Novel Regulation of the Synthesis of α-Amino-3-hydroxy-5-methyl-4-isoxazolepropionic Acid (AMPA) Receptor Subunit GluA1 by Carnitine Palmitoyltransferase 1C (CPT1C) in the Hippocampus*

Background: One interacting partner of the AMPA receptor (AMPAR) complex in the endoplasmic reticulum is carnitine palmitoyltransferase 1C (CPT1C). Results: CPT1C regulates synaptic AMPAR levels and synaptic transmission by post-transcriptional regulation of GluA1 protein synthesis. Conclusion: CPT1C is a new regulator of AMPAR translation efficiency. Significance: CPT1C modulation could be a new tool to prevent AMPAR decline and learning deficits. The regulation of AMPA-type receptor (AMPAR) abundance in the postsynaptic membrane is an important mechanism involved in learning and memory formation. Recent data suggest that one of the constituents of the AMPAR complex is carnitine palmitoyltransferase 1C (CPT1C), a brain-specific isoform located in the endoplasmic reticulum of neurons. Previous results had demonstrated that CPT1C deficiency disrupted spine maturation in hippocampal neurons and impaired spatial learning, but the role of CPT1C in AMPAR physiology had remained mostly unknown. In the present study, we show that CPT1C binds GluA1 and GluA2 and that the three proteins have the same expression profile during neuronal maturation. Moreover, in hippocampal neurons of CPT1C KO mice, AMPAR-mediated miniature excitatory postsynaptic currents and synaptic levels of AMPAR subunits GluA1 and GluA2 are significantly reduced. We show that AMPAR expression is dependent on CPT1C levels because total protein levels of GluA1 and GluA2 are decreased in CPT1C KO neurons and are increased in CPT1C-overexpressing neurons, whereas other synaptic proteins remain unaltered. Notably, mRNA levels of AMPARs remained unchanged in those cultures, indicating that CPT1C is post-transcriptionally involved. We demonstrate that CPT1C is directly involved in the de novo synthesis of GluA1 and not in protein degradation. Moreover, in CPT1C KO cultured neurons, GluA1 synthesis after chemical long term depression was clearly diminished, and brain-derived neurotrophic factor treatment was unable to phosphorylate the mammalian target of rapamycin (mTOR) and stimulate GluA1 protein synthesis. These data newly identify CPT1C as a regulator of AMPAR translation efficiency and therefore also synaptic function in the hippocampus.

mitochondrial intermembranes. Whereas liver CPT1A and muscle CPT1B isoforms catalyze the conversion of long-chain acyl-CoA to acyl-carnitines in fatty acid ␤-oxidation, the brainspecific isoform CPT1C exhibits low catalytic activity in vitro (1) and is located in the endoplasmic reticulum of neurons, largely in the hippocampus. Furthermore, it is exclusively present in mammals (1,2).
The biochemical function of CPT1C is poorly understood, although it has been reported to modulate ceramide metabolism in neurons (3). At the physiological level, it is well demonstrated that hypothalamic CPT1C contributes to the control of food intake and energy balance (4 -6) and the role of CPT1C in motor function (7,8). Recently, the involvement of hippocampal CPT1C in cognition and spinogenesis has been described (3). CPT1C knock-out (KO) mice were shown to present strongly compromised spatial learning and disrupted dendritic spine morphology by increasing immature filopodia and decreasing mature spines. Interestingly, high-resolution proteomic analyses have revealed CPT1C as one of the constituents of the complex of ␣-amino-3-hydroxyl-5-methyl-4-isoxazole-propionate-type glutamate receptors (AMPARs) (9 -11), and a recent study has described the involvement of CPT1C in GluA1 trafficking (12). However, given that CPT1C only interacts with AMPARs in the ER, the role of CPT1C in AMPAR synthesis has been scarcely examined.
