Abstract
During decidualization in rodents, uterine stroma undergoes extensive reprograming into distinct cells, forming the discrete regions defined as the primary decidual zone (PDZ), the secondary decidual zone (SDZ) and the layer of undifferentiated stromal cells respectively. Here we show that uterine deletion of Men1, a member of the histone H3K4 methyltransferase complex, disrupts the terminal differentiation of stroma, resulting in chaotic decidualization and pregnancy failure. Genome-wide epigenetic profile reveals that Men1 binding in chromatin recapitulates H3K4me3 distribution. Further transcriptomic investigation demonstrates that Men1 directly regulates the expression of PTX3, an extra-cellular trap for FGF2 in decidual cells. Decreased Ptx3 upon Men1 ablation leads to aberrant activation of ERK1/2 in the SDZ due to the unrestrained FGF2 signal emanated from undifferentiated stromal cells, which blunt BMP2 induction and decidualization. In brief, our study provides genetic and molecular mechanisms for epigenetic rewiring mediated decidual regionalization by Men1 and sheds new light on pregnancy maintenance.
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Introduction
Successful pregnancy requires rapid remodeling of the endometrium in a process termed decidualization, which requires the blastocyst attachment as a trigger and occurs in a region-specific manner in mice1. At the initiation of decidualization, stromal cells surrounding the implanted blastocyst undergo proliferation and postmitotic differentiation extensively, forming the primary decidual zone (PDZ) between day 5 (day 1 = the day of positive of vaginal plug) and day 6 of pregnancy2. Subsequently, stromal cells adjacent to the PDZ continue to proliferate and differentiate into decidual cells to form the secondary decidual zone (SDZ) at the antimesometrial (AM) pole by day 8. A large portion of decidual cells experience polyploidization, characterized by large mono or bi-nucleated cells that undergo repeated DNA replication without cytokinesis3. In addition, a thin layer of undifferentiated stromal cells lines between the myometrium and the SDZ4. It is believed that the regionalized decidual structure is not only important for the supply of nutrition to the developing embryo but also acts as a barrier against excessive invasion of trophoblast cells1,5. While only small incrementation has been made about the underlying mechanism directing programmed stromal cells differentiation in recent decades.
Several studies have demonstrated that a set of central genes in evolutionarily conserved signaling pathways during embryogenesis, such as BMP (bone morphogenetic protein), WNT (wingless-type MMTV integration site family), FGF (fibroblast growth factor) signaling, and HOX (homeobox) genes, possess the potential function in building the regional pattern of decidualization4,6,7. BMP2, an indispensable factor for the differentiation of stromal cells into decidual cells, is intensively expressed in PDZ and SDZ6,8. The expression of WNT ligand Wnt4, which is also critical for uterine stromal cell differentiation, largely overlapped with Bmp24. Meanwhile, Sfrp4, a WNT antagonist, is observed in the layer of undecidualized stromal cells outside the SDZ4. In addition to Sfrp4, Fgf2, a member of FGF family, also exhibits a similar expression pattern6. The fine-tuned interplay of these regionalization determinants synergistically or antagonistically promotes tissue homeostasis during decidualization. However, how these genes are coordinated to specify the allocation of decidual cells remains largely unknown.
Menin, encoded by the Men1, is a multifunctional scaffold protein participating in a variety of cellular functions, whose deficiency contributes to embryonic lethality at E11.5-E13.5 with defects in multiple organs9,10. Menin regulates target genes expression in a cell type-specific manner, including Hox genes, Cdkn1b, and Cdkn2c, Esr1 and p35, by interacting with chromatin-modifying enzymes, in particular, the histone methyltransferase (HMT) MLL1/2 that catalyze histone 3 lysine 4 trimethylation (H3K4me3)11,12,13,14,15. Regarding that early pregnancy is a precisely regulated process, whether the target genes of Menin-MLL complex and how Menin and its interplay with H3K4me3 modification participate in embryo implantation and decidualization remain elusive.
In the current study, we utilize a combination of genetic, biochemical, and pharmacological approaches to investigate the role of Men1 in peri-implantation uteri and reveal that Men1 ablation disrupts the appropriated differentiation of decidual stromal cells, resulting in unordered regionalization of decidualization and compromised pregnancy success. The reduction of Bmp2 caused by aberrantly activated FGF2-ERK1/2 signaling pathway deranges the adequate development of the SDZ due to disorganized genomic H3K4me3 modification in the absence of Men1. PTX3, an extracellular protein trapping FGF2, is identified as a Menin directly regulated downstream gene and provides insightful information for the orchestration of decidualization and pregnancy maintenance in curbing the cross-talk between FGF2-ERK1/2 and BMP2.
Results
Men1 is expressed in the peri-implantation mouse uterus in a spatiotemporal manner
Highly heterogeneous uterine endometrium is comprised of different cell types that undergo tremendous changes during early pregnancy. To elucidate the physiological significance of Men1 during early pregnancy, we first examined the cell-specific and temporal expression of Men1 in peri-implantation uteri using in situ hybridization. There was weak Men1 expression in the pre-implantation uterus on days 1 and 4. After embryo implantation, Men1 transcript was moderately upregulated in proliferating stromal cells surrounding the blastocyst on day 5. Accompanied by the initiation of decidualization, stromal cells underlying the implantation chamber exit mitosis and differentiate into epithelioid cells to form the PDZ. The transcript of Men1 became undetectable in the PDZ but was intensely expressed in proliferating stromal cells outside the PDZ on day 6, which was further supported by the co-staining of Ki67 and Menin (Fig. 1a and Supplementary Fig. 1a, b). After the SDZ was established by day 8, Men1 expression was restricted in the mesometrial (M) pole (Fig. 1a). These observations indicated that Men1 expression was tightly correlated with the progress of decidualization. Consistent with its mRNA expression pattern, Menin protein was widely expressed in the uterus during decidualization and located mainly in nucleus (Fig. 1b). It was interesting to note that Menin protein possessed wider expression than its transcript which is perhaps due to the discrepant stability between mRNA and protein (Fig. 1b). Account for the well overlapping between Men1 mRNA and proliferating cells, it was conceivable to speculate that the newly transcribed Men1 was probably for Men1 translation for daughter cells during mitosis. The spatiotemporal expression pattern of Men1 indicates that it could be a considerable regulator in peri-implantation events.
