Abstract
Understanding the regulatory networks for germ cell fate specification is necessary to developing strategies for improving the efficiency of germ cell production in vitro. In this study, we developed a coupled screening strategy that took advantage of an arrayed bi-molecular fluorescence complementation (BiFC) platform for protein-protein interaction screens and epiblast-like cell (EpiLC)-induction assays using reporter mouse embryonic stem cells (mESCs). Investigation of candidate interaction partners of core human pluripotent factors OCT4, NANOG, KLF4 and SOX2 in EpiLC differentiation assays identified novel primordial germ cell (PGC)-inducing factors including BEN-domain (BEND/Bend) family members. Through RNA-seq, ChIP-seq, and ATAC-seq analyses, we showed that Bend5 worked together with Bend4 and helped mark chromatin boundaries to promote EpiLC induction in vitro. Our findings suggest that BEND/Bend proteins represent a new family of transcriptional modulators and chromatin boundary factors that participate in gene expression regulation during early germline development.
Similar content being viewed by others
Avoid common mistakes on your manuscript.
INTRODUCTION
Understanding the mechanisms of germ cell lineage development is central to reproductive medicine and offers valuable insight into origin-dependent imprinting as well as imprinting disorders. Despite the differences between human and mouse germ cell development, in vitro and in vivo mouse models remain indispensable due to technical and ethical constraints in studying human development. Indeed, studies in mouse have proven especially informative, revealing a spatially and temporally coordinated developmental process that progresses from primordial germ cell (PGC) specification (E6.25–7.25) to PGC migration and gonadal ridge formation (E8.0–12.5) and sex determination (after E13.5) (Saitou and Yamaji, 2010). Once arriving at the gonadal ridge, PGCs can differentiate into either oocytes or spermatozoa (Saitou and Yamaji, 2010; Saitou et al., 2012).
Epigenetic regulation (e.g., DNA demethylation, histone modifications, and chromatin remodeling) is integral to germ cell development (Kurimoto et al., 2015; von Meyenn et al., 2016). For instance, DNA methylation peaks during PGC specification and then declines during PGC migration before reaching its lowest level at E13.5 (Nakaki et al., 2013; Smith and Meissner, 2013). Throughout extensive epigenetic reprogramming occurs, including the erasure of parental imprints and reestablishment of DNA methylation in gametes (von Meyenn et al., 2016). DNA methylation erasure is an active demethylation process (Hajkova et al., 2002; Lee et al., 2002), mediated by ten-eleven translocation (Tet) proteins that catalyze the hydroxylation of 5-methylcytosine (5mC) to 5hmC (Wu and Zhang, 2017; Hill et al., 2018; Verma et al., 2018). Tet methylcytosine dioxygenase 1 and Tet methylcytosine dioxygenase 2 (Tet1/Tet2)-deficient mice have abnormal methylation at imprint loci (Zhang et al., 2010; Hackett et al., 2013; Vincent et al., 2013; Yamaguchi et al., 2013; Okashita et al., 2014).
Many factors, such as the TGFβ superfamily, are known to play crucial roles in germ cell development (de Sousa Lopes et al., 2004; Saitou and Yamaji, 2010; Senft et al., 2019). Another well-known marker for established PGCs is developmental pluripotency-associated 3 (Dppa3/Stella), which is expressed in oocytes, blastocysts, and during PGC development in vivo (Payer et al., 2006). Although Stella deficiency alone does not affect PGC fate (Bortvin et al., 2004), its overexpression can promote germline differentiation (Wongtrakoongate et al., 2013). It was shown recently that Tet protein inactivation could downregulate Stella expression in mouse embryonic stem cells (mESCs) (Mulholland et al., 2020), indicating a role of DNA methylation in regulating Stella expression, although how Stella is upregulated during early embryonic development for PGC commitment remains unclear. Several PR/SET domain zinc finger proteins (e.g., Prdm1/Blimp1 and Prdm14), which can function as chromatin remodeling and transcription factors, are also critical to early PGC specification. For example, Prdm1 or Prdm14 knockout (KO) mouse embryos lacked PGCs (Ohinata et al., 2005; Yamaji et al., 2008; Kurimoto et al., 2008a, b; Vincent et al., 2013). Prdm14 could also associate with Tet1 and enhance Tet1 recruitment to demethylate germ line-specific genes and imprinted loci in mESCs (Okashita et al., 2014).
In the past decade researchers have successfully recapitulated development in vitro, generating mouse PGCs that were capable of developing into gametes and viable animals (Hayashi et al., 2012; Nakaki et al., 2013; Hikabe et al., 2016). For example, through a two-step culturing scheme, pluripotent mESCs can be converted to epiblast-like cells (EpiLCs) and then PGC-like cells (PGCLCs) (Hayashi et al., 2011, 2012). The efficiency of EpiLC/PGCLC derivation from mESCs remains low, even with the overexpression of PGC specification master regulators such as Prdm1, Stella, Prdm14, and transcription factor AP-2 gamma (Tfap2c) or pluripotency factors such as Nanog homeobox (Nanog) (Nakaki et al., 2013; Murakami et al., 2016). Pluripotency transcription factors are key to maintaining pluripotency and sufficient to reprogram differentiated cells into pluripotent stem cells (Loh et al., 2006; Takahashi and Yamanaka, 2006; van den Berg et al., 2010). In addition to mESCs and primed epiblast cells, they are also expressed in PGCs and critical to germ cell lineage determination (Kehler et al., 2004; Okamura et al., 2008; Radzisheuskaya et al., 2013). We reasoned that identifying and studying proteins that interact with these core pluripotency factors during PGC cell fate determination should reveal new regulators of germ line development and help improve in vitro PGC derivation.
Through a genome-wide protein-protein interaction screen using human POU class 5 homeobox 1 (POU5F1 or OCT4), NANOG, SRY-box transcription factor 2 (SOX2), and Kruppel like factor 4 (KLF4) as baits and the arrayed bi-molecular fluorescence complementation (BiFC) platform (Lee et al., 2011), we singled out candidate proteins that could interact with multiple pluripotency factors and examined them in a secondary EpiLC induction screen in reporter mESCs, which uncovered BEN-domain (BEND/Bend) family proteins as novel pluripotency factor-binding partners that could also regulate germ cell differentiation. We showed that Bend5 worked together with Bend4 to promote EpiLC induction in vitro. In addition, ATAC-seq analysis indicates that Bend4 and Bend5 did not bind open chromatin. Our findings suggest that BEND/Bend proteins represent a new family of transcriptional modulators and chromatin boundary factors that participate in genes expression regulation during early germline development.
