The cells were isolated as described from Dong et al. (21). Briefly, cows with no signs of genital disease or microbial infection were selected in the slaughterhouse, based on the presence of foul smell, characteristic visual appearance, and vaginal discharge (1). The uterus was collected aseptically and stored on ice at 4°C until further treatment in the laboratory. The uterine horn was cut into 3–4-cm-long tissue blocks and was washed with PBS (pH value from 7.2 to 7.4). Then the tissue blocks were transferred to 0.1% streptose (P5147, Sigma, USA) diluted with DMEM/F-12 (D8900, Sigma, USA) and digested at 4°C for 16–20 h. Under sterile conditions, the tissue block was removed, and the endometrial tissue was scraped with a sterilized scalpel. The cell suspension was centrifuged at 100 × g for 5 min and washed with PBS three times. The cells were then collected and resuspended with DMEM/F-12 containing 15% fetal bovine serum (FBS, Gibco, USA) and 50 U/ml penicillin/streptomycin, and inoculated into a 25-cm² bottle. The cells were cultured in the incubator at 37°C and 5% CO₂ saturation humidity. The medium was changed every 1–2 days. The primary cells could be obtained after 3–4 days.

MEL (M3935, Sigma-Aldrich, USA) was dissolved in DMSO and stored at −20°C. It has been reported that the injection dose of 0.5 mg/kg MEL could maintain the blood concentration of 0.2 μg/ml MEL in cows with endometritis (22). In addition, MEL was used in a bovine lymphocyte test (23, 24), which provided references for MEL concentration in this experiment. In this study, two concentrations of MEL, 0.5 and 5 μM, were selected. First, 100 mg MEL was dissolved in 26.782 ml DMSO. Then, a 1 ml DMSO–MEL solution was added in 49 ml DMEM/F-12 for storage at −20°C. This storage concentration was 200 μM. MEL was filtered before use. The experiment was divided into four groups: the control group, the LPS group, the MEL group, and the LPS plus MEL co-treatment (LPS-MEL) groups. According to the results of previous reports in our lab, 10 μg/mL LPS (L2630, Sigma, USA) did not influence the cell viability of BEEC (25). Therefore, 10 μg/ml LPS was selected for this study.

The Cell Counting Kit-8 (CCK-8, Dojindo Molecular Technologies, Inc., Japan) was used to determine the effect of MEL and LPS on cell viability. The cells were seeded on 96-well plates with a density of 1 × 10³ cells per well and grew to 80% fusion in a 5% CO₂ incubator at 37°C. Then the cells were treated with 5 × 10⁻², 5 × 10⁻¹, 5, or 5 × 10¹ μM MEL or with 10 μg/ml LPS. CCK-8 was added into each well and incubated at 37°C for 2–4 h. The optical density was then read at 450 nm using a microplate (Tecan, Austria).

BEEC was treated with MEL or LPS or LPS–MEL for 24 h. The cells were washed twice with cold PBS and fixed with 70% ethanol at 4°C for 12–24 h. Then the cells were washed twice with cold PBS and resuspended with RNase A and propidium iodide (C1052, Beyotime, China) in the dark at 37°C for 30 min. Cell cycle was detected by flow cytometry (LSRFortessa, BD Biosciences, USA) and was analyzed by FlowJo software 7.6 (Becton, Dickinson, and Company, Ashland, USA) to obtain the relative number of cells in each phase of the cell cycle.

Before cell culture, three parallel lines, each 0.5 cm apart, were drawn on the back of a six-well plate using a marker pen. The cells were then seeded on this plate with a density of 1 × 10⁶ cells per well and were cultured overnight in a cell incubator with 5% CO₂ at 37°C. The cell scratch test started when the cells reached 90% fusion. The cells were scratched by using the tip of a 200 μl sterilized pipette. This scratching line was perpendicular to the previous three lines and was along the diameter of the well. The cells were quickly washed with PBS at least three times until no cell was visible at the scratch microscopically. Then the DMEM/F-12 containing LPS or MEL was added to the well. The cell treatments were as follows: LPS, MEL (0.5 or 5 μM), or LPS–MEL (0.5 or 5 μM).

