The H9c2 cardiomyocyte cell line (cat. no. ZQ0102) was provided by Shanghai Zhongqiao Xinzhou Biotechnology Co., Ltd. THP, Sc, dexrazoxane (Dex; a drug particularly approved by the US Food and Drug Administration for the treatment of CTP), GSK2795039 (GSK), ferrostatin-1 (Fer-1) and erastin were purchased from MedChemExpress. The brain natriuretic peptide (BNP, cat. no. H166-1-2), creatine kinase MB (CK-MB, cat. no. H197-1-1) and cardiac troponin T (cTnT, cat. no. H149-4-2) kits were purchased from Nanjing Jiancheng Bioengineering Institute. Cell Counting Kit-8 (CCK-8), ROS (cat. no. S0033M) and TUNEL (cat. no. C10088) apoptosis assay kits were purchased from Beyotime Institute of Biotechnology. DMEM and FBS were obtained from Gibco (Thermo Fisher Scientific, Inc.) and BioAgrio, respectively. The reduced glutathione (GSH, cat. no. A006-2-1), glutathione peroxidase (GSH-Px, cat. no. A005-1-2), catalase (CAT, cat. no. A007-1-1), malondialdehyde (MDA, cat. no. A003-1-2), superoxide dismutase (SOD, cat. no. A001-3-2), lactate dehydrogenase (LDH, cat. no. A020-2-2) and total antioxidant capacity (T-AOC, cat. no. A015-2-1) assay kits were obtained from Nanjing Jiancheng Bioengineering Institute. An iron assay kit (, cat. no. ab83366) was purchased from Abcam, while the antibodies against glutathione peroxidase 4 (GPX4), NOX2, NOX4, erythroid 2-related factor 2 (NRF2), Bax, Bcl-2, GAPDH, caspase 3 and caspase 9 from Proteintech Group, Inc.

In the present study, a total of 50 male Sprague-Dawley (SD) rats (weight, 180–200 g) were obtained from the Experimental Animal Center of Chongqing Medical University. Rats were maintained under specific pathogen-free conditions at 23±2°C, 55±5% relative humidity, a 12-h light/dark cycle and had free access to food and water. The rats were randomly divided into the following five groups (n=10 rats/group): i) The normal diet group (ND), where rats were fed standard chow and injected with an equal volume of normal saline via the tail vein, once a week for eight weeks; ii) the Sc group (Sc), where rats were fed with Sc feed (100 mg/kg) and injected with an equal volume of normal saline via the tail vein, once a week for eight weeks; iii) the THP group (THP), where rats were fed with standard chow, while 3 mg/kg THP was injected into the tail vein once a week for eight weeks (25); iv) the Sc + THP group (Sc + THP), were rats were fed with Sc feed (100 mg/kg) and 3 mg/kg THP was injected into the tail vein once a week for eight weeks; and v) the Dex + THP group (Dex + THP), where rats were fed with standard chow, while 3 mg/kg THP and 30 mg/kg Dex was injected into the tail vein and abdominal cavity, respectively, once a week for eight weeks. The survival of rats was recorded every day, while food consumption and rat weight were recorded once a week.

The experiment was completed at week 8. Rats were first anesthetized by isoflurane inhalation (2% for induction and 2% for maintenance). Subsequently, after removing the chest hair of rats, the VIVID E95 and L8-18I-D probes (General Electric Company) were used to perform doppler echocardiography to measure ejection fraction (EF), fractional shortening (FS), left ventricular end-diastolic diameter (LVIDd) and left ventricular end-systolic diameter (LVIDs).

Following overnight fasting, rats were weighed and euthanized by cervical dislocation following anesthesia with 1% pentobarbital (40 mg/kg). Rat hearts were then removed, weighed and stored at −80°C until further use. A part of the heart tissues was homogenized and the levels of iron, GSH, GSH-Px, MDA, SOD and T-AOC were immediately measured, according to the manufacturer's instructions. Within 2 h, blood samples were collected from the abdominal aorta and centrifuged at 900 × g for 30 min at room temperature. The supernatant was then stored at −80°C. The serum levels of LDH, BNP, CK-MB and cTnT were directly determined using the corresponding kits.