RESULTS
A coupled genome-wide screening strategy using BiFC and germ cell differentiation assays
To better understand the protein interaction networks of core pluripotency factors and identify possible new regulators of PGC cell fate, we developed a coupled screening strategy utilizing the yellow fluorescent protein (YFP)-based BiFC assay (Hu and Kerppola, 2003) and the EpiLC differentiation assay using Stella-GFP reporter mESCs (Payer et al., 2006; Hayashi et al., 2011). The BiFC assay enables detection of pairwise protein-protein interactions that bring YFP N terminal (YFPN) and C terminal (YFPC) in two separate proteins to close proximity and allow for their co-folding into a functional fluorescent protein in live cells (Lee et al., 2011). Co-expression of the YFPN and YFPC fragments alone has extremely low YFP background signals (Lee et al., 2011). The YFP-based BiFC assay has been successfully used to map the interactomes governing telomere maintenance (Lee et al., 2011). To carry out the screen, we first generateÔd bait HTC75 cell lines stably expressing YFPN tagged human OCT4, NANOG, SOX2, or KLF4 and then transduced these cells with retroviruses encoding the human ORFeome library fused to YFPC (Fig. 1A). YFP fluorescence complementation was subsequently analyzed by flow cytometry and the CytoArray program to derive candidate gene lists for each bait (Lee et al., 2011). Because the four bait proteins are known to interact with each other, each candidate was further ranked based on its appearance in all four screens to derive a list of overlapping candidates (Fig. 1B). Since many of the human candidate genes share high sequence and functional homology with their mouse counterparts, the top overlapping candidate genes were subsequently stably expressed in Stella-GFP reporter mESCs for verification using the EpiLC differentiation assay (Fig. 1A). In these reporter cells, the sequences encoding eGFP were inserted into the first exon of the mouse Stella/Dppa3 locus. Following EpiLC induction, upregulation of Stella expression would allow eGFP to be expressed and detected (Nakaki et al., 2013). Candidate genes that enabled GFP expression during EpiLC induction were thus identified by microscopy and flow cytometry (Table S1).
Identification of interaction networks of pluripotency factors and novel players in PGC cell fate regulation
Several known interacting pairs were among the higher ranked candidates from our arrayed BiFC screens (e.g., SOX2/KLF4 with OCT4, KLF4 with NANOG/SOX2, and SOX2 with KLF4) (Figs. 1C and S1A), validating our protein-protein interaction screening approach. Of the potential interacting partners, some appeared in all four candidate lists. We selected 93 candidates that ranked high and appeared in at least two BiFC datasets (Table S2). Of this list, OCT4/NANOG have the most overlapping candidates (69/93), followed by NANOG/SOX2 (63/93) and OCT4/SOX2 (57/93), further underscoring the interconnectedness of the pluripotency factor interaction networks. Gene ontology analysis revealed transcription, positive regulation of transcription, transcriptional regulation, and mRNA splicing to be among the top categories (Fig. 1D).
Next, the 93 overlapping human candidate genes were individually expressed in the Stella-GFP reporter mESCs and assessed for their activity in EpiLC induction assays (Fig. 1A). By day 2 cells overexpressing several genes (i.e., BEN domain-containing protein 5 (BEND5), Homeobox A3 (HOXA3), Chromosome 4 open reading frame 27 (C4ORF27), and NME/NM23 family member (NME7)) had significantly higher GFP signals compared with controls when analyzed by fluorescence microscopy (Fig. 1E) and FACS (Fig. S1B). In the two-step culturing scheme where EpiLCs were further cultured in PGCLC-inducing medium (Hayashi et al., 2012), ectopic expression of these genes also resulted in significantly higher Stella-GFP signals (Fig. S1C). These experiments not only uncovered previously unknown players in PGC cell fate determination but also imply that their interaction with pluripotency factors may be important to this process.
Bend5 is a novel interacting protein of pluripotency factors and promotes EpiLC induction from mESCs
Named for its presence in BANP/E5R/NAC1, the BEN domain is a highly conserved bioinformatically defined motif (Abhiman et al., 2008). BEN domain-containing proteins can be found from Drosophila to mammals and have been implicated in chromatin regulation during early development (Dai et al., 2013). In our BiFC screens, BEND5 was not only identified from all four baits but also one of the highest ranked interaction candidates for OCT4, NANOG, and SOX2 (Figs. 1C and S1A). It was very potent in EpiLC-induction assays, at levels comparable to known PGC-promoting factors such as PRDM1/BLIMP1 and PRDM14 (Fig. 1F). In mouse, Bend5 appeared to be highly expressed in PGCs as well as in tissues such as testis (Fig. S2A). When we examined mouse Bend5 in GST pulldown and pairwise BiFC assays, we confirmed that it indeed could interact with mouse Oct4 and Sox2 (Figs. 2A and S2B). When Stella-GFP reporter mESCs stably expressing mouse Bend5 were cultured in EpiLC-inducing medium, increased GFP expression was observed as well (Fig. 2B). And RT-qPCR analysis of the GFP-positive cells confirmed that increased Bend5 expression was accompanied by increased Stella messages and decreased Oct4 expression as the cells differentiated (Fig. S2C and S2D). In embryoid body (EB) formation assays, mESCs can aggregate and spontaneously differentiate into cells of different germ layers, including PGC-like cells at relatively low frequency (Wei et al., 2008). When the Bend5-expressing reporter mESCs were examined in EB formation assays, increased Stella-GFP positive (SG+) cells were detected compared to controls (Fig. S2E), indicating that overexpressing Bend5 could indeed upregulate Stella expression during differentiation.
During early germ cell development, Prdm1/Blimp1 was activated first in a few lineage-restricted PGCs, which then became double positive for both Blimp1 and Stella (Ohinata et al., 2005). To better probe the activity of Bend5, we took advantage of the dual-reporter mESC line expressing Blimp1-mVenus (BV) and Stella-ECFP (SC), where a small number of double-positive (BVSC+) cells could be detected following EpiLC induction (Hayashi et al., 2011, 2012; Nakaki et al., 2013). When Bend5 was stably overexpressed in the dual-reporter cells, increased BVSC+ cells were seen in both EpiLC induction and EB formation assays (Fig. S2F). More importantly, RNAi-mediated knockdown of Bend5 resulted in a decrease in BVSC+ cells (Fig. S2G). These data together support the notion that Bend5 may facilitate in vitro early germ cell differentiation of mESCs.
