Differential Processing of Excitation by GABAergic Gain Modulation in Canine Caudal Ventral Respiratory Group Neurons

doi:10.1152/jn.00761.2002

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Differential Processing of Excitation by GABAergic Gain Modulation in Canine Caudal Ventral Respiratory Group Neurons

V. Tonkovic-Capin,¹^,² A. G. Stucke,¹^,² E. A. Stuth,¹^,² M. Tonkovic-Capin,¹^,² F. A. Hopp,¹^,² D. R. McCrimmon,³ and E. J. Zuperku¹^,²

¹Zablocki Veterans Affairs Medical Center, Milwaukee, Wisconsin 53295; ²Department of Anesthesiology, Medical College of Wisconsin, Milwaukee, Wisconsin 53226; and ³Department of Physiology and Institute for Neuroscience, Northwestern University Medical School, Chicago, Illinois 60611

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Tonkovic-Capin, V., A. G. Stucke, E. A. Stuth, M. Tonkovic-Capin, F. A. Hopp, D. R. McCrimmon, and E. J. Zuperku. Differential Processing of Excitation by GABAergic Gain Modulation in Canine Caudal Ventral Respiratory Group Neurons. J. Neurophysiol. 89: 862-870, 2003. The discharge frequency (F_n) patterns of medullary respiratory premotor neurons are subject to potent tonic GABAergic gainmodulation. Studies in other neuron types suggest that the synapticinput for tonic inhibition is located on the soma where it canaffect total neuronal output. However, our preliminary data suggestedthat excitatory responses elicited by highly local applicationof glutamate receptor agonists are not gain modulated. In addition,modulation of the amplitude of spike afterhyperpolarizations cangain modulate neuronal output, and this mechanism is located nearthe spike initiation zone and/or soma. The purpose of this studywas to determine if these two gain-modulating mechanisms havedifferent functional locations on the somatodendritic membraneof bulbospinal inspiratory and expiratory neurons. Four-barrelmicropipettes were used for extracellular single-neuron recordingand pressure ejection of drugs in decerebrate, paralyzed, ventilateddogs. The net increases in F_n due to repeated short-duration picoejectionsof the glutamate receptor agonist, $alpha$ -amino-3-hydroxy-5-methylisoxazole-4-propionicacid (AMPA), was quantified before and during locally inducedantagonism of GABA_A receptors by bicuculline or small-conductance,calcium-activated potassium channels by apamin. The AMPA-inducednet increases in F_n were not significantly altered by BIC, althoughit produced large increases in the respiratory-related activity.However, the AMPA-induced net responses were amplified in accordancewith the gain increase of the respiratory-related activity byapamin. These findings suggest that GABAergic gain modulationmay be functionally isolated from the soma/spike initiation zone,e.g., located on a dendritic shaft. This could allow other behavioralsignals requiring strong neuronal activation (e.g., coughing,sneezing, vomiting) to utilize the same neuron without being attenuatedby the GABAergicmodulation.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The discharge patterns of respiratory neurons of the caudal ventral respiratory group (cVRG) are subject to potent GABAergicgain modulation. Local application of the competitive GABA_A receptorantagonist bicuculline (BIC) (MacDonald and Olsen 1994) amplifiesthe underlying discharge frequency (F_n) patterns that are mediatedby endogenous excitatory and inhibitory synaptic inputs (Dogaset al. 1998; McCrimmon et al. 1997). These results imply a tonicGABAergic mechanism that constrains the baseline F_n and reflexlyinduced activities of these bulbospinal respiratory premotor neuronsto ~35-50% of their discharge rate in the absence of this inhibitoryinput.

The functional location of this form of inhibition on respiratory neurons is not known. On other types of neurons, such asmost principal cortical cells and granule cells of the hippocampaldentate gyrus, synaptic inputs arising from distinct groups ofinhibitory neurons innervate segregated regions of the targetneuron such as the axon initial segment, soma, and various partsof the dendrites (Soltesz et al. 1995). Such spatial segregationof the inputs from GABAergic neurons suggests the possibilitythat distinct inhibitory inputs may play different functionalroles (Nicoll 1994). In other neurons, such as hippocampal granulecells, it has been shown that tonic inhibition is due to GABAergicterminals located near the soma, where it is likely to play animportant role in regulating the input-output relations of theneurons (Soltesz et al. 1995). Due to the characteristics of GABAergicgain modulation of respiratory neurons (Dogas et al. 1998; McCrimmonet al. 1997), it is possible that this gain modulation takes placenear the soma and/or spike initiation zone. Alternatively, thesite of modulation could be on the dendrites. This more distallocation is consistent with our preliminary data in which thelocalized application of glutamate receptor agonists, presumablyto the somal region, are not gain modulated while the spontaneousneuronal activity is modulated (Tonkovic-Capin et al. 2001a).

