Homeostatic Effects of Depolarization on Ca2+ Influx, Synaptic Signaling, and Survival

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The Journal of Neuroscience, March 1, 2003, 23(5):1825

Homeostatic Effects of Depolarization on Ca²⁺ Influx, Synaptic Signaling, and Survival
Krista L. Moulder, Robert J. Cormier, Amanda A. Shute, Charles F. Zorumski, and Steven Mennerick
Departments of Psychiatry and Neurobiology, Washington University School of Medicine, St. Louis, Missouri 63110

  ABSTRACT

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Depolarization promotes neuronal survival through moderate increases in Ca²⁺ influx, but the effects of survival-promoting depolarization(vs conventional trophic support) on neuronal signaling are poorlycharacterized. We found that chronic, survival-promoting depolarization,but not conventional trophic support, selectively decreased thesomatic Ca²⁺ current density in hippocampal and cerebellar granule neurons.Depolarization rearing depressed multiple classes of high-voltageactivated Ca²⁺ current. Consistent with the idea that these changes also affectedsynaptic Ca²⁺ channels, chronic depolarization presynaptically depressed hippocampalneurotransmission. Six days of depolarization rearing completelyabolished glutamate transmission but altered GABA transmissionin a manner consistent with the alterations of Ca²⁺ current. The continued survival of depolarization-reared neuronswas extremely sensitive to the re-establishment of basal cultureconditions and was correlated with the effects on intracellularCa²⁺ concentration. Thus, compared with cells reared on conventionaltrophic factors, depolarization evokes homeostatic changes inCa²⁺ influx and signaling that render neurons vulnerable to cell deathon activityreduction.

Key words: depolarization; HVA Ca²⁺ current; glutamate; GABA; synaptic depression; neuronal survival

  Introduction

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

During development, correlated with the period of rapid synaptogenesis, excess neurons are removed by apoptosis, or physiologicalcell death. Classical studies have indicated that limiting quantitiesof peptide neurotrophic factors (NTFs) support neuronal survivalduring this period (Burek and Oppenheim, 1996). However, for manyCNS neurons, endogenous NTFs remain undefined, and accumulatingevidence strongly suggests that electrical excitation itself,perhaps from the activity of nascent synapses, can sustain neuronalsurvival (Gallo et al., 1987; Ikonomidou et al., 1999, 2000; Verhageet al., 2000). To some extent, the intracellular survival pathwaysactivated by NTFs and electrical activity may overlap (Milleret al., 1997; Mennerick and Zorumski, 2000). However, one mightexpect phenotypic differences in the signaling properties of neuronssustained by electrical activity versus NTFs. For instance, activity-dependenthomeostatic mechanisms might influence the membrane and signalingproperties of a neuron supported by excess activity (Turrigianoet al., 1998). Alternatively, excess activity may increase electricalsignaling (Bliss and Lomo, 1973), potentially enhancing the survivaleffects ofactivity.

Moderate Ca²⁺ influx and associated rises in intracellular Ca²⁺ levels participate in activity-dependent survival in many systems(for review, see Franklin and Johnson, 1994). Also, the depressionof electrical activity with excess GABA_A receptor activation orethanol exposure results in the persistent depression of Ca²⁺ influx, changes beyond the acute actions of these drugs on membranepotential (Xu et al., 2000; Moulder et al., 2002). The depressionof Ca²⁺ current may participate in the observed neuronal death (Xu etal., 2000; Moulder et al., 2002). Here we investigated the hypothesisthat excess depolarization may result in opposite changes: anupregulation of Ca²⁺ channel function that could potentially participate in the protectionafforded by depolarization. In contrast to our expectations, depolarizationdepressed Ca²⁺ current density in hippocampal neurons and cerebellar granuleneurons, two cell types whose survival is sensitive to activity(D'Mello et al., 1993; Xu et al., 2000). Synaptic signaling wasdownregulated in a manner consistent with decreased Ca²⁺ influx into presynaptic terminals. Furthermore, the continuedsurvival of depolarization-reared neurons was more sensitive tothe re-establishment of basal culture conditions than was thesurvival of NTF-reared neurons. These results suggest that presynaptichomeostatic mechanisms shape the signaling properties of neuronswhose survival is sustained by depolarization, at the expenseof vulnerability to electricalinhibition.

