Changes in calcium dynamics following the reversal of the sodium-calcium exchanger have a key role in AMPA receptor-mediated neurodegeneration via calpain activation in hippocampal neurons

Proteolytic cleavage of the Na+/Ca2+ exchanger (NCX) by calpains impairs calcium homeostasis, leading to a delayed calcium overload and excitotoxic cell death. However, it is not known whether reversal of the exchanger contributes to activate calpains and trigger neuronal death. We investigated the role of the reversal of the NCX in Ca2+ dynamics, calpain activation and cell viability, in α-amino-3-hydroxy-5-methylisoxazole-4-propionate (AMPA) receptor-stimulated hippocampal neurons. Selective overactivation of AMPA receptors caused the reversal of the NCX, which accounted for approximately 30% of the rise in intracellular free calcium concentration ([Ca2+]i). The NCX reverse-mode inhibitor, 2-[2-[4-(4-nitrobenzyloxy)phenyl]ethyl]isothiourea (KB-R7943), partially inhibited the initial increase in [Ca2+]i, and prevented a delayed increase in [Ca2+]i. In parallel, overactivation of AMPA receptors strongly activated calpains and led to the proteolysis of NCX3. KB-R7943 prevented calpain activation, cleavage of NCX3 and was neuroprotective. Silencing of NCX3 reduced Ca2+ uptake, calpain activation and was neuroprotective. Our data show for the first time that NCX reversal is an early event following AMPA receptor stimulation and is linked to the activation of calpains. Since calpain activation subsequently inactivates NCX, causing a secondary Ca2+ entry, NCX may be viewed as a new suicide substrate operating in a Ca2+-dependent loop that triggers cell death and as a target for neuroprotection.

The sodium-calcium exchanger (NCX) plays a fundamental role in controlling Na þ and Ca 2 þ homeostasis. 1,2 NCX primarily extrudes Ca 2 þ in exchange for Na þ , whereas upon neuronal depolarization, Na þ is pumped out by NCX, while Ca 2 þ is pumped in. In pathophysiological conditions, overactivation of glutamate receptors can cause the reversal of NCX, leading to Ca 2 þ entry into the cell. 3 Three NCX genes have been identified, NCX1, 4 NCX2 5 and NCX3. 6 In excitotoxic cell death, an increase in intracellular free calcium concentration ([Ca 2 þ ] i ) may directly cause activation of Ca 2 þ -dependent cysteine proteases, the calpains. Calpains modulate a variety of physiological processes, 7 and are important mediators of cell death. 8,9 Calpains mediate the neurotoxic effect of N-methyl-D-aspartate (NMDA) in cultured hippocampal neurons by a caspase-independent cell death mechanism of excitotoxicity. 10 Calpains are also involved in the neurotoxic effect caused by a-amino-3-hydroxy-5-methylisoxazole-4-propionate (AMPA) receptor activation in cultured hippocampal neurons, 11 and in hippocampal slice cultures. 12 During excitotoxic neurodegeneration, calpains are responsible for the proteolysis of several cytoskeletal and associated proteins, kinases and phosphatases, membrane receptors and transporters. 13 Recently, the involvement of calpains in the cleavage of NCX was described in cultured cerebellar granule neurons exposed to glutamate and following brain ischemia. 14 The NCX3 subtype is inactivated by proteolytic cleavage by calpains, and is no longer able to pump Ca 2 þ out of the cell, thus enhancing cell death. Furthermore, NCX3 was shown to be more relevant for cell survival than NCX1 or NCX2, namely in cultured cerebellar granule neurons. 14, 15 We recently reported that neurotoxicity induced by activation of AMPA receptors is characterized by calpain activation, lack of caspase activation, nuclear condensation/fragmentation, release of cytochrome c from mitochondria, decreased intracellular ATP levels, production of nitric oxide, moderate superoxide production and increased levels of peroxynitrite. [16][17][18] In this in vitro model of excitotoxicity, the cell death mechanisms are mostly dependent on calpains, 11 providing a good model for studying calpain-dependent phenomena. Nevertheless, it is not known whether the influx of Ca 2 þ through reversal of the exchanger is related to activation of calpains in this model, where calpains are the main executioners of cell death, and whether inhibition of this component of Ca 2 þ entry during AMPA receptor activation is neuroprotective.
