Thirty male BALB/c mice (age, 6–8 weeks old, weight, 23±4 g) were maintained in a standard animal laboratory under controlled conditions (light between 7:00 a.m. and 6:00 p.m.; 50–70% humidity; 24°C) and with ad libitum access to food and water. The mice were purchased from SLAC Laboratory Animal Co., Ltd. (Shanghai, China). All experimental procedures were approved by the Institutional Animal Care and Ethics Committee of The First Affiliated Hospital of Dalian Medical University (Dalian, China).

HI/R method was performed according to previous guidelines, with minor modifications (21–24). Briefly, mice were anesthetized with 99% ether (Invitrogen, Grand Island, NY, USA). Following anesthesia, the abdomen was shaved and cleansed with 10% povidone-iodine. Subsequently, mice underwent a median laparotomy. The hepatoportal vein, hepatic artery and hepatic duct were sought out and separated, after which they were clamped for 30 min, and the abdomen was temporarily closed with a suture. Mice were sacrificed by decollation for experimental assays following a 6 h reperfusion period with an atraumatic vascular clamp, during which they were maintained at a constant temperature via the use of a heated blanket.

The chemical structure of PF is shown in Fig. 1. PF (Sigma-Aldrich China, Inc., Shanghai, China), with a purity >98%, was dissolved in physiological saline, according to the manufacturer's instructions and injected into the tail vein of the mice 5 min prior to HI/R injury. A total of 30 mice were randomized into five groups, each containing six animals: Sham, Vehicle, and PF treatment groups (5, 10 and 20 mg/kg) (25). The sham (control) group did not undergo the clamping operation, whereas the vehicle group underwent the procedure before injections of the same volume of physiological saline. PF treatment groups underwent the procedure of HI/R prior to injection with 5, 10, or 20 mg/kg of PF via the tail vein. Following the reperfusion period, and 24 h following clip removal, the blood and liver samples of all mice were collected and stored at −80°C prior to analysis. Blood samples were taken from the suprahepatic inferior vena cava and were centrifuged at 3,500 × g for 5 min, in order to obtain serum at room temperature for determination of ALT and AST levels. Liver tissue samples from each animal were measured for hepatic tissue SOD, MDA, glutathione (GSH), glutathione peroxidase (GSH-PX, NF-κB, TNF-α, IL-1β and IL-6 levels, together with evaluating the activities of caspase-3.

Liver injury was measured by serum levels of ALT and AST. Blood samples were centrifuged at 3,500 × g for 5 min, in order to obtain serum at room temperature. Serum levels of ALT and AST were measured using an automated analyzer (Model 200; Toshiba, Tokyo, Japan). ALT and AST levels were determined as described previously (26) and expressed as international units per liter (U/l).

Liver tissue was homogenized using a homogenizer (ZW-800D, Wenzhou Weike Biological Laboratory equipment Co., Ltd., Wenzhou, China) and centrifuged at 13,200 × g for 20 min at 4°C. Following centrifugation, the supernatant was retained for storage at −80°C. Subsequently, 15 µg nuclear protein, extracted from liver tissue using a powder with liquid nitrogen and lysed in radioimmunoprecipitation assay buffer, was analyzed, in order to detect NF-κB, TNF-α, IL-1β and IL-6 levels using commercially available ELISA kits (R&D Systems, Inc., Minneapolis, MN, USA), and absorbance was measured using a TECAN Sunrise ELISA Reader (Tecan Group Ltd., Männedorf, Switzerland) at 450 nm.

Blood samples were centrifuged at 1,000 × g for 10 min to obtain serum at room temperature. The supernatant was stored at −80°C until assays for SOD, MDA GSH, and GSH-PX were established. The enzymatic activities of SOD, MDA GSH, and GSH-PX in the serum homogenate was evaluated according to the manufacturer's instructions (Shimadzu Corporation, Kyoto, Japan).

