key: cord-0012139-e6em3k17
authors: Xiao, Li; Pei, Tianjiao; Huang, Wei; Zhou, Min; Fu, Jing; Tan, Jing; Liu, Tingting; Song, Yong; Yang, Shiyuan
title: MicroRNA22-5p targets ten-eleven translocation and regulates estrogen receptor 2 expression in infertile women with minimal/mild endometriosis during implantation window
date: 2020-07-13
journal: PLoS One
DOI: 10.1371/journal.pone.0234086
sha: 25bbd9b3477b12e9096439b04ece636b64568074
doc_id: 12139
cord_uid: e6em3k17

Based on microRNA (miR) microarray analysis, we previously found that miR22-5p expression is decreased in the mid-luteal endometrium of women with minimal/mild endometriosis. Bioinformatics analysis predicted that miR22-5p targets ten-eleven translocation (TET2) 3′-untranslated region. This study aimed to determine the regulation and roles of miR22-5p in the pathogenesis of minimal/mild endometriosis-associated infertility. MiR22-5p and TET2 expression in the mid-luteal endometrium from women with or without minimal/mild endometriosis was analyzed. After transfection with miR22-5p mimics or inhibitor, TET2 expression was analyzed by quantitative reverse transcription (RT-q) PCR, western blotting and immunohistochemistry. 5-Hydroxymethylcytosine was determined by immunofluorescence and dot blotting. Expression and promoter methylation of estrogen receptor 2 (ESR2) was measured by RT-qPCR and western blotting, and by bisulfite sequencing, respectively. We first established that miR22-5p expression decreased and TET2 expression increased in minimal/mild endometriosis during implantation window. TET2 was found to be a direct target of miR22-5p. MiR22-5p regulated the expression of ESR2, but did not directly affect methylation of its promoter region (–197/+359). Our results suggest that an imbalance in miR22-5p expression in the mid-luteal endometrium may be involved in minimal/mild endometriosis-associated infertility.

Endometriosis is characterized by the implantation and growth of endometrial tissue (glands and stroma) outside the uterine cavity. Women with endometriosis generally experience cyclical chronic pelvic pain, dyspareunia, and infertility, which significantly affect their quality of life. An estimated 30-50% of women with the disease are infertile, and 25-50% of infertile women are diagnosed as having endometriosis [1] . It has been suggested that endometriosisassociated infertility may be due to impaired pelvic anatomy, folliculogenesis, fertilization, and endometriosis according to the revised American Fertility Society classification system (Table 1) . Participants with adenomyosis, leiomyomas, endometrial hyperplasia, genital tumors, acute pelvic inflammatory disease, or receiving hormonal treatment within the previous three months were excluded. Secretory-phase endometrial tissues, assessed based on the timing of the last menstrual period and histological analysis, were used in the study.

ESCs were isolated from eutopic endometrium (n = 3) and normal endometrium (n = 3) as described previously. Isolated ESCs were cultured in DMEM/F12 (1:1) supplemented with 10% fetal bovine serum (FBS) at 37˚C. 293T human embryonic kidney cells were obtained from Sichuan University, Chinese University of Hong Kong Joint Laboratory for Reproductive Medicine, and were maintained in DMEM supplemented with 10% FBS. When cells reached 80% confluency, they were trypsinized and seeded into 6-well plates at 1.0 × 10 5 cells/mL. When the cells reached 30-40% confluency, they were transfected with Hsa-miR22-5p mimics or inhibitor (100 nM, Guangzhou RiboBio, Guangzhou, China), using Lipofectamine 3000 transfection reagent (Invitrogen, Carlsbad, CA), according to the manufacturer's protocol.

After 48-72 h of culture, the cells were harvested and collected for mRNA isolation or protein extraction. All experiments were performed in triplicate.

