Metabolic and cardiorespiratory responses to hypoxia in fetal sheep: adenosine receptor blockade

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Metabolic and cardiorespiratory responses to hypoxia in fetal sheep: adenosine receptor blockade

Andrew Chau and Brian J. Koos

Department of Obstetrics and Gynecology, Nicholas S. Assali Perinatal Research Laboratory, and School of Medicine, The Brain Research Institute, University of California, Los Angeles, California 90095-1740

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

8-Phenyltheophylline (PT), a potent and specific inhibitor of adenosine receptors, was infused intra-arterially into unanesthetizedfetal sheep to determine the role of adenosine in hypoxic inhibitionof fetal breathing. PT in normoxic fetuses increased heart rateand the incidence of low-voltage electrocortical activity, rapideye movements (REM), and breathing. Mean breath amplitude increasedby 44%. Hypoxia (preductal arterial PO₂ = 14 Torr) induceda metabolic acidemia, a transient bradycardia, and hypertensionwhile virtually eliminating REM and breathing. PT administrationduring hypoxia enhanced the metabolic acidemia, blocked the bradycardiaand hypertension, increased the incidence of REM and breathing,and elevated mean breath amplitude. The results indicate that1) adenosine is involved in fetal glycolytic and cardiovascularresponses to hypoxia, 2) activation of central adenosine receptorsmediates about one-half the inhibitory effects of hypoxia on REMand breathing, and 3) the depression of breathing may criticallydepend on a hypoxia-induced reduction in phasic REMsleep.

heart rate; blood pressure; brain; breathing; eye movements; sleep; thalamus

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

ADENOSINE (ADO) concentrations in fetal plasma are about four times greater than maternal levels (35) because of lower fetalarterial PO₂ (Pa_O₂) (28) and possibly placental releaseof the purine nucleoside (35). Because ADO is a vasodilatorin most tissues, these increased levels of ADO are likely involvedin vasoregulation of the brain (21), heart (21), ductus arteriosus(28), and the umbilical circulation (32, 34). Hypoxia (Pa_O₂~ 13 Torr) increases fetal plasma ADO concentrations by abouttwofold (21), and these elevated ADO levels mediate severalfetal responses to acute O₂ deficiency, including bradycardiaand hypertension, through effects on the autonomic nervous system(18, 20). ADO also contributes to hypoxia-induced metabolicacidemia (20) and to the release of arginine vasopressin (23)and atrial natriuretic peptide (30).

Fetal administration of ADO (25) and ADO analogs (4, 36, 37) inhibits fetal breathing. Because hypoxia increasesfetal brain ADO concentrations (24), ADO may be involved inthe central mechanism that triggers hypoxic inhibition of breathing.Theophylline, a comparatively weak ADO receptor antagonist, bluntsthe inhibitory effects of hypoxia on fetal breathing (3, 25),providing further evidence that ADO contributes to hypoxic inhibition.However, these latter findings must be interpreted with caution,because the respiratory effects of theophylline may have beencaused by other actions of the drug, such as inhibition ofphosphodiesterase.

We recently reported that 8-(p-sulfophenyl)-theophylline (SPT), a highly specific ADO receptor antagonist, failed to reversethe inhibitory effects of hypoxia on fetal breathing (20). Thisinability of SPT to blunt hypoxic inhibition may have resultedfrom the lack of involvement of ADO receptors in hypoxic inhibitionor the reduced antagonism of central ADO receptors caused by adecreased ability of this polar drug to penetrate the fetal brain.This study was designed to determine whether a potent and specificADO receptor inhibitor with greater access to the fetal brainwould abolish the inhibitory effects of hypoxia on fetal breathing.The results indicate that central ADO receptor activation accountsfor about one-half, but not all, of the inhibitory effects ofhypoxia on fetalbreathing.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Eleven pregnant ewes (Rambouillet-Columbia cross) were operated on at ~120 days gestation (~0.8 term). Under halothane anesthesia,polyvinyl catheters (1.0 mm ID) were placed in the right brachiocephalictrunk, external jugular vein, and carotid artery of the fetusand in the amniotic sac (27). Bipolar stainless steel electrodes(Cooner Wire, Chatsworth, CA) were sutured to the medial and lateralcanthus of an eye to record eye movements and on the parietaldura to record electrocortical activity (27). The fetus andewe were allowed to recover from surgery for $>=$ 4 days before experimentswerebegun.

