Sox9 transcriptionally regulates Wnt signaling in intestinal epithelial stem cells in hypomethylated crypts in the diabetic state
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Distinctive structures called crypts harbor intestinal epithelial stem cells (IESCs) which generate progenitor and terminally differentiated cells in the intestinal epithelium. Mammalian IESCs and their daughter cells require the participation of DNA methylation and the transcription factor Sox9 for proliferation and differentiation. However, the association between Sox9 and DNA methylation in this process remains elusive.
The DNA methylation of small intestinal epithelial crypts in db/db mice was detected via combining methylated DNA immunoprecipitation with microarray hybridization. DNA methylation of Sox9 promoter in crypts and IESCs was validated using bisulfite sequence analysis. The target sequence of the transcription factor Sox9 in IESCs was investigated via chromatin immunoprecipitation (ChIP) combined with deep sequencing (ChIP-seq).
Increased Sox9 expression is accompanied by the loss of methylation in its promoter in IESCs. Sox9 targets the enhancers of the Wnt signaling pathway-related genes. Sox9 predominantly acts as a transcriptional activator at proximal enhancers of Wnt4, Tab2, Sox4, and Fzd8, but also functions as a potential transcriptional inhibitor at a distant enhancer of Cdk1. Lack of Sox9 transcriptional activation in specific repressors of the Wnt signaling pathway leads to the loss of intrinsic inhibitory action and ultimately produces overactivation of this pathway in db/db mice.
Our study sheds light on the connections among DNA methylation, transcription factor modulation, and Wnt signaling in IESCs in the diabetic state. Hypomethylation in the Sox9 promoter is correlated to increased Sox9 expression in db/db IESCs. Although there is increased expression of Sox9 in db/db IESCs, the loss of Sox9 transcriptional activation in specific repressors of the Wnt signaling pathway might result in abnormalities in this pathway.
KeywordsSox9 Wnt signaling Intestinal epithelium stem cells DNA methylation Diabetes mellitus
Chromatin immunoprecipitation combined with deep sequencing
Differential methylation enrichment peak
DNA methyltransferase 1
Fluorescence-activated cell sorting
Intestinal epithelium stem cell
Leucine-rich repeat-containing G protein-coupled receptor 5
Magnetic bead-activated cell sorting
Quantitative real-time polymerase chain reaction
Sry (sex determining region Y)-box 9
Transcription start site
The small intestinal epithelium has a distinctive organization, with intestinal epithelial stem cells (IESCs) harbored at the base of crypts. IESCs produce progenitors and differentiated cells. The length of the crypt-villus unit is significantly increased in 4- to 10-week-old diabetic mice, with increased proliferation labeling indexes in the small intestine . Furthermore, the proportion of cells positive for leucine-rich repeat-containing G protein-coupled receptor 5 (Lgr5), which represent bona fide stem cells limited to the IESCs , is markedly increased in the crypts of diabetic mice . In general, the signaling most closely connected to the abnormal proliferation and differentiation of IESCs is Wnt signaling . Enhanced intestinal epithelial cell proliferation in diabetes mellitus (DM) has been demonstrated not only in experimental diabetic mice but also in recent clinical trials [4, 5]. Excessive activation of Wnt signaling in stem cells increases intestinal epithelial cell proliferation and even promotes formation of adenomas .
A controversial transcription factor (TF), Sry (sex determining region Y)-box 9 (Sox9), is correlated with the Wnt signaling pathway and plays a significant role in intestinal crypts. Traditionally, Sox9 is considered to function as a negative transcriptional regulator of Wnt signaling [7, 8]. However, recent studies using Sox9 chromatin immunoprecipitation (ChIP) combined with deep sequencing (ChIP-seq) analysis have reported that Sox9 can activate canonical Wnt/β-catenin signaling in hepatocellular carcinoma  and prostate cancer . In another Sox9 knockout mouse model, Wnt target genes appear to be unaltered in telogen hair follicles . To date, it remains unclear how Sox9 modulates IESCs via Wnt signaling pathways.
