at each
pH level in the control and chronically hypercapnic groups, were compared with
a one-way repeated measures (RM) analysis of variance (ANOVA) followed by a
Dunn's multiple comparison test with a single control point (the highest pH
value). In series 1, differences between the control and chronically
hypercapnic group were analysed using a two-way ANOVA with pH and control/CHC
as the two factors. In series 2, the effects of midbrain transection, CHC and
pH were assessed with a three-way ANOVA. In series 1 and 2, the slopes of the
dose response curves were compared using a t-test (control
versus CHC).
In vivo: in series 3, the values on each day were compared using a one-way RM ANOVA followed by a Dunn's multiple comparison test. In series 4, the effects of acute hypercapnia were analysed within each group using a one-way RM ANOVA. The effects of CHC and midbrain transection were analysed using a three-way ANOVA. In series 5, the effects of CHC and olfactory denervation were compared using a two-way ANOVA.
All statistical analysis was performed using commercial software (SigmaStat 3.0, Jandel Scientific (SPSS), Chicago, IL, USA). The software determined the appropriate parametric or non-parametric tests as well as the appropriate post-hoc multiple comparison test, which followed all analyses of variance. In all cases, the limit of significance was set at 5% (P=0.05).
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Series 2 (midbrain transection in vitro)
In this series, consistent with the data in series 1, CHC caused an
increase, compared with the control group, in fictive breathing frequency at
each pH level (Fig. 2A;
P<0.001). These differences were a result of an increase in the
number of fictive episodes per minute (Fig.
2B; P<0.001) rather than the number of fictive breaths
per episode (Fig. 2C). Midbrain
transection had no effect on the frequency response to altered aCSF pH in
either the control (P=0.901) or CHC (P=0.803) groups
(Fig. 2A). By contrast,
midbrain transection caused a significant increase (P=0.008) in the
number of fictive episodes per minute in the control group at pH levels of 8.0
and 7.8. This increase did not translate into an increase in fictive breathing
frequency because of the non-significant trend for transection to reduce the
number of fictive breaths per episode in the control group (P=0.218;
Fig. 2C).
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With respect to fictive breathing frequency and episodes per minute, the results of the three-way ANOVA did not reveal any interactive effects between CHC, transection and pH. However, further analysis revealed that the slope of the breathing frequency response curve (pre-transection) in Fig. 2A was greater (P=0.016) in the CHC group (slope=–15.1±3.8 fictive breaths min–1 pH unit–1) than in the control group (–4.2±1.6 fictive breaths min–1 pH unit–1). There was also a significant (P=0.014; three-way ANOVA) interaction between CHC, pH and transection with respect to fictive episodes per minute.
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Series 4 (hypercapnic ventilatory responses in vivo)
Exposure to acute hypercapnia in vivo, with the midbrain intact,
caused a significant increase in breathing frequency in both the control
(P<0.001) and CHC (P=0.002) animals
(Fig. 4A, asterisks). This was
mediated by an increase in the number of breaths per episode (control,
P<0.001; CHC, P=0.004;
Fig. 4B) rather than the number
of episodes per minute (Fig.
4C). There was no effect of CHC on breathing frequency
(P=0.342), breaths per episode (P=0.579) or episodes per
minute (P=0.218).
Following transection of the midbrain, acute hypercapnia caused a large increase in breathing frequency (Fig. 4A, asterisks; control and CHC; P<0.001) that was mediated by changes in the number of episodes per minute (Fig. 4C, asterisks; control, P=0.001; CHC, P=0.017). In both the control and CHC groups, midbrain transection caused a significant increase in breathing frequency (Fig. 4A, double daggers; P<0.001) and episodes per minute (Fig. 4C, double daggers; P=0.023) as well as a significant decrease in the number of breaths per episode (Fig. 4B, double daggers; P<0.001). Acute hypercapnia did not alter breath amplitude in either group both before and after midbrain transection (Fig. 4D). In the CHC group, midbrain transection caused a significant decrease in breath amplitude when the animals were breathing 4.5% and 5.5% CO2 (P<0.001).
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Breath duration increased in the CHC group during exposure to acute hypercapnia before brain transection (Fig. 4F, asterisks; P<0.001). This did not occur in the control group (P=0.096). Brainstem transection caused a significant decrease in breath duration in both groups (Fig. 4F, double daggers; P<0.001).
Series 5 (olfactory denervation in vivo)
Fig. 5A,C illustrates that,
during the acute hypercapnic breathing trials, breathing frequency increased
during exposure to 5% CO2 in control and CHC toads
(P<0.001). Upon return to air (CO2-off), breathing
frequency increased in both groups in an identical manner (P=0.975).