Fetal pressures were measured with pressure transducers (Cobe Laboratories, Lakewood, CO), and heart rate was determined bya cardiotachometer triggered by the arterial pressure pulse. Fetalarterial and tracheal pressures (minus amniotic fluid pressure),heart rate, electrooculogram (EOG), and electrocorticogram (ECoG)were displayed on a chart recorder (Grass Instruments, Quincy,MA). Heart rate and arterial and tracheal pressures were sampledat 100 Hz by microcomputer, and minute averages of fetal heartrate, mean arterial pressure, and breathing measurements (numberof breaths, inspiratory time, breath interval, and breath amplitude)were stored on disk (8). Blood gases and pH were measured usingblood gas electrodes (model 1304, Instrumentation Laboratories),with values corrected to fetal temperature (39.5°C).

Three types of cell surface receptors mediate the physiological effects of ADO: A₁, A₂, and A₃, with A₂ subdivided into A_2a(high-affinity) and A_2b (low-affinity) subtypes. 8-Phenyltheophylline(PT) has high affinity for the A_2b receptor, with intermediateaffinity for A₁ and A_2a receptors; PT does not bind to the A₃receptor (12). PT has greater affinity for the A₁ and A₂ receptorsthan SPT (12). PT is $>=$ 10 times more potent as an ADO receptorantagonist than theophylline, with virtually no phosphodiesteraseactivity (12). PT was dissolved in a minimum volume of a polyethyleneglycol-0.1 N NaCl (50:50 vol/vol) solution and diluted with salineto 20 ml. PT was infused into the right brachiocephalic arteryat 1.7 mg · min¹ · kg¹ for 3 min, then at 0.25 mg · min¹ · kg¹ for 1 h. The dose of PT was calculated by the amount of theophyllinerequired to block fetal ADO receptors (25), with the ~10-foldgreater affinity of PT for ADO receptors taken into account. Thefollowing studies were performed in varied order on separate daysto minimize carryovereffects.

Normoxia. PT was administered to nine chronically catheterized fetuses to determine the effects of ADO receptor blockade on breathingactivity in the basal state. In separate experiments the vehiclefor PT was infused into the right brachiocephalic artery for 1h to control for possible vehicle effects on thefetus.

ADO. ADO was infused (14 mg · min¹ · kg¹) into the right external jugular vein of nine fetuses for 1 h to demonstrate the inhibitoryeffects of ADO on fetal breathing (25). In other experiments,PT was infused into the right brachiocephalic artery for 1 h whileADO was administered intravenously. These studies determined whetherthe PT dose was sufficient to block the inhibitory effects ofADO on fetal breathing. Infusions of the vehicle (saline) forADO were not performed, because previous work has shown that slowinfusions of saline do not significantly affect fetal heart rate,mean arterial pressure, or breathing activity (25).

Hypoxia. Fetal hypoxia was induced for 1 h in nine fetuses by having the ewe breathe a hypoxic gas mixture (9% O₂-3% CO₂-88% N₂) froma plastic bag (27). Hypoxia was initiated within 5 min of thestart of a breathing episode; these experiments demonstrated theinhibitory effects of hypoxia on fetal breathing. Fetal hypoxiawas also induced while PT was infused to determine whether PTwould blunt the inhibitory effects of hypoxia on fetalbreathing.

Data analysis. Fetal breathing was easily distinguished from characteristic negative deflections (>1 mmHg) in tracheal pressure. Inspiratorytime, breath interval, and mean breath amplitude were determinedfrom the digitized tracheal pressure recordings with use of dataacquisition software (8). These breathing variables were calculatedfrom respiratory efforts having a breath interval $<=$ 3 s and thusexcluded isolated breaths or gasps (9).

The incidence of breathing was used as a measure of respiratory activity because of the episodic nature of fetal respiratoryactivity. Incidence was determined as the number of breaths perminute from computer analysis and the number of minutes per hourof breathing from visual inspection of the chart recordings. Inthe latter analysis, breathing was considered to be present ifit occurred during $>=$ 20 s of each 1-min epoch (25).

In near-term (>0.8 term) fetal sheep the ECoG is clearly differentiated into episodes of high- and low-voltage electrocorticalstates, which are associated with fetal breathing (9). Rapid,irregular respiratory activity and rapid eye movements (REM) coincidewith low-voltage electrocortical states (LV ECoG), but these movementsdo not occur during high-voltage states (HV ECoG). In these experimentsthe incidence of REM, LV ECoG, and HV ECoG was determined fromvisual analysis of the chart recordings, as previously described(18). Breathing, REM, LV ECoG, and HV ECoG were determined tobe present if the activity occurred during $>=$ 20 s of each 1-minepoch (25).

