Calcium-/Calmodulin-Dependent Protein Kinase II (CaMKII) Inhibition Induces Learning and Memory Impairment and Apoptosis

Objectives Inhibition of calcium-/calmodulin- (CaM-) dependent kinase II (CaMKII) is correlated with epilepsy. However, the specific mechanism that underlies learning and memory impairment and neuronal death by CaMKII inhibition remains unclear. Materials and Methods In this study, KN93, a CaMKII inhibitor, was used to investigate the role of CaMKII during epileptogenesis. We first identified differentially expressed genes (DEGs) in primary cultured hippocampal neurons with or without KN93 treatment using RNA-sequencing. Then, the impairment of learning and memory by KN93-induced CaMKII inhibition was assessed using the Morris water maze test. In addition, Western blotting, immunohistochemistry, and TUNEL staining were performed to determine neuronal death, apoptosis, and the relative signaling pathway. Results KN93-induced CaMKII inhibition decreased cAMP response element-binding (CREB) protein activity and impaired learning and memory in Wistar and tremor (TRM) rats, an animal model of genetic epilepsy. CaMKII inhibition also induced neuronal death and reactive astrocyte activation in both the Wistar and TRM hippocampi, deregulating mitogen-activated protein kinases. Meanwhile, neuronal death and neuron apoptosis were observed in PC12 and primary cultured hippocampal neurons after exposure to KN93, which was reversed by SP600125, an inhibitor of c-Jun N-terminal kinase (JNK). Conclusions CaMKII inhibition caused learning and memory impairment and apoptosis, which might be related to dysregulated JNK signaling.


Introduction
Epilepsy is a type of chronic neurological disorder characterized by the unnatural, rapid discharge of neurons [1,2]. The tremor rat (TRM) (tm/tm) has been cultivated in a Kyoto-Wistar colony [3] and is an advantageous model of animal for genetic epilepsy because of the similarity in pathogenesis to the human epileptic circumstance. Our previous studies found that abnormal variations in the CaMKII pathway are involved in epileptogenesis in TRM rats [4][5][6][7][8][9][10][11]. CaMKII is a vital regulator of multiple signaling pathways initiated by calcium signaling. First, CaMKII couples with calciumbound calmodulin and phosphorylates target substrates in neurons, such as voltage-gated sodium channels, mitogenactivated protein kinases (MAPKs), and the cAMP response element-binding protein (CREB) [12][13][14]. Additionally, CaMKII is widely distributed in the hippocampus and cortex [15]. Decreased CaMKII levels have been reported in various epileptic models [16][17][18][19]. However, the function of CaMKII in epileptogenesis remains unknown.
A series of studies have shown that MAPKs, comprising extracellular signal-regulated kinase1/2 (ERK1/2), p38 MAPK, and c-Jun N-terminal kinase (JNK), are involved in numerous cellular pathways triggered by extracellular apoptotic stimuli, which also play critical roles in cell death and survival [20,21]. Bioinformatics studies could reveal how the MAPK pathway influences the molecular mechanisms underlying memory loss in temporal lobe epilepsy (TLE) [22].
CREB is a transcription factor, which plays vital physiological and biochemical roles by combining with the conserved sequence of cAMP response elements, mainly involved in the remodeling, learning, and memory of neurons [23]. Additionally, CREB exhibits neuroprotective roles when its expression is upregulated, which increases expression of prosurvival genes [24]. However, changes in MAPK signaling and CREB in epilepsy and their relationship with CaMKII have not been elucidated.
To illustrate the effect of CaMKII in the context of epilepsy, we used KN93, a specific CaMKII inhibitor, in epileptic models in vitro and in vivo. In the present research, for the first time, our data demonstrate that inhibiting CaMKII contributes to learning and memory impairment and apoptosis associated with dysregulated JNK signaling.

