Mitochondrial Control of Acute Glutamate Excitotoxicity in Cultured Cerebellar Granule Cells

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The Journal of Neuroscience, December 15, 1998, 18(24):10277-10286

Mitochondrial Control of Acute Glutamate Excitotoxicity in Cultured Cerebellar Granule Cells
Roger F. Castilho, Oskar Hansson, Manus W. Ward, Samantha L. Budd, and David G. Nicholls
Neurosciences Institute, Department of Pharmacology and Neuroscience, University of Dundee, Dundee DD1 9SY, Scotland, United Kingdom

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Mitochondria within cultured rat cerebellar granule cells have a complex influence on cytoplasmic free Ca²⁺ ([Ca²⁺]_c) responses to glutamate. A decreased initial [Ca²⁺]_c elevation in cells whose mitochondria are depolarized by inhibitionof the ATP synthase and respiratory chain (conditions which avoidATP depletion) was attributed to enhanced Ca²⁺ extrusion from the cell rather than inhibited Ca²⁺ entry via the NMDA receptor. Even in the presence of elevatedextracellular Ca²⁺, when [Ca²⁺]_c responses were restored to control values, such cells showedresistance to acute excitotoxicity, defined as a delayed cytoplasmicCa²⁺ deregulation (DCD) during glutamate exposure. DCD was a functionof the duration of mitochondrial polarization in the presenceof glutamate rather than the total period of glutamate exposure.Once initiated, DCD could not be reversed by NMDA receptor inhibition.In the absence of ATP synthase inhibition, respiratory chain inhibitorsproduced an immediate Ca²⁺ deregulation (ICD), ascribed to an ATP deficit. In contrast toDCD, ICD could be reversed by subsequent ATP synthase inhibitionwith or without additional NMDA receptor blockade. DCD could notbe ascribed to the failure of an ATP yielding metabolic pathway.It is concluded that mitochondria can control Ca²⁺ extrusion from glutamate-exposed granule cells by the plasmamembrane in three ways: by competing with efflux pathways forCa²⁺, by restricting ATP supply, and by inducing a delayed failureof Ca²⁺ extrusion. Inhibitors of the mitochondrial permeability transitiononly marginally delayed the onset ofDCD.

Key words: glutamate; excitotoxicity; mitochondria; calcium; granule cell; NMDA

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In common with many other cultured neurons, rat cerebellar granule cells die after extended NMDA receptor activation (Garthwaite,1986; Novelli et al., 1988; Manev et al., 1989). There is increasingevidence that mitochondrial dysfunction plays a primary role inthe initiation of both necrotic and apoptotic neuronal cell death(for review, see Beal, 1996; Petit et al., 1996; Richter et al.,1996; Henneberry, 1997; Nicotera and Leist, 1997; Nicholls andBudd, 1998). However, unraveling the multiple roles of the organellein this context is not trivial, because each mitochondrial functioncan in turn influence, and be influenced by, the other parameters.In particular, the mitochondrial membrane potential ( $Delta$ $Psi$ _m) or thefull proton electrochemical potential ( $Delta$ p) controls ATP generationby the ATP synthase (Nicholls and Ferguson, 1992), Ca²⁺ sequestration within the mitochondrial matrix (Nicholls and Åkerman,1982; Gunter and Gunter, 1994), and superoxide generation by therespiratory chain (Beal et al., 1997; Korshunov et al., 1997;Nègre-Salvayre et al., 1997), and may additionally affect themitochondrial permeability transition (Halestrap et al., 1997;Scorrano et al., 1997), outer membrane rupture, and cytochromec release (Liu et al., 1996; Yang et al., 1997; Kroemer et al.,1998; but see Kluck et al., 1997; Bossy-Wetzel et al., 1998).

Glutamate-induced neuronal necrosis is preceded by a rapid uncontrolled increase in cytoplasmic free Ca²⁺ ([Ca²⁺]_c) concentration, which occurs stochastically within a fieldof neurons (Dubinsky et al., 1995) and has been termed delayedCa²⁺ deregulation (DCD) (Tymianski et al., 1993). Mitochondrial depolarizationafter glutamate exposure has been reported to be an early eventassociated with neuronal Ca²⁺ loading (Ankarcrona et al., 1996; Isaev et al., 1996; Khodorovet al., 1996b; Schinder et al., 1996; White and Reynolds, 1996;Keelan et al., 1998). However, the distinction is not always drawnbetween a reversible, physiological response to increased energydemand and a pathological depolarization after mitochondrial damage.Because we (Budd and Nicholls, 1996b) and others (Tan et al.,1997; Stout et al., 1998) have reported that complete depolarizationof mitochondria before glutamate exposure is acutely neuroprotective,the implication is that polarized mitochondria, perhaps in responseto excessive Ca²⁺ loading, generate a factor or create a condition triggering subsequentnecrotic cell death. However, the nature of this factor, whichcould be a high cytoplasmic Ca²⁺ per se, the mitochondrial permeability transition, reactive oxygen-induceddamage, metabolic inhibition, etc., remainsunclear.