In this work, we investigated whether reversal of NCX is involved in the activation of calpains in cultured hippocampal neurons, as well as in the changes in [Ca 2 þ ] i , proteolytic events and neuronal death, following selective activation of AMPA receptors.
Using single-cell analysis of the changes in [Ca 2 þ ] i by measuring Fura-2 fluorescence, we observed that exposure to KA plus CTZ for 5 min caused a mean peak increase in the fluorescence ratio of excitation (340/380) of 0.4170.03 (199 cells analysed, from three independent cultures) ( Figure 1c). KB-R7943 decreased the mean peak increase in the fluorescence ratio to 0.2570.05 (164 cells analysed, from three independent cultures) (Figure 1d), as compared to KA plus CTZ alone (Po0.05; two-tailed t-test).
Furthermore, a population of cells showed a delayed sustained increase in [Ca 2 þ ] i , starting approximately 40 min after the 5 min exposure to KA, in the presence of CTZ. In cultures treated with KA plus CTZ alone, 30.1711.9% of the cells deregulated (Figure 1c Blockade of NCX reversal prevents calpain activation. Several intracellular proteins are cleaved by calpains in a time-dependent manner during excitotoxic neurodegeneration, such as spectrin, [22][23][24][25] neuronal nitric oxide synthase (nNOS), 17 and the GluR1 subunit of AMPA receptors. 17,26 In the present study, we analyzed by Western blot the effect of inhibiting the reversal of NCX on the cleavage of spectrin, nNOS and GluR1 in cultured hippocampal neurons, after non-desensitizing activation of AMPA receptors with KA. The appearance of spectrin breakdown products (SBDPs) is a marker of calpain activity during excitotoxicity. 18,22 The specific SBDPs produced by calpain-mediated proteolysis are observed at molecular weights of approximately 145 and 150 kD (Figures 2a  and b), after the exposure of cultured hippocampal neurons to KA (100 mM), in non-desensitizing conditions (CTZ present; 30 mM). The appearance of SBDPs corresponding to caspase activity, which would have a molecular weight of 120 kD, was not observed, confirming the absence of caspase activation. KB-R7943 prevented the appearance of the 145 kD SBDPs (Figure 2a), as did the blockade of AMPA receptors by NBQX or the direct inhibition of calpains by MDL 28170 (Figure 2b).
The protein levels of the endogenous calpain substrates nNOS and GluR1 were also determined. We have shown previously that the levels of nNOS and GluR1 decrease after a 5 min exposure to KA plus CTZ (with a parallel increase in breakdown products for these proteins), and this effect is completely blocked by the calpain inhibitor MDL 28170. 17 Thus, nNOS and GluR1 levels can also be used as indicators of calpain activation in this model. nNOS levels decreased to 32.9712.7% of the control after a 5 min exposure to KA, in non-desensitizing conditions, and this effect was significantly prevented by KB-R7943 (Po0.01) (Figure 2c). GluR1 levels decreased to 49.979.9% of the control after activation of AMPA receptors. KB-R7943 also significantly inhibited this effect (Po0.01) (Figure 2d).
