AMPA Exposures Induce Mitochondrial Ca2+ Overload and ROS Generation in Spinal Motor Neurons In Vitro

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The Journal of Neuroscience, January 1, 2000, 20(1):240-250

AMPA Exposures Induce Mitochondrial Ca²⁺ Overload and ROS Generation in Spinal Motor Neurons In Vitro
Sean G. Carriedo³, Stefano L. Sensi¹, Hong Z. Yin¹, and John H. Weiss¹^,²^,³
Departments of ¹ Neurology, ² Anatomy and Neurobiology, and ³ Neurobiology and Behavior, University of California, Irvine, Irvine, California 92697-4292

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The reason for the selective vulnerability of motor neurons in amyotrophic lateral sclerosis (ALS) is primarily unknown. Apossible factor is the expression by motor neurons of Ca²⁺-permeable AMPA/kainate channels, which may permit rapid Ca²⁺ influx in response to synaptic receptor activation. However,other subpopulations of central neurons, most notably forebrainGABAergic interneurons, consistently express large numbers ofthese channels but do not degenerate in ALS. Indeed, when subjectedto identical excitotoxic exposures, motor neurons were more susceptiblethan GABAergic neurons to AMPA/kainate receptor-mediated neurotoxicity.Microfluorimetric studies were performed to examine the basisfor the difference in vulnerability. First, AMPA or kainate exposuresappeared to trigger substantial mitochondrial Ca²⁺ loading in motor neurons, as indicated by a sharp increase inintracellular Ca²⁺ after addition of the mitochondrial uncoupler carbonyl cyanidep-(trifluoromethoxy)phenyl hydrazone (FCCP) after the agonistexposure. The same exposures caused little mitochondrial Ca²⁺ accumulation in GABAergic cortical neurons. Subsequent experimentsexamined other measures of mitochondrial function to compare sequelaeof AMPA/kainate receptor activation between these populations.Brief exposure to either AMPA or kainate caused mitochondrialdepolarization, assessed using tetramethylrhodamine ethylester,and reactive oxygen species (ROS) generation, assessed using hydroethidine,in motor neurons. However, these effects were only seen in theGABAergic neurons after exposure to the nondesensitizing AMPAreceptor agonist kainate. Finally, addition of either antioxidantsor toxins (FCCP or CN) that block mitochondrial Ca²⁺ uptake attenuated AMPA/kainate receptor-mediated motor neuroninjury, suggesting that the mitochondrial Ca²⁺ uptake and consequent ROS generation are central to the injuryprocess.

Key words: glutamate; kainate; hydroethidine; oxidative stress; mitochondria; GABA; ALS

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Amyotrophic lateral sclerosis (ALS) is a neurodegenerative disease characterized by the progressive loss of upper (Betz cells)and lower (ventral horn) motor neurons. Although of unknown cause,abnormalities in glutamate uptake (Rothstein et al., 1992) andmetabolism (Plaitakis and Caroscio, 1987; Hugon et al., 1989a;Rothstein et al., 1990) suggest that excitotoxic injury may contribute(Leigh and Meldrum, 1996; Rothstein, 1996; Shaw and Ince, 1997).Although NMDA receptors likely contribute critically to neuronalinjury in various acute conditions, several observations supportthe hypothesis that AMPA/kainate receptors may be of greater importanceto the neurodegenerative process seen in ALS. First, three syndromeswith prominent motor system manifestations, lathyrism (Spenceret al., 1986), domoic acid toxicity (Teitelbaum et al., 1990),and $beta$ -N-methylamino-L-alanine toxicity (Spencer et al., 1987),are linked to the consumption of AMPA/kainate receptor agonistsfound in the environment (Ross et al., 1987; Bridges et al., 1989;Debonnel et al., 1989; Weiss et al., 1989). In addition, kainateexposures preferentially injure motor neurons both in vivo (Hugonet al., 1989b) and in vitro (Carriedo et al., 1995, 1996; Rothsteinand Kuncl, 1995), and AMPA/kainate receptor antagonists protectagainst motor neuron degeneration caused by chronic blockade ofglutamate uptake in both spinal cord slice cultures (Rothsteinet al., 1993) and dissociated cultures (Carriedo et al., 1996).

Considerable evidence supports a link between Ca²⁺ influx and glutamate receptor-mediated neurodegeneration. Brief periods ofactivation of highly Ca²⁺-permeable NMDA channels can result in substantial intracellularCa²⁺ accumulation and widespread neuronal injury (Hartley et al.,1993; Lu et al., 1996; Hyrc et al., 1997). Although mitochondriacan buffer these large Ca²⁺ loads (Wang et al., 1994; Werth and Thayer, 1994; White and Reynolds,1995; Babcock et al., 1997; Peng et al., 1998), they do so atthe expense of triggering injurious reactive oxygen species (ROS)production (Lafon-Cazal et al., 1993; Dugan et al., 1995; Reynoldsand Hastings, 1995; Bindokas et al., 1996). In contrast to NMDAreceptors, AMPA/kainate receptors are generally Ca²⁺ impermeable and trigger injury more slowly, with prolonged (severalhours) periods of activation needed before significant neuronalinjury occurs (Koh et al., 1990). Subpopulations of central neurons,however, are highly vulnerable to AMPA/kainate receptor-mediatedinjury (Koh and Choi, 1988; Weiss et al., 1994; Yin et al., 1994),likely attributable in part to the expression of large numbersof AMPA/kainate channels with high Ca²⁺ permeability (Ca²⁺-A/K channels) (Iino et al., 1990; Pruss et al., 1991; Brorsonet al., 1992; Turetsky et al., 1994; Lu et al., 1996). Althoughmechanisms of Ca²⁺-A/K channel-dependent neuronal injury have been studied relativelylittle, we found recently that brief kainate exposures triggerhigh [Ca²⁺]_i elevations and subsequent mitochondrial ROS production in GABAergiccortical neurons (Carriedo et al., 1998), a well defined neuronalpopulation that strongly expresses these channels (Jonas et al.,1994; Yin et al., 1994; Geiger et al., 1995).

Recent studies indicating that motor neurons often possess Ca²⁺-A/K channels (Carriedo et al., 1995, 1996; Launey et al., 1998;Terro et al., 1998; Bar-Peled et al., 1999) support the idea thatthe presence of these channels contributes to their high vulnerability.However, GABAergic cortical neurons, which also possess Ca²⁺-A/K channels and are vulnerable to rapidly triggered AMPA/kainatereceptor-mediated injury (Yin et al., 1994), do not degeneratein ALS. The broad aim of the present study was to compare thevulnerability of GABAergic cortical neurons with that of spinalmotor neurons to AMPA/kainate receptor-mediated injury and toexamine downstream sequelae of Ca²⁺ entry through Ca²⁺-A/K channels expressed on these populations that might accountfor differences in vulnerability. Specifically, because of evidencethat Ca²⁺ influx interferes with mitochondrial function, our studies focusedon assessments of mitochondrial Ca²⁺ buffering, mitochondrial depolarization, and ROSgeneration.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Chemicals and reagents. Hydroethidine (HEt) and tetramethylrhodamine ethylester (TMRE) were purchased from Molecular Probes(Eugene, OR). Fura-2FF was purchased from Texas Fluorescence Lab(Austin, TX). MK-801 was purchased from Research Biochemicals(Natick, MA). Tissue culture media and serum were from Life Technologies(Grand Island, NY). 2,3-Dihydroxy-6-nitro-7-sulfamoylbenzo(F)quinoxaline(NBQX) was kindly provided by Novo Nordisk (Malov, Denmark). NMDA,kainate, rotenone, cyanide, trolox, and carbonyl cyanide p-(trifluoromethoxy)phenylhydrazone (FCCP) were obtained from Sigma (St. Louis, MO). U74500was kindly provided by Upjohn (Kalamazoo, MI). All other chemicalsand reagents were obtained from common commercialsources.