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Cell culture. Hippocampal cultures were prepared from postnatal rat pups according to established protocols (Mennerick etal., 1995). Briefly, tissue was digested with papain and mechanicallydissociated before plating on a collagen-coated culture dish inEagle's medium (Invitrogen, Gaithersburg, MD) supplemented withheat-inactivated horse serum (5%), fetal calf serum (5%), 17 mMglucose, 400 µM glutamine, 50 U/ml penicillin, and 50 µg/ml streptomycin.For measurement of Ca²⁺ currents and cell death, mass cultures were plated at 2000 cells/mm². For synaptic studies, cells were plated at 100 cells/mm² on microdots of collagen to facilitate the formation of autapticconnections. Neurons plated in microcultures exhibited a depolarization-induceddecrease in Ca²⁺ current amplitude similar to that seen for mass cultures (datanot shown). In synaptic experiments only solitary neurons wereused, thus excluding polysynaptic contributions to measuredresponses.

Granule neuron culture techniques were adapted from those of Levi et al. (1984) and have been described in detail previouslyby Miller and Johnson (1996). In brief, cerebella were dissectedfrom rat pups at postnatal day 7, digested with trypsin, and mechanicallydissociated before plating at a density of 2.3 × 10⁵ cells/cm². Before plating, dishes were coated with 0.1 mg/ml poly-L-lysine.The plating medium for granule neurons consisted of Eagle's mediumcontaining 10% fetal bovine serum, with KCl added to a final concentrationof 25 mM, 100 U/ml penicillin, and 100 µg/mlstreptomycin.

Additions to the hippocampal culture medium (35 mM total K⁺, 50 ng/ml IGF-I) were made at 4 d in vitro (DIV). Ca²⁺ currents were recorded at 9-11 DIV, and synaptic responses wererecorded at 11-13 DIV. For cerebellar granule cells, medium changeswere made at 5 DIV, and Ca²⁺ currents were recorded at 8 DIV. Chlorophenylthio-cAMP (CPT-cAMP),a membrane-permeant analog of cAMP, was used as the cAMPsource.

Cell survival was quantified by an observer who was unaware of the hypotheses. Under phase-contrast optics, live neurons in10 random microscopic fields (20× objective) were counted in eachdish. Numbers refer to the number of independent platings (litters)on which the experiments wereperformed.

Electrophysiology. For recording, the culture medium was exchanged for a saline solution containing (in mM): 138 NaCl, 4 KCl,2 CaCl₂, 1 MgCl₂, 10 glucose, 10 HEPES, and 0.025 D-APV, pH 7.25.For Ca²⁺ current recordings, Ba²⁺ was used as the charge carrier to increase the current size andto improve the passive properties of the cell; a 3 mM concentrationwas used for most experiments, but 15 mM was used for experimentsexamining the contributions of Ca²⁺ channel subtypes to total current (see Fig. 2). Also, 500 nMtetrodotoxin (TTX), 1 µM 2,3-dihydroxy-6-nitro-7-sulfonyl-benzo[f]quinoxaline(NBQX), and 25 µM bicuculline were included to block sodium currentsand spontaneous synaptic currents. For the measurement of K⁺ currents, 50 µM Cd²⁺ was also present in the extracellular solution to block Ca²⁺ current and Ca²⁺-activated K⁺ current. All Ba²⁺ currents were digitally leak-subtracted using a trace obtainedin the presence of 50 µM Cd²⁺. Whole-cell recordings were obtained with pipettes 3-5 M $Omega$ forhippocampal neurons and 6-8 M $Omega$ for granule cells. For Ca²⁺ current and Na⁺ current recordings, the whole-cell pipette contained (in mM):140 cesium methanesulfonate, 4 NaCl, 0.5 CaCl₂, 5 EGTA, 10 HEPES,0.5 GTP, and 2 ATP, pH 7.25. Cells were stimulated with 30-50msec (Ca²⁺ currents) or 15 msec (Na⁺ currents) pulses to 0 mV from the holding potential of $-$ 70 mV.For potassium currents, the pipette solution contained 140 mMpotassium gluconate in place of cesium methanesulfonate, and 300msec pulses to +20 mV were used to elicit currents. Capacitancewas estimated as described previously (Xu et al., 2000; Moulderet al., 2002).

