Fetal bovine serum (FBS) (MF191-01) and high glucose Dulbecco's modified Eagle's medium (H-DMEM) (MF219-01) were purchased from Mei5 Biotechnology Co., Ltd. (Beijing, China). MTT Cell Proliferation and Cytotoxicity Assay kit (M1020), Lip2000 transfection reagent (L7800) and G418 (G8160) were purchased from Solarbio (Beijing, China). HindIII (R0104L), EcoRI (R0101L), Quick Ligase (M2200S) and T4 PNK (M0201S) were purchased from New England Biolabs, Inc. (NEB; Ipswich, MA, USA). FastDigest BsmBI (FD0454) was purchased from Fermentas (Thermo Fisher Scientific, Inc.). Protease inhibitor cocktail (CW2200), phosphatase inhibitor cocktail (CW2383), Ultrapure RNA kit (CW0597) and Super TaqMan OneStep RT-qPCR kit (CW2695) were purchased from CWbio Biological Technology Company (Beijing, China). TRITC phalloidin (40734ES75), DAPI stain solution (40728ES03) and PI staining solution (40755ES64) were purchased from Yeasen Biotechnology Co. (Shanghai, China). Anti-BRMS1 (ab180852), p-AKT (ab38449), AKT (ab179463), p-mTOR (ab137133), mTOR (ab134903), p-ERK (ab50011), ERK (ab17942), p-BIM (ab17935), BIM (ab32158), p-PTEN (ab109454), PTEN (ab32199), Bax (ab32503), Bcl-2 (ab196495), TNF-α (ab109322), caspase-9 (ab52298), caspase-3 (ab13847) antibodies and human IGF1 (ab211651), TGF-β (ab100647) and VEGF (ab100662) ELISA kits were purchased from Abcam (Cambridge, UK). Sorafenib (BAY 43-9006) was purchased from Enzo Life Science (Farmingdale, NY, USA). HepG2 cells (TCHu 72) and 293T cells (SCSP-502) were purchased from the Cell Library of the Typical Culture Preservation Committee of the Chinese Academy of Sciences.

The cDNA of BRMS1 was cloned from cells using PCR methods using the following primers: Forward, 5′-ATCGAAGCTTACTATGCCTGTCCAGCCTCCAAGC-3′ and reverse, 5′-ATGCGAATTCTCAAGGTCCATCCGATTC-3′. Blank pCNDA3.1 vector and PCR product of BRMS1 were digested with HindIII and EcoRI, and the BRMS1 fragment was cloned into the vector to construct the pCDNA3.1-BRMS1 overexpression vector. HepG2 cells were transfected with pCDNA3.1-BRMS1 and pcDNA3.1 blank vector using Lip2000 transfection reagent for 48 h according to the manufacturer's protocol. Stable BRMS1 overexpression cells and blank vector cells were screened using 800 µg/ml G418. The BRSM1 knockdown vector was constructed according to a previous study (11). Briefly, the CRISPR vector was firstly digested with BsmBI according to the protocol, and annealed oligos were constructed using the following primers: Forward, 5′-CACCGCTACACAGTGCAATTGCCTCC-3′ and reverse, 5′-AAACGATGTGTCACGTTAACGGAGC-3′. Ligation reactions were subsequently performed using annealed oligos and digested CRISPR vector according to the Quick Ligase protocol to construct the BRSM1 knockdown vector. Stable BRMS1 knockdown cells were screened using 2 µg/ml puromycin.

Cells were cultured in a humidified atmosphere supplied with 5% CO₂ at 37°C with H-DMEM and 10% FBS. Cells were divided into four groups: Controls (NC), sorafenib treatment (ST), sorafenib treatment with BRMS1 overexpression (BO) and sorafenib treatment with BRMS1 knockdown (BD). The concentration and treatment period for sorafenib used in this experiment (10 µM for 24 h) was determined according to a previous study (12).