Dissociated cultures. Dissociated cortical and spinal cord cultures were prepared primarily as described previously. Neocorticalcell suspensions were prepared from 15- to 16-d-old embryonicSwiss-Webster mice and plated 1-2 × 10⁵ cells/cm² (Yin et al., 1994). Spinal cord suspensions (removed of bothmeninges and dorsal root ganglia) were prepared from 13 d mouseembryos and plated at a density of 3 × 10⁵ cells/cm² (approximately "4 spinal cords" per 24-well plate) (Carriedoet al., 1996). Cells were plated on a previously established layerof cortical astrocytes grown on either 15 mm Primaria-coated cultureplates (Falcon, Franklin Lake, NJ) or poly-L-lysine-coated glass-bottomeddishes. Plating medium consisted of Eagle's minimal essentialmedium (MEM; Earle's salts supplied glutamine free; Life Technologies),supplemented with 10% heat-inactivated horse serum (Life Technologies),10% fetal bovine serum (Life Technologies), glutamine (2 mM; LifeTechnologies), and glucose (total, 25 mM). Cultures were maintainedin a 37°C, 5% CO₂ incubator. After 4-6 d in vitro, non-neuronalcell division was halted by exposure to 10⁵ M cytosine arabinoside for 1-3 d. The cells were then shiftedinto a maintenance medium identical to the plating medium butlacking fetal serum. Subsequent media replacement occurred twicea week. Cultures were studied after 13-17 d in vitro.

Glial cultures were prepared similarly except that tissue was obtained from early postnatal (1-3 d) mice and plating mediawas supplemented with epidermal growth factor (10 ng/ml). Cellsuspensions were plated directly on Primaria tissue culture-treatedmultiwell plates or poly-L-lysine-coated glass-bottomeddishes.

Identification of motor neurons and GABAergic cortical neurons. Motor neurons were identified using both morphological criteria(soma > 20 µm and extensive dendritic arborization) (Schaffneret al., 1987) and labeling for Sternberger Monoclonal Inc. (SMI)-32,an antibody to nonphosphorylated neurofilaments that has beenfound to label motor neurons in dissociated spinal cultures (Gotowand Tanaka, 1994; Carriedo et al., 1996; Bar-Peled et al., 1999).GABAergic cortical neurons were labeled using glutamic acid decarboxylase(GAD; Developmental Studies Hybridoma Bank at the University ofIowa, Iowa City, IA) immunohistochemistry (Yin et al., 1994).For staining, cultures were fixed for 40 min in 4% paraformaldehyde,washed three times with PBS, and incubated for 30 min with "blockingsolution" (10% heat-inactivated horse serum in PBS) to minimizebackground staining. For SMI-32, the blocking solution also included0.2% Triton X-100. Primary antibody exposures (in blocking solutionat 1:6000 for SMI-32 and 1:500 for GAD) were performed for 48-72hr at 4°C. Biotinylated secondary antibody (Vector Laboratories,Burlingame, CA), ABC solution (Vector Laboratories), and 3-amino-9-ethyl-carbazole(Sigma) were used to visualize stainedcells.

Neurotoxicity experiments. Brief (5-20 min) toxic exposures were performed in room air, using a HEPES-buffered salt solution(HSS) with the following composition (in mM): Na⁺ 130, K⁺ 5.4, Mg²⁺ 0.8, Ca²⁺ 1.8 (except where indicated), Cl 130.6, HEPES, pH 7.4 at 25°C, 20, and glucose 15. Exposures wereterminated by replacing the exposure solution with MEM + glucose,along with the ionotropic glutamate receptor antagonists MK-801and NBQX (both at 10 µM), and returning the cultures to the 37°C,5% CO₂ incubator. Longer (24 hr) exposures were in MEM + glucosein the 37°C, 5% CO₂ incubator. MK-801 (10 µM) was added duringall toxicity exposures to prevent activation of NMDA receptorsfrom endogenously released glutamate and thereby to ensure a pureAMPA/kainate receptor-mediated injurymechanism.

Overall neuronal injury was assessed 20-24 hr after the start of the exposure both by morphological examination and by quantitativemeasurement of lactate dehydrogenase (LDH) in the bathing medium,an index that is proportional to the total number of neurons damagedby excitotoxic exposure (Koh and Choi, 1987). LDH values werescaled to the near maximal mean value found in sister culturesexposed to 300 µM kainate for 24 hr (equal to 100% cellloss).

Damage to motor neurons or GABAergic neurons was assessed as the difference between the mean number of intact labeled cells(determined by direct counts) in neuronal cultures exposed toan excitotoxic agonist and the mean number in sister culturesexposed to sham wash alone (typically 200-500 labeled cells countedper culture well), expressed as a percentage of thelatter.

Imaging studies. Spinal or cortical cultures were plated on poly-L-lysine-coated glass-bottomed dishes (Mattek Cultureware,Ashland, MA) and mounted to a stage adapter on an inverted microscope(Nikon Diaphot). All agonist exposures were performed at roomtemperature (25°C) in HSS either constantly perfused or in a 1.5ml static bath. Preselected fields (typically containing 20-50healthy-appearing nonoverlapping neurons) were illuminated bya xenon light source using a Nikon 40× magnification and 1.3 numericalaperture epifluorescence oil immersion objective, and the emittedfluorescence was collected using a Hamamatsu intensified CCD camera.In all experiments, the electronic background signals (obtainedwith the camera shutter closed) were obtained at each wavelengthand subtracted from measured signals. To analyze experiments,we outlined neuronal somata and gathered data on an 80486-basedcomputer using Image-1/Fluor software from Universal Imaging Corporation(West Chester,PA).

For intracellular Ca²⁺ ([Ca²⁺]_i) measurements, cultures were loaded in the dark with 5 µM Fura-2FF AM in HSS containing 0.2% pluronicacid and 1.5% dimethylsulfoxide (DMSO) for 30-45 min at 25°C.Cultures were then washed in HSS (three times) and kept in thedark for an additional 30 min to allow for complete dye deesterification.Cells were alternately illuminated at 340 and 380 nm, and fluorescencewas monitored at 510 nm. [Ca²⁺]_i was determined by the equation: [Ca²⁺]i = K_D (F_min/F_max) [(R $-$ R_min)/(R_max $-$ R)], where R is the observed340:380 fluorescence ratio (Grynkiewicz et al., 1985) and theK_D used was 35 µM (Golovina and Blaustein, 1997). F_min indicates380 nm fluorescence at R_min, and F_max indicates 380 nm fluorescenceat R_max. Because of the very low affinity of Fura-2FF for Ca²⁺, R_min is the 340:380 fluorescence ratio determined at the startof each experiment. Control experiments revealed a negligibledifference (<0.1 ratio unit) between this value and the R_min obtainedin the presence of 2 mM EGTA, 0 Ca²⁺, and 2 µM ionomycin. R_max is the 340:380 fluorescence ratio valuedetermined in the same neurons exposed to 10 µM ionomycin in thepresence of 30 mM Ca²⁺. R_min (and baseline ratios) ranged from 0.5 to 0.8, whereas R_maxranged from 5.5 to 7.5. The system was recalibrated after anyadjustments to theapparatus.