Mice with uterine deletion of Men1 show severe subfertility
To explore the functional role of uterine Men1 in pregnancy, we generated mice with uterine deletion of Men1(Men1d/d) by crossing Men1 floxed mice (Men1f/f) with PR-Cre mice (PgrCre/+)10,16. These mice show efficient deletion of Men1 in the pregnant uterus at both mRNA and protein levels (Fig. 1c–e). To interrogate the role of Men1 in female fertility, Men1d/d mice and their littermate controls (Men1f/f) were mated with wild type fertile males. Only 25% plug-positive Men1d/d mice gave birth to offspring and the litter size was significantly lower than those in littermate Men1f/f mice (Fig. 1f, g). These results demonstrated uterine Men1 was crucial for a successful pregnancy.
Ablation of uterine Men1 causes defective decidualization and miscarriage at mid-gestation
Early pregnancy is a highly programmed dynamic process involving blastocyst attachment, decidualization, and placentation. Defects at any stage will give rise to adverse pregnancy outcomes. To dissect out the defects causing subfertility in Men1d/d mice, we first assessed the early pregnancy events on day 5 with increased vascular permeability at the attachment site17. The number of implantation sites and the embryo spacing were comparable in Men1f/f and Men1d/d mice on day 5 as visualized by intravenous injection of Chicago blue (Fig. 2a, b). The gross morphology and embryo attachment reaction as revealed by H&E staining and COX2 expression, respectively, were also similar between Men1f/f and Men1d/d (Supplementary Fig. 2a and Fig. 2c). Stromal cells surrounding the blastocyst undergo extensive proliferation and differentiation into decidual cells under the initiation of BMP22,8. The semblable proliferation and expression pattern of Bmp2 and BMP antagonist Dan in Men1f/f and Men1d/d implantation sites confirmed that mice with uterine deletion of Men1 had normal initiation of decidualization (Fig. 2d and Supplementary Fig. 1b–e). Moreover, IGFBP5, which provides a favorable environment for blastocyst growth by coupling with IGF118, had a similar subepithelial expression pattern in Men1f/f and Men1d/d implantation sites (Supplementary Fig. 1f).
Since the deficiency of Men1 has no severe defects in the blastocyst attachment reaction and the initiation of decidualization, we next examined the progress of decidualization. The morphology of the decidual bulge and the number of implantation sites were comparable between Men1f/f and Men1d/d mice on day 6 with the termination of stromal cell proliferation in the established PDZ (Fig. 2e, f and Supplementary Fig. 3a). Our results showed that there were comparable expressions of OCT4, Ki67, Dtprp, COX2, Bmp7, β-Catenin, and Wnt4 in day 6 uteri, implying normal embryo development, stromal cell proliferation, PDZ formation19,20,21,22 (Supplementary Fig. 3b–h). We also noticed that the glands distribution was abnormal with increased number in the lateral areas near the M pole in stroma of Men1d/d mice as characterized by FOXA223 from pregnant day 4–6 (Supplementary Fig. 4). Collectively, these results indicated that uterine Men1 was dispensable for blastocyst attachment, implantation, and PDZ formation during early pregnancy.
Following the formation of PDZ, stromal cells adjacent to the PDZ continue to proliferate and differentiate to form SDZ until day 8. The reduced average weight of implantation sites with retarded embryos was emerged in Men1d/d mice on day 8 in comparison to Men1f/f mice (Fig. 2g–i). From day 9–12, more obvious defects appeared at the implantation sites, including abnormal placentation and severe embryo absorption (Fig. 2j–l). These data hinted that the development of SDZ was hindered from day 7–8. In order to further confirm the effect of Men1 deletion in the progress of decidualization, an oil-induced artificial decidualization model24 was applied (Supplementary Fig. 5a). Men1f/f mice uteri exhibited a robust decidual response 96 h after intraluminal oil injection, while the Men1d/d uteri showed a remarkably weakened or disappeared decidual response (Supplementary Fig. 5b, c). Collectively, these results demonstrated that uterine-specific deletion of Men1 disturbed the progression of decidualization and ultimately resulted in embryo resorption and miscarriage at mid-gestation.
Uterine deletion of Men1 leads to inadequate differentiation of decidual cells in the SDZ
The observations of abnormal decidualization on day 8 led us to investigate the cellular defects in Men1d/d uteri. Polyploidization, a hallmark of mature decidual cells in the SDZ, was marked by mono or bi-nucleated cells through endoduplication. Indeed, the ablation of Men1 in uteri resulted in decreased decidual cell polyploidy and smaller nuclear size (Fig. 3a). H3K27me3 was critical epigenetic modification for X chromosome inactivation for dose complementary effect of female somatic cells25. Our results showed that polyploid decidual cells in Men1f/f mice possessed >4 puncta H3K27me3 staining, indicating at least four sets of homologous chromosomes in polyploid decidual cells (Fig. 3b). While the number of polyploid decidual cells with four or more puncta H3K27me3 staining was obviously reduced in Men1d/d mice (Fig. 3b). Consistently, we found aberrantly increased PCNA (DNA replication in S-phase) and BrdU (DNA synthesis in S-phase) in Men1d/d decidual cells on day 8 of pregnancy (Fig. 3b). Further, flow cytometric analysis of DNA content revealed that 2 N cells were significantly increased with a concomitant decrease of >4 N cells in Men1 deletion decidual tissues on day 8 (Fig. 3c, d and Supplementary Fig. 6). In Men1d/d mice, both Dtprp mRNA and protein were significantly reduced on day 8 (Fig. 3e, f), suggesting that the terminal differentiation of decidual cells was impaired. These results indicated Men1 was critical for the progression of polyploidy during decidualization.