Statistical analysis. Two-hour control measurements for ECoG, REM, and breathing were averaged for comparison with the respective measurements duringexperimental manipulations. Statistical significance was determinedusing repeated-measures ANOVA with post hoc comparison by Tukey'sleast significant difference criterion. Single comparisons betweencontrol and experimental measurements were performed using Student'st-test. A logarithmic transformation of the data was carried outbefore analysis when it normalized a skewed distribution. Differenceswere significant at P < 0.05. Values are means ±SE.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Normoxia. During the control period, Pa_O₂ (23.2 ± 0.8 Torr), arterial PCO₂ (Pa_CO₂, 49.9 ± 0.7 Torr), and pH (7.337 ± 0.008)in nine fetuses were within the normal range; after 30 min ofPT infusion the fetal Pa_O₂ decreased slightly (P < 0.05) to 20.9± 0.9 Torr and returned to control values within 60 min. Pa_CO₂and pH were not significantlyaffected.

Fetal mean heart rate, 159 ± 5.7 beats/min during the control period, increased by ~18 beats/min during the last 30 min ofPT infusion; mean arterial pressure (44.3 ± 2.7 mmHg in control)was not significantlychanged.

PT increased the incidence of LV ECoG by ~33% (Fig. 1) and reduced the incidence of HV ECoG from 21.4 ± 1.0 to 14.9 ± 8.0min/h. PT administration was also associated with an ~26% increasein the incidence of REM (Fig. 1).

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Fig. 1. A-C: effects of 8-phenyltheophylline (PT, shaded vertical bar) on incidence (min/h) of low-voltage electrocortical activity (LV ECoG), rapid eye movements, and breathing averaged in 9 fetuses. D: breathing incidence (breaths/h). PT (dashed line) and vehicle (solid line) were infused in separate experiments. * P < 0.05 compared with time 0. $dagger$ P < 0.05 compared with vehicle.

PT stimulated breathing as indicated by a 75% increase in breathing incidence, a nearly twofold rise in the number of breathsper hour (Fig. 1), and a 44% increase in mean breath amplitude(control, 2.5 ± 0.2 mmHg; PT, 3.6 ± 0.4 mmHg; P < 0.05). Inspiratorytime (0.54 ± 0.02 s) and breath interval (1.43 ± 0.12 s) werenot significantlyaffected.

In control experiments the vehicle for PT was infused over 1 h in nine fetuses. Fetal arterial blood gases (Pa_O₂ = 22.2 ±1.0 Torr, Pa_CO₂ = 50.7 ± 1.2 Torr) and pH (7.316 ± 0.010) werenot significantly affected, nor was heart rate or mean arterialpressure. The incidence of LV ECoG, HV ECoG, REM, and breathingactivity was not affected; other respiratory measurements (meanbreath amplitude, inspiratory time, and breath interval) alsowere not significantlyaltered.

ADO. ADO administration to nine fetuses was associated with a significant reduction in arterial pH for measurements 30 (7.305 ±0.007) and 60 (7.297 ± 0.004) min after the onset of infusioncompared with the control of 7.336 ± 0.005. Fetal Pa_O₂ (23.9 ±1.5 Torr) and Pa_CO₂ (49.5 ± 0.8 Torr) were not significantly affectedby ADO. Fetal mean heart rate increased by ~30 beats/min duringthe last 30 min of ADO infusion, but mean arterial pressure wasnot significantlyaffected.

ADO significantly reduced the incidence of LV ECoG (Fig. 2) while increasing the incidence of HV ECoG (control, 20 ± 4.0 min/h;ADO, 32 ± 2.4 min/h; P < 0.05) and virtually abolishing REM andbreathing activity (Fig. 2). Breath amplitude (2.5 ± 0.1 mmHg),inspiratory time (0.51 ± 0.04 s), and breath interval (1.45 ±0.12 s) were not significantly changed by ADO.

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Fig. 2. A-C: effects of adenosine (ADO, shaded vertical bar) on incidence (min/h) of LV ECoG, rapid eye movements, and breathing averaged in 9 fetuses. D: breathing activity (breaths/h). Solid line, effects of ADO; dashed line, effects of simultaneous infusion of ADO and PT. * P < 0.05 compared with time 0; $dagger$ P < 0.05 compared with ADO.