Bend5 overexpression upregulates gene expression in mESCs
Given the apparent role of Bend5 in promoting EpiLC differentiation and gene transcription, we decided to investigate by RNA-seq possible transcriptomic changes in Bend5-overexpressing Stella-GFP mESCs that were induced to differentiate. Compared with control cells, ectopic expression of Bend5 led to an increase in the number of genes up-regulated upon differentiation induction (fold change > 2) (Fig. 2C), including canonical primed epiblast cell markers such as Fgf5 and Fgf15 (Fig. 2D), as confirmed by RT-qPCR using FACS-sorted GFP+ cells (Fig. 2E). Bend5-expressing cells also showed a corresponding drop in the number of genes down-regulated during differentiation (Fig. 2C), such as pluripotency genes Klf4 and Nanog (Fig. 2D and 2E). TGFβ/Activin signal pathways are critical to PGC development in vitro and act primarily through SMADs (Duggal et al., 2013, 2015; Yakhkeshi et al., 2018). Smad3/Smad4 can cooperate with AP-1 (c-Jun/c-Fos) to mediate TGFβ-induced transcription (Zhang et al., 1998). Consistent with these findings, Fos appeared highly expressed in PGCs compared to MEFs and mESCs (Fig. S2H). Upon EpiLC induction, cells overexpressing Bend5 exhibited increased expression of Fosb and Fos as well as metabolic enzyme (e.g., Car4) and developmental genes (e.g., Rab25, Gadd45γ, and H19) (Fig. 2D and 2E) (Table S3). These results combined implicate Bend5 in promoting EpiLC induction through upregulating genes associated with primed epiblast cells and the TGFβ/Activin signaling pathway. Interestingly, we found a collection of genes that specifically expressed in spermatogonial stem cells (SSCs) were upregulated in Bend5 overexpressed cells compared with control cells, including Usp26 (Ubiquitin specific peptidase 26), Thy1 (Thy-1 cell surface antigen), Sox3 (SRY-box transcription factor 3) (Table S4). These results suggested that Bend5 overexpression might promote germ cell differentiation in vitro.
Bend5 regulates DNA demethylation by recruiting Tet1 during EpiLC induction
It has been well established that PGC development is often accompanied by demethylation of differentially methylated regions (DMRs). For instance, the methylation of imprint genes appears to be erased in 13.5 dpc PGCs (Hajkova et al., 2002; Lee et al., 2002). Activin A treatment can upregulate Stella in vitro and inhibiting DNA demethylases Tet1 or Tet2 can downregulate Stella expression in mESCs, suggesting that DNA methylation is key to Stella expression (Duggal et al., 2013, 2015; Mulholland et al., 2020). The findings of upregulated gene expression in Bend5-overexpressing cells led us to further examine the effects of Bend5 overexpression on DNA methylation in mESCs. We first carried out bisulfite sequencing to analyze the DNA methylation status of imprint genes during EpiLC induction in Stella-GFP reporter mESCs expressing Flag-Bend5. As reported before, DNA methylation on H19 and Igf2r were absent in control 13.5 dpc PGCs (Fig. 3A) (Lucifero et al., 2002; Kagiwada et al., 2013). By bisulfite sequencing, we observed that the methylation level in H19 and Igf2r decreased as mESCs passaged in Lif and 2i on feeder-free conditions (called 2i/L mESCs), but not in serum and Lif on feeder cells (called S/L mESCs) conditions (Fig. S3A). In particular, the methylation levels of H19 and Igf2r in 2i/L mESCs at passage P1 and P3 were unchanged, while P11 or P16 showed decreased methylation (Fig. S3B). Furthermore, we observed that Bend5 overexpression did not affect imprint methylation (H19 and Igf2r) at P1 compared with control cells (Fig. S3C), but decreased imprint methylation (H19 and Igf2r) at P3 during EpiLC induction (Fig. 3A). During EpiLC induction, Bend5 overexpression decreased H19 methylation at D0 by nearly 2 fold (62.5% to 31.9%) but not Igf2r (38.6% to 40.5%) compared with control (Fig. 3A). The result indicated that the demethylation of H19 was partially dependent on the overexpression of Bend5. Upon EpiLC induction, vector alone cells showed minimal change in DNA methylation at the H19 locus (62.5% to 66.9%). In contrast, H19 methylation decreased by nearly 3 fold (66.9% to 20.9%) in Bend5-expressing cells when analyzed two days after induction. Similarly drastic reduction of DNA methylation also occurred at the Igf2r locus (69.8% to 15.9%) in Bend5-expressing cells after induction (Fig. 3A). These data indicate that Bend5 likely promoted DNA demethylation of imprinted genes during EpiLC differentiation. Next, we examined the methylation status of CpG islands upstream of Stella. Again, the level of CpG island methylation in control cells remained essentially unchanged after differentiation, but decreased significantly in Bend5-expressing cells (Fig. 3B).
The dramatic decrease in DNA methylation with Bend5 overexpression suggests involvement of DNA demethylases. Given that Tet1/Tet2 can be targeted to within −2~3 kb upstream of Stella (Mulholland et al., 2020), we investigated Tet1/Tet2 occupancy in this region of the Stella locus by ChIP-qPCR (chromatin immunoprecipitation and real-time polymerase chain reaction) using mESCs stably expressing Flag-Bend5. Before induction (D0), these cells already exhibited a slight enrichment of Tet1 over control cells (Fig. 3C). After two days of EpiLC induction, Tet1 occupancy at the P2 position increased dramatically (Fig. 3C). In comparison, we found no specific enrichment of Tet2 at position P2 before or after EpiLC induction in Bend5-expressing cells (Fig. S3D). To better explore the enrichment of Tet1 at the Stella locus during EpiLC induction, we performed ChIP-seq (chromatin immunoprecipitation followed by sequencing) analyses using Stella-GFP mESCs expressing Flag-tagged Bend5. Consistent with the ChIP-qPCR results, in uninduced cells, a slight enrichment of Tet1 could be seen in regions upstream of TSS (transcription start site) (Box1) as well as the gene body (Box2) (Fig. 3D). Following induction, the amplitude of some of these Tet1-binding peaks increased dramatically (red arrows in Box 1 and 2). Notably, Tet1 expression in induced EpiLCs appeared to have decreased relative to D0 mESCs (Fig. S3E), suggesting that the enrichment was likely not a result of increased Tet1 levels. Tet1 was highly expressed in PGCs and responsible for active DNA demethylation of imprints and germline-specific genes (Vincent et al., 2005; Williams et al., 2011; Pastor et al., 2013; Zhang et al., 2016). Notably, dysfunction of Tet1 protein caused hypermethylation at the imprints (H19, Igf2r, Peg1, Mest etc.) and Tet1 knockout also led to hypermethylation at the imprints (H19 and Igf2r) (Liu et al., 2015; Zhang et al., 2016). These studies suggested that Tet1 indeed negatively regulated DNA methylation level of imprint genes. We speculated that Bend5 might promote DNA demethylation by actively recruiting Tet1 to the Stella promoter during EpiLC induction.
To test this idea, we co-expressed Flag-Bend5 and HA-tagged Tet1 in 293T cells and examined their interaction. As shown in Fig. 3E, Bend5 could indeed co-immunoprecipitate (co-IP) with Tet1. Our data thus far support the hypothesis that upon EpiLC differentiation, Tet1 may target to the Stella locus (and possibly other DMRs) through interaction with Bend5, thereby promoting DNA demethylation and activating gene transcription.