For synaptic recordings, TTX, NBQX, and bicuculline were omitted from the extracellular solution, and whole-cell pipette solutioncontained potassium chloride in place of cesium methanesulfonate.Cells were stimulated with 1.5 msec pulses to 0 mV from $-$ 70 mVto evoke transmitter release (Mennerick et al., 1995). Pairedpulses were delivered at an interval of 50 msec, and sweeps werecollected at a rate of <0.05 Hz. All results are reported as means± SEM. Paired and unpaired t tests were used to evaluate statisticalsignificance. In all instances, cells were excluded from analysisif a leak current >300 pA wasobserved.

[Ca²⁺]_i imaging. Cells were loaded with membrane permeant fura-2 AM (5 µM) for 45 min at 37°C. Cells were initially imaged instandard electrophysiology recording solution supplemented withthe relevant trophic factor (30 mM K⁺ or 100 ng/ml IGF-I). After establishing baseline [Ca²⁺]_i, cells were washed and imaged in standard recording saline,without added trophic factor. Ratiometric imaging (excitationat 340 and 380 nm) was performed on a Nikon (Tokyo, Japan) invertedmicroscope equipped with a filter wheel and intensified CCD camera.In vitro calibrations were performed as described previously (Grynkiewiczet al., 1985).

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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Decrease in Ca²⁺ current density in depolarization-reared hippocampal neurons

In cultures reared in standard serum-containing medium, 20-80% of neurons were lost between 4 and 10 DIV, depending on theplating (47 ± 15% cell loss; n = 5 platings). Nearly all neuronspresent at 4 DIV were protected by 35 mM total extracellular K⁺, which pilot work suggested was optimal (15 ± 14% cell loss between4 and 10 DIV, n = 5 platings; p < 0.05 compared with untreated).The resting membrane potential of K⁺-reared neurons, measured at 11 DIV, was $-$ 20.6 ± 1.1 mV (n = 15),depolarized from a resting potential of $-$ 47.9 ± 1.5 mV (n = 17)in cells reared in unsupplemented culturemedium.

Because the Ca²⁺ influx through high-voltage activated (HVA) Ca²⁺ channels under similar depolarizing conditions has been implicatedin depolarization-induced survival (Franklin and Johnson, 1994;Moulder et al., 2002; but see Yu et al., 1997), we examined thepersistent effects of chronic depolarization on HVA current. Theelectrical inhibition of neurons with GABAergic agents or ethanolproduced decreases in Ca²⁺ influx beyond the acute actions of the drugs (Xu et al., 2000;Moulder et al., 2002). Therefore, we initially hypothesized thatchronic depolarization might increase Ca²⁺ influx. Instead, we observed that Ca²⁺ current density, measured in recording saline with 4 mM K⁺, was smaller in K⁺-reared neurons than in untreated cells (Fig. 1A,B).

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Figure 1. Depolarization rearing specifically decreases Ca²⁺ current density in hippocampal neurons and in cerebellar granule neurons. A, Representative Ca²⁺ currents elicited by voltage steps from $-$ 70 to 0 mV in a hippocampal neuron reared in control medium and a neuron reared in medium containing 35 mM K⁺. The capacitance of the control cell was 22.0 pF, and that of the K⁺-treated cell was 22.3 pF. B, Summary of the Ca²⁺ current densities in control cultures (Ctrl), K⁺-reared cultures, and cultures reared in 50 ng/ml IGF-I. *p < 0.05 compared with control. C, Representative Na⁺ currents elicited by 15 msec voltage steps from $-$ 70 to 0 mV in a hippocampal neuron reared in control medium and a neuron reared in medium containing 35 mM K⁺. Na⁺ currents were leak-subtracted using 500 nM TTX. D, Representative K⁺ currents elicited by voltage steps from $-$ 70 to +20 mV in a hippocampal neuron reared in control medium and a neuron reared in medium containing 35 mM K⁺. Potassium currents were obtained with a potassium-based pipette solution in the presence of extracellular 50 µM Cd²⁺ and 500 nM TTX. Currents were linearly leak-subtracted. E, Scaled current-voltage relationship for Ca²⁺ currents in hippocampal neurons reared in control medium or in medium supplemented with 35 mM K⁺ or 50 ng/ml IGF-I (n = 9 for each condition). Scaled currents (I/I_p) were normalized to the peak current at 0 mV. F, Summary of the Ca²⁺ current density in cerebellar granule neuron cultures maintained in the presence of 25 mM K⁺ (K25+S), 100 ng/ml IGF-I, 800 µM CPT-cAMP, 50 µM NMDA, or 25 mM Na⁺ (plus 100 ng/ml IGF-I to promote survival). *p < 0.05 compared with 25 mM K⁺. Inset, Ca²⁺ current from a granule neuron maintained in IGF-I (left) and a granule neuron maintained in 25 mM K⁺ (right). Calibration: 100 pA, 25 msec.

