Abstract
Energy deprivation, as a result of aglycemia, leads to depression of the central synaptic transmission. Endogenous adenosine has been implicated in this depressant effect. We have studied the possible involvement of endogenous adenosine in the depression of corticostriatal excitatory transmission induced by glucose deprivation by using intracellular recordings in brain slices. After stimulation of corticostriatal fibers, EPSPs were recorded from striatal spiny neurons. Adenosine (3–300 μm) or brief periods (5–10 min) of aglycemia reduced the EPSP amplitude but did not alter the membrane potential and the resistance of the recorded cells. These inhibitory effects were not associated with an alteration of the postsynaptic sensitivity to exogenous glutamate but were coupled with an increased paired-pulse facilitation, suggesting the involvement of presynaptic mechanisms. A delayed postsynaptic membrane depolarization/inward current was detected after 15–20 min of glucose deprivation. The presynaptic inhibitory effects induced by adenosine and aglycemia were both antagonized either by the nonselective adenosine receptor antagonist caffeine (2.5 mm) or by the A1 receptor antagonists 8-cyclopentyl-1,3-dimethylxanthine (CPT, 1 μm) and 1,3-dipropyl-8-cyclopentylxanthine (CPX, 300 nm). Conversely, these antagonists affected neither the delayed membrane depolarization/inward current nor the underlying conductance increase produced by glucose deprivation. The ATP-sensitive potassium channel blockers tolbutamide (1 mm) and glipizide (100 nm) had no effect on the aglycemia-induced decrease of EPSP amplitude. Our data demonstrate that endogenous adenosine acting on A1 receptors mediates the presynaptic inhibition induced by aglycemia at corticostriatal synapses, whereas ATP-dependent potassium channels do not play a significant role in this presynaptic inhibition.
Clinical consequences of glucose deprivation are the suppression of encephalographic activity, rapid loss of consciousness, and irreversible neuronal injury (Auer et al., 1984;Kalimo et al., 1985; Auer and Siesjo, 1988). Depression of excitatory synaptic transmission during aglycemia has been reported in different brain areas (Bachelard et al., 1984; Burke and Nadler, 1989; Crepel et al., 1992; Shoji, 1992). This decrease might be produced by different mechanisms: (1) a reduction in the release of excitatory amino acids from the synaptic terminals, (2) an alteration of postsynaptic glutamate receptors, and (3) an abnormal coupling of postsynaptic receptors with synaptic conductances. Alternatively, a decrease of the electrochemical forces on ions involved in generating synaptic currents also might contribute to the aglycemia-induced depression of excitatory synaptic transmission (Martin et al., 1994).
Experimental evidence suggests that endogenous adenosine might represent a possible pathogenetic factor in the aglycemia-induced depression of synaptic transmission (Martin et al., 1994). Adenosine is released during aglycemia (Butcher et al., 1987), and the activation of adenosine receptors causes a presynaptic inhibitory action on nerve terminals releasing excitatory amino acids in different brain areas (Malenka and Kocsis, 1988; Greene and Haas, 1991; Uchimura and North, 1991; Thompson et al., 1992; Ulrich and Huguenard, 1995). Moreover, extracellular studies have shown that adenosine receptor antagonists reduce the aglycemia-induced depression of field potentials in hippocampal slices (Zhu and Krnjevic, 1993). An alternative mechanism that might account for the aglycemia-induced depression of synaptic transmission is the possible activation of presynaptic ATP-sensitive potassium channels (Ashcroft, 1988; Freedman and Lin, 1996).