The existence of specific mitochondrial inhibitors allows each function of the organelle to be investigated separately. Thus,it is possible to eliminate a failure of oxidative phosphorylationas a cause of DCD in cerebellar granule cells, because the delayand extent of glutamate-induced deregulation are unaffected incells whose mitochondrial ATP synthase has been inhibited by oligomycin(Budd and Nicholls, 1996b) and thus rely on glycolysis to maintainATP/ADP ratios (Budd and Nicholls, 1996a). In the present report,we investigate the significance of other mitochondrial parametersin the induction of DCD, as well as the basis of the counter-intuitivefinding that cytoplasmic Ca²⁺ transients in these cells are consistently decreased when mitochondriaare depolarized, without depleting ATP (Budd and Nicholls, 1996b),an observation which has recently been challenged (Khodorov etal., 1996c). It is concluded that mitochondrial Ca²⁺ accumulation influences Ca²⁺ efflux from the granule cells both acutely, accounting for theeffect on the initial Ca²⁺ transients, and progressively, culminating inDCD.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
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Materials. Fura-2 acetoxymethyl ester (fura-2 AM) was obtained from Molecular Probes (Leiden, The Netherlands). (5R,10S)-(+)-5-methyl-10,11-dihydro[a,d]cyclohepten-5,10-iminehydrogen maleate (MK-801) was obtained from Research Biochemicals(SEMAT, St. Albans, Hertfordshire, UK). Fetal calf serum and minimalessential medium were obtained from Life Technologies (Paisley,Strathclyde, UK). Bongkrekic acid and N-methylval-4-cyclosporin(SDZ 220-384) were kindly donated by Dr. M. Klingenberg (Universityof Munich, München, Germany) and Novartis Pharma Inc. (Basel,Switzerland), respectively. Cyclosporin A, ionomycin, ketamine,oligomycin, rotenone, and all other reagents were obtained fromSigma (Poole, Dorset,UK).

Preparation of cerebellar granule cells. Granule cells were prepared as described previously (Courtney et al., 1990) from7-d-old Wistar rats. Cells were plated on poly-D-lysine-coatedglass coverslips (13 mm circular for nonperfusion experimentsand 22 mm square for use with the perfusion chamber in Fig. 1A-C)at a density of 280,000 cells per coverslip for imaging studiesand 750,000 per coverslip for ⁴⁵Ca²⁺ determination. Cells were cultured in minimal essential mediumcontaining Earle's salts (Life Technologies) plus 10% (v/v) fetalcalf serum, 25 mM KCl, 30 mM glucose, 2 mM glutamine, 100 µg/mlstreptomycin, and 100 U/ml penicillin. After 24 hr, 10 µM cytosinearabinoside was added to inhibit non-neuronal cell proliferation.Cells were maintained at 37°C in a humidified atmosphere of 5%CO₂-95% air and were used after 6-8 d in vitro.

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Figure 1. Mitochondrial depolarization depresses the cytoplasmic free Ca²⁺ response to glutamate. A-C, Granule cells were perfused with incubation medium at 25°C and exposed to three sequential 60 sec pulses of 100 µM glutamate-10 µM glycine (glut). [Ca²⁺]_c was monitored in a minimum of 10 randomly selected somata. A, Individual somata show highly reproducible [Ca²⁺]_c transients in response to three pulses. B, Oligomycin (2.5 µg/ml) (oligo) did not affect the second [Ca²⁺]_c transient, but the addition of 2 µM rotenone (rot) depressed the third transient. C, Antimycin A (0.5 µM) (AA) caused a similar depression of the response in the presence of oligomycin. Under energy-deficient conditions, when in the presence of rotenone minus oligomycin (D) or in the absence of glucose (E), glutamate-glycine produces a large transient, followed by immediate deregulation. Data are representative of at least four independent experiments.

Incubation conditions. The incubation medium contained 120 mM NaCl, 3.1 mM KCl, 0.4 mM KH₂PO₄, and 20 mM N-tris(hydroxymethyl)methyl-2-aminoethanesulfonicacid, pH adjusted to 7.4 at the temperature of the subsequentexperiment (37°C, except for Fig. 1), with NaOH, 5 mM NaHCO₃,1.2 mM Na₂SO₄, and 1.3 mM CaCl₂. Unless otherwise stated, allexperiments were performed at 37°C in Mg²⁺-free incubation medium in the presence of 15 mM glucose. Experimentsshown in Figure 1A-C were designed to correspond to the conditionsused by Khodorov et al. (1996c) and were performed at 25°C inthe presence of 5 mMglucose.

Imaging of [Ca²⁺]_c in single cells. Single cell imaging was performed in a MiraCal Imaging facility (Life Science Resources,Cambridge, UK) using a Nikon DIAPHOT-TMD inverted epifluorescencemicroscope equipped with a 40× oil immersion objective and Sutterfilter wheel (excitation, 340 and 380 nm; emission >505 nm). Cellswere loaded with 3 µM fura-2 AM for 25 min in incubation mediumcontaining an additional 30 µg/ml bovine serum albumin, 15 mMglucose, and 1.2 mM MgCl₂. In all experiments, the objective wasfocussed on cell somata rather than neurites. All experiments,apart from those in Figure 1, were performed in a nonperfusingthermostatted chamber with a volume of 300 µl.

To approximate the conditions used by Khodorov et al. (1996c), the experiments shown in Figure 1 used square coverslips mountedin a Warner RC-21B closed bath imaging chamber on a Warner PH-2heater platform. Cells were superfused at 2 ml/min with incubationmedium (25°C) lacking Mg²⁺ and containing 5 mM glucose. Cells were exposed to three 60 secpulses of 100 µM glutamate-10 µM glycine separated by 10 min intervalsby introducing concentrated glutamate-glycine into a mixing chamberimmediately upstream of the chamber. Where indicated, incubationmedium was supplemented with 2.5 µg/ml oligomycin, 1 µM rotenone,and 0.5 µM antimycin A. Calibration was performed by the sequentialaddition of 10 µM ionomycin and 10 mM Na-EGTA. The time coursefor [Ca²⁺]_c was plotted from a minimum of ten randomly selected cellsomata.

Manganese quenching of cytoplasmic fura-2 was monitored by alternate excitation at 340 and 380 nm and emission at >505 nm.Emission intensity corresponding to the isobestic point was calculatedby interpolation using the following algorithm: F_isobestic = {(2× F_340nm) + F_380nm}/3. Cells were incubated under nonperfusingconditions at 37°C in the presence of 2.5 µg/ml oligomycin and1 µM nifedipine, with the further additions of 2 µM rotenone or2 µM ketamine, where indicated. To each experiment, 100 µM MnCl₂was added, followed by 100 µM glutamate-10 µMglycine.