On day 8, the expression of COX2 in the presumptive site of placentation was disordered, foreboding impaired placentation in Men1d/d mice (Fig. 3g, h). Accompanied by normal decidualization, abundant uterine natural killer (uNK) cells accumulated at the mesometrial pole on day 826. In contrast to numerous DBA+ uNK cells in Men1f/f mesometrial pole, Men1 null uteri exhibited dramatic decrease of uNK cells (Fig. 3h). Aberrant decidualization tends to give rise to abnormal trophoblast invasion and compromised placentation5. Eccentric expression pattern of trophoblast giant cells marker PL1 in Men1d/d uteri signified shallow trophoblast invasion on day 8 (Fig. 3i). All these observations strongly proved the defective decidualization in the absence of uterine Men1.
The morphological and physiological changes of stromal cells during decidualization are mainly regulated by steroid hormones from ovary1. Progesterone is indispensable for decidualization maintenance through its cognate nuclear receptor progesterone receptor (PR)5. There was no significant difference in circulating levels of E2 and P4 in both groups on day 6 with similar expression of progesterone biosynthetic enzymes cytochrome P450 cholesterol side-chain cleavage enzyme (P450scc) and 3β-hydroxysteroid dehydrogenase (3β-HSD) in the ovary as well as comparable expression PR and its target genes, Hand2 and Hoxa10, in day 6 and day 8 uterus (Supplementary Fig. 7a, b and Supplementary Fig. 8a–f). These data suggested that the defect decidualization was primarily originated from local dysfunction of Men1 in stromal cells.
Procedures for decidualization dysregulated in the absence of uterine Men1
To further excavate the underlying molecular mechanism for the defective terminal differentiation of decidual cells in the SDZ observed in Men1d/d mice, decidual tissues were isolated from Men1f/f and Men1d/d uteri on day 8 and subjected to gene expression profiles analysis using RNA sequencing (RNA-seq). A total of 1669 genes were differentially expressed (RPKM > 0.5, p < 0.05) with 870 downregulated genes (Supplementary Data 1) and 789 up-regulated genes (Supplementary Data 2) in Men1d/d mice in comparison to wild type (Fig. 4a). Decidualization involves a series of biological changes including the proliferation and differentiation of stromal cells, angiogenesis, and immunological adaptation5,22,27. Functional annotation revealed that downregulated genes upon Men1 deletion mainly enriched in the terms of cell proliferation inhibition, fatty acid metabolic process, multicellular organism development, and negative regulation of angiogenesis (Fig. 4b and Supplementary Data 3). In contrast, genes up-regulated in Men1d/d decidual tissues were enriched in categories that were resistant to cell differentiation such as positive regulation of ERK1/2 cascade and categories detrimental to the development of decidua such as apoptotic process and inflammatory response (Fig. 4b and Supplementary Data 4).
The downregulated genes in negative regulation of cell proliferation, including Bmp2, Ptn, Fgf10, and Igf1, possessed specific expression patterns and were important for decidualization6,28,29 (Fig. 4c, d). On the contrary, genes associated with the activation of MAPK activity that promotes cell proliferation (Fgfr1, Pdgfa) were upregulated in Men1d/d uteri (Fig. 4c). Besides, genes expressed in the thin layer of undecidualized stromal cells were increased after Men1 knockouts, such as Sfrp4 and Prlr (Fig. 4c, d).
Increased vascular permeability and angiogenesis are crucial to successful decidualization. Angiopoietins (ANGPT1 and ANGPT2) and their receptor TIE2 directs angiogenesis during decidualization22,27. ANGPT1 induces vessel maturation and maintains vessel leakiness, whereas ANGPT2, acting as a natural antagonist of ANGPT1, induces vessel destabilization required for further sprouting and regression of vessels30. Our RNA-seq data indicated several genes in promoting angiogenesis (Angpt1, Edn1, Ednra) were upregulated, and genes in inducing destabilization of blood vessels and endothelial sprouting (Angpt2, Hif3a, Mmp2) were downregulated due to uterine Men1 deletion (Fig. 4c, e). Furthermore, NK-specific genes (Prf1, Klrg1, Ctsg, Il15r) and several granzyme genes (Gzma, Gzmb, Gzmc, Gzmd, Gzme, Gzmg) were significantly decreased in Men1d/d decidua (Fig. 4c), indicating the maturation of uNK was compromised. Moreover, Corin, functions in promoting trophoblast invasion and spiral artery remodeling31, was decreased substantially in Men1d/d females (Fig. 4c).
Interestingly, loss of Men1 led to decreased Cdkn1b (encoding p27) in both mRNA and protein levels (Fig. 4c, f). Especially, the immunohistochemical analysis indicated that the expression of p27 was higher in polyploid cells (Fig. 4f). Previous studies manifest that increased p27 level in liver cells causes a failure to enter mitosis and thereby induces polyploidy32. Reduced polyploid decidual cells in Men1d/d decidual tissues might be accountable for the reduction of p27. In addition, gene set enrichment analysis (GSEA) analysis showed that cytokinesis-associated genes (Rhoc, Rhob, Dstn)33 were significantly enriched by Men1 loss (Fig. 4g, h and Supplementary Data 5). Consistently, there were more stromal cells undergoing proliferating in Men1 knockout SDZ as evidenced by significant increase of mitotic marker pH3 (Fig. 4i, j). Above all, Men1 loss had a strong negative impact on normal physiological changes in decidualization.