In the present study, we show that CPT1C binds to endogenous GluA1 and GluA2 subunits and regulates their expression in mouse hippocampi and in cultured hippocampal neurons, which is crucial for AMPARs to reach the synapsis and for synaptic transmission. Furthermore, we reveal that this regulation is exerted post-transcriptionally, at the level of the de novo protein synthesis, without affecting protein degradation. Consequently, synaptic AMPARs are diminished in CPT1C KO hippocampal cultures, correlating with a reduction in the amplitude of AMPAR-mediated miniature excitatory postsynaptic currents (mEPSCs). These data may explain the previously described involvement of CPT1C in dendritic spinogenesis and learning.
Animals-CPT1C knock-out mice were developed as described previously (3). After 8 back-crosses with C57BL/6J mice, littermate homozygous CPT1C KO and wild type (WT) mice were crossed separately to obtain a line for each genotype, which were used in the experiments. Hippocampi were obtained from adult male mice. All animal procedures met the guidelines in Spanish legislation (BOE 32/2007) and were approved of by the local ethics committee.
Neuronal Cultures-Primary hippocampal mouse neurons were prepared from embryonic day 16 WT or CPT1C KO embryos and cultured as described previously (13).
Electrophysiology-For recordings of cultured hippocampal neurons at 15-16 days in vitro (DIV), coverslips were mounted and placed on the stage of an inverted microscope (Olympus IX50). Whole-cell patch clamp currents were recorded with an Axopatch 200B amplifier-Digidata1440A series interface board using pClamp10 software (Molecular Devices). To isolate AMPAR-mediated mEPSCs, the following blockers were added to the extracellular solution: 1 M tetrodotoxin, 50 M D-AP5, 25 M 7-CK, and 20 M SR95531/gabazine (all from Abcam). Series resistance (R s ) was typically 15-22 megaohms and was monitored at the beginning and at the end of the experiment. Cells that showed a change in R s greater than 20% were rejected (14). There was no significant difference in membrane capacitance when comparing WT and CPT1C KO neurons. For electrophysiology data analysis, mEPSCs were filtered at 5 kHz and digitized at 10 kHz. Data were analyzed using IGOR Pro (Wavemetrics) together with Neuromatic (Jason Rothman). Events were detected using amplitude threshold crossing (15), with the threshold (typically ϳ7-8 pA) set according to the baseline current variance. For amplitude and kinetic analyses, only events with monotonic fast rise (Ͻ1 ms) and uncontaminated decay were included.
Immunocytochemistry-For labeling surface AMPARs, neurons at 17-18 DIV were fixed with 4% (w/v) paraformaldehyde, blocked with 2% goat serum, and incubated with anti-AMPAR N terminus antibodies. After washing, cells were incubated with the appropriate Alexa Fluor-conjugated secondary antibodies. Neurons were then permeabilized with 0.1% (v/v) Triton X-100 and then blocked once more. Buffer was substituted with the appropriate anti-PSD95 antibody. After washing, cells were incubated with secondary antibodies. Coverslips were mounted using Fluoromount mounting medium. Imaging was performed with the confocal laser-scanning microscope ZEISS LSM 700 using a ϫ63 1.4 numerical aperture oil objective. For quantification, sets of cells were cultured and stained simultaneously and imaged using identical settings. The region of interest was randomly selected. Measurements with the Fiji image processing package were performed as described previously (16).
Immunoprecipitation-Neurons were collected using Triton buffer (50 mM Tris-HCl, pH 8, 150 mM NaCl, and 1% Triton X-100) supplemented with protease and phosphatase inhibitor cocktails and solubilized for 30 min at 4°C in an orbital shaker. Samples were processed as described previously (17).
Western Blot-Dissected hippocampi and neuronal cultures were collected in radioimmune precipitation assay buffer and HEPES buffer (10 mM HEPES, 10 mM KCl, 1.5 mM MgCl 2 ), respectively, and supplemented with protease and phosphatase inhibitor mixtures. Next, protein extracts were separated on SDS-polyacrylamide gels and then transferred onto Immo-bilon-P PVDF membranes (Millipore). Blots were blocked with 5% (w/v) dry milk in TBS-T and incubated at 4°C overnight with primary antibodies in TBS-T 0.2% (w/v) BSA. After washing, blots were incubated with horseradish peroxidase-conjugated secondary antibodies and developed using the Luminata TM Forte Western HRP substrate (Millipore). Semiquantitative analysis was performed using densitometry with Fiji software.
