Abstract
The recent identification of the mitochondrial Ca2+ uniporter gene (Mcu/Ccdc109a) has enabled us to address its role, and that of mitochondrial Ca2+ uptake, in neuronal excitotoxicity. Here we show that exogenously expressed Mcu is mitochondrially localized and increases mitochondrial Ca2+ levels following NMDA receptor activation, leading to increased mitochondrial membrane depolarization and excitotoxic cell death. Knockdown of endogenous Mcu expression reduces NMDA-induced increases in mitochondrial Ca2+, resulting in lower levels of mitochondrial depolarization and resistance to excitotoxicity. Mcu is subject to dynamic regulation as part of an activity-dependent adaptive mechanism that limits mitochondrial Ca2+ overload when cytoplasmic Ca2+ levels are high. Specifically, synaptic activity transcriptionally represses Mcu, via a mechanism involving the nuclear Ca2+ and CaM kinase-mediated induction of Npas4, resulting in the inhibition of NMDA receptor-induced mitochondrial Ca2+ uptake and preventing excitotoxic death. This establishes Mcu and the pathways regulating its expression as important determinants of excitotoxicity, which may represent therapeutic targets for excitotoxic disorders.
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Introduction
For ~50 years, it has been known that mitochondria are able to take up Ca2+, achieved through the action of a membrane potential-driven carrier named the mitochondrial calcium uniporter (Mcu)1,2. The neurotoxic potential of the excitatory neurotransmitter glutamate has been appreciated for a similarly long time3. Glutamate excitotoxicity was found to be due to excessive Ca2+ influx through the NMDA subtype of glutamate receptor, and is implicated in promoting neuronal death and dysfunction in a variety of acute and chronic neurological disorders including stroke, traumatic brain injury and Huntington's disease3,4,5,6.
Many important studies into the responses of mitochondria to NMDA receptor (NMDAR) activity suggest that mitochondrial Ca2+ uptake by the uniporter has a role in excitotoxicity7,8,9. Inappropriate levels of mitochondrial Ca2+ uptake, in concert with nitric oxide production and activation of poly(ADP-ribose) polymerase-1 (PARP-1), lead to loss of mitochondrial membrane potential, which in turn energetically compromises the neuron and may lead to ROS generation7,8,9,10,11. However, a definitive answer to the question of whether mitochondrial Ca2+ uptake mediates excitotoxicity has been lacking because the molecular identity of the Mcu was not known. Early attempts to interfere with mitochondrial Ca2+ uptake in neurons indirectly involved the use of protonophores in order to depolarize the mitochondria (the membrane potential is essential for uniporter activity)12. However, this intervention can dramatically impact the cell’s bioenergetics as well as potentially triggering changes to the plasma membrane potential7. Moreover, the protective effects of prior mitochondrial depolarization are controversial13. The use of a cocktail of mitochondrial toxins to dissipate the mitochondrial membrane potential, while preventing ATP depletion, has also been employed to indirectly prevent mitochondrial Ca2+ uptake, with protective consequences14.
Pharmacological agents based on the hexavalent cation ruthenium red have also been utilized. Ruthenium red itself is able to selectively block the uniporter in isolated mitochondria, but has non-selective effects on certain ion channels in intact cells and is unable to cross the plasma membrane of many cell types15,16. The derivative Ru360 has been proposed to be more selective and cell-permeant (although there remain some doubts in these areas15,16,17). Effects of Ru360 on glutamate-induced mitochondrial depolarization have been observed11, although investigations have focussed on early events, as it is unstable in aqueous solutions (it quickly becomes oxidized). Ru360 is of limited use for long-term experiments needed to assess the role of mitochondrial Ca2+ uptake in excitotoxic cell death.
In two recent papers, the gene product encoding the uniporter channel (Mcu) was identified as the ubiquitously expressed gene previously known as Ccdc109a18,19, which acts in concert with regulatory proteins such as Micu1 and Mcur1 to mediate potential-driven mitochondrial Ca2+ uptake20,21. This finding now allows selective approaches involving exogenous Mcu expression and knockdown to be employed to determine the role of mitochondrial Ca2+ uptake in all aspects of cellular physiology and pathology.
Here we have manipulated Mcu expression in order to directly investigate the long-standing issue of a role for mitochondrial Ca2+ uptake in excitotoxicity. Overexpression and knockdown of Mcu reveals that it has an important role in mitochondrial Ca2+ uptake following NMDAR activation, as well as in subsequent cell death. Furthermore, we find that the Mcu gene is subject to dynamic regulation: it is transcriptionally repressed by neuroprotective nuclear Ca2+ signals via a mechanism involving induction of the transcriptional regulator Npas4.