In addition to GABAergic input, an additional mechanism of gain modulation of respiratory neuronal activity is produced bychanges in the size of the medium-spike afterhyperpolarizations(AHPs). These AHPs are produced by increases in the conductanceof small-conductance, calcium-activated potassium channels (SKchannels). Block of the SK channels with the highly selectiveantagonist apamin abolishes AHPs and increases discharge frequency(F_n) (Viana et al. 1993). Local application of apamin to respiratoryneurons produces an increase in their F_n patterns that is proportionalto the underlying pattern (i. e., gain modulation). In a previousstudy, we have shown that GABAergic gain modulation and SK-channel-mediatedgain modulation act in a cascade fashion (Tonkovic-Capin et al.2001b), where the total modulation is the product of the two stagesof attenuation. Because AHPs are the direct result of Ca²⁺ entry during the action potential, the AHP mechanism is likelyto be located near or at the spike initiation zone. This is inthe final output pathway of the neuron and should affect all formsof excitation whether endogenously or exogenouslyinduced.

The purpose of the present study was to determine if, or to what extent, the GABAergic gain mechanism modulates the excitatoryresponses elicited by activation of excitatory receptors on thesoma of respiratory neurons in vivo. Modulation might be expectedif the GABAergic input is functionally located near the soma and/orspike initiation zone. On the other hand, it was expected thatblock of the AHPs with apamin would modulate both exogenouslyas well as endogenously induced activities. Accordingly, the effectson the net increases in F_n produced by repeated short-durationpicoejections (for 2 respiratory cycles) of the glutamate receptoragonist, $alpha$ -amino-3-hydroxy-5-methylisoxazole-4-propionic acid(AMPA), were quantified before and during locally induced antagonismof GABA_A receptors by BIC or SK channels by apamin. The resultsfrom these protocols showed that the average AMPA-induced increasesin F_n were not significantly altered by BIC but were amplifiedby apamin in accordance with the gain increase of the respiratory-relatedactivity. These findings suggest that the mechanism for GABAergicgain modulation may be functionally isolated from soma/spike initiationzone, e.g., located on a dendritictrunk.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

This research was approved by the Subcommittee on Animals Studies of the Zablocki VA Medical Center in accordance with provisionsof the Animal Welfare Act, the National Institutes of Health Guidefor the Care and Use of Laboratory Animals, and VA policy. Datawere obtained from 15 mongrel dogs of either sex weighing from8 to 15 kg. Mask induction with a volatile anesthetic (isofluraneor halothane) was used, and anesthesia was maintained during thesurgical procedure with isoflurane (1.4-2.0% end-tidal concentration).Airway concentrations of isoflurane, CO₂, and O₂ were continuouslymonitored with an infrared analyzer (POET II, Criticare Systems,Waukesha, WI). The animals were monitored for signs of inadequateanesthesia (e.g., salivation, lacrimation, and/or increases inblood pressure and heart rate), and if required, the depth ofanesthesia was increasedimmediately.

Surgical procedure

Dogs were intubated with a cuffed endotracheal tube and mechanically ventilated with an air-O₂-isoflurane mixture. The surgicalprocedures, monitoring, and maintenance of body homeostasis havebeen previously described in detail elsewhere (Dogas et al. 1998).Briefly, after cannulating the femoral artery (for blood pressurerecording and blood-gas sampling) and vein (for continuous infusionof maintenance fluids and drugs), a bilateral pneumothorax wasperformed to reduce motion artifacts. A bilateral vagotomy wasperformed to remove the ventilator-induced effects of pulmonarymechanoreceptors on the breathing pattern. The animal was thendecerebrated (Tonkovic-Capin et al. 1998). This procedure leadsto an anatomically well-defined, midcollicular decerebration.After completion of the decerebration, isoflurane was discontinued,and the dogs were ventilated with an air-O₂ mixture and maintainedin hyperoxic normocapnia (PO₂>400 mmHg, PCO₂ 35-45 mmHg). Thedorsal surface of the medulla oblongata was exposed by an occipitalcraniotomy.

Phrenic nerve activity was recorded from the central end of the desheathed right C₅ rootlet. The phrenic neurogram (PNG) wasobtained from the moving-time average (100 ms) of the amplifiedphrenic nerve activity and was used to produce timing pulses correspondingto the beginning and end of the inspiratory phase. The neuromuscularblocker pancuronium (0.1 mg/kg, followed by 0.1 mg · kg¹ · h¹) was then given to reduce motion artifacts during neuronal recordings.Four-barrel micropipettes, (10-30 µm composite tip diameter),consisting of one recording barrel containing a carbon filamentand three drug barrels, were used for extracellular neuronal recordingsand pressure ejection of nanoliter/picomol amounts of drug solutions.BIC (200 µM; Sigma), apamin (0.125-0.150 µM; Alomone Labs), and $alpha$ -amino-3-hydroxy-5-methylisoxazole-4-propionic acid (AMPA, 7and 20 µM; Sigma) were dissolved in an artificial cerebrospinalfluid (ACSF) vehicle that also served as a control solution. Dueto the potent effect of 20 µM AMPA observed in the first two experiments(8 neurons) we reduced the AMPA concentration to 7 µM (last 20neurons). Further details of the picoejection technique and itslimitations have been previously described (Dogas et al. 1998;Krolo et al. 1999; Stuth et al. 1999). Unit activities from cVRGinspiratory (I) and expiratory (E) neurons were recorded froma region extending 2-4 mm caudal and 2-4.5 mm lateral from theobex and 2-4.5 mm below the dorsal medullary surface. >88% ofthe respiratory-related neurons within this region have been shownto be bulbospinal premotor neurons (Bajic et al. 1992; Stuth etal. 1994).