H9c2 cells were cultured in DMEM supplemented with 10% (v/v) FBS in a humidified incubator with 95% air and 5% CO₂ at 37°C. To establish an in vitro injury model, H9c2 cells were treated with 5 µmol/l THP for 24 h. Subsequently, to evaluate the association between oxidative stress, ferroptosis and apoptosis in CTP, the in vitro experiments were carried out into two parts. Therefore, cells were grouped as follows: a) Direction of oxidative stress, including i) the control (CON) group, where cells were cultured in DMEM; ii) the THP group (THP), where cells were treated with 5 µmol/l THP for 24 h; iii) the Sc + THP group (Sc + THP), where cells were pretreated with 100 µmol/l Sc for 1 h followed by treatment with 5 µmol/l THP for 24 h; iv) the GSK group (GSK), where cells were treated with 25 µmol/l GSK for 24 h (26); v) the GSK + THP group (GSK + THP), where cells were co-treated with 5 µmol/l THP and 25 µmol/l GSK for 24 h; and vi) the Sc + GSK + THP group (Sc + GSK + THP), where cells were pretreated with 100 µmol/l Sc for 1 h followed by co-treatment with 5 µmol/l THP and 25 µmol/l GSK for 24 h. b) Direction of ferroptosis, including i) the CON group (CON), where cells were cultured in DMEM; ii) the THP group (THP), where cells were treated with 5 µmol/l THP for 24 h; iii) the Sc + THP group (Sc + THP), where cells were pretreated with 100 µmol/l Sc for 1 h, followed by treatment with 5 µmol/l THP for 24 h; iv) the Fer-1 group, where cells were treated with 10 µmol/l Fer-1 for 24 h (27); v) the Fer-1 + THP group (Fer-1 + THP), where cells were co-treated with 10 µmol/l Fer-1 and 5 µmol/l THP for 24 h; vi) the erastin group (erastin), where cells were treated with 5 µmol/l erastin for 24 h (28); and the erastin + Sc group (erastin + Sc), where cells were pretreated with 100 µmol/l Sc for 1 h, followed by co-treatment with 5 µmol/l erastin for an additional 24 h.

H9c2 cells were seeded in 96-well plates at a density of 5×10³ cells/well for 12 h, prior to use. Following treatment, a CCK-8 assay kit was used to evaluate cell viability. Briefly, cells in each well were supplemented with 10 µl CCK-8 reagent followed by incubation for 2 h. Subsequently, the absorbance in each well was measured at a wavelength of 450 nm using a single-wavelength microplate reader.

Cells were seeded into 24-well plates and after reaching 50–60% confluency, they were treated with the indicated compounds. Subsequently, cells were stained with DCFH-DA dye (37°C, 20 min), provided by the ROS kit, according to the manufacturer's instructions (Beyotime Institute of Biotechnology). Cells were observed under a fluorescence microscope and the positive stained area was measured using ImageJ v1.53c software (National Institutes of Health).

For cell apoptosis assessment, cells were seeded into 24-well plates and after reaching 50–60% confluency, the cells were treated as previously described. Subsequently, cell apoptosis was assessed using a TUNEL apoptosis assay kit, according to the manufacturer's instructions. Briefly, following fixing at room temperature for 30 min (Immunostaining fixative, Beyotime Institute of Biotechnology, cat. no. P0098), H9c2 cells were washed with ice-cold PBS and stained with DAPI (at room temperature for 5 min, Beyotime Institute of Biotechnology, cat. no. C1005) and TUNEL dyes (protected from light, at 37°C for 60 min). After washing, fluorescent images were captured under a fluorescence microscope and analyzed using ImageJ v1.53c software.