Animals and Drug Administration.
Male and female wild-type Wistar and TRM rats (12 weeks old, 50% male and 50% female) were individually housed in a standard environment. All rats were allowed access to water and food ad libitum and housed under controlled circumstances of appropriate temperature with a 12-hour light/dark cycle. The rats were separated into three groups, including, control, low-dosage, and high-dosage groups. Rats in the control group were given an intraventricular bolus of phosphatebuffered saline (PBS) containing DMSO and sulfobutylether-β-cyclodextrin (SBE-β-CD). Rats in the low-dosage group were administered 9 μg/kg body weight of KN93 (Tocris, Dallas, TX, USA), and those in the high-dosage group were administered 18 μg/kg body weight of KN93. All lateral ventricular injections were performed at a volume of 5.5 μL. In this study, we administered KN93 at a modified concentration compared with the previous dosage chosen for Sprague-Dawley rats on the seventh day (P7) postpartum [25]. We used both low and high doses of KN93 to in vivo experiments. The Institutional Animal Care and Use Committee of the China Medical University confirmed the scheme and procedures of the experiment. Animals were processed with KN93 for 24 hours. In the in vitro experiments, the incubation of cells was executed with 5 μM KN93 in DMSO for 24 hours. The control group was exposed to DMSO in hippocampal primary cultured neurons and PC12 cells.

Morris Water Maze
Test. Animals were subjected to the Morris water maze, comprising navigation assessments and a probe analysis, for seven consecutive days, as previously described [26]. Briefly, rats were permitted to swim freely for 1 minute without a platform as the experimental baseline (day 0). During training days, a platform was located under the water in the tank for navigation assessments and each rat was tested four times a day with an interval of 60 seconds for spatial acquisition. If the rats could not detect the platform during 60 seconds, they were picked up and located on the platform for the next 60 seconds. The period and path length required for each rat to find the hidden platform were observed in each experiment. On the sixth day, we used exploratory tests to evaluate memory consolidation. In the current experiment, the platform was eliminated from the tank and the rats were permitted to swim freely for 60 seconds. We chose a position that was 180°from the original position of the platform as the new starting position to ensure that the memory capacity for the target position could be reflected in the spatial preference, rather than a specific path of swimming. The frequency of each rat passing through the center of the quadrant and the percentage of time each that rat stayed in the quadrant were observed 2 Oxidative Medicine and Cellular Longevity within 60 seconds. A system of video tracking (Chengdu Taimeng Tech. Co. Ltd., Chengdu, China) was used to record all data.

Cresyl Violet Staining.
To assess the morphological modifications in the brain, brain sections were prepared randomly and Nissl bodies were stained with Cresyl violet (CV). The dissolution of Cresyl violet (0.5 g of crystalline acetate powder) was performed in distilled water (500 mL) containing 1.25 mL of glacial acetic acid with a magnetic stirrer at 60°C. Deparaffinized and rehydrated sections were stained by utilizing 0.1% CV staining solution (50-60 minutes) and fixed in neutral gum solution. CV-stained coronal sections were determined using an optical microscope. The morphological characteristics of pyramidal neurons in the hippocampus (CA1 and CA3) and granular cells in the DG area were analyzed. In addition, cell density was evaluated using the ImageJ software. Solarbio, Beijing, China). The images were captured using a confocal microscope and were analyzed using ImageJ.
2.6. TUNEL Staining. TUNEL staining was conducted following the standard protocols described in the manual of the One-step TUNEL apoptosis assay kit (Beyotime, Jiangsu, China). The apoptotic cells were double immunofluorescent stained for the TDT-mediated dUTP nick end labeling (TUNEL) assay (green) and the nuclear counter stain DAPI (blue).