A DNA methyltransferase 1 (Dnmt1) deletion mouse model has been reported to show significantly expanded crypts, increased Sox9 expression, and reduced DNA methylation in the crypts of the small intestine . Dnmt1-mediated developmentally programmed epigenetic mechanisms are involved in the regulation of IESC function [13, 14]. Moreover, DNA methylation is required for the modulation of stem cell proliferation and differentiation in the small intestine. In the present study, we identify morphological and physiological changes in db/db mice, a well-established animal model of type 2 DM  that is similar to Dnmt1-deletion mice. More importantly, increased Sox9 expression is accompanied by hypomethylation of promoters in IESCs. Based on ChIP-seq analysis in IESCs, among Sox9 binding sites related to Wnt signaling, Sox9 targets the enhancers of genes related to the Wnt signaling pathway. It is not only predominantly acting as a transcriptional activator at proximal enhancers but also as a potential transcriptional inhibitor at a distant enhancer. Lack of Sox9 transcriptional activation in specific repressors of the Wnt signaling pathway eventually produces abnormal signaling in this pathway.
BKS.Cg-Dock7m +/+ Lepr db /JNju (db/db) male mice were obtained from the Model Animal Research Center of Nanjing University (Nanjing, Jiangsu, China) and were maintained under a 12-h light/12-h dark cycle in a specific pathogen-free animal facility. The experiments were conducted using 16-week-old male homozygous mice, which were maintained for 8 weeks with hyperglycemia (random blood glucose level ≥16.7 mmol/l) prior to euthanasia. Identical genetic background BKS heterozygote db/+ mice (random blood glucose level <11.1 mmol/l) were used as the controls. All experiments with mice were approved by the Animal Care Committee of Sun Yat-Sen University (Permit Number: 201412000091).
Isolation of intestinal crypts and villus fractions
The upper half of the small intestine (from the duodenal end to the middle of the intestine) was dissected out from the mice and sliced longitudinally to expose the crypts and villi, in ice-cold phosphate-buffered saline (PBS) (with Mg2+/Ca2+). The intestine was subsequently incubated in ice-cold dissociation reagent #1 (47 ml DPBS without Mg2+/Ca2+; 3 ml 0.5 M EDTA (Sigma, St. Louis, MO, USA); 75 μl 1 M DTT (Sigma)) in a 15-ml tube and embedded in ice for 20 min, followed by the addition of dissociation reagent #2 (47 ml DPBS, 3 ml 0.5 M EDTA) and incubation at 37 °C for 10 min. Following incubation, each tube containing intestine was shaken for 30 s to release the epithelium from the basement membrane. The remaining intestinal tissue was removed, and cells shed into dissociation reagent #2 were collected and labeled as fraction 1. The solution containing dissociation reagent #2 was filtered through a 70-μm nylon cell strainer (BD Falcon, Corning, New York, NY, USA). The tissue retained on the filter, which consisted of villi, was stored in PBS (Mg2+/Ca2+) on ice (fraction 2). The incubation, shaking, and straining steps were repeated until eight fractions were collected. Fractions 3–6 comprised pure villus tissue identified as differentiated cells, and fractions 7 and 8 isolated as the flow-through from the cell strainer comprised pure crypt tissue. Pure crypt tissues were confirmed by traditional microscope.
Promoter methylation microarray
Crypts were collected from six independent mice, with the control db/+ mice designated C1, C2, and C3, and the diabetic db/db mice designated D1, D2, and D3. Immunoprecipitation of methylated DNA was performed using Biomag™ magnetic beads (Bangs Laboratories, IN, USA) coupled with a mouse monoclonal antibody against 5-methylcytidine. The total input and immunoprecipitated DNA were labeled with Cy3- and Cy5-labeled random 9-mers, respectively, and hybridized to ArrayStar Mouse RefSeq Promoter Arrays, which consisted of a multiplex slide with four identical arrays per slide; each array contained 22,327 well-characterized RefSeq promoter regions, from approximately −1300 bp to +500 bp of transcription start site (TSS), covered by 180,000 probes. Scanning was performed using an Agilent Scanner G2505C (Agilent Technologies, Santa Clara, CA, USA).
At least one of the two groups has a median (log2 MeDIP/Input) ≥0.3 and M’ >0.
At least half of the probes in a peak may have a coefficient of variability (CV) ≤0.8 in both groups.
The dataset is available in the GEO database under the accession number GSE87044.
Collection of IESCs
The crypts obtained as described above were resuspended in 10 ml Hank’s balanced salt solution (HBSS) containing 8 mg dispase (Gibco, Carlsbad, CA, USA). The cell solution was incubated for 10 min at 37 °C, with vigorous shaking every 2 min, followed by the addition of 10% fetal bovine serum (FBS) and 50 μl 10 mg/ml DNase (10 mg/ml; Roche, Basel, Switzerland). The solution was sequentially passed through 70- and 40-μm filters to collect the cell suspension. Single-cell suspension was confirmed under microscope. The primary antibodies Lgr5 (Abcam, Cambridge, MA, USA) and CD45-FITC (BD Pharmingen, San Jose, CA, USA) and the secondary antibody goat anti-rabbit IgG-PE (BD Pharmingen) were used for fluorescence-activated cell sorting (FACS). Lgr5hiCD45neg cells, identified as IESCs, were sorted using a FACSVerse (BD Bioscience, San Jose, CA, USA) machine. All data analyses were performed using FlowJo V10 software (Treestar, USA).