We have investigated the possible involvement of adenosine receptors and ATP-sensitive potassium channels in the aglycemia-induced depression of the excitatory transmission at corticostriatal synapses by using intracellular recordings from a brain slice preparation. Moreover, we also have investigated the presynaptic action of exogenous adenosine on striatal neurons to compare this action with the effects produced by glucose deprivation at corticostriatal synapses. Morphological findings have shown that the striatum is highly vulnerable to hypoglycemia (Kalimo et al., 1985). Because pharmacological and biochemical studies suggest that corticostriatal projection is one of the most important glutamatergic pathways in the brain (Reubi and Cuenod, 1979) (for review, see Calabresi et al., 1996), overactivity of this projection might be implicated in the pathogenesis of acute and chronic neurological disorders involving the basal ganglia (Globus et al., 1988; Beal, 1995). Stimulation of corticostriatal fibers produces EPSPs, which are mediated by the release of endogenous excitatory amino acids acting on ionotropic glutamate receptors localized on striatal spiny neurons (Cherubini et al., 1988; Calabresi et al., 1996). Thus, the aglycemia-induced changes of these potentials might provide information concerning the action of energy metabolism failure on the corticostriatal transmission.
MATERIALS AND METHODS
Wistar rats (150–250 gm) were used. The preparation and maintenance of coronal slices have been described previously (Calabresi et al., 1990, 1991, 1995a,b). Briefly, corticostriatal coronal slices (200–300 μm) were prepared from tissue blocks of the brain with the use of a vibratome. A single slice was transferred to a recording chamber and submerged in a continuously flowing Krebs’ solution (35°C, 2–3 ml/min) gassed with 95% O2/5% CO2. To study glucose metabolism in striatal neurons, we deprived slices of glucose by removing glucose totally from the perfusate and by adding saccharose to balance the osmolarity. In some experiments the osmolarity was balanced by increasing the NaCl concentration (Jiang and Haddad, 1992). Because experiments performed by using these different procedures to replace glucose gave similar results, all of the data were pooled together. Aglycemic solutions entered the recording chamber no later than 20 sec after a three-way tap was turned. Complete replacement of the medium in the chamber took ∼90 sec, as detected by the speed of diffusion of a colored solution. The composition of the control solution was (in mm): 126 NaCl, 2.5 KCl, 1.2 MgCl2, 1.2 NaH2PO4, 2.4 CaCl2, 11 glucose, and 25 NaHCO3.
The intracellular recording electrodes were filled with 2 mKCl (30–60 MΩ). An Axoclamp 2A amplifier (Axon Instruments, Foster City, CA) was used for recordings either in current-clamp or in voltage-clamp mode. In single-microelectrode voltage-clamp mode the switching frequency was 3 kHz. The headstage signal was monitored continuously on a separate oscilloscope. Current–voltage relationships and changes in membrane conductance were detected by the application of voltage steps both in positive and negative directions (1–3 sec duration, 5–15 mV amplitude). Traces were displayed on an oscilloscope and stored on a digital system. For synaptic stimulation, bipolar electrodes were used. These stimulating electrodes were located either in the cortical areas close to the recording electrode or in the white matter between the cortex and the striatum to activate corticostriatal fibers. Quantitative data on modifications induced by aglycemia are expressed as a percentage of the controls, the latter representing the mean of responses recorded during a stable period (15–20 min) before the aglycemic phase. Values given in the text and in the figures are mean ± SEM of changes in the respective cell populations. Student’s t test (for paired and unpaired observations) was used to compare the means. Drugs were applied by dissolving them to the desired final concentration in the saline and by switching the perfusion from control saline to drug-containing saline. Glutamate also was applied by ejecting (pressure application; Picospritzer, General Valve, Fairfield, NJ) a few nanoliters of a 10–100 mmsolution from the tip of a blunt pipette beneath the surface of the superfusing solution and just above the tissue slice. 6-Cyano-7-nitroquinoxaline-2,3-dione (CNQX) was obtained from Tocris Cookson (Bristol, UK). Adenosine andd-2-amino-5-phosphonovalerate (d-APV) were obtained from Sigma (St. Louis, MO). Caffeine, CPT, and CPX were purchased from RBI (Natick, MA). Glipizide and tolbutamide were gifts from Dr. N. B. Mercuri (S. Lucia, Rome). CGS 15943 was a gift from Drs. Ongini and Dionisotti (Schering Plough, Milano, Italy).