Results
Mcu expression promotes neuronal mitochondrial Ca2+ uptake
Mcu is a ubiquitously expressed gene19 (although absent in yeast2) and we confirmed expression of Mcu in mouse cortical and hippocampal neurons: western analysis of whole-cell lysates using a previously validated anti-Mcu antibody18 revealed a band of expected size that was enriched in neurons over-expressing Mcu (Fig. 1a, Supplementary Fig. S1a). We employed immunofluorescence and biochemical fractionation approaches to show that Mcu fused to the fluorescent proteins eGFP or tDimer localized to neuronal mitochondria, consistent with its known subcellular distribution (Fig. 1b, Supplementary Fig. S1b and data not shown). Our overarching aim was to investigate the effect of manipulating Mcu expression on responses of forebrain neurons to NMDA treatment, focusing on mitochondrial and cytoplasmic Ca2+ increases, mitochondrial depolarization, and cell death.
Throughout the study, we present data using two complementary approaches: (a) Liposome-mediated transfection of an Mcu expression vector or Mcu-directed siRNA in mouse cortical neurons, and (b) Recombinant adeno-associated virus (rAAV)-mediated transduction of expression vectors encoding Mcu (tagged with GFP or tDimer) or Mcu-directed shRNA in mouse hippocampal neurons. The reason for the liposome-mediated transfection approach was to achieve low efficiency, enabling a direct comparison between transfected and juxtaposed untransfected cells, while the viral transduction technique was chosen for high efficiency of infection (80–90%), which facilitates ease of data analysis, particularly cell death. The two neuronal types used served to broaden the applicability of our findings.
We first studied the effect of Mcu overexpression on NMDAR-dependent increases in mitochondrial Ca2+, loss of mitochondrial membrane potential and cell death. In all Ca2+ imaging experiments we performed experiments with control and 'treated' conditions using sister cultures interleaved on the same day to control for any culture-to-culture variation in NMDA-induced Ca2+ influx. Thus, the only 'control' data shown in any particular figure are those data collected on the same day on the same culture as when the ‘treated condition’ data (for example, Mcu overexpression) were collected. As an important additional control, we verified that Mcu overexpression did not have any effect on NMDA-evoked whole-cell currents (Fig. 1c).
Rhodamine-based Ca2+ indicators are a useful tool for measuring mitochondrial Ca2+22,23, as they partition preferentially into polarized mitochondria due to their positive charge, and responses of transfected and juxtaposed untransfected cells can be analyzed. Neurons loaded with Rhod-2 showed a punctate distribution of the indicator that closely resembled that obtained with mitotracker red23 and the pattern was abolished by the mitochondrial uncoupler FCCP (Supplementary Fig. S1c), confirming a predominant mitochondrial localization of the dye. Using Rhod-2 imaging, we found that Mcu over-expressing neurons (co-transfected with an eGFP marker for identification) exhibited a larger NMDA-induced increase in [Ca2+]mit, compared with surrounding untransfected neurons (Supplementary Fig. S1d,e). In control experiments, neurons transfected with control plasmid (ß-globin) responded no differently than surrounding untransfected neurons (Supplementary Fig. S1d,e).
Although Rhod-2 imaging is well-suited for comparing the responses of adjacent transfected versus untransfected cells, its localization to mitochondria is not completely clear-cut: some cytoplasmic localization is unavoidable, potentially leading to an underestimation of the effects on mitochondrial Ca2+. We therefore complemented our Rhod-2 imaging studies with those involving a genetically encoded, mitochondrially targeted Ca2+ indicator, GCaMP2-mt24 (Fig. 1d). The GCaMP2-mt signal obtained in resting control neurons was ~30% of the maximum signal obtained by ionomycin treatment and the indicator was found to have a Fmin (obtained with ionomycin in zero Ca2+ medium) that was barely detectable over background (data not shown). Using this technique, we also found that Mcu overexpression strongly increased both basal [Ca2+]mit and NMDA-induced increases in [Ca2+]mit, compared with control-transfected neurons treated in parallel experiments (Fig. 1e–g).
We next studied the effect of Mcu overexpression on NMDA-induced mitochondrial Ca2+ uptake using an rAAV-based approach. We co-infected neurons with an rAAV containing an expression cassette for Mcu (tagged with tDimer for identification) and an rAAV containing an expression cassette for the FRET-based mitochondrial Ca2+ indicator 4mtD3cpv25. The effect of Mcu overexpression was compared with parallel experiments in which the neurons were infected with only rAAV–4mtD3cpv. The rAAV-mediated infection resulted in high efficiency (80–90%) expression of Mcu–tDimer in mouse hippocampal neurons (data not shown). Compared with parallel experiments performed on control neurons Mcu–tDimer overexpression led to enhanced elevation of [Ca2+]mit, following NMDAR activation (Fig. 1h–j). We have thus shown using independent methods of gene transfer and imaging, that Mcu overexpression in neurons leads to enhanced mitochondrial Ca2+ uptake following activation of NMDARs.