Lentiviral Infection-Two lentiviral vectors, pWPI-IRES-GFP and pWPI-CPT1C-IRES-GFP, were constructed to drive cell expression of GFP and CPT1C plus GFP, respectively. The map and the sequences of these plasmids, kindly provided by Dr. Trono (Laboratory of Virology and Genetics, Ecole Polytechnique Fédérale de Lausanne, Switzerland), are available from Addgene. Lentiviruses were propagated and titrated as described previously (18). Infection was performed on the day of seeding in complete DMEM medium at 1 virus/cell and left to stand for 5 h. The medium was then replaced with supplemented neurobasal medium. Fourteen days later, cells were collected for the analysis of GFP and CPT1C expression. The percentage of infected cells reached at least 75% in cultured hippocampal neurons.
Real-time PCR-For expression analysis, template cDNA was prepared from 1 g of total RNA by reverse transcription (Moloney murine leukemia virus). Gene expression was quantified using real-time PCR with SsoFast Probes Supermix (Bio-Rad) and gene-specific primer VIC, FAN, or HEX dye-labeled as follows: Gapdh forward, reverse, and probe (4352339F; Applied Biosystems); Gria1 (64845347; IDT); and Gria2 (64845351; IDT) on a CFX96 real-time system (Bio-Rad). All biological samples were amplified in the same run for each experiment. Relative gene expression between paired samples was estimated using the 2 Ϫ⌬⌬Ct method.
Bio-orthogonal Noncanonical Amino Acid Tagging Analysis-The de novo protein synthesis rate was determined by a bio-orthogonal noncanonical amino acid tagging assay in WT or CPT1C KO hippocampal neurons as described previously (19), using copper sulfate and tris(2-carboxyethyl) phosphine to generate the Cu(I) catalyst for the copper-catalyzed azidealkyne cycloaddition reaction (20). Briefly, cells were depleted of methionine for 30 min before treatment with azidohomoalanine at 1 mM (an effective surrogate for methionine; Jena Bioscience) for 4 h. After cell lysis with 0.05% SDS in PBS, pH 7.6, and protease and phosphatase inhibitors, the copper-catalyzed azide-alkyne cycloaddition reaction was prepared as follows: 200 M triazole ligand, 50 M biotin-alkyne, 400 M tris(2carboxyethyl) phosphine, and 200 M copper sulfate, incubated at 4°C overnight under agitation. The excess reagents were removed by gel filtration using PD-10 columns and eluted in 0.05% SDS in PBS, pH 7.6. A dot-blot analysis was performed to determine the newly synthesized protein concentration tagged with biotin. Desalted samples were precipitated with NeutrAvidin resin (Pierce) overnight at 4°C. NeutrAvidin beads were then washed three times with 1% Nonidet P-40 in PBS, pH 7.6, and samples were eluted with SDS sample buffer. Proteins were detected using immunoblotting.
Statistics-Statistical analysis was performed using PRISM (GraphPad Software). Significance between two groups was determined according to data normality according to the Shapiro-Wilk test, using either Student's t test or a Mann-Whitney U test (parametric and non-parametric, respectively). For comparisons among 3-4 groups, ANOVA was performed, followed by the Bonferroni post-test.

CPT1C-AMPAR Interaction in Hippocampal Neurons-It
has been demonstrated that CPT1C binds AMPARs in solubilized membrane fractions from the hippocampus in rodents (9 -11). We therefore first analyzed whether CPT1C was able to interact with AMPARs in cultured hippocampal neurons. We performed immunoprecipitation studies using specific anti-CPT1C antibodies developed in our laboratory (1). Fig. 1A shows how CPT1C interacts with GluA1 and GluA2 but not with other synaptic glutamatergic proteins, such as NMDAtype glutamate receptor subunit GluN2A or the AMPAR auxiliary subunit stargazin (also called TARP ␥ 2; transmembrane AMPA regulatory protein). We also performed reverse immunoprecipitation using a GluA1 antibody and confirmed that interaction (Fig. 1B). It is worth noting that GluA1-GluA2 and GluA1-stargazin bindings were not found to be disrupted in the absence of CPT1C (Fig. 1C). To prove antibody specificity, CPT1C immunoprecipitation was performed in the hippocampi of CPT1C KO animals; in those samples, we did not detect CPT1C or GluA1 in immunoblotting (data not shown). These data demonstrate that CPT1C binds AMPARs in cultured hippocampal neurons.

