The murine intestinal epithelial cell line MODE-K (Shanghai Jining Industrial Co., Ltd., Shanghai, China) was adopted for the study. The cells were washed with a cell culture solution that was comprised of the 1640 medium (PM150910; Procell, Wuhan, China) +10% fetal bovine serum (FBS, Gibco, Carlsbad, NM, United States) solution (pH 7.2–7.4) +1% penicillin-streptomycin (Sigma, St. Louis, MO, United States) to remove DMSO. The resuscitated cells were cultured in a fresh cell culture solution and under 5% CO₂ saturated humidity at 37°C. The cell culture experiments were performed in triplicate with α-chaconine treatment at concentrations of 0, 0.4, and 0.8 μg/mL. α-Chaconine stock solution (16 mg/100 mL) was made and diluted with the cell culture solution. The choice of the concentrations was based on pilot trials. Measurements were performed in triplicate after incubation for 24, 48, and 72 h.

The transepithelial electrical resistance (TEER) values of the MODE-K cells after 24, 48, and 72 h of incubation with α-chaconine were measured using a Millicell ERS-2 V-Ohm Meter (MERS00002, EMD Millipore Ltd., Watford, United Kingdom). Measurements were conducted in triplicate at three points in different directions in each Transwell (Corning^® Transwell polycarbonate membrane inserts, Cat No. 3422, 8 μm pore size; 6.5 mm membrane diameter, Corning Incorporated, Tewksbury, MA, United States) according to the manufacture’s instructions. The measured datum multiplied by the Transwell membrane area (0.6 cm²) gave the TEER value of the sample in units of Ω × cm² (Pan et al., 2013). The activities of alkaline phosphatase (AKP) and lactate dehydrogenase (LDH) in cells were measured according to the kit instructions (Nanjing Jiancheng Bioengineering Research Institute, Nanjing, China).

The distribution of tight junction proteins zonula occludens-1 (ZO-1) and occludin were determined using immunofluorescence staining (Im et al., 2019). MODE-K cells were grown on glass slides and treated with 0, 0.4, or 0.8 μg/mL α-chaconine for 24, 48, or 72 h. After washing with PBS three times for 3 min each time, the cells were fixed with 4% paraformaldehyde for 15 min at room temperature and washed again as previously described. The cells were then permeabilized with 0.5% Triton X-100 (made with PBS) for 20 min. After washing as before and the medium removed, the cells were blocked with goat serum for 30 min at room temperature. After the blocking solution was removed by drawing off with paper tissue, the cells were incubated with rabbit anti-claudin (59 KD; diluted 1:100; 13409-1-AP) and anti-ZO-1 (230 KD; diluted 1:100; 21773-1-AP) antibodies (Wuhan Sanying Biotechnology Ltd., Wuhan, China) overnight at 4°C. The cells were washed three times with PBST (phosphate buffered saline Tween-20) and incubated with Cy3-conjugated secondary antibody goat anti-rabbit IgG (diluted 1:100; CWBIO, Beijing, China) for 2 h at 37°C. For staining, after three washes with PBST, DAPI (4’,6-diamidino-2-phenylindole) was added and incubated for 5 min in the dark. The stained cells were washed thoroughly with PBST four times for 5 min. After the slides were sealed with a slide containing an anti-fluorescence quenching agent, images were captured using a fluorescence microscope (Olympus BX53; Olympus, Center Valley, PA, United States) and attached a camera (Olympus DP72; Olympus, Center Valley, PA, United States).