RESULTS
Properties of the recorded cells
In the present study, data from 110 intracellularly recorded striatal spiny neurons were included. The membrane properties of these neurons previously have been described in vitro (Kita et al., 1984; Calabresi et al., 1987, 1990, 1991, 1995a,b; Kawaguchi et al., 1989; Wilson, 1993; Surmeier et al., 1994). The membrane potential of the recorded cells was −84 ± 5 mV. Input resistance was 39 ± 8 MΩ. All of the recorded cells were silent at rest and showed membrane rectification and tonic firing activity during depolarizing current pulses. Stimulation of the corticostriatal fibers produced an EPSP that was fully blocked by coadministration of 10 μm CNQX plus 30 μm APV (n = 5) (data not shown). These physiological and pharmacological characteristics are in agreement with previous findings indicating that cortically evoked EPSPs are mediated by the release of excitatory amino acids within the striatum (for review, see Calabresi et al., 1996).
Effect of exogenous adenosine on corticostriatal EPSPs
Bath application of adenosine produced a dose-dependent and reversible inhibition of corticostriatal EPSPs (Fig.1A,C,D). This inhibitory action was coupled neither with alterations of intrinsic membrane properties such as resting membrane potential and current–voltage relationship (n = 8; Fig. 1B) nor with changes of the postsynaptic sensitivity to local pressure applications of exogenous glutamate (in control medium: 25 ± 9 mV,n = 5; in 30 μm adenosine: 26 ± 10 mV, n = 5; p > 0.05). As shown in Figure 2, the inhibitory action of adenosine was antagonized by either CPT or by CPX (data not shown), adenosine A1 receptor antagonists. In fact, the adenosine-induced depression of EPSP amplitude (30 μm adenosine = −56 ± 9%) was reduced to −14 ± 5% in 1 μm CPT (n = 4, p < 0.001) and to −12 ± 4% in 300 nm CPX (n = 4, p< 0.001). These concentrations of CPT (Fig. 2) and of CPX (data not shown) not only antagonized the inhibitory action of adenosine, but they also induced a slight but significant increase of the control EPSP amplitude (CPT: +15 ± 4%, n = 8,p < 0.01; CPX: +14 ± 5%, n = 8,p < 0.01). Neither CPT nor CPX affected the intrinsic membrane properties of the five recorded cells (p > 0.05). In fact, the resting membrane potential was −85 ± 6 mV in CPT (n = 8) and −84 ± 5 mV in CPX (n = 8), whereas the input resistance was 38 ± 6 MΩ in CPT (n = 8) and 38 ± 6 MΩ in CPX (n = 8).
Effect of aglycemia on corticostriatal EPSPs
Glucose deprivation produced a progressive decrease of the EPSP amplitude. This inhibitory action mimicked the adenosine-induced depression of corticostriatal transmission. In fact, brief periods of aglycemia (5–10 min) produced a depression of the EPSP amplitude that was not coupled with changes of the membrane potential, current–voltage relationship, and responses to the application of exogenous glutamate (Fig. 3). Longer periods of aglycemia (15–20 min) produced a further decrease of the EPSP amplitude (Figs. 4, 5,filled circles). However, in this case the effect on synaptic transmission was coupled with a progressive membrane depolarization (n = 20; Fig. 5B) or an inward current that was associated with an increased membrane conductance (n = 12; data not shown). Both the early synaptic inhibition and the delayed membrane depolarization induced by glucose deprivation were fully reversible after the washout of the aglycemic solutions.
