AMPA Receptor Current Density, Not Desensitization, Predicts Selective Motoneuron Vulnerability

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The Journal of Neuroscience, October 1, 2000, 20(19):7158-7166

AMPA Receptor Current Density, Not Desensitization, Predicts Selective Motoneuron Vulnerability
Wim Vandenberghe¹^,³, Eva C. Ihle², Doris K. Patneau², Wim Robberecht³, and James R. Brorson¹
Departments of ¹ Neurology and ² Neurobiology, Pharmacology and Physiology, The University of Chicago, Chicago, Illinois 60637, and ³ Department of Neurology, University of Leuven, 3000 Leuven, Belgium

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Spinal motoneurons are more susceptible to AMPA receptor-mediated injury than are other spinal neurons, a property that hasbeen implicated in their selective degeneration in amyotrophiclateral sclerosis (ALS). The aim of this study was to determinewhether this difference in vulnerability between motoneurons andother spinal neurons can be attributed to a difference in AMPAreceptor desensitization and/or to a difference in density offunctional AMPA receptors. Spinal motoneurons and dorsal hornneurons were isolated from embryonic rats and cultured on spinalastrocytes. Single-cell RT-PCR quantification of the relativeabundance of the flip and flop isoforms of the AMPA receptor subunits,which are known to affect receptor desensitization, did not revealany difference between the two cell populations. Examination ofAMPA receptor desensitization by patch-clamp electrophysiologicalmeasurements on nucleated and outside-out patches and in the whole-cellmode also yielded similar results for the two cell groups. However,AMPA receptor current density was two- to threefold higher inmotoneurons than in dorsal horn neurons, suggesting a higher densityof functional AMPA receptors in motoneuron membranes. Pharmacologicalreduction of AMPA receptor current density in motoneurons to thelevel found in dorsal horn neurons eliminated selective motoneuronvulnerability to AMPA receptor activation. These results suggestthat the greater AMPA receptor current density of spinal motoneuronsmay be sufficient to account for their selective vulnerabilityto AMPA receptor agonists in vitro.

Key words: amyotrophic lateral sclerosis; excitotoxicity; kainate; glutamate; kinetic; spinal cord; dorsal horn; rat; culture

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Motoneurons selectively die in amyotrophic lateral sclerosis (ALS), a fatal neurodegenerative disease. AMPA receptor-mediatedexcitotoxicity has been implicated in the selective motoneuronloss of ALS (Rothstein, 1996). Motoneurons are more vulnerableto AMPA receptor agonists than other spinal neurons, both in vivo(Hugon et al., 1989; Ikonomidou et al., 1996) and in vitro (Rothsteinet al., 1993; Carriedo et al., 1996; Bar-Peled et al., 1999; Carriedoet al., 2000; Vandenberghe et al., 2000). However, the mechanismsunderlying this selective susceptibility of spinal motoneuronsto AMPA receptor-mediated death are poorly understood. In principle,the difference in vulnerability to AMPA receptor agonists betweenmotoneurons and other spinal neurons must result from differencesin AMPA receptor expression and/or from differences in eventsoccurring "downstream" from AMPA receptor-mediated cation influx.Substantial interest has focused on the possibility that selectivemotoneuron vulnerability might result from predominant expressionof highly Ca²⁺-permeable AMPA receptors and a lack of the AMPA receptor subunitGluR2 in this cell type (Williams et al., 1997). However, we haverecently shown that there is no difference between spinal motoneuronsand dorsal horn neurons in terms of whole-cell relative Ca²⁺ permeability of AMPA receptors or relative abundance of GluR2mRNA (Vandenberghe et al., 2000).

Another property of AMPA receptors that modulates the magnitude of AMPA receptor-mediated Ca²⁺ influx and might affect vulnerability to excitotoxicity is theirdesensitization to prolonged agonist stimulation. Glutamate-inducedAMPA receptor-mediated currents rapidly desensitize in the continuedpresence of glutamate to steady-state levels far smaller thanthe peak currents (Kiskin et al., 1986; Trussell et al., 1988;Patneau and Mayer, 1991). AMPA receptor desensitization protectsneurons against the excitotoxic effects of AMPA receptor activation,as demonstrated by the fact that pharmacological reduction ofdesensitization enhances AMPA receptor-mediated neuronal death(Zorumski et al., 1990; Brorson et al., 1995; Carriedo et al.,2000). Different neuronal cell types diverge widely in the desensitizationproperties of their AMPA receptors (Raman et al., 1994; Geigeret al., 1995). This divergence in AMPA receptor desensitizationproperties arises from different expression patterns of the fourAMPA receptor subunits and their flip/flop alternative splicevariants (Sommer et al., 1990; Mosbacher et al., 1994; Geigeret al., 1995). The differences in AMPA receptor desensitizationbetween neuronal cell types could be an important determinantof selective neuronal vulnerability, as has been shown in cerebellarcultures (Brorson et al., 1995). In motoneurons, some qualitativestudies have suggested high levels of the flip splice variantsof AMPA receptor subunits, which might contribute to expressionof AMPA receptors with relatively less desensitization (Tölleet al., 1993; Jakowec et al., 1995). However, analyses of theAMPA receptor desensitization characteristics of mammalian motoneuronshave not been reported. Therefore, the first aim of the presentstudy was to test the hypothesis that motoneurons are selectivelyvulnerable to AMPA receptor agonists because their AMPA receptorsdesensitize more slowly or less completely than those of otherspinalneurons.

A second hypothesis examined in this study attributes the selective vulnerability of spinal motoneurons to the high numberor density of AMPA receptors expressed by this cell type. FunctionalAMPA receptor density (the number of functional AMPA receptorsper unit of cell surface area) can best be estimated by electrophysiologicalmeasurements of AMPA receptor current density. Our previous preliminaryevidence suggested a considerably higher AMPA receptor currentdensity in motoneurons than in spinal dorsal horn neurons (Vandenbergheet al., 2000). In the present study, we provide a detailed analysisof AMPA receptor current density in motoneurons and dorsal hornneurons and investigate the role of this parameter in selectivemotoneuronvulnerability.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell cultures
Spinal motoneurons and dorsal horn neurons were dissociated from 15-d-old Holtzmann rat embryos and cultured as describedpreviously (Vandenberghe et al., 1998, 2000). The procedures thatwere followed were in accordance with a protocol approved by theUniversity of Chicago Institutional Animal Care and Use Committee.A motoneuron-enriched neuronal population was purified from theventral spinal cord by centrifugation on a 6.5% metrizamide (Sigma,St. Louis, MO) cushion and cultured on preestablished spinal astrocyticfeeder layers. Dorsal horn neurons were dissociated from the dorsalhalf of the spinal cords of the same embryos. The preparationand culture procedures for dorsal horn neurons were the same asfor motoneurons except that the metrizamide centrifugation stepwas omitted. All cultures were kept in a 6% CO₂ humidified incubatorat 37°C. All experiments were performed on neurons after 10-13d in vitro.

