Adult male Sprague-Dawley (SD) rats, weighing 300–400 g, were used in the experiments. The rats were kept at room temperature with a 12 h light/dark cycle following surgery. They had access to food and water ad libitum and were food-deprived for 12 h before surgery. The study was approved by the ethics committee of Central South University and conducted according to the National Institutes of Health (NIH) Guide. All efforts were made to minimize animal suffering during the experiments.

A rat model of CA was established by the delivery of alternating current between the esophagus and the chest wall to induce ventricular fibrillation based on our previous study (Huang et al., 2013). All animals were fasted but given free access to water on the night prior to the experiment. All animals were anesthetized by single dose intraperitoneal injection of chloral hydrate (350 mg/kg, IP). After trachea intubation, all animals were mechanically ventilated (Harvard Model 683 Small Animal Ventilator, Harvard Apparatus, Massachusetts) with a mixture of N₂O and O₂ (70:30%) at a tidal volume of 8 ml/kg, a breathing rate of ~60 min⁻¹, adapted to maintain normocapnia (assessed by blood gas analyses) and no positive end-expiratory pressure. Polyethylene catheters were inserted into the left femoral artery and vein to monitor arterial blood pressure or inject drugs. An electrocardiogram was recorded by three subcutaneous needle electrodes, and a tympanic membrane temperature (Tty) probe was used to maintain Tty at 37.5 ± 0.2°C by using a lamp and heating pad. A BL-420s multichannel physiological signal recording system (Chengdu Taimeng Science and Technology Co., Ltd., Chengdu, China) was used to record the electrocardiogram, rectal temperature and arterial blood pressure. Ventricular fibrillation was initiated using alternating current (12 V, 50 Hz) via an esophageal electrode and ventilation was stopped. CA was identified using the following criteria: (1) the systolic arterial pressure after electrical stimulation gradually fell to below 25 mmHg; and (2) pulsations in the arterial pressure waveform disappeared. After reaching the criteria for CA, electrical stimulation was performed for 2 min followed by 5 min of observation without treatment. After 7 min of CA, cardiopulmonary resuscitation (CPR) was started: 60 breaths/min (100% oxygen), external manual chest compression at a rate of 200 min⁻¹, duty cycle 50%, and compression depth of 25% of the anterior-posterior diameter of the chest. After 2 min of CPR without restoration of spontaneous circulation (ROSC), a defibrillation attempt was performed with one biphasic shock of 1 Joule (M-Series, Zoll Corporation, Germany). CPR was continued and adrenaline administered (epinephrine, 20 μg/kg), if ROSC could not be achieved 30 s after the first defibrillation attempt. Defibrillation procedures were repeated after 30 s each. In case of 6 min of unsuccessful CPR, resuscitation was stopped and the animal was declared dead. ROSC was defined as maintenance of an unassisted MAP beyond values of 50 mmHg for at least 10 consecutive minutes. No further defibrillation or cardioversions, vasopressors or antiarrhythmic drugs were allowed after ROSC was achieved once. Breathing rate was adjusted to reach normocapnia 20 min after ROSC and maintain it until sufficient spontaneous ventilation and extubation. Application of sodium bicarbonate (8.4%) was titrated according to the blood gas analyses aiming at a base excess of 0 to –5 mmol/L, 20 min after ROSC. Animals without ROSC following standard cardiopulmonary resuscitation (CPR) for 15 min were defined as resuscitation failures.

The rats were randomly assigned into three groups for the first experiment: a sham group (no CA), a CA group, and a CA+sevoflurane post-conditioning group (CA+SE). The core temperature of the rats was continuously measured with a rectal temperature probe, which was maintained at 37 ± 0.5°C using an infrared thermolamp until awake or 4 h after ROSC. Arterial and venous catheterization, anesthesia and endotracheal intubation were performed in the sham group. An esophageal electrode was implanted in the sham group with a length of 10 cm from the incisor, and then electrical stimulation using the same parameters was performed for 90 s to induce generalized twitching but not CA. In the CA groups, ventricular fibrillation was induced for 7 min and then standard CPR was performed. Sevoflurane post-conditioning group (CA+SE): rats were subjected to ischemia induced by cardiac arrest plus sevoflurane post-conditioning. Sevoflurane, which was delivered to gas admixture (oxygen) at a concentration of 2.5% via acalibrated vaporizer (Sevorane Vapor 15.3, Abbott), was administered after 60 min stable phase via an endotracheal tube for 30 min and the inhalational oxygen and sevoflurane concentrations were maintained and monitored constantly by a gas analyzer (Datex-Oheda, Helsinki, Finland).