The relative levels of tight junction proteins ZO-1 and occludin in MODE-K cells were determined using the Western Blot method (Pan et al., 2013). After the removal of the culture medium, the α-chaconine-treated cells were washed with 10 mM PBS (pH 7.2–7.3) three times. Proteins were extracted from the cells with PMSF (ST506, Beyotime Biotechnology, Shanghai Ltd., China)-containing cell lysate (P0013B; Beyotime Biotechnology Ltd., Shanghai, China). The extracted proteins were determined for total protein content using a BCA assay kit (P0010; Beyotime Biotechnology Ltd., Shanghai, China). After the preparation of 5–12% sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE), 15 μL of cell protein extracts (1 mg/mL) was loaded for separation. The separated proteins were transferred onto nitrocellulose using the semidry transfer film method. The membranes were blocked in 3% non-fat milk/TBST (tris buffered saline Tween-20) (pH 7.6) at room temperature for 2 h and then incubated with polyclonal rabbit anti-claudin (59 KD; diluted 1:1000; 13409-1-AP; Wuhan Sanying Biotechnology Ltd., Wuhan, China), polyclonal rabbit anti-ZO-1 (230 KD; diluted 1:800; 21773-1-AP; Wuhan Sanying Biotechnology Ltd., Wuhan, China), or monoclonal mouse anti- β-actin (42 KD; diluted 1:200; BM0627; Boster Biological Technology Co., Ltd., Wuhan, China) antibodies diluted in TBST buffer overnight at 4°C. After washing with the TBST buffer 5–6 times for 5 min, the membranes were incubated with goat anti-rabbit IgG HRP-conjugated secondary antibodies (diluted 1:50000, BA1054; Boster Biological Technology Co., Ltd., Wuhan, China) for 1.5 h at 37°C. The membranes were washed with TBST buffer 5–6 times for 5 min and visualized for immunoreactive bands using chemiluminescence with an ECL detection kit (Santa-Cruz Biotechnology, Santa Cruz, CA, United States). The bands were scanned for gray levels and quantification was performed using Quantity One software with the integrated density value of β-actin for normalization.

The total RNA was extracted using the Aidlab kit (Aidlab Biotechnologies Co., Ltd., Beijing, China) in the TRIzol method (Heidary and Kakhki, 2014) and stored at −80°C for later use. RNA was reverse transcribed into cDNA using the common reverse primer Oligo (dT) with a cDNA synthesis kit (Vazyme Biotech Co., Piscataway, NJ, United States). The reverse transcription reaction system is shown in Table 1. The cDNA was diluted 10-fold and detected using the real-time fluorescence quantitative PCR detection technique. The reaction system is shown in Table 2. The primers were designed and synthesized by Wuhan Biofavor Biotech Services Co. Ltd. (Wuhan, China) and are listed in Table 3. The quantification of mRNA expression of genes was made with β-actin as the internal reference gene.

The levels of malondialdehyde (MDA) and total glutathione (T-GSH) and the enzyme activities of superoxide dismutase (SOD), catalase (CAT), glutathione peroxidase (GSH-Px), and γ-glutamylcysteine synthetase (γ-GCS) were all determined using test kits (Nanjing Jiancheng Bioengineering Research Institute, Nanjing, China) in accordance with corresponding instructions.

Triplicate readings for each measurement were averaged before statistical analysis. The data for statistical analysis were put to the general linear model with α-chaconine concentration, incubation time, and their interaction as the fixed effects and incubation time as the repeated measurement and analyzed using SPSS19.0 software. The Ducan’s multiple comparison test was used to determine statistical differences among the means. Probability levels below 0.05 were considered statistically significant.

α-Chaconine concentration and incubation time had statistically significant effects on the proliferation, cell cycle, and apoptosis of mouse intestinal epithelial cells (Table 4).

The cell proliferation rate did not change significantly over time in the control (0 μg/mL) cells, however, it significantly decreased with increasing incubation time in the 0.4 and 0.8 μg/mL groups. The cell proliferation rate significantly decreased with increased α-chaconine concentration at the same incubation time.

The G₀/G₁ ratio significantly increased with incubation time in all treatments and with α-chaconine concentration. The proportion of cells in the S stage of the cell cycle was less by 10% (P < 0.001) at 48 h of incubation than at 24 h and did not further decrease (P > 0.05) until 72 h for the control group. The proportion also significantly decreased with incubation time for the α-chaconine-treated groups and the extent of decrease was similar (P > 0.05) for the two α-chaconine-treated groups. The average decrease was 13% (P < 0.001) at 48 h and 24% (P < 0.001) at 72 h compared with 24 h. The G₂/M ratio in the control group first increased and then decreased with time. When α-chaconine was added at 0.4 μg/mL, the G₂/M ratio did not change until 48 h (P > 0.05) but was significantly lower at 72 h than at 24 and 48 h of incubation. When the α-chaconine concentration was increased to 0.8 μg/mL, the G₂/M ratio significantly decreased with incubation time. At 24 h of incubation, α-chaconine concentration had no significant effect on G₂/M ratios, however, at 48 and 72 h, the G₂/M ratio significantly decreased with the concentration.