Bend5 binds to the promoter region of Stella through its BEN domain
Oct4 has been reported to bind the ATTTGCAT sequence in the Stella promoter region (−1.74 kb) for stem cell pluripotency maintenance (van den Berg et al., 2008). Given the interaction between Bend5 and Oct4 and the ability of BEN domains to bind DNA in a sequence-specific manner (Dai et al., 2015, 2013), we hypothesized that in addition to recruiting DNA demethylases, Bend5 might also directly target to the Stella locus to upregulate Stella expression. To test this idea, we first examined Bend5 occupancy in the promoter region of Stella by ChIP using Flag-Bend5 expressing mESCs. Before EpiLC induction, significant enrichment of Bend5 could be detected in Bend5-expressing cells at several positions upstream (within ~3 kb) of Stella TSS compared with control cells (Fig. 4A). Once cells were cultured in EpiLC induction medium, Bend5 enrichment at the Stella locus became less pronounced but remained significantly higher than in control cells two days after induction (Fig. 4A), even though expression of Bend5 itself had been drastically downregulated by this time (Fig. S2C), supporting the notion that Bend5 could target directly to the Stella promoter. Moreover, these Bend5-binding sites appeared to overlap with those of Oct4 (Fig. 4A) (van den Berg et al., 2008). In fact, Bend5 overexpression also increased Oct4 occupancy on Stella, suggesting that co-occupancy of Oct4 and Bend5 may be important for Stella upregulation.
When we compared Stella-GFP reporter mESCs expressing full-length Bend5 vs. the BEN domain deletion mutant (Bend5∆BEN), we found much lower Bend5 enrichment at the Stella locus in Bend5∆BEN-expressing cells (Fig. 4B and 4C), even though Bend5∆BEN showed similar nuclear localization as full-length Bend5 (Fig. S3F). Importantly, BEN domain deletion led to reduced GFP+ cells following EpiLC induction (Figs. 4D and S3G). To further probe the DNA-binding activity of Bend5, we performed electrophoretic mobility shift assays (EMSA) using recombinant full-length and BEN domain deletion Bend5 proteins (Figs. 4E and S3H). Multiple DNA oligos corresponding to sequences in the promoter region of Stella could be shifted by full-length Bend5 but not Bend5∆BEN, indicating the importance of the BEN domain in mediating Bend5 binding to DNA (Fig. S3I). These data together strongly support a role of Bend5 in regulating Stella expression during EpiLC differentiation and underline the importance of the BEN domain to Bend5 function.
The BEN domain-containing protein Bend4 can also interact with Oct4 and regulate Stella activation
Of the four BEN-domain family members present in the ORFeome library (BEND3, BEND5, BEND6, and BEND7), only BEND5 met all the criteria we set for the coupled screen. When we examined the relative mRNA levels of several BEN-domain family members, we found high expression of Bend4 in not only PGCs and mESCs but also testis (Fig. S4A and S4B). Of the two Bend4 isoforms, only isoform 1 contains the BEN domain and appeared to be the predominant isoform in mESCs (Fig. S4C). We therefore focused on this longer isoform for this study. Similar to Bend5, Flag-tagged mouse Bend4 could also co-IP with GST-tagged Oct4 (Fig. 5A). When Stella-GFP reporter mESCs overexpressing Bend4 were induced to differentiate into EpiLCs, there were more GFP+ cells as well (Figs. 5B, 5C and S4D), with upregulated expression of epiblast cell-related genes such as Fgf5, Car4, and Rab25 and increased Oct4 and Tet1 binding to the Stella locus (Fig. 5D and 5E). These results combined support the notion that Bend4 is another BEN-domain family member that can interact with pluripotency factors and participate in regulating gene expression during PGC development.
Bend5 synergizes with Bend4 in induction of Stella expression
To further probe the relationship between Bend5 and Bend4, we next carried out EpiLC induction assays using Stella-GFP reporter mESCs co-expressing Bend4 and Bend5 (Fig. S4D and S4E). While cells ectopically expressing either Bend5 or Bend4 showed comparable increase in GFP+ cells following induction, Bend4/Bend5 co-expression resulted in more GFP+ cells than expression of either gene alone (Fig. 5F), indicating possible synergy and non-redundant functions of the two genes. Compared to Bend5, Bend4 appeared to be expressed at much higher levels in mESCs than in MEFs (Figs. S2A and S4A). We therefore decided to target Bend4 in Bend5-expressing Stella-GFP reporter mESCs using the CRISPR/Cas9 technology with a sgRNA that targets the Bend4 BEN domain (Fig. S4F). Two clones with deletions in the BEN domain were isolated. As shown in Fig. 5G, disrupting the Bend4 BEN domain led to markedly reduced numbers of GFP+ cells, suggesting that Bend5 regulation of Stella expression was dependent on the BEN domain of Bend4. The above findings support the model in which Bend5 and Bend4 facilitate transcriptional activation of the Stella gene by cooperating with Oct4 and Tet1 in response to EpiLC induction signals.
Bend5 co-occupies PGC-related genes with Bend4
To better define the activities of Bend5 and Bend4 and their target genes during EpiLC induction, we performed ChIP-seq analyses using Stella-GFP mESCs individually expressing Flag-tagged Bend5 or Bend4. At the Stella locus, the overall binding patterns of Bend5 and Bend4 showed some overlapping peaks but were not identical (Fig. 6A, D0 orange arrows and D2 black arrows). A noticeable increase in both the number and amplitude of Bend5/Bend4 binding peaks could be detected by day 2 of EpiLC induction (Fig. 6A, Box 1), which is consistent with our findings in the region upstream of Stella TSS (−3 kb). Within the gene body of Stella, there were obvious changes as well in the location and amplitude of Bend5/Bend4 binding peaks following differentiation induction (Fig. 6A, Box 2). Based on published Oct4 ChIP-seq data using mESCs induced to differentiate into EpiLCs by Activin A (Buecker et al., 2014), increased Oct4 binding to the −1.74 kb and TSS regions of the Stella gene could be observed by day 2. These peaks partially overlap with those of Bend5 and Bend4 (Fig. 6A, green arrows), which is consistent with our ChIP-qPCR results (Fig. 4A) and further supports the idea that Bend5/Bend4 can co-occupy the Stella locus with Oct4.
In addition to Stella, Bend5/Bend4 binding could also be detected at the loci of transcription factors Prdm1, Prdm14, Tfap2c, and Lin28a (Figs. 6B, 6C, S5A and S5B), which have been shown to promote PGC development (Kurimoto et al., 2008a, 2008b; Yamaji et al., 2008). The binding peaks were distributed in the gene body as well as regions upstream of TSS. Some of these peaks (red arrows) also increased in amplitude following EpiLC induction (Figs. 6B, 6C, Box 1 and 2; S5A and S5B). Again, we found overlap in binding peaks with Oct4 on Prdm1 and Lin28a (Fig. 6B and 6C, Box 3), adding additional support to the notion that Bend5/Bend4 can cooperate with Oct4 on genes important for PGC development.