In the second set of experiments, rats were randomly assigned into five separate experimental groups. In the sham (S) and CA groups, rats were subjected to the same procedures as those in the first part of this experiment. The rats in the wortmannin group (CA+W) were injected intravenously with wortmannin (Sigma, St. Louis, MO, USA) at 0.6 mg/kg 45 min after successful ROSC and the rest of the procedure was same as that described in the CA group. Wortmannin was dissolved in normal saline at a concentration of 5 ml/kg. In the sevoflurane post-conditioning group (CA+SE+SAL), equal volume saline was administered in the same manner 15 min before sevoflurane exposure and the rest of protocol was same as that described in CA+SE group. Sevoflurane plus wortmannin group (CA+SE+W) was administered intravenously with wortmannin 0.6 mg/kg 15 min before sevoflurane exposure via the right femoral vein and the rest of protocol was the same as that described in the SE group above (Figure 1).

Paraffin-embedded brain tissues were cut into 5 μm sections, and Nissl staining and TUNEL assays (Beyotime Institute of Biotechnology, Nantong, China) were performed for in situ detection of apoptosis. Five fields of vision (magnification of 400×) in the hippocampal CA1 area were randomly sampled from each brain tissue sample, and Nissl-stained neuronal cells were counted. For TUNEL assay, One Step TUNEL Apoptosis Assay Kit (Beyotime, China) was used according the manufacturer's instruction. For each section, the density of TUNEL-positive cells was expressed as the number of apoptotic cells per mm². For each animal, the mean density of apoptotic cells was calculated in each region of the brain based on up to 5 sections.

Total RNA was isolated from frozen hippocampal samples using RNeasy Mini kit (Qiagen) according to the manufacturer's instructions. Five microgram RNA was used to synthesize the first strand of cDNA using random hexamer primers and SuperScript First-strand synthesis system for RT-PCR (Invitrogen). PCR was performed using SYBR Green PCR Master Mix (Applied Biosystems). Fluorescence was quantified using SDS v1.2x system software (Applied Biosystems). The forward and reverse primers used were: TFAM, GAAAGCACAAATCAAGAGGAG, CTGCTTTTCATCATGAGACAG; NRF-1, TTACTCTGCTGTGGCTGATGG, CCTCTGATGCTTGCGTCGTCT; PGC-1α, GTGCAGCCAAGACTCTGTATGG, GTCCAGGTCATTCACATCAAGTTC; and GADPH, GGGTCAGAAGGATTCCTATG, GGTCTCAAACATGATCTGGG.

The mitochondrial DNA (mtDNA) copy number was measured using real-time PCR as described in a previous study (Edwards et al., 2010). The animals were decapitated at 4, 12, 24, and 72 h after reperfusion and the hippocampal tissue was isolated rapidly. Total DNA was extracted from the brain tissue using QIAamp DNA extraction kit (Qiagen, Shanghai, China). In total, 10 ng of genomic DNA was used for amplifying mtDNA and nuclear DNA markers. The mtDNA was amplified using primers specific for the mitochondrial cytochrome b (Cyt B) gene, and the mitochondrial DNA copy number was normalized to nuclear DNA copy number by amplifying β-actin nuclear gene. The oligonucleotides (probes) for TaqMan PCR were labeled with fluorescent reporter dye FAM (6-carboxyfluorescein) at the 5′ end and fluorescent BHQ-1 dye at the 3′ end. Real-time PCR amplification was performed using a LightCycler™ 480 II Probes Master kit (Roche Applied Science, Mannheim, Germany). The fluorescence threshold (Ct) value was calculated using LightCyclerTM 480 II Probes system software (Roche Applied Science, Germany), and the 2^−ΔΔCt method was used to calculate the relative levels of expression (Livak and Schmittgen, 2001). The primer and probe sequences are listed in Table 1.

The mitochondrial fraction of the harvested brain tissues (hippocampus) was prepared as previously described (Liao et al., 2014). The cytosolic and mitochondrial fractions of the harvested brain tissues were prepared. Each brain tissue sample was homogenized in ice-cold lysis buffer [200 mM mannitol, 80 mM HEPES-KOH (pH 7.4), and protease inhibitor cocktail] by 35 strokes of gentle pounding in a glass tissue grinder. Homogenates were centrifuged at 750 × g for 10 min at 4°C. After removing a portion of the supernatant, the remaining supernatant was centrifuged at 8000 × g for 20 min at 4°C. The mitochondrial fraction was obtained after washing the resultant pellets three times and resuspending the pellets in lysis buffer.