The apoptosis rate was significantly higher at 72 h than at 24 h in the untreated cells, higher at 48 and 72 h than at 24 h in the 0.4 μg/mL treated cells, and higher at 72 h than at 24 and 48 h in the 0.8 μg/mL treated cells. When a comparison was made for different α-chaconine concentrations at the same incubation time, the apoptosis rate was always related with α-chaconine concentration.

The α-chaconine concentration and incubation time significantly affected the concentrations of MDA and T-GSH, the activities of GSH-Px and γ-GCS, but did not significantly affect the level of the activities of SOD and CAT (Table 8).

In the control cells, levels of measured parameters were unchanged with incubation time, but the addition of α-chaconine increased the content of MDA and decreased the levels of other measured parameters. The responses changed linearly with incubation time, but the responses to α-chaconine concentration differed in extent for different measurements. The treatment of 0.4 μg/mL α-chaconine at 24 h resulted in a decrease by 2, 5, 8, 11, and 3% for the content of T-GSH and for the activities of SOD, CAT, GSH-Px, and γ-GCS, respectively, compared with the control. When α-chaconine was added at 0.8 μg/mL, the extent of decrease in these measurements was 33, 25, 27, 36, and 22%, respectively, compared with the control.

The α-chaconine concentration and incubation time on mouse intestinal epithelial cells had significant effects on the mRNA expression of SOD, CAT, GSH-Px, and γ-GCS genes (Table 9). In the control cells, the mRNA expression of these genes did not change over time gene. However, in the 0.4 μg/mL treated cells, at 24 h, exception for SOD which dropped slightly (by 6%, P > 0.05), the expression of all the other genes was significantly decreased (P < 0.05) by 18–23% compared with the control cells. The expression was further decreased by 25–30% at 48 h and by 51–61% at 72 h of incubation compared with the control cells for all the four genes. The difference between 24 and 48 h of incubation was not significant but was significantly different (P < 0.05) between 48 and 72 h. In the case of the 0.8 μg/mL treated cells, the mRNA expression of all genes was 31–44% lower than the control cells at 24 h of incubation. The decrease in the mRNA expression was greater than at 24 h, being 42–55% at 48 h and 57–69% at 72 h of incubation in comparison to the control cells.

The cell proliferation measured by the MTT method can reflect the cell survival and growth ability and can also indirectly reflect the degree of epithelial cell membrane damage (Wang et al., 2017). The results obtained in this study showed that the MTT value of the cells decreased with the increase of α-chaconine concentration and the prolongation of incubation time, suggesting that α-chaconine leads to damage to cell morphology, a reduction in cell viability, and to cytotoxicity. It has been reported that α-chaconine had toxicity to intestinal crypt epithelial cells (IEC-6) and ileal cells (IEC-18) of rats and reduced the MTT values of these cells (Gee et al., 1996). It can be speculated that after α-chaconine reaches the epithelial cells, it may alter or destroy the structure of the cell in some way to affect the metabolism of the cell, and eventually lead to the blocking of cell proliferation.

The cell cycle and apoptosis processes synergize to some extent, in that some key cell cycle regulatory proteins are involved in the regulation of the apoptosis process (Xu et al., 2020). The start and the end of apoptosis are dependent on the operation of the cell cycle, and the stage of the cell cycle phase dictates the exact time when apoptosis begins during the completion of the cell cycle (Dong et al., 2019). Drug based apoptotic agents interfere with the cell proliferation cycle, inhibit the normal transformation during the cell cycle, and promote cell death (Zhang and Shi, 2011). Hence, the process of apoptosis can cause a series of changes in the structure of cell membranes, loss of mitochondrial function, degradation of proteins in cells, and changes in DNA cleavage, etc.

