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Department of Physiology, Texas Tech University Health Sciences Center, Lubbock, Texas 79430
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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The present study was designed to investigate the role of adenosine in the hypoxic depression of synaptic transmission in rat hippocampus. An in vivo model of hypoxic synaptic depression was developed in which the common carotid artery was occluded on one side in the urethane-anesthetized rat. Inspired oxygen levels were controlled through a tracheal cannula. Rats were placed in a stereotaxic apparatus for stimulation and recording of bilateral hippocampal field excitatory postsynaptic potentials. The percent inspired oxygen could be reduced to levels that produced a reversible and repeatable depression of evoked synaptic transmission restricted to the hippocampus ipsilateral to the occlusion. Further reduction in the level of inspired oxygen depressed synaptic transmission recorded from both hippocampi. The adenosine nonselective antagonist caffeine and the A1 selective antagonist 8-cyclopentyltheophylline prevented the initial depression in synaptic transmission. We conclude that the initial depression of synaptic transmission observed in the rat hippocampus in vivo is due to endogenous adenosine acting at neuronal adenosine A1 receptors.
hypoxia; ischemia
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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ONE OF THE EARLIEST RESPONSES to cerebral hypoxic and/or ischemic conditions is a reversible inhibition of evoked synaptic potentials. This early inhibition of evoked potentials is primarily due to a suppression of synaptic function (6, 7, 10, 21, 27). There is substantial evidence from in vitro preparations that the initial reversible loss of synaptic activity during exposure to hypoxia or ischemia-like conditions is due to the release of endogenous adenosine acting at neuronal A1 receptors. Hypoxia and ischemia-like conditions increase the efflux of purines, including adenosine, from the rat hippocampal slice (9, 19). Graded hypoxia results in proportionate changes in both adenosine levels and the depression of the evoked potential (8). Adenosine outflow temporally correlates with the hypoxic depression of the evoked potential (18). Finally, adenosine A1-selective antagonists significantly attenuate the early depression of synaptic transmission in hippocampal slices exposed to either hypoxia or ischemia-like conditions (6, 7, 12).
Although a strong case can be made for adenosine's role in hypoxic-ischemic cerebral vascular autoregulation (2, 29, 34), current evidence is more equivocal with regard to adenosine's role in the hypoxic-ischemic inhibition of synaptic transmission in vivo. Presently, there is only indirect evidence suggesting that adenosine modulates hippocampal synaptic transmission during hypoxia-ischemia in vivo. Perhaps the most suggestive evidence of an adenosine-mediated depression of synaptic activity during hypoxia-ischemia in vivo is in its ability to inhibit excitatory amino acid release (4, 13, 33). However, the efflux of excitatory amino acids induced by hypoxia-ischemia can originate from both synaptic and nonsynaptic pools (15). Thus it is not clear whether A1-receptor-mediated inhibition of glutamate release reflects an adenosine A1-receptor-mediated inhibition of synaptic transmission or whether this is an indirect effect of adenosine's other neuroprotective actions.
The purpose of this study was to characterize an in vivo model exhibiting a repeatable and reversible depression of hippocampal synaptic transmission in response to hypoxia. A unilateral carotid occlusion model coupled with systemic hypoxia was found to be appropriate (20). Experiments were designed to examine the role of adenosine in this hypoxic depression of synaptic transmission.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Animal preparation. All surgical and experimental procedures followed institutional animal care guidelines. Male Sprague-Dawley rats, weighing 200-300 g, were anesthetized with urethane (1.5 g/kg ip). The right jugular vein was exposed and catheterized with polyethylene (PE-50) tubing for administration of supplemental anesthesia (typically 10% of initial dose). A tracheostomy was performed, and a cannula was inserted to ensure a patent airway. The distal end of the cannula was inserted into a T-tube to allow for the control of the percent inspired oxygen administered. Inspired air was provided on a flow-by basis through the T-tube. During normoxia, the animals were administered 21-25% O2 to maintain normal blood gas values. During hypoxia, the inspired O2 was between 8 and 12% attained by mixing compressed air with N2. The animals were allowed to breathe spontaneously, and the flow rate of inspired gas was adjusted to ensure removal of expired air without alteration of ventilation. One common carotid artery was exposed and permanently occluded by ligature with Ethicon 4/0 surgical silk. In some animals, the carotid artery was cannulated proximal to the ligature for the purpose of monitoring arterial pressure and obtaining samples for arterial blood gas measurements. Body temperature was monitored by a rectal probe and was maintained between 37 and 38°C using heating pads. Animals were killed while still fully anesthetized by intravenous administration of 2 M KCl.
