All samples were collected from the Department of Gynecology of The Second Affiliated Hospital of Kunming Medical University from July 2019 to January 2022. EMs patients (n = 24) with were confirmed by laparoscopy and histopathological examination. A total of 23 eutopic endometrium (EU) and 24 paired ectopic endometrium (EC) were collected from patients with EMs. 18 normal endometrium (NE) specimens were collected from healthy women who were hysteroscopically proven to be free of EM. All study women had normal menstrual cycles and had not received hormone therapy for the 3 months prior to surgery. Specimens for RNA and protein extraction were immediately stored in liquid nitrogen, the rest were used for histological examination. The study was conducted in accordance with the Declaration of Helsinki (as revised in 2013) and approved by the Ethics Committee of the Second Affiliated Hospital of Kunming Medical University (PJ-2021–110). All patients signed informed consent.

Human Endometrial Stromal Cells (HESCs) were isolated from the ectopic endometrium of women with endometriosis according to the method of Sung et al.[11]. Briefly, hESCs were isolated and maintained in monolayer cultures. HESCs were isolated and maintained in monolayer cultures. Minced endometrial tissue was washed, minced, and digested with collagenase and trypsin. After removing cellular debris, filter through a 38 µm sterile sieve to isolate stromal cells. Cells were plated in 6-well plates and assayed for cell purity by immunofluorescence.

HESCs were seeded on 6-well culture plates and cultured in DMEM/F12 medium containing 20% fetal bovine serum (Gibco, Carlsbad, USA), 100 μg/mL glutamine, 100 U/mL penicillin, and 100 μg/mL streptomycin (Sigma-Aldrich, St. Louis, MO, USA). The passage when cells reach 80% confluency.

Cell viability was determined using the MTT assay (St. Louis, MO, USA). Briefly, hESCs were seeded into 24-well plates at a density of 2 × 104 cells/mL for 24 h. 50 μL MTT solution (5 mg/mL prepared in phosphate buffered saline) was added to each well and incubated at 37 °C for 4 h. Next, removed the solution and added DMSO to the plates. The absorbance at 570 nm was measured using a plate reader.

Total protein was extracted from tissue and hESC cells using RIPA Lysis Buffer (Invitrogen; USA), and the total protein concentrations were determined by using a BCA Protein Assay kit (Beyotime, China). Then, after boiling and denaturation, the extracted protein was separated by SDS-PAGE gel electrophoresis and transferred onto PVDF membranes. After that, the membranes were blocked with 5% Bovine Serum Albumin (BSA) for 1 h. After that, the membrane was incubated with primary antibodies (DNMT3B, Twist, and GAPDH [Abcam, USA]) at 4 °C overnight. After incubation, the membranes were washed three times with PBS and incubated with secondary antibodies at room temperature for 1 h. Then, the bands were visualized using an enhanced chemiluminescence kit (Bio-Rad Laboratories, Hercules, CA, USA).

The total RNA of tissues and hESCs cells was isolated using the TRIzol reagent (Takara Kyoto, Japan), and the isolated total RNA was reverse transcribed using a cDNA Reverse Transcription Kit (Takara, Kyoto, Japan). Next, Real-time quantitative PCR amplifications were performed using SYBR® Premix Ex Taq™ (Takara, Kyoto, Japan). The relative abundance of MEG3 or miR-21–5p was determined by normalization to the level of GAPDH and U6, and analyzed using the 2−ΔΔCt method. The primers were listed below: MEG3 forward: 5′-CTGCCCATCTACACCTCACG-3′, and reverse: 5′-ATCCTTTGCCATCCTGGTCC-3′; miR-21–5p forward: 5′-GCGCGTAGCTTATCAGACTGATG-3′, and reverse: 5′-CTGAAGTCGCCATGCAGATA-3′; U6 forward: 5′-ATGGACTATCATATGCTTACCGTA-3′, and reverse: 5′-GCTTCACGAATTTGCGTGTCATCCTTGC-3′. GAPDH forward: 5′-CAGGAGGCATTGCTGATGAT-3′, and reverse: 5′-GAAGGCTGGGGCTCATTT-3′.