Protocols

After decerebration and discontinuation of the anesthetic, a period of $>=$ 1 h was allowed for washout of isoflurane (airwayconcentration <0.05%) and for stabilization of the neural breathingpattern. On establishing a stable recording of single-unit activity,repeated automatic short-duration picoejections (for 2 respiratorycycles) of the glutamate receptor agonist AMPA were made beforeand after picoejection of BIC (protocol 1) and apamin (protocol2). Short-duration picoejections of AMPA were set to occur every7-14 respiratory cycles and triggered at the onset of I phase(for E neurons) or E phase (for I neurons) of the respiratorycycle. Volume-ejection rate was measured as a change in meniscusheight/time with a ×100 microscope equipped with a reticule. Thedose rate (i.e., volume-rate) of AMPA was constant throughouteach neuron study. Dose rates during the two respiratory cycleperiod were determined before and after picoejection of BIC orapamin. The total volume ejected divided by the sum of the two-cycledurations was used to determine the AMPA ejection rates. Picoejectionsof antagonists (i.e., BIC and apamin) were done in dose ratesthat were known to produce a near maximal increase in F_n (Tonkovic-Capinet al. 2001b). Picoejections of ACSF were routinely used to verifythat the ACSF constituents and/or ejected volumes were withouteffect.

In Protocol 1, the average net increases in F_n of I and E cVRG neurons produced by the short-duration picoejection of AMPAwere quantified before and during locally induced antagonism ofGABA_A receptors by BIC. Protocol 2 was similar to protocol 1,but instead of inducing antagonism of GABA_A receptors, we usedapamin to block SKchannels.

Data analysis

Cycle-triggered histograms (CTHs; bin width: 50 ms), triggered from either the onset of the E or I phase and based on 5-19respiratory cycles were used to quantify the discharge frequencypatterns before and during picoejection of AMPA. The values ofF_n for each bin were calculated as the number of spikes per bin/binduration in seconds. For each time increment (bin) within thetriggered cycle, these values were averaged over the number ofcycles used to generate the CTH. In addition, the SD and SE ofeach bin were calculated. Because plots of CTHs ± SDs indicatedthat the size of the bin SDs appeared to be uniform throughoutthe active phase of the respiratory cycle, the bin SDs were averagedover the active phase of each CTH. These values served as an indexof F_n variability and for calculations of the coefficient of variationfor peak F_n. The highest mean bin value was used as an estimateof peak F_n.

Drug-induced changes in the gain and offset of the discharge frequency pattern were analyzed via plots of the F_n(drug) versusF_n(control) values obtained from the CTHs. This method has theadvantage of being insensitive to the geometric shape of the pattern.It can detect the amount by which a pattern is shifted up or down,i.e., the amount of parallel shift or offset (y intercept) andthe amount by which a pattern is amplified, i.e., the change ingain (slope), regardless of pattern trajectory. The net increasein F_n produced by AMPA was time-averaged over the neuron's activephase, and these values were computed for the period before andthe period during locally induced antagonism of GABA_A receptorsby BIC or SK channels by apamin. The time-average values duringthe antagonist effect were then normalized relative to their controlvalues, which were assigned a value of 100%. These values wereseparately collected for each neuron and pooled according to neurontype (I or E neurons) and according to protocol (BIC and apamin).In addition, for each protocol, gain factors were determined foreither BIC or apamin from respiratory cycles without AMPA-inducedexcitation, i.e., the gains of the endogenously induced activitywere determined. These gain factors were then multiplied by thecorresponding AMPA-induced net responses during the control periodto estimate the expected increases in the net response, if infact such responses were subject to gain modulation. Normalizedvalues of the average AMPA-induced net increase during the controlperiod, during the period of enhanced activity in response toBIC or apamin (termed BIC or apamin effect), and correspondingpredicted gain-modulated values were compared with each otherwith one-way, repeated-measures ANOVA procedures. Differenceswere considered significant for P < 0.05, using the false discoveryrate procedure for multiple comparisons (Curran-Everett 2000).Values are expressed as means ±SE.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Protocol 1: effect of bicuculline on AMPA-induced responses