Mcu promotes NMDAR-dependent mitochondrial depolarization
A reduction of mitochondrial membrane potential (Ψm) is one of the earliest observable events in response to excitotoxic insults, and mitochondrial Ca2+ uptake is thought to be a key factor in this process11,26,27. We therefore studied the effect of manipulating Mcu expression on NMDA-induced Ψm loss, assayed using the indicator rhodamine-12310,28. We found that Mcu overexpressing neurons (co-transfected with an expression vector for mCherry for identification of the manipulated cells) exhibited a greater percentage change in rhodamine-123 signal following NMDA treatment, compared with surrounding untransfected neurons, indicative of a greater loss of Ψm (Fig. 2b, see 2a for an example experiment). In control experiments, neurons transfected with control plasmid (expression vector for ß-globin) responded no differently than surrounding untransfected neurons (Fig. 2b). Thus, overexpression of Mcu exacerbates NMDA-induced loss of Ψm, consistent with its effect on mitochondrial Ca2+ uptake.
Mcu enhances vulnerability to NMDAR-dependent excitotoxicity
We next investigated the effect of manipulating Mcu expression on the vulnerability of neurons to excitotoxic insults. Pictures of cortical neurons transfected (Lipofectamine) with control or Mcu-encoding vectors plus an eGFP marker were taken before and 24 h after a 1-h exposure to an excitotoxic dose of NMDA, and their viability scored. We found that Mcu overexpression increased the level of basal toxicity in neurons (Fig. 3a). In addition, levels of neuronal death were higher in NMDA-treated neurons over-expressing Mcu compared with control-transfected neurons (Fig. 3a). Similar results were obtained using hippocampal neurons infected with rAAV–Mcu–GFP: the expression of Mcu–GFP led to increased basal cell death rates in neurons and elevated levels of NMDA-induced cell death (Fig. 3c). For both cortical and hippocampal neurons, we additionally analyzed the above data to calculate whether Mcu overexpression made neurons more vulnerable to NMDA treatment, taking into account the increased basal death (see Methods). This revealed that Mcu makes neurons significantly more vulnerable to 20 and 30 μM NMDA in cortical neurons and more vulnerable to all doses of NMDA in hippocampal neurons (Supplementary Fig. S2a,b).
Mcu knockdown impairs Ca2+mit and is neuroprotective
We then performed loss-of-function experiments to investigate the effect of interfering with endogenous Mcu expression on NMDAR-dependent increases in mitochondrial Ca2+, loss of mitochondrial membrane potential and cell death. Two independent approaches were taken: liposome-mediated transfection of Mcu-targeted pre-made siRNA, and rAAV-mediated expression of Mcu-directed small hairpin RNA (shRNA). The efficacy of the pre-made siRNA was investigated using a high-efficiency transfection approach (nucleofection), which revealed a partial (50%) knockdown at protein and mRNA levels (Fig. 4a, Supplementary Fig. S1a) and no effect on NMDA-evoked whole-cell currents (Fig. 4c). Given the nucleofection efficiency is never greater than 70–80%, the 50% knockdown reflects a >50% knockdown in transfected cells. We found that neurons transfected with Mcu-directed siRNA exhibited a smaller NMDA-induced increase in [Ca2+]mit, assayed either using the Rhod-2 indicator and comparing the results to surrounding untransfected neurons (Supplementary Fig. S3a,b), or using GCaMP2-mt and comparing the results to control-transfected neurons (Fig. 4d-f). Neurons transfected with Mcu-directed siRNA also exhibited a smaller loss of Ψm than surrounding cells, while control-transfected neurons did not show differences compared with surrounding cells, (Fig. 4g). We then investigated whether Mcu knockdown influenced NMDA-induced excitotoxicity, and found this indeed to be the case: levels of NMDA-induced death were lower than in control-transfected cells (Fig. 4i). Moreover, we confirmed that the mitochondrial membrane potential of surviving cells (24 h after the NMDA insult) was intact and no different from control cells (Supplementary Fig. S3c). We also confirmed that the resting cytoplasmic Ca2+ concentration of surviving cells was low and no different from that of control cells (Supplementary Fig. S3d). This showed that protection due to Mcu knockdown is (as expected) associated with the long-term preservation of mitochondrial capacity and Ca2+ homeostasis. Additionally, we found that the effect of Mcu-directed siRNA on neuronal survival was abolished by overexpression of a specially engineered siRNA-resistant form of Mcu, confirming the specificity of the effect (Supplementary Fig. S3e,f). Using the rAAV-mediated expression of Mcu-directed shRNAs, we achieved a >90% knockdown of Mcu (Fig. 5a, Supplementary Fig. S1aii), which when compared with control neurons (infected with an rAAV containing an expression cassette for a scrambled control shRNA) led to a reduction in NMDA-induced [Ca2+]mit increases (Fig. 5c), a reduction in NMDA-induced mitochondrial membrane depolarization (Fig. 5f), and protection against NMDA-induced excitotoxicity (Fig. 5g).