Liver tissue was homogenized using a homogenizer (ZW-800D, Wenzhou Weike Biological Laboratory equipment Co., Ltd.), and the enzymatic activity of SOD in hepatic tissue homogenate was evaluated by determining the rate (U/mg protein) of inhibition of nucleotide oxidation. The level of MDA (nmol/mg protein) in the serum homogenate was measured spectrophotometrically using the Sunrise Remote R-microplate reader at 532 nm. The level of GSH (mmol/mg protein) in the serum homogenate was evaluated by monitoring the reduction of dithiobis-2-nitrobenzoic acid (4 mg/ml in methanol), after which, readings were taken spectrophotometrically using the Sunrise Remote R-microplate reader at 412 nm. GSH-PX activity (U/mg protein) in the serum homogenate was determined at the end of the reaction, using the Sunrise Remote R-microplate reader, by measuring absorption at 412 nm.

Caspase-3 activity was analyzed 6 h following HI/R injury. Liver tissue was homogenized using a homogenizer (Haimen Botai Experimental Equipment) and centrifuged at 13,200 × g for 20 min at 4°C. Following centrifugation, the supernatant was stored at −80°C for subsequent analysis. In accordance with the manufacturer's instructions, the activity of caspase-3 was analyzed by the cleavage of chromogenic caspase substrates (Beyotime Institute of Biotechnology, Nantong, China).

All results were expressed as the mean ± standard deviation. Comparisons between groups were performed using Student's t-test and one-way analysis of variance. All statistical analyses were performed using SPSS 15.0 software (SPSS, Inc., Chicago, IL, USA). P<0.05 was considered to indicate a statistically significant difference.

Levels of serum ALT in the vehicle group were significantly increased from 18.53±3.23 to 1956.53±34.89 U/l (P<0.01, n=6) 6 h following HI/R, as compared with the sham group (Fig. 2A). Following treatment with PF, the levels of serum ALT were significantly reduced from 1956.53±34.89 to 200.89±36.44 (5 mg/kg treatment group, P<0.01, n=6), 189.53±26.89 (10 mg/kg treatment group, P<0.01, n=6) and 168.46±20.14 U/l (20 mg/kg treatment group, P<0.01, n=6), as compared with the vehicle group (Fig. 2A). Similarly, the serum levels of AST in the vehicle group were significantly enhanced from 20.58±3.45 to 3546.89±45.89 U/l (P<0.01, n=6) 6 h following HI/R, as compared with the sham group (Fig. 2B). Conversely, the serum AST levels of the PF-treated groups markedly decreased from 3546.89±45.89 to 486.56±26.78 (5 mg/kg treatment group, P<0.01, n=6), 351.46±32.89 (10 mg/kg treatment group, P<0.01, n=6) and 298.46±46.11 U/l (20 mg/kg treatment group, P<0.01, n=6), as compared with the vehicle group (Fig. 2B).

In order to corroborate the effects of PF on oxidative stress during HI/R injury of mice, the levels of MDA, and the activities of SOD, GSH and GSH-PX in hepatic tissue were evaluated (Fig. 3A–D). The levels of MDA in the vehicle group were significantly increased from 2.15±0.12 to 6.23±0.52 nmol/mg protein (P<0.01, n=6) 6 h following HI/R, as compared with the sham group (Fig. 3A). Following treatment with PF, the levels of MDA were significantly reduced from 6.23±0.52 to 4.12±0.32 (5 mg/kg treatment group, P<0.01, n=6), 3.62±0.31 (10 mg/kg treatment group, P<0.01, n=6) and 2.89±0.45 nmol/mg protein (20 mg/kg treatment group, P<0.01, n=6), as compared with the vehicle group (Fig. 3A).

Conversely, the activity of SOD in the vehicle group was significantly reduced from 189.36±5.64 to 86.89±8.69 U/mg protein (P<0.01, n=6) 6 h following HI/R, as compared with the sham group (Fig. 3B). In the PF treatment groups, the activity of SOD was significantly enhanced from 86.89±8.69 to 114.86±6.53 (5 mg/kg treatment group, P<0.01, n=6), 126.89±7.56 (10 mg/kg treatment group, P<0.01, n=6), and 149.26±9.56 U/mg protein (20 mg/kg treatment group, P<0.01, n=6), as compared with the vehicle group (Fig. 3B).