Complete protocols with BIC were obtained for seven I and seven E neurons. Figure 1 shows a typical example of the responsesof a cVRG I neuron to repeated short-duration picoejections ofAMPA before and during the BIC-induced effect. The effect of AMPAwas usually visible almost immediately from the onset of picoejection,and full recovery usually required 10-20 s. As can be seen, AMPAproduced about the same net increase in F_n before and during theBIC effect. CTHs were used to quantify the magnitude of the AMPA-inducedresponses. Data for the control CTHs were taken from the respiratorycycles immediately preceding each of the seven AMPA picoejectionsin the pre-BIC period (e.g., Fig. 1, bottom, control). Data forthe CTHs of the AMPA-induced effect were taken from the secondcycle during AMPA picoejections (Fig. 1, bottom, AMPA). Data duringthe BIC-induced effects were obtained using a similar procedure.For this example, the shaded areas between the CTHs of Fig. 2quantify the net AMPA-induced responses. Plots of the differencebetween CTHs ( $Delta$ F_n, Fig. 2, bottom) indicate that the AMPA-inducedresponses are relatively constant throughout the I phase and thatBIC had little affect on the responses. The time-averaged netincreases in F_n (shown as horizontal lines through differenceCTHs) were $approx$ 49 and $approx$ 55 Hz for pre- and post-BIC periods, respectively.AMPA also increased activity during the normally silent phaseboth before and after BIC, but this activity was not constantbecause the subthreshold drive varies with time. This activitywas not analyzed because the subthreshold drive level cannot bemeasured with extracellular recordings. The constant nature ofthe AMPA-induced response during the neuron's active phase isalso confirmed by the plot of F_n(AMPA) versus F_n(control) wherethe slope is nearly one (i.e., 1.02, Fig. 2, top right). The averageBIC-induced gain increase for the endogenously mediated activity,obtained from the F_n(BIC) versus F_n(control) plot (Fig. 2, middleright) was 1.96. If the AMPA-induced response had been gain modulated,the expected response magnitude would have been 1.96 × 49 $approx$ 96 Hzrather than the observed 55 Hz.

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Fig. 1. AMPA-Induced responses of a caudal ventral respiratory group (cVRG) inspiratory neuron pre- and postbicuculline picoejection. Repeated (every 12 respiratory cycles) short-duration (2 respiratory cycles) picoejections of AMPA produced similar net increases ( $approx$ 50 Hz) in F_n before and during the bicuculline (BIC) effect. Thick arrow: time-expanded view of the phrenic neurogram (PNG), picoejection marker (PEM), neuronal activity (NA), and neuronal discharge frequency (F_n) during the short-duration picoejection of AMPA. Net effects were determined from the difference of the 2nd cycle (AMPA) after the start of picoejection and the cycle labeled control. Dashed horizontal lines: reference line through the peak F_n of the control cycles as an aid to visualizing the net AMPA-induced response.

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Fig. 2. Cycle-triggered histograms (CTHs) of unit activity of the inspiratory (I) neuron of Fig. 1. Top left: pre-BIC period: AMPA increased F_n by $approx$ 49 Hz throughout the I phase of the control period as seen by the parallel shift in the CTH (shaded area). This is confirmed by the lack of change in the slope of the plot of F_n(AMPA) vs. F_n(control) (top right; slope: 1.02). - - -, line of identity. Middle, left: BIC postejection period. Picoejection of BIC produced a gain modulated increase in the F_n (thick line CTH). The plot of F_n(BIC) vs. F_n(control) estimated the gain of the endogenously mediated activity to be 1.96 with an offset of -27.5 (Middle right, lower plot). Picoejection of AMPA again produced a parallel shift in the F_n pattern during the BIC effect (shaded). CTHs of the differences ( $Delta$ F_n, bottom) show that over the time period indicated (vertical dashed lines) the average net increases in F_n are similar for the pre- and post-BIC periods, i.e., the AMPA-induced response is not gain modulated ( $approx$ 49 vs. $approx$ 55 Hz; thin and thick lines through difference CTHs, respectively). 7 cycles/CTH.

Pooled data for bicuculline-induced gain modulation

The average AMPA-induced increase in F_n obtained from seven I neurons during the BIC response was 96.0 ± 5.2% of control,indicating that BIC had no effect on the net neuronal responseto AMPA (bar "a," Fig. 3, top, bicuculline). The average predictedAMPA-induced response, based on gain factors obtained from theeffects of BIC on endogenous activity, was significantly largerthan the actually observed responses during the BIC effect (172.6± 18.5%, bar "p," Fig. 3 top, bicuculline).

