All experiments and animal care were conducted in accordance with the Provision and General Recommendation of Chinese Experimental Animals Administration Legislation and were approved by the Ethics Committee of Science and Technology Department of Jiangsu [approval no. SYXK (SU) 2016-0011]. A total of 30 Male C57BL/6 mice (6-8 weeks old; weight: 18-22 g) were purchased from Nanjing Biomedical Research Institute and were randomly maintained on a basal diet [the normal diet (ND group); 360 kcal/100 g; comprising 13.3 g/100 g fat, 26.2 g/100 g protein and 60.5 g/100 g carbohydrate] or a HFHC diet (506.8 kcal/100 g; comprising 10 g/100 g lard, 2 g/100 g cholesterol, 5 g/100 g egg yolk power, 10 g/100 g sucrose, 2 g/100 g propylthiouracil and basal diet, 72.8 g/100 g). Animals were housed at 24˚C and 55% relative humidity in a barrier facility under a 12 h light/dark cycle with free access to food and water. The basal diet and HFHC diet were provided by the Jiangsu Xietong Medical and Biological Corporation. Subsequently, mice were randomly divided into the following three groups (n=6-8 per group): Vehicle-treated chow group, vehicle-treated HFHC group and GAA-treated HFHC group (25 or 50 mg/kg/day). The administration concentration was determined to have therapeutic effect in a previous study (20). HFHC-fed mice were gavaged with GAA, which was purchased from Shanghai Yousi Biotechnology Co., Ltd. and was dissolved in 0.5% sodium carboxymethyl cellulose (Sigma-Aldrich; Merck KGaA) for 12 weeks. All mice were sacrificed by cervical dislocation after overnight fasting at the termination of the experiment. Subsequently, mouse liver tissue was obtained. Before euthanasia, 300 µl blood was collected in the 3% isoflurane-anaesthetized (ForeneTM; Abbott Laboratories SA; oxygen flow rate of 4 l/min) mice by retroorbital venous plexus method. All animal experiments were performed in accordance with the approved guidelines.

Serum was collected after sacrifice instantaneously by centrifugation at 1,200 x g for 15 min at room temperature. The serum lipids, including total cholesterol (TC; cat. no. A111-1-1), total triglycerides (TG; cat. no. A110-1-1), low-density lipoprotein cholesterol (LDL-c; cat. no. A113-1-1) and high-density lipoprotein cholesterol (HDL-c; cat. no. A112-1-1) were detected. Aspartate transaminase (AST; cat. no. C010-2-1) and alanine transaminase (ALT; cat. no. C009-2-1) levels were evaluated to assess the hepatic injury. All serum lipids were evaluated by commercial kits (Nanjing Jiancheng Bioengineering Institute). ELISA measurements of serum IL-1β (cat. no. EMC001b.96), TNF-α (cat. no. EMC102a.96) and IL-6 (cat. no. EMC004.96) were performed following the manufacturer's protocol (Neobioscience Technology Co., Ltd.).

Histopathological analysis was performed with standardized specimens from specified portions of liver. Liver tissues were fixed in 4% paraformaldehyde for 4 h at room temperature, dehydrated in a series of ethanol and embedded in paraffin wax. Sections (4-mm-thick) were stained with hematoxylin-eosin (H&E) at room temperature for 15 min before being analyzed under a light microscope (BX53; Olympus Corporation). The NAFLD activity score (NAS) of each group was calculated as previously described (21). Lipid droplets of the fresh liver samples were stained by Oil Red O (cat. no. O8010; Beijing Solarbio Science & Technology Co., Ltd.) for 15 min at room temperature and analyzed to quantify lipid content by cell imaging under an Olympus-BX53 light microscope. Sirius Red (SR; cat. no. ab150681; Abcam) staining, anti-CD68 (cat. no. ab31630; Abcam; 1:200) and anti-F4/80 antibodies (cat. no. ab16911; Abcam; 1:200) were used for histological analysis under a light microscope (BX53; Olympus Corporation). Areas of stained droplets (Sirius Red staining for 1 h at room temperature) or SR and the intensity of immunohistochemical staining were determined using ImageJ 1.8.0 (National Institutes of Health).