Following olfactory denervation, breathing frequency increased during exposure
to 5% CO2 in both the control
(Fig. 5B) and CHC
(Fig. 5D) groups. However, upon
return to air (CO2-off) the breathing frequency in the denervated
animals did not change in the control group
(Fig. 5B; P=1.00) but
decreased in the CHC group (Fig.
5D; P<0.001).
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The increase in central pH/CO2 chemosensitivity could be
explained by a change (increase) in any of the stages in the signal
transduction pathway (Lahiri and Forster,
2003) from the chemoreceptor cell to respiratory motor output.
Reid et al. (Reid et al.,
2000a) demonstrated, using in vitro
brainstem–spinal cord preparations from the bullfrog, that a transection
slightly caudal to the optic chiasma converted episodic fictive breathing to
continuous fictive breathing with a concomitant increase in fictive breathing
frequency. A recent study from this laboratory (J. McAneney and S. Reid,
unpublished) demonstrated that, in cane toads, 10 days of exposure to chronic
normobaric hypoxia (10% O2) tended to cause a decrease in central
pH/CO2 chemosensitivity measured using the in vitro
brainstem–spinal cord preparation. Furthermore, a transection caudal to
the optic chiasma greatly enhanced the pH/CO2 chemosensitivity that
had been attenuated by chronic hypoxia. Given these previous results, we
hypothesised that the increase in central pH/CO2 chemosensitivity
observed in this current study may have resulted from modulation of medullary
pH/CO2 chemoreceptors by midbrain influences.
If CHC caused changes in mechanisms within the midbrain that influence central chemosensitivity, then one could predict that transection of the midbrain would abolish this enhancement. In the current study in vitro, the dose response curves in the CHC group were the same before and after midbrain transection (two-way ANOVA). This suggests that descending inputs do not appear to be involved in the CHC-induced increase in the overall magnitude of fictive breathing at each pH level (see below, in vivo versus in vitro differences for further discussion).
Other possible mechanisms responsible for CHC-induced augmentation of fictive breathing
Another possible explanation for the increase in central pH/CO2
sensitivity is an increase in the activity or amount of carbonic anhydrase
(CA) within the respiratory-related chemoreceptor cells. CA catalyses the
hydration of CO2 to H+ and
HCO3– ions and has been shown to be important in
H+/CO2 sensing in the carotid body glomus cells as well
as in the O2–CO2 interaction in the carotid body
(Iturriaga and Lahiri, 1991).
Lipid membranes are generally impermeable to H+ ions but diffusion
of CO2 into a chemoreceptor cell can cause intracellular
acidification. An increase in CA activity may account, at least in part, for
the increased central chemosensitivity following CHC.
Another possibility is that altered feedback from lung pulmonary stretch
receptors (PSR), during the period of CHC, may have modulated the function of
the central CO2 chemoreceptors. In anurans, pulmonary vagotomy
eliminates the acute hypercapnic ventilatory response
(Reid et al., 2000b) and
electrical stimulation of the pulmonary vagus nerve, in vitro,
enhances central CO2 chemosensitivity
(Kinkead et al., 1994). PSR
feedback, therefore, is important for regulating respiratory-related central
pH/CO2 chemosensitivity. Furthermore, PSR are CO2
sensitive, with increased levels of CO2 causing a decrease in
receptor activity (see below).
Alternately, given that CHC leads to elevated levels of breathing during the 9 day exposure to elevated CO2, it is possible that CHC is also associated with elevated arterial PO2 levels. Given that cane toads are discontinuous breathers, arterial gas levels fluctuate depending upon whether or not the animals are breathing, the time taken between breathing episodes and the presence or absence of cardiac shunting. If CHC induces more-or-less continuous breathing (as it appears to do based on Fig. 3A), then arterial PO2 levels would probably be elevated compared to an animal breathing air in a discontinuous manner. Given this, one may hypothesise that reduced levels of afferent input from the carotid labyrinth/aortic arch O2 chemoreceptors may have altered central pH/CO2 chemoreceptor function. However, these arterial chemoreceptors are also sensitive to pH/CO2 so increased afferent input may have occurred during CHC. Regardless, the possibility remains that peripheral chemoreceptor input modified central chemoreceptor function. We are currently investigating the role of carbonic anhydrase, PSR feedback and O2 chemoreceptor afferent input on central pH/CO2 chemosensitivity following CHC.