⁴⁵Ca²⁺ content of cells. Coverslip-attached granule cells (7-9 d in vitro) were removed from culture medium, transferred to 24-wellplates, and preincubated for 30 min at 37°C in 350 µl of incubationmedium lacking Mg²⁺. Oligomycin (8 µg/ml) and rotenone (5 µM) were added to one seriesof experiments 2 min before addition of 100 µM NMDA plus 10 µMglycine and 1 µM nifedipine. ⁴⁵CaCl₂ (6000 Bq/well) was added 20 sec before addition of the agonist.At specified times, individual coverslips were removed from theirwells and rapidly washed three times with ice-cold incubationmedium containing 1.2 mM MgCl₂, 1 mM EGTA, and 1.3 mM unlabeledCaCl₂. ⁴⁵Ca²⁺ associated with the cells was counted by liquid scintillationcounting. Results reported are the mean ± SEM of four independentexperiments.

Statistics. Each set of single cell responses shown is representative of at least three independent experiments from differentcell preparations. Significance was assessed by unpaired-varianceStudent's t test (see Fig. 3).

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Mitochondrial depolarization and glutamate-induced cytoplasmic Ca²⁺ transients

In the absence of selective cell-permeant inhibitors of the mitochondrial Ca²⁺ uniporter, the most common approach to establishing the functionalrole of mitochondrial Ca²⁺ accumulation in neuronal Ca²⁺ homeostasis has been to collapse $Delta$ $Psi$ _m (Thayer and Miller, 1990;Duchen and Biscoe, 1992; Friel and Tsien, 1994; White and Reynolds,1995; Budd and Nicholls, 1996a,b; Park et al., 1996). Because $Delta$ $Psi$ _m is the major component of the $Delta$ p driving ATP synthesis, simpleprotonophore addition results in reversal of the ATP synthaseand rapid depletion of cytoplasmic ATP (Duchen and Biscoe, 1992a;Budd and Nicholls, 1996a; Leyssens et al., 1996). We have reportedpreviously that the increased [Ca²⁺]_c transients observed in the presence of protonophores were aconsequence of inhibited ATP-dependent Ca²⁺ efflux from the cell rather than inhibited mitochondrial Ca²⁺ sequestration (Budd and Nicholls, 1996a). Indeed, when granulecells maintained by glycolytic ATP, i.e., in the presence of theATP synthase inhibitor oligomycin, are depolarized by the furtheraddition of a respiratory chain inhibitor, acute cytoplasmic Ca²⁺ responses to KCl (Budd and Nicholls, 1996a) and glutamate (Buddand Nicholls, 1996b) are insteaddecreased.

The inference from these studies, that mitochondrial control of plasma membrane Ca²⁺ fluxes is more important than mitochondrial Ca²⁺ sequestration itself in regulating cytoplasmic Ca²⁺ responses, has been questioned by a report (Khodorov et al.,1996c) in which granule cells were superfused under somewhat differentconditions, and addition of oligomycin plus the complex III inhibitorantimycin A resulted in an initial [Ca²⁺]_c transient in response to glutamate that was essentially unchangedbut was followed by a secondary increase in [Ca²⁺]_c, similar to that seen under conditions of ATP depletion (Buddand Nicholls, 1996a). Because fundamentally opposite conclusionswere reached in these studies concerning the effect of mitochondriaon neuronal Ca²⁺ homeostasis, it is important to resolve thisdiscrepancy.

In Figure 1, [Ca²⁺]_c responses are reported for granule cells superfused under the conditions used by Khodorov et al. (1996c).Eighty percent of coverslips showed highly reproducible [Ca²⁺]_c responses in individual somata to three 60 sec pulses of 100µM glutamate-10 µM glycine with full subsequent recovery (Fig.1A); these were used for the following experiments to avoid complicationscaused by acute glutamate excitotoxicity that was seen in theremaining fraction of coverslips. In subsequent experiments, thefirst pulse acted as a control, oligomycin was present duringthe second pulse, and oligomycin plus rotenone (Fig. 1B) or antimycinA (Fig. 1C) was present for the third pulse. Although oligomycindid not affect the response of individual somata, oligomycin plusrotenone (Fig. 1B) or oligomycin plus antimycin A (Fig. 1C) substantiallyreduced the response to the subsequent glutamate-glycine pulse.The only conditions in which we have been able to reproduce therapid secondary rise in [Ca²⁺]_c after glutamate addition reported by Khodorov et al. (1996c)has been when the respiratory chain is inhibited in the absenceof oligomycin (Fig. 1D) or when substrate is limiting (Fig. 1E),both of which will result in ATPdepletion.

To account for the counter-intuitive decreased cytoplasmic Ca²⁺ response in cells whose major Ca²⁺ sink is inhibited, we have investigated whether this is attributableto inhibited uptake of Ca²⁺ or to accelerated efflux across the plasma membrane. We haveobserved previously that the total ⁴⁵Ca²⁺ accumulation of granule cells exposed to glutamate for 20 minis decreased in cells with depolarized mitochondria. Figure 2shows that this is caused by a rapid inhibition of net accumulationwithin 5 min of NMDA receptor activation.

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Figure 2. Net accumulation of ⁴⁵Ca²⁺ into NMDA-exposed cells is decreased by mitochondrial depolarization. Cells were incubated in the presence ( $bullet$ ) or absence ( $open circle$ ) of 8 µg/ml oligomycin plus 5 µM rotenone for 2 min before the addition of 100 µM NMDA, 10 µM glycine, and 1 µM nifedipine (t = 0). ⁴⁵Ca²⁺ was added 20 sec before the agonist. Results are the mean ± SEM of four independent experiments.