The contents of GSH in the vehicle group were significantly decreased from 52.63±3.56 to 22.56±4.01 µg/g protein (P<0.01, n=6), as compared with the sham group, 6 h following HI/R(Fig. 3C). Whereas, following PF treatment, the levels of GSH significantly increased to 36.89±5.01 (5 mg/kg treatment group, P<0.01, n=6), 39.58±8.23 (10 mg/kg treatment group, P<0.01, n=6) and 43.56±9.26 µg/g protein (20 mg/kg, treatment group, P<0.01, n=6) (Fig. 3C).

The activity of GSH-PX in the vehicle group declined from 63.89±6.35 to 21.86±3.59 U/mg protein (P<0.01, n=6) as compared with the sham group (Fig. 3D0 6 h following HI/R. In the PF treatment groups, the activity of GSH-PX was significantly increased to 38.95±6.36 (5 mg/kg treatment group, P<0.01, n=6), 42.98±6.31 (10 mg/kg treatment group, P<0.01, n=6) and 49.86±8.29 U/mg protein (20 mg/kg treatment group, P<0.01, n=6) (Fig. 3D).

In order to investigate the effects of PF on inflammatory mediators during HI/R injury in mice, the present study evaluated the expression levels of NF-κB, TNF-α, IL-1β and IL-6 in hepatic tissue (Fig. 4A–D). Expression levels of NF-κB in the vehicle group significantly increased from 9.63±1.23 to 45.26±3.65 ng/mg protein (P<0.01, n=6) 6 h following HI/R, as compared with the sham group (Fig. 4A). In the PF treatment groups, the expression of NF-κB significantly decreased from 45.26±3.65 to 29.86±2.56 (5 mg/kg treatment group, P<0.01, n=6), 22.59±3.01 (10 mg/kg treatment group, P<0.01, n=6), and 19.68±2.99 ng/mg protein (20 mg/kg treatment group, P<0.01, n=6), as compared with the vehicle group (Fig. 4A).

Similarly, the expression levels of TNF-α in the vehicle group were increased from 76.56±6.59 to 289.65±8.56 pg/mg protein (P<0.01, n=6) as compared with the sham group (Fig. 4B). Following treatment with PF, the expression levels of TNF-α significantly decreased from 289.65±8.56 to 210.98±9.21 (5 mg/kg treatment group, P<0.01, n=6), 195.89±8.56 (10 mg/kg treatment group, P<0.01, n=6) and 168.56±6.89 pg/mg protein (20 mg/kg treatment group, P<0.01, n=6), as compared with the vehicle group (Fig. 4B).

The expression levels of IL-1β in the vehicle group were markedly increased from 2.65±0.25 to 5.26±0.59 pg/mg protein (P<0.01, n=6), as compared with the sham group (Fig. 4C). In the PF treatment groups, the expression levels of IL-1β were significantly reduced to 3.99±0.68 (5 mg/kg treatment group, P<0.01, n=6), 3.25±0.98 (10 mg/kg treatment group, P<0.01, n=6) and 3.04±0.58 pg/mg protein (20 mg/kg treatment group, P<0.01, n=6) (Fig. 4C).

The expression levels of IL-6 in the vehicle group were markedly increased from 1.65±0.26 to 5.01±0.35 mg/g protein (P<0.01, n=6), as compared with the sham group (Fig. 4D). In the PF treatment groups, the expression levels of IL-6 were significantly reduced to 3.14±0.31 (5 mg/kg treatment group, P<0.01, n=6), 2.98±0.36 (10 mg/kg treatment group, P<0.01, n=6) and 2.56±0.33 pg/mg protein (20 mg/kg treatment group, P<0.01, n=6) (Fig. 4D).

In order to confirm that PF was able to reduce caspase-3 activity, a colorimetric analysis was conducted (Fig. 5). Caspase-3 activity in the vehicle group was markedly increased to 6.58±0.16 (P<0.01, n=6), as compared with the sham group. Whereas, in the PF treatment groups (5, 10 and 20 mg/kg), there was a marked decrease in caspase-3 activity to 3.25±0.21 (P<0.01, n=6), 2.98±0.25 (P<0.01, n=6), and 2.26±0.31 (P<0.01, n=6), respectively, as compared with the vehicle group.