Electrophysiology.
Animals were placed in a stereotaxic apparatus. A midline incision,
made just posterior to the eye orbits and extending to the interaural
line, was used to expose the skull. Small burr holes (3-4 mm
diameter) were drilled in the skull at each of four sites. Concentric
bipolar stimulating electrodes were placed ~3.0 mm posterior to
bregma, 1.6 mm bilaterally to midline, and 2.7 mm below the cortical
surface. Recording electrodes, pulled from glass micropipettes and
filled with 1 M NaAc, were positioned 5 mm posterior to bregma, 3.2 mm
bilaterally to the midline, and 2.5-3.0 mm below the cortical
surface. The recording electrodes had a 2-5 M
resistance, and
2% Pontamine sky blue was used for position marking.
Hypoxia-ischemia. In experiments where unilateral fEPSP recordings were measured, the permanent carotid occlusion was coupled with a transient, 2-min exposure to moderate hypoxia. With the recording of simultaneous bilateral fEPSPs, the protocol was modified by coupling the vascular occlusion with a level of hypoxia that produced the maximum depression of the fEPSP on the side ipsilateral to the occlusion with little or no effect on the contralateral fEPSP. The hypoxic levels required to achieve this response ranged between 8 and 12% O2, but a 10% O2 hypoxic level was sufficient in most animals. Once the optimum level of hypoxia was established using the above criteria, it was left unchanged for subsequent hypoxic exposures.
Blood gas measurements. Arterial pH, PCO2, and PO2 were measured at 37°C with a Radiometer Copenhagen Blood Microsystem (BMS 3MK2) and a pH/blood gas monitor (pHm73). The electrodes were calibrated before and after each measurement. The pH electrode was calibrated with standard Radiometer buffers with pH values of 7.838 and 6.841 at 37°C. The PCO2 and PO2 electrodes were calibrated with Radiometer-certified calibration gases. The body temperature was measured with a thermistor and maintained at ~37°C with heating pads. Blood samples for hypoxic measurements were drawn during the fEPSP depression. Recovery blood samples were taken 5 min after the end of the hypoxic period. The blood gases were corrected for differences between the animal body temperature and 37°C with the appropriate correction factors for blood.
Cardiovascular parameters. In a separate group of experiments, heart rate (HR), blood pressure, and respiratory rate were recorded under the same experimental conditions; however, in these animals, electrophysiological recordings of the hippocampus were not taken. A lead II electrocardiogram was recorded using stainless steel needles placed subcutaneously as electrodes. The HR was determined from the R-R intervals. Blood pressure was recorded using a Gould P23 transducer, and tracheal airway pressure was monitored continuously using a differential pressure transducer via a small tube inserted into the tracheal cannula. All measurements were recorded using a Grass model 7P polygraph.
Agonist and antagonist application.
8-Cyclopentyltheophylline (8-CPT, 2.5 mg/kg, Sigma, St. Louis, MO) was
dissolved in 2-hydroxypropyl-
-cyclodextrin (45% wt/vol, RBI,
Natick, MA) and injected intraperitoneally. Trials with this solvent
alone did not alter either the normoxic amplitude or the hypoxic
depression of the fEPSP (n = 3). Caffeine (50 mg/kg, Sigma) was dissolved in saline and administered intraperitoneally.
Data analysis. Data were statistically analyzed using either a Student's paired t-test or a one-way ANOVA followed by Student-Neuman-Keuls test for group comparisons. A P value of <0.05 indicated a significant difference.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Evoked synaptic potentials are reversibly inhibited by hypoxia.