Synaptic Transmission Is Reduced in CPT1C KO Animals-
Because CPT1C binds to GluA1/GluA2 and previous results from our laboratory clearly showed that spatial learning and dendritic spine maturation are impaired in CPT1C KO mice (3), we wondered whether excitatory synaptic transmission was altered in those animals. To address this issue, we performed whole-cell voltage clamp recordings of cultured hippocampal neurons and measured AMPAR-mediated mEPSCs. Cells were treated with tetrodotoxin to block synaptic transmission and with D-AP-5, 7-CK, and SR95531 to block NMDA and GABA A receptors. We found that mEPSC amplitude was decreased in neurons from CPT1C KO animals (Fig. 2, A-C) when compared with WT neurons (Ϫ18.96 Ϯ 0.95 pA for WT versus Ϫ15.46 Ϯ 0.99 pA for KO; n ϭ 26 and n ϭ 18, respectively; p ϭ 0.0175; t test). Cumulative amplitude histograms for mEPSCs ( Fig. 2D) revealed that the distribution of amplitudes in CPT1C KO neurons shifted toward smaller values, indicating a decrease in the quantity of postsynaptic AMPARs. We then examined the frequency of AMPA-mediated mEPSCs and found no significant differences (4.12 Ϯ 0.84 Hz for WT versus 3.83 Ϯ 1.24 Hz for KO; p ϭ 0.3519; Mann-Whitney test; Fig.  2E), demonstrating that no presynaptic alteration is present in CPT1C KO cells.
In summary, our results demonstrate that the number of AMPARs in synaptic puncta is clearly reduced and that basal  OCTOBER 16, 2015 • VOLUME 290 • NUMBER 42 synaptic activity is compromised in CPT1C KO animals. Based on these findings, we asked whether these deficits could be explained because CPT1C was involved in the regulation of AMPAR expression. CPT1C Regulates AMPAR Protein Expression-AMPAR protein levels were first analyzed in hippocampal cultured neurons over DIV from 4 to 16 DIV. GluA1 and GluA2 expression intensified in the same manner as CPT1C during neuronal maturation (Fig. 4A). However, AMPAR levels in CPT1C KO cultured neurons were clearly diminished when compared with WT cells (1.00 Ϯ 0.02 GluA1 levels for WT versus 0.45 Ϯ 0.08 for KO at 14 DIV; p ϭ 0.0001; and 1.00 Ϯ 0.07 GluA2 levels versus 0.46 Ϯ 0.10; p ϭ 0.0018; n ϭ 5; t test; Fig. 4B). Other synaptic proteins, including PSD95, synapsin I, and GluN2A, remained unaltered (not significantly different at 14 DIV; n ϭ 3; t test; Fig.  4, C and D).

CPT1C Regulation of AMPAR Expression
Previous results in our group demonstrated that the requirement of CPT1C for efficient spinogenesis is related with its ability to regulate ceramide levels; exogenous ceramide treatment rescues CPT1C KO phenotype on spine morphology. Therefore, we decided to analyze whether ceramide could reverse an AMPAR decrease in CPT1C-deficient neurons. Surprisingly, neither soluble C6 ceramide nor the treatment with the ceramide precursor serine increased GluA1 or GluA2 protein levels in KO cells (not significantly different; n ϭ 6; t test; Fig. 4, E-H).