Due to limited cell quantities when using FACS, single-cell suspensions were also sorted by magnetic bead-activated cell sorting (MACS; BD IMag™ Streptavidin Particles Plus-DM; BD Biosciences). Cells were resuspended in cell-staining buffer at a concentration of 2 × 107 cells per ml; then, the biotinylated antibody Lgr5-Biotin (20 μl per 2 × 107 cells; Biorbyt, Cambridge, UK) was added, followed by incubation on ice for 30 min. The labeled cells were subsequently washed with buffer, and 50 μl magnetic nanoparticles were added and incubated at 6–12 °C for 30 min. Finally, the labeled cells were washed with buffer three times using a magnetic device. The cells collected, predominantly IESCs, were used for Western blot analysis.
The IESCs sorted by FACS or MACS were validated for cell purity by quantitative real-time polymerase chain reaction (qRT-PCR).
RNA extraction and quantitative real-time RT-PCR
Total RNA from samples was extracted using TRIzol® Reagent (Life Technologies, Carlsbad, CA, USA), and the concentration was calculated from the absorbance at 260 nm as determined using an ND-2000 instrument (NanoDrop Technologies, Wilmington, DE, USA), followed by reverse transcription with PrimeScript™ RT Master Mix (TaKaRa Bio, Kusatsu, Shiga, Japan). qRT-PCR was performed on a CFX Connect™ real-time PCR detection system (Bio-Rad, Hercules, CA, USA) using SYBR® Premix Ex Taq™ (TaKaRa Bio, Kusatsu, Shiga, Japan). The primers are shown in Additional file 1 (Table S1). Data were analyzed using the △△Ct method with β-actin as an internal control. The qRT-PCR experiments were performed in sextuplicate using independent samples.
Western blot analysis
Isolated crypts or IESC samples were incubated in RIPA buffer (Thermo Scientific, Carlsbad, CA, USA). The protein samples were separated by 12% SDS-PAGE and transferred to PVDF membranes. The membranes were probed overnight at 4 °C with the following primary antibodies: rabbit anti-mouse Dnmt1 antibody (1:2000; Abcam, Cambridge, MA, UK), rabbit anti-mouse Dnmt3a antibody (1:1000; Abcam), rabbit anti-mouse Sox9 antibody (1:1500; Abcam), and rabbit anti-mouse β-actin antibody (1:2000; Cell Signaling Technology, Danvers, MA, USA). The data were analyzed using relative intensity with β-actin as the internal control. The Western blot experiments were performed in three repetitions using independent samples.
Cell culture and transfection
The cell lines HCT116, Caco-2, DLD-1, and HT-29 were purchased from the Institute of Biochemistry and Cell Biology of the Chinese Academy of Sciences (Shanghai, China). Cells were cultured in RPMI 1640 medium or DMEM (Gibco, Carlsbad, CA, USA) supplemented with 10% FBS, 100 U/ml penicillin, and 100 mg/ml streptomycin (Gibco) in humidified air at 37 °C with 5% CO2. For SOX9 overexpression and knockdown, SOX9-pcDNA (SOX9 expression plasmid) and SOX9 small interfering RNA (siRNA) were respectively transfected using Lipofectamine® 3000 Transfection Reagent (Invitrogen, Carlsbad, CA, USA). For qRT-PCR and Western blot analysis, cells were collected at 48 h and 72 h after transfection, respectively. The qRT-PCR and Western blot experiments were performed in quadruplicate using independent samples.
Luciferase reporter assay
The human embryonic kidney (HEK) 293FT cell was used to transfect in 96-well plates. For each well, 300 ng of the pCMV-SOX9-3FLAG-SV40-Neomycin construct or the negative control pCMV-3FLAG-SV40-Neomycin backbone were transfected in combination with 50 ng of firefly luciferase reporter constructs and 50 ng of the pDC315-3FLAG-SV40-renilla luc vector (Gene Chem, Shanghai, China) using as the renilla luciferase reference. Luciferase activity was measured after 48 h using the Dual-Luciferase® Reporter Assay System (Promega, Madison, WI, USA) according to the manufacturer’s protocol.