Cells were fixed with 4% formaldehyde (at room temperature for 15 min), washed with PBS and were then permeabilized with 0.2% Triton X-100 (at room temperature for 20 min). Following blocking with goat serum (cat. no. C0265; Beyotime Institute of Biotechnology) at room temperature for 30 min, the cells were first incubated at 4°C, overnight with primary antibodies against NOX2 (cat. no. 19013-1-AP; 1:200; Proteintech Group, Inc.) and then with the corresponding secondary antibody [FITC-labeled goat anti-rabbit IgG (H+L); cat. no. A0562; 1:500; Beyotime Institute of Biotechnology] at room temperature for 90 min. Finally, the cell nuclei were stained with DAPI (at room temperature for 5 min) and images were captured under a fluorescence microscope.

The protein expression levels of GAPDH (cat. no. 10494-1-AP; 1:5,000), NOX2 (cat. no. 19013-1-AP; 1:1,000), NOX4 (cat. no. 14347-1-AP; 1:1,000), NRF2 (cat. no. 16396-1-AP; 1:2,000), GPX4 (cat. no. 30388-1-AP; 1:500), Bax (cat. no. 50599-2-Ig; 1:2,000), Bcl-2 (cat. no. 26593-1-AP; 1:500), cleaved and total caspase 3 (cat. no. 19677-1-AP; 1:500), and cleaved and total caspase 9 (cat. no. 10380-1-AP; 1:500) were detected by western blot analysis. Briefly, H9c2 cells or cardiac tissue were lysed in RIPA lysis buffer (Beyotime Institute of Biotechnology) with 1% (v/v) phenylmethylsulfonyl fluoride. Following centrifugation at 13,700 × g for 15 min at 4°C, the supernatants were collected and then the protein concentration was measured using a BCA protein determination kit. An equal amount of protein extracts (30 µg) was separated by 12% SDS-PAGE and proteins were then transferred onto a PVDF membrane. Following blocking with 5% (w/v) skimmed milk (at room temperature for 2 h), the membrane was cut into strips according to the molecular weight of each target-protein. Subsequently, the membrane was first incubated with primary antibodies overnight at 4°C and then with the corresponding horseradish peroxidase-conjugated secondary antibodies (cat. no. SA00001-2; Proteintech Group, Inc.; 1:5,000). The protein bands were visualized using an ECL reagent (Biosharp life sciences, cat. no. BL520B). GAPDH served as an internal control for protein loading and analysis. ChemiDoc™ XRS+ with Image Lab Software (BIO-RAD) was used for densitometry.

GraphPad Prism 8.0 (Dotmatics) was used for statistical analysis. All experiments were repeated at least three times. The data are expressed as the mean ± standard deviation. First, the normal distribution and homogeneity of variance of the data were assessed. The differences between groups were compared using one- or two-way ANOVA, followed by Tukey's multiple comparison post hoc test. P<0.05 was considered to indicate a statistically significant difference.

As shown in Fig. 1, compared with the ND group, food intake was significantly reduced from the third week in the THP group (THP vs. ND, P<0.01; Fig. 1B). In addition, rat weight was also notably decreased in the THP group at the fourth week compared with the ND group (THP vs. ND, P<0.01; Fig. 1A). After eight weeks, the survival rate of rats in the THP group was markedly reduced compared with the ND group (Fig. 1C), while the cardiac mass index was notably enhanced (THP vs. ND, P<0.01; Fig. 1D). However, co-treatment of rats with Sc and Dex significantly restored the aforementioned changes (Sc + THP vs. THP: P<0.05, cardiac mass index and P<0.01, body weight and food intake; Dex + THP vs. THP: P<0.05, cardiac mass index and P<0.01, body weight and food intake; Fig. 1A-D).