Lipids extracted from murine liver tissue were dissolved in isopropanol, after which hepatic TG and TC contents were detected as aforementioned. Hepatic malondialdehyde (MDA) was measured using a MDA assay kit (TBA method; cat. no. A003-1-2; Nanjing Jiancheng Bioengineering Institute) in accordance with the manufacturer's protocols. Briefly, 0.1 ml sample was mixed with 1,1,3,3-tetramethoxypropane, 0.75 ml TBA working solution (0.37%) and perchloric acid. The resulting solution was incubated at 95˚C for 45 min. After cooling (10 min in ice water bath), the flocculent precipitate was removed by centrifugation (4,000 x g 10 min at room temperature). The supernatant was analyzed at 532 nm using a multi-scan spectrum microplate spectrophotometer at room temperature. Hepatic superoxide dismutase (SOD) levels was measured using a SOD assay kit (WST-1 method; cat. no. A001-3-2; Nanjing Jiancheng Bioengineering Institute). Briefly, the tissue were lysed with No-nidet P-40 lysis buffer (1% NP-40, 50 mmol/l Tris-HCl [pH 7.5], 0.05 mmol/l ethylenediamine tetra-acetate) for 20 min at 4˚C. The lysates were centrifuged at 300 g for 10 min, and 20 µl of this sample solution was used for determination of SOD enzyme activity according to the manufacturer's instructions. The value for each treatment group was converted to the percentage of control.

Total RNA extraction was performed using TRIzol^® (Vazyme Biotech Co., Ltd.) according to the manufacturer's protocol. The purity and concentration of RNA was determined by spectrophotometric analysis via absorbance at 260/280 and 260/230 nm. RNA concentrations were equalized and converted to cDNA using Hiscript II reverse transcriptase (Vazyme Biotech Co., Ltd.) according to the manufacturer's protocol. Gene expression was measured using a LightCycler 96 Real-Time PCR System (Roche Diagnostics) using SYBR-green dyes (Roche Diagnostics). The thermocycling conditions were as follows: Initial denaturisation at 95˚C for 10 min followed by 40 cycles for 10 sec at 95˚C, 10 sec at 55˚C and 30 sec at 72˚C, with a final elongation step at 72˚C for 7 min. All data were analyzed using GAPDH gene expression as an internal standard. Relative gene expression levels were analyzed using the 2^-ΔΔCq method (22,23). The sequences of the murine PCR primers were as follows: TNF-α forward, 5'-AAGGGAGAGTGGTCAGGTTG-3' and reverse, 5'-TCTGTGAGGAAGGCTGTGC-3'; IL-1β forward, 5'-AACCTGCTGGTGTGTGACGTTC-3' and reverse, 5'-CAGCACGAGGCTTTTTTGTTGT-3'; IL-6 forward, 5'-CGGAGAGGAGACTTCACAGAG-3' and reverse, 5'-CATTTCCACGATTTCCCAGA-3'; α-smooth muscle actin (α-SMA) forward, 5'-CCCTGAAGTATCCGATAGAACA-3' and reverse, 5'-TGCCTGGGTACATGGTAGTG-3'; TGF-β forward, 5'-CTTTGTACAACAGCACCCGC-3' and reverse, 5'-TAGATTGCGTTGTTGCGGTC-3'; MMP-13 forward, 5'-GTGACTCTTGCGGGAATCCT-3' and reverse, 5'-CAGGCACTCCACATCTTGGT-3'; and GAPDH forward, 5'-AACAGCAACTCCCACTCTTC-3' and reverse, 5'-CCTGTTGCTGTAGCCGTATT-3'.