Adenosine receptor antagonists on aglycemia-induced synaptic depression
To investigate the possible role of endogenous adenosine in the aglycemia-induced decrease of corticostriatal EPSP, we applied the glucose-free medium after the incubation of the slices in the presence of adenosine receptor antagonists. The aglycemia-induced depression of EPSP was reduced by 0.2 mm caffeine (n = 5,p < 0.001), a nonselective adenosine receptor antagonist (Fig. 4), and by the A1 adenosine receptor antagonists CPT (1 μm, n = 7, p < 0.001; Fig. 5) and CPX (300 nm, n = 6,p < 0.001; Fig. 5). CPT (n = 6,p > 0.05) and CPX (n = 7,p > 0.05) altered neither the membrane depolarization/inward current induced by glucose deprivation (Fig.5B) nor the membrane conductance increase coupled with these electrophysiological events (data not shown). We also tested the effects of CGS 15943, a nonxanthine derivative showing both A1 and A2 adenosine receptor antagonist action. This compound, in fact, does not show inhibitory activity on phosphodiesterases (Dionisotti et al., 1994). Incubation of the slices with 1 μm CGS 15943 prevented the inhibitory actions of both exogenous adenosine and aglycemia on the EPSP amplitude. In fact, in the presence of this antagonist the depression of the EPSP amplitude induced by 30 μm adenosine was reduced to −14 ± 5% (n = 3), whereas the depression induced by 10 min of aglycemia was reduced to −10 ± 5% (n = 3). These values were significantly different from those observed in control medium (p < 0.001).
Effect of glucose deprivation and adenosine on paired-pulse facilitation
Paired-pulse modification of neurotransmission has been studied extensively and is attributed to a presynaptic change in release probability (Manabe et al., 1993; Schulz et al., 1994). An increase in the ratio of the second pulse response to the first pulse response (EPSP2/EPSP1) indicates a decrease in the release probability. The decrease in transmitter release probability is consistent with the observations that manipulations depressing transmitter release usually increase the magnitude of this ratio. Therefore, we measured the magnitude of EPSP2/EPSP1 before, during, and after the application of glucose-free medium and of adenosine. Synaptic responses to a pair of stimuli were recorded with interstimulus interval of 60 msec. As shown in Figure 6, the application of glucose-free medium reversibly increased the magnitude of EPSP2/EPSP1 in all of the neurons tested (n = 7, p < 0.001). This effect also was mimicked by exogenous adenosine (n = 6,p < 0.001; Fig. 6).
Blockers of ATP-dependent potassium channels on aglycemia-induced synaptic depression
Because it has been postulated that ATP-dependent potassium channels might play a role in the decrease of excitatory transmission during energy deprivation (Ashcroft, 1988; Martin et al., 1994;Freedman and Lin, 1996), we have studied whether the incubation of the slice in the presence of the ATP-dependent potassium channel blockers tolbutamide and glipizide could affect the aglycemia-induced depression of corticostriatal transmission. Tolbutamide (1 mm,n = 5, p > 0.05) and glipizide (100 nm, n = 5, p > 0.05) failed to alter the inhibitory action of glucose deprivation (Fig.7). Moreover, these antagonists did not modify the intrinsic membrane properties of the recorded cells and the EPSP amplitude measured under control conditions.
DISCUSSION
Main findings
The present study demonstrates that adenosine as well as brief periods (5–10 min) of glucose deprivation exert a prominent presynaptic inhibitory action at corticostriatal synapses. In fact, in both of these conditions the reduction of the EPSP amplitude was associated neither with alterations of postsynaptic intrinsic membrane properties of the recorded neurons nor with changes of the postsynaptic sensitivity to exogenous glutamate. A presynaptic site of action for both adenosine and aglycemia is suggested also by the increase in paired-pulse facilitation. A presynaptic inhibitory action of adenosine on corticostriatal transmission has been postulated previously (Malenka and Kocsis, 1988; Lovinger and Choi, 1995). Accordingly, our intracellular experiments clearly demonstrate that this presynaptic inhibition is not coupled with significant changes of the postsynaptic properties that we measured. Moreover, we have shown that endogenous adenosine plays a major role in the aglycemia-induced presynaptic inhibition of glutamate release at corticostriatal synapses. In fact, this depressant effect was greatly reduced either by caffeine, a nonselective adenosine receptor antagonist, or by CPT and CPX, adenosine A1 receptor antagonists. Accordingly, the presence of adenosine A1 receptors located on corticostriatal terminals has been postulated previously (Alexander and Reddington, 1989). Interestingly, we also found that adenosine A1 receptor antagonists produced, per se, a slight but significant increase of EPSP amplitude, suggesting that endogenous adenosine does influence corticostriatal transmission not only during energy deprivation but also in physiological conditions. Conversely, tolbutamide and glipizide, blockers of ATP-dependent potassium channels, did not affect the presynaptic inhibitory action of aglycemia, suggesting that these channels might play a role in the modulation of the postsynaptic responses to energy deprivation, but they are not involved in the control of glutamate release in the striatum during aglycemia. The latter observation is in line with data obtained in other brain areas showing that blockers of ATP-dependent potassium channels do not influence the synaptic changes induced by glucose deprivation (Shoji, 1992; Zhu and Krnjevic, 1993).