When the cultured hippocampal neurons were exposed to KA plus CTZ, rapid calpain activation was observed, as shown by the appearance of SBDPs as early as 1 h after the 5 min stimulation (Figure 3b). Concomitantly, a decrease in microtubule-associated protein 2 (MAP-2) labelling was observed. We previously characterized the rapid activation of calpains by MAP-2/SBDP double labelling that occurs following nondesensitizing activation of AMPA receptors, 17 starting as early as 15 min after the exposure to KA plus CTZ, and peaking at 1 h after the exposure, so this time point was chosen to be evaluated in the present study. KB-R7943 prevented the appearance of SBDPs and the loss of MAP-2 immunoreactivity Since VSCC also contribute to the entry of Ca 2 þ following activation of AMPA receptors, we addressed the question of whether blocking this pathway would also prevent calpain activation. Interestingly, nimodipine did not prevent spectrin breakdown or the appearance of SBDPs (Figure 4a). When nimodipine was added together with KB-R7943, the effect on spectrin proteolysis was similar to that of KB-R7943 alone, suggesting that only the reversal of NCX is relevant for the activation of calpains, despite the fact that a similar amount of Ca 2 þ enters hippocampal neurons by VSCC, as shown in Figure 1b. We further explored this pathway of Ca 2 þ entry and analysed cell viability 24 h following the exposure to KA plus CTZ. Nimodipine had no protective effect against the toxicity of KA plus CTZ (Figure 4b), whereas co-treatment with nimodipine and KB-R7943 together (Po0.001) had a neuroprotective effect similar to that of KB-R7943 alone (Po0.001), suggesting that VSCC are not involved in the neurodegeneration induced by activation of AMPA receptors.

Cleavage
of NCX following AMPA receptor activation. We investigated whether NCX was cleaved by calpains following non-desensitizing activation of AMPA receptors. Western blot analysis showed that NCX3, but not NCX1 or NCX2, underwent a proteolytic cleavage following exposure to KA (5 min exposure, followed by 24 h recovery), in non-desensitizing conditions (Figure 5a). KB-R7943 prevented the proteolysis of NCX3. MDL 28170 also prevented the appearance of the 60 kDa NCX3 breakdown product, suggesting that calpains are likely responsible for this phenomenon (Figure 5b). An hour after the stimulus, it Blockade of NCX by KB-R7943 prevents the neurotoxic effect of KA in non-desensitizing conditions. In order to find whether NCX plays a role following AMPA receptor activation, we next examined the potential neuroprotective effect of blocking NCX reversal during exposure to KA plus CTZ. A 5 min exposure decreased the reduction of 3-(4,5dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) to 81.871.5% of the control (Po0.001), 24 h after the exposure to the drugs (Figure 6a). In the presence of KB-R7943, the reduction of MTT following exposure to KA plus CTZ was similar to that in control conditions (90.273.2% of the control; Po0.05). KB-R7943 alone did not affect the viability of the cultures. Nuclear condensation was also evaluated as a measure of cell death. Cells showing nuclear suggesting that reversal of NCX has deleterious consequences. NBQX was used as a positive control for neuroprotection, 11 and the number of condensed nuclei was similar to control conditions. KB-R7943 is considered more selective for NCX3 than for NCX1 or NCX2. To our knowledge, there are no selective blockers of the NCX2 reverse mode, but such an inhibitor is available for NCX1. In order to better understand whether NCX1 participates in the excitotoxic cell death elicited by activation of AMPA receptors, we used SN-6, which showed improved preference for the reverse mode of NCX1. 26 In the range of 10 to 50 mM, SN-6 did not prevent cell death induced by activation of AMPA receptors (Figure 7). SN-6 (1-30 mM) also did not prevent the 45 Ca 2 þ uptake induced by KA plus CTZ, nor did it prevent calpain activation (Figure 7). These results suggest that the NCX1 subtype is not the main NCX subtype involved in the neurotoxic effect of AMPA receptor activation, thus reinforcing the possibility that NCX3 is preferentially involved in these mechanisms.