DNA extraction and bisulfite sequence analysis
Genomic DNA was extracted from crypts or IESCs using a Quick-DNA™ Universal Kit (Zymo Research, Tustin, CA, USA). DNA concentration was calculated from the absorbance at 260 nm with an ND-2000 instrument (NanoDrop Technologies, Wilmington, DE, USA). Purified genomic DNA was subjected to bisulfite conversion using an EZ DNA Methylation-Gold™ Kit (Zymo Research, Tustin, CA, USA). Converted DNA was PCR amplified using primer sets designed to target the methylated peaks of Dnmt3b and Sox9. A two-step amplification method was performed using a TaKaRa EpiTaq™ HS DNA polymerase system (TaKaRa Bio, Kusatsu, Shiga, Japan) under the following conditions: 98 °C for 2 min and 40 cycles of 98 °C for 10 s, 55 °C for 30 s, and 72 °C for 30 s. PCR products were subcloned into bacteria using a pMD™19 T-Vector Cloning Kit (TaKaRa Bio, Kusatsu, Shiga, Japan), and 10 colonies per group were sequenced using a BigDye Terminator v3.1 Cycle Sequencing kit and a 3730xl DNA Analyzer (Applied Biosystems, Carlsbad, CA, USA). The PCR primer sets are described in Additional file 1 (Table S2).
Independent immunoprecipitations were performed on FACS-sorted populations. Due to the limited numbers of IESCs in individual mice, a pooled cohort of four db/db mice was collected as the db/db group, and cells from five db/+ mice were collected as the control group. Immunoprecipitated DNA was obtained using an EZ-Magna ChIP™ HiSens kit (Millipore, Temecula, CA, USA). Chromatin was sonicated into 200–500 bp fragments using the BioRuptor UCD-200 (Diagenode, Seraing, Belgium). Immunoprecipitation was performed using 4 μg rabbit polyclonal anti-mouse Sox9 antibody (Abcam, Cambridge, MA, UK) and 200 μl chromatin for each sample. Paired-end sequencing was performed on an Illumina HiSeq 2000 (50-bp reads). ChIP-seq reads were aligned to the mouse genome (mm9, build 37), and peaks were called with Model-based analysis of ChIP-Seq . The Integrative Genomics Viewer was used to visualize signal tracks. The MEME software suite was applied to the sequences under the Sox9 peaks (200 bp around summit) to identify enriched motifs. The dataset is available in the GEO database under the accession number GSE87583.
To establish the significance between two groups, comparisons were performed using unpaired two-tailed Student’s t tests in Prism 5 (GraphPad software). For all statistical tests, the 0.05 level of confidence was considered statistically significant.
Decreased DNA methylation of promoter regions in crypts was correlated to the diabetic state
We subdivided promoters into three classes based on the CpG ratio, GC content, and length of the CpG-rich region: high CpG-density promoters (HCPs; promoters that contained a 500 bp interval within −0.7 kb to +0.2 kb with a [G + C]-fraction ≥0.55 and a CpG observed to expected ratio (O/E) ≥0.6), low CpG-density promoters (LCPs; promoters that contained less than 500 bp interval with CpG O/E ≥0.4), and intermediate CpG-density promoters (ICPs; those between HCPs and LCPs). Of the 3146 methylated promoter regions, many regions were HCPs. Only slight differences in the percentages of HCPs or LCPs were identified between the two groups (Fig. 1d).
Taken together, these findings demonstrated decreased DNA methylation of promoter regions in crypts of db/db mice; however, the percentages of methylated HCPs, LCPs, or ICPs were not markedly different between the two groups.
Expression of DNA methyltransferases in the intestinal epithelium was correlated with methylation pattern and diabetic state
In crypts, significantly lower Dnmt1 expression was observed in the db/db mice compared with the db/+ mice, whereas no difference in Dnmt3a was observed between the two groups. Moreover, a markedly reduced expression of Dnmt1 was identified in terminally differentiated cells (Fig. 2a and b). Previous studies have reported that Dnmt1 was restricted to the crypts of intestinal epithelium [12, 17]. Similarly, we found that Dnmt1 was limited to the crypt regions in both groups (Fig. 2f), while Dnmt3a exhibited increased expression in crypts but was also expressed in other positions in the epithelium (Fig. 2g).