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Fig. 3. Summary data of the effects of bicuculline or apamin on the net AMPA-induced responses of cVRG I and E neurons. Data are presented as net responses normalized to their respective control levels before application of either bicuculline or apamin ( $Delta$ F_n). Data are from 7 I and 7 E neurons. Bars labeled "a": actual net responses; Bars labeled "p": predicted net responses. Predicted responses were obtained from the product of the control period AMPA response and the gain factor obtained from plots of F_n(BIC or apamin) vs. F_n(control). Top: I neurons. The net responses during the effects of bicuculline (a bar, bicuculline) were not significantly different from control (100%, dashed horizontal line) but significantly less than their respective predicted responses (p bar, bicuculline). The net response during apamin was significantly greater than control (a bar, apamin) and no different from their respective predicted responses (bar p, apamin). Net responses during apamin were significantly greater than those during bicuculline (a bars). Similar results were found for the net AMPA-induced responses of E neurons (bottom). P values for comparisons with control responses: ##, P < 0.01 and ###, P < 0.001. P values for comparisons indicated by brackets: *, P < 0.05, **, P < 0.01, ***, P < 0.001. See text for further explanation.

Similar results were obtained for the pooled data from 7 E neurons (Fig. 3, bottom, bicuculline). The average AMPA-inducedresponse of 112.6 ± 5.9% during the BIC-induced effect was notdifferent from control and was significantly less than the predictedgain modulated response of 144.2 ± 4.3%.

Protocol 2: effect of apamin on AMPA-induced responses.

Complete protocols with apamin were obtained for seven I and seven E neurons. Figure 4 shows a typical example of the responsesof a cVRG I neuron to repeated short-duration picoejections ofAMPA before and during the apamin-induced effect. The net AMPA-inducedresponses during the apamin effect are significantly larger thanthe responses during the control period. AMPA produced a parallelupward shift in the F_n patterns [shaded area between CTHs, Fig.5, left, and slope of 1.00 for F_n(AMPA) vs. F_n(control) plot,Fig. 5, top right]. The CTH analysis of this data shows that thetime-averaged AMPA-induced response increased from $approx$ 39 Hz to $approx$ 72Hz post apamin picoejection, an 84.6% increase ( $Delta$ F_n, horizontallines, Fig. 5, bottom left). This increase is commensurate withthe 91% increase in the gain of the endogenous activity producedby apamin [1.91, slope of F_n(apamin) vs. F_n(control) plot, Fig.5, middle right].

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Fig. 4. AMPA-induced responses of a cVRG inspiratory neuron, pre- and postapamin picoejection. Repeated (every 11 respiratory cycles), short-duration (2 respiratory cycles) picoejections of AMPA produced larger net increases in F_n during the apamin block of Ca²⁺-activated K⁺ channels. Thick arrow: time-expanded view of PNG, PEM, NA, and F_n before and during picoejection of AMPA. Net effects were determined from the difference of the 2nd cycle (AMPA) after the start of picoejection and the cycle labeled control. Dashed horizontal line: reference line through the peak F_n of the control cycles as an aid to visualizing the net AMPA-induced response.

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Fig. 5. Cycle-triggered histograms (CTHs) of unit activity of the I neuron of Fig. 4. Top left: preapamin period; AMPA increased F_n by $approx$ 39 Hz throughout the I phase of the control period as seen by the parallel shift in the CTH (shaded). This parallel shift is verified by the slope of 1.00 in the plot of F_n(AMPA) vs. F_n(control) (top right). Dashed line: line of identity. Middle, left: picoejection of apamin produced a gain modulated increase in F_n that is most noticeable near the end of the I phase (thick line CTH). The plot of F_n(apamin) vs. F_n(control) estimated the gain to be 1.91 with an offset of -65.9 (middle right). Picoejection of AMPA now produced a large parallel shift in F_n (shaded CTH). CTHs of the differences ( $Delta$ F_n, bottom left) show that the average net increase in F_n over the time period indicated (vertical dashed lines) is much greater during the apamin effect than that of the preapamin period, i.e., the response is amplified by $approx$ 1.8 (i.e., $approx$ 72 vs. $approx$ 39 Hz; thick and thin lines through difference CTHs, respectively). 7-10 cycles/CTH.

Pooled data for apamin-induced gain modulation

The average AMPA-induced response of 161.7 ± 8.4% of control, obtained from seven I neurons during the apamin-induced effect,was not significantly different from the predicted response of146.6 ± 7.8%, based on gain factors obtained from the effectsof apamin on endogenous activity (Fig. 3, top right,apamin).

Similar results were obtained for the pooled data from seven E neurons. The average AMPA-induced response of 151.9 ± 13.6%during the apamin-induced effect was significantly different fromcontrol, and not significantly different from the predicted responseof 152.3 ± 9.6% (Fig. 3, bottom,apamin).

Comparison of bicuculline and apamin effects

Even though the gain increases in endogenous neuronal activity produced by BIC and apamin were similar in magnitude (58.1± 10.0 and 47.1 ± 6.4%, respectively, n = 14 each), the effectson the AMPA-induced responses were markedly different for BICand apamin. This differential effect is illustrated by the netAMPA-induced responses for two cVRG E neurons in Fig. 6. The nettime-averaged responses pre- and post-BIC application were essentiallythe same, 22.6 and 20.5 Hz, respectively (shaded regions, Fig.6A). In contrast, the net time-averaged response postapamin of29.3 Hz was markedly larger ( $approx$ 45%) than the time-averaged controlresponse of 20.4 Hz (shaded regions, Fig. 6B). The pooled AMPA-inducedresponse data for BIC and apamin are contrasted in Fig. 3 ("a"bars, bicuculline vs. apamin).