To determine whether the reduction in net ⁴⁵Ca²⁺ accumulation in the presence of the mitochondrial inhibitors was attributableto an inhibition of the NMDA receptor, the rate at which cytoplasmicfura-2 fluorescence is quenched by exogenous manganous ions (Miyataet al., 1991) was determined in the presence of oligomycin plusor minus rotenone. This technique has been used extensively tomonitor NMDA receptor activity in granule cells (Simpson et al.,1995; Khodorov et al., 1996a; Savidge and Bristow, 1997). Figure3 shows that addition of Mn²⁺ to the extracellular medium initiated a slow quenching of fura-2fluorescence in oligomycin-treated cells. This rate was not inhibitedby MK-801 (data not shown). Addition of glutamate-glycine increasedthe rate of quenching ninefold. No significant decrease in therate of glutamate-induced quenching was seen in cells whose mitochondriawere depolarized in the presence of both rotenone and oligomycin(Fig. 3).

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Figure 3. Mitochondrial depolarization does not inhibit the rate of NMDA receptor-induced manganese quenching of fura-2. Cells were incubated in the presence of 5 µg/ml oligomycin (control) or with the further addition of 2 µM rotenone or 2 µM ketamine, as indicated. Where indicated, 100 µM Mn²⁺ and 100 µM glutamate-10 µM glycine were added. *p < 0.05, statistically significant compared with the same condition in the absence of ketamine; n = 5.

The Mn²⁺ quench technique can detect a partial inhibition of the NMDA receptor. Thus, the competitive antagonist ketamine (2µM), which reduced the initial [Ca²⁺]_c transient to the same extent as that seen in the presence ofoligomycin plus rotenone (data not shown), produced a 30% inhibitionin the rate of Mn²⁺ quenching. Thus, if mitochondrial depolarization were producingits effects on [Ca²⁺]_c by inhibiting NMDA receptor activity, this would have beenclearly detectable. Importantly, the residual fluorescence ofcells after exposure to Mn²⁺ and glutamate was not punctate; thus, there was no contributionto the cytoplasmic [Ca²⁺]_c response by fluorescence from any fura-2 accumulated withinthe mitochondria. As a consequence, the influence of mitochondrialdepolarization on the cellular fluorescence cannot be ascribedto a decrease in a mitochondrialsignal.

Mitochondrial polarization and glutamate-induced delayed [Ca²⁺]_c deregulation

When granule cells are exposed continuously to glutamate, a high proportion of cells show a delayed failure of Ca²⁺ homeostasis. This DCD precedes and accurately predicts subsequent,predominantly necrotic cell death (Tymianski et al., 1993). Asreported previously (Budd and Nicholls, 1996b), glutamate-inducedDCD also occurs in oligomycin-treated cells and thus cannot beascribed to a failure of mitochondrial ATP synthesis, whereasmitochondrial depolarization by the further addition of rotenonebefore glutamate greatly decreases DCD. Representative tracesare shown in Figure 4, A and B. The decreased initial transientin the presence of rotenone-oligomycin is again apparent, afterwhich the cells maintain a stable plateau with only occasionalcells showing a rather sudden deregulation (Fig. 4B).

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Figure 4. DCD is controlled by the duration of mitochondrial polarization. Granule cells were incubated in the presence of 5 µg/ml oligomycin. Two micromolar rotenone was added 2 min before (B), 5 min after (C), or 35 min after (D) addition of 100 µM glutamate-10 µM glycine. Inset in C shows the change in [Ca²⁺]_c produced by rotenone addition 5 min after the amino acids. E-H, The frequency with which the indicated range of [Ca²⁺]_c is observed in individual somata 60 min after glutamate-glycine addition, corresponding to experiments shown in A-D, respectively. Each histogram contains the data from at least 130 somata and four independent experiments. Lysed cells were characterized by a loss of fluorescence and the disappearance of phase-bright somata.

The net accumulation of ⁴⁵Ca²⁺ by glutamate-exposed cells with polarized mitochondria is virtually complete within the first 5min of glutamate exposure (Fig. 2, $open circle$ ). By then, [Ca²⁺]_c has peaked and declined to an initially stable plateau (Fig.4A). Thus, because neither free cytoplasmic Ca²⁺ nor total cellular Ca²⁺ are changing at 5 min, this suggests that mitochondrial Ca²⁺ accumulation has reached a steady state by this time. To establishwhether the initial period of mitochondrial Ca²⁺ loading during the first 5 min of glutamate exposure initiatesthe sequence of events leading to deregulation or whether chronicmaintenance of the mitochondria in the Ca²⁺-loaded state is necessary, the mitochondria were subjected todelayed depolarization by the further addition of rotenone aftereither 5 (Fig. 4C) or 35 min (Fig. 4D) of glutamate exposure.Previous experiments have shown that rotenone plus oligomycincauses $Delta$ $Psi$ _m to decay within 60 sec (Budd and Nicholls, 1996a),while protons leak back into thematrix.

In contrast to the transient spike of [Ca²⁺]_c that is seen when the mitochondria within Ca²⁺-loaded cells suddenly release their Ca²⁺ to the cytoplasm (Budd and Nicholls, 1996a), after rotenone addition,the [Ca²⁺]_c of individual cells falls to a lower plateau level with nodetectable spike but with a time course consistent with the relativelyslow depolarization of the mitochondrial membrane (Fig. 4C, inset).Because the Mn²⁺ quench rate is unaffected by mitochondrial depolarization (Fig.3), it can be concluded that the activity of the plasma membraneCa²⁺ efflux pathways is enhanced such that the steady-state betweenNMDA receptor-mediated uptake and efflux from the cell is achievedat a lower bulk cytoplasmic free Ca²⁺.

