The human DLBCL cell lines SU-DHL-4, SU-DHL-6, SU-DHL-8, SU-DHL-10 and DoHH2 were provided by Professor Fengting Liu. Curcumin and Q-VD-OPh were obtained from MedChemExpress and olaparib was acquired from Selleck Chemicals.

To ensure consistent drug concentrations and maintained bioactivity under experimental conditions, the storage and preparation protocols for all drugs used in the present study were standardized. Curcumin, Q-VD-OPh and olaparib were dissolved in dimethyl sulfoxide (DMSO) to prepare stock solutions of 50, 1 and 50 mM, respectively. Aliquots were stored at −80°C in a cryogenic freezer. Working concentrations were prepared by diluting in complete RPMI-1640 medium (Gibco; Thermo Fisher Scientific, Inc.) immediately before use.

To ensure that post-thaw cells retained their original biological functions, morphology and capacity for normal proliferation and metabolism-thereby providing a stable and healthy cellular source for subsequent culture and pharmacological assays-the cryopreservation and thawing procedures were carefully optimized. The cells were recovered using standard cryopreservation reversal procedures. Briefly, the water bath was pre-warmed to 37°C. Cryovials containing frozen cells were promptly removed from the liquid nitrogen and immersed in a water bath with gentle agitation to accelerate thawing. After thawing, the external surfaces of the cryovials were wiped with 75% ethanol and transferred to a biological safety cabinet. The cell suspension was transferred into a centrifuge tube containing 5 ml pre-warmed complete medium [RPMI-1640 basal medium + 10% fetal bovine serum (FBS; ZETA Life) + 1% penicillin-streptomycin (dual antibiotics); pre-warmed to 37°C), followed by centrifugation at 200 × g for 5 min at room temperature. The supernatant was carefully aspirated and the cell pellet was gently resuspended in fresh complete medium (RPMI-1640 basal medium + 10% FBS + 1% penicillin-streptomycin). The resuspended cells were then transferred into a labeled culture flask and incubated in an upright position in a humidified incubator maintained at 37°C with 5% CO₂.

To maintain cells in the logarithmic growth phase and ensure consistent cell state and absence of contamination during experiments, cell culture and subculturing were performed according to the following standard procedures.

Cell lines (SU-DHL-8, SU-DHL-10 and DoHH2) were maintained in RPMI-1640 (Gibco; Thermo Fisher Scientific, Inc.) medium containing 10% FBS (ZETA Life) and 1% penicillin-streptomycin at 37°C in a humidified 5% CO₂ incubator. The cells were routinely monitored for growth, medium clarity and signs of contamination. Depending on the cell condition, the culture medium was replaced every 2–3 days to prevent bacterial contamination. All cell lines used in the present study were suspension cultures. At a high density, the cells formed aggregates and the medium became turbid upon gentle agitation. The cells were subcultured or diluted when reaching to appropriate densities to maintain exponential growth.

To evaluate the inhibitory effect of curcumin on DLBCL cell proliferation and calculate its IC₅₀ values, the following procedures were performed: SU-DHL-8 and SU-DHL-10 cells were seeded in 24-well plates at 1×10⁵ cells/well (n=5). The cells were then treated with increasing concentrations of curcumin (0, 10, 20, 40 and 60 µM). After 24 h, cell viability was measured using a CCK-8 assay according to the manufacturer's protocol. Specifically, 10 µl CCK-8 solution was added to each well and incubated for 1–1.5 h. Absorbance was measured at 450 nm using a microplate reader. Cell viability was calculated as: (ODsample-ODblank)/(ODcontrol-ODblank) ×100%, with control groups set as 100% viability.

Following treatment, cells were collected by centrifugation at 200 × g for 5 min at 4°C. The supernatant was discarded, and the cell pellet was washed with PBS, transferred to a new microcentrifuge tube and centrifuged again under the same conditions. The supernatant was then carefully removed. The cell pellet was resuspended in 70–110 µl ice-cold lysis buffer (Beyotime Biotechnology) supplemented with 1% protease and phosphatase inhibitors. The suspension was vortexed for 15 sec at 5 min intervals and incubated on ice for 30 min. The lysate was centrifuged at 15,000 × g for 20 min at 4°C. The supernatant was collected, and the protein concentration was determined using a BCA protein assay kit (cat. no. 23227; Thermo Fisher Scientific, Inc.). Protein samples were mixed with 5X loading buffer (1:4 ratio) and denatured by heating at 95°C for 10 min. Samples were either used immediately or stored at −80°C for subsequent western blot analysis of relevant protein expression.