Silencing of NCX3 reduces Ca 2 þ uptake and decreases calpain activation. To confirm the preferential involvement of NCX3 in the initial Ca 2 þ influx suggested by the use of pharmacological inhibitors, NCX3 was silenced using siRNA delivery. siRNA transfection to hippocampal neurons was optimized using a non-silencing siRNA sequence conjugated with Alexa Fluor 488 (green). Cells were transfected 5 days after plating, and 48 h after the transfection procedure labelled and viable hippocampal neurons were observed, as compared to mock-transfected cultures (no siRNA) (Figure 8a). Transfection efficacy was evaluated using a control siRNA against a housekeeping control gene, GAPDH, showing that 10 nM of siRNA-GAPDH decreased GAPDH protein levels after 48 h to 50% of control (mocktransfected cells) (Figure 8b). siRNA-NCX3 (at 10 or 50 nM) decreased NCX3 protein levels by 20 and 50%, respectively ( Figure 8c). We observed that siRNA-NCX3-transfected cells had a smaller 45 Ca 2 þ uptake during exposure to KA plus CTZ (10.170.5 nmol Ca 2 þ /10 6 cells, and 9.570.4 nmol Ca 2 þ /10 6 cells, for 10 or 50 nM siRNA-NCX3, respectively; Po0.01 and Po0.001, respectively), as compared to mocktransfected cells (12.270.8 nmol Ca 2 þ /10 6 cells) (Figure 8e). Cells transfected with a non-silencing scrambled control siRNA had a 45 Ca 2 þ uptake similar to mock-transfected cells. 45 Ca 2 þ uptake in unstimulated cells was similar to all conditions.
Silencing of NCX3 also caused a decrease in spectrin proteolysis, as compared to mock-transfected cells (Figure 8d), and had a neuroprotective effect on hippocampal neurons, 24 h after the exposure to KA plus CTZ (Figure 8f). The decrease in cell viability observed in mock-transfected cells upon exposure to KA plus CTZ was significantly prevented by 50 nM siRNA-NCX3 (Po0.01, as compared to mock-transfected cells).

Discussion
In this work, we show that inhibition of the reversal of NCX reduced the initial increase in intracellular Ca 2 þ in cultured hippocampal neurons and also decreased the number of cells showing a secondary Ca 2 þ overload. The reversal of NCX activated calpains, but not caspases, and decreased cell viability upon exposure to KA, in non-desensitizing conditions. Blocking the reversal of NCX during AMPA receptor overactivation prevented the activation of calpains, the cleavage of the NCX3, and was neuroprotective. Although VSCC contribute to the initial Ca 2 þ entry during AMPA receptor stimulation, Ca 2 þ entry through VSCC does not contribute to calpain activation or cell death. Furthermore, selective In excitotoxic conditions, delayed Ca 2 þ deregulation usually develops. It is characterized by a dramatic increase in [Ca 2 þ ] i following the activation of Ca 2 þ -permeable receptors, particularly glutamate receptors, even after the stimulus has ended, thought to be due to loss of the mitochondrial ability to buffer intracellular Ca 2 þ . [28][29][30][31] More recently, it was demonstrated that, in cerebellar granule neurons, NCX also participates in this process of secondary Ca 2 þ overload, 14 due to its loss of the ability to pump Ca 2 þ out of the cell, following its proteolytic inactivation by calpains upon exposure to glutamate, providing a new hypothesis for the origin of delayed Ca 2 þ deregulation. Hoyt et al. 32 have shown in cultured rat forebrain neurons that, although reversal of NCX contributes to Ca 2 þ transients and to the immediate rise in intracellular Ca 2 þ levels upon exposure to glutamate, it has no effect in the mean peak increase caused by a prolonged exposure to glutamate nor does it contribute to neuronal injury. In Purkinje cerebellar neurons, NCX also contributes to Ca 2 þ transients upon activation of AMPA receptors, although the consequences for cell viability were not addressed. 33 Here we show, for the first time, that in conditions of selective activation of AMPA receptors, NCX contributes not only to initial Ca 2 þ influx but also to a delayed increase in intracellular Ca 2 þ , following the AMPA receptor activation in hippocampal neurons. This increase is not as dramatic as the canonical delayed Ca 2 þ deregulation but, nevertheless, a significant population of cells present a sustained increased in [Ca 2 þ ] i 30-40 min after the stimulation with KA plus CTZ.