Men1-deficient uteri show diminished BMP responsiveness but enhanced FGF responsiveness
As aforementioned, the uterine with Men1 deletion had an insufficient terminal differentiation of stromal cells in the SDZ. Interestingly, the FGF signaling pathway that positively regulated cell proliferation was significantly enriched among the upregulated genes in Men1d/d uteri. In contrast, the gene set responding to BMP which motivated differentiation of stromal cells was significantly suppressed in Men1d/d uteri (Fig. 5a, b and Supplementary Data 5). During decidualization, the Fgf2 transcript was localized in the undifferentiated stromal cells underneath the myometrium6. FGF2 binds and activates the tyrosine kinase receptor complex FGFR1-FRS2 and recruits the downstream GRB2-SOS1 complex to incite ERK1/2 signaling cascade which is a major pathway controlling cell proliferation34. Fgfr1 and Frs2 but not the ligand Fgf2 were significantly increased by Men1 deletion (Fig. 5b, c). BMP2 is a well-known decidual marker critical for the differentiation of stromal cells during decidualization6,8. The expression of Bmp2 and its target Id1 was substantially lower in Men1d/d mice uteri on day 8 of pregnancy (Fig. 5b, d). BMPs execute their effects by inducing the phosphorylation of SMAD1/5/8 proteins. Accordingly, the protein level of p-SMAD1/5/8 was decreased in Men1d/d decidual cells (Fig. 5e and Supplementary Fig. 9). Interestingly, both the significant elevated expression of Fgfr1 and reduced expression of Bmp2 caused by Men1 deletion mainly occurred in the SDZ (Fig. 5f). We also observed an elevation of phosphorylated ERK1/2 in Men1d/d stromal cells in the SDZ (Fig. 5g). These observations were consistent with enrichment of ERK1/2 cascade and decreased cell differentiation observed in Men1d/d decidual tissues (Fig. 4b, c). Thus, spatiotemporal decidualization regulated by programmed FGF signaling and BMP signaling was disorganized in Men1 deficiency uterine. Indeed, mutually inhibitory effects between FGF and BMP signaling are common modules throughout embryogenesis35. Next, we explored whether there was a cross-talk between BMP2 and FGF2-ERK1/2 signals, and what role Menin played in this communication during the development of the SDZ.
Menin positively regulates the expression of Ptx3 in an H3K4me3-dependent manner
Menin is an indispensable component of MLL1/2 HMT complex that catalyzes H3K4me3 in a locus-specific manner, which is usually associated with transcriptional activation of genes9,36. We speculated that Menin activated gene expression through H3K4me3 during decidualization. Total H3K4me3 protein level was not affected by Men1 ablation as previously reported14,37,38 (Supplementary Fig. 10a). Although deficiency of Men1 does not disrupt global H3K4me3, Menin regulates the H3K4me3 levels across regions proximal to TSSs of a limited number of cell-specific genes38,39. In order to define its relevance to specific gene expression in decidual cells, we performed ChIP-seq for Menin and H3K4me3 in decidual tissues on day 8. Consistent with the published literature, Menin and H3K4me3 is predominantly positioned at gene promoter (Menin peaks: n = 13,347, 76.65% at promoters; H3K4me3 peaks: n = 29,040, 70.62% at promoters) (Fig. 6a). Almost 80% of peaks bound by Menin were also H3K4me3 modified (Supplementary Fig. 10b). Combined with RNA-seq data, we found that Menin and H3K4me3 were significantly enriched at the transcription start site (TSS) of expressed genes (RPKM > 1) (Fig. 6b and Supplementary Fig. 10c). A direct comparison of Menin and H3K4me3 ChIP-seq peaks at TSSs showed a strong positive correlation (R2 = 0.5888291) (Fig. 6c). Specifically, read coverage of H3K4me3 around TSSs was modestly reduced in the absence of Men1 (Fig. 6b, d). These results suggested that Menin is involved in H3K4me3 modification across regions proximal to TSSs during decidualization. We, therefore, focused on the potential function of Menin-dependent H3K4me3 in transcriptional activation of specific genes during decidualization.
Analysis of ChIP-seq data revealed that although Menin-H3K4me3 typical target genes identified in other cell types (e.g. Cdkn1b, Cdkn2c, Esr1, Hoxa cluster, and Meis1) were also bound by Menin in decidual tissue, none of them had H3K4me3 reduction after Men1 deletion at the promoters (Fig. 6e). Correspondingly, except for the decreased expression of Cdkn1b, the mRNA levels of other Menin target genes had no significant difference in the absence of Men1 (Figs. 4c, 6e). There might be an alternative mechanism different from the H3K4me3 dependent mechanism as previously reported participated in the transcriptional regulation of Cdkn1b by Menin13. Researches investigating genome-wide function of Menin yielded cell-specific results in terms of the expression of H3K4me3 dependent target genes15,38,39,40. According to these results, we hypothesized that Men1 regulates the transcription of a subset of decidual-specific target genes through H3K4me3 modification. H3K4me3 peaks at regions proximal to TSSs were classified into two clusters depending on the changes after Men1 deletion (Fig. 6f and Supplementary Fig. 10d). Cluster 1 contains loci where H3K4me3 ChIP-seq signal was decreased following Men1 deletion, representing 6469 associated genes (Fig. 6f). While loci in cluster 2 have no significant change of H3K4me3 levels, representing 5644 associated genes (Supplementary Fig. 10d). To identify the direct Menin-H3K4me3 target genes responsible for the decidualization defects observed in Men1d/d uteri, we intersected the RNA-seq data with genes bound by Menin as well as 6469 genes in cluster 1 and found 2995 potential Menin-H3K4me3 direct target genes. Among the 348 genes that were differentially expressed after Men1 deletion, only 217 genes had significantly reduced mRNA levels (Fig. 6g). We listed the top-ranked downregulated genes that are most likely to be the targets of Menin-H3K4me3 in decidual cells (Fig. 6h, i). We also determined the H3K4me3 accumulation in promoters of Menin target genes (e.g. Sfrp2, Twist2, Snx10, and 378 Adora2b) by ChIP-qPCR assays, and it displayed a reduced H3K4me3 modification in decidual cells upon uterine Men1 deletion (Supplementary Fig. 11a–d). These results suggested that loss of Men1 resulted in reduction of H3K4me3 at regions proximal to TSSs of a very limited number of genes expressed in decidua cells.
In these potential target genes, Ptx3 attracted our attention since the deletion of Ptx3 resulted in compromised decidualization41 (Fig. 6g). Indeed, the peak of H3K4me3 was significantly reduced at the Ptx3 locus, and RNA-seq tracks for Ptx3 were profoundly decreased in Men1d/d uteri following Men1 deletion (Fig. 7a). Men1 loss decreased Ptx3 expression in decidual tissues on day 8 of pregnancy (Fig. 7b). Through Menin ChIP assays using a pair of specific primers targeting the Ptx3 promoter locus, we further confirmed that Ptx3 was a direct target gene of Menin in decidual cells (Fig. 7c). Meanwhile, H3K4me3 occupancy at the Ptx3 promoter locus was dramatically decreased in Men1-knockout stromal cells (Fig. 7d). These results suggest that Menin upregulates Ptx3 expression in an H3K4me3 dependent manner.