Hippocampal tissues were harvested from each of the two hemispheres at 24 and 72 h after reperfusion. Hippocampal protein extracts and Western blot analysis were performed as previously described (Kocki et al., 2015) using 20–50 μg of protein extract per lane. Equal amounts of protein were loaded in each well and subjected to 10% sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE). Separated proteins were then transferred from the gel to polyvinylidene fluoride (PVDF; Millipore, Bedford, MA, USA) membranes and blocked in 5% non-fat dry milk prepared in 1× TBST. The membranes were incubated with primary antibodies overnight at 4°C. The membranes were incubated with primary antibodies for caspase-3 and -9; PGC-1α, NRF-1, and HSP 60 (all from Santa Cruz Biotechnology Inc.); TFAM, p-Akt (Ser⁴⁷³), Akt and GAPDH (Cell Signaling Technology, Beverly, MA, USA); Trx-2, Prx-3, and VDAC (Abcam, Cambridge, MA, USA). The membranes were washed with 1X TBST and the membranes incubated with appropriate secondary antibodies for 2 h at room temperature. The blots were developed using an ECL plus detection system (Beyotime Institute of Biotechnology) and relative band density was measured using FluorChem FC2 System (NatureGene Corp., USA).

ROS formation was assayed using a previously described dichlorodihydrofluorescein diacetate (DCFH-DA) assay (HaMai et al., 2001). In brief, 10 μl of mitochondria (5–10 μg) was suspended in 170 ml HEPES buffer (120 mM NaCl, 2.5 mM KCl, 1.2 mM NaH₂PO₄, 0.1 mM MgCl₂, 5.0 mM NaHCO₃, 6.0 mM glucose, 1.0 mM CaCl2, 10 mM HEPES, pH 7.4) in 96-well-plates; 20 ml of 100 mM DCFH-DA was added to each well, for a final volume of 200 ml. Fluorescence was read at an excitation wavelength of 485 nm and an emission wavelength of 530 nm using a fluorescent plate reader (Genios, TEC AN). Increased fluorescence intensity was considered to be indicative of an increase in intracellular ROS.

Changes in MMP were monitored in the presence of the fluorescent dye Rhodamine 123 (Rh123), as described previously (Emaus et al., 1986) with modifications. In brief, 10 μl of mitochondria (5–10 μg) was suspended in 90 μl of assay buffer (15 mM sucrose, 5 mM MgCl₂, 5 mM sodium succinate, 5 mM K₂HPO₄, 20 mM HEPES, pH 7.4) in 96-well-plates and was incubated for 30 min in the presence of 20 μl of 100 μg/mL Rh123. The change of MMP was determined by measuring the fluorescence change in the reaction mixture at an excitation wavelength of 485 nm and an emission wavelength of 538 nm. The results were expressed as fluorescence intensities.

MPTP opening was determined using a commercially available kit (GENMED SCIENTIFICS INC. U.S.A) according to the manufacturer's instructions. Isolated mitochondria were co-loaded with 1 mM calcein AM and 1 mM CoCl₂ at room temperature in working solution (pH = 7.2). The working solution consists of 10 mM EGTA-CaEGTA buffer (free Ca²⁺ concentration 100 nM), 3 mM free Mg²⁺, 20 mM taurine, 0.5 mM dithiothreitol, 20 mM imidazole, 0.16 M potassium 4-morpholineethanesulfonate and 10 mg/ml fatty acid-free bovine serum albumin. MPTP opening was measured directly using a combination of calcein AM and CoCl₂. Calcein AM, which fluoresces upon binding with Ca²⁺, was used to detect transient MPTP opening in isolated mitocchondria. This was achieved by monitoring changes in mitochondrial Ca²⁺ levels in the presence of CoCl₂, which quenched the cytosolic Ca²⁺ signal produced by calcein AM. The fluorescence of calcein AM was monitored at an emission/excitation wavelength of 530/488 nm. The extent of Ca²⁺-induced MPTP opening was estimated by determining the difference in fluorescence intensity.

All measurement data were expressed as mean ± standard deviation (SD), and all statistical analyses were performed using statistical software (SPSS version 13.0). Comparison of the same parameters among groups was done using one-way analysis of variance (ANOVA), and the difference between pairs of means was tested post-hoc with Fisher's Least Significant Difference (LSD) test. The difference in survival rates among the various groups was compared using Wilcoxon (Gehan) survival analysis. P < 0.05 was considered statistically significant.