IESCs serve as the source of all types of enterocytes and perform more prominent proliferation and differentiation activity. Thus, we were interested in the changes in DNA methyltransferases in IESCs. We isolated cells expressing high levels of Lgr5, the genuine stem cells of the small intestine , using FACS and MACS (Additional file 3: Figure S2a). Lgr5hiCD45neg cells were identified as IESCs. Confirmation of cell purity was performed by qRT-PCR for the stem cell-specific markers Lgr5, CD24, Olfm4, and Ascl2, the enterocyte marker Lct, the endothelial cell marker CD31, and the lymphocyte marker CD45 (Additional file 3: Figure S2b).
Interestingly, Dnmt1 exhibited distinctly higher expression in Lgr5hiCD45neg IESCs than in the crypts as a whole. Moreover, significantly decreased expression of Dnmt1 was identified in db/db mice compared with the db/+ mice; however, there was still no difference in the level of Dnmt3a between the two groups (Fig. 2a and b). These findings suggested that decreased Dnmt1 in db/db mice was correlated with the degree to which DNA methylation was reduced. Furthermore, alterations in the DNA methylation pattern and Dnmt1 expression in crypts may be mostly inherited from IESCs. In fact, reduction of DNA methylation by acute deletion of Dnmt1 in the intestinal epithelium has been reported to cause crypt expansion in vivo .
Hypomethylation of Wnt signaling was correlated to its overactivation in diabetic db/db crypts and IESCs
To further investigate Wnt signaling, we focused on the base of crypts, the IESCs. They were bona fide stem cells that showed fast cycling and were responsive to Wnt signaling . We performed qRT-PCR in IESCs for the DMEP-related genes related to Wnt signaling. Surprisingly, most of the genes, including Pou5f1, Egr1, Grem1, Strn, Stk11, Sox9, and Rac1, exhibited increased expression in IESCs compared with crypts (Fig. 3c). One of the most obvious differentially expressed genes between crypts and IESCs was Sox9. Increased Sox9 expression was detected in the db/db crypts, more remarkably in the db/db IESCs (Fig. 3b–d). In fact, Sox9 expression was mainly restrained to the crypts (Fig. 3e) , and cells showing low levels of Sox9 were considered IESCs, which were capable of forming cryptoid structures under in vitro culture conditions [23, 24].
Together, these observations indicated that hypomethylation of gene promoters correlated to ectopic Wnt signaling in db/db crypts, especially in IESCs. Several TFs, such as Sox9, were also under the regulation of hypomethylation and might cooperate in the control of this aberrant signaling.
Hypomethylation in the Sox9 promoter was correlated to its overexpression in IESCs
In the microarray results, loss of methylation in Sox9 promoters was detected in the three db/db samples (Fig. 4b). Validation by bisulfite sequence analysis revealed that, on average, 50.8% of CpG sites were identified as methylated in the db/db mice intestinal crypts compared with 68.5% in the db/+ (P < 0.05; Fig. 4c). However, in IESCs, the methylation status was reduced in both groups, with only 5% in the db/db mice and 25% in the db/+ mice (P < 0.01; Fig. 4d). Combined with the gene expression of Sox9 (Fig. 3b–d), we speculated that hypomethylation in the Sox9 promoter might contribute to the altered gene expression in diabetic db/db crypts. Moreover, the degree of methylation of the Sox9 promoter was decreased in both groups in IESCs compared with crypts and was markedly decreased in db/db IESCs, which in part contributed to the increased Sox9 level.
Sox9 acted as a transcriptional regulator in Wnt signaling
Sox9 functioned as a TF and regulated gene expression by targeting gene regulatory sequences [8, 10, 11, 27]. We therefore investigated the mechanism by which Sox9 regulated gene expression in db/db IESCs. Thus, using FACS-sorted IESCs, we conducted Sox9 ChIP-seq to investigate the interaction of this TF and the genomic DNA sequences in vivo. Quality assessments of chromatin preparation and raw data are provided in Additional file 4 (Figure S3).
To further comprehensively investigate Sox9 binding sites related to the Wnt signaling pathway, we defined a promoter (±2 kb of TSS) and an “extended enhancer” (−100 kb upstream of and +5 kb downstream from the gene body) with reference to previous studies [11, 27]. Subsequently, among the Sox9 binding sites, we identified a list of Wnt signaling pathway-related genes (Fig. 5c). The mRNA level with respect to these genes was detected by qRT-PCR in IESCs and crypts. Moreover, overexpression and knockdown of SOX9 were performed through an overexpression plasmid in the human colorectal carcinoma cell lines Caco-2 and DLD-1 and through siRNA in HCT116 and HT-29 cells, respectively (Fig. 5e and f).