Mcu is transcriptionally repressed by synaptic activity
It has long been known that episodes of synaptic activity can promote neuroprotection against excitotoxic insults23,29,30,31. While multiple parallel mechanisms are likely to mediate this effect, the key role of Mcu-driven mitochondrial Ca2+ uptake in excitotoxic cell death led us to investigate whether neuroprotective electrical activity influences Mcu-mediated effects. Burst activity was initiated in cortical neurons by treatment with the GABAA receptor antagonist bicuculline in the presence of the weak K+ channel blocker 4-aminopyridine (BiC/4-AP), as employed previously32,33. Consistent with previous studies, we found that BiC/4-AP pre-treatment, followed by wash-out, rendered neurons resistant to subsequently applied excitotoxic doses of NMDA (Fig. 6a). Strikingly, we also observed that the same stimulation resulted in the downregulation of Mcu expression at both protein and mRNA levels in cortical and hippocampal neurons (Fig. 6b).
This raises the exciting possibility that neuroprotective synaptic activity may actually influence the degree of mitochondrial Ca2+ uptake following subsequent NMDA treatment. Indeed, this was found to be the case: mitochondrial Ca2+ uptake during NMDA treatment was substantially reduced in BiC/4-AP pre-treated cortical neurons (Fig. 6d) and BiC pre-treated hippocampal neurons (Fig. 6e). Importantly, BiC/4-AP pre-treatment of neurons did not reduce NMDAR whole-cell currents (Supplementary Fig. S4a) and moreover, Ca2+ imaging using a non-mitochondrially targeted, cytoplasmic GCaMP2 revealed that basal and NMDA-induced cytoplasmic Ca2+ levels were not reduced by BiC/4-AP pre-treatment (Supplementary Fig. S4b). In fact, they were in both cases slightly larger, potentially a consequence of reduced mitochondrial Ca2+ uptake. Thus, compared with control, neurons that had recently experienced strong synaptic activity showed a striking difference in the relationship between cytoplasmic Ca2+ increases and subsequent mitochondrial Ca2+ uptake. Collectively these data support a model whereby prior firing activity suppresses toxic mitochondrial Ca2+ uptake following cytoplasmic Ca2+ increases, at least in part via the repression of Mcu expression. Of note, we found that forced expression of Mcu promotes increased vulnerability to excitotoxicity even in synaptically active neurons (Fig. 6f). In other words, Mcu overexpression increases the level of neuronal death to a point that is that is beyond the protective effects of synaptic activity.
Mcu is repressed by nuclear Ca2+-dependent CaM kinases
Finally, we investigated the mechanism by which synaptic activity represses Mcu expression. The observed lowering of Mcu mRNA in response to synaptic activity was suggestive of either transcriptional repression or reduced mRNA stability (that is, elevated degradation rate). We studied mRNA stability using the standard method of inhibiting transcription with Actinomycin D and harvesting RNA at multiple time points thereafter. By comparing the level of Mcu mRNA with a relatively stable mRNA (18S), one can gain a measure of mRNA degradation, and assess the influence of prior synaptic activity on this stability. An episode of prior synaptic activity had no significant difference in the decay kinetics of Mcu mRNA levels (Supplementary Fig. S5). This result strongly suggests that repression of Mcu mRNA levels is due to the repression of transcription.
We then investigated the mechanism of this transcriptional repression. We found that activity-dependent repression of Mcu was blocked by cycloheximide, indicative that de novo gene expression is required (that is, Mcu regulation is not ‘immediate-early’ in nature, Fig. 7a). Moreover, repression of Mcu by synaptic activity was blocked both by CaM kinase inhibition with KN-62 (Fig. 7b) and also by the nuclear-localized Ca2+/Calmodulin inhibitor CaMBP433,34,35 (Fig. 7c). This suggested a mechanism of Mcu repression that involved the nuclear Ca2+ and CaM kinase-dependent induction of a gene product that in turn (directly or indirectly) represses Mcu expression.