MTT assay was performed according to the protocol of MTT Cell Proliferation and Cytotoxicity Assay kit. Briefly, cells were firstly cultured and grouped as previously described, seeded into a 96-well plate at a concentration of 1×10₄ cells/well, and cultured until cell confluence reached 80–85%. Then, the cells were incubated with 5 mg/ml MTT reagent for 4 h after washing with phosphate-buffered saline (PBS), and optical density (OD) values were determined at 560 nm using the SuPerMax 3100 microplate reader (Shanghai, China) after formazan was added. Cell viability was calculated as (OD_Experiment-OD_Blank/OD_Control-OD_Blank) × 100%.

RNA extraction was performed according to t Ultrapure RNA Kit protocol. Briefly, cells were lysed in lysis buffer for 5 min at room temperature, followed by vigorous shaking for 15 sec after mixing with chloroform. The mixture was then centrifuged at 13,523 × g for 5 min after thorough mixing with 70% ethanol and loaded onto an adsorption column. RNA was adsorbed onto the column after samples were centrifuged at 13,523 × g for 1 min. RNA was eluted from adsorption columns using elution buffer after washing with designated wash buffer.

Reverse transcription and qPCR were performed according to the Super TaqMan OneStep RT-qPCR Kit protocol. Primers used were as follows: IL-1β: Forward, 5′-ATAAGCCCACTCTACAGCT-3′ and reverse, 5′-ATTGGCCCTGAAAGGAGAGA-3′; IL-2: Forward, 5′-GTCCAAGGACACAGGCTTCTT-3′ and reverse, 5′-AAATTTTGGCTGGTGCCAAGG-3′; IL-6: Forward, 5′-GGCTACGAGTGGGATACTG-3′ and reverse, 5′-GGCTGGAAGGAGAAGATG-3′; Bcl-2: Forward, 5′-TGGCCTTCTTTGAGTTCGGT-3′ and reverse, 5′-GTTCCACAAAGGCATCCCAGC-3′; Bax: Forward, 5′-ACACCTGAGCTGACCTTGGA-3′ and reverse, 5′-AGTTCATCGCCAATTCGCCT-3′; TNF-α: Forward, 5′-CAGAGGGAAGAGTTCCCCAG-3′ and reverse, 5′-CCTTGGTCTGGTAGGAGACG-3′. Reaction mixtures were prepared as recommended by the protocol, and the PCR cycle was set as follows: Reverse transcription at 45°C for 20 min, predegeneration at 95°C for 5 min, and degeneration at 95°C for 15 sec with extension at 60°C for 45 sec repeated for 45 cycles. Relative gene expression was determined using the 2^−ΔΔCq method (13). GAPDH was used as an internal reference, and the quantified results for each target gene were normalized to GAPDH. Each experiment was repeated three times.

Cells in each group were first cultured and grouped as described above, and then lysed with lysis buffer [50 mM Tris (pH, 8.1), 1% SDS and protease inhibitor cocktail, phosphatase inhibitor cocktail] for 30 min on ice after washing with sterile PBS. The supernatant was collected after centrifugation at 13,523 × g for 10 min, and the protein concentration was determined using a BCA assay. Protein samples (60 µg) from each group were separated using 10% SDS-PAGE electrophoresis, and transferred onto 0.22-µm nitrocellulose membranes using the Trans-Blot Turbo system (Bio-Rad). Membranes were incubated with 5% skim milk, and then incubated with primary antibodies (dilution 1:1,000) at 4°C overnight followed by incubation with secondary antibodies (dilution 1:5,000) at room temperature for 1 h. Chemiluminiscence was performed using ECL reagents to detect expression levels of the target proteins. The gray values of bands were quantified using Scion Image software (version 4.0.3.2; Scion Corp., Frederick, MD, USA) and normalized to GAPDH. Each experiment was independently repeated three times.