Among the Wnt signaling pathway-related genes, the mRNA levels of Vangl1 (vang-like 1), Rora (RAR-related orphan receptor alpha), and Sfrp2 (secreted frizzled-related protein 2) were extremely low in IESCs and crypts (Additional file 5: Figure S4a and b). Thus, we focused on the following eight genes: Wnt4 (wingless-type MMTV integration site family, member 4), Tab2 (TGF-beta activated kinase 1/MAP3K7 binding protein 2), Rac1, Sox9, Fzd8 (frizzled class receptor 8), Ctbp1 (C-terminal binding protein-1), Sox4 (sex determining region Y box 4), and Cdk1 (cyclin-dependent kinase 1). In a previous study, a Sox9 far-upstream enhancer located at −70 kb of the TSS was identified; Sox9 dimers directly bound to multiple sites of this sequence and thereby cooperatively activated the enhancer . Surprisingly, in the db/db mice, we also discovered a strong peak signal at the third exon of Sox9, which was located at +3011 of the TSS (Fig. 5d).
In the db/+ mice, three enriched peak signals of Sox9 binding sites were located at the enhancers of Wnt4, Tab2, and Rac1 (Fig. 5c). Wnt4 was abundantly expressed in β cells in an obese mouse model and acted as an inhibitor of canonical Wnt signaling, as well as an activator of noncanonical Wnt signaling . In our study, the expression of Wnt4 was decreased in the db/db mice, and it was correlated with a lack of the Sox9 binding signal. However, in the db/+ mice, a peak signal was located at −16,676 bp upstream of TSS (Fig. 5g and h). From the SOX9 regulation experiments in cultured cells emerged a corresponding positive correlation of mRNA level between SOX9 and WNT4 (Fig. 5i). In addition to WNT4, TAB2 is a putative TAK1 interacting protein that plays an inhibitory role in canonical Wnt/β-catenin signaling . Decreased Tab2 expression was observed in db/db IESCs, and Sox9 targeted the enhancer of Tab2 in the db/+ mice at −17,872 bp of the TSS (Fig. 5j and k). The cell experiments also confirmed a positive transcriptional regulation of SOX9 on TAB2 (Fig. 5l). Another Sox9 binding site in the db/+ was related to Rac1, locating at −37,247 bp upstream of the TSS (Fig. 5m). Although peak signal was also observed in the db/db mice, it was eliminated as a ghost signal by the algorithm. Indeed, abundant expression of Rac1 was identified in crypts and IESCs, and significantly increased Rac1 expression was observed in the db/db mice (Fig. 5n). However, the cell experiments showed no relationship between Rac1 expression and the Sox9 TF action (Fig. 5o).
In short, these findings indicated that, in normal controls, Sox9 targeted the enhancers of Wnt4 and Tab2, positively regulating gene expression. However, in the db/db mice, the expression of Wnt4 and Tab2, both repressors of Wnt signaling, was decreased, and both lacked the Sox9 binding signal. Thus, the lack of Sox9 transcriptional regulation in the repressors of the Wnt signaling pathway may result in abnormalities in this pathway for reducing adequate repressors.
In the db/db mice, the strongest enriched peak signal of Sox9 binding sites related to Wnt signaling was located at the enhancer of Fzd8, a receptor component in the Wnt pathway, located at −20,391 bp upstream of its TSS (Fig. 5p). There was no significant difference in the expression of Fzd8 in crypts between the two groups; however, Fzd8 expression in IESCs was significantly increased in db/db mice (Fig. 5q). Moreover, the mRNA level of FZD8 was dramatically reduced when SOX9 expression was decreased by siRNA in HCT116 and HT-29 cells. Similarly, the expression of FZD8 was increased in Caco-2 and DLD-1 cells, accompanied by overexpression of SOX9 (Fig. 5r). These observations suggested that expression of Fzd8 was raised by Sox9 transcriptional activation in the db/db mice.
In addition, a faint Sox9 binding peak signal in the db/db mice was associated with another family member of Sox TFs, Sox4 (Additional file 5: Figure S4c). Sox4 protein stabilized β-catenin and thereby boosted canonical Wnt signaling . We identified increased expression of Sox4 in db/db crypts and IESCs (Additional file 5: Figure S4a and b). Furthermore, the cell experiments also suggested a positive correlation between the mRNA levels of SOX4 and SOX9 (Additional file 5: Figure S4d). This suggested that Sox9 bound to the enhancer of Sox4 may act as a transcriptional activator. Another weak Sox9 binding peak signal in the db/db mice was related to CtBP1, a Wnt signaling repressor (Additional file 5: Figure S4e). However, in the cell experiments, there was no regulatory effect (Additional file 5: Figure S4f). Finally, a distant Sox9 binding peak signal was identified at −95,988 bp upstream of the Cdk1 TSS (Additional file 5: Figure S4g). Since autoregulation of Sox9 by a far-upstream (−70 kb) enhancer was previously demonstrated in somatic tissues , distant enhancers may be possible. Intriguingly, we discovered a negative correlation for mRNA levels between SOX9 and CDK1 in cultured cells. Decreased SOX9 expression markedly increased the CDK1 level, whereas overexpression of SOX9 limited the expression of CDK1 (Additional file 5: Figure S4h). This suggested that SOX9 inhibited the transcription of CDK1. These findings were in contrast to the previously described results showing the function of Sox9 as a transcriptional activator.