PT was infused intra-arterially in nine fetuses receiving simultaneous administration of ADO. Compared with control (7.332± 0.006), the average arterial pH fell significantly to 7.310± 0.008 and 7.304 ± 0.006 at 30 and 60 min, respectively, afterthe onset of infusions. Fetal Pa_O₂ (22.3 ± 1.4 Torr) and Pa_CO₂(50.3 ± 1.3 Torr) were not significantly altered. Fetal heartrate increased by ~25 beats/min during the last 30 min of infusion,while mean arterial pressure was not significantlychanged.

The incidence of LV ECoG, REM, and breathing increased significantly during simultaneous administration of ADO and PT (Fig.2). The incidence of HV ECoG decreased significantly from 21 ±1.3 (control) to 12 ± 2.0 min/h (ADO + PT). These infusions wereassociated with a 44% increase in breathing amplitude (control,2.5 ± 0.1 mmHg; infusions, 3.6 ± 0.3 mmHg), but inspiratory time(control, 0.51 ± 0.03 s; infusions, 0.44 ± 0.05 s) and breathinterval (control, 1.39 ± 0.10 s; infusions, 1.19 ± 0.12 s) wereunaffected.

The overall effects of combined ADO and PT administration on ECoG, EOG, and breathing (Fig. 2) were similar to those observedfor PT infusion alone (Fig. 1). These experiments showed thatPT (0.25 mg · min¹ · kg¹) completely blocked the inhibitory effects of ADO on fetal breathing,indicating that the appropriate dose was used for blocking fetalADO receptors related tobreathing.

Hypoxia. In eight fetuses, preductal Pa_O₂ fell by ~10 Torr during 1 h of hypoxia (Fig. 3). This acute O₂ deprivation was associatedwith a minimal decrease in Pa_CO₂ and a progressive acidemia. Theaverage fetal heart rate fell by ~15% during the first 15 minof hypoxia and increased toward control values during the last30 min of O₂ deficiency (Fig. 4); mean arterial pressure increasedsignificantly by the end of hypoxia, but the incidence of LV ECoG(Fig. 5) or HV ECoG (control, 18 ± 2.1 min/h; hypoxia, 21 ± 1.0min/h) was not significantly affected. Hypoxia reduced the incidenceof REM ~75% and virtually eliminated breathing (Fig. 5). Breathamplitude, inspiratory time, and breath interval were not significantlyaffected.

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Fig. 3. Effects of hypoxia on preductal arterial blood gases and pH averaged in 8 fetuses. Horizontal bar, 1 h of hypoxia with infusion of PT (dashed line) or vehicle (solid line). * P < 0.05 compared with time 0; $dagger$ P < 0.05 compared with vehicle.

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Fig. 4. Efects of PT on fetal heart rate and mean arterial pressure averaged in 7 fetuses. Horizontal bar, 1 h of hypoxia with infusion of PT (dashed line) or vehicle (solid line). * P < 0.05 compared with time 0. $dagger$ P < 0.05 compared with vehicle.

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Fig. 5. A-C: effects of hypoxia (shaded vertical bar) on incidence (min/h) of LV ECoG (5 fetuses), rapid eye movements (6 fetuses), and breathing (8 fetuses). D: breathing activity (breaths/h). PT (dashed line) and vehicle (solid line) were infused during 1 h of hypoxia. * P < 0.05 compared with time 0. $dagger$ P < 0.05 compared with vehicle.

PT was infused into eight fetal sheep in which preductal Pa_O₂ was reduced by ~10 Torr (Fig. 3). Hypoxia was associated witha slight fall in Pa_CO₂ and a decrease in pH after 60 min of O₂deficiency. The fall in pH with PT was significantly greater formeasurements at the end of hypoxia and during the first 10 minof the recovery period during hypoxiaalone.

Hypoxia did not significantly change fetal heart rate, but the average heart rate increased significantly after terminationof PT infusion and restoration of normoxia (Fig. 4). Acute O₂deficiency did not significantly alter mean arterialpressure.

Hypoxia with PT administration was not associated with significant changes in LV ECoG (Fig. 5) or HV ECoG (control, 18 ± 2.2min/h; hypoxia, 19 ± 2.1 min/h) in the five fetuses in which theECoG was recorded. Although REM declined during hypoxia, the incidence(15 ± 3.4 min/h) was about twice that observed during hypoxiaalone (Fig. 5).