PC12
Cell Line Culture. The frozen cell seeds were revived at 37°C for 30 min and poured into a Petri dish with culture medium. The morphology of the cells was observed every 6 hours. When the culture dishes appeared confluent, the cell fluid in the culture dishes was discarded. Then, the cells were slowly transferred into preheated serum-free culture medium and washed thrice. Trypsin was added to the media, and the state of the cells was observed. After complete digestion, medium was added to terminate the digestion and the cell suspension was centrifuged. Then, the cell-free supernatant was discarded and 100 μL DMSO (cell cryopreservation solution) was added. Bovine and horse serum suspension (900 μL) was added, and cells were transferred to cryopreservation tubes for gradient cryopreservation.
2.8. Primary Hippocampal Neuron Culture. Within two days after birth, newborn Wistar rat pups were anesthetized and decapitated; the brain was quickly removed, soaked in Hank's solution, and stored at 4°C. The hippocampus was dissected rapidly under a microscope ice bath, and the hippocampal tissue was cleaned three times with refrigerated cell culture medium (5 mL DME/F-12; HyClone, Logan, UT, USA). The hippocampal tissue was digested with 2 mL pectinase and gently agitated twice. The cell suspension was removed to repeat the process with pectinase until complete digestion was achieved. After digestion, the cells were evenly mixed with the culture medium from hippocampal neurons and counted for lamination. Half-volume of medium was replaced every other day 24 hours after adhesion of cells. After culturing cells for 7 days, the neuronal state was observed for 9 days and the subsequent experiments were carried out.
2.9. Cell Counting Kit 8 Cytotoxicity Test (CCK8 Cytotoxicity Test). The cell subculture process was repeated, and the cell suspension was transferred to a plate containing 96 wells with 5000-7000 cells per well (note mixing). After adhering to the cell wall, cells were processed with varying concentrations of the drug (0, 0.1, 0.3, 1, 3, 10, 30, and 100) for 24 hours and the final reaction volume was 100 μL. Then, CCK-8 reagent was added at a 1 : 10 ratio and the cells were incubated for 2 hours. The absorbance at 450 nm was evaluated by employing an enzyme-linked immunosorbent assay (ELISA). If the absorbance was not up to the standard, the absorbance was remeasured every 30 minutes. The rate of survival for the cells was evaluated by applying the following equation: 2.10. RNA Sequencing and Data Analysis. RNA-sequencing was performed by the Wuhan SeqHealth Technology Company. Cells treated with KN93 and the vehicle control (DMSO) were harvested, and the extraction of RNA was carried out by employing TRIzol (Invitrogen, Carlsbad, CA, USA). An RNA library was prepared first, after which a HiSeq X 10 sequencer (Illumina) was used to enrich and sequence products that ranged in size from 200 to 500 bp. Common upregulated or downregulated differentially expressed genes (DEGs) in the selected datasets were extracted with the cutoff criteria of |logFC | >0:585 and p < 0:05. Biological information was obtained based on biological functional annotation information. The DEGs were merged into a gene list that was submitted to DAVID, a biological information database, for functional annotation. We further conducted gene ontology (GO) enrichment analysis.
2.11. Flow Cytometry. In an ice bath, cells were digested with trypsin and then pelleted by centrifugation. The binding buffer (4 mL) was mixed with 36 mL of deionized water, and the binding buffer reagent was diluted 10 times. The cells were washed with 900 μL PBS. The suspension was centrifuged for 5 minutes at 1000 rpm. Following the elimination of the supernatant, the cells were gently agitated with 1000 μL binding buffer and centrifuged for 5 minutes. The above procedure was repeated twice. After centrifugation, the supernatant was removed and the cell suspension treated with 1000 μL binding buffer was retained in each tube. In  5 Oxidative Medicine and Cellular Longevity addition to PI single staining and a blank control group, 5 μL of FITC (green) was added per tube for 10 minutes. Thereafter, PI (5 μL) was added per tube for 1 hour. Then, 300 μL PBS was added to each tube and flow cytometry was performed. Staining and data statistics: late apoptosis of PI and early apoptosis of FITC. Q4: early; Q2: late; Q1: necrotic. The cell injury was generally dominated by Q2 + Q4.
2.12. Statistical Analysis. SPSS (version 11.5; SPSS Inc., Chicago, IL, USA) was employed for statistical assessments, and all analysts were blinded to the treatment of each group. All achievements are represented as the mean ± SEM. Student's t-test or ANOVA followed by Tukey's test were performed. p < 0:05 was set to illustrate the statistical significance.   Figure 1(c). The 915 DEGs were subjected to GO enrichment analysis (Figures 1(d) and 1(e)). These downregulated DEGs were related to cognition (GO: 0050890, 22 genes), learning or memory (GO: 0007611, 18 genes), and long-term memory (GO: 0007616, 6 genes), suggesting that CaMKII inhibition can cause learning and memory impairment.