Single-cell RT-PCR and restriction analysis
Aspiration of the cell content into the patch pipette, reverse transcription, and first-round PCR for quantification of therelative abundance of the four AMPA receptor subunits were performedas described previously in detail (Brorson et al., 1999; Vandenbergheet al., 2000). The relative abundance of the flip and flop splicevariants of each AMPA receptor subunit was quantified accordingto a previously published protocol (Lambolez et al., 1996; Brorsonet al., 1999), with minor modifications. In brief, bands of successfulfirst-round PCR reactions were excised from the agarose gel andpurified with the QIAquick gel extraction kit (Qiagen, Valencia,CA). The purified products of first-round PCR were subjected tosubunit-specific, second-round PCR reactions, using subunit-specificupstream primers and a common downstream primer (Brorson et al.,1999). Second-round PCR reactions were performed in a 100 µl PCRmix containing PCR buffer (Perkin-Elmer, Foster City, CA), 10pmol of each primer, 0.05 mM dNTPs (Amersham Pharmacia Biotech),2.5 U Taq polymerase (Perkin-Elmer, Norwalk, CT), and 1.5 mM MgCl₂,for 30 cycles (94°C for 30 sec, 55°C for 30 sec, 72°C for 45 sec),followed by 72°C for 10 min. For GluR4 an annealing temperatureof 60°C instead of 55°C was used. The second-round PCR productswere ethanol-precipitated and resuspended in H₂O for subsequentrestriction analysis. The specificity of the second-round PCRfor each subunit was verified for each sample by complete (>95%)digestion with a subunit-specific restriction enzyme (BglI forGluR1, Bsp1286I for GluR2, Eco47III for GluR3, and EcoRI for GluR4).Products of second-round PCR were then digested with restrictionenzymes that distinguish the flip and flop splice variants ofeach subunit. The flip/flop proportion of the GluR1 subunit wasdetermined by digesting the 634 bp GluR1 product with BfaI (whichselectively cuts GluR1 flip into fragments of 570 and 64 bp) andMseI (which selectively cuts GluR1 flop into fragments of 579and 55 bp). The 634 bp GluR2 product was digested with MseI (whichcuts GluR2 flip into fragments of 585 and 49 bp, and GluR2 flopinto fragments of 516, 69, and 49 bp), the 651 bp GluR3 fragmentwas digested with MseI (which cuts GluR3 flip into fragments of586 and 65 bp, and GluR3 flop into fragments of 518, 65, 56, and12 bp), and the 626 bp GluR4 fragment was digested with HpaI (whichselectively cuts GluR4 flop into fragments of 558 and 68 bp).HpaI digestion of GluR4 product was always performed in parallelwith HpaI digestion of a pure GluR4 flop fragment to verify completedigestion of GluR4 flop. Restriction digestions with BfaI, MseI,and HpaI were performed overnight at 37°C. The digestion productswere separated on 5% polyacrylamide gels and quantified by digitalfluorimetric scanning (corrected for lengthdifferences).

Electrophysiology
Recording from patches. For recording from membrane patches, borosilicate glass pipettes were coated with Sylgard and fire-polished.Electrodes typically had a resistance of 2-4 M $Omega$ when filled withintracellular solution, which contained (in mM): 115 CsMeSO₃,15 CsCl, 10 CsF, 10 HEPES, 5 Cs₄BAPTA, 0.5 CaCl₂, 3 MgCl₂ and2 Na₂ATP, pH 7.2 with CsOH; osmolarity 305-310 mOsm/l. Neuronswere voltage-clamped in the whole-cell configuration at $-$ 60 mVusing an Axopatch 200A amplifier (Axon Instruments, Foster City,CA) and standard techniques (Hamill et al., 1981). Nucleated macropatches(Sather et al., 1992; Patneau et al., 1993) or conventional outside-outpatches (Hamill et al., 1981) were pulled after achieving thewhole-cell configuration. All recordings from patches were madeat room temperature at a holding potential of $-$ 60 mV in an extracellularsolution containing (in mM): 145 NaCl, 3 KCl, 2 CaCl₂, 1 MgCl₂,10 HEPES, and 10 glucose, pH 7.4 with NaOH, supplemented withMK-801 (10 µM), tetrodotoxin (0.5 µM), and Cd²⁺ (100 µM) to block NMDA receptors, voltage-gated Na⁺ channels and Ca²⁺ channels, respectively. Resistance in series with the patch wastypically 4-8 M $Omega$ and was compensated by 60-90%. Data for on-linerecording were filtered at 3 kHz and sampled at 20-40 kHz usingpCLAMP (Axon Instruments).
For fast perfusion of patches, solutions were gravity fed through four-barreled, square glass tubing pulled to a width of~100 µm per barrel. The tubing was mounted on a piezo translatordriven by a 100 V power supply (PZ 100; Burleigh Instruments,Fishers, NY). A patch was positioned in the control solution stream,near the interface between control and agonist-containing solutions.The interface between solutions was rapidly moved across the patchduring charging and discharging of the piezo element. This systemachieves solution exchange on a patch in <300 µsec, as determinedfrom the 10-90% rise and decay time for a sodium concentrationchange in the presence of kainate. To apply different solutionsto the patch, the recording pipette was displaced vertically betweenthe upper and lower pair of barrels. At the end of each recording,the patch was disrupted, and junction potentials were recordedto verify the correct positioning of the patch for optimal solutionexchange (the [Na⁺] was ~6 mM lower in the control solutions). Data were excludedif the junction potentials indicated that the patch was not properlypositioned at the solutioninterface.
Whole-cell recordings. Whole-cell electrophysiological experiments were performed in the continuous single-electrode voltage-clampmode using an Axopatch 1D amplifier (Axon Instruments), as describedpreviously (Vandenberghe et al., 2000). All recordings were performedat room temperature, using unpolished borosilicate pipettes placedat the cell soma. Pipettes had a resistance of 1.8-2.5 M $Omega$ whenfilled with intracellular solution, which consisted of (in mM):120 CsF, 3 MgCl₂, 5 EGTA, and 10 HEPES, pH adjusted to 7.25 with12 mM CsOH. Ag-AgCl electrodes served as pipette electrode andground electrode. The latter was connected to the bath by meansof a 3 mM KCl-agar bridge. Cells were accepted for study if afterforming a G $Omega$ seal and breaking into the whole-cell mode a stableseal persisted with a whole-cell resistance of at least 120 M $Omega$ and a series resistance of <10 M $Omega$ . Series resistance was compensatedto ~30-40%, yielding a final, effective series resistance of <7M $Omega$ . Agonists were applied with a solenoid valve-based system viaa theta tubeapplicator.
The usual extracellular perfusion buffer was the same 145 mM Na⁺ buffer used for recording from patches. A critical issue in thesewhole-cell studies was the adequacy of voltage clamp, becauseagonist-evoked currents in 145 mM Na⁺ at holding potentials of $-$ 60 to $-$ 90 mV could exceed 5 nA in amplitude.Two different approaches were used to reduce the driving forcefor agonist-evoked currents. The first approach was to recordin 145 mM Na⁺ at a depolarized holding potential ( $-$ 10 mV); the reversal potentialof AMPA receptor-mediated currents in 145 mM Na⁺ was +12.2 ± 1.2 mV in motoneurons (n = 8) and +11.6 ± 0.7 mVin dorsal horn neurons (n = 11). The second approach was to reducethe Na⁺ concentration of the extracellular solution. Where indicated,recordings were made in 20 mM Na⁺ at $-$ 80 mV or in 10 mM Na⁺ at $-$ 90 mV. The 20 mM Na⁺ solution contained (in mM): 15.3 NaCl, 4.7 NaOH, 2 CaCl₂, 10HEPES, 10 glucose, and 228 sucrose, pH 7.4; osmolarity 315 mOsm/l;the reversal potential of AMPA receptor-mediated currents in thissolution was $-$ 43.2 ± 1.1 mV in motoneurons (n = 9) and $-$ 41.8 ±0.9 mV in dorsal horn neurons (n = 9). The 10 mM Na⁺ solution contained (in mM): 7.5 NaCl, 2.5 NaOH, 1 Ca(OH)₂, 10HEPES, 10 glucose, and 233 sucrose, pH 7.4; osmolarity 305 mOsm/l;the reversal potential of AMPA receptor-mediated currents in thissolution was $-$ 62.0 ± 1.0 mV in motoneurons (n = 7) and $-$ 62.7 ±0.6 mV in dorsal horn neurons (n = 6). By recording in 145 mMNa⁺ at $-$ 10 mV, in 20 mM Na⁺ at $-$ 80 mV, or in 10 mM Na⁺ at $-$ 90 mV, AMPA- and kainate-induced current amplitudes werereduced to <1.3 nA, so that with an effective series resistanceof <7 M $Omega$ , the resulting voltage error was <10 mV. As in the recordingsfrom patches, all extracellular solutions were supplemented withMK-801 (10 µM), tetrodotoxin (0.5 µM), and Cd²⁺ (100 µM) to block NMDA receptors, voltage-gated Na⁺ channels, and Ca²⁺ channels,respectively.
The membrane surface area of a neuron was estimated from the measurement of whole-cell capacitance. First, the residual uncompensatedpipette capacitance was calculated from the capacitative currenttransient during a 10 mV voltage step in the cell-attached modeafter formation of a G $Omega$ seal; the residual pipette capacitancewas 2.8 ± 0.1 pF (n = 155). The whole-cell capacitance was thencalculated from the capacitative transient during a 10 mV voltagestep in the whole-cell mode, after subtraction of the residualpipettecapacitance.