Liver tissues were homogenized at 4˚C with lysis buffer (50 mM Tris-HCl, pH 8.0, 150 mM NaCl, 1% Nonidet P-40, 0.5% sodium deoxycholate, 0.1% SDS, 1 mM EDTA and protease inhibitors). After sonication, the samples were centrifuged for 10 min at room temperature at 13,000 x g. The protein concentration were then detected by performing a BCA assay (Beyotime Institute of Biotechnology). 10% SDS-PAGE was conducted by loading equal amounts of protein per lane (40 µg). Gels were then transferred to PVDF membranes (EMD Millipore) and blocked with 5% non-fat milk in TBST buffer for 1 h at room temperature. The membranes were then incubated with the indicated primary antibodies overnight at 4˚C, and washed three times with TBST (containing 0.1% Tween 20 in TBS) for a total of 10 min. Thereafter, the membranes were incubated with horseradish peroxidase-conjugated secondary antibody (1:2,000; cat. no. A0208; Beyotime Institute of Biotechnology) for 1 h at room temperature and washed three times with TBST. The blots were visualized with the Amersham ECL Plus (Amersham; Cytiva) western blotting detection reagents according to the manufacturer's protocol. The primary antibodies (all dilutions were 1:500) including glucose-regulated protein 78 (GRp78; cat. no. 3177), phosphorylated (p)-eukaryotic initiation factor-2α (eIF-2α; cat. no. 3398), eIF-2α (cat. no. 5324), p-JNK (cat. no. 4668), JNK (cat. no. 9252), ERp57 (cat. no. 2887S), p-AKT (cat. no. 4060), AKT (cat. no. 9272) p-MAPK (cat. no. 4370), MAPK (cat. no. 9102) and GAPDH (cat. no. 8884) were obtained from Cell Signaling Technology, Inc. Immunoreactive signals were detected with Chemi-Lumi One Ultra (Tanon Science and Technology Co., Ltd.). The densitometric analysis of the blots was performed by Image Pro Plus 6.0 software (Media Cybernetics, Inc.).

Statistical analysis was performed using Prism version 7.0 statistical software (GraphPad Software Inc.). All quantitative values are presented as the mean ± SEM. Statistical data were analyzed using one-way ANOVA with Dunnett's post hoc test. P<0.05 was considered to indicate a statistically significant difference.

The effect of GAA on the weight gain and metabolic features of serum lipids in C57BL/6J mice is demonstrated in Fig. 1. Mice fed with a HFHC diet had significantly increased body weights, without significant difference in food intake, compared with the ND-fed mice (Fig. 1A and B). Weight gain was also accompanied by serum lipid disorder, including higher TG, TC, LDL-cholesterol (LDL-c) and HDL-cholesterol (HDL-c) in the HFHC group compared with the ND-fed group (Fig. 1C-F). In addition, serum ALT and AST levels of mice were significantly increased in the HFHC group compared with the ND group, which revealed hepatic injury in model group (Fig. 1G and H). The chemical structure of GAA is presented in Fig. 1I.

Compared with the model group, the body weight of HFHC-fed mice treated with GAA was significantly reduced (Fig. 1A). Serum lipid disorders (increased levels of TG, TC, LDL-c) were also reversed by GAA treatment in HFHC-fed mice (Fig. 1C-F). Additionally, the serum ALT and AST levels were significantly lower in both GAA groups compared with the HFHC group, demonstrating a hepatoprotective role of GAA against liver injury (Fig. 1G and H). These results suggested that GAA improved the metabolic profiles of HFHC-fed mice.

Hepatic lipid accumulation was evaluated by Oil Red O staining and biochemical parameter assays. As revealed in Fig. 2A and B, compared with the ND group, the Oil Red O staining positive area in HFHC group mice was increased significantly. By contrast, the positive area was reduced by GAA in a dose-dependent manner compared with the model group (Fig. 2A and B). Similar results were observed following liver biochemical parameter assays. The ratio of liver weight to body weight and the levels of hepatic TG and TC were significantly increased in the HFHC group compared with the ND group. Conversely, oral administration of 25 or 50 mg/kg of GAA reduced the HW/BW, TG and TC levels (Fig. 2C-E). These results indicated that GAA alleviated hepatic steatosis in HFHC-fed mice.