Total RNA was extracted from endometrial tissues and primary cultured ESCs using TRIzol reagent (Life Technologies, Carlsbad, CA), according to the manufacturer's protocol. RNA quality and purification were analyzed using a NanoVue Plus spectrophotometer (Healthcare Bio-Sciences AB, Uppsala, Sweden). cDNA was synthesized from purified total RNA using a PrimeScript RT reagent kit (TaKaRa Biotechnology, Dalian, China). Primer sequences for TET2, ESR1, ESR2, and GAPDH (Sango Biotech, Shanghai, China) are listed in Table 2 . qPCRs were run using SYBR Green real-time PCR Master Mix (Toyobo, Osaka, Japan) on an Applied Biosystems 7900 Real-time PCR Detection System (ABI, Foster City, CA). The thermal cycles were 95˚C for 20 s followed by 40 cycles of 95˚C for 10 s and 60˚C for 20 s. The specificity of PCR products was confirmed by dissociation curve analysis. GAPDH was used as an endogenous control to normalize target gene expression, and relative expression was calculated using the 2 -ΔΔCt method. For the quantitation of mature miRNAs, miRNA RT-qPCR was conducted using specific primers for miR22-5p and U6 small nuclear RNA (as an internal control) from the Bulge-Loop qRT-PCR Primer Set (Guangzhou RiboBio, Guangzhou, China), according to the manufacturers' protocol. All experiments were repeated three times.

Total protein was extracted using radio immunoprecipitation lysis buffer (P0013B, Beyotime Biotechnology, Shanghai, China) according to the manufacturer's instructions. Protein concentrations were determined using a bicinchoninic acid assay kit (Beyotime Biotechnology). Proteins (30 μg) from each sample were separated by 10% sodium dodecyl sulfate-polyacrylamide gel electrophoresis and were transferred to polyvinylidene fluoride membranes (Millipore, Billerica, MA). The membranes were blocked in 5% defatted milk at room temperature for 1 h. Then, the membranes were incubated with mouse anti-human TET2 (1:400; ab94580, Abcam, Cambridge, UK), polyclonal rabbit anti-human ESR2 (1:400; ab3577, Abcam), polyclonal mouse anti-β-actin (1:30000; bs-2188R, Bioss, Beijing, China) antibodies at 4˚C overnight and then with horseradish peroxidase-conjugated secondary anti-mouse/rabbit antibody at room temperature for 1 h. Proteins bands were visualized using an enhanced chemiluminescence system (Millipore) and were analyzed with ImageJ 2X (National Institutes of Health, Bethesda, MD). Protein levels were normalized to that of β-actin.

The base sequences of TET2 3 0 -UTR fragments were identical to the sequences in the NCBI public bioinformation resource (www.ncbi.nlm.nih.gov/gene/54790). MiR22-5p targets were predicted using TargetScan (http://www.targetscan.org) and microRNA.org (http://microrna. org). Three potential miR22-5p target sites were identified in the 3 0 -UTR of the TET2 mRNA sequence. Reporter genes were constructed by PCR amplification, gel purification, and restriction digest of the TET2 3 0 -UTR. Three wild-type (WT) TET2 3 0 -UTR fragments each containing one of the predicted miR22-5p-binding sites were cloned into the pmiR-RB-REPORT vector (Promega, Fitchburg, WI). The constructed reporter plasmids were designated TET2 3 0 -UTR WT1, TET2 3 0 -UTR WT2, and TET2 3 0 -UTR WT3. The differential expressed TET2 3'-UTR WT1, mutation of TET2 3'-UTR WT1 (TET2 3'-UTR M1) was also designated. 293T cells were transfected with the reporter plasmids and 50 nM of miR22-5p mimic or miRNA negative control (Guangzhou RiboBio, Guangzhou, China). After 48 h, the cells were harvested and luciferase activity was measured using a dual-luciferase reporter assay system (Promega) according to the manufacturer's protocol. All transfections and assays were performed three times, with six technical replicates.