Bend5 and Bend4 dynamically associate with DNA during EpiLC induction
Individual BEN domains can vary greatly in actual sequences and consensus binding motifs (Dai et al., 2015). For instance, motif analysis by CentriMo predicts quite distinct consensus motifs for Bend5 and Bend4 (either before or after induction) compared to the Drosophila Bend protein Insv, which functions as a transcriptional repressor in neural development (Fig. S5C) (Bailey and Machanick, 2012; Dai et al., 2013). Our ChIP-seq data indicate partial overlap (<20%) of Bend5/Bend4-binding sites throughout the genome (Fig. S5D). The BEN domains of Bend5 and Bend4 share 26% sequence identity and 44% similarity (Fig. S5E), which may help explain their overlapping but different DNA-binding patterns in cells and support the idea that these two genes can function both collaboratively and independently during germ cell development. Results from the EM-based MEME (long motifs of ≤30 bp in length) and novel word-based DREME (shorter motifs of ≤8 bp) algorithms for de novo motifs suggest somewhat similar binding motifs for Bend5/Bend4 before differentiation (Fig. 6D) (Bailey, 2011). Differentiation induction not only increased the number of predicted motifs but also altered the specific motif sequences, although motif #1 remained largely unchanged and all of the predicted motifs can be found at the Stella locus (Fig. S5F). These alterations signal the dynamic nature of Bend5/Bend4 binding to their target sites during EpiLC differentiation. Coupled with their apparent abilities to elevate enrichment of Tet1 and Oct4 at the Stella locus, these results also hint at chromatin re-organization that resulted from Bend5/Bend4 overexpression.
To assess globally how chromatin accessibility might change in mESCs stably expressing Bend5/Bend4, we decided to employ ATAC-seq (assay transposase-accessible chromatin with high-throughput sequencing) (Buenrostro et al., 2013) and performed peak overlapping analyses using data from ATAC-seq and ChIP-seq for Bend5/Bend4-binding sites. We found very little overlap (<5%) between Bend5/Bend4-binding sites and ATAC-seq peaks throughout the genome with or without EpiLC induction (Fig. S6A), suggesting a lack of Bend5/Bend4 binding to accessible chromatin. When we superimposed ATAC-seq and Flag ChIP-seq peaks at the Stella locus, we found Bend5/Bend4-binding peaks to concentrate near the boundaries of open and closed chromatin (Fig. 7A, red box). Similar patterns were also apparent on other PGC-related genes (e.g., Prdm14, Lin28a, and Tfap2c) (Fig. S6B). When the data were cross-referenced with our RNA-seq results for the Stella locus, it was clear that Bend5 and Bend4 significantly promoted the expression of Stella exon 1 and exon 2 compared to controls, with concentrated ATAC-seq and Flag ChIP-seq peaks in this region. These observations indicate that Bend5 and Bend4 might act as boundary factors and collectively contribute to Stella expression upon EpiLC induction.
Bend5 and Bend4 are a new family of chromatin boundary factors
The organization of genomes is critical to genome replication and gene expression. Eukaryotic chromosomes have been found to fold into domains where intra- and inter-domain interactions can occur through contact regions known as topologically associating domains, which are evolutionarily conserved features and formed with the help of special elements called chromatin boundaries or insulators that are capable of pairing with each other (Beagan and Phillips-Cremins, 2020; Dixon et al., 2016, 2012; Pope et al., 2014). Boundary element pairing may be achieved through the action of sequence-specific DNA-binding proteins such as the CCCTC-binding factor (CTCF) and their co-factors. CTCF is a multi-functional ubiquitously expressed protein with 11 tandem C2H2 zinc fingers (Lobanenkov et al., 1990; Fischer et al., 1993). It functions in transcriptional regulation and genome organization (Gaszner and Felsenfeld, 2006; Wendt et al., 2008; Handoko et al., 2011; Plasschaert et al., 2014). CTCF-null embryos could not implant and died by pre-implantation (Wan et al., 2008; Moore et al., 2012), and conditional CTCF KO mice were infertile with a 90% reduction in sperm count (Hernandez-Hernandez et al., 2016). CTCF can homodimerize and interact with cohesion to mediate long-distance chromatin interaction and plays a critical role in cell type-specific genomic organization and chromatin boundary function (Ji et al., 2016; Beagan et al., 2017; Arzate-Mejia et al., 2018).
To investigate possible interplay between Bend5/Bend4 and CTCF during EpiLC induction, we performed CTCF ChIP-seq analyses using Stella-GFP mESCs individually expressing Flag-tagged Bend5 or Bend4. Results from CTCF ChIP-seq were then compared to Flag ChIP-seq data using the same cells (Fig. 7B). Before EpiLC induction, there was minimal overlap (<5%) between CTCF unique peaks and those of either Bend5 or Bend4 throughout the genome (Fig. 7B). The percentage of overlap increased to <20% after EpiLC induction, indicating that the majority of Bend5/Bend4 peaks remained distinct from CTCF peaks. Furthermore, when we overlaid the CTCF peaks with those of Bend5 or Bend4 on the Stella locus we found little overlapping as well regardless of EpiLC induction (Fig. 7C). Similar results were obtained when we compared CTCF and Bend5/Bend4 binding on other PGC-related genes (e.g., Prdm14, Lin28a, and Tfap2c) (Fig. S6C).
Whole-genome analysis of CTCF in chromatin boundary regions revealed demarcation of repressive and active chromatin domains (Cuddapah et al., 2009). Given the apparent binding difference between Bend5/Bend4 and CTCF, we analyzed the distribution of Bend5/Bend4-binding sites and ATAC-seq peaks throughout the genome after EpiLC induction. We found reverse correlation between Bend4-binding sites and whole-genome ATAC-seq peaks, and between Bend5-binding sites and exons and introns of ATAC-seq peaks (Fig. 7D), suggesting that Bend4 and Bend5 likely bind to closed chromatin. Our data support the model where Bend5 and Bend4 help mark the boundary of open/closed chromatin after EpiLC induction and activate the transcription of epiblast-related genes during early germ cell differentiation (Fig. 7E). Our study should provide insights into the mechanism of germ cell differentiation and new transcription factor combinations to enhance germ cell generation.
DISCUSSION
Studying the mechanisms and regulatory factors of germ cell fate specification is necessary to improving the efficiency of in vitro germ cell production and developing effective strategies to combat genetic diseases. The understanding of human PGC specification has relied heavily on studies using murine models, such as in vitro mouse PGC specification from mESCs (Hayashi et al., 2018). Many transcription factors including several core pluripotency genes are important in both human and mouse PGC development (Kehler et al., 2004; Irie et al., 2015; Fang et al., 2018). For instance, OCT4/Oct4 can target to genes important for PGC development (e.g., Stella, BlIMP1, NANOS2) and is essential for germ cell lineage determination (Kehler et al., 2004; van den Berg et al., 2008; Murakami et al., 2016; Fang et al., 2018). By carrying out genome-wide protein-protein interaction screens of four core pluripotency factors and selecting overlapping candidates for further analysis, we sought to identify genes that promote PGC specification in vitro. Although Stella is not essential for PGC development, its upregulation may help maintain DNA hypomethylation in hypomethylated PGCs (Payer et al., 2003; Nakamura et al., 2007; Han et al., 2018, 2019; Li et al., 2018; Mulholland et al., 2020). In this study, we used Stella expression as a reporter to assess whether candidates obtained from BiFC screens in human cells could promote EpiLC induction. Several genes proved highly efficient at inducing EpiLC formation when overexpressed in mESCs. In particular, we showed that two BEND/Bend family members—Bend5 and Bend4—are sequence-specific DNA-binding proteins that could synergistically promote EpiLC induction from mESCs. BEND/Bend family proteins are found in a wide array of organisms (Abhiman et al., 2008). Further studies into these new functions of the BEND/Bend family, such as transcriptional control and chromatin boundary demarcation, should provide new insights into the mechanisms of germ cell differentiation and alternative strategies for enhancing human PGC specification and PGC induction in vitro.