When attempts were made to induce a reversible inhibition of
evoked synaptic transmission by coupling an acute common carotid artery
occlusion with graded levels of hypoxia, it proved very difficult to
obtain conditions that produced a consistent and reversible depression
of the hippocampal fEPSP. More consistent responses were
obtained by completing a permanent unilateral common carotid artery
occlusion 1-2 h before exposure to hypoxic conditions. Subsequent
recording and stimulation were performed in a single hippocampus either
ipsilateral or contralateral to the occlusion. Under these conditions,
it became apparent that the evoked potential recorded from the
hippocampus ipsilateral to the carotid occlusion was more sensitive to
the level of imposed hypoxia. A 2-min exposure to 10% O2
consistently resulted in a reversible depression of the evoked
fEPSP when recording from the hippocampus ipsilateral to the
occlusion (Fig. 1). The depression of the
fEPSP averaged 14.4 ± 2.9% of the prehypoxic amplitude
(n = 8). After reintroduction of normoxia, the
amplitude of the fEPSP recovered to 100.8 ± 2.4% of
prehypoxic amplitude within a 5-min recovery period.
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Responses to hypoxia are not affected by the side of stimulation.
The differential sensitivity to hypoxia suggested the benefit of
simultaneously recording from both hippocampi ipsilateral and
contralateral to the side of occlusion. It was observed that stimulation of commissural fibers in the stratum radiatum of either hippocampus resulted in evoked potentials in both hippocampi. Stimulation intensity was adjusted to minimize any contamination of the
fEPSP by population spikes. Under these conditions, the side
of stimulation had no significant effect on the amplitude of the evoked
potential in each hippocampus or in their individual responses to an
hypoxic insult (Fig. 3). The normoxic
fEPSP amplitudes recorded from the hippocampus ipsilateral to
the occlusion measured 6.32 ± 1.5 mV (n = 8) when
the ipsilateral side was stimulated and measured 6.28 ± 2.1 mV
(n = 8) when the contralateral hippocampus was
stimulated. The same consistency in normoxic fEPSP amplitudes was observed for the hippocampus contralateral to the occlusion. Furthermore, the depression in fEPSP amplitude, during a
hypoxic period, was also shown to be independent of the side of
stimulation. As shown in Fig. 3, the fEPSP ipsilateral to the
occlusion was similarly depressed during hypoxia when either the
ipsilateral or contralateral hippocampus was stimulated [compare Fig.
3A (top) with B (top)].
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Hypoxic depression of evoked potentials is proportionate to the
level of hypoxia.
Figure 4 illustrates the proportionate
responses to graded hypoxia and the differential sensitivity of the
ipsilateral and contralateral hippocampus. Various levels of hypoxia
(8, 10, and 12% O2), each 2 min in duration, were given in
one animal. The level of hypoxia could be adjusted to depress solely
the ipsilateral response in a graded manner or could be increased
sufficiently to reversibly depress evoked activity in both hippocampi.
In this animal, the recovery of the fEPSP from the hippocampus
ipsilateral to the occlusion was significantly delayed after 2 min of
8% O2 compared with 2-min exposures to 10 and 12%
O2.
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Adenosine antagonists attenuate the hypoxic depression.
Figure 5 illustrates the ability of
adenosine antagonists to significantly attenuate the hypoxic depression
of the fEPSP. With simultaneous, bilateral recordings, a level
of hypoxia was chosen that produced the greatest depression of the
ipsilateral fEPSP with little or no effect on the
contralateral fEPSP. The drugs used were the nonselective
adenosine antagonist caffeine and the adenosine A1-subtype
receptor selective antagonist 8-CPT. The effect on the hypoxic
depression was examined 20 min after intraperitoneal injection of each
drug. Neither drug altered the normoxic amplitude of the
fEPSP. However, the depression of the evoked potential in
response to a 2-min hypoxic insult was significantly attenuated by the
administration of either drug. Hypoxia alone reduced the fEPSP
to 14.4 ± 2.9% of control (n = 8). Caffeine (50 mg/kg ip) significantly blocked the hypoxic depression so that the
fEPSP declined to 67.4 ± 5.7% of prehypoxic baseline amplitude (n = 7, P < 0.05). In the
presence of 8-CPT (2.5 mg/kg ip), the hypoxic depression was also
attenuated so that the fEPSP was reduced to 81.8 ± 5.8%
of control (n = 8, P < 0.05).