Treated cells were collected by centrifugation at 200 × g for 5 min at 4°C. After discarding the medium, the cell pellet was washed with PBS, transferred to a new tube and centrifuged as previously described. The supernatants were carefully aspirated. The pellet was resuspended in 200 µl ice-cold Cytoplasmic Extraction Reagent A (cat. no. P0028-1; Beyotime Biotechnology) containing 1% protease/phosphatase inhibitors, vortexed vigorously for 5 sec and incubated on ice for 15 min. Cytoplasmic Extraction Reagent B (10 µl) (cat. no. P0028-2; Beyotime Biotechnology) was added, followed by vortexing for 5 sec, incubation on ice for 1 min and vigorous shaking for 1 min. The tube was vortexed again for 5 sec and centrifuged at 14,000 × g for 10 min at 4°C. The cytoplasmic supernatant was transferred to a pre-chilled tube for immediate use or storage at −80°C. The nuclear pellet was washed three times with 200 µl ice-cold PBS by centrifugation at 3,000 × g (4°C). The pellet was resuspended in 50 µl Nuclear Extraction Reagent (cat. no. P0028-3; Beyotime Biotechnology) with inhibitors and vortexed vigorously for 15–30 sec. The suspension was incubated on ice with intermittent vortexing (15–30 sec every 1–2 min) for 30 min. After centrifugation at 14,000 × g for 10 min (4°C), the nuclear extract (supernatant) was collected. The protein concentrations of the cytoplasmic and nuclear fractions were determined separately using a BCA assay. The fractions were mixed with 5X loading buffer (1:4) and denatured at 95°C for 10 min. Samples were used immediately or stored at −80°C for analysis of nuclear translocation of proteins such as AIF and MIF.

Cell suspensions were mixed with an equal volume of 0.4% trypan blue solution. A 10 µl aliquot was loaded onto a hemocytometer, incubated for 3 min at room temperature and viable cells were counted using an automated cell counter. Cell viability was expressed as a percentage of the control group (set as 100%). This was conducted for direct evaluation of the effects of curcumin and its combined treatments on cell viability.

Protein concentrations were determined using the BCA assay to ensure consistent sample loading in western blot and related experiments, as detailed in the following protocol.

Briefly, a working solution was prepared by mixing the BCA reagents A and B in a 50:1 ratio. A standard curve was generated by adding 0–20 µg standard protein to a 96-well plate, followed by volume adjustment to 25 µl with deionized water. Subsequently, 2 µl each protein sample was loaded into the plate and also adjusted to 25 µl with deionized water. Then, 200 µl BCA working solution was added to each well, followed by incubation at 37°C for 30 min protected from light. Finally, the absorbance was measured at 562 nm using a microplate reader, and sample protein concentrations were calculated based on a standard curve.

Western blot was performed to detect the expression and localization changes of PAR polymers, PARP-1, AIF, MIF and apoptosis- and necroptosis-related proteins, following the detailed procedures below.

Whole-cell lysates were prepared using lysis buffer (Sigma-Aldrich; Merck KGaA) with 1% protease/phosphatase inhibitors on ice for 30 min, followed by centrifugation at 14,000 × g for 30 min at 4°C. Protein concentration was determined using the BCA method. Nuclear and cytoplasmic fractions were isolated using a commercial extraction kit (cat. no. P0028; Beyotime Biotechnology) according to the manufacturer's instructions. Proteins (20 µg) were separated using 7.5, 10 and 12.5% SDS-PAGE gels according to their molecular sizes and transferred to PVDF membranes. Membranes were blocked with 5% skim milk and incubated with primary antibodies at 4°C overnight. After washing with TBST (0.1% Tween, 3×10 min), the membranes were incubated with horseradish peroxidase-conjugated secondary antibodies (1:5,000; cat. nos. AS014 and AS0003; ABclonal Biotech. Co., Ltd.) for 1 h at room temperature. Signals were detected using an ECL substrate and a chemiluminescence imaging system (Tanon). The following primary antibodies were used: GAPDH (1:10,000; cat. no. 600-GAPDHt; Trevigen Inc.), AIF (1:1,000; cat. no. #4642; Cell Signaling Technology, Inc.), MIF (1:1,000; cat. no. ab7207; Abcam), PAR (1:1,000; cat. no. #84510; Cell Signaling Technology, Inc.), PARP (1:1,000; cat. no. #9542; Cell Signaling Technology, Inc.), BCL-2 (1:1,000; cat. no. #3498; Cell Signaling Technology, Inc.), BCL-6 (1:1,000; cat. no. WL03134; Wanleibio Co., Ltd.), c-Myc (1:1,000; cat. no. A5011; Selleck Chemicals), Bax (1:1,000; cat. no. A19684; ABclonal Biotech Co., Ltd.), receptor interacting protein 1 (RIP1; 1:1,000; cat. no. #3493; Cell Signaling Technology, Inc.), receptor interacting protein 3 (RIP3; 1:1,000; cat. no. #13526; Cell Signaling Technology, Inc.), mixed lineage kinase domain like pseudokinase (MLKL; 1:1,000; cat. no. #14993; Cell Signaling Technology, Inc.), cleaved caspase-3 (1:1,000; cat. no. #9661; Cell Signaling Technology, Inc.) and caspase-3 (1:1,000; cat. no. #9662; Cell Signaling Technology, Inc.). Band intensities from three independent experiments were quantified using ImageJ 1.53t software (National Institute of Health).