The six-well plate was observed under the inverted microscope at ×100 magnification. Photos were taken immediately after the scratching (0 h) and at 3, 6, 12, and 24 h at fixed positions, which were localized with the help of the three parallel lines (Figure 1). The photos were analyzed by Image-Pro Plus software 6.0 (Media Cybernetics, Rockville, USA). The healing rate of the scratch reflects cell proliferation. The calculations were as follows:

The cells were seeded into a six-well plate and were treated with LPS, MEL (0.5 and 5 μM), or LPS–MEL (0.5 and 5 μM) for 0, 3, 12, and 24 h. Total RNA was extracted using TRIzol reagent (ET111, TRAN, China) according to the manufacturer's instruction. A Nanodrop 2000 spectrophotometer (Thermo, USA) was used to detect the quantity and purity of the RNA. The absorption ratio (A260/A280) was determined to be between 1.8 and 2.1. The total RNA was reverse-transcribed into cDNA by a PrimeScript RT regent kit gDNA eraser (DRR047A, Takara, Japan). The cycle conditions were as follows: 95°C for 2 min; 95°C for 5 s and 60°C for 34 s, 40 times; 95°C for 15 s; 60°C for 5 s; 60–95°C, 0.5°C gradient heating. The reaction system included 10 μl SYBR Premix Ex Taq™ II (RR820A, TaKaRa, Japan), 1 μl of each primer, 1 μl cDNA template in a final volume of 20 μl per reaction. The 2^−ΔΔCT method was used to calculate the relative abundances of mRNA transcripts (26). Each group was repeated three times. The β-actin (ACTB) was used as the internal control. The primers were designed according to the mRNA sequences of bovine ACTB, PTGS1, PTGS2, TLR4, VEGFA, cellular communication network factor 2 (CCN2), insulin-like growth factor 1 receptor (IGF1R), TGFB1, and TGFB3 published in GenBank. A single product was amplified by each primer pair. All the polymerase chain reaction (PCR) products were purified and sequenced (TsingKe Biotech, Beijing, China), and the sequence results were analyzed using BLAST and compared to the GenBank database (http://blast.ncbi.nlm.nih.gov/blast.cgi). The primer sequences are shown in Table 1.

BEECs were treated with LPS, MEL (0.5 and 5 μM), or LPS–MEL (0.5 and 5 μM). The total protein was extracted and quantified by a bicinchoninic acid protein assay kit (P0010, Beyotime, China). The protein (20–30 μg) was separated by 10% SDS–polyacrylamide gels and was transferred to the polyvinylidene difluoride (PVDF) membrane (Millipore, Germany). The PVDF membrane was incubated in 5% skimmed milk diluted by TBST (0.05% Tween-20 Tris-HCl buffer) to prevent its binding to non-specific protein. The primary antibody used for incubation included β-catenin, c-Myc, cyclin D1, glycogen synthase kinase-3β (GSK-3β), p-PI3K, PI3K, p-AKT, AKT, and β-actin at 4°C overnight. Then the PVDF membrane was incubated with horseradish peroxidase (HRP)-conjugated secondary antibody (diluted with 5% skimmed milk to 1:2,000) for 1 h at room temperature. Proteins were detected using a chemiluminescence assay. The antigen–antibody complex was visualized using a HRP substrate (Millipore, Billerica, MA, USA) and the ChemiScope 5300 Pro CCD camera (Clinx Science Instruments, Shanghai, China). The band intensity quantification was analyzed by Quantity One software (Bio-Rad, CA, USA). The primary antibodies of c-Myc (#5605), cyclin D1 (#2978), p-PI3K (#4228), PI3K (#4292), p-AKT (#4060), AKT (#4691), and β-actin (#4970) were purchased from Cell Signaling Technology. The β-catenin primary antibody (#ab32572) was purchased from Abcam (UK), and the GSK-3β primary antibody (#A2081) was purchased from ABclonal (China).

The cells were seeded on a 24-well cell culture plate and were treated with LPS, MEL (0.5 μM), or LPS–MEL (0.5 and 5 μM) for 15 min. Then the cells were fixed with 4% paraformaldehyde for 15 min. After washing with PBS, the membrane was penetrated with 0.4% Triton X-100 (ST797, Beyotime, China) for 15 min. The cells were washed with PBS three times and were blocked by 5% BSA for 1.5 h at room temperature. The cells were incubated with anti-β-catenin (all at 1:250 in 5% BSA) at 4°C overnight. After PBS washings for three times, the cells were incubated with an FITC-conjugated secondary antibody (A0423, Beyotime, China) for 1.5 h at room temperature. The nuclei were stained with DAPI (C1005, Beyotime, China). Finally, the cells were visualized with a fluorescence microscope (Leica TCS SP8, Leica Corporation, Germany).

The experiment was repeated at least three times. All the data were analyzed using SPSS 21.0 software (IBM, NY, USA). Statistically significant differences throughout this study were calculated by one-way ANOVA, followed by Dunnett's test. The data were shown as means ± standard error of means (SEM). A bilateral P < 0.05 was considered statistically significant.