Toxicity experiments
Prolonged (24 hr) exposures to kainate were performed in a 6% CO₂ incubator at 37°C, using an exposure medium of L15 supplementedwith glucose (3.6 mg/ml) and sodium bicarbonate (0.15%, w/v),as described previously (Vandenberghe et al., 2000). Brief (10min) exposures to kainate were performed in room air at 37°C,using an extracellular solution with the following composition(in mM): 133 NaCl, 3 KCl, 10 CaCl₂, 1 MgCl₂, 10 HEPES, 15 glucose,and 10 mg/ml phenol red. After brief exposures, cultures werewashed twice with agonist-free exposure solution and returnedto the 37°C, 6% CO₂ incubator in the initial, complete culturemedium. The NMDA receptor antagonist MK-801 (10 µM) was addedduring all kainateexposures.
Neuronal survival was quantified, as described previously in detail (Vandenberghe et al., 2000), by morphological examinationof neurons under phase-contrast optics immediately before exposureand again 24 hr later, followed by immunostaining for the motoneuronmarkerperipherin.

Data analysis
All values and all error bars in figures denote mean ± SEM, unless indicated otherwise. Statistical analyses were performedwith SigmaStat (SSPS, Chicago, IL). Statistical significance ofdifferences was analyzed with two-tailed Student's t test forcomparison between two groups with equal variances, with Mann-Whitneyrank sum test for comparison between two groups with unequal variances,and with one-way ANOVA and Student-Newman-Keuls test for comparisonbetween more than two groups with equal variances. Differenceswere considered significant at p < 0.05.
Measurements of peak and steady-state amplitudes and kinetics were based on the average of 3-10 agonist-evoked responses.Decay time constants and rates of onset of desensitization ofpeak responses recorded from patches were fitted with one or thesum of two exponentials using a Chebyshev (pCLAMP) fitting algorithm.Dose-response curves were fitted to the Hill equation I = I_max/(1+ (EC₅₀/[agonist])ⁿ), where [agonist] is the agonist concentration, I is the currentproduced by [agonist], I_max is the maximum current at infinite[agonist], EC₅₀ is the agonist concentration producing 50% ofI_max, and n is the Hillcoefficient.

Materials
Cloned cDNA for the flip and flop forms of the four AMPA receptor subunits were gifts from Dr. Stephen Heinemann (The SalkInstitute, San Diego, CA) and Dr. Peter Seeburg (Max-Planck-Institutefor Medical Research, Heidelberg, Germany). All restriction enzymeswere purchased from New England Biolabs (Beverly, MA). GYKI 53655and cyclothiazide were gifts from Eli Lilly (Indianapolis, IN).AMPA was purchased from Tocris Cookson (Ballwin, MO) as the activeenantiomer S-AMPA. MK-801 was also obtained from Tocris Cookson.SYBR Green-1 and tetrodotoxin were purchased from Molecular Probes(Eugene, OR). Other chemicals were obtained fromSigma.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A motoneuron-enriched neuronal population from rat ventral spinal cord was cultured on a feeder layer of spinal astrocytes.Between 80 and 90% of neurons in these cultures are motoneurons,as determined by immunostaining for the motoneuron markers peripherinand SMI-32 (Fig. 1) (Vandenberghe et al., 2000). For single-cellexperiments, motoneurons were identified according to previouslydefined morphological criteria (Vandenberghe et al., 2000). Inthis study, we compared motoneurons with rat dorsal horn neuronsgrown in the same culture conditions.

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Figure 1. Motoneurons and dorsal horn neurons in culture. A, Immunostaining of motoneuron-enriched culture for the motoneuron marker peripherin on day 10 in vitro. B, Lack of peripherin immunostaining in dorsal horn neurons on day 10 in vitro. In these cultures, motoneurons and dorsal horn neurons reach a high degree of morphological differentiation. Shown are Nomarski differential interference optics images. Scale bars, 50 µm.

Expression of the flip and flop isoforms of the AMPA receptor subunits in motoneurons and dorsal horn neurons

The desensitization properties of AMPA receptors are affected by multiple molecular determinants, in particular by subunitcomposition and alternative splicing of the flip/flop region ofthe receptor subunits (Sommer et al., 1990; Mosbacher et al.,1994; Partin et al., 1994; Geiger et al., 1995; Koike et al.,2000). AMPA receptors consisting of subunits in the flip isoformdesensitize more slowly and less completely than receptors composedof flop subunits. We have previously quantified the relative abundanceof the four AMPA receptor subunits in spinal motoneurons and foundno major difference in average AMPA receptor subunit expressionpattern between this cell type and dorsal horn neurons (Vandenbergheet al., 2000). Several groups have used in situ hybridizationto qualitatively assess the expression of the flip and flop splicevariants in spinal motoneurons, with results ranging from preferentialflip isoform expression (Tölle et al., 1993; Jakowec et al.,1995) to predominant flop isoform expression (Tomiyama et al.,1996).