Comparison with other studies
Adenosine blocks excitatory synaptic transmission by suppressing transmitter release in several brain areas (Siggins and Schubert, 1981;Proctor and Dunwiddie, 1987; Greene and Haas, 1991; Scholz and Miller, 1991; Lupica et al., 1992; Prince and Stevens, 1992; Thompson et al., 1992). This presynaptic inhibitory action, however, usually is associated with postsynaptic changes such as membrane hyperpolarization and increased conductance (Siggins and Schubert, 1981; Proctor and Dunwiddie, 1987; Greene and Haas, 1991; Pape, 1992; Thompson et al., 1992). Interestingly, also in the nucleus accumbens, a brain area that shares a similar cytological organization with the dorsal striatum, adenosine-induced blockade of excitatory synaptic transmission is coupled with a membrane hyperpolarization and an increased conductance (Uchimura and North, 1991). Thus, our finding that adenosine exerts a selective presynaptic action on spiny neurons recorded from dorsal striatum suggests that in these cells adenosine exerts a particular modulatory function by affecting presynaptic mechanisms in the absence of postsynaptic changes.
The electrophysiological effects reported in various brain regions after aglycemia strongly resemble the changes observed in the presence of exogenous adenosine. In fact, during glucose deprivation both inhibition of excitatory transmission and membrane hyperpolarization have been reported in hippocampus (Bachelard et al., 1984; Spuler et al., 1988; Burke and Nadler, 1989; Knopfel et al., 1990; Crepel et al., 1992) and in the dorsolateral septal nucleus (Shoji, 1992). We found that brief periods (5–10 min) of aglycemia, as well as exogenous adenosine, selectively cause presynaptic inhibition in the striatum. Longer periods of aglycemia (15–30 min) were required to induce postsynaptic changes. We recently have characterized these postsynaptic changes in two neuronal striatal subtypes (Calabresi et al., 1997b). Prolonged aglycemia (15–30 min) depolarizes spiny neurons while it hyperpolarizes large aspiny interneurons; both of these membrane potential changes are mediated by postsynaptic mechanisms. Interestingly, adenosine A1 receptor antagonists reduced the aglycemia-induced presynaptic inhibitory effect (present study), but they did not antagonize the postsynaptic changes observed in these two striatal subpopulations during glucose deprivation (Calabresi et al., 1997b). Accordingly, it has been reported that A1 receptor antagonism can delay the hypoxia-induced depression of synaptically evoked excitatory potentials in hippocampal slices (Fowler, 1989;Katchman and Hershkowitz, 1993; Khazipov et al., 1995). However, if energy deprivation is continued, synaptic depression still occurs in the presence of adenosine antagonists, albeit after a longer delay and at a slower rate (Gribkoff et al., 1990). Thus, we have to conclude that, during sustained energy metabolism failure, other mechanisms, independent of endogenous adenosine, contribute to the depression of excitatory synaptic transmission.
Possible mechanisms underlying presynaptic inhibition and functional implications
Adenosine blocks voltage-dependent calcium channels (Dolphin et al., 1986; Scholz and Miller, 1991; Mogul et al., 1993) and inhibits presynaptic calcium fluxes (Wu and Saggau, 1994). Thus, it is likely that the major mechanism underlying the aglycemia-induced EPSP inhibition is represented by the blockade of presynaptic calcium channels via the activation of adenosine A1 receptors. Alternatively, endogenous adenosine may act presynaptically to inhibit release at a point downstream from the calcium channels rather than or in addition to inhibiting the calcium channel function. It is also possible that adenosine activates presynaptic potassium channels and attenuates evoked neurotransmitter release by hyperpolarizing the presynaptic membrane.