UVB irradiation was employed to mimic the DNA-damaging stimuli of radiotherapy, thereby investigating the synergistic effects of curcumin combined with ultraviolet treatment. A Bio-Rad UVB irradiation system (Bio-Rad Laboratories, Inc.) was used, which emits ultraviolet light at wavelengths of 280–320 nm to generate UVB radiation. Before UVB exposure, the irradiation device was thoroughly sterilized with 75% ethanol. Subsequently, the cells were covered with 6-well plate lids and placed on a UV-transparent tray and irradiated at an intensity of 50 mJ/cm². Following UVB exposure, the cells were returned to the incubator for further incubation, allowing subsequent experiments to proceed. To ensure consistency and comparability in the present study and based on preliminary research findings (data not shown), the UVB irradiation time for SU-DHL-8 cells across all groups was set at 60 sec, whereas for SU-DHL-10 cells it was set at 120 sec across all groups.

Immunofluorescence staining was conducted to directly visualize the subcellular localization of target proteins.

SU-DHL-10 cells (1×10⁶ cells/ml) were seeded in 6-well plates and treated as indicated for 24 h. Cells were fixed with 4% paraformaldehyde (20 min, room temperature), permeabilized with 0.5% Triton X-100 (20 min) and washed with PBST. After blocking with 5% BSA (15 min, room temperature), cells were incubated with primary antibodies (AIF, cat. no. #4642; 1:50; PARP-1, cat. no. #9542; 1:200; Cell Signaling Technology, Inc.) overnight at 4°C. The cells were then incubated with an FITC-conjugated secondary antibody (1:200; cat. no. AS014; ABclonal Biotechnology Co., Ltd.) for 1 h at room temperature counterstained with DAPI and mounted with an anti-fade reagent. Images were acquired using a fluorescence microscope (Nikon Corporation).

To distinguish between apoptotic and non-apoptotic cell death, cell death modalities were assessed via nuclear staining and membrane integrity markers. SU-DHL-10 cells (1×10⁶ cells/ml) were seeded in 6-well plates, treated as indicated and incubated for 24 h. The cells were harvested and incubated in the dark at room temperature for 20 min with a solution containing DAPI (1:100 in PBS; Beijing Solarbio Science & Technology Co., Ltd.) and propidium iodide (PI; 1:20 in PBS; Beyotime Biotechnology). The cells were then washed three times with PBS. The stained cells were visualized using a fluorescence microscope (Nikon Corporation).

Statistical analyses were performed using SPSS 22.0 (IBM Corp.) and GraphPad Prism 8.0.1 (Dotmatics). For comparisons among multiple groups, one-way analysis of variance (ANOVA) was used, followed by Tukey's HSD test for post hoc pairwise comparisons. Data are presented as the mean ± SD from at least three independent experiments. A P-value of <0.05 was considered statistically significant, and a P-value of <0.01 was considered highly statistically significant. All experiments were performed at least in triplicate.