We have previously described an RT-PCR method that allows reliable quantification of the relative abundance of the mRNAs ofthe flip and flop splice variants in single neurons (Brorson etal., 1999). For the present study, additional control experimentswere performed, confirming the ability of this protocol to quantifythe fractional expression of the flip and flop isoforms of eachAMPA receptor subunit (Fig. 2).

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Figure 2. Validation of quantification of relative abundance of flip and flop splice variants by RT-PCR. Three control mixtures of RNAs transcribed from cDNA clones of the AMPA receptor subunits were designed to span the set of two splice variants of each of the four subunits. The composition of the mixtures is designated by shorthand representation of AMPA subunits (1i for GluR1 flip, 2o for GluR2 flop, and so forth). The RT-PCR protocol was applied to ~0.004 fmol RNA copies of each mixture to test whether ratios of flip and flop splice variants were maintained during RT-PCR. In a first step, the relative abundance of each of the four subunits was determined by first-round PCR and digestion with four subunit-specific restriction enzymes (Vandenberghe et al., 2000). Next, the relative abundance of the flip and flop splice variants of each AMPA receptor subunit was quantified by second-round, subunit-specific PCR, followed by digestion of second-round PCR products with restriction enzymes that distinguish the two splice variants of each subunit (see Materials and Methods). The digestion products were visualized on 5% polyacrylamide gels by digital fluorimetric scanning. A, Products of second-round PCR using primers specific for the subunit indicated above each lane were digested with the indicated restriction enzymes (see Materials and Methods for the length of the different digestion fragments). The RNA mixture is indicated below each gel. B, Quantification of the relative flip/flop composition of each subunit present in the control RNA mixtures by RT-PCR and restriction digestion (mean ± SD; n = 3 for each mix). The RNA mixture is indicated below each graph.

Using this single-cell RT-PCR assay, we determined the relative abundance of the flip and flop splice variants of each ofthe four AMPA receptor subunits in 11 motoneurons and 13 dorsalhorn neurons (Fig. 3). Most of these neurons (10 motoneurons and11 dorsal horn neurons) were included in the previously publishedanalysis of relative abundance of the four AMPA receptor subunits(Vandenberghe et al., 2000). In motoneurons, the flip and flopisoforms were approximately equally abundant for the subunitsGluR1, GluR3, and GluR4, whereas GluR2 was expressed predominantlyin the flop isoform (Fig. 3). Of all eight AMPA receptor subunitmRNA species in motoneurons, GluR2 flop was by far the most heavilyexpressed, accounting for approximately one-third of total AMPAreceptor subunit mRNA. No significant differences in the flip/flopratios of the four AMPA receptor subunits were found between motoneuronsand dorsal horn neurons (Fig. 3).

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Figure 3. Flip/flop alternative splicing pattern of AMPA receptor subunits in motoneurons and dorsal horn neurons. A, Fractional expression of flip and flop splice variants of AMPA receptor subunits in one motoneuron (left) and one dorsal horn neuron (right). Second-round PCR products specific for the subunit indicated above each lane were digested with the indicated restriction enzymes that distinguish the flip and flop splice variants of each subunit (see Materials and Methods for the length of the different digestion fragments). The digestion fragments were separated on 5% polyacrylamide gels and visualized by digital fluorimetric scanning. The dorsal horn neuron shown did not express GluR3 at detectable levels. B, Summary of fractional subunit and flip/flop splice variant expression in motoneurons (left; n = 11) and dorsal horn neurons (right; n = 13). There were no significant differences in relative abundance of the flip/flop splice variants between the two cell groups. Most of these neurons were included in the previously published description of relative abundance of the four AMPA receptor subunits (Vandenberghe et al., 2000). The additional cells (1 motoneuron and 2 dorsal horn neurons) did not alter the previous conclusion that no significant difference in relative abundance of GluR1-4 existed between the two cell populations.

Desensitization characteristics of AMPA receptors in motoneurons and dorsal horn neurons

The similar expression profiles of AMPA receptor subunit mRNAs and their flip/flop splice variants in motoneurons and dorsalhorn neurons suggest that AMPA receptors in the two cell populationsmay have similar desensitization properties. However, mRNA expressiondoes not necessarily reflect protein expression and assembly ofsubunits into functional receptors. We therefore performed patch-clampelectrophysiological experiments to provide a direct, functionalassessment of AMPA receptor desensitization properties in thetwo cellgroups.

The kinetics of AMPA receptor desensitization in motoneurons and dorsal horn neurons were studied using fast application ofthe physiological AMPA receptor agonist glutamate to nucleated(Sather et al., 1992; Patneau et al., 1993) and conventional (Hamillet al., 1981) outside-out membrane patches isolated from neuronalsomata. Glutamate-induced currents were recorded in the presenceof MK-801 (10 µM) to block NMDA receptors. To determine whetherkainate receptors contributed to the observed glutamate responses,currents were recorded in both the absence and presence of lanthanum(10 µM), an inhibitor of kainate receptors (Huettner et al., 1998;Li et al., 1999). Lanthanum did not produce any significant changein amplitude or time course of glutamate-induced currents, indicatingthat kainate receptors did not contribute to the observed responses(n = 11 motoneuron patches and 11 dorsal horn neuron patches;data notshown).

AMPA receptor desensitization kinetics were measured in 12 nucleated and two conventional outside-out patches from motoneurons.AMPA receptor kinetics were similar in both patch configurations.As illustrated in Figure 4A, patches from motoneurons respondedto 100 msec pulses of 3 mM glutamate with a current that roserapidly to a peak and showed rapid desensitization. The time courseof desensitization was best fitted by the sum of two exponentials,of time constants $tau$ _fast = 3.41 ± 0.84 msec and $tau$ _slow = 13.90 ±1.15 msec, with a relative amplitude of the fast component of75.0 ± 2.9%. The desensitization of AMPA receptors was extensive,with only 2.3 ± 0.5% of the peak current remaining at the endof the pulse.

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Figure 4. Desensitization and deactivation kinetics of AMPA receptors in motoneurons and dorsal horn neurons. A, B, Examples of responses evoked by 100 msec (A) and 1 msec (B) applications of 3 mM glutamate to nucleated macropatches from a motoneuron and a dorsal horn neuron, in 145 mM Na⁺ at $-$ 60 mV. The time of agonist application is indicated above each current trace by the junction potential trace recorded after disrupting the patch after recording (see Materials and Methods). C, The bar graph shows the mean time constants determined from exponential fits to data as illustrated in A and B. Desensitization kinetics were measured by fitting the decay of responses to 100 msec glutamate applications with the sum of two exponentials (n = 14 motoneurons and 14 dorsal horn neurons); $tau$ _des(fast) and $tau$ _des (slow) are the time constants of the fast and slow components of desensitization, respectively. Deactivation kinetics were determined from the decay of the response to a 1 msec application of glutamate fitted with a single exponential with time constant $tau$ _deact (n = 11 motoneurons and 9 dorsal horn neurons). There were no significant differences in the time constants of desensitization and deactivation between the two cell groups.