ROS production and changes in mitochondrial polarization ( $Delta$ $Psi$ _m) were monitored using the oxidation-sensitive dye HEt (Bindokaset al., 1996; Carriedo et al., 1998) and the $Delta$ $Psi$ _m-sensitive dyeTMRE (Farkas et al., 1989; Schinder et al., 1996; Carriedo etal., 1998), respectively. Advantages of HEt over other oxidation-sensitivedyes include its relative resistance to both auto- and photo-oxidation(permitting fluorescence monitoring for prolonged periods) andthe increasing intensity of the dye fluorescence seen after intercalationof ethidium within nuclear DNA (increasing sensitivity for ROSdetection). Cultures were loaded in the dark with 5 µM HEt inHSS (45 min; 25°C) or 0.5 µM TMRE in MEM (30 min; 37°C). Afterloading, cultures were washed (four times) into a static bathof HSS containing either probe. Cells were excited at 510-560nm, and emission was monitored at >590 nm. To minimize photobleaching,we attentuated the fluorescence intensity with neutral densityfilters (Omega Optical, Battleboro, VT). Camera gain was adjustedto give baseline maximal florescence levels of 20-40 (HEt experiments)or of 150-200 (TMRE experiments) arbitrary units of a maximaleight-bit signal output of 256. Fluorescence measurements foreach cell (F_x) were normalized to the fluorescence intensity forthat cell at the beginning of the experiment (F₀). In the TMREexperiments, fluorescence changes were monitored only in "mitochondria-rich"perinuclear regions of the soma, which undergo sharp decreasesin fluorescence after mitochondrial depolarization. In HEt experiments,ROS production causes an increase in somatic and nuclear fluorescence.Because HEt fluorescence is cumulative, the rate of ROS generationwas assessed as the rate of increase (or slope) of the F_x/F₀ curvesover time, and net ROS production was assessed as the increasein F_x/F₀ overbaseline.

After completion of imaging experiments, cultures were then fixed and stained for either SMI-32 (for identifying spinal motorneurons) or GAD (for identifying GABAergic cortical neurons).Only imaged fields containing labeled neurons wereanalyzed.

Experiment replication. All experiments reported represent at least four independent replications. All imaging studies representat least 7 motor and 150 other spinal neurons or 15 GABAergicand 150 other corticalneurons.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Motor neurons are more vulnerable than GABAergic cortical neurons to AMPA/kainate receptor-mediated neurotoxicity

Before comparing downstream injury mechanisms, we first set out to compare directly the vulnerability of motor neurons withthat of GABAergic cortical neurons after identical exposures tokainate or to the rapidly desensitizing agonist AMPA. To performthese studies, we prepared spinal cord cultures as described (Carriedoet al., 1996) and used the cultures after 15 d in vitro. Previouscharacterization of these cultures indicated that ~1.5% of thespinal cells in our culture system were motor neurons as assessedby morphological appearance (soma > 20 µm and extensive dendriticarborization) (Schaffner et al., 1987) and intense staining withthe neurofilament marker SMI-32, which has been found to identifymotor neurons in culture and in slice (Gotow and Tanaka, 1994;Carriedo et al., 1996). Using this culture system we find that>80% of the motor neurons express Ca²⁺-A/K channels (Carriedo et al., 1996), as indicated by histochemicallabeling for kainate-stimulated Co²⁺ uptake (Pruss et al., 1991). Previous characterization of ourcortical neuronal cultures indicated that ~9% of the neurons areGABAergic, as indicated by glutamic acid decarboxylase immunohistochemistry,and that 90% of these GABAergic neurons express Ca²⁺-A/K channels (Yin et al., 1994; Carriedo et al., 1998).

Initial neurotoxicity studies examined injury induced by prolonged (24 hr) kainate (5-10 µM) or AMPA (2.5-5 µM) exposures.After each of these exposures, both motor neurons and GABAergiccortical neurons (identified by glutamic acid decarboxylase immunohistochemistry)(Yin et al., 1994) were preferentially damaged in comparison withthe overall neuronal population (see Materials and Methods). However,in each case, the damage to the motor neurons was significantlygreater than was the damage to the GABAergic neurons (Fig. 1A).Further studies used a brief exposure paradigm with AMPA as theagonist. Although 10 min exposures to AMPA alone caused littleinjury, motor neurons and GABAergic cortical neurons were preferentiallydamaged if the AMPA receptor desensitization inhibitor cyclothiazide(100 µM) (Yamada and Tang, 1993) was added during the exposure.Again, the damage to the motor neurons was greater than was thedamage to the GABAergic neurons (Fig. 1B). The injury to bothof these populations was Ca²⁺ dependent; removal of extracellular Ca²⁺ substantially prevented injury.

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Figure 1. Spinal motor neurons are more vulnerable than GABAergic cortical neurons to AMPA/kainate receptor-mediated injury. A, Slowly triggered neurotoxicity. Spinal or cortical cultures were exposed to kainate (5-10 µM + 10 µM MK-801) or AMPA (2.5-5 µM + 10 µM MK-801) for 24 hr, followed by assessment of injury. Identification of motor neurons was based on morphology and staining for SMI-32; GABAergic cortical neurons were identified by staining for GAD. Injury to the overall spinal population (gray bars) and cortical population (hatched bars) was assessed by LDH measurement, whereas injury to motor neurons (black bars) and GABAergic cortical neurons (white bars) was assessed by direct cell counts (see Materials and Methods). B, Rapidly triggered neurotoxicity. Spinal or cortical cultures were exposed to AMPA (50 µM + 10 µM MK-801; 10 min), either alone (left) or in the presence of the AMPA receptor desensitization inhibitor cyclothiazide (100 µM; right), in either Ca²⁺-containing or Ca²⁺-free buffer as indicated. Twenty-four hours after the exposure, injury was assessed as described above. Values represent the means ± SEM compiled from at least four experiments; n = 10-12 cultures per condition. An asterisk indicates motor neuron or GABAergic cell loss significantly different from overall cell loss; an ampersand indicates motor neuron cell loss significantly different from GABAergic cell loss (p < 0.01 by two-tailed t test).