Taken together, these observations suggested that Sox9 targeted the enhancers of specific Wnt signaling-related genes. Sox9 was not only predominantly acting as a transcriptional activator at proximal enhancers (Tab2, Fzd8, Sox4, and Wnt4) but was also acting as a potential transcriptional inhibitor at a distant enhancer (Cdk1). The lack of Sox9 transcriptional activation of specific repressors of the Wnt signaling pathway contributed to the formation of abnormal activity of this pathway in db/db mice.
We identified hypomethylated promoters and overactivated Wnt signaling in intestinal crypts in diabetic db/db mice. Moreover, the expression of Dnmt1 was decreased in db/db crypts, especially in IESCs. Consequently, hypomethylation that contributes to aberrant proliferation and differentiation in the diabetic intestinal epithelium may exist in IESCs. The hypomethylation pattern of promoters in crypts may derive from the methylation status of IESCs. Although dynamic DNA methylation during IESC differentiation has been recognized, the degree of this dynamic process has not yet reached consensus [12, 14, 31, 32]. Nevertheless, there is no doubt that the epigenetic characteristics of IESCs can be at least partially passed on to their daughter cells. Low methylation of Wnt-related genes is observed in IESCs and progenitor cells in Dnmt1-deficient mice . Moreover, we detected overactivated Wnt signaling in diabetic db/db mice not only in crypts but also in IESCs, particularly significantly in the latter. Further evidence is required to demonstrate the methylation connection between IESCs and their daughter cells in the intestinal epithelium. We consider that reduced DNA methylation in promoters driving gene expression participates in the aberrant proliferation and differentiation in intestinal epithelium due to overactivated Wnt signaling.
Of the differentially methylated genes related to Wnt signaling, we focused on Sox9. Sox9 is known as a Wnt-responsive IESC gene marker [22, 23, 24]. Furthermore, Sox9 functions as a TF, regulating gene expression. Nevertheless, the behavior of Sox9 in Wnt signaling remains controversial. On the one hand, in HEK 293 cells, Sox9 inhibits the activation of β-catenin-dependent promoters and stimulates the degradation of β-catenin. Similarly, in Xenopus embryos, Sox9 inhibits the β-catenin-mediated induction of the secondary axis . In chondrocyte differentiation, the Sox9 N-terminus promotes β-catenin degradation, whereas the C-terminus inhibits β-catenin transcriptional activity without affecting its stability. Nuclear localization of Sox9 enhances β-catenin phosphorylation and its subsequent degradation . In cancer cells, Sox9 and Krüppel-like factor 4 (KLF4) interact with β-catenin and reduce its binding to TCF4  and showed anti-oncogenic activity by inhibiting the activity of the Wnt/β-catenin signaling pathway . These reports suggest that Sox9 serves as a negative transcriptional regulator of Wnt signaling. On the other hand, recent ChIP studies have demonstrated a direct correlation between Sox9 and Wnt signaling. In hepatocellular carcinoma, Sox9 activates the canonical Wnt pathway through direct binding with Fzd7 . Analyses of prostate cancer on xenografts and clinical samples both reveal that SOX9 positively regulates multiple WNT pathway genes, including frizzled (FZD), lipoprotein receptor-related protein (LRP) family members, and the downstream β-catenin effector TCF4 . Furthermore, in colon carcinoma cells, an active β-catenin-TCF4 complex is required for physiological targeting of SOX9 . One study suggests a bimodal role for Sox9 in the intestinal epithelium, in which a low level of Sox9 supports proliferative capacity through Wnt/β-catenin signaling, whereas a high level of Sox9 suppresses this process . In a Sox9 knockout mouse model, Wnt target genes appear to be unaltered in telogen hair follicles .