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Attenuation of the hypoxic depression by 8-CPT wanes over time.
Figure 6 illustrates, from a single
animal, that the effect of 8-CPT waned over time so that a return of
the hypoxic depression could be recorded. Two initial hypoxic periods
depressed the fEPSP to ~2% of the baseline amplitude. The
injection of 8-CPT attenuated the hypoxic depression of the
fEPSP to ~75% of the baseline amplitude. The depression in
response to 10% O2 returned to predrug levels 3 h
after the intraperitoneal injection of 8-CPT. In a group of animals,
3 h postdrug, a 2-min hypoxic challenge reduced fEPSP to
18.2 ± 3.1% of baseline amplitude (n = 8, data
not shown). This sensitivity to hypoxia was not significantly different
from the predrug control fEPSP at 14.4 ± 2.9% of
baseline amplitude.
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Attenuation of the hypoxic depression with 8-CPT did not affect
blood acid-base or cardiovascular responses.
In another group of animals (n = 5), it was shown that
although 8-CPT administration was able to prevent the hypoxic
depression of the fEPSP, it did not alter the blood acid-base
responses to hypoxia. Blood gas measurements and electrophysiological
data were simultaneously collected in these animals. Table
1 shows that hypoxia resulted in a
significant decline in PO2 and
PCO2, as well as a significant depression of
the fEPSP amplitude. The administration of 8-CPT did not
significantly alter normoxic blood gas values or normoxic
fEPSP amplitudes. Hypoxia, in the presence of 8-CPT, showed
similar declines in PO2 and
PCO2 despite the significant reduction in the
depression of the fEPSP amplitude.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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We conclude from these studies that the initial hypoxic depression of hippocampal synaptic transmission observed in vivo is mediated by locally released adenosine acting at central A1 receptors. The adenosine antagonists caffeine and 8-CPT attenuated the hypoxic depression of synaptic transmission by 53 and 67%, respectively. Our observations with the selective antagonist 8-CPT are consistent with the numerous demonstrations of the role of the neuronal A1 receptor in inhibition of the in vitro hippocampal synaptic response during hypoxic or hypoxic-hypoglycemic conditions (1, 6, 7, 12, 16, 36).
It is unlikely that activation of other adenosine receptor subtypes directly contributes to the hypoxic depression of synaptic transmission. Activation of the A3 and A2a receptors facilitate synaptic transmission in the hippocampus primarily by negatively modulating A1-mediated inhibition (5, 23). The activation of these receptors would oppose the hypoxic depression we observe. It is unlikely these receptors are substantially activated during the brief hypoxic-ischemic exposures applied in this study as both receptors appear to require an extended duration of activation and/or relatively high concentration of adenosine before antagonizing A1-mediated inhibition (5, 17).
Under ischemia-like conditions, adenosine is released from hippocampus as adenosine rather than converted extracellulary from a nucleotide (22). The source of adenosine seems to be AMP dephosphorylation (19). However, it is difficult to quantitatively correlate adenosine outflow with nucleotide degradation because the adenosine efflux represents only a small fraction of the total nucleotide pool (19).
Adenosine is most likely released locally within the hippocampus. It is unlikely that the released adenosine is of peripheral origin given its half-life of <2 s in blood (28) and its inability to cross the blood-brain barrier (2, 3). Locally active adenosine is consistent with its rapid appearance in cerebral cortex within seconds of the onset of systemic hypoxia (35). There are several possible sources for the local production of adenosine. Adenosine pools exist in neurons, astrocytes, and endothelial cells. The adenosine originating from endothelial cells is unlikely to have access to neuronal receptors because it appears to be confined to the vascular side of the blood-brain barrier (3). However, both astrocytes and neurons exhibit vigorous transport and metabolism of adenosine (14, 25).