Endometrial cells (25 × 10 3 ) were seeded on glass coverslips in 24-well plates. After treatment, the cells were fixed in 4% paraformaldehyde in 1× PBS for 15 min, washed in PBS, and treated with 0.2% Triton X-100 in PBS for 15 min. Permeabilized cells were denatured with 2 N HCl for 15 min and neutralized with 100 mM Tris-HCl (pH 8.5) for 10 min. Proteins were blocked in 1% BSA in PBS for 30 min and then, the cells were incubated with rabbit anti-human 5-hmc antibody (1:100) and mouse anti-human TET2 antibody (1:200) at room temperature for 2 h, followed by Alexa Fluor 488-labeled anti-mouse antibody (Life Technologies). After washing, the cells were counterstained with 4 0 ,6-diamidino-2-phenylindole.

Genomic DNA was extracted from primary cells using a DNeasy Blood & Tissue Kit (Qiagen) according to the manufacturer's protocol. DNA samples were diluted with 2 N NaOH and 10 

miR22-5p targets TET2 and regulates ESR2 in minimal/mild endometriosis mM Tris Cl (pH 8.5) and blotted onto a nitrocellulose membrane. After baking at 80˚C for 30 min and blocking in 5% nonfat milk at room temperature for 1 h, the membrane was incubated with a polyclonal rabbit anti-human 5-hmC antibody (Active Motif 39769, 1:10,000) at 4˚C overnight. 5-hmC was visualized using chemiluminescence. The membranes were stained with methylene blue to assess equal DNA loading.

Tissue was embedded in paraffin, cut into 5-μm sections, and mounted onto gelatin-coated slides. Sections were dried at 37˚C overnight, deparaffinized in xylene, and rehydrated through a graded ethanol series. The slides were immersed in citrate antigen retrieval buffer (pH 6) at 120˚C for 10 min to retrieve the epitopes, incubated with 3% H 2 O 2 for 10 min to block endogenous peroxidase activity after cooling, blocked with 10% normal goat serum for 30 min, and incubated with the primary antibody (TET2 1:200, 5-hmc 1:200) at 4˚C overnight. Biotinylated secondary antibody and streptavidin-peroxidase conjugate were applied according to the manufacturer's instructions (Beijing Zhongshan Biotech, Beijing, China). Immunoreactivity was visualized with diaminobenzidine, and the sections were counterstained with hematoxylin and mounted. Isotype controls were performed with matched concentrations of mouse IgG for TET2 and rabbit IgG for 5-hmC.

Genomic DNA was extracted from miR22-5p inhibitor-and control-transfected primary ESCs (n = 3) from infertile women without endometriosis using the DNeasy Tissue Kit (Qiagen) and was used for bisulfite modification and sequencing analysis (Sangon Biotech, Shanghai, China). Three microliters of bisulfite-modified DNA was PCR-amplified a reaction volume of 50 μl, using the following primers for ESR2: forward: 5 0 -ATTATTTTTGTGGGTGGATTAG GAG-3 0 , and reverse: 5 0 -AACCCCTTCTTCCTTTTAAAAACC-3 0 . Thermal cycles were as follows: 98˚C for 4 min, 20 cycles of denaturation at 94˚C for 45 s, annealing at 66˚C for 45 s, and elongation at 72˚C for 1 min, and 20 cycles of denaturation at 94˚C for 45 s, annealing at 56˚C for 45 s, and elongation at 72˚C for 1 min, and finally, 72˚C for 8 min. PCR products (166 bp) were gel-purified and cloned into the pUC18-T vector (Sangon Biotech). Following transformation, ten clones with the correct insert were randomly picked for each PCR product and were sequenced using an Applied Biosystems 3730XL instrument.

Statistical analysis was performed using SPSS version 18.0 (IBM Corp., USA). All data were expressed as the mean ± SD. Means of two groups were compared using Student's t-test. P < 0.05 was considered statistically significant (two-tailed).

