Nancy strain CVB3 was purchased from the Wuhan Institute of Virology of the Chinese Academy of Sciences (Wuhan, China). A total of 120 male healthy BALB/c mice, aged 5 weeks and weighing 16–20 g, were provided by Shanghai SLAC Experimental Animals Co., Ltd. [Shanghai, China; animal quality license, SCXK (HU) 2007-0005]. Mice were randomly divided into five groups as follows: Blank control group (n=20), negative control group (n=28), ribavirin group (n=24), low-dose SFI group (n=24) and high-dose SFI group (n=24). Blank control group was administered 0.1 ml Dulbecco's modified Eagle medium (Gibco; Thermo Fisher Scientific, Inc., Waltham, MA, USA) without CVB3 and after 0.5 h, 0.4 ml NaCl (0.9%) was injected into the abdominal cavity and mice were provided with a normal diet for 30 days. The remaining four groups were injected with 5×10² 50% tissue culture infective dose of CVB3 fluid (0.1 ml) and, after 0.5 h, 0.4 ml NaCl (0.9%), 0.4 ml ribavirin, 0.4 ml SFI and 0.9 ml SFI, respectively, and were provided with normal diet for 30 days.

Terminal deoxynucleotidyl transferase dUTP nick-end labeling (TUNEL) assay kits were purchased from Roche Diagnostics (Basel, Switzerland). Rabbit anti-Fas (sc-1024) and FasL (sc-834) primary polyclonal antibody and biotinylated FasL secondary antibody (sc-834) kits were purchased from Santa Cruz Biotechnology, Inc. (Dallas, TX, USA). Antibody dilution-protection fluid was purchased from Applygen Technologies, Inc., (Beijing, China), and 3,3′-diaminobenzidine (DAB) kits were purchased from Beijing Zhongshan Golden Bridge Biotechnology Co., Ltd. (Beijing, China).

SFI containing Radix Codonopsis, astragalus, and the formulation additives sodium chloride and sodium metabisulfite was produced by Lizhu Group Limin Pharmaceutical Factory (Shaoguan, China), and each 250 ml SFI contained 10 g Radix Codonopsis and Astragalus, respectively. Ribavirin (Virazole^®) was purchased from Tianjin Kingyork Group Co., Ltd., (Tianjin, China) and supplemented with normal saline to form a 0.6825 mg/ml ribavirin solution prior to abdominal injection.

The protocol of the study was approved by the Animal Ethics Committee and University Committee on the Use and Care of Animals of Fujian Medical University (Fuzhou, China), in accordance with the guidelines outlined by the Ethics Committee of the Ministry of Health of China. Cardiac tissue samples were harvested from randomly chosen mice, following sacrifice via spinal dislocation at 8:00 a.m. on days 3, 10 and 30. Samples were fixed using 10% paraformaldehyde and sliced to 4–6 µm following paraffin embedding to be used for TUNEL and immunohistochemical detection.

Following conventional dewaxing and hydration, cardiac muscle sections were incubated with proteinase K (20 mg/ml in Tris/HCl, pH 7.4–8.0) for 15 min at room temperature. TUNEL reaction mixture (50 µl TdT and 450 µl fluorescein-dUTP) was added, the sections were placed in a humidified box at 37°C for 60 min and the sections were analyzed using immunofluorescence under an Olympus BH2 fluorescence microscope (Olympus Corporation, Tokyo, Japan). Transforming agent was added, and the sections were incubated in humidified box at 37°C for 30 min. Sections were developed by incubation with DAB at room temperature, which was monitored using an Olympus BH2 fluorescence microscope. Subsequently, the sections were counterstained using hematoxylin (Abcam, Cambridge, MA, USA), washed with tap water, dehydrated, treated with xylene and sealed with neutral rubber. Apoptotic cells were stained brown and visualized under an Olympus BH2 fluorescence microscope. From each section, the mean of five fields of view was selected and the apoptotic index (AI) was calculated using Motic Images Advanced computed imaging software (version 3.2; Motic, Xiamen, China) as follows: AI (%) = (number of positive nuclei/total number of nuclei) × 100.