The CCK-8 method was used to detect the effect of MEL on BEEC viability. The viability of BEEC was not influenced (P > 0.05) by various concentrations (5 × 10⁻², 5 × 10⁻¹, 5, and 5 × 10¹ μM) of MEL (Figure 2). As shown in Figure 3, no difference (P > 0.05) was observed in the cell viability between the cells treated with only LPS and the cells co-treated with LPS and MEL (0.5 and 5 μM).

The effect of MEL on the healing rate of BEEC was detected using the scratching test. There was no difference (P > 0.05) in cell migration at 24 h in cells treated with 0.5 or 5 μM MEL alone (Figure 4). The cell healing rate of the LPS group was lower (P < 0.01) than that of the blank control group. Compared with the LPS group, the cell healing rate decreased (P < 0.01) in the LPS–MEL groups (Figure 5).

The influence of MEL on the cell cycle of BEEC was determined using flow cytometry. As shown in Figure 6, MEL had no effect (P > 0.05) on the number of cells in each cell cycle. After treatment with LPS for 24 h, the number of cells increased (P < 0.01) in the S phase and decreased (P < 0.01) in the G2 phase, indicating the cell cycle arrest in the S phase. After treatment with LPS and MEL for 24 h, the number of cells decreased (P < 0.01) in the G1 phase and increased (P < 0.01) in the S phase, suggesting the cell cycle arrest in the G0/G1 phase (Figure 7).

The effects of MEL on the gene expressions of PTGS1, PTGS2, TLR4, and the growth factors (VEGFA, CCN2, IGF1R, TGFB1, and TGFB3) were detected using quantitative reverse-transcription PCR. As shown in Figures 8A,B, compared with the blank control, the gene expressions of PTGS2 and TLR4 increased (P < 0.01) after LPS stimulation at 3, 12, and 24 h. Compared with the LPS group, the PTGS2 gene expression decreased (P < 0.01) in LPS–MEL groups. There was no difference (P > 0.05) in the TLR4 transcription between the LPS group and the LPS–MEL groups. Compared with the blank control group, the gene expression of most growth factors showed no change (P > 0.05) or a downregulation (P < 0.05) after LPS treatment at observed time points, except TGFB3 at 12 and 24 h (Figures 8C–G). The gene expression of growth factors in LPS–MEL groups were generally lower (P < 0.05) than those in the LPS group at 3 and 12 h. Other than the decreased mRNA abundance of TGFB3 (P < 0.05) in the LPS–MEL groups as compared with the LPS group, we found no other differences (P > 0.05) at 24 h. The mRNA abundance of PTGS1 was not influenced (P > 0.05) by LPS or LPS–MEL treatment (Figure 8H).

The effects of MEL on the protein levels of β-catenin, c-Myc, cyclin D1, and GSK-3β were detected using western blot. As shown in Figure 9A, the protein level of β-catenin increased (P < 0.01) at 15 and 45 min and decreased (P < 0.01) at 60, 75, and 90 min. The levels of c-Myc and cyclin D1 increased (P < 0.05) at 15 and 30 min. The level of GSK-3β increased (P < 0.05) at 15, 30, and 45 min. Based on these results, we selected 15 min to detect the changes in the Wnt/β-catenin pathway in subsequent experiments.

MEL (0.5 and 5 μM) treatment alone did not influence (P > 0.05) the protein levels of β-catenin, c-Myc, cyclin D1, or GSK-3β as compared with the blank control (Figure 9B). LPS stimulation caused an increase (P < 0.01) in the levels of β-catenin, c-Myc, cyclin D1, and GSK-3β (Figure 9C). Compared with the LPS group, the levels of these proteins were lower (P < 0.01) in the LPS–MEL groups.

As shown in Figure 10, the β-catenin level on the cytomembrane in the MEL (0.5 μM) group was similar to that in the control group. In the LPS group, an increased number of β-catenin was observed to enter the nucleus. Compared with the LPS group, the amount of β-catenin in the nucleus in LPS–MEL groups seemed lower, and the β-catenin was mainly detected in the cytomembrane.

The influence of MEL on the PI3K/AKT pathway was detected using western blot and is depicted in Figure 11A. The phosphorylation levels of PI3K and AKT showed similar trends. The p-PI3K/PI3K ratio increased (P < 0.01) at 10 min, whereas the of p-AKT/AKT ratio increased (P < 0.05) at 5 and 10 min and decreased at 15 min. Based on these results, the time point of 10 min was selected for subsequent experiments.

MEL alone (0.5 or 5 μM) showed no effect (P > 0.05) on the PI3K/AKT pathway (Figure 11B). Compared with the blank control group, the phosphorylation levels of PI3K and AKT increased (P < 0.01) in the LPS group. Compared with the LPS group, the phosphorylation levels of PI3K and AKT decreased (P < 0.01) in the LPS–MEL groups (Figure 11C).