The physiological parameters (MAP, pH, and glucose) and levels of arterial blood gas tensions including PaCO₂ and PO₂ were monitored before, during, and after (1 and 3 h post-ROSC) CA (Table 2). The baseline parameters were similar across different animal groups with no significant difference. Additionally, there were no significant differences in body weight, basal body temperature, breathing frequency, and heart rate of the rats among three groups.

Ventricular fibrillation was successfully induced in all rabbits in the CA group and the two CA+SE groups. There were no significant differences in the resuscitation parameters among the groups (P > 0.05; Table 3). The 72 h survival rates in the sham group, CA group, CA+SE 100% (6/6), 43.75% (7/16), 62.5%, and (9/16), respectively. The survival rate of rabbits in the sham group was significantly different from those in the 2 groups with CA. In addition, a significant difference in the survival rate was found between the CA+SE and the CA group (P < 0.05; Figure 2). The number of deaths in different groups at each time point has shown in Table 4.

Delayed neuronal death in the hippocampus was detected at 72 h after reperfusion. Compared with the sham group (100%), the number of neurons in other two groups with CA was significantly reduced (P < 0.01). In the CA group, the number of neurons was significantly reduced (46.98 ± 8.36%), and the nucleus was compressed; a Nissl body was not found in the cytoplasm. Compared with the CA group, many neurons with normal nucleus were found in the CA+SE group (70.62 ± 6.23%) and there were many Nissl bodies observed in the cytoplasm, suggesting that sevoflurane preserved more intact neurons (Figures 3A,B).

TUNEL staining showed many strongly TUNEL-positive apoptotic cells in the CA group, and a few weakly positive cells in the CA+SE groups. However, no TUNEL-positive cells were found in the sham group. Compared with the sham group, the TUNEL positive cells were significantly increased in the CA and CA+SE groups (P < 0.01). However, the TUNEL positive cells in the CA+SE group were significantly lower than those in the CA group (185.36 ± 40.63/mm² in CA group vs. 95.69 ± 25.68/mm² in CA+SE group, P < 0.05, Figures 3C,D).

Figure 3E represents the typical results of Western blot analysis of cleaved caspase-3 and -9 at 24 and 72 h after reperfusion, respectively. There was low expression of cleaved caspase-3 and -9 in the sham group. The quantitative analysis in Figure 3F indicated that there were higher cleaved caspase-3 and -9 expressions in the CA group than in the CA+SE group, suggesting that sevoflurane post-conditioning can efficiently attenuate neuronal apoptosis (P < 0.05).

Mitochondrial DNA (mtDNA) replication is necessary for mitochondrial biogenesis and is a typical marker for this process. Hence, we detected the relative abundance of mitochondria in the reperfused cerebral hippocampal tissue by measuring the mtDNA content using quantitative real-time PCR. The mtDNA content was examined 4, 12, 24, and 72 h after reperfusion. Compared with the sham group, the mtDNA content was increased in the CA and CA+SE groups in a time-dependent manner and peaked at 24 h (P < 0.05). In the CA+SE group, the mtDNA content were 1.4-, 1.5-, 1.3- and 1.2-fold higher, respectively, than those of the CA group at each time point (P < 0.05, Figure 4A).

Additionally, to determine the intrinsic specificity in mitochondrial biogenesis, we examined PGC-1α, NRF-1, and TFAM -transcription factors that have been reported to control mitochondrial gene expression. The mRNA expression levels of PGC-1α, NRF-1and TFAM were examined at 4 h, 12, 24, and 72 h after reperfusion by quantitative real-time PCR. Low levels of PGC-1α, NRF-1, and TFAM mRNA were observed in the hippocampus of the sham group. Compared with the sham group, PGC-1α, NRF-1, and TFAM mRNA were significantly induced in CA and CA+SE groups in a time-dependent manner and peaked at 24 h (P < 0.05). However, in contrast with the CA group, sevoflurane post-conditioning markedly increased the expression of PGC-1α, NRF-1, and TFAM mRNA in the hippocampus after 72 h of reperfusion (P < 0.05, Figure 4B).