The proportion of cells treated with rotenone 5 min after glutamate addition (Fig. 4C) that maintain a low [Ca²⁺]_c over the next 60 min is not significantly different from thosein which rotenone is added before glutamate (Fig. 4B). In contrast,cells whose mitochondria have remained Ca²⁺-loaded for 35 min before rotenone addition show extensive deregulation,either at the time of rotenone addition or shortly afterward (Fig.4D). In Figure 4, a good correlation is seen between the behaviorof individual cells before and after the delayed rotenone addition;those with a low, stable [Ca²⁺]_c do not undergo deregulation after rotenone, those with a rapidlyrising [Ca²⁺]_c deregulate immediately, and intermediate cells deregulate aftera short delay. The sudden deregulation of Ca²⁺ after rotenone at 35 min may be attributable to the release ofCa²⁺ from the mitochondria, overwhelming an already compromised Ca²⁺ extrusion mechanism. Thus, it appears that it is the durationfor which the mitochondria maintain an accumulation of Ca²⁺, rather than the initial extent of Ca²⁺ loading (or the duration of glutamate exposure), that definesthe sensitivity of the cells to subsequent DCD. Figure 4, E-H,shows the frequency histograms of [Ca²⁺]_c observed at 60 min in randomly selected cells on four to sixcoverslips for eachcondition.

DCD is not controlled by [Ca²⁺]_c

Because the effect of mitochondrial depolarization is to lower the initial peak and subsequent plateau of cytoplasmic freeCa²⁺ (Fig. 4B) and to decrease the extent of ⁴⁵Ca²⁺ accumulation by the cells (Fig. 2), it could be argued that theimproved survival of the cells was a consequence of a decreasedcytoplasmic Ca²⁺ rather than a specific depletion of Ca²⁺ from the mitochondrial matrix. To distinguish these possibilities,the survival of cells was compared in the presence of normal (1.3mM) and elevated (2.6 mM) extracellular Ca²⁺. In the presence of oligomycin and 2.6 mM Ca²⁺, glutamate induced rapid and complete deregulation (Fig. 5A).In contrast, nearly all the cells survived elevated external Ca²⁺ for at least 60 min of glutamate exposure in the presence ofrotenone plus oligomycin (Fig. 5B), despite a substantial elevationin the [Ca²⁺]_c plateau to levels (470 ± 23.9 nM; n = 15) in excess of theinitial plateau seen 10 min after glutamate addition to oligomycin-treatedcells in the presence of the normal 1.3 mM Ca²⁺ (401 ± 23.2 nM; n = 15) (Fig. 4A). Thus, deregulation is nota function of the cytoplasmic Ca²⁺ elevation.

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Figure 5. Mitochondrial depolarization is still neuroprotective in the presence of elevated cytoplasmic Ca²⁺. Cells were incubated in the presence of 5 µg/ml oligomycin and 2.6 mM external Ca²⁺ and exposed to 100 µM glutamate-10 µM glycine for the indicated period in the absence (A) or presence (B) of 2 µM rotenone. Where indicated, 1 µM MK-801 was added. C, D, Frequency histograms of [Ca²⁺]_c observed at 60 min in individual somata from a minimum of four independent experiments under the same conditions in the absence (C) or presence (D) of 2 µM rotenone.

The retained viability of the cells in Figure 5B is indicated by the ability of the NMDA receptor antagonist MK-801 to restorethe basal [Ca²⁺]_c in the surviving cells (Fig. 5, compare A, B). We can thusconclude that a glutamate-induced elevation of cytoplasmic Ca²⁺ is not acutely excitotoxic as long as the mitochondria aredepolarized.

The reversibility of ICD

In the absence of oligomycin, protonophore addition (Fig. 6A) or respiratory chain inhibition by antimycin A (Fig. 6B) orrotenone (Fig. 6C) results in an acute failure of cytoplasmicCa²⁺ homeostasis. Under these conditions, the glycolytic capacityof granule cells is insufficient to generate sufficient ATP tofuel the plasma membrane Na⁺/K⁺-ATPase and Ca²⁺-ATPase and also to drive the reversed mitochondrial ATP synthase(Budd and Nicholls, 1996b). Because both acute and delayed Ca²⁺ deregulation are reported as increases in [Ca²⁺]_c, it is important to establish their mechanisms.

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Figure 6. ICD under conditions of energy limitation: conditions for reversal. Granule cells were incubated from t = 0 in the presence of 1 µM carbonyl cyanide p-trifluoromethoxyphenyl hydrazone (A), 1 µM antimycin A (B), or 2 µM rotenone (C-F). At 2 min, 100 µM glutamate-10 µM glycine were added. Where indicated, 5 µg/ml oligomycin (oligo) and/or 1 µM MK-801 and 2 mM Mg²⁺ were added. Note that NMDA receptor inhibition per se does not restore Ca²⁺ homeostasis. Representative experiments from a minimum of three independent experiments are shown. Values in the insets represent the proportion of cells (mean ± SEM) showing recovery of [Ca²⁺]_c to <500 nM after 60 min of amino acid exposure.

Acute deregulation of rotenone-treated cells is virtually immediate after glutamate addition, well before the initial Ca²⁺ "spike" decays to a stable plateau (Fig. 6C). No recovery (atleast to levels detectable by fura-2, below ~2 µM) occurs in thesubsequent hour. The acute Ca²⁺ deregulation in the presence of rotenone is glutamate-dependent,because rotenone-treated cells maintain Ca²⁺ homeostasis for at least 2 hr in the presence of MK-801 (datanot shown). However, although MK-801 reverses the acute glutamate-evoked[Ca²⁺]_c elevation in granule cells incubated in the absence of respiratorychain inhibitors (Fig. 5B), MK-801 fails to reverse the acuteCa²⁺ deregulation in rotenone-treated cells when added 5 min subsequentto glutamate (Fig. 6D). Possible explanations for this failureare that the cells have suffered irreversible damage or that theenergetic collapse triggered by NMDA receptor activation is self-sustaining,even after the receptor is inhibited. Addition of oligomycin 5min after glutamate allows a slow partial recovery of Ca²⁺ homeostasis in a subset of cells (Fig. 6E). Within the next hour,45% of cells recovered (defined as a [Ca²⁺]_c <500 nM). Inhibition of both the ATP synthase and the NMDAreceptor 5 min after glutamate resulted in an almost total restorationof Ca²⁺ homeostasis (Fig. 6F). Two conclusions can be drawn. First, acuteCa²⁺ deregulation can be readily reversed. Second, inhibition of theATP synthase facilitates such reversal. The latter suggests thatthe reversed ATP synthase continues to drain cytoplasmic ATP,even after NMDA receptorinhibition.