CaMKII Inhibition Induces Learning and Memory
Impairment in Both Wistar and TRM Rats. Based on the results of the RNA sequencing analysis, we next checked whether CaMKII inhibition caused learning and memory impairment. According to a previous study, we injected KN93 into the right ventricle of adult TRM rats (n = 6) at a dose of 30 μg per kilogram of body weight [25]. However, all TRM rats died following the administration of 30 μg/kg body weight KN93 (n = 6). Considering the toxicity, the dose of KN93 was decreased to 18 μg/kg body weight (n = 6). As anticipated, the dose of KN93 at 18 μg/kg body weight did not cause death in rats. Thus, we assumed that 18 μg/kg body weight of KN93 may approach the maximum tolerable dose for TRM rats. KN93 was used at two different doses (18 and 9 μg/kg body weight for high and low doses, respectively) in follow-up experiments.
We then investigated whether KN93 treatment affected learning and memory in Wistar and TRM rats by performing the Morris water maze test (Figure 2). From day to day, the escape latency was higher in the group of TRM compared with the group of Wistar rats, with similar results for path length, which was longer than that in the group of control (p < 0:01, n = 6, Figures 2(a)-2(c)). The frequency of passing across the goal in the KN93-treated Wistar rats (high dose) was lower than that observed in the Wistar rat control group (p < 0:01, n = 6, Figure 2(d)). The frequency of passing across the goal in the KN93-treated TRM rats decreased in comparison with that in the group of control (p < 0:01, n = 6, Figure 2(d)). Similar results were observed for time in the target quadrant (Figure 2(e)).
Previous investigations have shown that histone demethylase PHF2 is able to improve the CREB signaling pathway via regulation of genes related to memory [27]. We next determined the expression level of CREB in Wistar and TRM rats after treatment with of KN93 using Western blotting. The expression of p-CREB in KN93-treated TRM rats was decreased compared with control rats (p < 0:05, n = 6, Figures 2(f) and 2(g)). Additionally, the expression of p-CREB in Wistar rats after the application of KN93 (high and low dose) was significantly reduced compared with that in control Wistar rats (p < 0:01 and p < 0:05, n = 6, Figures 2(f) and 2(g)). Moreover, the p-CREB levels in TRM rats after the administration of KN93 (high dose)

CaMKII Inhibition Induces Neuronal Death In Vivo and
In Vitro. It has been observed in VaD rats that by regulating CaMKII-related signal pathways, apoptosis and inflammation can be inhibited [28]. Thus, we examined whether CaMKII inhibition induced neuronal death in TRM rats. We examined the effects of KN93 using CV staining and astrocyte immunofluorescence staining. Dead cells were recognized morphologically by changes in the size and shape and condensed nuclei. The nuclei of the pyramidal and granule cells with a well-described nuclear membrane and apparently visible nucleoli were identified as live cells. As shown in Figure 3(a), KN93 (high dose) induced death of neurons in the DG, CA3, and CA1 regions of the hippocampal regions of TRM and control Wistar rats. GFAP is a specific marker of astrocytes. As shown in Figure 3 In conclusion, our results indicate that CaMKII inhibition induced neuronal death and reactive astrocyte activation in both Wistar and TRM rat hippocampi. Furthermore, we determined the concentration-effect curve of KN93 in cells using the CCK8 assay. As shown in Figure 3(e), the cell survival rate decreased as KN93 concentration increased and 25 μmol was calculated as the halfmaximal inhibitory concentration (IC 50 ) of KN93 in PC12 cells. The protein expression of NeuN in PC12 cells and primary cultivated hippocampal neurons in the KN93processed group was lesser than that in the group of control (p < 0:05 and p < 0:01, respectively, n = 6, Figures 3(f) and 3(g)). Altogether, CaMKII inhibition by KN93 treatment caused neuronal death in vitro and in vivo.