Cells were cultured and grouped as described above. Phalloidin staining was performed according to the protocol, and cells were seeded onto a confocal plate at a concentration of 1×10₅ and cultured for 24 h. Cells were fixed with 4% formaldehyde at room temperature for 10 min, and then permeabilized with 0.5% Triton X-100 for 5 min at room temperature. Cells were stained with phalloidin staining buffer for 30 min and re-stained with DAPI for 5 min. DAPI/PI double staining was performed according to the protocol. Cells were digested with trypsin-EDTA buffer and then stained with DAPI and PI for 10 min followed by imaging using fluorescence microscopy. Images were analyzed using Image-Pro Plus software (version 6.0; Media Cybernetics, Inc., Bethesda, MD, USA).

Cells were seeded onto a 100-mm plate at a concentration of 1×10₆ cells, after being grouped and treated as described above. After treatment, cells were digested with trypsinization and washed with pre-cooled PBS. Then, the cells were incubated with propidium iodide (PI) for 15 min and apoptotic cells were quantified by FACScan flow cytometry (Becton Dickinson, Heidelberg, Germany).

ELISA was performed according to the protocol for each ELISA kit. Briefly, standards and supernatants of cultured medium in each group were added into each well of a 96-well plate, and incubated overnight at 4°C with gentle shaking. Biotinylated detection antibodies were added into each well after sufficient washing with wash buffer and incubation for 1 h at room temperature. Then, each sample was incubated with HRP-streptavidin solution for 45 min at room temperature followed by incubation with TMB One-Step substrate reagent for 30 min at room temperature, OD values were measured at 450 nm using a SuPerMax 3100 microplate reader (Shanghai, China).

Data are shown as the mean ± SD, and each experiment was independently repeated three times. One-way analysis of variance (ANOVA) was performed to compare differences between groups followed by Tukey's post hoc test. P<0.05 was indicative of a statistically significant difference. GraphPad version 7 (GraphPad Software, Inc., La Jolla, CA, USA) was used to analyze the data.

Cells were divided into four groups: Controls (NC), sorafenib treatment (ST), sorafenib treatment with BRMS1 overexpression (BO) and sorafenib treatment with BRMS1 knockdown (BD). As shown in Fig. 1A, the viability of HepG2 cells in the ST, BO and BD groups were 75.3±4.2, 60.5±3.6 and 89.3±5.4%, respectively, in response to 10 µM sorafenib treatment for 24 h. Compared with the NC group, cell viability was significantly decreased in the ST and BO groups (P<0.05), while remaining unchanged in the BD group. Compared to the ST group, cell viability was significantly decreased in the BO group (P<0.05) and significantly increased in the BD group (P<0.05).

Immunofluorescence results are shown in Fig. 1B, illustrating that PI-stained cells in the ST and BO groups were increased compared to the NC and BD groups. However, there were no significant changes noted between the NC and BD groups. As shown in Fig. 1C, the ratios of apoptotic cells were 21.24±2.12, 37.14±3.08, 42.57±4.52 and 18.32±2.20 in the NC, ST, BO and BD groups, respectively. The proportion of apoptotic cells was significantly increased in the ST and BO groups (P<0.05) compared with the NC group, and was significantly decreased in the BO group compared with the ST group (P<0.05). These results indicate that sorafenib inhibits the proliferation of HepG2 cells by inducing apoptosis in cancer cells, and overexpression of BRMS1 may synergize with sorafenib in enhancing the effects. As shown in Fig. 1D, the expression level of BRMS1 in each group was 0.63±0.08, 1.41±0.11, 1.81±0.13 and 0.86±0.09. Compared with the NC group, the expression of BRMS1 was significantly increased in the ST and BO group (P<0.05) and significantly decreased in the BD group (P<0.05). Expression of BRMS1 was significantly increased in the BO group (P<0.05) and significantly decreased in the BD group (P<0.05) when compared with the ST group. As shown in Fig. 1E, the expression levels of BRSM1 without sorafenib treatment in the normal, BRMS1 overexpression and BRMS1 knockdown groups were 0.68±0.05, 1.12±0.13 and 0.32±0.02. Compared with the NC group, the expression of BRMS1 was significantly increased in the overexpression group (P<0.05) and significantly decreased in the knockdown group (P<0.05), indicating that the cell model was successfully constructed.