Brief kainate exposure triggers large [Ca²⁺]_i elevations and mitochondrial Ca²⁺ loading in motor neurons

In previous microfluorimetric studies we found that AMPA/kainate receptor activation triggers high [Ca²⁺]_i rises (to tens of micromoles per liter) in GABAergic corticalneurons (Carriedo et al., 1998), consistent with their frequentexpression of Ca-A/K channels. Therefore, we used similar microfluorimetrictechniques to assess kainate-triggered [Ca²⁺]_i rises in motor neurons. [Ca²⁺]_i levels were measured using the low-affinity Ca²⁺-sensitive fluorescent dye Fura-2FF (K_D = 35 µM), because recentstudies indicate that high-affinity dyes, like fura-2, may markedlyunderestimate true [Ca²⁺]_i levels (Hyrc et al., 1997; Carriedo et al., 1998; Khodorovet al., 1999; Stout and Reynolds, 1999). After dye loading, afield containing one to three neurons with the morphological featuresof motor neurons was selected, and basal [Ca²⁺]_i levels were recorded before exposing cultures to kainate (100µM + 10 µM MK-801) for 5 min. After imaging, the phenotype ofthe putative motor neurons was further assessed by staining withSMI-32. Immediately after exposure, large increases in [Ca²⁺]_i levels were seen in motor neurons (with lesser increases seenin other spinal neurons; Fig. 2).

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Figure 2. Brief kainate exposure triggers large [Ca²⁺]_i rises in motor neurons. In Fura-2FF-loaded spinal cultures, [Ca²⁺]_i levels were monitored for 5 min before and 25 min after a 5 min exposure to kainate (100 µM + 10 µM MK-801; horizontal bar). Fields selected for imaging contained morphologically identified putative motor neurons (large soma size and extensive dendritic tree); after imaging their identity was verified by immunostaining for SMI-32. Traces represent the means ± SEM of 9 motor neurons and >150 other spinal neurons derived from six experiments.

Because mitochondria are important buffers of intracellular Ca²⁺ (Wang et al., 1994; Werth and Thayer, 1994; White and Reynolds,1995; Peng et al., 1998), we next compared their role in bufferingAMPA/kainate receptor-mediated Ca²⁺ loads in motor neurons and GABAergic neurons. These studies madeuse of the protonophore FCCP, which dissipates the mitochondrialmembrane potential and releases Ca²⁺ from mitochondria, while preventing further Ca²⁺ uptake (Wang et al., 1994; White and Reynolds, 1995; Stout etal., 1998). Fura-2FF-loaded cultures were subjected to a controlpulse of AMPA (50 µM + 10 µM MK-801) or kainate (100 µM + 10 µMMK-801) for 15 sec and allowed to recover for 20 min. Cultureswere then given a second identical pulse of agonist followed immediatelyby exposure to FCCP (750 nM + 10 µM MK-801 for 2 min) (Fig. 3).In both motor neurons and GABAergic cortical neurons, exposureto either agonist triggered immediate [Ca²⁺]_i rises, which returned to baseline within 5 min. However, additionof FCCP after exposure to either agonist resulted in dramaticallyincreased [Ca²⁺]_i rises in the motor neurons but only a mild prolongation inthe [Ca²⁺]_i rises in GABAergic neurons (Figs. 3, 4), suggesting that theseexposures cause particularly high levels of mitochondrial Ca²⁺ loading in motor neurons.

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Figure 3. AMPA exposure triggers mitochondrial Ca²⁺ loading in motor neurons. Spinal cultures were loaded with Fura-2FF, and basal [Ca²⁺]_i levels were recorded before cultures were exposed to an initial AMPA pulse (50 µM + 10 µM MK-801 for 15 sec). After a 20 min recovery period, the cultures were reexposed to AMPA (50 µM + 10 µM MK-801 for 15 sec), followed immediately by a 2 min pulse of the mitochondrial protonophore FCCP (750 nM + 10 µM MK-801). Fluorescent images were taken before AMPA exposure (A), at the peak [Ca²⁺]_i rise seen during the initial AMPA exposure (B), and at the peak [Ca²⁺]_i rise seen after the AMPA/FCCP exposure (C). After imaging, the cultures were fixed and stained for SMI-32 (D). Note that exposure to AMPA followed by FCCP (C) causes higher [Ca²⁺]_i rises than occur with AMPA exposure alone (B). The pseudocolor bar shows the Fura-2FF fluorescence ratio scale. Scale bar, 50 µm.

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Figure 4. AMPA/kainate receptor activation triggers greater degrees of mitochondrial Ca²⁺ loading in motor neurons than in GABAergic cortical neurons. Fura-2FF-loaded spinal (A, B) and cortical (C, D) cultures were exposed for 15 sec to either AMPA (50 µM + 10 µM MK-801; A, C) or kainate (100 µM + 10 µM MK-801; B, D) (thin lines) and allowed to recover for 20 min. After recovery, the cultures were given an identical 15 sec agonist exposure followed immediately by FCCP (750 nM + 10 µM MK-801 for 2 min; thick lines). Traces represent means ± SEM from 10 to 20 motor neurons and >20 GABAergic cortical neurons from at least seven experiments.

To examine the duration of mitochondrial Ca²⁺ loading in motor neurons after AMPA exposure, we exposed spinal cultures to AMPAfor 15 sec as described above, but with the addition of FCCP (750nM + 10 µM MK-801 for 2 min) at various intervals (0, 3, or 10min) after the exposure (FCCP alone caused no [Ca²⁺]_i rise). The magnitude of the FCCP-induced [Ca²⁺]_i rise decreased with the increasing interval after the AMPAexposure (Fig. 5). By 20 min after the AMPA exposure FCCP no longertriggered a rise in [Ca²⁺]_i, indicating probable clearance of the mitochondrial Ca²⁺ load.

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Figure 5. Time course of recovery of AMPA-triggered mitochondrial Ca²⁺ loading in motor neurons. Fura-2FF-loaded spinal cultures were exposed to AMPA (50 µM + 10 µM MK-801 for 15 sec; A; thick line) and allowed to recover for 20 min. After recovery, the cultures were given identical 15 sec AMPA exposures followed either immediately after (B; filled circles), 3 min after (C; open circles), or 10 min after (D; open squares) by FCCP (750 nM + 10 µM MK-801 for 2 min). Note the progressive decrease in the size of the FCCP-induced [Ca²⁺]_i rise with increasing duration between AMPA and FCCP exposures. Control studies showed that in the absence of AMPA preexposures, the FCCP exposures caused no change in [Ca²⁺]_i (E; thin line). Traces represent means ± SEM from 7 to 20 motor neurons from at least five experiments.

A possible additional affect of FCCP may be that uncoupling of electron transport from ATP production could result in reversalof the ATP synthetase with consequent depletion of cellular ATPand impairment of ATPase-driven extrusion of Ca²⁺ from the cell (Budd and Nicholls, 1996). However, recent studieshave found that FCCP exposures of several minutes at levels higherthan those used here caused little ATP depletion (White and Reynolds,1995; Wang and Thayer, 1996). In addition, our conclusions arenot substantively altered even if ATP levels are depleted. Specifically,because FCCP-triggered [Ca²⁺]_i rises only occur within a 10 min period after agonist-triggeredCa²⁺ loading, the FCCP-triggered rise must represent cytosolic accumulationof Ca²⁺ that had been sequestered during the brief agonistexposure.