In our previous microarray-based miRNA profiling analysis of mid-luteal endometrium from women with minimal and mild endometriosis, we observed a marked downregulation of miR22-5p [15] . To confirm these findings in this study, we subjected 13 endometrial tissues of mild/minimal endometriosis and 11 normal control tissues to RT-qPCR. MiR22-5p expression was significantly lower in eutopic endometrium of minimal/mild endometriosis than in normal tissues (Fig 1A) . Next, we investigated the biological significance of miR22-5p downregulation in the regulation of target TET2 mRNAs. Compared to endometrium from women without endometriosis, TET2 expression was significantly higher in endometrium from women with minimal/mild endometriosis during the secretory phase (Fig 1B) . TET2 protein levels were significantly higher in endometrium from women with minimal/mild endometriosis than in normal endometrium as indicated by western blot results (Fig 1C) . Immunohistochemistry revealed that TET2 was strongly expressed in both the nucleus and the cytoplasm of epithelial and stromal cells of eutopic endometrium of endometriosis, whereas normal endometrium exhibited weak to moderate expression (Fig 1D) . The above results suggested a correlation between miR22-5p and TET2 in minimal/mild endometriosis. The DNA pyrimidine nitrogen base 5-hmC was strongly expressed in both the nucleus and the cytoplasm of epithelial and stromal cells of eutopic and normal endometrium (Fig 1D) .

We examined the impact of miR22-5p on TET2 expression by transfecting primary ESCs with miR22-5p mimics and inhibitor. Successful miR22-5p mimic and inhibitor transfection was validated by a significant increase (0.85 ± 0.15 vs. 5189.65 ± 3062.38; P < 0.001; Fig 2A) and decrease (0.98 ± 0.22 vs. 0.17 ± 0.09; P < 0.001; Fig 2A) , respectively, in miR22-5p in ESCs. Upon miR22-5p mimic transfection, we observed significant decreases in the TET2 mRNA (1.03 ± 0.12 vs. 0.51 ± 0.24, P < 0.001, Fig 2B) and protein (1.05 ± 0.20 vs. 0.12 ± 0.04, P = 0.001, Fig 2C and 2E ) levels. Accordingly, following transfection with miR22-5p inhibitor, we observed significant increases in the TET2 mRNA (1.07 ± 0.17 vs. 1.52 ± 0.28, P < 0.001, Fig 2B) and protein (1.53 ± 0.14. vs. 1.02 ± 0.19, P = 0.02, Fig 2D and 2E ) levels. Next, we investigated 5-hmC expression in genomic DNA of ESCs following transfection with miR22-5p mimics and inhibitor by dot blot assays (Fig 2F) . Treatment with the miR22-5p mimics and inhibitor decreased and increased global 5-hmC, respectively. Consistent with the western blotting and DNA methylation dot blot assay results, immunofluorescence revealed that the expression of TET2 and 5-hmC was decreased in miR22-5p mimics-treated cells, whereas they were overexpressed in miR22-5p inhibitor-treated cells (Fig 3) .

We used a luciferase reporter assay to determine whether TET2 regulation was mediated by direct binding of miR22-5p to its 3 0 -UTR (Fig 4A) . 293T cells cotransfected with a reporter plasmid and miR22-5p mimics showed significantly decreased luciferase activity as compared to cells transfected with the reporter plasmid alone only for the TET2 3 0 -UTR WT1 construct, among the three wild-type constructs evaluated (Fig 4B) . Direct interaction of miR22-5p with TET2 was confirmed by using a luciferase reporter harboring a point mutation (Fig 4C) .