In the control (not chronically hypercapnic) animals, there was no increase
in fictive breathing with reduced aCSF pH in series 1 although there was a
small but significant increase in series 2. A reduced pH sensitivity in
vitro is not unexpected given the absence of afferent input to the
brainstem–spinal cord preparation
(Milsom et al., 1999). Indeed,
Morales and Hedrick (Morales and Hedrick,
2002) reported that fictive breathing frequency, recorded from an
adult bullfrog brainstem–spinal cord preparation, changed from
approximately 1.5 to 3.75 fictive breaths min–1 as the pH of
the aCSF was lowered from 8.3 to 7.5 at 20°C. The magnitude of this
relatively small change is similar to the small change observed in the current
study in the control preparations (5.5–8.5 fictive breaths
min–1 with a pH change from 8.2 to 7.4). Nevertheless, it is
without doubt that these preparations are pH sensitive. The observation that
central respiratory-related pH sensitivity is reduced in vitro,
compared to in vivo, further suggests that enhanced afferent input
during CHC may have altered central pH chemoreceptor function.
In vitro versus in vivo responses
The in vivo experiments (series 3) demonstrated that there was a
sustained increase, over resting levels (day 0) in breathing frequency during
the 9 days of CHC. Given that the central pH/CO2 chemoreceptors are
responsible for the majority of the acute hypercapnic ventilatory response in
anuran amphibians (Branco et al.,
1992; Smatresk and Smits,
1991), and that central chemoreceptor activity was elevated in the
in vitro experiments following CHC, it is possible that the sustained
increase in breathing frequency in vivo was a result of continual
activation of these receptors.
Studies on ventilatory responses and blood acid–base changes to
hypercapnia in anuran amphibians have typically focused on the time scale of
several minutes to 24 h. Toews and Heisler
(Toews and Heisler, 1982)
demonstrated, in Bufo marinus, that 24 h of hypercapnia (5%
CO2) produced a 30% pH compensation in the extracellular fluid and
44%, 65% and 77% compensation in the intracellular compartments of skin,
skeletal muscle and cardiac muscle, respectively. These authors concluded that
this species preferentially regulates intracellular, over extracellular, pH
during this time frame of hypercapnia. Boutilier and Heisler
(Boutilier and Heisler, 1988)
also demonstrated a relatively limited capacity to compensate extracellular pH
(approximately 30% compensation) following 24 h of exposure to 5%
CO2 in Bufo. Snyder and Nestler
(Snyder and Nestler, 1991)
demonstrated that the brain of Bufo marinus has a relatively low
buffering capacity compared to the liver. It is possible that a poor or
comparatively reduced buffering capacity may have contributed to the
maintained elevation of breathing during the 9 days of CHC in the current
study. A limited buffering capacity in the brain may have facilitated the
increased sensitivity of the central pH/CO2 chemoreceptors. The
continual elevation of breathing frequency over the 9 dayperiod suggests the
occurrence of a persistent respiratory acidosis. However, breathing frequency
had returned to resting levels following 1 h exposure to room air at the
beginning of the acute in vivo breathing trials (series 4). This
would suggest that the in vivo hypercapnic ventilatory chemoreflex,
that we measured, was not being attenuated by a continual respiratory
acidosis, although blood pH and PCO2 measurements would be
required to confirm this. The continual elevation of breathing frequency
during CHC is consistent with comparable studies on rats
[(Lai et al., 1981) 3 weeks of
CHC], dogs [(Jennings and Chen,
1976) 14 days of CHC] and humans
[(Schaefer et al., 1963) 42
days of CHC]. However, McKenzie et al.
(McKenzie et al., 2003)
demonstrated that 6 weeks of CHC (water PCO2=15–45
mmHg) did not result in an elevation of breathing in the European eel
(Anguilla anguilla).
Given that burrowing animals, exposed to relatively high levels of
CO2, generally have a reduced acute hypercapnic ventilatory
response, we hypothesised that CHC would reduce the respiratory response to a
subsequent bout of acute hypercapnia in cane toads. Clearly this hypothesis
was not supported by either the in vitro or in vivo
experiments. The results indicate that the increase in central
pH/CO2 sensitivity measured in vitro does not manifest as
an increase in the acute hypercapnic ventilatory response in vivo.
Furthermore, midbrain transection in vivo augmented the acute
hypercapnic ventilatory response whereas in vitro there was no
apparent effect. Given the multiple populations of CO2-sensitive
respiratory-related chemoreceptors in these animals and the central
integration of chemoreceptor drive
(Kinkead et al., 1997;
Gargaglioni and Branco, 2004),
this result perhaps is not surprising. In vivo, it is possible that
the transections (slightly caudal to the optic chiasma) may have influenced
the function of the nucleus isthmi which is a midbrain structure that has
previously been shown to be important in the hypercapnic ventilatory response
in anurans (Kinkead et al.,
1997; Gargaglioni and Branco,
2004). Further experiments will examine the role of the nucleus
isthmi on central chemosensitivity following CHC by pharmacologically ablating
(Kinkead et al., 1997) the
nucleus isthmi prior to CHC and in vitro experiments.