Blockade of the reversal of NCX prevented activation of calpains, which occurs shortly after non-desensitizing activation of AMPA receptors in cultured hippocampal neurons. Calpain activation can be detected as early as 15-30 min following stimulation in this model of excitotoxicity, 11 suggesting that calpain activation occurs before the delayed increase in intracellular Ca 2 þ levels, and depends on the initial rise in Ca 2 þ . Blocking the NCX reversal only partially prevented the initial increase in [Ca 2 þ ] i , although it appears to be enough to prevent activation of calpains and, thus, protect the cells from dying. The measurement of Ca 2 þ changes and evaluation of calpain activation clearly show that blocking the reversal of NCX is essential and sufficient to prevent calpain activation and the subsequent downstream events, like the delayed increase in intracellular Ca 2 þ and the cleavage of endogenous calpain substrates like NCX3.
The present study also shows that blocking the reversal of NCX during stimulation of AMPA receptors affords neuroprotection against cell death. Inhibition of NCX reversal or silencing of NCX3 prevented the decrease in cell viability that characterizes a short-term exposure to KA plus CTZ, an effect similar to that of pharmacologically inhibiting calpains, described earlier in the same model as used in this study. 11 Blocking the reversal of NCX prevents activation of calpains, stops excitotoxic cell death upstream of the calpain proteolytic system and downstream of ionotropic glutamate receptors. Blocking either reversal of NCX or VSCC prevented Ca 2 þ entry by approximately the same extent. Reversal of NCX clearly contributes to calpain activation, but Ca 2 þ entering through VSCC does not activate calpains and has no influence in promoting cell death. This observation is in agreement with previous studies by other groups, showing that the VSCC pathway of Ca 2 þ entry is not particularly toxic to cells 34 or involved in calpain activation. 35 Ca 2 þ entering the cell by specific entry points is more efficient in triggering cell death than other pathways -source-specificity hypothesis. 36 Up to now, Ca 2 þ -permeable glutamate receptors were considered to be associated with source-specific toxicity, particularly NMDA receptors. Our study shows that AMPA receptor-mediated toxicity involves in its early stages a specific influx pathway for toxic Ca 2 þ that is not a member of the glutamate receptor family, the Na þ /Ca 2 þ exchanger, and that appears to be a key factor in committing the cells to live or die.
Several aspects of the role of NCX in neuronal physiology have recently been reviewed by others, 37 emphasizing the relevance of NCX for the regulation of neuronal [Ca 2 þ ] i and for the prevention of the pathological Ca 2 þ overload. As summarized in Figure 9, Ca 2 þ entry during activation of AMPA receptors (Figure 9a) occurs in part through the reversal of the NCX (Figure 9b) and contributes to cell death by causing activation of calpains (Figure 9c), which then leads to the cleavage of several cellular proteins, including NCX (Figure 9d), causing the secondary Ca 2 þ increase due to impaired Ca 2 þ extrusion and finally neuronal cell death. Possibly, the secondary increase in Ca 2 þ shifts calpain activation from a transitory to a sustained active state. We also show that Ca 2 þ entry through the reversal of NCX contributes more relevantly to calpain activation and cell death, than Ca 2 þ entering the cell by other pathways, such as the VSCC, showing that toxic Ca 2 þ enters the cell at specific entry points. In this model, NCX appears to work in a Ca 2 þ loop that culminates with its own proteolysis and inactivation. NCX can be considered as a new suicide substrate for calpains during excitotoxic cell death induced by activation of AMPA receptors, since its reversal triggers a chain of events that result in NCX proteolysis and inactivation, contributing to a secondary increase in [Ca 2 þ ] i (Figure 9e), and ultimately neuronal demise. Blockade of the reversal of the NCX system may be considered as a therapeutic target for neuroprotection upstream of intracellular events, following AMPA receptor overactivation in pathophysiological conditions.