Similar results were obtained in the hippocampi of CPT1C KO animals. First, we analyzed CPT1C expression during hippocampal development in WT mice. As seen in hippocampal cultures, total CPT1C protein levels were regulated with the same pattern expression as GluA1 and GluA2, which increases progressively up to adult age, as well as synapsin I, PSD95, and GluN2A (Fig. 5, A and B). To examine whether CPT1C was involved in the regulation of AMPAR expression, we measured total GluA1 and GluA2 protein levels in the hippocampi of adult CPT1C KO mice (Fig. 5C). CPT1C KO hippocampi showed lower levels of AMPARs when compared with WT mice (1.00 Ϯ 0.04 GluA1 levels for WT versus 0.67 Ϯ 0.07 for KO; p ϭ 0.0012; 1.00 Ϯ 0.05 GluA2 levels versus 0.67 Ϯ 0.05; p ϭ 0.0002; n ϭ 9 for WT and n ϭ 13 for KO; t test; Fig. 5D). PSD95, synapsin I, and GluN2A remained unaffected (not significantly different; n ϭ 6; t test; Fig. 5, E and F). These findings  confirm that CPT1C expression in the hippocampus specifically regulates total AMPAR protein levels. CPT1C Regulates AMPAR Expression at the Post-transcriptional Level-In order to understand how CPT1C regulates AMPAR expression, we first analyzed Cpt1c, Gria1, and Gria2 mRNA levels in WT and CPT1C KO mice during hippocampal development. Fig. 6A shows that Cpt1c mRNA levels increased during the first developmental days and then remained unaltered during the rest of the period of study (until 6 months of age). Gria1 transcription exerted a similar pattern of expression than Cpt1c (Fig. 6B), whereas Gria2 mRNA levels did not significantly change during hippocampal development (Fig. 6C). Interestingly, no differences were detected between WT and CPT1C KO animals in Gria1 or Gria2 mRNA levels (n ϭ 3-6; t test; Fig. 6, B and C).
Moreover, hippocampal cultured neurons from CPT1C KO mice did not show any difference in mRNA levels when compared with WT neurons (not significantly different; n ϭ 6; t test; Fig. 6D). In addition, CPT1C overexpression did not induce any change in the mRNA levels of either AMPAR (not significantly   OCTOBER 16, 2015 • VOLUME 290 • NUMBER 42 different; n ϭ 6; ANOVA; Fig. 6E). These data indicate that CPT1C does not regulate AMPARs at the transcriptional level and suggest that CPT1C is directly involved in protein turnover. CPT1C Is Not Involved in AMPAR Degradation-The reduction in AMPAR protein levels observed in CPT1C-deficient neurons could be explained by enhanced degradation. To assay this possibility, we treated cells with a protein translation inhibitor, cycloheximide, and measured the decrease of AMPAR protein levels for 24 h. Results showed that GluA1 and GluA2 basal degradation was not enhanced in CPT1C KO neurons (not significantly different; n ϭ 3; t test; Fig. 7A). In fact, there is a tendency in the opposite direction: a decrease in the rate of degradation, which may be due to the lower levels of synaptic AMPARs in those cells.

CPT1C Regulation of AMPAR Expression
To further explore the degradation hypothesis, we analyzed whether activity-dependent GluA1 degradation was altered in CPT1C KO neurons. It is well described that chemical long term depression (chemLTD) triggers a persistent decrease in total GluA1 levels (22), a mechanism involving the proteasome (23). After NMDA treatment, the total levels of GluA1 decreased in both WT and CPT1C-deficient neurons (94.7 Ϯ 1.5% in WT versus 73.1 Ϯ 7.8% in KO; n ϭ 3; not significantly different; t test; Fig. 7B), indicating that GluA1 degradation was not increased in CPT1C KO cells. Interestingly, CPT1C protein levels were also decreased in response to chemLTD (100.0 Ϯ 12.5% for vehicle versus 50.8 Ϯ 11.0% for NMDA in WT; n ϭ 3; p ϭ 0.042; t test; Fig. 7C), confirming the correlation between CPT1C and GluA1 expression.