We also studied AMPA receptor deactivation, defined as the current decay after rapid removal of glutamate, in membrane patchesfrom 11 motoneurons. In all patches, AMPA receptor currents deactivatedrapidly after a 1 msec pulse of 3 mM glutamate (Fig. 4B). Thetime course of current deactivation was well fitted by a single-exponentialfunction with a time constant ( $tau$ ) of 1.06 ± 0.05msec.

AMPA receptor desensitization and deactivation kinetics were also measured in somatic membrane patches (eight nucleated patchesand six conventional outside-out patches) from dorsal horn neurons.AMPA receptor kinetics were again similar in both patch configurations.As in motoneuron patches, fast application of 3 mM glutamate for100 msec produced rapid and extensive desensitization in all dorsalhorn neuron patches studied (Fig. 4A). A double-exponential functionagain provided a better fit to the desensitization time coursethan a single exponential, with $tau$ _fast = 3.48 ± 0.23 msec (70.0± 2.9% of fitted amplitude) and $tau$ _slow = 12.9 ± 1.36 msec. Steady-statecurrent amplitude was 2.2 ± 0.3% of the peak amplitude. As inmotoneurons, AMPA receptor deactivation was fast and best fittedwith a single exponential, with $tau$ = 1.30 ± 0.10 msec (n = 9) (Fig.4B). None of the desensitization or deactivation parameters measuredin dorsal horn neurons were significantly different from thoseinmotoneurons.

The electrophysiological results described above reflect the properties of somatic AMPA receptors. However, somatic AMPA receptorsmay theoretically have different desensitization characteristicsthan dendritic AMPA receptors. To assess the desensitization propertiesof AMPA receptors in dendritic as well as somatic compartments,we also performed whole-cell electrophysiological experimentsin motoneurons and dorsal horn neurons. Because of the extensivedendritic arborization of the neurons, agonist application inthe whole-cell mode was not fast enough to allow accurate measurementsof AMPA receptor-mediated peak currents and of the kinetics ofAMPA receptor desensitization. However, the degree of desensitizationcan be estimated indirectly in whole-cell experiments by comparingthe amplitude of the steady-state currents elicited by saturatingconcentrations of a strongly desensitizing AMPA receptor agonist(such as AMPA or glutamate) and a weakly desensitizing AMPA receptoragonist (such as kainate) (Sommer et al., 1990; Patneau et al.,1993; Partin et al., 1994). The reported affinities of AMPA receptorsfor AMPA and kainate vary considerably between neuronal cell types;for example, the EC₅₀ of kainate at AMPA receptors ranges from80 µM in chick spinal motoneurons (O'Brien and Fischbach, 1986)to >400 µM in neurons of the chick cochlear nucleus (Raman andTrussell, 1992). To establish which concentrations of AMPA andkainate were saturating both in motoneurons and dorsal horn neurons,we measured concentration-response curves for both agonists inthe two cell groups (Fig. 5). Concentration-response analysisdemonstrated that there was no significant difference in apparentagonist affinity between motoneurons and dorsal horn neurons,and that 100 µM AMPA and 1 mM kainate were virtually saturatingconcentrations in both cell populations (Fig. 5). The specificAMPA receptor antagonist GYKI 53655 (50 µM) completely blockedthe currents evoked by 100 µM AMPA (n = 4 motoneurons and 3 dorsalhorn neurons) and by 1 mM KA (n = 4 motoneurons and 4 dorsal hornneurons), indicating that these currents were AMPA receptor-mediated(data not shown).

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Figure 5. Concentration-response relation for kainate- and AMPA-induced currents in motoneurons and dorsal horn neurons. A, Concentration-response relation for kainate-induced whole-cell steady-state currents in motoneurons () and dorsal horn neurons ( $open circle$ ). Currents were recorded in 10 mM extracellular Na⁺ at $-$ 90 mV, in response to kainate concentrations ranging from 3 µM to 3 mM, and were normalized to the responses obtained at 3 mM. Each point represents mean ± SEM of data from six cells. The Hill equation (see Materials and Methods) was used to fit the data from motoneurons (solid curve) and dorsal horn neurons (dashed curve). EC₅₀ values estimated from fits to pooled data were 106.7 µM for motoneurons and 119.6 µM for dorsal horn neurons, with Hill coefficients of 0.98 and 1.12, respectively. Insets show current traces evoked by 10 µM, 100 µM, 1 mM, and 3 mM kainate in a motoneuron (with whole-cell capacitance of 81.3 pF) and a dorsal horn neuron (with whole-cell capacitance of 20.3 pF). B, Concentration-response relation for AMPA-induced whole-cell steady-state currents in motoneurons () and dorsal horn neurons ( $open circle$ ). Currents were recorded in 20 mM extracellular Na⁺ at $-$ 80 mV, in response to AMPA concentrations ranging from 1 to 500 µM, and were normalized to the responses at 100 µM. Each point represents mean ± SEM from six to eight cells. Solid and dashed curves represent fits to pooled data from motoneurons and dorsal horn neurons, respectively. EC₅₀ values were 9.2 µM for motoneurons and 8.9 µM for dorsal horn neurons, with Hill coefficients of 1.40 and 1.44, respectively. Insets show current traces evoked by 1, 10, 100, and 500 µM AMPA in a motoneuron (with whole-cell capacitance of 61.7 pF) and a dorsal horn neuron (with whole-cell capacitance of 36.1 pF).

The ratio of the steady-state current evoked by 100 µM AMPA to the steady-state current evoked by 1 mM kainate (I_AMPA/I_KA)was determined in 10 motoneurons and nine dorsal horn neurons,in 145 mM extracellular Na⁺ at a holding potential of $-$ 10 mV (Fig. 6). There was no significantdifference in I_AMPA/I_KA between the two cell populations: I_AMPA/I_KAwas 0.22 ± 0.03 in motoneurons and 0.29 ± 0.09 in dorsal hornneurons.

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Figure 6. AMPA- and kainate-induced whole-cell currents in motoneurons and dorsal horn neurons. Whole-cell currents evoked by 100 µM AMPA and 1 mM kainate were recorded in 145 mM extracellular Na⁺ at $-$ 10 mV in a motoneuron (A) and a dorsal horn neuron (B). The motoneuron shown in A and the dorsal horn neuron shown in B had whole-cell capacitances of 121.2 and 37.1 pF, respectively.

We further compared the degree of AMPA receptor desensitization between motoneurons and dorsal horn neurons in the whole-cellmode by studying the effect of cyclothiazide, a compound thatallosterically inhibits AMPA receptor desensitization (Patneauet al., 1993; Yamada and Tang, 1993). In particular, we measuredthe ratio of peak current evoked by 100 µM AMPA in the presenceof 100 µM cyclothiazide to the steady-state current evoked by100 µM AMPA alone. In the presence of cyclothiazide, the decayof responses to AMPA is sufficiently slow to allow resolutionof the peak response in the whole-cell mode (Partin et al., 1994).The ratio of peak current evoked by AMPA in the presence of cyclothiazideto the steady-state current evoked by AMPA alone was 6.31 ± 1.18in motoneurons (n = 10) and 8.45 ± 1.63 in dorsal horn neurons(n = 9); this difference was not significant (p = 0.44).