Menin inhibits the cross-talk between FGF2-ERK1/2 and BMP2 by regulating the transcription of Ptx3
PTX3 has been shown to bind with selected FGFs, including FGF2 and FGF8b, through its N-terminal domain, and sequester them in the extra-cellular matrix, thus inhibiting their biological effects42. As described above, Men1 loss upregulated FGF response. We found Ptx3 specifically expressed in the SDZ close to the thin layer of undifferentiated stromal cells where Fgf2 located and significantly decreased following Men1 deletion (Fig. 7e). During embryogenesis, FGF2 is considered to be a paracrine factor and is essential for tissue patterning and organogenesis35. Based on these results, we considered that the decrease of Ptx3 caused by Men1 deficiency contributed to excessive ERK1/2 activation induced by paracrine FGF2 produced by the layer of undifferentiated stromal cells. To confirm this conjecture, primary mouse endometrial stromal cells (mESC) isolated from day 4 uterus of pseudopregnancy were cultured with or without recombinant mouse PTX3 in the presence of FGF2. PTX3 treatment for 72 h significantly inhibited the phosphorylation of ERK1/2 induced by FGF2 in mESC compared with cells without PTX3 treatment (Fig. 7f). Consistent with previous studies, the inhibitory effect of PTX3 on FGF2 was conserved during mouse decidualization. Thus, we concluded Menin suppressed the activation of FGF2-ERK1/2 signaling pathway in the SDZ by modulating Ptx3 transcription through epigenetic H3K4me3 modification.
In the preceding results, Men1 loss decreased BMP response program (Fig. 5). Indeed, suppression of BMP signaling by FGF2 sustained undifferentiated proliferation of human ES cells43. Next, we explored whether the reduction of BMP2 was caused by abnormal highly activated FGF2-ERK1/2 signal in the absence of Men1. During in vitro decidualization of mESC induced by E2 and P4, the expression pattern of Menin was almost consistent with that of BMP2 in spite of the slight decrease expression of Menin after 96 h of decidualization (Supplementary Fig. 12a, b). MI-503, a Menin inhibitor, blocks the Menin/MLL interaction and triggers Menin protein degradation via ubiquitin-proteasome pathway44. MI-503 treatment for 48 h reduced the expression of Menin protein without affecting the mRNA level of Men1 during the decidualization of mESC (Supplementary Fig. 12c, d). The expression of Menin target gene Ptx3 was also significantly reduced upon MI-503 treatment (Fig. 7g). However, MI-503 treatment for 72 h did not affect the expression of BMP2 and the activity of ERK1/2 during mESC decidualization (Supplementary Fig. 12e), implying Bmp2 was not a direct target of Menin and consistent with the ChIP data showing no Menin occupying and comparable H3K4me3 modification at Bmp2 promoter upon Men1 knockout (Supplementary Fig. 12f). While in the presence of exogenous FGF2, MI-503 treatment resulted in decreased BMP2 and elevated ERK1/2 phosphorylation (Fig. 7h), highlighting the significance of FGF2 for regulating BMP2 expression and appropriate decidualization. Meanwhile, co-treatment with MEK inhibitor PD0325901 reversed the reduction of BMP2 induced by MI-503 (Fig. 7h). These results demonstrated FGF2 acting as a paracrine factor had an inhibitory effect on BMP2 expression during decidualization. Supplementation of exogenous PTX3 also inhibited excessive activation of ERK1/2 and recovered BMP2 level (Fig. 7h). These results suggested Menin regulated the expression of BMP2 during decidualization by setting PTX3 as a trap for the FGF2-ERK1/2 pathway, thereby ensuring the success of decidualization (Fig. 8a, b).
Discussion
The regulatory machinery of endometrial heterogeneity and decidua regionalization after embryo implantation has disturbed scientists for a long time due to the scarcity of a suitable mouse model. Developmentally associated transcription factors HOXA10, whose expression expanded throughout the PDZ and SDZ, have been reported to play an important role in establishing region-specific decidual tissue during decidualization7,45. While, other potential participants in decidua regionalization remained largely unknown. Here, we demonstrated that uterine Men1, which was spatiotemporally expressed during decidualization, guided the stromal cells towards the fate of terminal differentiation by directing histone modification rewiring, guaranteeing the expansion of the SDZ boundary during regionalization of decidualization.
Previous studies indicated that spatiotemporal expression pattern of Bmp2 with the progression of decidualization contributed to highly heterogeneous decidual cells1,6. At the initiation of decidualization, distinct accumulation of Bmp2 in the subepithelial stroma was essential for blastocyst attachment reaction at the implantation site2,6,8. With the spatiotemporal progression of decidualization, expanded Bmp2 expression in the PDZ and SDZ was critical for the terminal differentiation of stromal cells6,8. A significant decrease of Bmp2 in the SDZ on day 8 caused by Men1 deficiency disturbed the terminal differentiation of stromal cells during the expansion of SDZ without affecting the blastocyst attachment reaction and the PDZ formation.
Menin has yielded cell-specific results in terms of H3K4me3 regulation and the expression of target genes including Hoxa genes, Cdkn1b and Cdkn2c, Esr1, and p35 through connecting with histone methyltransferases MLL1/211,12,13,14,15. There was a dramatic whole genomic chromatin alteration in human endometrium decidualization marked by histone modification and chromatin accessibility46,47. However, the role of H3K4me3 modification in decidual regionalization remained elusive. Distinctive histone methyltransferases in large COMPASS-like complexes performed non-redundant histone modifications in various cell types48. The SET1A/B family is responsible for genome-wide bulk H3K4me2/H3K4me3 modification and the MLL3/4 complex family mediates H3K4me1 modification at enhancers and super-enhancer48. MLL1/2 complex, containing unique subunit Menin, is responsible for H3K4me3 modification at certain genes in cell-specific manner11,48. In this study, we depicted the H3K4me3 profiling in regionalized decidualization during early pregnancy and unraveled its regulatory apparatus by Menin.