As shown in Fig. 2, after treatment of SD rats with THP for eight weeks, significant changes were observed in the echocardiography parameters in the THP group compared with the ND group (Fig. 2A), including decreased EF and FS (THP vs. ND, P<0.01; Fig. 2B and C) and increased LVIDd and LVIDs (THP vs. ND, P<0.01; Fig. 2D and E). At the same time, abnormal levels of the myocardial injury-related markers, BNP, CK-MB, cTnT and LDH, were recorded in the THP group (THP vs. ND, P<0.01; Fig. 2F-I). However, the aforementioned changes were improved following treatment of SD rats with Sc and Dex (Sc + THP vs. THP, P<0.05 for FS, LVIDd, LVIDs, cTnT and LDH, and P<0.01 for EF, BNP, CK-MB; Dex + THP vs. THP, P<0.05 for EF, FS, LVIDd, LVIDs, BNP and LDH, and P<0.01 for CK-MB and cTnT; Fig. 2A-I).

Sc alleviates the THP-induced abnormal changes in the oxidative stress- and ferroptosis-related indexes in blood and myocardial tissues of SD rats. Compared with the ND group, Fe²⁺, Fe³⁺ and total Fe levels were enhanced in the THP group (THP vs. ND, P<0.05 for Fe³⁺ and P<0.01 for Fe²⁺ and total Fe; Fig. 3A-C), while this effect was restored by rat treatment with Sc and Dex (Sc + THP vs. THP, P<0.05 for Fe²⁺ and total Fe; Dex + THP vs. THP, P<0.05 for Fe²⁺ and total Fe; Fig. 3A and C). In addition, the levels of CAT, GSH, GSH-Px, SOD and T-AOC were reduced (THP vs. ND, P<0.01; Fig. 3D-H), while the level of MDA was increased (THP vs. ND, P<0.01; Fig. 3I) in the THP group compared with the ND group, and these effects were also restored following treatment of SD rats with Sc and Dex (Sc + THP vs. THP, P<0.05 for CAT, GSH and SOD, and P<0.01for GSH-Px, T-AOC and MDA; Dex + THP vs. THP, P<0.05 for GSH, SOD and T-AOC, and P<0.01 for CAT, GSH-Px and MDA; Fig. 3D-I).

Effects of Sc and THP on the expression of oxidative stress-, ferroptosis- and apoptosis-related proteins in the myocardium of SD rats. The results of western blot analysis showed that THP increased the expression of oxidative stress-related proteins, such as NOX2 and NOX4, and decreased those of NRF2, in the myocardial tissues of SD rats (THP vs. ND, P<0.01 for NOX2 and NRF2, and P<0.001 for NOX4; Fig. 4A-D). Additionally, THP downregulated GPX4, a ferroptosis-related protein (THP vs. ND, P<0.01; Fig. 4E). In terms of apoptosis, THP notably enhanced the Bax/Bcl-2 ratio, the cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9 ratio (THP vs. ND, P<0.001 for Bax/Bcl-2, cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9; Fig. 4A and F-H), while these were restored by Sc and Dex (Sc + THP vs. THP, P<0.05 for NOX2, NRF2, GPX4, cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9, and P<0.01 for NOX4, Bax/Bcl-2; Dex + THP vs. THP, P<0.05 for NOX2, NRF2, GPX4, Bax/Bcl-2, cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9, and P<0.01 for NOX4; Fig. 4B-H).

In vitro experiments using CCK-8 assays, showed that 5 µmol/l THP and 100 µmol/l Sc were the optimal concentrations to treat cells (5 µmol/l THP vs. CON, P<0.001; 100 µmol/l Sc + THP vs. THP, P<0.01; Fig. 5A and B). CCK-8 assays showed that THP significantly reduced the viability of H9c2 cells, which was improved by cell treatment with Sc, GSK and Fer-1 (THP vs. CON, P<0.01; Sc + THP vs. THP, P<0.05; GSK + THP vs. THP, P<0.05; and Fer-1 + THP vs. THP, P<0.05; Fig. 5C-E). Furthermore, erastin had a similar effect with THP on cell viability, which was also alleviated by Sc (erastin vs. CON, P<0.01; and erastin + Sc vs. erastin, P<0.01; Fig. 5E).