The most proximate stimulus for adenosine release seems to be local tissue hypoxia. Brain adenosine levels are sensitive to a number of factors that contribute to the level of tissue oxygenation including cerebral blood flow (CBF), MAP, and arterial PO2 (24, 30, 35). With respect to this model, unilateral carotid occlusion in the absence of hypoxia should have had little effect on CBF, energy state, or cerebral metabolism (32). In this study, applied hypoxia resulted in combined hypotension and hypoxemia. Application of either one of these insults could result in reduced tissue oxygenation and metabolic derangement most prominently on the side ipsilateral to the carotid occlusion, with the hippocampus being one of the more vulnerable regions (11, 26, 32).
Although local tissue hypoxia may be the stimulus for adenosine release, it seems clear that the adenosine antagonists did not blunt the depression of the evoked potential by altering tissue oxygenation. The adenosine A1 receptor selective antagonist 8-CPT blocked the hypoxic depression of synaptic transmission but did not change the hypoxic alterations in MAP, PO2, and PCO2. The persistence of synaptic transmission during hypoxia in the presence of 8-CPT is consistent with the conclusion that the adenosine-mediated inhibition of synaptic transmission is a physiological compensatory response to metabolic stress before compromise of function from energy depletion.
Perspectives
Numerous features of the adenosine-mediated depression of synaptic transmission are consistent with it being a physiological regulatory mechanism balancing energy supply and demand. Particularly appealing is the suppression of synaptic activity before neural function is compromised by energy depletion. Thus this adaptive strategy appears designed to maintain metabolic integrity at the expense of neural function. Possible adenosine-mediated behavioral correlates of this strategy would include fainting and restorative sleep.It is not clear whether adenosinergic modulation functions to provide a continuous and proportionate adjustment of neural activity in response to varying energy supply or whether it acts as a "retaliatory" response to a relatively modest but critical threshold of energy compromise. Although evidence exists for a basal adenosinergic "tone," we did not observe the expected effects of blocking this tone with the administration of antagonists. Under either scenario, it is an open question as to how adenosinergic inhibition of neural activity is integrated with regional autoregulation of CBF. Adenosinergic modulation of neural activity could be coupled to ongoing autoregulation to effectively maintain a balance of energy supply and demand. Or adenosinergic inhibition of synaptic transmission may signal the failure of cerebrovascular autoregulation. Finally, the brain is a somewhat unique organ in that excessive expression of its "function," namely neurotransmitter release, can result in excitotoxic injury. Inhibitory modulation of synaptic function by endogenous adenosine as observed in this study should logically contribute to adenosine's well-known actions as an endogenous neuroprotectant during ischemia.
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ACKNOWLEDGEMENTS |
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This work was supported by a grant from the National Institute of Neurological Disorders and Stroke to J. C. Fowler.
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FOOTNOTES |
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Address for reprint requests and other correspondence: J. C. Fowler, Dept. Physiology, 3601 4th St., Texas Tech Univ. Health Sciences Center, Lubbock, TX 79430 (E-mail: phyjcf{at}ttuhsc.edu).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 19 May 2000; accepted in final form 25 October 2000.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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1.
Arlinghaus, L,
and
Lee KS.
Endogenous adenosine mediates the sustained inhibition of excitatory synaptic transmission during moderate hypoxia.
Brain Res
724:
265-268,
1996[ISI][Medline].
2.
Berne, RM,
Rubio R,
and
Curnish RR.
Release of adenosine from ischemic brain. Effect on cerebral vascular resistance and incorporation into cerebral adenine nucleotides.
Circ Res
35:
262-271,
1974
3.
Coney, AM,
and
Marshal JM.
Role of adenosine and its receptors in the vasodilatation induced in the cerebral cortex of the rat by systemic hypoxia.
J Physiol (Lond)
509:
507-518,
1998
4.
Dolphin, AC,
and
Archer ER.
An adenosine agonist inhibits and a cyclic AMP analogue enhances the release of glutamate but not GABA from slices of rat dentate gyrus.
Neurosci Lett
43:
49-54,
1983[ISI][Medline].