As a survival control, we reared neurons in 50-100 ng/ml IGF-I, a peptide factor that promotes hippocampal survival levelssimilar to those of KCl (see Fig. 5). In IGF-I-reared cultures,there was no difference in Ca²⁺ current density compared with untreated cells (Fig. 1B). Cellcapacitance was not statistically different in KCl-reared cellscompared with untreated or IGF-I-reared cells (22.6 ± 1.5, 26.9± 3.0, and 29.9 ± 5.1 pF; n = 8-12 in each group; p > 0.1).

Other voltage-gated currents were not affected by depolarization rearing. Compared with control cultures, K⁺-reared neurons exhibited no significant difference in Na⁺ current density (Fig. 1C) (control, $-$ 165.6 ± 15.7 pA/pF; K⁺-reared, $-$ 191.6 ± 15.9 pA/pF; n = 11 in both groups; p > 0.05).Likewise, there was no difference in either peak or steady-statevoltage-gated K⁺ current density (Fig. 1D) (n = 12 control and 12 K⁺-reared neurons; p > 0.05). Thus, the downregulation of Ca²⁺ current is a relatively selective effect of K⁺depolarization.

We examined the current-voltage (I-V) curve for HVA currents reared under different conditions. The I-V relationship was similaracross experimental conditions (Fig. 1E). This result suggeststhat the change in Ca²⁺ current density did not result from a change in the voltage dependenceof activation or the reversal potential. Rather, the current decreaseoccurred at all potentials, possibly consistent with the lossof functional channels in the depolarization-rearedcells.

Ca²⁺ current density decrease in depolarization-reared granule neurons

Because the survival of cerebellar granule neurons is also enhanced by depolarization rearing, we questioned whether the effectof depolarization on Ca²⁺ current extended to these cells. Unlike hippocampal neurons,basal medium supports the survival of almost no granule neurons;these cells are absolutely dependent on added trophic factorsor depolarization for survival (D'Mello et al., 1993; Miller andJohnson, 1996). We reared granule neurons from the day of platingin 25 mM K⁺, which provides optimal protection (Gallo et al., 1987). At 5DIV, cultures were continued in 25 mM K⁺ or switched to medium containing 5 mM K⁺ and either IGF-I or cAMP (D'Mello et al., 1993). IGF-I and cAMPproduced survival that was 71.4 ± 5.3 and 78.5 ± 2.1%, respectively,of K⁺-reared cultures, evaluated at 8DIV.

Depolarization-reared granule neurons exhibited depression of Ca²⁺ current density qualitatively similar to that in hippocampalneurons (Fig. 1F). Cells raised in IGF-I plus 25 mM NaCl (as anosmotic and charge control for KCl) exhibited no decrease in Ca²⁺ current density (Fig. 1F). As expected from cell size differences,granule neuron capacitance was significantly smaller than hippocampalcell capacitance. However, depolarization-reared granule neuronsexhibited larger capacitance (8.3 ± 0.3 pF; n = 9) than IGF-I-rearedneurons (6.2 ± 0.4 pF; n = 5; p < 0.001) or cAMP-reared neurons(5.7 ± 5.7 pF; n = 5; p < 0.001). Thus, despite the larger cellsize in K⁺-reared granule neurons (compared with no detected differencein hippocampal neurons), the Ca²⁺ current density was stilldepressed.

K⁺ rearing mimics the innervation of granule neurons by glutamatergic synapses in situ (Balazs et al., 1988). Therefore, weexamined the effect of 50 µM NMDA as a depolarizing agent. NMDAproduced an intermediate level of survival (60.7 ± 4.1% of thatof 25 mM KCl; n = 3) and an intermediate level of reduction inCa²⁺ current density, although not statistically different from thereduction observed with 25 mM K⁺ (Fig. 1F). These data strongly suggest that depolarization, ratherthan some other, unanticipated, result of K⁺ rearing, caused decreased Ca²⁺ currentdensity.