Germline development undergoes epigenetic reprogramming that includes changes in DNA methylation, histone modification, and chromatin remodeling, which ultimately leads to transcriptional activation/repression (Guibert et al., 2012; Kurimoto et al., 2015; Magaraki et al., 2017; Nakaki et al., 2013). For in vitro induction of mouse PGCLCs, EpiLC induction and subsequent generation of Stella/Blimp1 double positive PGCs (Hayashi et al., 2011; Nakaki et al., 2013) are concomitant with DNA demethylation of imprint loci and PGC-related genes (Guibert et al., 2012; Nakaki et al., 2013; Gkountela et al., 2015; Miyoshi et al., 2016; Tang et al., 2016). In previous studies, DNA methylation change on H19 in PGCLCs inducted using Blimp1, Prdm14 and Tfap2c was relatively small compared to EpiLCs (44.7% vs. 37.5%) (Nakaki et al., 2013). Here, we found that overexpression of Bend5 led to dramatic increases in DNA demethylation of both imprint loci (H19 and Igf2r, ~3-fold) and at the Stella locus (~10 fold) during EpiLC induction, which were coupled with increased Tet1 recruitment. During somatic cell reprogramming, Tet1 can activate germline regulatory genes (Bartoccetti et al., 2020). In PGCs, Tet1 appears to play a more limited role in DNA demethylation during PGC specification, mainly during late stages of germ cell development (Yamaguchi et al., 2013; Hill et al., 2018). In mESCs, Tet1 may be targeted to the Stella locus for active demethylation (Mulholland et al., 2020). In line with this, we observed increased Tet1 recruitment at the Stella locus in Bend5 and Bend4-expressing mESCs during EpiLC induction. Collectively, our data support the model that Bend5 and Bend4 along with Tet1 may promote active DNA demethylation during mESC differentiation towards germ cells.
The binding motifs of the BEN domains of Bend5 and Bend4 appear to be different from that of Insv (Dai et al., 2013; Fedotova et al., 2019), which may help explain how they target to different genomic regions and mediate different functions. Bend5 and Bend4 can both target to PGC-related genes, whose binding patterns shift upon EpiLC induction. During PGC specification, expression of germline genes (e.g., Blimp1 and T) appears correlated with low H3K27me3 and high H3K27ac levels, consistent with active/repressed chromatin re-organization (Barski et al., 2007; Kurimoto et al., 2015; Liu et al., 2016; Magaraki et al., 2017). With the global loss of H3K9me2 and DNA demethylation in PGC development, there is a genome-wide change in open/closed chromatin (Kurimoto et al., 2015). We provide evidence here that Bend5 and Bend4 may act as boundary factors of open-closed chromatin and upregulate the expression of genes such as Stella after EpiLC induction. Bend5 and Bend4 may thus cooperatively participate in marking dynamic chromatin boundaries during early PGC development. Probing further into the activities and mechanisms of these factors should provide new insights into the interplay between transcriptional control and chromatin boundary in germ cell differentiation.
MATERIALS AND METHODS
Vectors, cell lines, and antibodies
cDNAs encoding full-length human BEND5 were cloned into a retrovirus vector (EF1α promoter and Flag-HA c-terminal tag), while mouse Bend5, Bend4, and their truncation mutants were cloned into a lentivirus vector or pDEST27 (Invitrogen) for mammalian expression. cDNAs encoding mouse Oct4 and Sox2 were cloned into a MSCV-based retroviral vector (HA-Flag c-terminal tagging) or pDEST27.
Stella-GFP reporter mESCs (gift from Dr. Yuan Wang, East Normal University, China) were maintained on MEF feeder cells in Dulbecco’s modified Eagle’s medium supplemented with 15% fetal calf serum (Hyclone, Logan, UT, US), 0.1 mmol/L NEAA, 1 mmol/L sodium pyruvate, 0.1 mmol/L β-mercaptoethanol, 100 U/mL penicillin, 0.1 mg/mL streptomycin, 2 mmol/L L-glutamine, and LIF (1000 U/mL, Millipore, Billerica, MA). HTC75 and HEK293T cells were cultured in Dulbecco’s modified Eagle’s medium with high glucose supplemented with 15% fetal calf serum (Hyclone, Logan, UT, US).
Antibodies used in this study: anti-Flag (Sigma F7425 for ChIP and ChIPseq; ANTI-FLAG M2 Affinity beads (A2220) for IP, Abmart M20008 (Mouse) and Sigma F7425 (Rabbit) for WB), anti-CTCF (Active Motif, 61311), anti-Oct4 (Santa Cruz, sc5279), anti-Tet1 (Active Motif, 61443), anti-HA (Sigma, H3663), anti-GAPDH (ABclonal, AC027), mouse polyclonal anti-GST (Abmart, M20007), rabbit polyclonal IgG (Millipore, 12-370).
Sequences for Bend5 shRNAs and all primers and oligonucleotide are listed in Table S3.
Arrayed genome-wide bi-molecular fluorescence complementation (BiFC) screens
The arrayed BiFC screening strategy and data analysis procedures were as previously described (Lee et al., 2011). Briefly, HTC75 cells stably expressing YFPn-tagged (amino acids 1–155 of Venus YFP) bait proteins (OCT4, NANOG, SOX2, or KLF4) were generated and seeded into 96-well plates before being infected with retroviruses encoding YFPc-tagged (amino acids 153–239 of Venus YFP) prey library. Fluorescence complementation was determined by flow cytometry and data were analyzed by CytoArray, which calculates weighted positive ratios (WPR) based on fluorescence signals. Of the potential interacting partners from all four baits (Table S1), 93 candidates were chosen for further analysis (Table S2).