PT also blunted the inhibitory effects of hypoxia on fetal breathing (Fig. 5). Breathing incidence during hypoxia with PTwas about five times greater than that during hypoxia alone, aneffect that was also reflected in the number of breaths per hour.This incomplete arrest of hypoxic inhibition was not altered bydoubling the dose of PT, which indicated that the central ADOreceptors related to breathing were completely blocked. Duringhypoxia, PT increased mean breath amplitude (control, 2.3 ± 0.1mmHg; hypoxia, 3.3 ± 0.4 mmHg; P < 0.05) without significantlyaltering inspiratory time or breath interval. The effects of PTon these respiratory variables during hypoxia were similar tothose duringnormoxia.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

ADO receptor blockade with PT prevented ~50% of the hypoxia-induced decline in the incidence of fetal breathing. The bluntingof hypoxic inhibition by PT cannot be accounted for by the greaterdecline in arterial pH in these fetuses, because acidemia at thislevel of hypoxemia has virtually no effect on breathing incidence(5). These results with a highly specific and potent ADO receptorantagonist indicate that ADO is critically involved in hypoxicinhibition of fetal breathing. Because hypoxic inhibition is bluntedby nonpolar PT but not by polar SPT, ADO A₁ or A₂ receptors inthe fetal brain appear to mediate the respiratory depression associatedwith a hypoxia-induced rise in brain ADO concentrations (22,24).

Fetal breathing in sheep (>0.8 term) is associated with REM and LV ECoG states but is inhibited during HV ECoG activity (6,9). Episodes of rapid, irregular breathing during LV ECoG apparentlydepend on the excitatory drive of phasic REM sleep (14, 15,31) rather than changes in arterial blood gases or pH (9).The parallel inhibitory effects of hypoxia on fetal breathingand eye movements (27) suggest that hypoxic inhibition of fetalbreathing is related to reduced REM activity, although it is unknownhow sleep state and hypoxia modulate the hypothesized respiratorypacemaker neurons of the pre-Bötzinger complex (33).

The depressant effects of ADO on fetal breathing also appear to be associated with alterations in behavioral state, and theevidence for this is threefold: 1) ADO suppresses REM and breathingmovements (25), 2) ADO receptor antagonism by PT increases theincidence of REM and breathing, and 3) ADO receptor blockade byPT blunts hypoxic depression of REM and breathing activity. Hypoxia(Pa_O₂ ~ 14 Torr) increases fetal brain ADO concentrations throughextracellular degradation of adenine nucleotides (22); thusa hypoxia-induced rise in brain ADO may be critical to the decreasein phasic REM sleep and breathingactivity.

The increased breath amplitude associated with PT administration may be mediated by blockade of ADO receptors associated withbulbospinal synaptic transmission of inspiratory drive to phrenicmotoneurons (11). However, the ADO receptors that inhibit fetalbreathing are not likely associated with brain stem respiratoryneurons, because fetal breathing is not depressed by hypoxia orADO in fetuses with disruptions of the rostral midbrain (17)or thalamus (19).

We recently showed that the parafascicular nuclear complex (Pf) of the posterior thalamus is crucially involved in hypoxicinhibition of fetal breathing (19). Pf, part of the rostralpole of the "reticular activating system," participates in corticalactivation associated with increased discharge rates in wakefulnessand REM sleep and integrates sensorimotor function (2). ThusPf, or sectors associated with Pf, may contain ADO receptors crucialfor inhibition of breathing andREM.

PT failed to abolish hypoxic inhibition, indicating that other modulators/neurotransmitters contribute to the depression ofREM and breathing activity during acute O₂ deprivation. The relativeimportance of ADO and other factors involved in hypoxic inhibitionprobably depends on the gestational age and the severity of O₂deficiency. Additional mechanisms may include activation of central $alpha$ ₂-adrenergic receptors, which inhibit firing of noradrenergicnerves (1), and a reduction in the synthesis and/or releaseof excitatory amino acids, which contribute to neuronal hyperpolarization(29). Opioids (38), prostaglandins (16), $gamma$ -aminobutyricacid (38), and lactate (13) apparently have little or no rolein hypoxic inhibition of fetalbreathing.