Exposure of hippocampal neurons to drugs. Hippocampal neurons were exposed to KA (100 mM) and cyclothiazide (CTZ; 30 mM) for 5 min, and were allowed to recover in culture, for 24 h. Briefly, the cells were carefully washed twice with Krebs buffer (132 mM NaCl, 4 mM KCl, 1.4 mM MgCl 2 , 1 mM CaCl 2 , 6 mM glucose, 10 mM Hepes-Na, pH 7.4) after the incubation period with the drugs, and then further incubated without drugs for 24 h in supplemented Neurobasal medium. The drugs were diluted in small aliquots of conditioned medium and then added back to the correspondent well. Particularly, the calpain inhibitor MDL 28170 (50 mM), was added 15 min before, maintained throughout the incubation period and during the 24 h recovery period in supplemented Neurobasal medium. The ionotropic glutamate receptor antagonist, 2,3-dioxo-6-nitro-1,2,3,4-tetrahydrobenzoquinoxaline-7-sulphonamide (NBQX; 10 mM), SN-6 or the reversemode selective NCX inhibitor KB-R7943 (20 mM) were added during the exposure to KA plus CTZ.
Assessment of cell viability. Cell viability was assessed after exposure of cultured hippocampal neurons to drugs using either the MTT or the resazurin reduction assays. MTT, when taken up by living cells, is converted by cellular dehydrogenases from a yellow to a water-insoluble blue-coloured precipitate. 23 Briefly, Krebs buffer with MTT (0.5 mg/ml) was added to the cultures and incubated for 1 h at 371C in the incubation chamber. The precipitated dye was dissolved in 0.04 M HCl in isopropanol and spectrophotometrically (absorbance at 570 nm) quantitated. All experiments were carried out in triplicate.
Resazurin reduction was measured spectrophotometrically at 570 and 600 nm, following addition of 10% resazurin (in phosphate-buffered saline (PBS)) to the culture medium. The cultures were incubated with 10% resazurin for 2 h at 371C, in the dark, and then the media absorbance was quantified. All the experiments were carried out in duplicate (two independent wells per condition), and the results are expressed as percentage of control.
Immunocytochemistry. The culture medium was removed from the primary hippocampal cultures and the cells were washed three times with PBS, and fixed with 4% paraformaldehyde, at room temperature, for 20 min. Nonspecific binding was blocked with 3% bovine serum albumin (BSA) in PBS for 1 h. For staining of calpain-mediated SBDPs in neurons, 11 the cells were incubated with mouse anti-MAP2 (1:250), together with rabbit anti-SBDP (1:100), followed by incubation with the appropriate secondary antibodies, anti-rabbit IgG labelled with Alexa Fluor 488 (1:200) for SBDPs, and anti-mouse IgG labelled with Alexa Fluor 594 (1:200) for MAP-2, at room temperature, for 1 h. Finally, the coverslips were mounted using Dako fluorescent mounting medium. The cells were visualized using a fluorescence microscope (Axioskop 2 Plus, Zeiss) and the images were acquired with the Axiovision software 4.2.