AMPA exposure causes strong mitochondrial depolarization and ROS generation in motor neurons

Because above studies suggest that the degree of mitochondrial Ca²⁺ loading may be a key factor differentiating the responses ofmotor neurons from those of GABAergic neurons to AMPA/kainatereceptor activation, subsequent experiments focused on the comparisonof other indexes of mitochondrial function. To examine the AMPA/kainatereceptor-mediated changes in the mitochondrial membrane potential( $Delta$ $Psi$ _m) that might occur in response to mitochondrial Ca²⁺ uptake, we used the dye TMRE that rapidly equilibrates betweencellular compartments as a function of potential differences;the rapid loss of fluorescence from cellular domains rich in mitochondriais indicative of loss of $Delta$ $Psi$ _m (Farkas et al., 1989; Schinder etal., 1996). In a previous study we reported that rapid kainateexposure triggers abrupt loss of $Delta$ $Psi$ _m in GABAergic cortical neurons,reflecting the rapid Ca²⁺ influx through Ca²⁺-A/K channels expressed on these cells (Carriedo et al., 1998).

In TMRE-loaded spinal or cortical cultures, the fluorescence in mitochondrial-rich perinuclear regions was measured before,during, and for 30 min after a 10 min exposure to either AMPA(50 µM + 10 µM MK-801) or kainate (100 µM + 10 µM MK-801). Althoughmotor neurons typically showed strong basal TMRE fluorescence,presumably indicative of large numbers of mitochondria in theperinuclear region, AMPA and kainate exposures triggered substantialdecreases in TMRE fluorescence in motor neurons that persistedlong after the end of the exposure (Figs. 6, 7). In contrast,in GABAergic cortical neurons, kainate exposures triggered a moderatedecrease in TMRE fluorescence, while little change was seen inresponse to AMPA exposures. It is possible that slow decreasesin TMRE fluorescence could partially reflect Na⁺-dependent plasma membrane depolarization with redistributionof dye from the cytoplasmic space, in addition to more rapid fluorescencedecreases resulting from Ca²⁺-dependent loss of $Delta$ $Psi$ _m. However, the lack of comparable fluorescencechanges in the non-GABAergic cortical neurons and the nonmotorspinal neurons provides an internal control indicating that thesignal is caused by loss of $Delta$ $Psi$ _m, because kainate induces Na⁺-dependent neuronal depolarization in virtually all neurons. Infurther control studies, removal of Ca²⁺ from the media during kainate exposures (10 min; 100 µM) preventedTMRE fluorescence decreases in cortical neurons expressing Ca²⁺-A/K channels (normalized TMRE fluorescence at the end of theexposure, 1.02 ± 0.02 in the absence of Ca²⁺; 0.81 ± 0.04 with Ca²⁺; n > 28 neurons from four experiments in each condition).

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Figure 6. AMPA exposure causes mitochondrial depolarization in motor neurons. TMRE-loaded spinal cultures were exposed to AMPA (50 µM for 10 min). Fluorescent images were obtained before (A), during (8 min; B), and 30 min after termination of (C) the exposure. After imaging, the culture was stained for SMI-32 (D). Note the relatively selective and long-lasting decrease in TMRE fluorescence seen in the mitochondrial-rich perinuclear regions of the motor neuron, indicative of significant mitochondrial depolarization. The pseudocolor bar shows the eight-bit intensity scale used for TMRE fluorescence. Scale bar, 50 µm.

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Figure 7. AMPA/kainate receptor activation causes greater mitochondrial depolarization in motor neurons than in GABAergic cortical neurons. In TMRE-loaded spinal (A, B) and cortical (C, D) cultures, the fluorescence in mitochondrial-rich regions was measured for 10 min before, during, and for 30 min after a 10 min exposure to AMPA (50 µM + 10 µM MK-801; A, C) or kainate (100 µM + 10 µM MK-801; B, D). Note the substantially greater decrease in fluorescence in motor neurons compared with GABAergic neurons after AMPA exposure in contrast to the similar fluorescence changes after kainate exposures. Traces represent the means ± SEM compiled from 10 to 17 motor and 150 other spinal neurons and from 40 to 70 GABAergic and 200 other cortical neurons from at least seven experiments. KA, Kainate.

To address further the possible differences between motor neurons and GABAergic cortical neurons in downstream responses toAMPA/kainate receptor activation, we examined kainate-inducedROS production using the oxidation-sensitive dye HEt that readilypermeates living cells and is reported to be oxidized selectivelyby superoxide radicals into the highly fluorescent compound ethidium(Bindokas et al., 1996) (see Materials andMethods).

We reported previously that kainate exposure triggers HEt oxidation in GABAergic neurons. Thus before comparing HEt responsesbetween motor neurons and GABAergic neurons during and after briefagonist exposures, we first characterized changes in HEt fluorescencein motor neurons triggered by prolonged kainate exposures. InHEt-loaded cultures, fluorescence readings were acquired for 10min before and for 25 min after addition of kainate (100 µM +10 µM MK-801). Basal ROS production was minimal as evidenced bythe stable but small increases in neuronal HEt fluorescence seenduring the baseline period (Fig. 8). As we observed previouslyin GABAergic cortical neurons, motor neurons displayed noticeableincreases in fluorescence within 3 min of kainate exposure. Atthe end of the exposure, motor neurons showed substantially greaterincreases in HEt fluorescence than do most other spinal neurons(normalized fluorescence increase over baseline of 1.94 ± 0.49in motor neurons vs 0.40 ± 0.04 in other neurons; Fig. 8). Infurther studies, the electron transport chain inhibitor rotenonewas used to examine the role of mitochondria in kainate-triggeredROS production. In agreement with our previous findings in GABAergiccortical neurons, addition of rotenone (10 µM) for 40 min beforeand during the kainate exposure almost completely prevented theincrease in HEt fluorescence (Fig. 8).

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Figure 8. Kainate exposure triggers preferential ROS generation in motor neurons. HEt-loaded cultures were imaged for 10 min before and 25 min after addition of kainate (100 µM + 10 µM MK-801). To assess involvement of mitochondria in the ROS generation, in some cultures, we added the electron transport chain inhibitor rotenone (10 µM) for 40 min before and during the kainate exposure (broken line). After exposure, cultures were fixed and stained for SMI-32. Fluorescence changes for each neuron are expressed as the ratio of fluorescence at each time point (F_X) to its own baseline (F₀). Traces represent the means ± SEM of 7-10 motor neurons and >100 other spinal neurons derived from at least six experiments.

To address possible differences between motor neurons and GABAergic cortical neurons in downstream responses to AMPA/kainatereceptor activation, we used HEt to compare directly the ROS generationtriggered by identical 10 min AMPA or kainate exposures (Fig.9). Paralleling effects on mitochondrial potential, exposuresto either agonist triggered sharp increases in HEt fluorescencein motor neurons (normalized fluorescence increase over baselineof 3.46 ± 1.02 for AMPA; 4.43 ± 1.71 for kainate), with littleincrease in most spinal neurons (0.51 ± 0.03 for AMPA; 0.96 ±0.12 for kainate). In contrast, although kainate triggered comparableselective increases in HEt fluorescence in GABAergic neurons (3.55± 0.28 vs 0.73 ± 0.05 in most cortical neurons), AMPA exposurescaused only a moderate increase in GABAergic neurons (1.54 ± 0.2)compared with most other cortical neurons (0.61 ± 0.03).