To also measure agonist-evoked currents at more negative membrane potentials, I_AMPA/I_KA ratios and the effect of cyclothiazidewere measured at $-$ 90 mV in 10 mM extracellular Na⁺, but again showed no significant difference between the two cellgroups (data notshown).

Taken together, these electrophysiological results demonstrate that motoneurons and dorsal horn neurons do not differ fromeach other in the desensitization and deactivation propertiesof their AMPAreceptors.

AMPA receptor current density in motoneurons and dorsal horn neurons

To assess the density of functional AMPA receptors in the membranes of motoneurons and dorsal horn neurons, we recorded thecell capacitance of each neuron included in the analysis of whole-cellAMPA receptor-mediated currents described above. The capacitanceof a cell is directly proportional to the surface area of itscell membrane (Hille, 1984); the amplitude of AMPA receptor-mediatedcurrent, on the other hand, relates to the total number of functionalAMPA receptors. Therefore, AMPA receptor current density (definedas AMPA receptor-mediated current divided by capacitance) providesan estimate of functional AMPA receptordensity.

Amplitudes of whole-cell currents evoked by AMPA receptor agonists were dramatically larger in motoneurons than in dorsalhorn neurons. For example, the steady-state current evoked by3 mM kainate in 10 mM extracellular Na⁺ at $-$ 90 mV was 765.9 ± 91 pA in motoneurons (n = 12) comparedwith 72.8 ± 17.8 pA in dorsal horn neurons (n = 12) (see alsocurrent traces in Figs. 5, 6). This consistent, highly significantdifference in AMPA receptor-mediated current amplitude betweenthe two neuronal populations was considerably greater than couldbe explained by the larger membrane surface area of motoneurons,as estimated from capacitance measurements. Whole-cell capacitancetypically ranged from 60 to 140 pF in motoneurons and from 15to 45 pF in dorsal horn neurons. On average, the whole-cell capacitanceof motoneurons (95.3 ± 3.0 pF; n = 74) was approximately threefoldlarger than that of dorsal horn neurons (28.5 ± 1.0 pF; n = 74).As a result, despite a considerable variation in AMPA receptorcurrent density within each cell population (Fig. 7A), mean AMPAreceptor current density was ~2.5-fold higher in motoneurons thanin dorsal horn neurons (Fig. 7B-D). This striking difference inAMPA receptor current density between the two cell groups wasobserved with both AMPA and KA as agonists, was detected overthe full range of the agonist concentration-response curves, andwas independent of holding potential or composition of the extracellularsolution (Fig. 7B-D).

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Figure 7. AMPA receptor current density in motoneurons and dorsal horn neurons. A, Histograms summarizing distributions of AMPA receptor current density in 14 motoneurons (left) and 13 dorsal horn neurons (right). Whole-cell currents induced by 100 µM AMPA were recorded in 20 mM extracellular Na⁺ at $-$ 80 mV. B, Concentration-response curves for eight motoneurons () and seven dorsal horn neurons ( $open circle$ ) constructed from measurements of whole-cell steady-state current densities in response to AMPA concentrations ranging from 1 to 500 µM in 20 mM extracellular Na⁺ at $-$ 80 mV. C, Concentration-response curves for six motoneurons () and six dorsal horn neurons ( $open circle$ ) constructed from measurements of whole-cell steady-state current densities in response to kainate concentrations ranging from 10 µM to 3 mM in 10 mM extracellular Na⁺ at $-$ 90 mV. D, Whole-cell steady-state current density in 10 motoneurons and nine dorsal horn neurons in response to 1 mM kainate in 145 mM extracellular Na⁺ at $-$ 10 mV. In B-D, an asterisk indicates significant difference between the two cell populations.

AMPA receptor current density is a determinant of selective motoneuron vulnerability

We next performed toxicity experiments to determine to what extent the ~2.5-fold difference in AMPA receptor current densitybetween motoneurons and dorsal horn neurons could explain theirdifferential vulnerability to AMPA receptor agonists. As reportedpreviously (Vandenberghe et al., 2000), 24 hr exposure to 100µM kainate was considerably more toxic to motoneurons than todorsal horn neurons (Fig. 8A). We asked whether motoneurons wouldstill be more vulnerable to kainate than dorsal horn neurons iftheir AMPA receptor current density was reduced to the same averagelevel as in dorsal horn neurons. We used two different pharmacologicalapproaches to achieve a ~2.5-fold reduction of AMPA receptor currentdensity in motoneurons. First, we used GYKI 53655, a noncompetitiveAMPA receptor antagonist with an IC₅₀ between 1 and 1.5 µM (Bleakmanet al., 1996). In whole-cell electrophysiological experiments,1.5 µM of GYKI 53655 reduced kainate-induced current density inmotoneurons to 41.7 ± 3.13% of its control value (n = 4 motoneurons).Second, kainate concentration-response analysis (Figs. 5A, 7C)indicated that 30 µM kainate induced approximately the same currentdensity in motoneurons as did 100 µM kainate in dorsal horn neurons.Interestingly, when these treatments were applied, the toxicityinduced by 24 hr exposure of motoneurons to either 100 µM kainatewith 1.5 µM GYKI 53655 or 30 µM kainate was very similar to thetoxicity induced by 24 hr exposure of dorsal horn neurons to 100µM kainate alone (Fig. 8A). GYKI 53655 (1.5 µM) alone had no significanteffect on motoneuron survival (n = 3) (data not shown). Thesedata suggest that AMPA receptor current density may account formuch of the differential vulnerability of motoneurons and dorsalhorn neurons to AMPA receptor agonists.

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Figure 8. AMPA receptor current density is a determinant of the differential vulnerability of motoneurons and dorsal horn neurons to kainate. A, Motoneurons were exposed for 24 hr to either 100 µM kainate (KA), 30 µM kainate, or 100 µM kainate + 1.5 µM GYKI 53655; dorsal horn neurons were exposed for 24 hr to 100 µM kainate (n = 3 for each condition). MK-801 (10 µM) was added during all agonist exposures. Kainate (30 µM) and kainate (100 µM) + GYKI 53655 (1.5 µM) induce approximately the same average current density in motoneurons as does 100 µM kainate in dorsal horn neurons (see Results). An asterisk indicates motoneuron survival significantly different from the dorsal horn neuron survival after exposure to 100 µM kainate. B, Motoneurons were exposed for 10 min to either 1 mM kainate (KA), 60 µM kainate, or 1 mM kainate + 1.5 µM GYKI 53655; dorsal horn neurons were exposed for 10 min to 1 mM kainate (n = 3 for each condition). Cultures were exposed to agonist in the presence of 10 µM MK-801 and 10 mM extracellular Ca²⁺. Kainate (60 µM) and kainate (1 mM) + GYKI 53655 (1.5 µM) induce approximately the same average current density in motoneurons as does 1 mM kainate in dorsal horn neurons (see Results). An asterisk indicates motoneuron survival significantly different from the dorsal horn neuron survival after exposure to 1 mM kainate.