Brain transection did, however, alter the breathing pattern during acute hypercapnia. With the brains intact, the increase in breathing frequency was mediated by an increase in the number of breaths per episode while the number of episodes per minute remained constant. Following transection, the acute hypercapnic ventilatory response (frequency) was mediated by increases in episodes per minute while breaths per episode did not change. These data are consistent with the differential regulation of these two components of breathing frequency. At the higher levels of inspired CO2, this is also consistent with breathing becoming more-or-less continuous rather than clustered or episodic.
Olfactory CO2 chemoreceptors in the nares inhibit breathing
frequency. As such, following exposure to acute hypercapnia, there is an
immediate increase in breathing frequency following a return to breathing room
air. This paradoxical increase in breathing frequency, at a time when the
CO2 drive to breathe is decreasing, results from removal of this
inhibitory input (Kinkead and Milsom,
1996; Coates,
2001). Kinkead and Milsom
(Kinkead and Milsom, 1996)
observed that olfactory denervation in the bullfrog enhanced the increase in
breathing frequency during acute hypercapnia (6% CO2; 1 h). This
enhancement was not observed in the current study during acute hypercapnia (5%
CO2; 20 min). The differences may be due to the slightly different
experimental protocols.
We hypothesised that the lack of an augmented in vivo hypercapnic ventilatory response following CHC may have resulted from increased inhibitory input from these olfactory CO2 chemoreceptors, which in turn, may have nullified an augmentation of central chemoreceptor function. However, although olfactory denervation appeared to reduce breathing frequency during acute hypercapnia, this effect was observed in both the control and CHC groups, suggesting that CHC did not alter the inhibitory input from these receptors. Changes in these receptors do not appear to cause the in vitro versus in vivo differences observed in this study.
However, following olfactory denervation in the chronically hypercapnic
group, breathing frequency decreased upon return to normocapnic conditions
(Fig. 5D). This was not
expected, as any respiratory acidosis immediately following acute 5%
CO2 exposure would probably have had a greater stimulatory effect
in the chronically hypercapnic group because of the increased sensitivity of
the central CO2 chemoreceptors (had this effect occurred in
vivo). One possible explanation for the decrease in breathing frequency
following a return to room air is a change in the CO2 sensitivity
of lung PSR following CHC. Amphibian PSR are CO2 sensitive and
decrease their firing rate as CO2 levels are increased. Upon the
removal of the inspired 5% CO2, the [CO2] in the lung
gas would probably have decreased rapidly. This would reduce the inhibitory
effects of CO2 on the PSR and increase their rate of afferent
signalling to the brain. In this situation, it is possible that increased
amounts of PSR feedback (probably a tonic component) may have caused the
decrease in breathing frequency immediately following acute hypercapnia. Given
that this decrease did not occur in the control (i.e. not chronically
hypercapnic) group, it is possible that CHC increased the CO2
sensitivity of lung stretch receptors leading to a greater level of discharge
following the removal of CO2 from the lung gas. If tonic PSR
feedback dominated over phasic PSR feedback during this period
(Reid and West, 2004) then
this could have resulted in a reduced breathing frequency. The absence of PSR
feedback in the in vitro preparation is a significant difference from
the in vivo situation. Any effect of PSR feedback on chemosensitivity
following CHC is an area that we plan to actively investigate in the near
future.
Conclusion
This study demonstrates that exposure to chronic hypercapnia increased the
offset of CO2-sensitive fictive breathing in vitro
suggesting that CHC altered central CO2 chemoreceptor function.
This response does not appear to have been caused by CHC-induced changes in
central descending inputs originating from the midbrain. CHC did not augment
the in vivo acute hypercapnic ventilatory response whereas midbrain
transection enhanced the ventilatory response during acute hypercapnia and the
altered breathing pattern. The presence of multiple populations of
respiratory-related CO2-sensitive chemoreceptors in anurans may
explain why the increased CO2 sensitivity observed in
vitro was not manifest in vivo. We are continuing to investigate
the effects of olfactory CO2 chemoreceptors, PSR and arterial
O2/CO2 chemoreceptors on central chemosensitivity.
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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significant difference between the
control and chronically hypercapnic groups. The solid bold line through the
data in A is a first order regression line (control,
r2=0.83; chronic hypercapnia,
r2=0.96). The dotted lines are 95% confidence
intervals.
significant difference before and after transection in either
group.