Among the direct targets marked by Menin-H3K4me3 during stroma decidualization, Ptx3 involved in decidualization regulation possesses specific expression pattern in the SDZ41, but its physiological significance in stromal cell differentiation remains intangible. Several pieces of evidence showed that PTX3 acted as a natural FGF2 trap through its N-terminal domain to sequester FGF2-ERK1/2 signaling from promoting cell proliferation42. Interestingly, our investigation demonstrated that Men1-deficient uteri showed augmented FGF2-FGFR1-ERK1/2 signaling activity in the SDZ in the absence of PTX3. This abnormality subsequently reduced Bmp2 and blocked cell differentiation in the SDZ. Consistent with previous studies, the inhibitory effect of PTX3 on FGF2 was conserved during mouse decidualization. Indeed, the homeostasis between BMP and FGF has been described as “constituting a common module” throughout embryogenesis35,49. FGF signaling inhibited the expression of BMPs in dorsal mesoderm, thus limiting their expression to ventral mesoderm for proper dorsoventral axis specification50. Inhibition of BMP activity by the FGF signal promoted posterior neural development51. Furthermore, suppression of BMP signaling by FGF2 sustained undifferentiated proliferation of human ES cells43. Consistently, we evidenced that the discouraged cross-talk between BMP2 and FGF2 coordinated by Menin regulated PTX3 facilitated the maturation of decidua, which was further supported by the mutually exclusive expression of Bmp2 and Fgf2 in the SDZ and undifferentiated stromal cells, respectively. Together, we provided insightful evidence that the uncomfortable cross-talk between stromal cells in different regions through paracrine manner was curbed under the precise orchestrating of PTX3.
Moreover, Men1 deficiency disrupted the polyploidization in the SDZ with reduced large mono or bi-nucleated polyploid cells as evidenced by H3K27me3. In female somatic cells, the punctate immunostaining of H3K27me3 stands for inactivated X chromosome25. Somatic cells with two or more punctate H3K27me3 in nuclei were considered as polyploid cells. Currently, flow cytometry was the major way to evaluate the polyploid stromal cells. Here, we established a visible method to estimate polyploidization, which will greatly advance mechanisms to study polyploidy.
Previously studies suggested that endoreduplication and the absence of cytokinesis were the primary reasons for polyploidization of stromal cells which were mediated by various cyclin-associated proteins3,5,27. Here, we found that cytokinesis program was significantly enriched in Men1d/d decidual cells. We also provided a previously unappreciated mechanism for this black box. Cdkn1b (encoding p27), a recognized Menin-MLL1/2 target gene13, was decreased in Men1d/d uteri. Furthermore, multiple observations proved that female mice lacking functional p27 were infertile52,53,54. Furthermore, based on the observation that p27 induced polyploidy of liver cells without cytokinesis32,55, we speculated p27 also participated in regulating decidual cell polyploidization. Though the mRNA of Cdkn1b was reduced, the H3K4me3 modification at the promoter of Cdkn1b between Men1f/f and Men1d/d stroma was comparable, indicating an alternative regulation of Menin on Cdkn1b which deserved further investigation.
Collectively, our results provided a perspective that the patterning of decidual cells into disparate fates through the concerted activity of BMP and FGF signaling pathways underpinned the progression of decidualization. It’s known that the gland is also critical for the decidualization processing as reported in the Ltf-Cre mediated FOXA2 deletion mouse model23. In this study, we mainly investigated the role of Men1 in decidualization based on both in vivo and in vitro evidence. While how Men1 regulates glands growth and distribution in decidualized stroma and the physiological role of glandular Men1 in decidualization deserve further investigation. Results reported here revealed that the blunt induction of BMP2 caused by unrestrained FGF2-ERK1/2 signaling activity deranged the development of SDZ due to disorganized genomic H3K4me3 distribution in the absence of Men1. PTX3, an extra-cellular trap for FGF2, was identified as a critical Menin-H3K4me3 regulated downstream gene in decidual regionalization and pregnancy maintenance by curbing the cross-talk between FGF2-ERK1/2 and BMP2. Our findings will remarkably advance our knowledge on current model of decidualization and inspire future studies for human fertility improvement.
Methods
Animals
Two-month-old C57BL/6 male and female mice were used in the present study. Men1 floxed mouse line (Men1f/f) was constructed as previously described10. Uterine-specific knockout mice (Men1d/d) were generated by mating Men1f/f females with Pgrcre/+ males16. Mice were housed in the animal care facility of Xiamen University with a controlled environment (22 ± 2 °C, 50–60% humidity, 12-h light/dark cycle, lights on at 7 AM) and free access to food and water according to the guidelines for the care and use of laboratory animals. All experimental procedures were approved by the Animal Welfare Committee of Research Organization (X200811), Xiamen University.
Analysis of pregnancy events
Two-month-old female mice were mated with fertile wild-type males to induce pregnancy (vaginal plug = day 1 of pregnancy). Plug-positive females were kept separately for pregnant experiments. Pregnancy rate and litter size were monitored for the whole pregnancy process. For day 5 and day 6 pregnant mice, implantation sites were visualized by an intravenous injection of 100 µL of 1% Chicago blue in saline. The number and average weight of implantation sites demarcated by distinct blue bands was recorded. Uterine horns were flushed to check for the presence of embryos if no blue band was observed. Mouse blood samples were collected on day 6 and serum E2, as well as P4 levels, were measured by radioimmunoassay. At least three mice were used for every individual experiment in each mouse model.
Artificial decidualization model
Pseudopregnant mice were obtained by mating 2-month-old females with vasectomized males of the same strain. To induce artificial decidualization, one uterine horn of pseudopregnant mice was infused with sesame oil (25 μl) on day 4; the non-infused contralateral horn was taken as a control. The weight of infused and non-infused uterine horns was recorded 4 days after the oil infusion and the fold increase in uterine weights was served as an index of decidualization24.