Incomplete blockade of central ADO receptors cannot be totally excluded as a cause of the inability of PT to prevent completelyhypoxic inhibition. However, this possibility seems unlikely,because peripheral administration of lipid-soluble PT has beenshown to block central ADO receptors in adult rats (7) andbecause doubling the dose of PT in our fetal studies had no additionaleffect in attenuating the hypoxic arrest of breathing orREM.

Intravascularly administered ADO stimulates breathing (via the carotid bodies) in adult rabbits, but it depresses ventilationin newborn rabbits through a central mechanism (39). Increasedpermeability of the blood-brain barrier in the neonate to ADOmay underlie this developmental difference, although the exactmechanism remains to be elucidated (39). Thus, as in the neonate,the inhibitory effects of intravascularly infused ADO in the fetusappear to be mediated through a central action of the purine nucleoside.Such a mechanism is supported by observations that SPT, a peripherallyacting ADO receptor antagonist, has minimal effects on the hypoxicarrest of breathing, even though circulating levels of ADO duringhypoxemia increase to levels similar to those for intravascularinfusions of ADO that depress respiratory activity (21).

Although hypoxic inhibition appears to originate within the brain (10, 26), a peripheral contribution may also be involvedin initiating the response. For example, the mean lag time fromthe onset of hypoxia to the cessation of REM and breathing isabout two to three times greater than normal in fetuses with bilateralcarotid denervation and vagal section (26). These results suggestthat peripheral chemoreceptors trigger a more rapid inhibitoryresponse to acute hypoxemia and may represent a component of thehypoxic depression that is not mediated byADO.

Intravascular administration of ADO decreased fetal arterial pH without significantly altering arterial blood gases, suggestingthat activation of ADO receptors modulates lactic acid production.Surprisingly, this ADO-induced fall in pH occurred in the presenceof PT, indicating that the principal ADO receptor involved wasnot blocked by this antagonist. The metabolic effects of ADO,which may be triggered by adrenergic and/or direct effects onglycolysis (20), may be critical to the development of lacticacidemia during fetal O₂ deficiency. This latter possibility issupported by our previous studies in which SPT blunted the hypoxia-inducedfall in fetal arterial pH (20). In contrast, the present studyshowed that PT enhanced the fall in fetal arterial pH during hypoxia.This new finding is probably accounted for by a different distributionof these antagonists within fetal tissues. For example, SPT, apolar blocker, would be expected to have limited access to thefetal brain when administered intravascularly, while the nonpolarantagonist PT would be expected to diffuse freely into brain tissueand block central ADO receptors. The distribution of these ADOreceptor antagonists may also differ in peripheral tissues wherethe polar nature of SPT may limit its access to some receptortypes.

In our previous studies (20), SPT was shown to eliminate the bradycardia and rise in mean arterial pressure normally elicitedby hypoxia in fetal sheep (>0.8 term). These effects of ADO receptorblockade are confirmed by the present study in which PT blockedhypoxia-induced bradycardia and hypertension. Thus a rise in fetalADO concentrations (21) apparently triggers these fetal cardiovascularresponses to acute O₂ deficiency. The similar cardiovascular effectsof PT and SPT suggest that the ADO receptors that modulate autonomiccontrol of the fetal cardiovascular system reside outside theblood-brain barrier in association with the peripheral arterialchemoreceptors, circumventricular organs, or autonomic nerves(18, 20).

In summary, PT significantly enhanced fetal acidemia produced by acute O₂ deficiency, suggesting that ADO promotes fetal glycolyticresponses to hypoxia. The opposing effects of PT and SPT on hypoxia-inducedmetabolic acidemia may be explained by the heterogeneity of ADOreceptors and their accessibility to these ADO receptor antagonists.About 50% of the inhibitory effects of hypoxia on REM and fetalbreathing were abolished by ADO receptor blockade, indicatingthat ADO has a key role in hypoxic inhibition. The parallel effectsof PT in blunting hypoxic depression of REM and breathing areconsistent with the hypothesis that hypoxic inhibition of breathingdepends critically on a reduction in the phasic REM drive torespiration.

	ACKNOWLEDGEMENTS

We thank Leland Patron for technicalassistance.

	FOOTNOTES

This study was supported in part by National Institute of Child Health and Human Development Grant HD-18478.

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: B. J. Koos, 10833 Le Conte Ave., 22-177 CHS, UCLA School of Medicine, Los Angeles, CA 90095-1740 (E-mail: bkoos{at}obgyn.medsch.ucla.edu).

Received 27 May 1998; accepted in final form 10 February 1999.

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