To investigate the impact of miR22-5p on ESR2 expression, we assessed primary ESCs following transfection with miR22-5p mimics or its inhibitor. ESR2 mRNA expression was significantly downregulated after transfection with miR22-5p mimics (1.11 ± 0.30 vs. 0.42 ± 0.35 ,   Fig 1. MiR22-5p, TET2 , and 5-hmC expression in endometrium of minimal/mild endometriosis and normal endometrium. (A) RT-qPCR analysis of miR22-5p and (B) TET2 expression in endometrium of minimal/mild endometriosis (n = 13) and normal endometrium (n = 11). miRNA expression was normalized to U6 snRNA expression, and mRNA expression was normalized to GAPDH expression. (C) Western blot analysis of TET2 expression in mild endometriosis (n = 6) and in normal endometrium (n = 5), normalized to GAPDH expression. (D) Representative Immunohistochemistry images showing TET2 and 5-hmC in the cytoplasmic and nuclear regions of stromal and epithelial cells in endometrium of mild endometriosis and normal endometrium (n = 3). Black arrows indicate positive staining. Scale bars, 200 μm. Data represent the mean ± SD and were analyzed by Student's t-test. Fig 5A) , and significantly upregulated after treatment with the inhibitor (0.84 ± 0.20 vs. 1.83 ± 0.41, P < 0.001, Fig 5A) . There was no difference in ESR1 expression following either treatment. Accordingly, the ESR1/ESR2 mRNA ratio was significantly increased after transfection of miRNA22-5p mimics (1.07 ± 0.33 vs. 6.18 ± 0.33, P = 0.019, Fig 5A) or inhibitor (1.142 ± 0.48 vs. 0.68 ± 0.29, P < 0.001, Fig 5A) . ESR2 protein expression was significantly decreased in cells treated with miRNA22-5p mimics (0.87 ± 0.11 vs. 0.43 ± 0.15, P < 0.001, Fig 5B) and increased in cells treated with inhibitor (0.82 ± 0.31 vs. 1.47 ± 0.21, P < 0.001, Fig 5B) , as demonstrated by western blot analysis.

To investigate the role of miR22-5p in DNA methylation further, we assessed the transfected ESCs by bisulfite sequencing. We identified and approximately 550-bp classic CpG island (-197/+359) within the ESR2 promoter and the downstream untranslated exon 0N region. The CpG methylation status after treatments is shown in Fig 6A. The methylation status within this region after transfected with miRNA 22-5p inhibitor or controls was very low and it was not statistically significant ( Fig 6B) .

Endometriosis is an estrogen-dependent chronic inflammatory disease that contributes to cyclical chronic pain and infertility in reproductive women. Recent research has focused on microRNAs because of their roles in regulating epigenetic changes involved in the pathophysiology of infertility due to endometriosis. Previously, utilizing microRNA array analysis, we identified miR22-5p as one of 12 downregulated miRNAs in eutopic mid-luteal endometrium of minimal/mild endometriosis [15] . In the present study, we validated that miR22-5p expression was decreased in eutopic endometrium of minimal/mild endometrium during the midluteal phase. Utilizing a primary ESC model, we found that miR22-5p expression was inversely related to TET2 and 5-hmC expression. MiR22-5p regulated ESR2 expression, but did not directly affect ESR2 promoter methylation. These results support the hypothesis that miRNAs, and in casu, miR22-5p, contributes to the pathophysiology of endometriosis and may be a useful therapeutic target. Women with minimal/mild endometriosis are significantly less likely to achieve pregnancy than those with tubal factor infertility [20] . Endometriosis likely is the most common cause of endometrial receptivity defects, especially in cases of minimal/mild endometriosis, in which the loss of fertility cannot be explained by mechanical reasons [21] . How the endometrium in women with minimal/mild endometriosis is resistant to embryo implantation remains unknown. Maciejak et al. reported upregulation of miR22-5p in the plasma and serum following acute myocardial infarction as a novel diagnostic biomarker [22] . A direct relationship between miR22-5p and TET2 expression has been demonstrated in K562 cells, and in AML cells, low TET2 expression is related to proliferation [23] . However, it has been widely reported that miR-22 negatively regulates TET2 expression and that its overexpression closely phenocopies many of the characteristics observed upon TET2 inactivation both in vitro and in vivo [24] . MiR-22 contributes to the inactivation of TET2 and other TET family members in 

miR22-5p targets TET2 and regulates ESR2 in minimal/mild endometriosis tumorigenesis, and represents a tumorigenic pathway in addition to the more familiar TET family mutations and deletions [24, 25] . These studies indicated that the regulatory relationships between TET2 and miR-22 or miR22-5p are worth investigating in other tissues. Based on a comprehensive analysis of minimal/mild endometriosis patients, we found that TET2 is upregulated in the endometrium during implantation window, and is directly affected by the miR22-5p level.