Xanthine-like compounds might interact with phosphodiesterases. However, two findings indicate that the pharmacological effects of CPT and CPX in our experiments are not dependent on the modulation of phosphodiesterases. First, we recently have assayed the possible inhibitory activity of CPX on cGMP and cAMP phosphodiesterase in corticostriatal extracts. In fact, using the method described byThompson and Appleman (1971) on corticostriatal extracts, we have found that 300 nm CPX gave very little inhibitory effect on phosphodiesterase activity: 3.2 ± 0.2% (n = 4) on cAMP phosphodiesterase activity and 2.7 ± 0.02% (n = 4) on cGMP phosphodiesterase activity (P. Calabresi and M. Giorgi, unpublished observation). Second, the antagonistic effects of CPX and CPT on the adenosine and aglycemia-induced reduction of the EPSP amplitude are mimicked by the nonxanthine adenosine receptor antagonist CGS 15943.
Extracellular levels of adenosine can increase after a high metabolic demand, including hypoglycemia, hypoxia, and seizure activity (Snyder, 1985; Geiger and Nagy, 1990; Greene and Haas, 1991). This increase is attributable, most likely, to net breakdown of intracellular ATP to ADP and AMP. Adenosine, derived from intracellular AMP, is released from the cell by a nucleoside transporter (Martin et al., 1994). Adenosine also may be derived from extracellular AMP, because 5′-ectonucleotidase can metabolize the AMP to adenosine extracellularly.
It has been shown recently that coactivation of metabotropic and β-adrenoreceptors on glia in area CA1 of hippocampus induces a large synergistic increase in cAMP accumulation, which provides the source for the formation of extracellular adenosine. This transmitter, in turn, activates presynaptic A1 adenosine receptors located on the terminals of Schaffer collateral and reduces the release of glutamate from these fibers (Winder et al., 1996). Thus, it is possible that glial elements play a role in the formation of endogenous adenosine during aglycemia in the corticostriatal system.
A cytoprotective role of adenosine and adenosine analogs has been demonstrated in experimentally induced cerebral ischemia (Ramkumar et al., 1995). Several mechanisms have been postulated to mediate this neuroprotection: interaction with antioxidant enzymes, activation of potassium channels, inhibition of calcium influx, and inhibition of neurotransmitters such as glutamate (for review, see Ramkumar et al., 1995). Our study suggests that the latter mechanism might play a role in the pathophysiology of corticostriatal transmission during metabolic stress. By using in vivo microdialysis in the freely moving rat, researchers recently have reported an accumulation of extracellular adenosine in the hippocampus and in the striatum during lights-off periods (Huston et al., 1996). These authors have suggested that this transmitter plays a possible role in the regulation of sleep and in some motor and nonmotor behavioral activities related to these brain areas (Huston et al., 1996). Thus, the adenosine-mediated depression of corticostriatal transmission during aglycemia might account for some of the behavioral changes observed after acute glucose deprivation.
Footnotes
This study was supported partially by grants from Consiglio Nazionale delle Ricerche (P.C.), from the Italian Ministry of Health (Progetto Finalizzeto, Ospedale Santa Lucia) (P.C.), and by Progetto Nazionale Ricerche/Neurobiologia (G.B.). We thank G. Gattoni and M. Tolu for their technical assistance. We thank Dr. M. Giorgi (L’Aquila University) for the experiments on phosphodiesterase activity. We also thank Drs. E. Ongini and S. Dionisotti (Schering Plough, Milano, Italy) for helpful discussions.
Correspondence should be addressed to Dr. Paolo Calabresi, Clinica Neurologica, Dipartimento Sanitá, Universitá di Roma Tor Vergata, Via O. Raimondo 8, 00173 Rome, Italy.