CPT1C Regulates GluA1 Protein Synthesis-Because we did not observe significant differences at the level of transcription or degradation, we then explored whether CPT1C deficiency directly affected AMPAR protein synthesis. For this purpose, we measured GluA1 accumulation for 3 h after chemLTD by treating cultured neurons with inhibitors of proteasome and lysosome function to block protein degradation. We performed this analysis after chemLTD due to the very low AMPAR synthesis observed under basal conditions. As expected, an increase in GluA1 protein levels was detected in neurons from WT mice, whereas this increase was totally blocked in CPT1C KO neurons (145.2 Ϯ 33.6% for WT versus 5.3 Ϯ 11.9% for KO; n ϭ 3; p ϭ 0.0171; t test; Fig. 7C). Next, we used the bio-orthogonal noncanonical amino acid tagging method, which uses click chemistry to label methionine in newly synthesized proteins (see "Experimental Procedures" for a detailed description) to directly measure the de novo synthesis of GluA1 protein in both genotypes. WT or CPT1C KO hippocampal neurons were metabolically labeled with azidohomoalanine, and after conjugation to biotin, newly synthesized proteins were purified using NeutrAvidin beads. Immunoblotting of biotin-azidohomoalanine-labeled samples developed with NeutrAvidin showed similar total levels of the de novo synthetized proteins in both types of cells (Fig. 7D, left). In contrast, the levels of newly translated (nascent) GluA1 protein in KO neurons were highly decreased compared with WT ones (Fig. 7D, right), indicating that the decrease observed in total levels of GluA1 comes from the reduction in protein synthesis. The voltage-dependent anionselective channel, a mitochondrial protein not regulated by synaptic activity, did not show significant changes. Because CPT1C is an ER protein, we wanted to determine whether the decrease in GluA1 synthesis was the result of a hypothetical ER stress response caused by CPT1C deficiency. For this purpose, we analyzed the levels of different effectors of the unfolded protein response pathway (24). We studied the levels of phospho-PERK (RNA-activated, protein kinase-like ER-resident kinase), phospho-EIF2 (eukaryotic initiation factor 2␣), ATF4 (activating transcription factor 4), and GADD34 (a subunit of an EIF2-directed phosphatase) by immunoblotting; however, the unfolded protein response was not activated under basal conditions in CPT1C-deficient neurons (Fig. 7E).
CPT1C Is Required for Brain-derived Neurotrophic Factor (BDNF)-induced GluA1 Synthesis-It has been recently described that BDNF activates GluA1 translation through phos-phorylation of mTOR (25). Therefore, we decided to explore whether CPT1C was necessary for BDNF-induced GluA1 synthesis. As expected, BDNF treatment was found to increase GluA1 protein levels in WT neurons; however, this increase was blocked in CPT1C KO cells (   Recently, it has also been described that phosphorylation of AMPK triggers GluA1 translation (26). Interestingly, CPT1C KO neurons show a reduction in the phosphorylation of this kinase under basal conditions (1.00 Ϯ 0.07 for WT versus 0.41 Ϯ 0.04 for KO; n ϭ 8; p Ͻ 0.001; t test; Fig. 8, F and G). All of these data indicate that CPT1C is involved in GluA1 protein synthesis regulation under basal and stimulated conditions.