45
Ca 2 þ uptake experiments. The entry of Ca 2 þ from the extracellular milieu into the cytosol was investigated by measurement of 45 Ca 2 þ uptake, as previously described. 25 To measure the initial Ca 2 þ uptake upon stimulation with Fura-2 fluorescence measurements by video imaging. Hippocampal neurons plated on coverslips at a density of 0.032 Â 10 6 cells/cm 2 were loaded with 5 mM Fura-2/AM and 0.02% Pluronic F-127 for 30 min at 371C in Krebs buffer supplemented with 0.1% bovine BSA (w/v). 16 After the incubation, the coverslips were rinsed with Krebs buffer and placed in a perfusion chamber on the stage of an inverted Axiovert 200 (Zeiss) fluorescence microscope, equipped with a Â 40 oil-immersion objective. The cells were then perfused with Krebs buffer for 5 min, and then stimulated with KA plus CTZ, in the presence or absence of KB-R7943, for 5 min (in Krebs buffer, also in perfusion), and then continuously perfused with Krebs buffer for 60 min. Fluorescence ratio measurements were acquired with excitation at 340 and 380 nm, and emission above 510 nm, and the data are expressed as the fluorescence ration 340/380, as described Figure 9 Cellular events in response to activation of AMPA receptors and reversal of NCX in hippocampal neurons. Activation of AMPA receptors by KA, in nondesensitizing conditions (CTZ present), causes entry of Na þ through the receptor channel, leading to membrane depolarization; this induces Ca 2 þ entry into the cell, mainly by VSCC, although some Ca 2 þ may also permeate the receptor 36 (a). In resting state, the NCX is working in the forward mode, pumping Na þ into the cell and extruding Ca 2 þ . However, due to continuous agonist binding, the Na þ concentration inside the cell becomes sufficient to revert the Na þ gradient, and then NCX starts working in the reverse mode, pumping Ca 2 þ in, in exchange for Na þ , contributing to the initial rise in intracellular Ca 2 þ levels (b). Calpains are then activated by this rise in Ca 2 þ (c), and start cleaving several of their endogenous cellular substrates, like GluR1, nNOS and NCX3, as well as a plethora of other targets (d). The cleavage of NCX by calpains impairs the process of normal calcium extrusion from the cell, and can contribute to a secondary delayed increase in intracellular Ca 2 þ , which may be released from other sources, such as the ER and the mitochondria, contributing to the overall Ca 2 þ build-up (e). In such conditions, neuronal cell death is inevitable. Blockade of the reversal of NCX with KB-R7943 (KB) decreases the initial Ca 2 þ entry (a, b), prevents calpain activation (c), cleavage of the NCX (d), the delayed Ca 2 þ increase (e) and also prevents cell death, suggesting that the contribution of NCX reversal in the initial Ca 2 þ rise is a key event in triggering the cell death cascade elsewhere. 14,29 Image analysis was performed using the software MetaFluor 5.0r2 (Universal Imaging Corporation). The neurons that showed a delayed increase of 0.07 in the 340/380 fluorescence ratio (which corresponds to an increase of 17.5% of the overall free cytosolic Ca 2 þ , compared to the maximum mean peak increase of 0.41 in the condition of KA plus CTZ alone) were considered as having a delayed increase in [Ca 2 þ ] i . siRNA transfection. To determine transfection efficacy, we used a nonsilencing Alexa Fluor 488-conjugated siRNA control, sequence AAT TCT CCG AAC GTG TCA CGT, conjugated with Alexa Fluor 488 (Qiagen, Hilden, Germany; cat. #1027284). We observed approximately 90% of transfected cells.
The siRNA against NCX3 (GenBank accession number NM_079620) was obtained as a siGENOME SMARTpool, consisting of FOUR duplexes that target different regions of the open reading frame (Dharmacon, Thermo Fisher Scientific, Lafayette, CO, USA; cat. # M-094821-00). As a negative control, a non-silencing scrambled siRNA sequence was used (siRNA Negative Control #1; Ambion Inc., cat. # 4610). siRNA-GAPDH was used as a positive control for silencing, during optimization of the transfection conditions (GAPDH siRNA; Ambion Inc., cat. # 4624).
After 5 days in culture, the hippocampal neurons were transfected with 10 or 50 pmol siRNA (NCX3), using the INTERFERin siRNA Transfection Reagent (PolyPlus Transfection Inc., San Marcos, CA, USA), following the manufacturer's instructions. In brief, siRNA and INTERFERin were mixed together in 200 ml of Neurobasal medium for 10 min. Cells were overlaid with the transfection mix for 48 h. Transfected cells were used for calcium uptake experiments, assessment of cell viability and Western blot analysis, 7 days after plating, according to the methods described above.
Data analysis. Data are expressed as means7S.E.M. Statistical significance was determined by using two-tailed t-tests, one-or two-factor analysis of variance (ANOVA), followed by Bonferroni's post-tests, as indicated in the figure legends and in the text.