To explore the Ca²⁺ channel subtype specificity of depolarization effects, we pharmacologically dissected components of HVAcurrents in granule neurons. The contributions of N, P, L, andQ/R subtypes to the total Ca²⁺ current were unchanged by K⁺ rearing versus IGF-I rearing (Fig. 2). In depolarization-rearedcells the percentages of the total Ca²⁺ current attributable to each subtype were 11, 20, 15, and 54%for P, N, L, and Q/R type currents, respectively, and were similarto values reported previously in cerebellar granule cells (Randalland Tsien, 1995). These results suggest that depression occurredacross HVA classes. This uniform effect of depolarization differsstrikingly from the preferential role of L-type Ca²⁺ channels in the survival-promoting Ca²⁺ influx that initially accompanies K⁺ depolarization (Collins and Lile, 1989; Moulder et al., 2002).However, it is consistent with reports in other systems in whichboth inactivating and noninactivating (Franklin et al., 1992)and both low-voltage activated and HVA (Li et al., 1996) Ca²⁺ currents are depressed by chronic depolarization.

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Figure 2. Multiple subtypes of HVA Ca²⁺ current are depressed by depolarization rearing. A, Representative Ca²⁺ currents elicited by steps from $-$ 70 to 0 mV in cerebellar granule neurons. Currents were recorded sequentially in the absence of any Ca²⁺ channel blockers (Baseline), in the presence of the P-type blocker $omega$ -agatoxin IVA ( $omega$ -Aga IVA; 100 nM), in the presence of the N-type blocker $omega$ -conotoxin GVIA ( $omega$ -CgTx GVIA; 1 µM), and in the presence of the L-type blocker nifedipine (5 µM). The top traces were obtained from a neuron maintained in 100 ng/ml IGF-I. The bottom traces were obtained from a neuron maintained in 25 mM K⁺ (K25+S). B, Summary of the percentage of the total current accounted for by each subtype in K⁺- and IGF-I-treated neurons. The total current was determined using an application of 50 µM Cd²⁺ (n = 9 for each condition).

K⁺ rearing and hippocampal synaptic transmission

Because K⁺ depolarization appeared to affect multiple Ca²⁺ channel subtypes, including those responsible for driving transmitterrelease, we examined whether the persistent depression of somaticCa²⁺ influx extended to hippocampal synaptic terminals (Figs. 3, 4).We examined recurrent (autaptic) synaptic signaling in solitaryhippocampal microisland neurons reared in K⁺ or with no additions. The average IPSC size was depressed by~60% in K⁺-reared cells (Fig. 3A,D). In addition, there was less IPSC paired-pulsedepression in depolarization-reared neurons (Fig. 3A,E), consistentwith a depression of the baseline probability of vesicle release(p_r) (Thomson, 2000). Interestingly, EPSCs were completely eliminatedby K⁺ rearing (Fig. 3B,C). This EPSC loss was not attributable simplyto the death of excitatory cells, because the percentage of cellswith no autaptic response increased with the loss of EPSCs indepolarization-reared cultures (Fig. 3B). Also, there was no changein the percentage of neurons immunopositive for GABA (data notshown). Similar deficits in IPSCs and EPSCs were evident with14 hr of treatment with elevated K⁺ (data not shown), suggesting that the changes in synaptic functiondid not require days of tonic depolarization.

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Figure 3. Depolarization rearing depresses synaptic transmission. A, Representative autaptic IPSCs from solitary hippocampal neurons reared in control medium or in medium containing 35 mM K⁺. Presynaptic stimulus transients have been blanked for clarity. B, Summary of the incidence of glutamatergic autapses (black columns), GABAergic autapses (white columns), and nonresponding cells (gray columns) in control and K⁺-reared cultures. Glutamatergic transmission was abolished by K⁺ rearing, whereas the percentage of nonresponding cells increased proportionally. C, The absence of glutamate transmission was associated with no detectable Ca²⁺-independent transmission. Hypertonic sucrose (500 mM) was used to elicit the release of readily releasable vesicles, causing an NBQX (1 µM)-sensitive current from a control culture (left). The same hyperosmotic challenge produced no response in a K⁺-reared cell (right) that also exhibited no action potential-evoked autaptic response (data not shown). No sucrose response was elicited in any of the 13 nonresponding K⁺-reared neurons examined. All glutamate-releasing cells in control cultures exhibited sucrose-evoked release (n = 6). D, Summary of the effect of K⁺ rearing on initial peak amplitude; *p < 0.05. E, Summary of the effect of K⁺ rearing on paired-pulse modulation (PPM); *p < 0.001. For both D and E, n > 20 for each condition.