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Figure 9. AMPA/kainate receptor activation causes greater ROS generation in motor neurons than in GABAergic cortical neurons. HEt-loaded spinal (A, B) and cortical (C, D) cultures were imaged for 5 min before and 30 min after a 10 min exposure to AMPA (50 µM + 10 µM MK-801; A, C) or kainate (100 µM + 10 µM MK-801; B, D). Traces represent the means ± SEM compiled from 10 to 12 motor and 200 other spinal neurons and from 60 GABAergic and 200 other cortical neurons from at least six experiments. Note the substantially greater fluorescence increase in motor neurons than in GABAergic neurons after AMPA exposure in contrast to the comparable fluorescence increases seen after kainate exposure (p < 0.01 by two-tailed t test).

Because a recent report by Budd et al. (1997) suggested that mitochondrial depolarization (loss of $Delta$ $Psi$ _m) might cause a voltage-dependentrelease of oxidized ethidium from the mitochondria, we previouslyperformed control studies to examine the degree to which observedkainate-triggered HEt signals reflect ROS production. First, wefound that qualitatively similar increases in fluorescence wereseen after kainate exposures in cells loaded with only 1 µM HEt,a concentration at which Budd et al. (1997) found ethidium toremain bound within the mitochondria after loss of $Delta$ $Psi$ _m (Carriedoet al., 1998). In addition, although rotenone completely blockedthe agonist-triggered increase in HEt fluorescence (as above),it had no effect on the loss of $Delta$ $Psi$ _m assessed using the $Delta$ $Psi$ _m-sensitivedye TMRE (Carriedo et al., 1998; Sensi et al., 1999). Thus, theHEt signal that is blocked by rotenone cannot simply be explainedas a loss of $Delta$ $Psi$ _m and most likely reflects ROSproduction.

AMPA/kainate receptor-mediated injury to motor neurons is dependent on mitochondrial Ca²⁺ loading and ROS generation

Finally, we examined the hypothesis that Ca²⁺ accumulation within the mitochondria and consequent ROS generation contributedirectly to AMPA/kainate receptor-mediated motor neuron injury.To assess the role of mitochondrial Ca²⁺ accumulation in the injury, we made use of either the protonophoreFCCP (750 nM) or the electron transport chain inhibitor cyanide(CN; 3 mM). In agreement with previous studies of electron transportblockers (Budd and Nicholls, 1996; Khodorov et al., 1996; Stoutet al., 1998), in control experiments we found that, like FCCP,CN also appears to trigger release of mitochondrial Ca²⁺ (as evidenced by a sharp increase in [Ca²⁺]_i when added after AMPA/kainate receptor activation; data notshown). To maximize motor neuron injury while minimizing the neurotoxicityassociated with prolonged application of FCCP or CN, we induced toxicity by a 5 min exposure to AMPA (50 µM + 10µM MK-801) in the presence of the AMPA receptor desensitizationinhibitor cyclothiazide (100 µM) and elevated extracellular Ca²⁺ (10 mM). Under these conditions, AMPA triggered substantial motorneuron cell loss. The presence of either FCCP or CN during the exposure attenuated this injury (Fig. 10A).

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Figure 10. Mitochondrial Ca²⁺ uptake inhibitors and antioxidants attenuate AMPA/kainate receptor-mediated motor neuron injury. A, Effects of mitochondrial toxins. Cultures were exposed to AMPA for 5 min (50 µM + 10 µM MK-801, 100 µM cyclothiazide [CYZ], and 10 mM extracellular Ca²⁺) either alone or in the additional presence of FCCP (750 nM) or cyanide (CN; 3 mM). CYZ and elevated extracellular Ca²⁺ were included during the exposure to induce substantial injury in brief exposures that minimized the direct toxic effects of FCCP and CN. The following day, injury to the overall spinal population (white bars) and the motor neuron population (black bars) was assessed as described. Values represent the means ± SEM compiled from at least four experiments; n = 16-20 cultures per condition. An asterisk indicates motor neuron cell loss significantly different from overall cell loss; an ampersand indicates motor neuron cell loss significantly different from that caused by AMPA/CYZ exposure alone (p < 0.01 by two-tailed t test). B, Effects of the antioxidant trolox. Cultures were subjected to either a prolonged (15 µM for 24 hr) or brief (100 µM for 20 min) kainate exposure (+ 10 µM MK-801), in the presence or absence of the antioxidant trolox (3 mM). (For the 20 min exposures, trolox was present for 1 hr before, during, and after the exposure.) The following day, injury to the overall spinal population (white bars) and the motor neuron population (black bars) was assessed as described (see Materials and Methods). Values represent the means ± SEM compiled from at least four experiments; n = 13-19 cultures per condition. An asterisk indicates motor neuron cell loss significantly different from overall cell loss; an ampersand indicates motor neuron cell loss significantly different from that caused by kainate exposure alone (p < 0.01 by two-tailed t test).

To test the role of ROS in AMPA/kainate receptor-mediated motor neuron injury, we performed brief (100 µM for 20 min) andprolonged (15 µM for 24 hr) kainate exposures alone or with theantioxidant trolox (a vitamin E derivative) (Chow et al., 1994).For the brief exposures, trolox (3 mM) was added for 1 hr beforeand for 24 hr after as well as during the exposure. Injury wasassessed 24 hr after the start of the exposures (see Materialand Methods). In both toxicity paradigms, trolox significantlyattenuated motor neuron cell loss (Fig. 10B).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Expression of Ca²⁺-A/K channels by motor neurons likely contributes to their high vulnerability in ALS. However, GABAergic corticalneurons, which also strongly express these channels, are not conspicuouslydamaged in human disease. The broad aim of this study thus hasbeen to compare AMPA/kainate receptor-mediated injury betweenthese two populations with the hope of uncovering clues to theparticularly high vulnerability of motor neurons in disease. Wefind that motor neurons are indeed more vulnerable than GABAergiccortical neurons to AMPA/kainate receptor-mediated injury andhave identified two differences in the injury pathway downstreamfrom Ca²⁺ entry through Ca²⁺-A/K channels that may pertain to these differences in vulnerability.First, brief AMPA or kainate exposures triggered substantial mitochondrialCa²⁺ loading in motor neurons but not in GABAergic cortical neurons.Further differences concern the agonist specificity of mitochondrialeffects. In motor neurons, brief exposures to either AMPA or kainatetriggered abrupt mitochondrial depolarization and ROS generation.In GABAergic cortical neurons, however, these effects were onlyseen with kainate exposures (which, unlike AMPA, cause nondesensitizingactivation of AMPA channels). Finally, observations that bothmitochondrial poisons (which prevent Ca²⁺ uptake) and ROS scavengers are protective suggest that the mitochondrialCa²⁺ uptake and consequent ROS generation contribute directly to AMPA/kainatereceptor-mediated motor neuroninjury.