Cell invasion measurements were conducted using a Transwell chamber coated with Matrigel (Corning, NY, USA). Treated hESC cells were cultured in the upper chamber of a Transwell plate for 12 h, and cells were washed 3 times with PBS. Next, 700 μL of medium containing 10% FBS was added to the lower chamber, and the Transwell plate was incubated in a 5% CO2 atmosphere at 37 °C for 48 h. After 48 h, the cells on the lower side were fixed in cold 3.8% formaldehyde and stained with 0.1% crystal violet. Finally, invaded cells were counted under the microscope (Olympus, Tokyo, Japan) and five randomly selected visual fields were randomly chosen to count.

Genomic DNA was extracted from the tissues with the genomic DNA extraction kit (Qiagen, Dusseldorf, Germany). Next, the DNA was treated with sodium bisulfite. The methylated and unmethylated Twist were amplified using the following primers: Methylated: 5′-AAGGGCGAGAGAGTAGGTC-3′ (forward), 5′-TCCTAACCGCGATAACAAC-3′ (reverse); the unmethylated: 5′-AGAAGGGTGAGAGAGTAGGTT-3′ (forward), 5′-TCCTAACCACAATAACAACCC-3′ (reverse). The PCR-amplified products were separated in a 2% agarose gel and visualized.

The paraffin sections were placed in a constant temperature oven at 65 °C, deparaffinized, hydrated, permeabilized, rinsed with 0.01 moL/L PBS (Tangier, China) solution, antigen retrieval, rinsed again with 0.01 moL/L PBS solution, blocked with 3% hydrogen peroxide, protect from light and incubate at room temperature for 30 min. Next, Sections were incubated with primary antibodies (Abcam, USA) for 1 h at room temperature. After washing with PBS 3 times, add a secondary antibody and incubated for 1 h. After washing with PBS 3 times, DAB was added to develop the color and observed under the microscope for 3‒10 min, the positive color was brown.

Statistical analyses were performed by GraphPad Prism 7.0 software; p < 0.05 or p < 0.01 were considered statistically significant.

MEG3 has been confirmed to be involved in the occurrence of EMs[12]. To unfold the mechanism of MEG3 in EMs, the authors analyzed the expression of MEG3, miR-21–5p, and DNMT3B in clinical EMs tissues. The results showed that MEG3 and DNMT3B expressed exceptionally low in the ectopic endometrial group in EMs compared to the normal control group and the eutopic endometrial group in the EMs (Fig. 1A and Fig. 1C‒1D). In contrast, miR-21–5p exhibited the opposite findings, miR-21–5p expressed exceptionally high in the ectopic endometrial group in EMs compared to the normal control group and the eutopic endometrial group in the EMs (Fig. 1B). These results suggested that MEG3, miR-21–5p and DNMT3B might be involved in the development of endometriosis.

Fig. 1.

The expression of MEG3, miR-21–5p and DNMT3B in EMs tissues. The level of MEG3, miR-21–5p in tissues were measured by RT-qPCR (A‒B). The expression of DNMT3B was measured by IHC and western blotting (C‒D). Asterisks indicate statistical significance (*p < 0.05, **p < 0.01).

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Endometrial Stromal Cells (ESCs) continue to grow and spread in patients with EMs[13]. The authors isolated primary Endometrial Stromal Cells (hESCs) from ectopic endometrial and determine the success of separation by detecting the expression of vimentin (Fig. 2A). To clarify the effects of MEG3 on hESCs, the authors overexpression of MEG3 in hESCs and tested the efficiency of MEG3 overexpressing vector (Fig. 2B). Next, the authors examined the effect of MEG3 on cell viability and proliferation of hESCs. The cell growth of hESCs cells transfected with OE-MEG3 showed significantly lower compared with the OE-NC-transfected hESCs and untransfected hESCs (Fig. 2C). The effect of MEG3 on cell invasion was determined using transwell assays, transwell assays revealed that overexpression of MEG3 inhibited the invasion of hESCs cells in vitro As shown in Fig. 2D.

Fig. 2.

Overexpression of MEG3 inhibits hESCs cells proliferation, invasion. The expression of Vimentin in hESCs cells were measured by IF (the scale bar is 100 μm) (A). The level of MEG3 in hESCs cells were measured by RT-qPCR (B). The hESCs cells viability were measured by the MTT assay and microscope (200 ×) (C). The invasiveness of hESCs cells was evaluated by transwell invasion assay (the scale bar is 100 μm) (D). Asterisks indicate statistical significance (*p < 0.05, **p < 0.01).