It has recently been reported that AMPA receptor activation can trigger removal of AMPA receptors from the plasma membraneby ligand-induced endocytosis (Carroll et al., 1999). If thisphenomenon occurred to a different degree in motoneurons thanin dorsal horn neurons, the difference in AMPA receptor currentdensity observed at the beginning of the 24 hr kainate exposurewould not be representative of the difference in current densityduring the rest of the exposure; this could confound the interpretationof the toxicity experiments described above. To minimize the chanceof major changes in AMPA receptor surface expression during agonistexposure, we also studied toxicity resulting from brief (10 min)kainate exposures. Brief exposure of motoneurons and dorsal hornneurons to 1 mM kainate in 2 mM extracellular Ca²⁺ produced little or no cell death (data not shown). However, raisingextracellular Ca²⁺ from 2 to 10 mM markedly enhanced kainate toxicity, as reportedpreviously (Carriedo et al., 1996, 2000; Van Den Bosch et al.,2000). Therefore, the toxicity experiments shown in Figure 8Bwere performed in 10 mM extracellular Ca²⁺. Motoneurons were clearly more vulnerable than dorsal horn neuronsto brief exposure to 1 mM kainate (Fig. 8B). As in the 24 hr exposures,this difference in vulnerability to kainate between the two cellpopulations was essentially eliminated by pharmacological reductionof AMPA receptor current density in motoneurons to the same averagelevel as in dorsal horn neurons (Fig. 8B).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Motoneurons are more susceptible to AMPA receptor-mediated death than other spinal neurons (Hugon et al., 1989; Rothsteinet al., 1993; Carriedo et al., 1996, 2000; Ikonomidou et al.,1996; Bar-Peled et al., 1999; Vandenberghe et al., 2000); thisobservation was confirmed in the present study. Comparing spinalmotoneurons with other spinal neurons appears to be more relevantto ALS than comparing them with neurons from nonspinal regions,because the primary pathogenic abnormalities underlying ALS maybe regionally restricted. For example, the glial glutamate transporterdefect that may be involved in the pathogenesis of a subset ofALS cases was detected in spinal cord and motor cortex but notin other CNS regions such as cerebellum or hippocampus (Rothsteinet al., 1995). We and others have shown previously that motoneuronsexpress AMPA receptors with intermediate whole-cell relative Ca²⁺ permeability (Greig et al., 2000; Vandenberghe et al., 2000).However, this property does not distinguish them from spinal dorsalhorn neurons and therefore is not sufficient to account for theirselective vulnerability (Vandenberghe et al., 2000). The aim ofthe present study was to determine whether the difference in vulnerabilitybetween motoneurons and other spinal neurons can be explainedby a difference in AMPA receptor desensitization and/or a differencein density of functional AMPAreceptors.

AMPA receptor desensitization and selective motoneuron vulnerability

This study provides the first quantitative analysis of the desensitization and deactivation properties of the AMPA receptorsof mammalian spinal motoneurons. AMPA receptors in motoneuronsconsistently exhibited fast deactivation and rapid, extensivedesensitization. AMPA receptor desensitization kinetics in ratmotoneurons were similar to those previously measured in chickspinal motoneurons (Smith et al., 1991). Deactivation and desensitizationkinetics of AMPA receptors in motoneurons also resembled AMPAreceptor kinetics in cerebellar Purkinje neurons (Raman et al.,1994; Häusser and Roth, 1997), were slower than AMPA receptorkinetics in brain stem auditory neurons (Raman and Trussell, 1992;Raman et al., 1994), and were considerably faster than in hippocampaland neocortical pyramidal neurons (Geiger et al., 1995; Sprustonet al., 1995).

Because our analysis of AMPA receptor desensitzation was based on measurements from somatic membrane patches and on whole-cellrecordings, we probably did not fully assess the desensitizationcharacteristics of AMPA receptors expressed on distal dendrites.However, a major difference in desensitization between distaldendritic and more proximal AMPA receptors seems rather unlikelyin the light of evidence that AMPA receptor desensitization inhippocampal neurons and Purkinje neurons does not differ significantlybetween somatic and distal dendritic patches (Spruston et al.,1995; Häusser and Roth, 1997).

Although the molecular control of AMPA receptor kinetics is complex and incompletely understood, subunit composition and flip/flopalternative splicing of subunits appear to be important determinantsof AMPA receptor desensitization (Sommer et al., 1990; Mosbacheret al., 1994; Partin et al., 1994; Koike et al., 2000). We havepreviously quantified the relative abundance of the AMPA receptorsubunits GluR1-4 in motoneurons by single-cell RT-PCR (Vandenbergheet al., 2000). In the present study, single-cell RT-PCR productswere used to determine the relative proportion of the flip andflop splice variants of the AMPA receptor subunits in this celltype. Motoneurons were found to express mixed proportions of mRNAsfor the flip and flop isoforms of each subunit. The flip/flopalternative splicing pattern of motoneurons is compatible withthe desensitization characteristics of their AMPA receptors: AMPAreceptor desensitization time constants and I_AMPA/I_KA ratios measuredin motoneurons were similar to those observed in host cells expressingmixtures of flip and flop splice variants (Sommer et al., 1990;Mosbacher et al., 1994; Partin et al., 1994).

The desensitization and deactivation characteristics of AMPA receptors and flip/flop alternative splicing were also studiedin dorsal horn neurons. However, dorsal horn neurons did not significantlydiffer from motoneurons in any of these parameters. The AMPA receptordesensitization time constants in dorsal horn neurons were consistentwith earlier studies on spinal neurons from chick (Trussell andFischbach, 1989).

These results lead to the conclusion that AMPA receptor desensitization cannot explain the differential vulnerability of motoneuronsand dorsal horn neurons to AMPA receptoragonists.

Functional AMPA receptor density and selective motoneuron vulnerability

To assess the density of functional AMPA receptors in motoneurons and dorsal horn neurons, we measured the density of AMPAreceptor-mediated current in neurons of both populations. We chosethis approach for several reasons: AMPA receptor current densityis a quantifiable parameter, it can be measured at the single-celllevel, and it is directly proportional to functional AMPA receptordensity and unaffected by the presence of nonfunctional AMPA receptorprotein. The present study demonstrates that AMPA receptor currentdensity is, on average, ~2.5-fold higher in motoneurons than indorsal horn neurons. This remarkable difference between the twocell groups is in agreement with earlier, preliminary observationsmade under different ionic conditions (Vandenberghe et al., 2000).