As shown in Fig. 2A, expression levels of IL-1β in the NC, ST, BO and BD groups were 1.7±0.4, 2.6±0.6, 3.5±0.5 and 2.3±0.5, respectively. Expression of IL-1β was significantly increased in the BO groups when compared to that noted in the NC group (P<0.05). The expression levels of IL-2 in these groups were 1.6±0.2, 2.5±0.3, 3.6±0.4 and 2.1±0.2, respectively. As shown in Fig. 2B, IL-2 expression was significantly increased in all sorafenib-treated groups compared to the NC group (P<0.05), and was significantly increased in the BO group compared to the ST group (P<0.05). As shown in Fig. 2C, expression levels of IL-6 in these groups were 1.8±0.4, 3.0±0.5, 3.7±0.5 and 2.6±0.4. Expression of IL-6 was significantly increased in ST and BO groups compared to the NC group (P<0.05), and significantly increased in the BO group compared to the ST group (P<0.05). As shown in Fig. 2D, Bax expression in these groups was 1.6±0.3, 2.4±0.3, 3.1±0.5 and 2.1±0.4, respectively. The Bax expression was significantly increased in the ST and BO groups compared to the NC group (P<0.05). As shown in Fig. 2E, Bcl-2 expression in these groups was 1.9±0.3, 1.4±0.2, 0.8±0.1 and 1.7±0.2, respectively. Expression of Bcl-2 was significantly decreased in the ST and BO groups compared to the NC group (P<0.05), and was significantly decreased in the BO group compared to the ST group (P<0.05). As shown in Fig. 2F, expression levels of TNF-α in these groups were 1.3±0.2, 2.1±0.3, 2.8±0.5 and 1.6±0.3, respectively. TNF-α expression was significantly increased in the ST and BO groups compared to the NC group (P<0.05), and significantly increased in the BO group compared to the ST group (P<0.05).

As shown in Fig. 3A and B, the ratio of p-AKT/AKT was 1.41±0.07, 0.85±0.04, 0.65±0.03 and 1.33±0.07 in the NC, ST, BO and BD groups, respectively. Compared to the NC group, the ratio of p-AKT/AKT was significantly decreased in the ST and BO groups (P<0.05). Furthermore, and compared to the ST group, the ratio of p-AKT/AKT was significantly decreased in the BO group (P<0.05) and significantly increased in the BD group (P<0.05). As shown in Fig. 3A and C, the ratio of p-mTOR/mTOR was 0.80±0.04, 0.65±0.03, 0.52±0.03 and 0.65±0.03 in these groups, respectively. Compared to the NC group, the ratio of p-mTOR/mTOR was significantly decreased in all experimental groups (P<0.05), and compared with the ST group, the ratio of p-mTOR/mTOR was significantly decreased in the BO group (P<0.05). As shown in Fig. 3A and D, the ratio of p-ERK/ERK was 0.75±0.04, 0.80±0.03, 0.43±0.02 and 0.50±0.03 in these groups, respectively. Compared to the NC and ST group, the ratio of p-ERK/ERK was significantly decreased in the BO and BD groups (P<0.05). As shown in Fig. 3A and E, the ratios of p-BIM/BIM was 0.37±0.02, 0.80±0.04, 0.91±0.05 and 0.24±0.01 in these groups, respectively. Compared to the NC group, the ratio of p-BIM/BIM was significantly increased in the ST and BO groups (P<0.05) and significantly decreased in BD group (P<0.05). Compared to the ST group, the ratio was significantly increased in the BO group (P<0.05) and significantly decreased in the BD group (P<0.05). As shown in Fig. 3A and F, the ratio of p-PTEN/PTEN was 0.24±0.01, 0.59±0.03, 0.87±0.04 and 0.62±0.03 in these groups, respectively. Compared to the NC group, the ratio of p-PTEN/PTEN was significantly increased in all experimental groups (P<0.05), and compared to the ST group, the ratio was significantly increased in the BO group (P<0.05).