Following dewaxing and hydration using gradient alcohol, sections were incubated for 10 min with 3% hydrogen peroxide at room temperature in order to inhibit endogenous peroxidase activity. Fas and FasL were subjected to heat-induced antigen retrieval in Tris-EDTA (pH 9.0) buffer and citrate buffer, respectively. Sections were incubated with anti-Fas (X-2O; 1:25) and anti-FasL (N-2O; 1:40) primary antibodies overnight at 4°C in a humidified box. Following washing with five times with PBS for 2 min, the sections were incubated with biotinylated FasL secondary antibody (no dilution) for 20 min at room temperature. Horseradish peroxidase-conjugated avidin-biotin was subsequently added and the sections were incubated for 20 min at room temperature. Mean integral optical density of positive expression was measured in five randomly selected visual fields using Image Pro Plus 6.0 software (Media Cybernetics, Inc., Rockville, MD, USA).

Statistical analysis was performed using SPSS software, version 13.0 (SPSS, Inc., Chicago, IL, USA). All the data are expressed as the mean ± standard deviation. Intergroup differences were compared using one way-analysis of variance, whereas between group comparisons were performed using least significant difference test. P<0.05 was considered to indicate a statistically significant difference.

Myocardial apoptosis was identified by the presence of brown apoptotic cells, rounded nuclear karyopyknosis and oval brown masses (Fig. 1). In the blank control group, normal myocardial cells were detected; the nuclei were pale blue and nuclear pyknosis was not observed. However, in the model group, a large number of cardiac muscle cells contained brown round or oval nuclei and meniscus-shaped chromatin, which are characteristic of apoptosis. Strong TUNEL positive staining was detected in the nucleus, with minimal staining detected in the cytoplasm. The brown masses and changed to the nuclei became more evident at day 10, but cells appeared less apoptotic by day 30. In the virally infected cells, low- and high-dose SFI administration induced a reduction in the number of apoptotic cells in comparison with the model group at various time points, with the high-dose SFI group exhibiting the most evident difference from the model group (Fig. 1).

In the model group, the AI of cardiomyocytes was significantly increased, as compared with the blank group at all three time points (P<0.01). The AI of myocardial cells in each therapy group was not significantly reduced at day 3 (acute phase), as compared with the model group; however, the AI was significantly reduced by varying degrees on day 10 (acute phase; ribavirin and high-dose SFI, P<0.01; low-dose SFI, P<0.05). The greatest reduction was detected in the high-dose SFI group, which showed a significant difference compared with the ribavirin group (P<0.05). However, no significant difference was detected between the ribavirin and low-dose SFI groups on day 10. A significant reduction in the AI of cardiomyocytes was detected at day 30 in the high- and low-dose SFI groups as compared with the model group (P<0.01); however, no significant differences were detected between these groups. The low- and high-dose SFI groups exhibited significant differences from the ribavirin group on day 30 (P<0.05; Fig. 2 and Table I).

Fas protein expression was demonstrated by homogeneous brown staining of the cell membrane and cytoplasm and a lack of nuclear staining (Fig. 3, as indicated by an arrow). FasL protein expression was demonstrated by homogeneous brown staining or dark brown particles located in the cell membrane and cytoplasm, and a lack of nuclear staining (Fig. 4, as indicated by an arrow). Low expression levels of Fas and FasL proteins were detected in the blank group at each time point. The greatest amount of brown staining was detected in the model group on day 3, and no significant reduction in the amount was detected in the therapy groups. A significant increase in the amount of brown staining was detected in each group, with the exception of the blank group, on day 10, with the greatest increase demonstrated in the model group, and the smallest increase in the high-dose SFI group. The low-dose SFI and ribavirin groups exhibited more evident deposits of brown particles. At day 30, the number of brown particles was reduced in all the groups, with the greatest reductions detected in the high- and low-dose SFI groups.

A significant increase in the expression levels of Fas and FasL proteins was detected in the model group, as compared with the blank group at all time points (P<0.01). No significant reduction in Fas and FasL protein expression levels was detected in each of the therapy groups, as compared with the model group on day 3 (acute phase); however, all the groups demonstrated a reduction in the expression levels of Fas and FasL on day 10 (acute phase), to varying degrees (P<0.01 or P<0.05). The high-dose SFI group demonstrated the largest reductions compared with the model group (P<0.01), and also exhibited significant differences in Fas (P<0.01) and FasL (P<0.05) as compared with the ribavirin group (P<0.01). No significant differences were detected between the low-dose SFI and ribavirin groups. At day 30 (chronic phase), both the low- and high-dose SFI groups demonstrated significant reductions in the expression levels of Fas and FasL compared with the model group, although no significant differences were detected between the two SFI groups. Furthermore, Fas and FasL protein expression levels were significantly lower in the low- and high-dose SFI groups, as compared with the ribavirin group (P<0.05 and P<0.01, respectively) (Figs. 5 and 6; Tables II and III, respectively).