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Fig. 6. Examples of the effects of bicuculline and apamin on the AMPA-induced responses of 2 cVRG E neurons. A: CTHs of activity from an E neuron with an augmenting discharge frequency pattern. 5-12 cycles/CTH. Picoejection of AMPA produced an upward parallel shift in the pattern (top, shaded area: net response). Bicuculline increased the augmenting slope of the CTH (BIC, thick line, bottom). However, the net AMPA-induced response (shaded region) is very similar to the pre-BIC net response. B: CTHs of activity from an E neuron with a decrementing discharge frequency pattern. 6-9 cycles/CTH. The shaded area (preapamin) shows the control net AMPA-induced response. Apamin increased the decrementing slope of the CTH (apamin, thick line, bottom). Note that the net AMPA-induced response (shaded area, postapamin) is significantly greater that the control AMPA response.

Consistency of the transient AMPA-induced responses

The average AMPA-induced increase in activity was 43.2 ± 2.1 Hz (n = 28). The average AMPA picoejection rates prior to andafter the BIC or apamin application were not significantly different,0.144 ± 0.015 and 0.146 ± 0.016 pmol/min, respectively. To evaluatethe consistency of the responses to the transient picoejectionsof AMPA both during the control period and during the effectsof BIC and apamin, the time-averaged bin SD of each CTH was calculated.For the control cycles immediately preceding the AMPA picoejection,the SD serves as an index of the cycle-to-cycle variation of thespontaneous activity. The SD for the cycles with increased activitydue to AMPA reflects the variation of the spontaneous activityplus the variation in the net AMPA-induced responses. From thepooled data of 28 neurons, the average SD value for the AMPA excitedcycles (14.7 ± 0.7 Hz) was greater than that of control cycles(11.6 ± 0.5 Hz, P < 0.0001) prior to the local application ofBIC or apamin. The average difference of 3.1 Hz represents a 27.0± 3% increase in SD for the AMPA excited cycles. Similar datafor the period after BIC or apamin showed that the increase inSD for the AMPA excited cycles of 30.0 ± 4% was not significantlydifferent from that prior to BIC orapamin.

To appreciate the magnitude of the cycle-to-cycle variations, coefficients of variation (COV: 100*SD/peak F_n) were also compared.Prior to any picoejections, the average baseline peak F_n valuefor the I neurons of 93.2 ± 13.1 Hz was not significantly differentfrom the average baseline peak F_n value of 74.1 ± 6.2 Hz for theE neurons. In addition, the average COV values for I and E neuronswere not significantly different, and pooled COV values are given.Prior to BIC or apamin application, the COV of cycles with AMPA-inducedexcitation (11.8 ± 0.6%) was less than the COV for the controlcycles (15.6 ± 1.2%). Thus even though the SD increased with AMPA,the peak F_n increased relativelymore.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The major finding of this study is that the AMPA-induced increases in I and E neuronal activities were not gain modulatedby BIC but were gain modulated by apamin. This differential effectoccurred even though BIC and apamin produced similar increasesin the gain of the baseline endogenous activities (58.1 ± 10.0and 47.1 ± 6.4%,respectively).

AMPA-induced response variability

To determine the presence or absence of gain modulating effects on the AMPA-induced responses, it is necessary that thesetransient submaximal AMPA responses can be consistently reproduced.One important contributing factor is that of consistent dose ratesduring each response both before and after the application ofBIC or apamin. Comparison of the measured picoejected volumesof AMPA showed that there were no significant differences (<2%)in dose rates before and during the effects of BIC or apamin.Other factors contributing to the variability of the responsesmay include time-dependent alterations in the diffusion path andnatural variation in the neuronal response to AMPA. By repeatingthe AMPA picoejections several times (5-19) before and duringthe responses to BIC or apamin, the variability of the responsesof each neuron could be estimated. The finding, that the averageSD of the AMPA stimulated cycles (14.7 Hz) was greater than theaveraged SD of the control cycles (11.6 Hz), indicates that theadditional variation was due to the variation of the net AMPAresponse. That is, the variability of the AMPA stimulated cyclesis made up of two components: one due to the variability of thecontrol cycles and the other due to the variability of the netAMPA-induced response. Using the principle that the variance ofthe sum of two random variables is equal to the sum of each variance,the SD of the net response was found to be 9.0 Hz. This is 22%less than the SD of the control cycles and indicates that theAMPA-induced net responses were highly reproducible using thepicoejection protocol of this study. Every neuron tested respondedconsistently to the AMPA picoejections. The effect of desensitizationwas not observed (e.g., Figs. 1 and 4). This may be due to therapidity of AMPA receptor desensitization (1 ms < time constant< 5 ms), and what was observed may have been the postdesensitizationsteady-state response (Dingledine et al. 1999). Alternatively,our AMPA stimuli may have been brief enough and/or less intenseso as not to produce long-lasting changes in neuronal excitabilityas reported for NTS neurons in vitro (Zhou et al. 1997).