CaMKII Inhibition Induces Apoptosis in the Hippocampi
of Wistar and TRM Rats. We next investigated whether CaMKII inhibition can induce neuronal apoptosis in TRM rats. Surprisingly, we found that the apoptotic cells were showed in the CA1, CA3, and DG regions of both control Wistar and TRM rats after administration of KN93 (high dose) by TUNEL staining in Figure 4(a). However, the apoptotic cells did not appear in the hippocampi of untreated

Oxidative Medicine and Cellular Longevity
Wistar and TRM rats. Next, we detected the expression of proteins, related to apoptosis (Figure 4(b)). Caspase-3 expression was increased in the hippocampi of Wistar and TRM rats after treatment with high doses of KN93 (all p < 0:01, n = 6, Figures 4(b) and 4(c)). Additionally, protein expression of cytochrome c in the TRM hippocampus was increased in comparison to that in control Wistar rats (p < 0:01, n = 6, Figures 4(b) and 4(c)). Thus, CaMKII inhibition by KN93 treatment induced apoptosis in the hippocampal neurons of Wistar and TRM rats.   . (b, c) The representative protein bands and data analysis of caspase-3, Bcl-2, and cytochrome c in the hippocampus of Wistar rats, TRM rats, KN93-treated (low dose) Wistar rats, KN93-treated (low dose) TRM rats, KN93-treated (high dose) Wistar rats, and KN93-treated (high dose) TRM rats. * p < 0:05, compared with the control Wistar group; # p < 0:05, compared with the control TRM group; * * p < 0:01, compared with the control Wistar group; ## p < 0:01, compared with the control TRM group. 12 Oxidative Medicine and Cellular Longevity

CaMKII Inhibition Dysregulates MAPK Signaling in
Wistar and TRM Rats. MAPKs are extremely important in regulating cellular physiological activities, including apoptosis [29,30]. Thus, we determined MAPK expression levels in Wistar and TRM rats after administration of KN93. We observed that p-ERK expression in TRM rats did not differ compared with that in healthy rats. However, expression levels of p-ERK in the hippocampal neurons of control Wistar rats and TRM rats after treatment with KN93 were substantially decreased compared with those detected in control Wistar and TRM rats (all p < 0:01, n = 6, Figures 5(a) and  5(b)). Additionally, compared with the control Wistar rats, the expression of p-JNK in TRM rats increased (p < 0:01, n = 6, Figures 5(c) and 5(d)). The expression of p-JNK in the hippocampal neurons of control Wistar rats after treatment with KN93 (high and low dose) was substantially enhanced compared with that in control Wistar rats (all p < 0:01, n = 6, Figures 5(c) and 5(d)). Moreover, p-JNK expression was upregulated in TRM rat hippocampi after treatment with KN93 (high dose) compared with that in the untreated TRM group. However, the expression of p-p38 was unaltered in both TRM and Wistar rats after treatment with KN93 (all p > 0:05, n = 6, Figures 5(e) and 5(f)). In summary, CaMKII inhibition by KN93 treatment dysregulated MAPK signaling in Wistar and TRM rats.

p-JNK Signaling Pathway Participates in Cell Death via CaMKII
Inhibition. Next, we tested whether an ATPcompetitive inhibitor of JNK, SP600125, affected KN93induced cell death in vitro. First, the CCK8 assay was used to define the effect of the p-JNK inhibitor (SP600125) on KN93-treated cell death, as shown in Figure 6(a). We found that treatment of 25 μM KN93-treated cells with 10 μM and 20 μM SP600125 enhanced cell survival, compared with the SP600125-untreated group (all p < 0:05, n = 6, Figure 6(a)).
Western blotting results showed that NeuN and p-JNK expression was decreased in the group receiving SP600125 and KN93 expression was decreased in PC12 cells and primary cultured neurons compared with that in the SP600125-untreated group (all p < 0:05, n = 6, Figures 6(b) and 6(c)). Thus, the signaling pathway of p-JNK takes part in cell death via CaMKII inhibition.