The irreversibility of DCD

DCD occurs with the same facility after glutamate addition to both control and oligomycin-treated cells (Budd and Nicholls,1996b) and is thus not a consequence of a failure of the oligomycin-sensitiveATP synthase. The rise in [Ca²⁺]_c has been proposed to be primarily a consequence of failed Ca²⁺ efflux rather than accelerated Ca²⁺ uptake (Khodorov et al., 1993). Consistent with this, when Ca²⁺ channel inhibitors, including MK-801, are added sequentiallyto a coverslip whose individual neurons are at different stagesof deregulation (Fig. 7), it is found that although cells maintaina stable plateau, they generally show a decreased [Ca²⁺]_c on addition of the inhibitors (Fig. 7, trace c). In contrast,cells that are apparently just about to deregulate (Fig. 7, traceb) and cells that have already deregulated (Fig. 7, trace a) arenot rescued.

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Figure 7. Delayed calcium deregulation is not caused by Ca²⁺ entry through defined calcium channels. Granule cells were exposed to 100 µM glutamate-10 µM glycine at t = 2 min. After 50 min, a population of cells had deregulated. Ca²⁺ channel antagonists were added sequentially, where indicated by the dotted lines: (1) 1 µM nifedipine; (2) 5 µM Conus magnus toxin-MVIIC; (3) 1 µM 6-nitro-7-sulfamoyl-benzo[f]quinoxaline-2,3-dione; and (4) 1 µM MK-801. The [Ca²⁺]_c responses of three representative cells are shown: cell a had deregulated before addition of the inhibitors, cell b initiated deregulation, and cell c recovered to a lower [Ca²⁺]_c.

Population ATP/ADP ratios decline in granule cells exposed to glutamate in the presence or absence of oligomycin (Budd andNicholls, 1996b). Because ATP is required for two steps in glycolysis,a decline in ATP below a critical threshold can lead to an inhibitionof glycolysis that could rapidly feed forward to produce a suddencollapse in ATP production. Granule cells can be maintained byglucose in the presence of oligomycin [in which case, ATP generationis purely glycolytic (Fig. 4)] or in the absence of oligomycinand glucose by the addition of lactate (Fig. 8A) or pyruvate (Fig.8B), when ATP generation is purely by oxidative phosphorylation.In the absence of any added substrate, the cells deregulated within5-10 min of glutamate addition (Fig. 1E). The response of cellsin the presence of these nonglycolytic substrates (Fig. 8A,B)is remarkably similar to that in the presence of glucose, includinga similar time course for DCD. Thus, DCD is not a phenomenon thatis seen only during glycolysis. Furthermore, DCD in the presenceof glucose cannot be reversed by the subsequent addition of lactateplus pyruvate (Fig. 8C). Because pyruvate, added directly or generatedfrom lactate, is an effective substrate for the in situ mitochondria(Schurr et al., 1997) and does not require ATP for its metabolism,its addition (in the absence of oligomycin) might have reverseda delayed deregulation that was a consequence of failed glycolysis.

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Figure 8. DCD occurs in the presence of nonglycolytic substrates and is not reversed by additional substrate. Granule cells were incubated in the absence of glucose and the presence of 10 mM lactate (A), 10 mM pyruvate (B), or 15 mM glucose (C). In each case, cells were exposed to 100 µM glutamate-10 µM glycine for the period indicated. C, At 30 min, 10 mM lactate plus 10 mM pyruvate were added to provide additional mitochondrial substrate. Oligomycin was not present in these experiments.

DCD is not prevented by inhibitors of the mitochondrial permeability transition

The mitochondrial permeability transition (MPT) is a permeabilization of the inner membrane to solutes up to 1500 Da, whichcan be observed with isolated mitochondria as a consequence ofCa²⁺ overload in the presence of phosphate under oxidizing conditions(Zoratti and Szabo, 1995; Vercesi et al., 1997). The MPT resultsin mitochondrial swelling, rupture of the outer membrane, andrelease of cytochrome c. In isolated mitochondria, the MPT isinhibited by cyclosporin A and N-methylval-4-cyclosporin (Nicolliet al., 1996) and by bongkrekic acid, which locks the adeninenucleotide translocator in the M-conformation (Halestrap and Davidson,1990). Most of the experimental evidence for the MPT has comefrom liver or heart mitochondria or from cellular systems fromhepatocytes and astrocytes (Kristal and Dubinsky, 1997). Figure9 shows that preincubation of the cells with 1 µM cyclosporinA (Fig. 9B) or 1 µM N-methylval-4-cyclosporin (Fig. 9C) for 5min resulted in only a slight delay of the onset of DCD. Increasingthe concentration (up to 10 µM) or preincubation time (up to 30min) for the cyclosporins failed to produce more extensive protection(data not shown). Bongkrekic acid (20 µM preincubated for 5 min)also failed to delay DCD significantly (data not shown).