Ca²⁺ ion entry and vulnerability of motor neurons to AMPA/kainate receptor-mediated injury

The greater vulnerability of motor neurons than GABAergic cortical neurons to AMPA/kainate receptor-mediated injury couldin part reflect a greater quantity of Ca²⁺ entering the motor neurons. Differences in agonist-triggeredCa²⁺ entry would most likely reflect differences in AMPA/kainate receptorexpression, either in terms of numbers of channels or their subunitcomposition. There is considerable evidence of strong AMPA subunitexpression on both motor neurons and GABAergic cortical neurons(Furuyama et al., 1993; Yin et al., 1994; Williams et al., 1996).Furthermore, recent studies suggesting that both motor neurons(Bar-Peled et al., 1999; Shaw et al., 1999) and GABAergic corticalneurons (Bochet et al., 1994; Jonas et al., 1994; Yin et al.,1994) may express low levels of the GluR2 AMPA subunit (whichconfers Ca²⁺ impermeability to heteromeric AMPA channels) (Hollmann et al.,1991) support the idea that Ca²⁺-A/K channels expressed on both of these populations are comprisedof AMPA subunits lacking GluR2. Further support to this idea isprovided by the present observation that the selective AMPA receptordesensitization inhibitor cyclothiazide (Yamada and Tang, 1993)strongly increased Ca²⁺-dependent AMPA-mediated injury to both of thesepopulations.

Numerous studies have confirmed that the behavior of AMPA channels is dependent both on the agonist activating the channeland on the subunit splice variants of which the channel is comprised.Although AMPA channels generally display rapid desensitizationafter activation by AMPA or the endogenous agonist glutamate,these channels undergo a relatively nondesensitizing responseafter activation by kainate (Kiskin et al., 1986; Trussell etal., 1988). Thus, the substantial mitochondrial depolarizationand ROS generation seen with kainate but not AMPA exposures inGABAergic cortical neurons likely reflect the rapid channel desensitizationafter AMPA exposures, resulting in less Ca²⁺influx.

Splice variant-dependent changes in the function of channels comprised of AMPA subunits depend primarily on the sequence atthe "flip-flop" site of the subunits; channels with the flip spliceform show much slower desensitization rates and larger steady-statecurrents than do channels composed of subunits in the flop spliceform (Sommer et al., 1990; Lambolez et al., 1996). In agreementwith the idea that slowly desensitizing AMPA channels may be expressedon motor neurons, AMPA receptor subunits present in GABAergiccortical neurons primarily exist in the flop splice form (Bochetet al., 1994; Geiger et al., 1995; Lambolez et al., 1996), whereasthose on motor neurons may primarily be in the flip splice form(Tölle et al., 1993, 1995; Jakowec et al., 1995; Temkin et al.,1997). Thus, expression of such slowly desensitizing AMPA receptorscould in part account for the observed relative lack of differencebetween the effects of AMPA and kainate on motorneurons.

Intracellular Ca²⁺ handling and the vulnerability of motor neurons to AMPA/kainate receptor-mediated injury

In addition to potential differences in the magnitude of Ca²⁺ entry, the greater vulnerability of motor neurons to AMPA/kainatereceptor-mediated injury could also reflect a greater intrinsicsusceptibility to Ca²⁺-dependent injury mechanisms, downstream from the Ca²⁺ entry. Neuronal sensitivity to Ca²⁺-mediated injury may primarily reflect the cellular mechanismsused to neutralize heavy intracellular Ca²⁺ loads. One likely relevant factor that may differentiate thesensitivity of motor neurons and GABAergic cortical neurons to[Ca²⁺]_i elevations is the presence of Ca²⁺-binding proteins (CBPs). Indeed, GABAergic interneurons are characterizedby the strong expression of CBPs including parvalbumin (Celio,1986), calretinin (Rogers, 1992), and calbindin-D28K (Hendry andJones, 1991). Recent studies suggest that CBPs may serve importantroles in protecting neurons from intracellular Ca²⁺ loads by directly chelating free intracellular Ca²⁺ (Mattson et al., 1991; Lledo et al., 1992; Lukas and Jones, 1994;Roy et al., 1998). Motor neuron subpopulations that are relativelyresistant to degeneration in ALS express high levels of CBPs,suggesting that the expression of CBPs may modulate motor neuronvulnerability (Alexianu et al., 1994; Elliott and Snider, 1995;Reiner et al., 1995). Thus, a lack of CBPs in most motor neuronsmay compel them to resort to other mechanisms, such as mitochondrialuptake, for buffering Ca²⁺ loads. Indeed, mitochondria have been found to take up Ca²⁺ after AMPA/kainate receptor activation (Hoyt et al., 1998) aswell as NMDA receptor activation (Wang et al., 1994; White andReynolds, 1997; Peng et al., 1998).

Although mitochondrial Ca²⁺ uptake may have a physiological role in the coupling of neuronal activity to mitochondrial energyproduction (McCormack and Denton, 1990), there is compelling evidencethat mitochondrial Ca²⁺ overload plays a central role in mediating excitotoxic injury(Schinder et al., 1996). Mitochondrial Ca²⁺ loading has been shown to cause loss of $Delta$ $Psi$ _m with the consequentcessation of ATP production (Beatrice et al., 1980; Wang et al.,1994). In addition, Ca²⁺ entry through either NMDA channels (Lafon-Cazal et al., 1993;Dugan et al., 1995; Reynolds and Hastings, 1995; Bindokas et al.,1996) or Ca²⁺-A/K channels (Carriedo et al., 1998) can trigger mitochondrialROS production. Recent studies demonstrating that NMDA receptor-mediatedtoxicity is attenuated by mitochondrial toxins that prevent mitochondrialCa²⁺ uptake strengthen the idea that mitochondrial Ca²⁺ loading may be a key step in the translation of excitotoxic exposureinto neuronal injury (Budd and Nicholls, 1996; Khodorov et al.,1996; Stout et al., 1998). Indeed, the present finding that eitherinhibitors of mitochondrial Ca²⁺ uptake or ROS scavengers can protect motor neurons against injuryresulting from Ca²⁺ influx through Ca²⁺-A/K channels indicates that perturbations in mitochondrial functionare central to selective AMPA/kainate receptor-mediated motorneuroninjury.

Are the present findings of relevance to ALS pathogenesis?

Mounting evidence implicates a role for excitotoxicity in the pathogenesis of sporadic ALS (Leigh and Meldrum, 1996; Rothstein,1996; Shaw and Ince, 1997). Although one must be careful in extrapolatingfindings in murine cultures to human disease, it is notable that,even across species, motor neurons in vitro and in vivo seem toexpress similar glutamate receptor profiles and vulnerabilitiesto AMPA/kainate receptor-mediated injury. Thus, to the degreethat AMPA/kainate receptor-mediated injury contributes to theloss of motor neurons in ALS, the present findings may well pertainto their high susceptibility in thedisease.