The cell cycle consists of two phases: mitosis (M) and mitotic intervals (G₁, S, and G₂), while the proliferative capacity of cells is mainly reflected in the G₂ and S phases (Li and Xu, 2019). The increase in the length of G₀/G₁ phase with α-chaconine observed in this study suggests that α-chaconine can increase the number of MODE-K cells in the G₀/G₁ phase, resulting in more cells in DNA repair processes; while the decrease in the S phase leads to a reduction in the number of cells in DNA synthesis phases, with the decrease in the G₂/M phase causing a decrease in the synthesis of RNA and proteins. α-Chaconine can bind to cell homogenates of various tissues, but not to DNA or RNA fragments isolated from mouse hepatocytes (Sharma et al., 1983). Thus, α-chaconine induces apoptosis in more than one way, and other ways are suggested such as by increasing the synthesis of intracellular nitric oxide to reduce the mitochondrial membrane potential or intracellular Ca²⁺ concentration for the activation of apoptotic proteins (Toyoda et al., 1991).

The transepithelial electrical resistance (TEER) value is an important indicator reflecting the integrity of epithelial cells and cell membrane permeability (Sheridan et al., 2020). α-Chaconine can affect intestinal permeability in mice, thereby disrupting intestinal barrier function (Patel et al., 2002). In this study, the TEER value showed an α-chaconine dose- and incubation time-dependent decrease, which may be due to an α-chaconine-induced change in the structure of the epithelial cell membrane (Friedman et al., 1996; Friedman and McDonald, 1997). This result could account for the mechanism of the in vivo effects (Friedman et al., 1997) which result in the alteration of the ion transepithelial transport channel, a decrease in TEER, and an increase in the permeability of the intestine, consequently causing the loss of protein and other nutrients from the intestine, and the invasion of bacteria and other antigens into the bloodstream.

Alkaline phosphatase is an endogenous enzyme in tissues and cells. Intestinal AKP is distributed in large quantities in intestinal tissues and plays an important role in maintaining the integrity of intestinal epithelial cells. Alkaline phosphatase is an important binding protein on the cell membrane and plays an important regulatory role in cell growth, viability, and metabolism (Bol-Schoenmakers et al., 2010). If AKP is lost from the intestine, the permeability of epithelial cells will increase, causing inflammation and sepsis, and other diseases (Bates et al., 2007). Therefore, the determination of extracellular AKP activity is another important indicator for the detection of cell membrane permeability and integrity. The present study showed that α-chaconine treatment enhanced the extracellular AKP activity of mouse small intestinal epithelial cells, which may be due to α-chaconine changing the cell membrane structure and further causing the increased permeability. A study showing that soybean agglutinin induces an increased AKP activity of IPEC-J2 cells also highlighted the importance of intestinal AKP in the maintenance of the integrity of intestinal epithelial cells (Pan et al., 2013).

Lactate dehydrogenase is the key enzyme for cellular energy metabolism and exists in the cell cytoplasm. The change of LDH enzyme activity in the culture medium is a very sensitive indicator of cytotoxicity (Yuan et al., 2019). Under normal physiological conditions, the LDH enzyme is present within the cell. If the cell membrane is destroyed, the LDH enzyme in the cell will leak to the outside of the cell, increasing the activity of the extracellular LDH enzyme (Xiao et al., 2020). This study found that the LDH activity of the cells increased with α-chaconine treatment in a dose- and time-dependent manner, which is consistent with the findings that LDH activity increased with the addition of α-chaconine or α- solanine into rat glioma cells (Yamashoji and Matsuda, 2013). The effect of α-chaconine on rat IEC-6 and IEC-18 cells also led to the release of intracellular LDH and the increase of LDH content in the extracellular fluid (Gee et al., 1996). A similar result was also reported with human intestinal epithelial cell line Caco-2 (Mandimika et al., 2007). These results suggest that the cell structure is damaged by α-chaconine, resulting in increased permeability of the cell membrane and impaired mechanical barrier function of the cell, and consequently leading to a large number of intracellular enzymes, possibly including apoptotic signaling molecules, entering the extracellular space and stimulating cell apoptosis. Destructive effects on the cell membrane are considered to be the most important mechanism for glycoalkaloids by which the structural and functional integrity of cells or tissues of organisms are damaged (Roddick et al., 1988; Smith et al., 2001; Nenaah, 2011). From the results of this study, we concluded that α-chaconine destroys the mechanical barrier of intestinal mucosal cells by affecting the structure of the cell membrane and the transepithelial cell electrical resistance.