In situ hybridization
In situ hybridization with isotopes or digoxygenin (DIG) was modified according to the previously described method24. Frozen sections (10 μm) were mounted onto poly-L-lysine coated slides and stored at −80 °C until used. After removal from −80 °C, the slides were placed on a slide warmer (37 °C) for 3 min and then fixed in 4% paraformaldehyde in PBS for 15 min at 4 °C. Following prehybridization, uterine sections were hybridized to specific cRNA probes overnight at 65 °C. After hybridization, the slides were incubated with RNase A (10 mg/ml) at 37 °C for 30 min. RNase A-resistant hybrids were detected by autoradiography using liquid emulsion or Anti-Digoxigenin-AP, Fab fragments (Roche). Mouse-specific cRNA probes labeled with isotope or digoxin for Men1, Bmp2, Dan, Igfbp5, Bmp7, Wnt4, Prl8a2, Hoxa10, Ptn, Sfrp4, Ptx3, and Fgfr1 were used for hybridization.
Immunostaining
The tissue specimens were fixed overnight in 10% neutral buffered formalin and then dehydrated in increasing concentrations of ethyl alcohol, followed by clearing of alcohol by xylene. Uterine slices were deparaffinized and incubated in citrate buffer for antigen retrieval by hyperbaric heating and then incubated overnight at 4 °C with the primary antibodies including Menin (Bethyl, 1:1000), COX2 (Santa Cruz, 1:200), Dtprp (homemade, 1:200), Ki67 (Servicebio,1:200), PL1 (Santa Cruz, 1:200), 3β-HSD (Santa Cruz, 1:200), p450scc (Santa Cruz, 1:200), PR (Cell Signaling Technology, 1:200), HAND2 (Santa Cruz, 1:200), p27 (Abcam,1:100), pH3 (Cell Signaling Technology, 1:200), ERK1/2 (Cell Signaling Technology, 1:200) and p-ERK1/2 (Cell Signaling Technology, 1:200). A Histostain-SP Kit (Zhongshan Golden Bridge Biotechnology) was applied to visualize the antigen. Immunofluorescence staining for OCT4 (Cell Signaling Technology, 1:200), β-Catenin (Abcam, 1:200), H3K27me3 (Cell Signaling Technology, 1:200), BrdU (Abcam, 1:500), PCNA (Santa Cruz, 1:200) and FOXA2 (Abcam, 1:500) was performed in paraffin-fixed sections and secondary antibody CyTM3 AffiniPure Goat Anti-Rabbit IgG(H + L) (Jackson ImmunoResearch,1:200) were used. The images were captured by Leica DM2500 light microscope. Antibodies with detailed information are listed in Supplementary Table 1.
Western blot
Decidual cells were isolated as described previously17. The proteins were separated by using 10% SDS-PAGE and transferred to polyvinylidene difluoride membranes. And then the membranes with proteins were blocked with 5% skim milk in TBST for 1 h at room temperature (RT) and incubated overnight at 4 °C with primary antibody for Menin (Bethyl, 1:2000), β-Actin (Bioworld, 1:3000), Dtprp (homemade, 1:2000), ERK1/2 (Cell Signaling Technology, 1:1000), p-ERK1/2 (Cell Signaling Technology, 1:1000), BMP2 (Abcam, 1:500), SMAD1/5/8 (Cell Signaling Technology, 1:1000), p-SMAD1/5/8 (Cell Signaling Technology, 1:1000), H3K4me3 (Abcam, 1:2000) and H3 (Abmart, 1:2000). After incubation with primary antibody, membranes were incubated with specific secondary antibodies (Zhongshan Golden Bridge Biotechnology, 1:5000) for 2 h at RT. Bands were visualized using Supersignal West Pico (Thermo Scientific) according to the manufacturer’s instructions. Uncropped and unprocessed scans of the blots are presented in the Supplementary Fig. 13. Antibodies with detailed information are listed in Supplementary Table 1.
Quantitative real-time PCR
Total RNA was extracted from uterine tissues or cells using TRIzol reagent (Invitrogen) following the manufacturer’s protocol. About 1 μg RNA was used to synthesize cDNA. Expression levels of the genes were validated by quantitative real-time PCR analysis with SYBR Green (TAKARA). All assays were performed at least three times. All PCR primers are listed in Supplementary Table 2.
Flow cytometry
Day 8 decidual cells were digested and harvested. The cell pellet was suspended in 0.25 ml PBS after centrifugation; 1 ml of cold 80% ethanol was added dropwise under constant and gentle vortexing. Samples were incubated for 30 min on ice and subsequently overnight at −20 °C before being subjected to staining. Cell sediments were suspended in staining solution (PBS containing 5 mg/ml Propidium Iodide and 2 mg/ml DNase-free RNase A) the next day. Samples were incubated for 30 min at 37 °C in the dark. They were then returned to RT and subjected to flow cytometry using Beckman Cytoflex. Flow cytometry data were analyzed using FlowJo software (v10, Tree star). The intensity value of SSC-A and FSC-A of fluorescence-activated cell sorting (FACS) are used for loose gates. The intensity value of FSC-A and FSC-H of FACS are used to gate a single cell. The polyploid cells are distinguished by the intensity value of FSC-A which is proportional to cell size and the intensity value of Propidium iodide staining which is used to measure DNA content. The experiments were repeated three times.
RNA-seq
Total RNA was extracted from day 8 decidua (dissect out the embryo and muscle layer) of Men1f/f and littermates Men1d/d using TRIzol reagent (Invitrogen) according to the manufacturer’s protocol. Purified RNA was prepared and subjected to RNA sequencing using BGISEQ-500 platform (China, BGI). RNA-seq raw data were initially filtered to obtain clean data after quality control by Trimgalore. High-quality clean data were aligned to the mouse reference genome (mm10) using STAR.
RNA-Seq data analysis
Differential expression genes were normalized to fragments per kilobase of exon model per million mapped reads (RPKM) using the EdgeR3.9 package in R with the criteria of fold change significantly greater than 1.5 and p < 0.05. The visualization of RNA-Seq data was done by ggplot2 package in R. Gene ontology (GO) enrichment analysis of differential expression genes (DEGs) were analyzed by using DAVID (the Database for Annotation, Visualization, and Integrated Discovery, [https://david.ncifcrf.gov]). GO terms with corrected p < 0.05 were considered significantly enriched. Gene Set Enrichment Analysis (GSEA) was performed to determine whether a defined set of genes shows statistically significant differences between Men1f/f and littermates Men1d/d decidual tissues.