p-JNK Signaling Pathway Contributes to Apoptosis via
CaMKII Inhibition. We investigated whether p-JNK signaling participates in apoptosis via CaMKII inhibition in vitro. The expression of Q2 and Q4 was reduced in the SP600125 and KN93 groups compared with SP600125untreated cells, indicating that SP600125 reversed KN93induced apoptosis (n = 6, p < 0:05, Figures 7(a) and 7(b)). Next, several apoptosis-related proteins have been detected and the representative bands are shown in Figure 7(c). Expression of caspase-3, Bax, and cytochrome c was upregulated, but that of Bcl-2 decreased in both PC12 cells and primary hippocampal neurons treated with KN93, compared with the untreated group (all p < 0:05 or p < 0:01 or p < 0:001, n = 6, Figures 7(c) and 7(d)). These data demonstrated that KN93 activated the apoptosis pathway and induced apoptosis 24 hours after administration. Moreover, administration of SP600125 together with KN93 decreased the expression of caspase-3, Bax, and cytochrome c and increased Bcl-2 expression, in both PC12 cells and primary hippocampal neurons, compared with the SP600125untreated groups (all p < 0:05, n = 6, Figures 7(c) and 7(d)). Thus, administration of the p-JNK inhibitor SP600125 reversed the changes in these apoptosis-related proteins, indicating that p-JNK signaling participates in apoptosis through CaMKII inhibition.

Discussions
The aims of our study were at discovering the effect of CaM-KII in epilepsy and at demonstrating its relationship with neuronal death. We found that treatment with KN93 for 24 hours induced cell death in normal and TRM rats. The concentration of KN93 used in this study was based on a previous study that used the weight of Sprague-Dawley postnatal day 7 (P7) to determine KN93 dosage [25]. CaMKII is a significant component in the signaling of calcium, and its role is often debated [31]. As a small molecule and an inhibitor of CaMKII, KN93 has been shown to be neuroprotective against excitotoxic insults in vitro [32,33]. Moreover, CaM-KII performs a vital task in the survival and excitotoxicity of neurons [34]. In our study, we found that neurotoxicity, but not neuroprotection, was induced in vivo and in vitro by KN93, suggesting that sustained CaMKII inhibition (24 hours) resulted in toxic effect both in vitro and in vivo. CREB phosphorylation is the key to various extracellular signal transduction processes that play roles in the activation of downstream target genes and are involved in the occurrence and development of epilepsy [35]. Previous studies have indicated an elevated expression of CREB in epileptic animal models and patients with epilepsy. The expression of CREB in hippocampal neurons increased remarkably, compared with the control group, and the increase lasted for at least eight weeks in an epileptic pilocarpine mouse model [36]. Furthermore, p-CREB expression in the temporal lobe neocortex was enhanced in temporal lobe epileptic patients, compared with that in the group of control [37]. Nevertheless, decreased expression of p-CREB was detected in pentylenetetrazol-kindled rats compared with control rats, indicating a controversial result for p-CREB levels in different epileptic models [38]. In our study, the expression of p-CREB in TRM rats was decreased compared with that in control rats. Additionally, the expression of p-CREB in Wistar and TRM rats after treatment with KN93 was significantly decreased compared with that in control untreated animals, suggesting that p-CREB levels in CaMKII inhibition may be associated with epileptic models.
CREB is mainly involved in neuronal remodeling, learning, and memory in the mature brain [23]. Ca 2+ influx, CaMKII, and CREB in the hippocampus of chronic epilepsy rat models may be linked to damaged spatial learning and memory [38,39]. We found that TRM rats exhibited decreased CREB expression and higher escape latency and path length than the control group, suggesting that epileptic rats exhibited cognitive impairment. The path length in the KN93 treatment group increased, and the frequency of 14 Oxidative Medicine and Cellular Longevity passing across the goal and the time in the target quadrant was lower than that in the control Wistar rat group. Thus, our main finding is that CaMKII inhibition induced cognitive impairment in both Wistar and TRM rats. Furthermore, neuronal apoptosis was observed after the administration of KN93 in in vivo and in vitro experiments, although a previous study has indicated that apoptotic cell death was not found in SER rats [40]. Caspases have been considered the most important factors involved in programmed cell death in different experimental models of brain impairment, just like epileptic models. These enzymes usually exist in the cytoplasm in latent form and are activated during the later stage of apoptosis. Cytochrome c, when released into the cytoplasm, binds to apoptosisrelated factor 1 (Apaf-1) in the presence of dATP to activate the caspase family and induce apoptosis. Caspase-3 is a key mediator of apoptosis in epilepsy [41,42]. In this study, KN93 treatment led to enhanced levels of activated caspase-3. However, the expression of Bcl-2, an antiapoptotic protein found on the mitochondrial membrane, and cytochrome c was upregulated after the administration of KN93 in vitro, indicating that sustained CaMKII inhibition (24 hours) led to neuronal apoptosis.
The MAPK pathway is abundant in the central nervous system (CNS). Extracellular stimuli, such as neurotransmitters, nerve trophic factors, and growth factors, may affect synaptic transmission and cell survival via the MAPK pathway [43][44][45]. The MAPK family contains ERK1/2, JNK, and p38 MAPK proteins [46]. MAPKs are major factors regulating synaptic excitability, which participate in the regulation