Activity-dependent Mcu repression requires Npas4 induction
Our laboratories have previously described the neuroprotective effects of nuclear Ca2+ signaling33 and also discovered a series of nuclear Ca2+-induced neuroprotective genes, five of which were found to inhibit NMDA-induced mitochondrial depolarization35. We therefore screened these genes for an ability to repress Mcu expression and found that viral overexpression of Npas4 was sufficient to repress Mcu expression (Fig. 7d). Npas4 is a transcription factor that can promote negative gene regulation in neurons36, and it is an immediate-early gene: its induction by synaptic activity was not reduced by protein synthesis inhibition (cycloheximide treatment, Fig. 7e). Indeed, superinduction in the presence of cycloheximide was observed as is common with immediate-early genes. Moreover, Npas4 induction by synaptic activity was strongly inhibited by both KN-62 and CaMBP4 (Fig. 7e), the same interventions that prevented Mcu repression (Fig. 7b). To directly test whether Npas4 induction was required for activity-dependent Mcu repression, we performed shRNA-mediated knockdown of Npas4 (Fig. 7g) and found that this inhibited activity-dependent repression of Mcu (Fig. 7h). Thus, activity-dependent Mcu repression involves the nuclear Ca2+ and CaM kinase-dependent induction of Npas4, which in turn mediates the transcriptional repression of Mcu. These data establish Npas4 as a potentially central regulator of Mcu activity in neurons.
Discussion
In this study, we used gain- and loss-of-function experiments to demonstrate the central role of the Mcu gene product in the control of mitochondrial Ca2+ uptake in neurons following an excitotoxic insult. Moreover, we established that Mcu is an important mediator of death signal-induced loss of mitochondrial membrane potential and relays NMDA receptor stimulation to excitotoxic cell loss. Intriguingly, we also find that Mcu expression and mitochondrial Ca2+ uptake are subject to dynamic regulation by neuroprotective firing activity.
Several key pro-death pathways are activated in parallel in response to an excitotoxic insult, including nitric oxide and ROS production, oxidative stress, JNK and PARP-1 activation, and CREB shut-off3,37,38,39,40. Their relative importance may depend on the cell type, developmental stage, and severity of insult. Nevertheless, in most scenarios, it is likely that more than one pathway is important and that pathways can interact with each other. Future studies on Mcu-driven Ca2+ uptake will tell us what role this process has in several key pro-death cascades. For example, mitochondrial Ca2+ uptake is implicated in the activation of PARP-1 via mitochondrial ROS generation, which combine with NO to trigger ONOO−-mediated DNA damage, the trigger for PARP-1 activation11,41,42. Moreover, mitochondrial Ca2+ uptake and ROS production have also been implicated in JNK activation43. Another important issue surrounds the contribution of factors other than mitochondrial Ca2+ uptake in mitochondrial membrane depolarization. The coupling of the GluN2B C-terminal domain to downstream cell death pathways, including nitric oxide production, contributes to excitotoxicity3,44,45,46, and excitotoxic mitochondrial depolarization via Ca2+ uptake has been reported to involve nitric oxide10,47. Nitric oxide sensitizes mitochondria to Ca2+-dependent depolarization10, raising the possibility that it affects mitochondrial energy metabolism, Mcu activity itself, or even efflux via the mitochondrial Na+/Ca2+ exchanger. PARP-1 has also been shown to contribute to excitotoxic mitochondrial depolarization, likely via depletion of NADH levels11. Despite the existence of multiple mechanisms leading to excitotoxicity, it is thus apparent that there is crosstalk between pathways and that mitochondrial dysfunction is a convergent hub for some and an upstream effector for others. In seeking to minimize neuronal death and dysfunction in excitotoxic disorders such as stroke, targeting multiple sites of control may be optimal. One can envisage that targeting upstream (big effect, short therapeutic window) as well as downstream (smaller effect, longer window) events could be more effective than any one strategy. Future studies will help to illuminate and clarify these issues.
It will also be of interest to determine whether and how mitochondrial Ca2+ uptake contributes to the differential effects of synaptic versus extrasynaptic NMDAR activity28,38. Extrasynaptic NMDAR activity is particularly well-coupled to mitochondrial depolarization28, and Ca2+ influx triggered by bath activation of NMDARs is more strongly coupled to mitochondrial Ca2+ uptake than influx through other routes27. It is tempting to speculate that physical proximity of extrasynaptic NMDARs to mitochondria may contribute to this. Given the relatively low affinity and huge Ca2+-carrying capacity of the uniporter1 (half-saturation reached at 20 mM Ca2+), Ca2+ uptake may be substantially enhanced if mitochondria are positioned extremely near the site of Ca2+ entry where local Ca2+ levels are high. Synaptic NMDARs may be somewhat shielded from close proximity to mitochondria by the post-synaptic density, and more significantly by the fact that dendritic spines rarely contain mitochondria48. It will also be important to determine whether other mitochondrial Ca2+ transporters such as Letm1 or uncoupling proteins contribute in any way in neurons49,50, and which Mcu regulatory proteins (for example, Micu1/2 and Mcur1) are important. We occasionally observed biphasic kinetics in the increase of [Ca2+]mit (for example, see Fig. 1i), potentially indicating functionally different uptake mechanisms.