These studies suggest that a critical factor underlying the selective vulnerability of motor neurons may be their propensityto mitochondrial Ca²⁺ overload in response to Ca²⁺ entry through the Ca²⁺-A/K channels that they strongly express. Two considerations supportthe idea that these mechanisms may be well suited for the inductionof cumulative motor neuron injury that may occur in ALS. First,unlike NMDA channels, which are blocked by Mg²⁺ ions in the absence of postsynaptic depolarization, Ca²⁺-A/K channels permit direct Ca²⁺ entry whenever activated. In addition, the observation that substantialmitochondrial Ca²⁺ uptake occurs after brief exposures to the physiologically desensitizingagonist AMPA supports the possibility that similar mitochondrialCa²⁺ loading may readily occur in response to physiological synapticactivity in vivo. Disruption of mitochondrial function by Ca²⁺ may in itself be injurious to cells such as motor neurons withhigh metabolic rates. In addition, repeated mitochondrial Ca²⁺ loading and consequent ROS generation could be relevant to thefindings of mitochondrial dysfunction (Siklós et al., 1996; Beal,1998; Kong and Xu, 1998; Swerdlow et al., 1998), oxidative tissuedamage (Mecocci et al., 1993; Shaw et al., 1995; Ferrante et al.,1997), and deficiencies in glutamate uptake (Rothstein et al.,1992, 1995; Volterra et al., 1994; Trotti et al., 1999) seen inALS.

  FOOTNOTES

Received Aug. 6, 1999; revised Oct. 8, 1999; accepted Oct. 18, 1999.

This work was supported by National Institutes of Health Grants NS36548 and AG00836 (J.H.W.) and AG00919 (S.L.S.), a grantfrom the ALS Association (J.H.W.), and the National Research ServiceAward Predoctoral Fellowship HG00179 (S.G.C.). We thank SiminAmindari for her assistance in cell culture and Shyam Rao andJade Jeng for their thoughtful comments on thismanuscript.
Correspondence should be addressed to Dr. John H. Weiss, Department of Neurology, University of California, Irvine, Irvine,CA 92697-4292. E-mail: jweiss{at}uci.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alexianu ME, Ho BK, Mohamed AH, La Bella V, Smith RG, Appel SH (1994) The role of calcium-binding proteins in selective motoneuron vulnerability in amyotrophic lateral sclerosis. Ann Neurol 36:846-858[ISI][Medline].
Babcock DF, Herrington J, Goodwin PC, Park YB, Hille B (1997) Mitochondrial participation in the intracellular Ca2+ network. J Cell Biol 136:833-844[Abstract/Free Full Text].
Bar-Peled O, O'Brien RJ, Morrison JH, Rothstein JD (1999) Cultured motor neurons possess calcium-permeable AMPA/kainate receptors. NeuroReport 10:855-859[ISI][Medline].
Beal MF (1998) Mitochondrial dysfunction in neurodegenerative diseases. Biochim Biophys Acta 1366:211-223[Medline].
Beatrice MC, Palmer JW, Pfeiffer DR (1980) The relationship between mitochondrial membrane permeability, membrane potential, and the retention of Ca2+ by mitochondria. J Biol Chem 255:8663-8671[Abstract/Free Full Text].
Bindokas VP, Jordan J, Lee CC, Miller RJ (1996) Superoxide production in rat hippocampal neurons: selective imaging with hydroethidine. J Neurosci 16:1324-1336[Abstract/Free Full Text].
Bochet P, Audinat E, Lambolez B, Cr $theta$ pel F, Rossier J, Iino M, Tsuzuki K, Ozawa S (1994) Subunit composition at the single-cell level explains functional properties of a glutamate-gated channel. Neuron 12:383-388[ISI][Medline].
Bridges RJ, Stevens DR, Kahle JS, Nunn PB, Kadri M, Cotman CW (1989) Structure-function studies on N-oxaly-diamino-dicarboxylic acids and excitatory amino acid receptors: evidence that beta-L-ODAP is a selective non-NMDA agonist. J Neurosci 9:2073-2079[Abstract].
Brorson JR, Bleakman D, Chard PS, Miller RJ (1992) Calcium directly permeates kainate/alpha-amino-3-hydroxy-5-methyl-4-isoxazoleproprionic acid receptors in cultured cerebellar Purkinje neurones. Mol Pharmacol 41:603-608[Abstract].
Budd SL, Nicholls DG (1996) Mitochondria, calcium regulation, and acute glutamate excitotoxicity in cultured cerebellar granule cells. J Neurochem 67:2282-2291[ISI][Medline].
Budd SL, Castilho RF, Nicholls DG (1997) Mitochondrial membrane potential and hydroethidine-monitored superoxide generation in cultured cerebellar granule cells. FEBS Lett 415:21-24[ISI][Medline].
Carriedo SG, Yin HZ, Lamberta R, Weiss JH (1995) In vitro kainate injury to large, SMI-32(+) spinal neurons is Ca2+ dependent. NeuroReport 6:945-948[ISI][Medline].
Carriedo SG, Yin HZ, Weiss JH (1996) Motor neurons are selectively vulnerable to AMPA/kainate receptor-mediated injury in vitro. J Neurosci 16:4069-4079[Abstract/Free Full Text].
Carriedo SG, Yin HZ, Sensi SL, Weiss JH (1998) Rapid Ca²⁺ entry through Ca²⁺-permeable AMPA/kainate channels triggers marked intracellular Ca²⁺ rises and consequent oxygen radical production. J Neurosci 18:7727-7738[Abstract/Free Full Text].
Celio MR (1986) Parvalbumin in most gamma-aminobutyric acid-containing neurons of the rat cerebral cortex. Science 231:995-997[Abstract/Free Full Text].
Chow HS, Lynch JJ, Rose K, Choi DW (1994) Trolox attenuates cortical neuronal injury induced by iron, ultraviolet light, glucose deprivation, or AMPA. Brain Res 639:102-108[ISI][Medline].
Debonnel G, Beauchesne L, de Montigny C (1989) Domoic acid, the alleged "mussel toxin" might produce its neurotoxic effect through kainate receptor activation: an electrophysiological study in dorsal hippocampus. Can J Physiol Pharmacol 67:29-33[ISI][Medline].
Dugan LL, Sensi SL, Canzoniero LMT, Handran SD, Rothman SM, Lin T-S, Goldberg MP, Choi DW (1995) Mitochondrial production of reactive oxygen species in cortical neurons following exposure to N-methyl-D-aspartate. J Neurosci 15:6377-6388[Abstract/Free Full Text].
Elliott JL, Snider WD (1995) Parvalbumin is a marker of ALS-resistant motor neurons. NeuroReport 6:449-452[ISI][Medline].
Farkas DL, Wei MD, Febbroriello P, Carson JH, Loew LM (1989) Simultaneous imaging of cell and mitochondrial membrane potentials. Biophys J 56:1053-1069[Abstract/Free Full Text][Erratum(1990)57:684].
Ferrante RJ, Browne SE, Shinobu LA, Bowling AC, Baik MJ, MacGarvey U, Kowall NW, Brown RH, Beal MF (1997) Evidence of increased oxidative damage in both sporadic and familial amyotrophic lateral sclerosis. J Neurochem 69:2064-2074[ISI][Medline].
Furuyama T, Kiyama H, Sato K, Park HT, Maeno H, Takagi H, Tohyama M (1993) Region-specific expression of subunits of ionotropic glutamate receptors (AMPA-type, KA-type and NMDA receptors) in the rat spinal cord with