Discussion
In this study, we reveal that CPT1C regulates AMPAR protein levels by modulating its translational efficiency. CPT1C expression parallels GluA1 and GluA2 and other synaptic proteins during the development of the hippocampus and cultured hippocampal neurons. Moreover, CPT1C deficiency or CPT1C overexpression results in a specific decrease or increase, respectively, in total GluA1 and GluA2 levels without any change in their mRNA levels or degradation rate. The reduced expression of AMPARs results in reduced synaptic AMPAR content and diminished synaptic transmission in the hippocampal neurons of CPT1C KO mice, which may explain the impairment in dendritic spine maturation as well as the learning deficits we described previously in those mice (3). CPT1C Interaction with AMPARs-GluA1 and GluA2 were the first identified partners of CPT1C (9). The authors of that study demonstrated that CPT1C position within the macromolecular complex of AMPARs was more peripheral than other associated AMPAR constituents, but it appears to be one of the most abundant proteins of native AMPAR complexes in rodent brain solubilized membrane fractions. Unlike other AMPAR auxiliary proteins, CPT1C equally interacts with AMPARs in the hippocampus, cortex, and cerebellum (10), and CPT1C displays very similar richness profiles in AMPAR complexes across all brain regions (11). In the present study, we confirm the interaction of CPT1C with AMPARs in hippocampal neu-rons and show that CPT1C does not interact with other glutamate receptor constituents, such as GluN2A or stargazin. Interestingly, we observed a stronger interaction between CPT1C and GluA1 than between CPT1C and the GluA2 AMPAR subunit, suggesting that CPT1C has a greater influence on that subunit. Indeed, functional studies on expression systems have demonstrated that CPT1C enhances surface expression of homomeric GluA1 but has no effect on homomeric GluA2 (9), supporting the hypothesis of subunit specificity. The fact that CPT1C co-localizes with AMPARs only at the ER level and not at the Golgi apparatus or at the plasma membrane (12) AMPAR complexes, suggests that it could be involved in AMPAR synthesis or in AMPAR mobility and export from the ER to the surface, ultimately controlling AMPAR synaptic function. Recently, it has been demonstrated that CPT1C is involved in GluA1 trafficking (12). In the present study, we demonstrate that CPT1C is involved in GluA1 protein synthesis, confirming the role of CPT1C in both processes and indicating that CPT1C may be a key component in AMPAR homeostasis when located in the ER. It is important to note that biophysical gating properties of surface AMPARs (single channel conductance, peak open probability, and desensitization kinetics) are not modulated by CPT1C (12). CPT1C Expression Profile-Interestingly, the CPT1C expression profile during hippocampal maturation after birth or during neuronal maturation in primary cultures resembled those of GluA1 and GluA2. In the hippocampus, the three proteins increased after birth, reaching their maximum values after weaning, and in hippocampal cultures, they also increased over DIV, the maximum taking place at 14 DIV. This expression profile, which is followed by other synaptic proteins, suggests that CPT1C function is closely related to synaptic function. In fact, activity-dependent degradation of AMPARs induced by chemLTD also coincides with a decrease in CPT1C protein levels, indicating a parallelism in CPT1C and AMPAR expression not only in terms of development but also in synaptic plasticity.
CPT1C Regulation of AMPAR Translation-Unlike other auxiliary proteins of the AMPAR complex that influence AMPAR trafficking, kinetics, and channel properties (27), CPT1C improves AMPAR translation efficiency. We show that the regulation of AMPAR expression by CPT1C is not exerted at the transcriptional level; nor is the basal degradation of AMPARs enhanced in KO CPT1C cells. By contrast, we clearly demonstrate that CPT1C regulates de novo synthesis of GluA1 under basal conditions using labeled methionine and that GluA1 synthesis after chemLTD is dependent on CPT1C availability. It would be interesting to study whether other synaptic stimulus, such as long term potentiation, which induces the delivery of AMPAR at the synaptic level, could regulate AMPAR synthesis mediated by CPT1C.
Few proteins have been previously related with AMPAR synthesis. It has been demonstrated that BDNF treatment of hippocampal neurons triggers GluA1 translation through phosphorylation of mTOR (28). The activation of mTOR blocks the translation repressor 4E-BP2, which selectively inhibits the synthesis of GluA1 in hippocampal pyramidal neurons, resulting in an increase of GluA1 protein translation (29). mTOR has been implicated in the regulation of dendritic growth (30,31), spine formation (31)(32)(33), and synaptic function (32,34). In the present study, we demonstrate that CPT1C KO neurons are unable to synthetize GluA1 in response to a BDNF stimulus; nor are they able to phosphorylate mTOR. It is unknown whether an activation of 4E-BP2 could explain the reduced expression of AMPARs in CPT1C-deficient neurons; however, our results suggest that CPT1C acts upstream from mTOR activation. CPT1C does not seem to regulate the PI3K/AKT pathway, because BDNF-induced phosphorylation of AKT at serine 473 is not impaired in CPT1C-deficient neurons. We are cur-rently performing proteomic approaches to elucidate the mechanism by which CPT1C regulates GluA1 translation. The fact that we do not observe a complete loss of AMPARs in CPT1C KO neurons highlights the role of other mechanisms involved in AMPAR translation, such as the regulation of initiation and elongation by CPEB3 (35) or the control of expression by miRNA501-3p (36). Recently, it has been demonstrated that the activation of the energy sensor AMPK is involved in GluA1 translation (26). In our model, we observe a strong decrease in the phosphorylation of this kinase in CPT1C KO neurons. Interestingly, CPT1C has been previously associated with mTOR and AMPK in situations of energy homeostasis and metabolic stress (5,6,(37)(38)(39). CPT1C might be a link between energetic metabolism and learning through the direct regulation of AMPAR synthesis. We speculate that CPT1C is a sensor of the energetic status of the neuron through its ability to bind malonyl-CoA (2), an intermediate in the fatty acid synthesis, whose cellular levels in hippocampus fluctuate during fasting and feeding (40). In fact, it has been described that the regulation of energy metabolism contributes to AMPAR synaptic incorporation (41), synaptic plasticity (42,43), and memory processes (44).