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Figure 4. GABA synaptic depression is rescued by increasing [Ca²⁺]_o. A, Concentration-response curves for the initial peak amplitude of IPSCs recorded in hippocampal neurons maintained in control medium ( $open circle$ ) or in the presence of 35 mM K⁺ (). The solid lines represent fits to the plotted data with the Hill equation. For control cultures, the EC₅₀ value is 0.90, with a Hill coefficient of 2.31 (n = 8). For K⁺-treated cultures, the EC₅₀ value is 2.88, with a Hill coefficient of 1.46 (n = 10). B, Summary of the initial peak amplitudes of IPSCs recorded in the presence of 2 or 10 mM extracellular Ca²⁺ in both control and K⁺-treated cultures; *p < 0.01. C, Summary of the degree of paired-pulse modulation (PPM) in currents recorded in the presence of 2 or 10 mM extracellular Ca²⁺ in both control and K⁺-treated cultures; *p < 0.01.

Hypertonic solutions, which evoke the Ca²⁺-independent release of transmitter from readily releasable vesicle pools (Rosenmundand Stevens, 1996), failed to elicit EPSCs from presumed glutamatergiccells in K⁺-reared cultures (Fig. 3C). IPSCs were elicited normally by hypertonicsolution in K⁺-reared cultures (data not shown). The failure to elicit evenhypertonicity-evoked EPSCs suggests that depolarization rearingdepresses glutamate neurotransmission via mechanisms beyond thedepression of Ca²⁺ current, the focus of the present work. Therefore, we characterizedthe less severe deficit in IPSC signaling as potentially relevantto Ca²⁺-currentdepression.

If a decrease in synaptic-terminal Ca²⁺ current is responsible for the synaptic deficit in depolarization-reared neurons, depressedIPSCs might be at least partially rescued by increasing Ca²⁺ with elevated extracellular Ca²⁺. To test this, IPSCs were recorded in the presence of 0.5-10mM Ca²⁺ from potassium-reared and control neurons. Consistent with thishypothesis, the Ca²⁺ concentration response for IPSCs was significantly shifted tothe right in depolarization-reared cells, with no significantdifference in maximum response size (Fig. 4A,B). The Hill coefficientfor Ca²⁺ was slightly lower than that observed for autaptic EPSCs (Reidet al., 1998) but was within the range of cooperativity observedin other preparations (Wu et al., 1998). There was a nonsignificanttrend toward a decreased Hill coefficient in K⁺-reared cells (Fig. 4A), possibly suggesting a nonuniform depressionof Ca²⁺ influx across synaptic terminals (Reid et al., 1998). Importantly,we also overcame the deficit in paired-pulse depression by increasingCa²⁺ levels in the extracellular recording solution of depolarization-rearedcells (Fig. 4C). These data support the idea that in additionto effects on somatic Ca²⁺ influx, depolarization rearing depresses Ca²⁺-dependent neurotransmission at synapticterminals.

Depolarization rearing leaves neurons vulnerable to re-establishment of baseline culture conditions

If Ca²⁺ influx through L-type and perhaps other Ca²⁺ channels is important in the survival of neurons supported by depolarization,then depression of HVA Ca²⁺ currents might leave depolarization-reared neurons susceptibleto the re-establishment of basal culture conditions (hyperpolarizedmembrane potential and no added trophic factors). We tested thispossibility by rearing hippocampal neurons from 4 to 9 DIV in35 mM K⁺, in 50 ng/ml IGF-I, or with no additions. At 9 DIV, we countedsurviving cells. We then switched cultures to conditioned mediafrom untreated sibling cultures. We recounted cells in each condition24 hr after the switch back to basal conditions and compared survivalat the two time points. Depolarization-reared cells were significantlymore susceptible to the re-establishment of basal culture conditionsthan cells reared either in unsupplemented media or in the presenceof IGF-I (Fig. 5 A,B). The effect did not result from osmoticdifferences, because replacing KCl with NaCl at 9 DIV did notalter the results (n = 4 experiments) (data not shown).