Differential effects

The finding that BIC did not modulate the AMPA-induced responses, whereas apamin did, is in agreement with our previous study,which demonstrated that bicuculline methochloride does not blockSK channels via a nonspecific mode of action in vivo (Tonkovic-Capinet al. 2001b). The fact that apamin gain modulated both the baselineendogenously mediated and AMPA-induced neuronal activities bythe same degree is consistent with the assumption that the locationof the mechanism for the AHP is in the final common neuronal outputpathway (i.e., spike initiation zone), where all inputs are expectedto be similarly affected. The fact that apamin modulated the AMPA-inducedresponse, but BIC did not, suggests that the picoejected AMPAmay be acting at receptors located near the soma and/or spikeinitiation zone. Also, due to the rate limitation of the diffusionprocess, the rapidity of the onset and recovery of AMPA-inducedresponses suggests receptor locations near the recording electrode,which presumably is located near the soma where the extracellularaction potentials are largest. At greater distances from the electrodetip, responses would be expected to be more delayed, blunted,and prolonged. Furthermore, because of the steep diffusion-dependentconcentration gradient, the brisk responses to low pipette concentrationsof AMPA (e.g., 7 µM) suggest receptor locations near the electrodetip. It is also likely that AMPA receptors are located distalto the soma, but they are unlikely to have been stimulated bythe low pipette concentrations used (Krolo et al. 1999).

The finding that the AMPA-induced responses were not modulated by antagonism of the BIC-sensitive GABA_A receptors suggeststhat the GABA receptors are located distal to both the spike initiationzone/soma and the activated AMPA receptors. Our previous studiessuggest that this location is relatively close to the micropipettetip because the BIC-induced responses also have rapid onset times.A possible location would be on a major dendritic trunk, wherethe GABAergic mechanism may gain modulate the various more distalrespiratory-related dendritic inputs to the sameextent.

The data from this study and our previous studies (McCrimmon et al. 1997) do not rule out the possibility of GABAergic presynapticinhibition, which could also produce F_n patterns that are proportionalto the underlying baseline patterns. However, our evaluation ofthe various characteristics of GABAergic gain modulation suggestsa postsynaptic site. This suggestion is based on the observationthat the spontaneous phasic F_n patterns and their modificationby reflexly induced excitatory and inhibitory inputs appear tobe all modulated by the same gain factor. Although this phenomenoncould be explained by presynaptic inhibition, it would requirethat each of the excitatory and inhibitory synaptic inputs thatproduce the F_n pattern would have a corresponding presynapticgain modulating input of equivalent strength. As previously mentioned,the onset effects of BIC are relatively rapid suggesting antagonismof GABA_A receptors relatively close to the soma of these neuronsthat have large dendritic systems (Bianchi et al. 1995).

Other evidence for differential receptor distribution

While our data suggest functionally different locations for the GABAergic and AHP-mediated gain modulation mechanisms, thereis additional pharmacological evidence consistent with this interpretation.Champagnat et al. (1982) suggested that fast inhibitory postsynapticpotentials (IPSPs) mediated by GABA_A and glycine receptors arespatially segregated in brain stem respiratory neurons. In inspiratoryneurons, glycine-sensitive IPSPs are preferentially located onthe soma and are responsible for rapid inhibition at the beginningof expiration. In contrast, GABA_A-mediated IPSPs are primarilylocated on distal dendrites and serve to maintain synaptic inhibitionthroughout the expiratory phase. Additional evidence from anatomicallybased studies corroborates a physical separation of the receptorsresponsible for these mechanisms. Using combined immunohistochemistryand retrograde labeling in adult rats, Robinson and Ellenberger(1997) found that bulbospinal VRG neurons and phrenic motoneuronsshowed positive immunolabeling for N-methyl-D-aspartate (NMDA),AMPA, and kainate receptor subunits. Furthermore, there was aunique distribution for each receptor subtype along the neuronalmembrane. Immunoreactivity for AMPA receptor subunits was distributedthroughout the somata and proximal dendrites; NMDA receptor subunitimmunolabeling was localized to the soma, while kainate subunitimmunolabeling was confined mainly to dendrites. If a similardistribution of glutamate receptors exists for canine respiratoryneurons, it would suggest that the AMPA responses of the currentstudy were due to receptors located on or near the soma. Similarimmunolabeling studies for GABAergic synaptic inputs and GABA_Areceptor subunits on respiratory neurons have yet to beperformed.