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Oxidative Medicine and Cellular Longevity of cognitive impairment and epilepsy in animal models and human diseases [47,48]. A recent study found that the activity of MAPK was substantially greater in pentylenetetrazolekindled rats in comparison with the group of control [49]. The expression of p-ERK also increased during the spontaneous seizure period after pilocarpine-induced status epilepticus [50]. Blocking ERK1/2 signaling prevented epileptiform behavior in rats [51,52]. Additionally, several studies have shown that JNK is abnormally activated in epileptic models and is related to cell death [53,54]. The p38 inhibitor SB203580 decreased pathological damage to the hippocampus and reduced the epileptic frequency [55]. In our study, abnormal expression of MAPKs was observed in TRM rats, but only expression levels of p-JNK in control Wistar and TRM rats were significantly increased after treatment with KN93 compared with those in untreated animals. Moreover, the changes in apoptosis-related proteins in KN93-induced cell death were reversed by administration of the p-JNK inhibitor SP600125, indicating that p-JNK may be a potential therapeutic target for epileptic neuronal death.

Conclusions
Our study indicates that KN93-induced CaMKII inhibition results in learning and memory impairment, neuronal death, and apoptosis associated with dysregulated p-JNK. Based on the above experimental data, we found that cell death in epilepsy is partly due to the inhibition of CaM-KII. The cell death by CaMKII inhibition is related to the duration and concentration of KN93 treatment. However, elucidating the precise underlying mechanism will require further study. These experimental data lay a foundation for understanding the pathogenesis of epilepsy and clarify the toxicological effects and mechanism of CaMKII inhibition by KN93.

Data Availability
The (data type) data used to support the findings of this study are available from the corresponding author upon request.  Figure 7: The p-JNK signaling pathway contributes to KN93-induced apoptosis. (a, b) Apoptosis was observed in the control group, KN93 group, and KN93 + sp600125 group of PC12 cells using flow cytometry. * p < 0:05, compared with the control group. (c, d) Representative protein bands and analysis of data for caspase-3, Bcl-2, Bax, and cytochrome c in control groups, KN93 groups, and KN93 + sp600125 groups of PC12 cells and primary hippocampal neurons. * p < 0:05, compared with the control group; * * p < 0:01, compared with the control group; * * * p < 0:001, compared with the control group; # p < 0:05, compared with the KN93 group.