ChIP-Seq
Chromatin immunoprecipitation (ChIP) was modified and performed according to the previously described standard protocol56. Decidual tissue wetted with PBS quickly cut into small pieces with an iris scissor. Snipped tissue was fixed with 1% formaldehyde (Cell Signaling Technology) for 10 mins at RT (for H3K4me3 ChIP), or fixed with disuccinimidyl glutarate (DSG, Santa Cruz, 2 mM) for 30 mins at RT and then double fixed with 1% formaldehyde for another 10 mins at RT (for Menin ChIP). Fixation was stopped by glycine (0.125 M). Tissue homogenate obtained by using Dounce Tissue Grinder was filtered through a 200 μm cell strainer to remove connective tissue. Fixed cells were lysed by Lysis Buffer 1 (50 mM HEPES pH 7.5, 1 mM EDTA, 140 mM NaCl, 0.5% NP-40, 10% glycerol, 0.25% Triton X-100), Lysis Buffer 2 (10 mM Tris-HCl pH8.0, 1 mM EDTA, 0.5 mM EGTA, 200 mM NaCl) and Lysis Buffer 3 (10 mM Tris-HCl pH8.0, 1 mM EDTA, 0.5 mM EGTA, 100 mM NaCl, 0.1% Sodium Deoxycholate, 0.1% N-lauroylsarcosine). All lysis buffers should be supplemented with protease inhibitors cocktail (Roche) before use. Chromatin DNA was sheared to an average 300–500 bp by using a BioRuptor sonicator (Diagenode). Solubilized chromatin was centrifuged to remove debris and incubated overnight at 4 °C with antibody Menin (Bethyl, 1:50) and H3K4me3 (Abcam, 1:50) bound to 20 μl protein A magnetic beads (Invitrogen). After washing and elution, the protein-DNA complex was reversed by heating at 65 °C overnight. Immunoprecipitated DNA was purified by using QIAquick spin columns (Qiagen). Immunoprecipitated and input DNA were quantified using Qubit 4.0 fluorometer. ChIP-seq libraries were prepared by using the KAPA DNA Hyper Prep Kit (KK8502) following the manufacturer’s instruction and sequenced with an Illumina Nova PE150. Two biological replicates were performed for ChIP-seq. For ChIP-qPCR, chromatin was sheared by sonication until the average length of 500-1000 bp and pulled down by antibody Menin (Bethyl, 1:50), H3K4me3 (Abcam, 1:50) and Rabbit IgG (Cell Signaling Technology, 1:50) bound with 20 μl protein A magnetic beads (Invitrogen). Specific primers were used to detect immunoprecipitated chromatin fragments, as well as input chromatin. All PCR primers are listed in Supplementary Table 2.
Primary uterine stromal cell culture
Three to four pseudopregnant day 4 mouse uterine horns were cut into small pieces (2–3 mm). Tissue pieces were first digested in 3 ml fresh medium (HBSS antibiotic; Gibco) containing 6 mg/ml dispase (Gibco) and 25 mg/ml pancreatin (Sigma), and then incubated in fresh medium containing 0.5 mg/ml collagenase (Sigma) at 37 °C for 30 min. The digested cells were passed through a 70 μm filter to obtain the stromal cells. Cells were plated at 60 mm dishes or 6-wells plates, containing phenol red-free Dulbecco modified Eagle medium (DMEM) and Ham F12 nutrient mixture (1:1) (Gibco) with 10% charcoal-stripped fetal bovine serum (CS-FBS) and antibiotic. Two hours later, the medium was replaced with fresh medium (DMEM/F12, 1:1) with 10% CS-FBS. The next morning, the medium was replaced with DMEM/F12 containing 1% C-FBS, E2 (Sigma, 10 nM), P4 (Sigma, 1 μM) and antibiotic to induce decidualization. The media was changed every 48 h. For the treatment of primary uterine stromal cells, MI-503 (2 μM; MedChemExpress), recombinant murine FGF2 (PeproTech, 20 ng/ml), recombinant mouse PTX3 (R&D systems, 100 ng/ml) and MEK inhibitor PD0325901 (Selleck, 5 μM) were used.
Statistical analysis
All data are presented as mean ± SEM. Each experiment included at least three independent samples. Comparison between two groups was made by two-tailed unpaired Student’s t-test. P < 0.05 was considered to indicate a significant result.
Reporting summary
Further information on research design is available in the Nature Research Reporting Summary linked to this article.
Data availability
The sequencing data generated in this study have been deposited in the Gene Expression Omnibus database under accession code GSE182525, GSE191327, and GSE182539. Source data are provided with this paper.
Code availability
The data analysis pipeline used in this paper is deposited at [https://github.com/dwb0211/Menin].
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Acknowledgements
We are grateful to Prof. Francesco DeMayo (National Institute of Environmental Health Sciences) for providing us with the PgrCre/+ mice. Thanks to Bo He and Yufei Jiang in the lab for animal model establishment. Element for the mouse in Supplementary Fig. 5 was created with BioRender. This work was supported by the National Key R&D Program of China (2021YFC2700302 to H.W., 2018YFC1004400 to S.K., 2017YFC1001402 to H.W., 2018YFC1004100 to W.D.), National Natural Science Foundation of China (31970797 to Z.L., 81830045 and 82030040 to H.W., 81971388 to S.K, 81701483 and 81971419 to W.D.), Fundamental Research Funds for the Central Universities (20720190073 to W.D.).
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Mengy.L., W.D., L.T., M.L., and C.G. performed experiments and prepared figures. Mengy.L., W.D., J.L., S.K., H.W., and Z.L. designed experiments. C.Z. provided the Men1 loxP mouse model. Mengy.L., W.D., and S.K. analyzed data. Mengy.L., H.B., W.D., S.K., H.W., and Z.L. wrote the manuscript.
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Liu, M., Deng, W., Tang, L. et al. Menin directs regionalized decidual transformation through epigenetically setting PTX3 to balance FGF and BMP signaling. Nat Commun 13, 1006 (2022). https://doi.org/10.1038/s41467-022-28657-2
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DOI: https://doi.org/10.1038/s41467-022-28657-2
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