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Figure 9. Cyclosporin A and N-methylval-4-cyclosporin fail to protect cells against delayed calcium deregulation. Cells were exposed to 100 µM glutamate-10 µM glycine in the absence of oligomycin. A, Control. Cells were preincubated with 1 µM cyclosporin A (B) or 1 µM N-methylval-4-cyclosporin (C) for 5 min before addition of glutamate-glycine.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The complexity of the interactions between mitochondria and the rest of the cell during acute glutamate excitotoxicity hasto date hindered elucidation of the mechanism(s) responsible forDCD preceding neuronal necrosis (Tymianski et al., 1993). In thispaper, we have separated three conditions under which mitochondriainfluence glutamate-evoked [Ca²⁺]_c: during the initial response to glutamate, during acute energydeficit, and during DCDitself.

The acute subexcitotoxic [Ca²⁺]_c response of granule cells to glutamate is attenuated when mitochondria are depolarized (Fig.1) under conditions that do not deplete cytoplasmic ATP (Buddand Nicholls, 1996b). No effect on the entry of the Ca²⁺ surrogate Mn²⁺ can be detected (Fig. 3), and because both the total ⁴⁵Ca²⁺ content of the cells (Fig. 2) and [Ca²⁺]_c elevation (Fig. 1) are decreased, this suggests that Ca²⁺ efflux from the cell is facilitated, allowing a kinetic balancebetween uptake and efflux to be achieved at a lower indicated[Ca²⁺]_c. Because rotenone-oligomycin-induced depolarization also resultsin decreased KCl-evoked cytoplasmic elevations (Budd and Nicholls,1996a), it can be concluded that mitochondria can influence there-extrusion of Ca²⁺ entering via both NMDA receptors and voltage-activated ion channelsand that extrusion can be activated during the rising phase ofthe fura-2 transient sufficiently rapidly to limit the peak [Ca²⁺]_c.

The plasma membrane Na⁺ electrochemical gradient is decreased in the presence of glutamate as a consequence of plasma membranedepolarization and cytoplasmic Na⁺ elevation (Kiedrowski et al., 1994). Under these conditions,Na⁺/Ca²⁺ exchange would be thermodynamically incapable of extruding Ca²⁺, and the plasma membrane Ca²⁺-ATPase must be considered the dominant pathway of Ca²⁺ extrusion from the cell (Khodorov et al., 1995). In additionto requiring ATP, the activity of this calmodulin-activated ionpump is highly dependent on the local Ca²⁺ concentration in its environment (Monteith and Roufogalis, 1995;Werth et al., 1996) and will sense the high subplasmalemmal Ca²⁺ concentration resulting from the activation of proximal ion channels(Monteith and Roufogalis, 1995; Marsault et al., 1997). The localCa²⁺ in this domain, monitored by recombinant targeted aequorin, canexceed ten times the bulk [Ca²⁺]_c during ion channel activation (Marsault et al., 1997). Themitochondria within the small granule cell somata are locatedclose to the plasma membrane (Van-Vliet et al., 1989), and itis possible that they may compete for this local Ca²⁺, decreasing the activity of the Ca²⁺-ATPase and allowing the bulk cytoplasmic [Ca²⁺]_c detected by the Ca²⁺ indicator to rise. Additionally, it is clear that any restrictionin ATP synthesis by respiratory inhibition (Fig. 6) or substratelimitation (Fig. 1E) enhances the cytoplasmic Ca²⁺signals.

We reported previously that DCD was strongly inhibited when mitochondria were depolarized before glutamate (Budd and Nicholls,1996b), and the results reported in Figure 4 extend this by demonstratingthat DCD is a function of the period for which the mitochondriaare polarized. Thus, the correlation reported by Tymianski etal. (1993) between the duration of glutamate exposure and thesubsequent extent of DCD may be more accurately restated as theduration for which mitochondria are Ca²⁺-loaded. An important control (Fig. 5) is that mitochondrial depolarizationis protective, even in the presence of elevated external Ca²⁺, when the initial peak and plateau [Ca²⁺]_c responses of rotenone-oligomycin-pretreated cells (Fig. 5B)are at least as great as those seen in the presence of oligomycinand normal extracellular Ca²⁺ (Fig. 4A). Thus, the protective effect of mitochondrial depolarizationis not related to its ability to maintain lower cytoplasmic Ca²⁺concentrations.

Because we and most other groups rely heavily on measurements of cytoplasmic free Ca²⁺, it is important to establish the distinction between DCD andthe virtually ICD of cytoplasmic Ca²⁺ seen under conditions of acute energy limitation (Fig. 6) whenCa²⁺ extrusion from the cell will be inhibited. Glutamate-inducedICD can be seen in these cells during substrate limitation (Fig.1E) and after the addition of protonophore (Fig. 6A) or respiratorychain inhibitors (Fig. 6B,C) in the absence of oligomycin, whenATP synthase reversal rapidly depletes cytoplasmic ATP (Budd andNicholls, 1996b). Interestingly, although ICD is induced by glutamateaddition, it is not reversed by NMDA receptor inhibition (Fig.6D) unless the ATP synthase is inhibited (Fig. 6E,F). This suggeststhat ATP hydrolysis by the mitochondria may deplete cytoplasmicATP to the extent that the ATP-requiring steps in glycolysis areunable to reactivate glycolysis (Erecinska et al., 1996). Significantly,after an initial enhancement caused by the Pasteur effect, glycolysisrapidly fails in rotenone-treated isolated nerve terminals (Kauppinenand Nicholls, 1986).

Whereas ICD can be reversed by restoring metabolic competence, DCD cannot be reversed by NMDA receptor inhibition in the presence(Fig. 5A) or absence (Fig. 7) of oligomycin or by the additionof alternative substrates, such as lactate or pyruvate (Fig. 8C).ATP generation by lactate-derived pyruvate is by oxidative phosphorylation;thus, DCD cannot be ascribed to failed glycolysis. Conversely,the ability to see DCD in the presence of oligomycin eliminatesa failure of oxidative phosphorylation. Khodorov et al. (1996a)have reported no increase in the rate of Ca²⁺ entry into granule cells undergoing DCD, as determined by Mn²⁺-induced fura-2 quenching, and this is consistent with our failureto reverse or stop DCD by a cocktail of channel inhibitors (Fig.7).