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To explore the potential downstream gene involved in the regulation of MEG3 on proliferation, and invasion in hESCs, the potential miRNA target genes of MEG3 were predicted using the miRCode databases. Bioinformatics showed that MEG3 has a sequence complementary to the region of miR-21–5p (Fig. 3A). The authors further performed a dual-luciferase reporter assay. The results showed that overexpression of miR-21–5p effectively inhibits the luciferase activity of Wild-Type (WT) MEG3 but not Mutant (MUT). In parallel, Overexpression of MEG3 downregulated the expression of miR-21–5p and also confirmed this interaction (Fig. 3B and C). On the other hand, through the Starbase database, the authors found that miR-21–5p and DNMT3B have a region-complementary sequence AAGCU, similar to MEG3 and miR-21–5p (Fig. 3D). Meanwhile, the dual-luciferase reporter assay and western blotting resulted further confirmed this interaction (Fig. 3E and F). Collectively, these finds revealed that MEG3 functions as a ceRNA to modulate the expression of miRAN-21–5p/DNMT3B.

Fig. 3.

MEG3 regulates the expression of miR-21–5p and DNMT3B. The inferred binding regions between MEG3 and miR-21–5p, miR-21–5p and DNMT3B (A and D). Targeting relationship between MEG3 and miR-21–5p, miR-21–5p and DNMT3B determined by dual luciferase reporter genes (B and E). The level of miR-21–5p in cells were measured by RT-qPCR (C). The expression of DNMT3B was measured by western blotting (F). Asterisks indicate statistical significance (*p < 0.05, **p < 0.01).

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The authors evaluated the effect of MEG3 on the proliferation and invasion of hESCs cells via miR-21–5p/DNMT3B by transfecting miR-21–5p mimics in hESCs cells. The authors first investigated the expression of DNMT3B in OE-MEG3 and miR-21–5p mimics transfected and untransfected hESCs cells. The results showed that OE-MEG3 upregulated the expression of DNMT3B, in contrast, miR-21–5p mimics downregulated the expression of DNMT3B increased by OE-MEG3 (Fig. 4A). In addition, hESCs cells viability and proliferation showed that the miR-21–5p mimics downregulated the cells viability increased by OE-MEG3. Meanwhile, miR-21–5p mimics promoted cell invasion inhibited by OE-MEG3 (Fig. 4B and C). These finds revealed that MEG3/miR-21–5p/DNMT3B regulates hESCs cell proliferation and invasion.

Fig. 4.

MEG3 inhibits hESCs cells proliferation, invasion via miR-21–5p/DNMT3B. The expression of DNMT3B was measured by western blotting (A). The hESCs cells viability were measured by the MTT assay and microscope (200 ×) (C). The invasiveness of hESCs cells was evaluated by transwell invasion assay (the scale bar is 100 μm) (D). Asterisks indicate statistical significance (*p < 0.05, **p < 0.01).

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The twist is abnormally hypomethylated (highly expressed) in the development of EMs[14]. Thus, the authors further examined the methylation level of Twist in EMs and its relationship with the methyltransferase DNMT3B. IHC and Western blotting results showed that Twist expressed exceptionally high in the ectopic endometrial group in EMs compared to the normal control group and the eutopic endometrial group in the EMs (Fig. 5A and B). At the same time, Twist is hypomethylated in the ectopic endometrial group of EMs (U: Unmethylation, M: Methylation, Fig. 5C). Next, the authors investigated the regulation of Twist expression by DNMT3B by transfecting LV-DNMT3B in hESCs cells. The results showed DNMT3B expression is upregulated during LV-DNMT3B transfection, Meanwhile, the expression of Twist was downregulated (Fig. 5D and E). These results suggested that DNMT3B promotes Twist methylation and downregulates Twist expression

Fig. 5.

DNMT3B inhibits Twist methylation. The expression of DNMT3B was measured by IHC (A). The expression of DNMT3B and Twist were measured by western blotting (B, D and E). Methylation of Twist detected by MSP (C). Asterisks indicate statistical significance; m, Marker; U, Unmethylated, M, Methylated (*p < 0.05, **p < 0.01).

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