The tight junction is an important structure to maintain the mechanical barrier and permeability of mucosal epithelium. Cytoplasmic protein ZO-1 and the transmembrane protein occludin are two important proteins in tight junctions (Van Itallie and Anderson, 2014). They are not only involved in regulating cell material transport and maintaining epithelial polarity, but are also related to information transmission and the regulation of cell proliferation and differentiation, gene transcription, and other processes. The presence and quantity of ZO-1 and occludin proteins reflect the mechanical barrier of the intestine. As a result, their distribution and relative gene expression are reliable indicators for the state of intestinal tight junction and the disruption of barrier function (Cai et al., 2018). The expression of ZO-1 and occludin can affect the TEER value.

The results of this study showed that the distribution and relative expression of ZO-1 and occludin in cells decreased with α-chaconine treatment in a dose- and time-dependent manner. The reduction of ZO-1 and occludin protein levels damages mainly the intestinal mucosal barrier, which is consistent with reports in the literature (Zhao et al., 2015; Yang et al., 2017).

Malondialdehyde is one of the most important products in the process of membrane lipid peroxidation, which not only indicates the degree of free radical production but also reflects the degree of lipid peroxidation and indirectly suggests the degree of cell damage (Barrera et al., 2018). The content of MDA is an indicator of the degree of lipid peroxidation. Superoxide dismutase can scavenge free radicals in the body and catalyze the decomposition of peroxyl radicals to form hydrogen peroxide. Glutathione is a very important antioxidant enzyme in organisms. It can scavenge hydrogen peroxide and lipid peroxides produced in the body and block the damage caused by reactive oxygen radicals (Pastore et al., 2003). Hydrogen peroxide can be converted into water by GSH-Px (Motoori et al., 2001) so that cells are protected from oxidative damage by peroxyl radicals. The reduction in SOD enzyme activity indicates that there are more free radicals in the body to be scavenged (Goc et al., 2017). Catalase can decompose a large amount of H₂O₂ into water and molecular oxygen, or catalyze the reduction of H₂O₂ by the O^2– provided by the hydrogen donor molecule to prevent the primary initiation of lipid peroxidation reaction, and thus reduce the damage of organic hydroperoxides (Ighodaro and Akinloye, 2018). Glutathione peroxidase accelerates the decomposition of H₂O₂ into water, and specifically catalyzes the reduction reaction of reduced glutathione and H₂O₂, to protect the integrity and function of cell membrane structure (Zhang et al., 2020). Glutamylcysteine synthetase is a dimer composed of regulatory and catalytic subunits of glutamylcysteine ligase. It is a rate-limiting enzyme for glutathione (GSH) synthesis, while GSH can neutralize free radicals and reactive ROS.

In this study, MDA content increased with the dose of α-chaconine and incubation time. We speculate that with the action of α-chaconine, mouse small intestinal epithelial cells might produce a large number of free radicals that trigger membrane lipid peroxidation (Pisoschi and Pop, 2015), which causes damage to the cell membrane system, destroys the oxidative metabolic process of cells, and results in oxidative damage to mitochondria. The significant decrease in T-GSH level and activities of SOD, CAT, GSH-Px, and γ-GCS may be due to the consumption of various oxygen free radicals (Hayes and McLellan, 1999) with α-chaconine, which leads to an increase in the sensitivity of small intestinal epithelial cells to oxidative damage in the present study.

The study of antioxidant enzyme genes has become an important research direction. The activity of antioxidant enzymes is determined by the mRNA expression of their genes and the stability, survival, and activity of the proteins. The addition of exogenous nutrients can affect the mRNA expression of antioxidant enzyme genes in an animal (Baker et al., 1998). The results of the present study showed that the mRNA expression of SOD, CAT, GSH-Px, and γ-GCS was decreased by the treatment of cells with α-chaconine, which reduced the defense ability of the cell’s antioxidant enzyme system against ROS, leading us to conclude that α-chaconine results in oxidative damage which may be one of reasons for the apoptosis of small intestinal epithelial cells.