5.
Dunwiddie, TV,
Diao L,
Kim HO,
Jiang J-L,
and
Jacobson KA.
Activation of hippocampal adenosine A3 receptors produces a desensitization of A1 receptor-mediated responses in rat hippocampus.
J Neurosci
17:
607-614,
1997
6.
Fowler, JC.
Adenosine antagonists alter the synaptic response to in vitro ischemia in the rat hippocampus.
Brain Res
509:
331-334,
1990[ISI][Medline].
7.
Fowler, JC.
Adenosine antagonists delay hypoxia-induced depression of neuronal activity in hippocampal brain slice.
Brain Res
490:
378-384,
1989[ISI][Medline].
8.
Fowler, JC.
Changes in extracellular adenosine levels and population spike amplitude during graded hypoxia in the rat hippocampal slice.
Naunyn-Schmiedeberg's Arch Pharmacol
347:
73-78,
1993[ISI][Medline].
9.
Fowler, JC.
Purine release and inhibition of synaptic transmission during hypoxia and hypoglycemia in rat hippocampal slices.
Neurosci Lett
157:
83-86,
1993[ISI][Medline].
10.
Fujiwara, N,
Higashi H,
Shimoji K,
and
Yoshimura M.
Effects of hypoxia on rat hippocampal neurones in vitro.
J Physiol (Lond)
384:
131-151,
1987
11.
Ginsberg, MD.
Heterogeneities of regional cerebral blood flow during hypoxia-ischemia in the rat.
Stroke
7:
132-134,
1976
12.
Gribkoff, VK,
Bauman LA,
and
VanderMaelen CP.
The adenosine antagonist 8-cyclopentyltheophylline reduces the depression of hippocampal neuronal responses during hypoxia.
Brain Res
512:
353-357,
1990[ISI][Medline].
13.
Heron, A,
Lasbennes F,
and
Seylaz J.
Adenosine modulation of amino acid release in rat hippocampus during ischemia and veratridine depolarization.
Brain Res
608:
27-32,
1993[ISI][Medline].
14.
Hertz, L,
and
Matz H.
Inhibition of adenosine deaminase activity reveals an intense active transport of adenosine into neurons in primary cultures.
Neurochem Res
14:
755-760,
1989[ISI][Medline].
15.
Ikeda, M,
Nakazawa T,
Abe K,
Kaneko T,
and
Yamatsu K.
Extracellular accumulation of glutamate in the hippocampus induced by ischemia is not calcium dependent
in vitro and in vivo evidence.
Neurosci Lett
96:
202-206,
1989[ISI][Medline].
16.
Katchman, AN,
and
Hershkowitz N.
Adenosine antagonists prevent hypoxia-induced depression of excitatory but not inhibitory synaptic currents.
Neurosci Lett
159:
123-126,
1993[ISI][Medline].
17.
Latini, S,
Bordoni F,
Corradetti R,
Pepeu G,
and
Pedata F.
Effect of A2A adenosine receptor stimulation and antagonism on synaptic depression induced by in vitro ischaemia in rat hippocampal slices.
Br J Pharmacol
128:
1035-1044,
1999[ISI][Medline].
18.
Latini, S,
Bordoni F,
Corradetti R,
Pepeu G,
and
Pedata F.
Temporal correlation between adenosine outflow and synaptic potential inhibition in rat hippocampal slices during ischemia-like conditions.
Brain Res
794:
325-328,
1998[ISI][Medline].
19.
Latini, S,
Corsi C,
Pedata F,
and
Pepeu G.
The source of brain adenosine outflow during ischemia and electrical stimulation.
Neurochem Int
27:
239-244,
1995[ISI][Medline].
20.
Levine, S.
Anoxic-ischemic encephalopathy in rats.
Am J Pathol
36:
1-17,
1960.
21.
Lipton, P,
and
Whittingham TS.
Reduced ATP concentration as a basis for synaptic transmission failure during hypoxia in the in vitro guinea-pig hippocampus.
J Physiol (Lond)
325:
51-65,
1982
22.