To evaluate the effect of GAA on the hepatic injury process from NAFLD to NASH, liver histopathology was detected by typical H&E staining (Fig. 3A). Compared with mice in the ND group, the typical pathological phenomenon of NASH, including NAS, hepatocellular ballooning, lobular inflammation and inflammatory cell infiltration were observed in the livers of HFHC-fed mice (Fig. 3A). Furthermore, the number of CD68 positive marking Kupffer cells and F4/80 positive marking macrophage infiltration were significantly enhanced in the livers of HFHC-fed mice, compared with the ND group (Fig. 3B-E), which suggested that hepatic inflammation had occurred in the model group. Circulating inflammation factors, such as IL-1β, TNF-α and IL-6, were also significantly increased in the model group (Fig. 3F-H). In addition, the mRNA expression of inflammation factors, IL-1β, TNF-α and IL-6, was significantly increased, compared with the corresponding control group (Fig. 3I-K).

The typical pathology of NASH, including NAS, hepatocellular ballooning, lobular inflammation and inflammatory cell infiltration, was significantly decreased in the liver of GAA-treated (25 or 50 mg/kg) HFHC-fed mice (Fig. 3A). As demonstrated in Fig. 3B-E, GAA (25 or 50 mg/kg) treatment markedly reduced the number of Kupffer cells and macrophage infiltration in the livers of HFHC-fed mice. Additionally, the upregulated serum inflammation factors in HFHC-fed mice were significantly reduced by GAA treatment for 12 weeks (Fig. 3F-H). In consistency with these results, the mRNA expression of inflammation factors, such as IL-1β, TNF-α and IL-6, was significantly decreased in HFHC-fed mice treated with GAA (Fig. 3I-K). These results suggested that GAA reduced the hepatic inflammation response in HFHC-fed mice.

To certify the pathological progression from NASH to hepatic fibrosis, SR staining was used to indirectly reflect activated stellate cells in the livers of HFHC-fed mice. As presented in Fig. 4A and B, the hepatic collagen formation of model mice was increased, compared with the ND group. Additionally, the mRNA levels of α-SMA, TGF-β and MMP-13 were also significantly upregulated in HFHC-fed mice (Fig. 4C-E).

Administration of GAA (25 or 50 mg/kg) reduced the number of activated stellate cells in the livers of HFHC-fed mice, as determined by SR staining (Fig. 4A and B). The transcription of fibrosis-related genes, including α-SMA, TGF-β and MMP-13, was also decreased by GAA treatment (Fig. 4C-E). These results indicated that GAA could decrease the hepatic fibrosis in HFHC-fed mice.

It has been reported that oxidative stress plays a key role in the occurrence and development of NASH (24). To explore the underlying mechanisms of GAA, the contents of MDA and SOD in the livers of mice fed with an HFHC diet were evaluated. As revealed in Fig. 5A and B, the hepatic level of MDA was significantly increased in HFHC-fed mice compared with the ND group, whereas it was decreased in HFHC-fed mice treated with GAA when compared with the HFHC group. Conversely, the hepatic level of SOD was significantly decreased in HFHC-fed mice compared with the ND group, whereas it was increased in HFHC-fed mice treated with GAA.

Subsequently, the expression levels of essential ER stress-related genes were detected. As demonstrated in Fig. 5C-F, administration of the HFHC diet to mice resulted in an increase in GRp78, p-eIF-2α and p-JNK protein expression, which was significantly reversed by GAA treatment (25 or 50 mg/kg). Furthermore, compared with the ND group, the levels of ERp57, p-Akt, and p-MAPK were decreased in HFHC-fed mice, whereas GAA treatment increased their levels (Fig. 5G-J). These results suggested that the reduction of hepatic oxidative stress and the ER stress response by GAA may be related to the prevention of NASH progression in mice.