A subset of DNA hypomethylated canyons is maintained by the cooperative action of TET proteins, in particular, TET1 and TET2 [26] . Aberrant expression of epigenetic alterations in endometriosis include genomic DNA methylation of the gene encoding progesterone receptor-β [27] , HOXA10 [28] , ESR2 [13] , which are candidate genes responsible for the development of progesterone resistance and implantation failure. The ESR2 mRNA level was significantly increased in endometriotic ESCs when compared to normal ESCs. A hypomethylated (-197/+359) promoter region of ESR2 in endometriotic cells was previously considered the primary mechanism responsible for the differential ESR2 expression in endometriotic and normal endometrium [13] . We investigated whether increased TET2 expression due to decreased miR22-5p expression affected ESR2 expression, and we found that ESCs transfected with miR22-5p mimics demonstrated significantly attenuated ESR2 expression. Bioinformatics and genetic analyses revealed no potential miR22-5p target sites in the 3 0 -UTR of the ESR2 mRNA sequence. Indeed, it is speculated that miR22-5p may regulate ESR2 promoter methylation by directly targeting TET2. Bisulfite sequencing of this promoter region (-197/+359) showed that there was no significant difference in the methylation status after transfection with miR22-5p inhibitor. Methylation tended to be lower in miR22-5p inhibitor-transfected cells than in control cells, but the promoter was extremely hypomethylated in both cases, which was inconsistent with a previous study [13] . In Xue's study, eutopic endometrium was not compared between subjects with endometriosis and disease-free subjects, and the menstrual cycles of the study subjects were unknown [13] , whereas we utilized mid-luteal endometrium of infertile women with minimal/mild endometriosis in the embryo implantation phase. DNA methylation profiles of human endometrium differ in different phases of the cycle [29, 30] , which could explain the opposing findings in our and other studies. Overall, our findings suggested that miR22-5p directly dysregulates TET2, which modified the 5-hmC level and 

miR22-5p targets TET2 and regulates ESR2 in minimal/mild endometriosis altered ESR2, but not ESR1 expression in ESCs. This also contributed to an increase in the ESR1/ESR2 mRNA ratio. ESR2 is suggested to modulate ESR1 activity; thus, a change in the relative expression levels of ESR2 to ESR1 suggests a differential regulatory response in estrogen signaling [13] . PR expression in the secretory phase of the menstrual cycle is regulated through ESR1 [31] . Therefore, altered miR22-5p expression in the endometrium may lead to dysregulation of the progesterone response and consequently, implantation-related infertility in women with endometriosis.

To our knowledge, this is the first study to demonstrate downregulation of miR22-5p in eutopic endometrium of women with endometriosis during the secretory phase. Further, we showed that TET2 upregulation during implantation window in human endometrium was directly regulated by miR22-5p. MiR22-5p, which has not been thoroughly studied in endometriosis to date, directly dysregulated the expression of TET2, which is a key marker for DNA hydroxymethylation.

There are some limitations of our study. The first is that we found that ESR2 was also upregulated by miR22-5p, but it was not through the regulation of promoter region methylation of ESR2; hence, the regulatory mechanisms are needed to be further studied. In addition, some studies have revealed the functions of miR22-5p in other diseases [32, 33] . However, this study only focused on that miR22-5p dysregulates directly the expression of TET2 in the eutopic endometrium of endometriosis without the exploration of specific functions of miR22-5p. The role of miR22-5p in modulating the function of the eutopic ESCs and endometrial receptivity in endometriosis also requires exploration in the following study.

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We thank Dr. Shanti Gurung from The Ritchie Centre, Hudson Institute of Medical Research for language modification.