The effect of curcumin on DLBCL cell viability was assessed using the CCK-8 assay. Cells were treated with curcumin (0, 10, 20, 40 or 60 µmol/l) for 24 h. Curcumin significantly inhibited the viability of SU-DHL-8 and SU-DHL-10 cells in a concentration-dependent manner, with IC₅₀ values of 22.12 and 39.22 µmol/l, respectively (Fig. 1A). To distinguish apoptotic from non-apoptotic cell death, the pan-caspase inhibitor Q-VD-OPh was used (44,45). Based on preliminary data and literature (45), cells were treated with 20 nmol/l Q-VD-OPh and 10 or 20 µmol/l curcumin for 24 h. In SU-DHL-8 cells, co-treatment with Q-VD-OPh (Cur20 + Q) significantly rescued cell viability compared with treatment with curcumin alone (Cur20). By contrast, Q-VD-OPh had no protective effect on SU-DHL-10 cells (Fig. 1B). Consistently, DAPI/PI staining showed a significant increase in stained cells after curcumin (20 µmol/l) treatment in both cell lines. This increase was attenuated by Q-VD-OPh in SU-DHL-8 cells, but not in SU-DHL-10 cells (Fig. 1C and D), indicating that curcumin-induced death in SU-DHL-10 cells was largely caspase-independent.

To investigate the mechanism of curcumin-induced cell death, the basal expression of c-Myc, BAX, BCL-2 and BCL-6 was examined. The effects of curcumin on caspase 3 and PARP-1 cleavage were assessed using western blotting. SU-DHL-10 cells lacked BAX expression, but showed higher levels of BCL-2, BCL-6 and c-Myc than SU-DHL-8 cells (Fig. 1E). Upon curcumin treatment, cleaved caspase-3 and cleaved PARP-1 levels significantly increased in SU-DHL-8 cells. This effect was suppressed by Q-VD-OPh. By contrast, cleaved caspase-3 and cleaved PARP-1 were undetectable in SU-DHL-10 cells under all conditions (Fig. 1G). These results confirmed that curcumin induces caspase-dependent apoptosis in SU-DHL-8 cells but triggers a non-apoptotic cell death pathway in SU-DHL-10 cells. Although RIP1 expression was higher in SU-DHL-10 cells, the key necroptosis mediators RIP3 and MLKL were expressed at very low levels (Fig. 1F), which is consistent with a previous report (46). Thus, necroptosis is unlikely to contribute to cell death in SU-DHL-10 cells.

To investigate the role of parthanatos, SU-DHL-10 cells were treated with 20 µM curcumin for 24 h, and the levels of PAR polymers were measured. The PARP-1 inhibitor olaparib (10 µM) and the pan-caspase inhibitor Q-VD-OPh (20 nM) were used for mechanistic validation. Western blot analysis showed a significant increase in PAR polymer levels in curcumin-treated SU-DHL-10 cells compared with those in the untreated control group (Fig. 2A and B). This increase was significantly suppressed by olaparib (Cur20 + Ola), but not by Q-VD-OPh (Cur20 + Q) (Fig. 2A and B). Furthermore, curcumin treatment significantly increased the nuclear protein levels of PARP-1, AIF and MIF, which were reversed by olaparib (Fig. 2C and D). Immunofluorescence staining consistently revealed the enhanced nuclear localization of both AIF and PARP-1 after curcumin treatment, which was attenuated by olaparib treatment (Fig. 2E and F).

SU-DHL-10 cells are relatively insensitive to DNA-damaging stimuli such as UVB (47) (Fig. 3A). To explore the combined effects of radiotherapy, SU-DHL-10 cells were treated with a low-dose of curcumin and UVB irradiation for 24 h. The CCK-8 assay showed that combined treatment with curcumin (10 or 20 µM) and UVB significantly reduced cell viability compared with single-agent treatments (Fig. 3B). Notably, the addition of Q-VD-OPh to the curcumin (10 µM) and UVB combination further decreased cell survival in the trypan blue exclusion assay (Fig. 3C). DAPI/PI staining confirmed a synergistic increase in cell death with the Cur10 + UV combination, which was not inhibited by Q-VD-OPh (Fig. 3D and E). Western blotting analysis confirmed the absence of cleaved caspase-3 and cleaved PARP-1 in cells treated with curcumin alone or in combination with UVB (Fig. 3F).

To determine whether parthanatos mediated the combined effect, PAR polymer expression was evaluated in SU-DHL-10 cells treated with curcumin and UVB. The PAR polymer levels were significantly higher in the Cur10 + UV group than in either treatment alone. Olaparib, but not Q-VD-OPh, effectively suppressed this increase (Fig. 4A and B). Furthermore, the nuclear levels of PARP-1, AIF and MIF were significantly elevated by the Cur10 + UV combination compared with the single treatments, and this elevation was reversed by olaparib (Fig. 4C and D). Immunofluorescence staining confirmed the enhanced nuclear translocation of AIF and PARP-1 induced by the Cur10 + UV combination, which was inhibited by olaparib (Fig. 4E and F).