Synaptic Function in CPT1C KO Mice-Our data from mEPSCs demonstrate that AMPAR synaptic transmission is reduced in CPT1C KO animals, although the specific subunit composition seems not to be altered. These data correlate perfectly with the reduced quantity of both GluA1 and GluA2 receptors we observed in synaptic puncta in CPT1C KO hippocampal neurons. We propose that the 25-40% reduction in synaptic AMPARs is mainly due to the 40 -55% decrease in the total levels of GluA1 and GluA2, although we cannot rule out that other mechanisms, such as trafficking, are involved.
Interestingly, in CPT1C KO neurons, the number of PSD95 puncta increases, whereas the area of the PSD95 puncta and the quantity of AMPARs in synaptic puncta diminishes. These data suggest that the number of immature synapses is increased, whereas the number of functional synapses is decreased in CPT1C KO cells, which is in agreement with our previous observation of increased filopodia and reduced mature spines (3) in cultured hippocampal neurons. It is well known that filopodia contain fewer synaptic AMPARs than shorter regular spines (45). Therefore, reduced levels of synaptic AMPARs in CPT1C-deficient hippocampal neurons may contribute to the immature morphology of the dendritic spines.
We had previously demonstrated that the treatment of CPT1C KO neurons with exogenous ceramide increased spine maturation and reversed the KO phenotype (3). However, exogenous ceramide was not able to rescue the depletion of GluA1 and GluA2 levels observed in CPT1C KO cells. These results indicate that ceramide is not modulating AMPAR expression itself but might be necessary for other mechanisms in spinogenesis. In fact, other studies have described the involvement of GM1 ganglioside (a ceramide derivative) in the regulation of GluA2-containing AMPAR synaptic content by acting on endocytosis (46).
In summary, our results demonstrate that CPT1C is necessary for an efficient translation of AMPARs. In CPT1C-deficient neurons, total AMPAR levels are decreased, causing syn-aptic transmission impairment and most likely the learning deficits observed in CPT1C KO mice. In contrast, CPT1C overexpression increases AMPAR synthesis. The rise in AMPAR levels may be not sufficient to increase synaptic activity (47); however, it probably ensures an adequate GluA1 and GluA2 reservoir and availability for synapsis requirements. Because AMPAR disruption is a major causative agent of synaptic dysfunction in neurodegenerative diseases and aging (27), we hypothesize that CPT1C modulation could constitute a new tool to prevent AMPAR decline and learning deficits during aging and in neurodegenerative disease.
Author Contributions-R. F. designed, performed, and analyzed all the experiments with the exception of the electrophysiological study reflected in Fig. 2, which was designed, performed, and analyzed by D. S. and N. Y. A. J. M. and J. R. provided technical assistance, contributed to the interpretation of data, and provided important intellectual content. M. P. designed and constructed vectors for overexpression and silencing CPT1C and contributed to the preparation of figures. P. C. contributed to the conception and design of the experiments. N. C. conceived and coordinated the study and wrote the paper. All authors reviewed the results and approved the final version of the manuscript.