As shown in Fig. 4A and B, the expression level of caspase-3 was 0.19±0.01, 0.38±0.02, 0.49±0.02 and 0.42±0.02 in the NC, ST, BO and BD groups, respectively. Compared to the NC group, expression of caspase-3 was significantly increased in all experimental groups (P<0.05), and compared to the ST group, expression of caspase-3 was significantly increased in the BO group (P<0.05). As shown in Fig. 4A and C, the expression level of caspase-9 was 0.12±0.01, 0.43±0.02, 0.49±0.02 and 0.38±0.02 in these groups, respectively. Compared to the NC group, expression of caspase-9 was significantly increased in all experimental groups (P<0.05), and compared with the ST group, expression of caspase-9 was significantly increased in the BO group (P<0.05) and significantly decreased in the BD group (P<0.05). As shown in Fig. 4A and D, the TNF-α expression level was 0.08±0.01, 0.27±0.01, 0.41±0.02 and 0.35±0.02 in these groups, respectively. Compared to the NC group, expression of TNF-α was significantly increased in all experimental groups (P<0.05), and compared to the ST group, the expression of TNF-α was significantly increased in the BO and BD group (P<0.05). As shown in Fig. 4A and E, the expression level of Bax was 0.08±0.01, 0.18±0.01, 0.30±0.02 and 0.27±0.01 in these groups, respectively. Expression changes in Bax were similar to those for TNF-α. As shown in Fig. 4A and F, the expression level of Bcl-2 was 0.51±0.03, 0.29±0.01, 0.15±0.01 and 0.42±0.02 in these groups, respectively. Compared to the NC group, expression of Bcl-2 was significantly decreased in all the experimental groups (P<0.05), and compared to the ST group, expression of Bcl-2 was significantly decreased in the BO (P<0.05) and significantly increased in the BD group (P<0.05).

As shown in Fig. 5A, the concentration of IGF was 1,040.3±23.1, 922.5±21.2, 856.4±18.5 and 990.6±23.8 in the NC, ST, BO and BD groups, respectively. Compared to the NC group, the IGF concentration was significantly decreased in the ST and BO groups (P<0.05). Compared to the ST group, the concentration of IGF was significantly decreased in the BO group (P<0.05) and significantly increased in the BD group (P<0.05). As shown in Fig. 5B, the concentration of TGF-β was 858.3±15.6, 930.5±19.7, 1154.2±21.6 and 886.2±18.1 in these groups, respectively. The concentration of TGF-β was significantly increased in the ST and BO groups compared to the NC group (P<0.05). In addition, compared to the ST group, the concentration of TGF-α was significantly decreased in the BD group (P<0.05) and significantly increased in the BO group (P<0.05). As shown in Fig. 5C, the VEGF concentration was 1,823.0±28.4, 1,577.2±21.4, 1,085.6±18.2 and 1,780.5±23.2 in these groups, respectively. Compared to the NC group, the concentration of VEGF was significantly decreased in the ST and BO groups (P<0.05). Compared to the ST group, the concentration of VEGF was significantly decreased in the BO group (P<0.05), and significantly increased in BD group (P<0.05). As shown in Fig. 5D, the concentrations of EGF was 156.3±20.3, 114.5±10.2, 93.4±7.1 and 138.9±13.2 in these groups, respectively. Compared to the NC group, the concentration of VEGF was significantly decreased in the ST and BO group (P<0.05). Compared to the ST group, the concentration of VEGF was significantly decreased in BO group (P<0.05) and significantly increased in the BD group (P<0.05).