Our findings suggest that pharmacological modulation of Mcu offers a realistic therapeutic target for excitotoxic injury, as ischemia-induced excitotoxicity is likely to develop over a relatively long timescale. Interference with early events in the excitotoxic cascade can yield protective outcomes, such as those employing NMDAR antagonists, and PSD-95 and JNK inhibitors3,37,43,46,51. Now that the molecular machinery of the Mcu has been identified18,19, and its role in excitotoxicity established (this study), screens for small molecules that inhibit Mcu activity may lead to novel neuroprotective compounds. Of course, the appropriateness of the Mcu as a therapeutic target needs to be assessed in the light of all its physiological role(s). Evidence supports the notion that mitochondrial Ca2+ controls mitochondrial energy metabolism, including in neurons52,53. The impact of interfering with Mcu activity on these processes awaits further investigation, although we note from the current study that Mcu knockdown has no adverse effects on basal viability.
Our observations that Mcu is subject to transcriptional repression by neuroprotective Ca2+ signals may reflect an important facet of Mcu’s function in the cell. As Mcu-mediated mitochondrial Ca2+ overload contributes to mitochondrial dysfunction and neuronal death in response to excitotoxic insults, repression of Mcu expression by Ca2+ signals may represent a potentially important feedback mechanism acting to prevent mitochondrial Ca2+ overload, (potentially in concert with other mechanisms54). It is tempting to speculate that this mechanism enables a cell to tune its Mcu activity to reflect cytoplasmic Ca2+ levels, and that Mcu transcriptional repression is an important factor in Ca2+-dependent tolerance/preconditioning mechanisms.
Protection against excitotoxic insults by Ca2+-dependent transcriptional changes has centered mainly on the Ca2+ responsive transcription factors involved. Induction of CREB-mediated transcription and inhibition of FOXO-mediated gene expression have been shown to contribute to protection against excitotoxic insults by neuroprotective Ca2+ signals29,31. Our observation that repression of Mcu expression underlies an important part of the anti-excitotoxic effects of sub-toxic Ca2+ signals demonstrates that a central effector of excitotoxicity is under direct control by neuroprotective pathways. Furthermore, we have demonstrated that this repression is a delayed response to the immediate-early induction of Npas4, although whether Npas4 is acting directly on the Mcu promoter in an inhibitory capacity or acting indirectly (for example, by inducing the expression of a repressor) awaits further investigation. Given that the MCU gene is also subject to Ca2+-mediated transcriptional repression in human ESC-derived neurons (Qiu and Hardingham, unpublished observations), a search for phylogenetically conserved elements within the Mcu promoter may yield the sequences responsible for mediating Ca2+ sensitivity.
To conclude, we have established Mcu both as an effector of excitotoxic cell death and a target of neuroprotective signals. Exploiting these facts may lead to new interventions aimed at ameliorating neuronal dysfunction and death in disorders associated with aberrant NMDAR activity.
Methods
Neuronal culture
Hippocampal and cortical neurons from newborn C57Bl/6 mice (sex not determined) were cultured and maintained as described previously33,35. Neurons were cultured in Neurobasal media (Invitrogen, Gaithersburg, MD, USA) containing 1% rat serum and B27 (Invitrogen), and penicillin/streptomycin. Experiments were performed after a culturing period of 10–13 days during which cultured neurons develop a rich network of processes, express functional NMDA-type and AMPA/kainate-type glutamate receptors, and form synaptic contacts.
Transfection and nucleofection
Neurons were transfected in trophic transfection medium55 with plasmids (2 μg ml−1 total) and/or siRNA (100 nM) using Lipofectamine 2000. Nucleofection was performed using the Amaxa rat Neuron Nucleofector Kit (Lonza). See Supplementary Methods for further details and siRNA target sequences.
Western blotting and Subcellular fractionation
Gel electrophoresis and western blotting were performed using the Xcell Surelock system (Invitrogen) using precast gradient gels (4–20%) as described45. The following antibodies were used: Ccdc109a (Sigma, 1:500), ß-actin (Abcam, 1:2,000), α-Tubulin (Sigma, 1:400,000), anti PDH-E1-alpha (Abcam, 1:1,500); anti C-V-alpha (Abcam, 1:1,500); anti Erk 1/2 (NEB, 1:5,000). For visualization of western blots, HRP-based secondary antibodies were used followed by chemiluminescent detection on Kodak X-Omat film. Western blots were analyzed by digitally scanning the blots, followed by densitometric analysis (ImageJ). For figure preparation of western blots, linear adjustment of brightness/contrast was applied (Photoshop) equally across the image. See Supplementary Methods for details of subcellular fractionation.
Plasmids and virus generation
The vector containing the mouse CaMKIIα promoter used to construct and package rAAV has been described previously56. For knockdown using shRNA, we used a rAAV vector containing the U6 promoter driving shRNA expression and that also contained a CaMKII promoter driving mCherry expression (to identify infected neurons). See Supplementary Methods for details of cloning and sequences used to generate rAAV vectors encoding Mcu, 4mtD3cpv and shRNA targeting Mcu and Npas4.