It is important to note that current density is not determined by functional AMPA receptor density alone but is also determinedby single-channel conductance and open probability of the receptors.Therefore, the observed difference in AMPA receptor current densitybetween motoneurons and dorsal horn neurons might also resultfrom differences in AMPA receptor single-channel conductance and/oropen probability between the two cell groups. AMPA receptor single-channelconductance strongly depends on subunit composition: AMPA receptorslacking GluR2 in its Q/R site-edited form exhibit a considerablyhigher conductance (Swanson et al., 1997). However, a major differencein AMPA receptor single-channel conductance based on differentialsubunit composition is unlikely to exist between motoneurons anddorsal horn neurons, given our previous finding that the relativeabundance of GluR2, the degree of Q/R site editing of GluR2, andthe whole-cell relative Ca²⁺ permeability of AMPA receptors are similar in the two cell populations(Vandenberghe et al., 2000). AMPA receptor open probability, onthe other hand, is mainly determined by receptor desensitization.In addition, AMPA receptor single-channel conductance and openprobability can be modulated by AMPA receptor phosphorylation(Derkach et al., 1999; Banke et al., 2000). Changes in AMPA receptorphosphorylation have been implicated in long-term potentiationand long-term depression in hippocampal neurons (Swope et al.,1999). However, constitutive differences in the level of AMPAreceptor phosphorylation between different neuronal cell typeshave not been reported. Therefore, the most parsimonious explanationfor the observed difference in AMPA receptor current density betweenmotoneurons and dorsal horn neurons appears to be that motoneuronsexpress a greater density of functional AMPA receptors. It remainsto be established whether the difference in whole-cell AMPA receptorcurrent density between the two populations reflects a differencein synaptic or extrasynaptic AMPA receptors, orboth.

Considerable evidence supports a link between glutamate receptor-mediated Ca²⁺ influx, intracellular Ca²⁺ accumulation, and subsequent neuronal death (Hartley et al.,1993; Lu et al., 1996). The difference in AMPA receptor currentdensity between motoneurons and dorsal horn neurons, in the absenceof a major difference in whole-cell relative Ca²⁺ permeability (Vandenberghe et al., 2000) or desensitization ofAMPA receptors, predicts that, per unit of cell membrane area,glutamate will trigger a ~2.5-fold larger AMPA receptor-mediatedCa²⁺ influx in motoneurons than in dorsal horn neurons. How does thisdifference in AMPA receptor-mediated Ca²⁺ entry per cell surface area between the two cell populationstranslate into a comparison of cytoplasmic Ca²⁺ loads, distributed throughout the cell volume? To answer thisquestion, one has to take into account the fact that motoneuronsare larger cells than dorsal horn neurons and consequently havea smaller surface/volume ratio. If motoneurons and dorsal hornneurons were spherical, the following equation would apply: (I_MN/V_MN)/(I_DH/V_DH)= [(I_MN/A_MN)/(I_DH/A_DH)]·(A_DH/A_MN)^1/2, where I is AMPA receptor-mediated current, V is cell volume,and A is cell surface area of motoneurons (MN) and dorsal hornneurons (DH). The whole-cell capacitance measurements indicatethat (A_DH/A_MN) is approximately one-third; the current densitymeasurements indicate that (I_MN/A_MN)/(I_DH/A_DH) is ~2.5. Then,according to the above equation, (I_MN/V_MN)/(I_DH/V_DH) would equal~1.44. Thus, even under the simplifying assumption of sphericalneuronal geometry, the ~2.5-fold larger AMPA receptor currentdensity in motoneurons would, during AMPA receptor activation,lead to a nearly 50% larger Ca²⁺ load per cell volume. In dendritic regions, the difference insurface/volume ratio between motoneurons and dorsal horn neuronsis likely to be considerably smaller than predicted from a sphericalmodel, producing even greater volumetric Ca²⁺ loads in motoneurons compared with dorsal horn neurons. In addition,recent functional studies indicate that the Ca²⁺ buffering capacities of spinal motoneurons are poor comparedwith those of other, less vulnerable neuronal cell types (Paleceket al., 1999). The large AMPA receptor-mediated Ca²⁺ influx in motoneurons, combined with their low Ca²⁺ buffering capacities, may explain the observation that AMPA receptoractivation triggers much larger increases in cytoplasmic [Ca²⁺] in motoneurons than in other spinal neurons (Carriedo et al.,1996, 2000). This large rise in intracellular [Ca²⁺] in motoneurons during AMPA receptor activation may lead to mitochondrialCa²⁺ overload, generation of reactive oxidant species, and cell death(Carriedo et al., 2000).

Recent work on NMDA receptor-mediated injury indicates that localized [Ca²⁺] increases in submembrane domains closely surrounding NMDA receptorsmay be more critical in the induction of toxicity than the overallcytoplasmic [Ca²⁺] increase, because of physical coupling of NMDA receptors tomolecular triggers of Ca²⁺-dependent toxicity (Sattler et al., 1999). If, similarly, certainCa²⁺-dependent neurotoxic cascades are physically located in the immediatevicinity of AMPA receptors, localized submembrane [Ca²⁺] increases might be more crucial in the induction of AMPA receptor-mediatedtoxicity than the general elevation of cytoplasmic [Ca²⁺]. Such a mechanism would further enhance the importance of AMPAreceptor current density as a predictor of AMPA receptor-mediatedtoxicity, because localized [Ca²⁺] increases in submembrane regions would correlate better withAMPA receptor-mediated Ca²⁺ entry per cell membrane area than with Ca²⁺ entry per cellvolume.

As shown in our toxicity experiments, pharmacological reduction of AMPA receptor current density in motoneurons to the sameaverage level as in dorsal horn neurons essentially eliminatesthe difference in vulnerability to AMPA receptor agonists betweenthe two cell populations. Therefore, the difference in AMPA receptorcurrent density between motoneurons and dorsal horn neurons maybe sufficient to explain their differential susceptibility toAMPA receptor-mediated injury in this culture model. To whichextent these in vitro findings can be extrapolated to the intacthuman spinal cord remains an openquestion.

In conclusion, this study demonstrates that the selective vulnerability of cultured motoneurons to AMPA receptor agonistsis determined, at least in part, at the level of AMPA receptor-mediatedion entry and suggests that the presence of a high density offunctional AMPA receptors, rather than preferential expressionof a unique AMPA receptor subtype, may account for selective motoneuronvulnerability in this model. In addition, given the evidence fora role for AMPA receptor-mediated excitotoxicity in the pathogenesisof ALS (Rothstein, 1996), the present findings may be relevantto selective motoneuron degeneration in human motoneurondisease.

  FOOTNOTES

Received May 3, 2000; revised June 30, 2000; accepted July 14, 2000.

This work was supported by the ALS Association and by National Institute of Neurological Disease and Stroke Grant NS36260(J.R.B.). W.V. is supported as Aspirant of the Fund for ScientificResearch (FWO)-Flanders and by the D. Collen Research Foundation.W.R. is supported as a Clinical Investigator of the FWO-Flanders.
Correspondence should be addressed to Dr. James R. Brorson, Department of Neurology, MC2030, The University of Chicago, 5841S. Maryland Avenue, Chicago, IL 60637. E-mail: jbrorson{at}neurology.bsd.uchicago.edu.

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RESULTS
DISCUSSION
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