The MPT can be readily observed with isolated mitochondria incubated with Ca²⁺ in the presence of phosphate and is facilitated by oxidativestress and inhibited by adenine nucleotides, bongkrekic acid,oligomycin, and certain cyclosporin derivatives (for review, seeZoratti and Szabo, 1995; Bernardi and Petronilli, 1996). Evidencefor the involvement of the MPT in intact cells is based primarilyon the action of cyclosporin A. However, this immunosuppressant,in complex with its cyclophilin, is a potent inhibitor of calcineurin(Sabatini et al., 1997) and will result in a hyperphosphorylatedstate of a multiplicity of proteins. Thus, although cyclosporinA inhibits glutamate-induced necrosis and apoptosis in granulecells (Ankarcrona et al., 1996), this is attributable to calcineurininhibition rather than inhibition of the MPT. We observed onlya marginal retardation of DCD with cyclosporin A, the more selectiveN-methylval-4-cyclosporin, or bongkrekic acid and thus have noconvincing evidence for a significant role for the MPT under theseconditions. Specifically, DCD occurs in the presence of each ofthese agents (Fig. 9); thus, assuming their effectiveness in thispreparation, DCD cannot be a manifestation of the permeabilitytransition. It should also be borne in mind that oligomycin, whichis present routinely in these experiments, is also an inhibitorof the MPT (Nicholls and Åkerman, 1982).

What then is the mechanism of DCD and by extension acute glutamate-induced neuronal necrosis? Failure of oxidative phosphorylationcan be eliminated, because the phenomenon occurs after the samedelay in oligomycin-treated cells (Budd and Nicholls, 1996b);this also argues against an inexorable rise in cellular ATP demand,because oligomycin-treated cells have a restricted ATP-generatingcapacity, relying entirely on glycolysis. Failure of glycolysisitself is inconsistent with the inability of the additional substratelactate to rescue deregulating cells (Fig. 8). Activation of Ca²⁺ entry pathways is inconsistent with the failure of a cocktailof channel inhibitors to affect the final rise in [Ca²⁺]_c (Fig. 7) and with the failure to observe enhanced Mn²⁺ quenching during DCD (Khodorov et al., 1996a). Release of mitochondrialCa²⁺ stores caused by the MPT is inconsistent with the ineffectivenessof three inhibitors of the permeability transition (four includingoligomycin) (Figure 9). A factor dependent on an elevation in[Ca²⁺]_c can be eliminated, because cells with depolarized mitochondriawithstand a high cytoplasmic Ca²⁺ without undergoing DCD (Fig. 5). Almost by elimination, one isforced to focus on inhibition of the plasma membrane Ca²⁺-ATPase as a consequence of a process dependent on the durationfor which the closely adjacent mitochondria are polarized andloaded with Ca²⁺ (Fig. 4). It is notable that plasma membrane efflux can copewith Ca²⁺ released by depolarizing mitochondria after 5 min (Fig. 4C) butnot after 35 min (Fig. 4D).

Oxidative stress is an obvious candidate for this mechanism. Enhanced superoxide generation by glutamate-exposed neurons hasbeen extensively reported (Lafon-Cazal et al., 1993; Culcasi etal., 1994; Gunasekar et al., 1995), although assays involvingthe generation of products whose fluorescence is dependent on $Delta$ $Psi$ _m (e.g., hydroethidine oxidation to ethidium monomer and dihydrorhodamine-123oxidation to rhodamine-123) may be ambiguous under conditionsthat are associated also with mitochondrial depolarization (Buddet al., 1997). However, enhanced mitochondrial superoxide generationper se may be insufficient to induce DCD, because the protectionafforded by the combination of oligomycin and antimycin A (Nichollsand Budd, 1998), which leads to enhanced superoxide generation(Budd et al., 1997), is similar to that seen with rotenone-oligomycin,which does not (R. F. Castilho and D. G. Nicholls, unpublishedobservations). Finally, although the plasma membrane Ca²⁺-ATPase has been reported to be very sensitive to oxidative damage(Zaidi and Michaelis, 1998), definitive proof of oxidative damageto the Ca²⁺-ATPase is stilllacking.

Two additional studies have demonstrated the acute neuroprotective effect of mitochondrial depolarization. Sengpiel et al.(1998) have recently reported that rotenone-oligomycin protectedprimary rat hippocampal neurons from NMDA excitotoxicity, whereasStout et al. (1998) observed that protonophore increased the cytoplasmicCa²⁺ responses of rat forebrain neurons but decreased excitotoxicity.Thus, our observation may be applicable to a variety ofneurons.

  FOOTNOTES

Received June 22, 1998; revised Sept. 25, 1998; accepted Sept. 25, 1998.

This work was supported by Wellcome Trust Grant 040237 and the Medical Research Council (research studentships to S.L.B. andM.W.W.). We thank Hazel Leith for expert technicalassistance.
Correspondence should be addressed to D. G. Nicholls, Neurosciences Institute, Department of Pharmacology and Neuroscience,University of Dundee, Ninewells Medical School, Dundee DD1 9SY,Scotland, UnitedKingdom.

Dr. Hansson's present address: Wallenberg Neuroscience Center, Department of Physiology and Neuroscience, Lund University,Soelvegatan 17, Lund S-223 62,Sweden.

Dr. Budd's present address: Cerebrovascular and Neuroscience Institute, Harvard Medical School, 221 Longwood Avenue, Brighamand Women's Hospital, Boston, MA02115.

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Materials & Methods
Results
Discussion
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