Neurons were infected with 1011 rAAV particles per μl at DIV 4. Infection efficiencies were determined at DIV 10 by analyzing the fluorescence of eGFP or mCherry; they ranged from 80 to 90% of the viable neurons. rAAV expression vectors for Npas4, CaMBP4 and mCherry have been described previously35,56. Mcu-GFP was a gift from Vamsi Mootha18, pCAGGS-GCaMP2 was a gift from Karel Svoboda57; GCaMP2-mt was a gift from Xianhua Wang24, Mt-cameleon-pcDNA3 (containing 4mtD3cpv cDNA) was a gift from Roger Tsien25.
Electrophysiological recording and analysis
NMDA-evoked whole-cell steady-state currents (normalized to cell capacitance) were measured 48 h after transfection as described45. NMDA (150 μM) was applied for 30 s, repeated twice for each cell. Data were filtered at 1 kHz and digitized at 5 kHz for subsequent off-line analysis.
Mitochondrial Ca2+ imaging
In all Ca2+ imaging experiments, we performed experiments with control and 'treated' conditions using sister cultures interleaved on the same day to control for any culture-to-culture variation in NMDA-induced Ca2+ influx. Thus, the only 'control' data shown in any particular figure are those data collected on the same day on the same culture as when the 'treated condition' data (for example, Mcu overexpression) were collected. Several imaging approaches were used: (a) Rhod-2 imaging: this was performed as described23 using a Leica AF6000 LX imaging system, with a DFC350 FX digital camera. Neurons loaded with Rhod-2 showed a punctate distribution of the indicator that very closely resembled that obtained with mitotracker red (data not shown) and the pattern was abolished by the mitochondrial uncoupler FCCP (Supplementary Fig. S1c), confirming the mitochondrial localization of the dye. Transfected cells were identified by co-transfecting eGFP expression plasmid. The NMDA-induced increase in Rhod-2 signal (ΔF/F, ex 546±6 nm; em 600±20 nm) of each transfected cell was compared to that observed in surrounding untransfected cells in a 100 μm radius and subsequently expressed as a percentage of that observed in those untransfected cells. (b) GCaMP2-mt imaging: neurons were transfected with GCaMP2-mt-encoding vector, the fluorescence signal of which was detected using a standard GFP filter set (ex 480±20; em 527±15). NMDA-induced changes in mitochondrial Ca2+ were expressed as (F−Fmin)/(Fmax−F) according to the equation [Ca2+]=Kd × (F−Fmin)/(Fmax−F). Fmax was obtained when cells were treated with the cell-permeable Ca2+ ionophore ionomycin which both inserts into the plasma membrane and passes into the cell, inserting into mitochondrial membranes58, leading to saturation of the indicator when in regular medium (2 mM Ca2+). Fmin was obtained under the same conditions except in zero Ca2+ medium. The linear relationship between [Ca2+] and (F−Fmin)/(Fmax−F) was confirmed by calibrating the indicator as expressed in neurons, exposing them to ionomycin in the presence of sequentially different solutions of precise [Ca2+], obtained by mixing K2EGTA and CaEGTA solutions (Calcium Calibration Buffer Kit, Invitrogen) at different ratios (data not shown). (c) 4mtD3cpv imaging was performed as described25. Fluorescence images were acquired at 2 Hz using a cooled CCD camera (iXon, Andor) through a × 20 water-immersion objective (XLMPlanFluor, Olympus) on an upright microscope (BX51W1, Olympus). Fluorescence excitation (CFP 430±12; YFP 500±10) was provided by a xenon arc lamp in combination with an excitation filter wheel (cell^R, Olympus). CFP (470±12) and YFP (535±15) emission wavelengths were separated and filtered using a DualView beam splitter (MAG Biosystems). Data were collected using proprietary software (cell^R, Olympus), and analyzed using ImageJ and IgorPro (WaveMetrics). When appropriate, only cells co-expressing both a Ca2+ indicator and an mCherry or tDimer tag were chosen for analysis. Ca2+ concentration changes were quantified using the crosstalk- and bleaching-corrected FRET ratio25. Mitochondrial Ca2+ responses to NMDA were expressed as (%Rfret/(ΔRmax−%Rfret))1/n according to the equation [Ca2+]=K′d × (%Rfret/(ΔRmax−%Rfret))1/n25, where %Rfret represents the percent of the maximum response obtained in SGG medium containing 10 μM ionomycin and 10 mM Ca2+. The values for DRmax and n (105.3% and 0.74, respectively) were derived from published calibrations25. The linear relationship between [Ca2+] and (%Rfret/(DRmax−%Rfret))1/n was confirmed in neurons exposed to ionomycin in the presence of sequentially different solutions of precise [Ca2+], obtained by mixing K2EGTA and CaEGTA solutions (Calcium Calibration Buffer Kit, Invitrogen) at different ratios (data not shown). Control values for mitochondrial [Ca2+] obtained using 4mtD3cpv were subject to some culture-to-culture variation, which is likely to be due to the fact that it is operating closer to it's maximum than GCaMP2-mt is. As a result of this, we have normalized all 4mtD3cpv [Ca2+] data to the average NMDA-induced [Ca2+] obtained in control cells on that day of recording. This allows us to directly assess the effect of Mcu expression, Mcu knockdown, or BiC pre-treatment on NMDA-induced mitochondrial [Ca2+], expressed as a percentage of the NMDA-induced mitochondrial [Ca2+] level obtained in that exact day of recording.