Lloyd, HGE,
Lindstrom K,
and
Fredholm BB.
Intracellular formation and release of adenosine from rat hippocampal slices evoked by electrical stimulation or energy depletion.
Neurochem Int
23:
173-185,
1993[ISI][Medline].
23.
Lopes, LV,
Cunha RA,
and
Ribeiro JA.
Cross talk between A1 and A2A adenosine receptors in the hippocampus and cortex of young adult and old rats.
J Neurophysiol
82:
3196-3203,
1999
24.
Matsumoto, K,
Graf R,
Rosner G,
Shimada N,
and
Heiss W-D.
Flow thresholds for extracellular purine catabolite elevation in cat focal ischemia.
Brain Res
579:
309-314,
1992[ISI][Medline].
25.
Matz, H,
and
Hertz L.
Effects of adenosine deaminase inhibition on active uptake and metabolism of adenosine in astrocytes in primary cultures.
Brain Res
515:
168-172,
1990[ISI][Medline].
26.
Mendelow, AD,
Graham DI,
McCulloch J,
and
Mohamed AA.
The distribution of ischemic damage and cerebral blood flow after unilateral carotid occlusion and hypotension in the rat.
Stroke
14:
704-710,
1984.
27.
Misgeld, U,
and
Frotscher M.
Dependence of the viability of neurons in hippocampal slices on oxygen supply.
Brain Res Bull
8:
95-100,
1982[ISI][Medline].
28.
Moser, GH,
Schrader J,
and
Deussen A.
Turnover of adenosine in plasma of human and dog blood.
Am J Physiol Cell Physiol
256:
C799-C806,
1989
29.
Phillis, JW.
Adenosine in control of the cerebral circulation.
Cerebrovasc Brain Metab Rev
1:
26-54,
1989[Medline].
30.
Rubio, R,
Berne RM,
Bockman EL,
and
Curnish RR.
Relationship between adenosine concentration and oxygen supply in rat brain.
Am J Physiol
228:
1896-1902,
1975.
31.
Rudolphi, KA,
Schubert P,
Parkinson FE,
and
Fredholm BB.
Neuroprotective role of adenosine in cerebral ischaemia.
Trends Pharmacol Sci
13:
439-445,
1992[Medline].
32.
Salford, LG,
Lund S,
Plum F,
and
Siesjo BK.
Graded hypoxia-oligemia in rat brain. I. Biochemical alterations and their implications.
Arch Neurol
29:
227-233,
1973[ISI][Medline].
33.
Simpson, RE,
O'Regan MH,
Perkins LM,
and
Phillis JW.
Excitatory transmitter amino acid release from the ischemic rat cerebral cortex: effects of adenosine receptor agonists and antagonists.
J Neurochem
58:
1683-1690,
1992[ISI][Medline].
34.
Winn, HR,
Morii S,
and
Berne RM.
The role of adenosine in autoregulation of cerebral blood flow.
Ann Biomed Eng
13:
321-328,
1985[ISI][Medline].
35.
Winn, HR,
Rubio R,
and
Berne RM.
Brain adenosine concentration during hypoxia in rats.
Am J Physiol Heart Circ Physiol
241:
H235-H242,
1981.
36.
Zeng, YC,
Domenici MR,
Frank C,
Sagretella S,
and
Scotti de Carolis A.
Effects of adenosinergic drugs on hypoxia-induced electrophysiological changes in rat hippocampal slices.
Life Sci
51:
1073-1082,
1992[ISI][Medline].
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| Visit Other APS Journals Online |
, n = 8) but not contralateral to the
occlusion (
, n = 7). The inspired
oxygen was decreased to 10% to induce the 2-min period of hypoxia. The
field excitatory postsynaptic potential (fEPSP) was recorded
from either the ipsilateral or contralateral hippocampus in each
animal. Recording of the fEPSPs was every 10 s, and the
amplitude of each fEPSP was plotted as percentage of baseline
amplitude. Means are plotted without SE to improve clarity of the
figure. The fEPSP traces a, b, and
c (inset) are representative waveforms for their
respective times (
) recorded from the ipsilateral hippocampus.