In vitro EpiLC induction and flow cytometry analysis and cell sorting (FACS)
EpiLC induction was performed as previously described (Hayashi et al., 2011). Briefly, mESCs that were maintained on MEF feeder cells in mESC medium were transferred to feeder-free KSR medium (Knock-out Dulbecco’s modified Eagle’s medium with 10% KnockOut™ Serum Replacement (KSR) (ThermoFisher, 10828028, US), 0.1 mmol/L NEAA, 1 mmol/L sodium pyruvate, 0.1 mmol/L β-mercaptoethanol, 100 U/mL penicillin, 0.1 mg/mL streptomycin, 2 mmol/L L-glutamine, LIF and 2i (CHIR99021 3 µmol/L; PD0325901 1 µmol/L)) and cultured for two passages before being induced to EpiLCs with N2B27 medium (KSR (1%), Activin A (20 ng/mL), bFGF (12 ng/mL), and 2i) for two days with medium change daily. EpiLCs were collected and filtered on Day 2 for flow cytometry analysis. FACS sorting was performed with a FACSAria or FACSAriaIII (BD) cell sorter and results were analyzed with FACSDiva (BD) or Flowjo (Tree Star) software.
Primordial germ cells like cells (PGCLCs) Induction and flow cytometry analysis
PGCLCs induction was performed as previously described (Hayashi et al., 2011). EpiLCs (~103) were seeded in U-bottom 96-well plates with low cell binding surface (NUNC), and cultured in serum-free medium (GMEM [Invitrogen] with 15% KSR, 0.1 mmol/L NEAA, 1 mmol/L sodium pyruvate, 0.1 mmol/L β-mercaptoethanol, 2 mmol/L L-glutamine, LIF (1000 U/mL; Invitrogen), BMP4 (500 ng/mL; R&D Systems), BMP8b (500 ng/mL; R&D Systems), SCF (100 ng/mL; R&D Systems), and EGF (50 ng/mL; R&D Systems) for six days with medium change every day. PGCLCs was collected and filtered, Stella-GFP positive or Blimp1-mVenus (BV) and Stella-ECFP (SC) positive cells were detected with the FITC and AmCyan Horizon V500 channel, respectively. The results were analyzed with FACSDiva (BD) or Flowjo (Tree Star) software.
GST pull down
To detect the interaction between ectopic expressed Bend5 and pluripotent factors (Oct4 and Sox2), HEK393T cells were transfected with HA-Bend5 and GST-Oct4 (or GST-Sox2). GST pull down was performed with GST beads (Glutathione SepharoseTM 4B, 17-0756-01, GE healthcare), followed by Western blot with rabbit anti-HA and mouse anti-GST antibodies.
Co-immunoprecipitation (Co-IP)
To detect Bend5 and Tet1 interaction, HEK293T cells were transfected with Flag-Bend5 and HA-Tet1. Immunoprecipitation was performed with rabbit anti-Tet1 antibody followed by Western blot with HA and Flag antibodies. To detect Bend4 and Oct4 interaction, HEK293T cells were transfected with Flag-Bend4 and GST-Oct4. Immunoprecipitation was performed with mouse anti-FLAG antibody followed by Western blot with rabbit Flag and mouse GST antibodies.
GST tagged recombination protein purification and Electrophoretic gel-mobility shift (EMSA) assays
GST-Bend5 and GST-Bend5ΔBEN plasmid was transformed into E. coli strain BL21, and the fusion protein expression was induced by adding isopropyl thio-β-D-galactosidase (IPTG) in 1 mmol/L final concentration at 37 °C. After 2 h, cells were collected and the cell pellets were dissolved, followed by sonicator. Cells lysis were centrifuged at maximum speed, the supernatant and GST beads (Glutathione SepharoseTM 4B, 17-0756-01, GE healthcare) incubation for 2 h at 4 °C, followed by wash, elution by specific buffer and SDS-PAFE detection. For EMSA, purified GST-tagged proteins (1 µg) were incubated with appropriate oligonucleotides (Table S3) (0.5 µg) in binding buffer (10 mmol/L Tris-Cl, pH 7.5, 50 mmol/L NaCl, 5 mmol/L MgCl2, 1 mmol/L DTT, 0.05% NP-40, 5% glycerol, 50 ng/μL poly (dI-dC)) for 20 min at room temperature. The reaction mixtures were then analyzed on agarose gels.
Immunofluorescent staining
To detect the cell localization of Flag-Bend5 and Bend5∆BEN, the stably expressed cells were seeded on 15 mm microscope cover glasses. For immunofluorescent staining, cells were fixed with 4% paraformaldehyde, permeabilized (5% Triton-X, 20 mmol/L HEPES, 3 mmol/L MgCl2·6H2O, 300 mmol/L Sucrose), blocked (3% goat serum, 0.1% BSA in PBS) and incubated with rabbit anti-Flag antibody (GenScript A00170-40). Then they were stained with Alexa Fluor conjugated secondary antibodies Goat anti-Rabbit IgG (H + L). Nuclear staining was performed with DAPI.
Reverse transcription and qPCR
Cells were dissolved by Trizol (Invitrogen) and total RNA was isolated using phenol chloroform. Following cDNA synthesis was performed with PrimeScript™ RT Reagent Kit (TaKaRa), and RT-qPCR was performed using GoTaq® qPCR Master Mix (Promega) and qPCR primers by ABI Step One Plus Real-Time PCR System. Gene expression data were normalized with Ct values from day 0 (D0) samples.
Bisulfite sequencing and data analysis
For bisulfite sequencing, genomic DNA was extracted using the DNeasy Mini Kit (Qiagen) and processed using the EpiTect Bisulfite Kit (Qiagen) for bisulfite conversion. PCR amplification using specific primers, rTaq enzyme treatment, pEASYT1 cloning (TransGen Biotech) and sequencing were then performed as described previously (Lucifero et al., 2002). After bisulfite treatment, the gained DNA sequence was blasted with original sequence (unmethylated CG is changed to TG, methylated CG is not changed). We examined a total of 7 CpG sites within intron2 in Igf2r (GeneBank acc. no. L06446), 16 sites in the 5′ end of H19 (GeneBank acc. no. U19619). Primer sequences are listed in the Table S3.
Knocking out Bend4 in Bend5-expressing mESCs by CRISPR/Cas9
Bend5-expressing Stella-GFP mESCs were transduced with lentiviruses (pLenti-based vector) encoding Bend4 gRNA sequences targeting the BEN domain of Bend4 and selected with blasticidin. The px330-Cas9 plasmid (1 μg) (Addgene) was then electroporated into these cells to induce knockout. Cells were maintained in blasticidin for another 10 days. Single clones were subsequently isolated and verified for successful knockout by T7 endonuclease I (T7E1) assays and Sanger sequencing. Bend4 gRNA: 5′-CCGCCGCCCGTCCTTCTTGG (AGG).
RNA-seq and data analysis
The cells were harvested and dissolved in Trizol for total RNA extraction and treated with DNase I (Ambion) to remove any potential contaminated DNA fraction. The following library generation and sequencing were conducted by Ruibo Biotechnology Co., Ltd in Guangzhou. The raw data were used to map the RNA-seq reads to the UCSC mouse genes (mm10). Cuffdiff (version 2.0.2) was employed to calculate expression abundance measured as Fragment Per Kilobase per Million mapped fragments (FPKM) and identify the DE genes (fold change > 2) (Table S4). The consistency degree of gene expression profiles was measured by Pearson correlation coefficient and visualized by scatter plots. Pearson correlation analysis was performed based on gene expression levels (FPKM) and visualized by heatmaps.
