The murine B16F10 and 4T1 cell lines were obtained from the American Type Culture Collection and maintained at 37°C in Eagle's minimal essential medium or RPMI-1640 medium (Nissui Pharmaceutical Co., Ltd.) containing 10% FBS (Nichirei Biosciences, Inc.), respectively. Human HaCaT keratinocytes (provided by Dr Takeda, Juntendo University, Tokyo, Japan) were maintained at 37°C in culture medium consisting of DMEM (Nissui Pharmaceutical Co., Ltd.) supplemented with 10% FBS, 100 U/l penicillin G and 100 mg/l streptomycin at 37°C with 5% CO₂. Human recombinant TRAIL (rTRAIL) was purchased from PeproTech, Inc.

B16F10NFκB and 4T1NFκB cells expressing firefly luciferase under the control of an NF-κB response element were established as previously described (11,12) and maintained at 37°C in RPMI-1640 medium containing 10% FBS. Briefly, B16F10NFκB and 4T1NFκB cells were generated by transfecting the B16F10 and 4T1 cell lines with pGL4.32-luc2P/NF-κB-RE/Hygro vector (Promega Corporation) using Lipofectamine^® 2000 (Invitrogen; Thermo Fisher Scientific, Inc.). The cells were selected on hygromycin B and cloned by limiting dilution.

B16F10NFκB cells and 4T1NFκB cells in the exponential growth phase were seeded at a final concentration of 4×10⁴ cells/well in a 96-well plate. After 3-h incubation, the cells were co-cultured with 50 µg/ml extract from 112 natural products (Table SI) for 24 h. At the end of the assay, 900 µg/ml D-luciferin was added, and the plates were incubated for another 30 min. Luciferase activity was measured by the GloMax^®-Multi Detection System (Promega Corporation).

Cell viability was quantified using the WST-1 cell proliferation reagent (Dojindo Molecular Technologies, Inc.). B16F10NFκB or 4T1NFκB cells were seeded on a 96-well plate and co-cultured with extracts from 112 natural products (Table SI) at 50 µg/ml for 24 h. In a separate experiment, HaCaT cells were seeded on a 96-well plate at a density of 10⁴ cells/well and pre-treated with 20 ng/ml rTRAIL for 1 h. The cells were then cultured with or without Sohakuhi extract (6.25 to 50 µg/ml) for 24 h. After incubation, WST-1 solution was added and used according to the manufacturer's instructions, and absorbance was measured at 450 nm using a microplate reader. Cell viability was calculated as a percentage of the control.

For measurement of the activities of caspase-3 and −7, the Caspase-Glo^® 3/7 assay system (Promega Corporation) was used according to the manufacturer's instructions. Briefly, HaCaT cells (5×10³ cells/well in a 96-well plate) were pre-treated with 20 ng/ml rTRAIL for 1 h. The cells were then cultured with Sohakuhi extract for 24 h, and the Caspase-Glo^® 3/7 reagent was then added. After 30-min incubation, caspase-3 and −7 activities were measured using the GloMax^®-Multi Detection System (Promega Corporation).

To identify the bioactive components of Sohakuhi extract, 200 g root bark of Morus alba Linn. was decocted in 1 l water for 50 min. The water extract was fractionated by water-methanol gradient reverse-phase medium-pressure liquid chromatography (RP-MPLC) fractionation. Mass spectrometry and ¹H-nuclear magnetic resonance (NMR) analysis were used to identify compounds in the isolated fractions. Extraction and isolation of Sohakuhi was conducted using a water-methanol gradient MPLC fractionation system and high-performance liquid chromatography (Accela™ HPLC system; Thermo Fisher Scientific, Inc.) profiles of water extracts of Sohakuhi were determined at 254-nm ultraviolet wavelength. A Capcell Pak C18 MG III S-5 (4.5×250 mm, 5 µm; Shiseido Co., Ltd.) column was used for HPLC analysis at a flow rate of 1 ml/min at 40°C. A gradient elution system composed of 5% CH₃CN (v/v) (A) and H₂O was used as follows: 0–4 min, 5% A; 4–8 min, 5–10% B; 8–12 min, 10–15% B; 12–15 min, 15–20% B; 15–18 min, 20–25% B; 18–21 min, 25–30% B; 21–25 min, 30–35% B; 25 min, 40% B. The active fraction was further analyzed using a CHCl₃-MeOH gradient RP-MPLC fractionation system with mass spectrometry and ¹H-NMR analysis to identify the active compounds of Sohakuhi. The MS conditions were set as follows: Negative ESI mode, spray voltage 4.5 kV, capillary voltage 40.0 kV, tube lens 150 V, capillary temperature 270°C, sheath gas flow rate 50 units, aux gas flow rate 10 units, and scan range m/z 50–2,000. A polytyrosine solution was used for instrument calibration before each experiment.