Most previous reports concerned with Sox9 functions on Wnt signaling are focused on cancer cells or embryonic cells. Notably, these are rapidly cycling cells, some of which are outside the normal regulation of the organism. Moreover, embryonic cells are also involved in developmental mechanisms. Thus, it is difficult to use them to represent the condition of adult stem cells. IESCs are bona fide stem cells that are fast cycling and responsive to Wnt signaling , which seems to be similar to cancer cells. The intestinal epithelial cells are renewed every 4–5 days. However, these rapid physiological processes of proliferation and differentiation related to Wnt signaling are under intricate control by the organism, requiring multiple intrinsic inhibitors of this signaling. In our research, we specifically consider the influence of methylation on Sox9 expression in IESCs. In crypts, the db/db mice show a lower degree of methylation of Sox9, which is accompanied by increased gene expression. In IESCs, promoter methylation of Sox9 in both groups is significantly reduced, especially in diabetic db/db IESCs. The loss of promoter methylation of Sox9 might induce its prominently increased expression in diabetic db/db IESCs. Thus, we consider that the differential expression of Sox9 in diabetic db/db IESCs results in part from the loss of methylation in its promoter. Sox9 is predominately expressed in crypts, and cells that express “low” levels of Sox9 in crypts are considered bona fide IESCs [23, 24, 25]. IESCs represent a small percentage of the total crypt cells; however, these cells present prominent proliferation and differentiation in response to Wnt signaling.
Combining ChIP-seq on Sox9 in IESCs with overexpression and knockdown of SOX9 in cultured cells, we demonstrate that, among Sox9 binding sites related to Wnt signaling, Sox9 targets the enhancers of Wnt signaling pathway-related genes in IESCs, acting not only as a transcriptional activator at proximal enhancers, such as the enhancers of Wnt4, Tab2, Sox4, and Fzd8, but also as a potential transcriptional inhibitor at a distant enhancer, such as the enhancer of Cdk1. More significantly, lack of Sox9 transcriptional activation of specific repressors of Wnt signaling pathway in the db/db mice contributes to the development of abnormal activity of this pathway. Therefore, the overactivated Wnt signaling pathway in db/db IESCs might not result directly from Sox9 transcriptional activation of Wnt signaling; rather, it might be a result of losing the intrinsic inhibitory action of repressors.
Notably, in addition to Sox9, other regulators of Wnt signaling may exist in IESCs. Our current study provides a unique research method called the net-to-net method on an abnormal state. An organism is a complex and integrated organic system that can be considered as similar to a multinetwork. Alteration of each point may impact one or more networks. We performed our study using a high-throughput methylation microarray of whole genomic promoters (starting from one network) and subsequently determined the key regulator (here, Sox9) that more or less affects the entire network. Next, we investigated the network changed by the key regulator by using another round of high-throughput sequencing (to another network). We provide a distinctive research perspective on the connections of DNA methylation, TF modulation, and Wnt signaling in IESCs in an animal model of type 2 DM, a common disease with a high risk of transformation to cancer .
Our study sheds light on the connections among DNA methylation, TF modulation, and Wnt signaling in IESCs in the diabetic state. Hypomethylation in the Sox9 promoter is correlated with increased Sox9 gene expression in db/db IESCs. Although db/db IESCs showed increased expression of Sox9, the loss of Sox9 transcriptional activation in specific repressors of the Wnt signaling pathway might result in abnormal activity of this pathway.
We are grateful to Zhao-Fei Dong for technical assistance on ChIP-seq analysis. We thank the members of KangChen Bio-tech for assistance with methylation analysis.
This work was supported by grants from the Key Laboratory of Malignant Tumor Molecular Mechanism and Translational Medicine of Guangzhou Bureau of Science and Information Technology (Grant 163); the Key Laboratory of Malignant Tumor Gene Regulation and Target Therapy of Guangdong Higher Education Institutes (Grant KLB09001); and the National Natural Science Foundation of China (No. 81270442 and No. 81370475).
Availability of data and materials
The datasets generated and/or analyzed during the current study are available in the GEO database, accession numbers: GSE87044 and GSE87583.
CZH, TY, and QKC designed and conceptualized the experiment. CZH, JHX, WZ, SYW, and DC performed the experiments and analyzed the data. ZSX, JYL, and TFW validated and visualized the data. CZH and JHX wrote the original draft. TY and QKC reviewed and edited the final draft. All authors read and approved the final manuscript.
The authors declare that they have no competing interests.
Consent for publication
Ethics approval and consent to participate
All experiments with mice were approved by the Animal Care Committee of Sun Yat-Sen University (Permit Number: 201412000091).
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