As shown in Fig. 5D and F, THP enhanced ROS production in H9c2 cells, while Sc and GSK antagonized this effect (THP vs. CON, P<0.01; Sc + THP vs. THP, P<0.01; and GSK + THP vs. THP, P<0.01; Fig. 5F). Furthermore, erastin also increased ROS production in H9c2 cells, which was alleviated by Sc (erastin vs. CON, P<0.01; erastin + Sc vs. erastin, P<0.01; Fig. 5F). Consistently, Fer-1 also improved the THP-mediated increase in ROS production (Fer-1 + THP vs. THP, P<0.01; Fig. 5F).

TUNEL staining results indicated that THP promoted H9c2 cell apoptosis (THP vs. CON, P<0.01; Fig. 6A and B). This effect was abrogated by cell treatment with GSK, Fer-1 and Sc (Sc + THP vs. THP, P<0.01; GSK + THP vs. THP, P<0.01; and Fer-1 + THP vs. THP, P<0.01; Fig. 6A and B). In addition, erastin also enhanced H9c2 cell apoptosis, which was also improved by Sc (erastin vs. CON, P<0.01; erastin + Sc vs. erastin, P<0.01; Fig. 6A and B).

Effects of Sc, THP, GSK, Fer-1 and erastin on the expression of oxidative stress-, ferroptosis- and apoptosis-related proteins in H9c2 cardiomyocytes. The in vitro immunofluorescence results shown in Fig. 6C and D, revealed that compared with the CON group, NOX2 was upregulated in the THP group (THP vs. CON, P<0.01; Fig. 6C and D). The protein expression levels of NOX2 were restored following cell treatment with Sc and GSK (Sc + THP vs. THP, P<0.01; and GSK + THP vs. THP, P<0.01; Fig. 6C and D). However, Fer-1 and erastin did not significantly affect NOX2 expression. Furthermore, the western blot results also demonstrated that THP markedly upregulated NOX2, increased the Bax/Bcl-2, cleaved caspase 3/total caspase 3, cleaved caspase 9/total caspase 9 ratio and downregulated GPX4 (THP vs. CON, P<0.01 for cleaved caspase 3/total caspase 3; P<0.001 for GPX4, cleaved caspase 9/total caspase 9; and P<0.0001 for NOX2 and Bax/Bcl-2; Fig. 7C). The aforementioned results were restored by cell treatment with Sc (Sc + THP vs. THP, P<0.05 for NOX2, GPX4, Bax/Bcl-2, cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9; Fig. 7C). At the same time, the aforementioned effects were also improved by GSK treatment (GSK + THP vs. THP, P<0.05 for NOX2, GPX4, Bax/Bcl-2, cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9; Fig. 7C). Consistent with the immunofluorescence results, erastin and Fer-1 had no effect on NOX2 expression (Fig. 7D). Notably, H9c2 cell treatment with erastin increased the Bax/Bcl-2 ratio, upregulated cleaved caspase 3/9, total caspase 3/9 and downregulated GPX4 (erastin vs. CON, P<0.01 for cleaved caspase 3/total caspase 3, cleaved caspase 9/total caspase 9; and P<0.001 for GPX4 and Bax/Bcl-2; Fig. 7D), while Sc improved some aforementioned effects (erastin + Sc vs. erastin, P<0.05 for cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9; and P<0.01 for GPX4 and Bax/Bcl-2; Fig. 7D). In addition, Fer-1 improved aberrant protein effects in H9c2 cells induced by THP (Fer-1 + THP vs. THP, P<0.05 for GPX4, cleaved caspase 3/total caspase 3 and cleaved caspase 9/total caspase 9; and P<0.01 for Bax/Bcl-2; Fig. 7D).