HaCaT cells were seeded at a density of 5×10⁵ cells/well and cultured for 24 h in a 6-well plate. After treatment, the cells were washed in cold PBS, scraped and lysed in whole-cell lysis buffer (25 mmol/l HEPES, pH 7.7; 300 mmol/l NaCl; 1.5 mmol/l MgCl₂; 0.2 mmol/l EDTA; 0.1% Triton X-100; 20 mmol/l β-glycerophosphate; 1 mmol/l Na₃VO₄; 1 mmol/l phenylmethylsulfonylfluoride; 1 mmol/l dithiothreitol; 10 mg/ml aprotinin; 10 mg/ml leupeptin). Cell lysates (10 µl/lane) were resolved by SDS-PAGE on 7.5–15% gels, then transferred to an Immobilon-P nylon membrane (EMD Millipore). The membranes were treated with Block Ace (Dainippon Sumimoto Pharma Co., Ltd.) for at least 2 h at room temperature, then probed with primary antibodies at 4°C overnight, followed by horseradish peroxidase-conjugated secondary antibodies (1:2,000; cat. nos. P0448 and P0260; Dako; Agilent Technologies, Inc.). Bands were visualized using ECL reagents (Amersham; Cytiva). The primary antibodies used were specific for Bcl-2 (clone no. D55G8; cat. no. 4223), Bcl-xL (clone no. 54H6; cat. no. 2764), p65 (clone no. L8F6; cat. no. 6956), phosphorylated-p65, (clone no. 93H1; cat. no. 3033; all Cell Signaling Technology, Inc.) and β-actin (clone no. C4; cat. no. sc-47778; Santa Cruz Biotechnology, Inc.). All primary antibodies were used at 1:1,000 dilution.

All data are presented as the mean ± SEM of three independent experiments. SPSS versions 23 and 25 software (IBM Corp.) were used to analyze data. Statistical analysis was carried out using one-way ANOVA followed by Bonferroni correction. P<0.05 was considered to indicate a statistically significant difference.

To identify novel anti-inflammatory agents in plant products, 112 medicinal plant extracts (Table SI) were screened for their effect on NF-κB activity using cell lines that express luciferase under the control of an NF-κB response element. Among the tested extracts, Sohakuhi markedly suppressed NF-κB activity without affecting the viability of 4T1 cells (Fig. 1A). Furthermore, NF-κB activity was suppressed by Sohakuhi extract in 4T1 cells and B16F10 cells in a dose-dependent manner (Fig. 1B). However, Sohakuhi extract did not display any cytotoxic effect, even at doses reaching 50 µg/ml (Fig. 1C).

To examine the biological utility of Sohakuhi extract, human HaCaT keratinocytes were incubated with rTRAIL as an inflammatory stimulus to induce NF-κB activation and cytotoxicity. Compared with the control, rTRAIL treatment induced significant cytotoxicity in HaCaT cells. However, pre-treatment with Sohakuhi extract significantly protected HaCaT cells from TRAIL-induced cytotoxicity in a dose-dependent manner (Fig. 2A). The cytoprotective effect of Sohakuhi extract was evident from microscopic observation of cell morphology (Fig. 2B). These results indicated the cytoprotective effect of Sohakuhi extract against TRAIL-induced cellular damage in human keratinocytes.

To confirm whether Sohakuhi extract affects NF-κB activation in HaCaT cells, the expression of the p65 subunit of NF-κB and its phosphorylation status following rTRAIL stimulation was assessed in the presence or absence of Sohakuhi extract (Fig. 3A). Phosphorylation of p65 was detectable in HaCaT cells following rTRAIL stimulation, but suppressed in the presence of Sohakuhi extract. While Sohakuhi extract treatment reduced total p65 expression in rTRAIL-stimulated HaCaT cells, there was almost no effect on the basal expression of p65 in unstimulated HaCaT cells, suggesting that the effect of Sohakuhi extract might be specific to TRAIL-induced NF-κB activity. Treatment with the Sohakuhi extract also showed an inhibitory effect on TRAIL-induced apoptosis, as seen in the suppression of caspase-3/7 activation (Fig. 3B). Importantly, the anti-apoptotic proteins Bcl-xL and Bcl-2 were upregulated in Sohakuhi extract-treated HaCaT cells following TRAIL stimulation (Fig. 3C). These results indicated that the cytoprotective effect of Sohakuhi extract might result from inhibition of TRAIL-induced apoptosis and regulation of anti-apoptotic proteins.

As Sohakuhi extract significantly inhibited NF-κB activity and displayed a cytoprotective effect against inflammation-associated cellular damage of human keratinocytes, the bioactive components of Sohakuhi extract were then analyzed. A total of 8 yield fractions were isolated from a Sohakuhi water extract using RP-MPLC with methanol-water gradient (Fig. 4A). The preparative HPLC data for these 8 yield fractions are presented in Fig. 4B. Amongst those fractions, fraction 8 effectively and exclusively inhibited NF-κB activity (Fig. 4C). Considering that fraction 8 was eluted with 100% methanol in the water-methanol gradient, the methanol extract of Sohakuhi was then fractionated into hexane, ethyl acetate, n-butanol and a residual water layer (Fig. 5A) to test the activity of each layer with respect to NF-κB inhibition. Amongst those layers, the ethyl acetate layer displayed very potent inhibition of NF-κB activity in 4T1 cells, even at the lowest dose tested, 5 µg/ml (Fig. 5B). These results indicated that the active component of Sohakuhi was fractionated into an ethyl acetate layer from the methanol extract.

Using a CHCl₃-MeOH gradient RP-MPLC fractionation system with mass spectrometry and ¹H-NMR analysis, two major compounds, moracin O and P, were identified in the ethyl acetate layer of Sohakuhi methanol extract (Fig. 6A). Importantly, both moracin O and P significantly inhibited NF-κB activity in 4T1 cells, starting at a dose of 3 nM (Fig. 6B). Additionally, both moracin O and P showed significant cytoprotective effects against TRAIL-induced cellular damage in HaCaT cells (Fig. 6C). Thus, moracin O and P were identified as active compounds of Sohakuhi that suppressed NF-κB activity and exerted a cytoprotective effect against TRAIL-induced damage in HaCaT cells.