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Figure 5. Depolarization rearing leaves neurons vulnerable to the re-establishment of baseline culture conditions. A, Effect of K⁺ depolarization or IGF-I addition on neuronal survival at 9 DIV. Survival is plotted as follows: (experimental counts)/(average control counts) $-$ 1, such that positive values represent increased survival compared with control. B, Effect of switching cultures to basal medium conditions at 9 DIV, with survival measured at 10 DIV. Survival is plotted as follows: (counts at 10 DIV)/(counts at 9 DIV) $-$ 1, such that negative values represent decreased survival compared with 9 DIV; *p < 0.001. For both A and B, n = 9. C, Changes in [Ca²⁺]_i consistent with increased vulnerability. Ca²⁺ levels, reported as fluorescence ratios at 340 and 380 nm excitation (340/380), were imaged in cultures at 10 DIV, while cells were still in either IGF-I- or K⁺-containing medium (Baseline). The cells were imaged again 10 min after the exchange of medium to standard recording solution containing no trophic support (Switch). Note that the K⁺-reared cells initially contained higher Ca²⁺ levels than IGF-I-reared cells, but levels fell to below those of IGF-I controls after trophic withdrawal (*p < 0.01; K⁺ vs IGF-I; n = 37 IGF-I cells and 48 K⁺ cells from three independent platings). Calibrated Ca²⁺ concentrations for the conditions were 78 ± 6 nM (baseline IGF), 102 ± 3 nM (baseline K⁺), 93 ± 10 nM (switch IGF), and 61 ± 3 nM (switch K⁺). Ctrl, Control.

We have shown previously that neuronal death induced by agents that depress electrical activity is associated with depressed[Ca²⁺]_i (Xu et al., 2000; Moulder et al., 2002). To determine whether[Ca²⁺]_i depression is associated with K⁺ withdrawal, we examined basal [Ca²⁺]_i levels using ratiometric fura-2 imaging in IGF-I- and K⁺-reared cells before and after K⁺ withdrawal. We found that basal [Ca²⁺]_i was elevated in K⁺-reared cells while they were maintained in elevated K⁺ (Fig. 5C). However, on withdrawal of K⁺, levels dropped below those of control (IGF-reared) cultures(Fig. 5C). These results are consistent with the idea that thedepression of Ca²⁺ current, and the resulting depression of [Ca²⁺]_i, participates in the enhanced cell death observed after K⁺withdrawal.

  Discussion

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Membrane depolarization is essential to neuronal function, apparently including the regulation of neuronal survival duringdevelopment. Because electrical activity and conventional NTFslikely produce different effects on the long-term signaling propertiesof neurons, we have begun to explore explicitly the effects ofdepolarization rearing on neuronal signaling. We find evidencefor homeostatic changes in response to tonic depolarization thathave implications for both synaptic function andsurvival.

We examined the effect of depolarization rearing on Ca²⁺ influx for two reasons. First, moderate increases in Ca²⁺ influx are implicated in the improved survival of neurons withdepolarization (Franklin and Johnson, 1994). Second, persistentdownregulation of Ca²⁺ current is implicated in inactivity-induced neuronal death (Xuet al., 2000; Moulder et al., 2002). In contrast to our expectations,we found that depolarization rearing produced robust downregulationof Ca²⁺ influx, a homeostatic response to depolarization that actuallyrendered the supported neurons more vulnerable to subsequent inhibitionthan neurons reared on peptide trophic factors. In other celltypes the depression of Ca²⁺ current with tonic depolarization has been observed in some (Franklinet al., 1992; Murrell and Tolkovsky, 1993; Li et al., 1996) butnot all (Garcia et al., 1994; Toescu, 1998) studies. Furthermore,a single study that examined depolarization and peptide growthfactors in the same system found similar depression of Ca²⁺ current with both forms of trophic support (Stewart et al., 1995).This clearly differs from our results, which suggest that depolarizationand peptide growth factors produce very different outcomes inthe signaling properties ofneurons.