Mitochondrial membrane potential imaging
Mitochondrial membrane potential was analyzed as described10,28 using Rh123 (Molecular Probes). Briefly, neurons were loaded with Rh123 (10 μg ml−1 or 26 μM) in SGG medium for 10 min followed by extensive washing with SGG. Rh123 partitions into polarized mitochondria where it self-quenches at the concentration used. When mitochondria depolarize, Rh123 leaks out of the mitochondria into the cytoplasm where it dequenches and fluoresces strongly. Maximum Rh123 signal (ex 480±20; em 527±15) was obtained by completely eliminating the mitochondrial potential by exposing the neurons to the mitochondrial uncoupler FCCP (5 μM; Sigma). For analyzing the effect of transfecting Mcu expression vectors or Mcu-directed siRNA, transfected cells were identified by co-transfecting mCherry expression plasmid. The NMDA-induced increase in Rh123 signal of each transfected cell (as a % of the FCCP-induced level for that cell) was compared with that observed in surrounding untransfected cells in a 100-μm radius and subsequently expressed as a percentage of that observed in those untransfected cells. The NMDA-induced increase in Rh123 signal in Mcu-1 shRNA-infected hippocampal neurons was compared with that observed in Scr shRNA-infected cultures analyzed in parallel.
Studying transfected neurons after excitotoxic insult
Excitotoxicity experiments performed on Lipofectamine-transfected neurons were performed as described45,59 (for full details see Supplementary Methods). The induction and analysis of NMDA-induced neuronal cell death of rAAV-infected neurons were performed as described60, with slight changes. For full details, see Supplementary Methods. Also see Supplementary Methods for details of methodology used to calculate whether Mcu overexpression specifically rendered neurons more vulnerable to NMDA exposure, taking into account the increased basal death observed.
Quantitative reverse transcriptase PCR
To determine Mcu silencing by the pre-made Mcu-directed siRNA, and study activity-dependent Mcu regulation in cortical neurons, QRT–PCR was performed using an Mx3000P QPCR System as described45. For further details including primer sequences, see Supplementary Methods. To determine Mcu silencing by Mcu-directed rAAV–shRNA, and study activity-dependent Mcu regulation in hippocampal neurons, QRT–PCR was performed using real-time TaqMan technology with a sequence detection system model 7300 Real Time PCR System (Applied Biosystems, Foster City, CA, USA). For further details including primer sequences see Supplementary Methods.
Statistical analysis
Statistical testing involved a two-tailed paired or unpaired Student’s t-test, as appropriate. For studies employing multiple testing, we used a one-way ANOVA followed by Bonferroni post hoc test. All data were presented as mean±s.e.m.
Additional information
How to cite this article: Qiu, J. et al. Mitochondrial calcium uniporter Mcu controls excitotoxicity and is transcriptionally repressed by neuroprotective nuclear calcium signals. Nat. Commun. 4:2034 doi: 10.1038/ncomms3034 (2013).
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Acknowledgements
We are grateful to Vamsi Mootha and Xianhua Wang for providing plasmids. This work is supported by a MRC Senior Non-Clinical Research Fellowship (G.E.H.), an ERC Advanced grant (H.B.), the BBSRC, the Wellcome Trust and the German Ministry of Education and Research (BMBF, 01GQ1003A).
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G.E.H and H.B. conceived the project and designed the research. G.E.H., H.B., P.A.S. and D.J.A.W. supervised the research. J.Q., Y-W.T., A.M.H., M.M., N.K. and G.E.H. performed the experiments. G.E.H. and H.B. wrote the manuscript.
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Qiu, J., Tan, YW., Hagenston, A. et al. Mitochondrial calcium uniporter Mcu controls excitotoxicity and is transcriptionally repressed by neuroprotective nuclear calcium signals. Nat Commun 4, 2034 (2013). https://doi.org/10.1038/ncomms3034
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DOI: https://doi.org/10.1038/ncomms3034