However, there is evidence for a differential distribution of GABA inputs and receptors from studies of nonrespiratory neurons.For example, granule cells of the hippocampal dentate gyrus receiveinhibitory inputs from a least five types of GABAergic neurons(Halasy and Somogyi 1993; Han et al. 1993). These interneuronsmainly terminate on mutually exclusive domains along the longitudinalaxis of granule cells. Chandelier cells form axo-axonic contactsexclusively with the initial segment of the axon, whereas basketcells make contact with the somata and proximal dendrites. Varioustypes of hilar cells innervate the different levels of the granulecell's dendritic system. In addition, the dendritic trees of theseGABAergic interneuron types can occupy nonoverlapping domains(Soltesz et al. 1995). This strict spatial segregation of theinputs and outputs of these GABAergic neurons suggests that theymay play different functional roles (Nicoll 1994). In view ofthese observations, it is possible that the GABA_A receptors responsiblefor gain modulation are strategically located on dendritic shaftsand/or trunks that are sufficiently close to the soma to affectthe respiratory related synaptic inputs, but distal enough soas not to affect the responses to exogenously appliedAMPA.

Hypothetical model for gain control of respiratory neurons

Based on our current and past studies, we propose the following hypothetical model to aid in summarizing and explaining thefindings of this study (Fig. 7). The working hypothesis is thatboth excitatory glutamatergic and inhibitory GABA_A and glycinergicrespiratory-related tonic and phasic synaptic inputs are locatedon dendrites. Together these inputs generate the dendritic currentI_DEN. As I_DEN flows toward the soma, it is subjected to an attenuationthat is controlled by a BIC-sensitive tonic GABAergic input. Thisattenuation may be mediated by shunting inhibition (Koch et al.1983; Vu and Krasne 1992). This mechanism is assumed to be strategicallylocated on a dendritic trunk because BIC produces a dischargepattern that is an amplified replica of the underlying spontaneousas well as reflexly induced discharge patterns (McCrimmon et al.1997). It is also electrically isolated from the soma/spike initiationzone to prevent interactions that could alter the magnitude ofthe other inputs and/or AHPs. This latter assumption is supportedby the fact that the AMPA-induced responses were unaffected byBIC.

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Fig. 7. Hypothetical model for gain control of respiratory neurons. Scheme to aid the explanation of the current and past observations regarding GABAergic gain modulation and the role of the afterhyperpolarizations. See text for details.

A proportional, but attenuated I^*_DEN is supplied to the soma, where it is combined with other inputs (e.g.,behavioral). The latter may or may not be gain modulated. We assumethat the excitatory current responsible for the AMPA-induced responseis also an input to the soma. Together these input currents makeup the somatic current I_SOMA that provides the input to the spikegenerating process. The discharge frequency of the neuron (F_n)is assumed to be proportional to I_SOMA. However, this proportionalityconstant is highly dependent on the magnitude of the AHPs thatare mediated by small conductance Ca²⁺-activated K⁺ (SK) channels. Thus neuromodulatory inputs or drugs such as apamin,which can affect or block SK channels, alter the overall excitabilityof the neuron and result in gain modulation of F_n. Because thismechanism is located in the final common output pathway of theneuron, all inputs, including those exogenously induced, are subjectto its effect. The SK channels may also play a fundamental rolein limiting the discharge frequency of the neuron and protectthe neuron from the deleterious effects of continuous high ratesof activity (Vergara et al. 1998).

Summary

The results of this study suggest that gain modulation of the discharge frequency of respiratory neurons can be mediated bytwo distinctly different mechanisms that operate in a cascademanner, at least on endogenously mediated respiratory-relatedactivity. The functional isolation of the GABAergic mechanismfrom the SK channel mechanism suggests that the processing ofinputs to respiratory neurons may be more complex than frequentlythought of in that processing may take place in multiple neuronalcompartments rather than in a single somatic compartment. Distributiveprocessing of neuronal signals could provide a possible mechanismfor the reconfiguration of neuronal activities during, for example,coughing (Shannon et al. 1998) or for gating different centralpattern generators to premotor neurons as might occur during thetransitions from breathing to vomiting (Fukuda and Koga 1997).GABAergic gain modulation may also provide a means for adaptivecontrol, optimizing the respiratory neuronal discharge frequencypatterns for changes in conditions or states (e.g., sleep-wakecycles).

	ACKNOWLEDGMENTS

The authors are indebted to J. Tomlinson for expert surgicalassistance.

This work was supported by the Department of Veterans Affairs Medical Research Funds, the National Institute of General MedicalSciences Grant GM-59234-01 to E. A. Stuth and the Department ofAnesthesiology of the Medical College of Wisconsin,Milwaukee.

	FOOTNOTES

Address for reprint requests: E. J. Zuperku, Research Service/151, Zablocki VA Medical Center, Milwaukee, WI 53295 (E-mail:ezuperku{at}mcw.edu).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

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Differential Processing of Excitation by GABAergic Gain Modulation in Canine Caudal Ventral Respiratory Group Neurons

0022-3077/03 $5.00 Copyright © 2003 The American Physiological Society