In vivo, depolarization may interact with peptide trophic factors to support young neurons (Schmidt and Kater, 1993). In ourwork, 25-35 mM total K⁺ was used to depolarize neurons, in the absence of added trophicpeptides, and provide maximal survival benefit. In situ it seemslikely that more moderate depolarization and limiting quantitiesof trophic factors may act together to promote optimal survival.Accordingly, the effects on Ca²⁺ influx and signaling observed in our model systems are likelyto be more extreme than might be observed in situ. Nevertheless,our results highlight the possibility that during developmentthe nervous system may produce neurons with varied signaling propertiesby altering the proportion of depolarization used to support thecells.

How K⁺ depolarization supports survival downstream of increased [Ca²⁺]_i remains unclear, as do the intracellular pathways responsiblefor the signaling changes observed in the present study. The biochemicalcascades responsible for depolarization-induced survival may beparallel to or interact with those activated by NTFs. Some studieshave linked depolarization with an increase in NTF sensitivityor production (Ghosh et al., 1994; Meyer-Franke et al., 1995).Other studies have linked depolarization to the activation ofintracellular pathways activated by NTFs, such as the phosphatidylinositol3-kinase pathway (Miller et al., 1997) and potential downstreamtargets such as proapoptotic Bcl-2 family members, and Forkhead,a transcription factor (for review, see Datta et al., 1999). Ifsimilar pathways are indeed responsible for survival mediatedby depolarization and survival mediated by NTFs, our results suggestthat depolarization must trigger additional parallel changes,because NTF support did not cause the same signaling changes causedbydepolarization.

We found two major changes in depolarization-reared neurons predicted by the observed downregulation of Ca²⁺ influx. First, we found Ca²⁺-sensitive depression of synaptic currents in hippocampal cultures.As the most parsimonious explanation, we favor the interpretationthat increased [Ca²⁺]_o rescued the synaptic deficit in hippocampal IPSCs by compensatingfor depressed Ca²⁺ current in the presynaptic terminal. However, we cannot excludethe possibility that depolarization rearing had more direct effectson the secretory machinery, perhaps on the Ca²⁺ sensor itself. Although the effects of prolonged disuse (inactivity)on neurotransmission have been examined previously (Sharpless,1975; O'Brien et al., 1998; Turrigiano et al., 1998; Bacci etal., 2001; Luthi et al., 2001; Murthy et al., 2001), few reportshave examined the effect of depolarization on neurotransmission.One recent study found decreased postsynaptic responsiveness (Leslieet al., 2001); another reported presynaptic depression of transmission(Shi et al., 2001).

Our results also suggest severe changes in glutamate neurotransmission beyond effects that can be accounted for by changesin Ca²⁺ current. Work is underway to characterize the mechanisms of thisphenomenon and to determine whether this deficit reflects a developmentalarrest of glutamate synapse formation or a more dynamic plasticitymechanism operating on glutamate synapses. The severe depressionof glutamate neurotransmission that we observed appears to representyet another homeostatic regulatory mechanism in response to tonicdepolarization.

A second major effect of depolarization rearing was a change in the susceptibility of neurons to a return to basal cultureconditions. This vulnerability could be important physiologically.Inhibition tends to develop later than excitation in many brainareas. Thus, inhibition could actually participate in sculptingthe final numbers of neurons in the developing brain. Neuronsreared primarily on depolarization may find themselves particularlyvulnerable to apoptosis triggered by the maturation of inhibitionduringdevelopment.

  FOOTNOTES

Received Oct. 3, 2002; revised Dec. 2, 2002; accepted Dec. 9, 2002.

This work was supported by National Institutes of Health (NIH) Grants AA12952 and NS40488, by the Klingenstein Fund (S.M.),and by Grants AA12951 and MH45493 and a gift from the Bantly Foundation(C.F.Z.). K.L.M. was supported by NIH Grant 5T32DA07261. We thankAnn Benz for preparing the hippocampal cultures and members ofour laboratory for advice andcriticism.

Correspondence should be addressed to Dr. Steve Mennerick, Department of Psychiatry, Washington University School of Medicine,660 South Euclid Avenue, St. Louis, MO 63110. E-mail: menneris{at}psychiatry.wustl.edu.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

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