To gain additional evidence for sevoflurane protective effect on the mitochondrial biogenesis, the protein expression levels of PGC-1α, NRF-1, and TFAM were investigated using Western blot analysis. Protein levels of PGC-1α, NRF-1, and TFAM were significantly increased at 24 and 72 h after reperfusion, when compared to the sham group (P < 0.05). Compared with the CA group, administration of sevoflurane significantly elevated the protein expression levels of PGC-1α, NRF-1, and TFAM (P < 0.05, Figures 4C,D).

Additionally, PI3K and its downstream protein Akt are known to play an important role in survival against ischemia/reperfusion-induced brain damage. To investigate whether Akt is involved in sevoflurane-induced neuroprotection, we evaluated the expression of Akt and its activated, phosphorylated form [p-Akt (Ser⁴⁷³)]. Total Akt expression was comparable in all experimental groups. p-Akt (Ser⁴⁷³) expression was significantly increased in the CA and CA+SE groups compared with sham-operated controls (P < 0.05). However, the expression of p-Akt (Ser⁴⁷³) was apparently increased by sevoflurane post-conditioning, when compared with the CA group (P < 0.05, Figures 4E,F).

To gain additional evidence for the neuroprotection induced by sevoflurane post-conditioning, the expression level of several proteins normally enriched in mitochondria was investigated. Heat-shock protein 60 (HSP60), an abundant protein located primarily in mitochondria, was found to rise significantly 24 and 72 h after reperfusion in the CA+SE group, when compared with the CA group. Similarly, mitochondria-specific antioxidant enzymes such as peroxiredoxin 3 (Prx3) and thioredoxin 2 (Trx2) were examined by Western blot analysis at 24 and 72 h after reperfusion in the mitochondrial fraction. Compared with the CA group, the sevoflurane post-conditioning group had much higher protein expression of mitochondrial Prx3 and Trx2 at 24 and 72 h after reperfusion (Figures 5A,B).

To determine if the protective effect of sevoflurane post-conditioning is due to a reduction in ROS production, mROS production was measured by using DCFH-DA at 24 and 72 h after reperfusion. As shown in Figure 6A, ROS production in mitochondria of hippocampal neurons in the CA group markedly increased to 269.7% at 1 day, then gradually decreased to 203.5% at 3 days compared to sham group. On the other hand, sevoflurane exhibited mROS production levels of 156.8% at 1 day and 137.3% at 3 days compared to sham group, which suggested that sevoflurane was able to inhibit the generation of mROS in hypoxic hippocampal neurons.

To determine mitochondrial integrity, we detected the opening of mitochondrial permeability transition pore (MPTP), as well as mitochondrial membrane potential (MMP). Opening of the MPTP is important for mitochondrial events leading to programmed cell death. As compared to the sham group, the activity of MPTP in hippocampal neurons significantly increased in the CA group (356.8% at 1 h and 276.1% at 3 days, P < 0.05) and sevoflurane post-conditioning could decline the activity of MPTP in hippocampal neurons (214.5% at 1 day and 189.2 at 3 days, P < 0.05, Figure 6B).

The loss of MMP is the result of the opening of permeability transition pores. As shown in Figure 6C, global ischemic injury induced a significant loss of MMP in the CA group in mitochondria hippocampal tissue (80.25% at 1 h and 82.37% at 3 days, P < 0.05). However, sevoflurane post-treatment rescued markedly the loss of MMP in the therapy group (90.63% at 1 h and 87.25% at 3 days, P < 0.05).

Similarly as aforementioned, sevoflurane significantly increased p-Akt (Ser⁴⁷³), mitochondrial biogenesis-related proteins such as PGC-1α, NRF-1 and TFAM, and mitochondria-specific antioxidants including HSP60, Trx2, and Prx2 in hippocampal tissue, compared with the sham and control groups at 24 h after reperfusion. Administration of PI3K inhibitor wortmannin decreased the elevation of p-Akt level, mitochondrial biogenesis-related proteins and mitochondria-specific antioxidants induced by sevoflurane post-conditioning (P < 0.05, Figures 7A–D). However, total Akt expression was not obviously changed in all groups (P > 0.05). There was no significant difference in protein levels between the control group and the wortmannin alone (CA+W) group (P > 0.05).

Sevoflurane post-conditioning also ameliorated mitochondrial ROS generation and restored the mitochondrial integrity. Nevertheless, wortmannin treatment eliminated the beneficial biochemical processes of sevoflurane, shown as increased mitochondrial ROS generation, and loss of MMP and opening of MPTP at 24 h of reperfusion (P < 0.05, Figures 7E–G). There was no significant difference in all the parameters between the control group and the CA+W group (P > 0.05).

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.