Chromatin immunoprecipitation followed by sequencing (ChIP-seq) and data analysis
ChIP-seq was performed as previously described (Yao et al., 2018). Briefly, the cells (2 × 107) were collected, then crosslinked by 1% Formaldehyde solution (Sigma-Aldrich F8775) for 10 min and quenched by final concentration 250 mmol/L glycine solution. The cells were lysed in ChIP lysis buffer (50 mmol/L Tris pH 8.0, 10 mmol/L EDTA, 1%SDS, protein inhibitor cocktail) and sonicated (Bioruptor for 30 cycles of on (30 s)/off (30 s)), then crosslinking. Cell lysis was dialyzed in ChIP dilution buffer (0.01% SDS, 1.1% Triton X-100, 1.2 mmol/L EDTA, 16.7 mmol/L Tris-HCl pH 8.0, 167 mmol/L NaCl) at 4 °C for 4 h before incubation with the appropriate antibodies. Each reaction was sequentially washed with low salt buffer (0.1% SDS, 1% Triton X-100, 2 mmol/L EDTA, 20 mmol/L Tris-HCl pH 8.0, 150 mmol/L NaCl ), high salt buffer (0.1% SDS, 1% Triton X-100, 2 mmol/L EDTA, 20 mmol/L Tris-HCl pH 8.0, 500 mmol/L NaCl), LiCl buffer (0.25 mol/L LiCl, 1% Igepal, 1 mmol/L EDTA, 10 mmol/L Tris-HCl pH 8.0, 1% deochyacid) and TE buffer (10 mmol/L Tris-HCl pH 8.0, 1 mmol/L EDTA) at 4 °C. Co-precipitated DNA was recovered using Mini-Elute PCR Purification Kit (28004, Qiagen). About 10 ng IPed DNA and input DNA measured by Qubit Fluorometer (Invitrogen) were used to construct DNA library. The following library generation and sequencing were conducted by Ruibo Biotechnology Co., Ltd in Guangzhou.
In this study, anti-Flag, Tet1, and CTCF ChIP-seq experiments were performed. Oct4 ChIP-seq data (GSE56098, GSM1355154, GSM1355155, GSM1355167) were download from the NCBI website. All raw data were uploaded to Galaxy server (http://usegalaxy.org) to perform reads quality check by the FastQC software integrated into the tool shed of the Galaxy server home page (Afgan et al., 2018). Low-quality reads and Illumina universal adapters were removed by Trim Galore. Then control input and ChIPed clean data were respectively mapped by Bowtie2 to the built-in index of mm10 mouse reference genome. The Bam files obtained from the Bowtie2 software were filtered by the Bam/Sam filter software to remove low-quality data (<20) and those mapped to the mitochondrial genome. To better visualize the results, the filtered Bam files were converted to the bigWig file format with bin size 5 by the bamCoverage software and displayed in the Integrative Genomic Browser (IGB). All tracks were selected and synchronized for the same Y-axis value (no expression) which demonstrated the lower and upper range values for any base position in the current view. The results of transcript factor binding events was summarized by the MACS2 software. The result files with bed format were obtained from MACS2 on Bam files with the threshold of FDR > 0.05 (False Discovery Rate). The last annotation step was performed in the Linux system by the Homer software and gene ontology analysis was conducted through the MEME website.
Assay for transposase-accessible chromatin using sequencing (ATAC-seq) and data analysis
ATAC-seq was performed as previously described (Buenrostro et al., 2013). Stella-GFP positive EpiLCs were sorted after EpiLC induction D2, about 1 × 104 cells were collected and centrifugation at 500 ×g for 5 min, which was followed by a wash using cold PBS and centrifugation at 500 ×g for 5 min. The cells were lysed using 50 µL of cold lysis buffer (10 mmol/L Tris-HCl, pH 7.4, 10 mmol/L NaCl, 3 mmol/L MgCl2 and 0.2% IGEPAL CA-630) for 10 min on ice, then nuclei were collected at 500 ×g for 10 min. The pellet was immediately resuspended in the transposase reaction mix (Vazyme, TD502 kit, 20 µL each reaction), then the reaction was carried out for 30 min at 37 °C. The sample was purified using 40 µL magnetic beads (Beckman Coulter AMPure XP A63881). Following purification, we amplified library fragments using Vazyme, TD502 kit (50 µL each reaction), using the following PCR conditions: 72 °C for 3 min; 98 °C for 30 s; and thermocycling at 98 °C for 15 s, 60 °C for 30 s and 72 °C for 30 s for 15 cycles, then 72 °C for 5 min. Following PCR, the libraries were purified using 60 µL magnetic beads. The purified libraries were detected by agarose gel electrophoresis and final concentration was detected by Qubit 3.0 (Invitrogen). The sequenced insert size was between 40 bp and 1 kb with a mean of ~120 bp. Following library QC and quantification, sequencing was performed by Guangzhou RiboBio Co., Ltd.
The reads were aligned to mm10 using Bowtie2 and only unique aligned reads were collected. For all data, duplicates were removed using Picard. Then mitochondrial sequences were removed and peaks were called using dfilter (Kumar et al., 2013). BigWig files were produced using genomeCoverageBed and displayed in the Integrative Genomic Browser (IGB).
REFERENCES
Abhiman S, Iyer LM, Aravind L (2008) BEN: a novel domain in chromatin factors and DNA viral proteins. Bioinformatics 24:458–461
Afgan E, Baker D, Batut B, van den Beek M, Bouvier D, Cech M, Chilton J, Clements D, Coraor N, Gruning BA et al (2018) The Galaxy platform for accessible, reproducible and collaborative biomedical analyses: 2018 update. Nucleic Acids Res 46:W537–W544
Arzate-Mejia, R.G., Recillas-Targa, F., and Corces, V.G. (2018). Developing in 3D: the role of CTCF in cell differentiation. Development 145.
Bailey TL (2011) DREME: motif discovery in transcription factor ChIP-seq data. Bioinformatics 27:1653–1659
Bailey TL, Machanick P (2012) Inferring direct DNA binding from ChIP-seq. Nucleic Acids Res 40:e128
Barski A, Cuddapah S, Cui K, Roh TY, Schones DE, Wang Z, Wei G, Chepelev I, Zhao K (2007) High-resolution profiling of histone methylations in the human genome. Cell 129:823–837
Beagan JA, Phillips-Cremins JE (2020) On the existence and functionality of topologically associating domains. Nat Genet 52:8–16
Beagan JA, Duong MT, Titus KR, Zhou L, Cao Z, Ma J, Lachanski CV, Gillis DR, Phillips-Cremins JE (2017) YY1 and CTCF orchestrate a 3D chromatin looping switch during early neural lineage commitment. Genome Res 27:1139–1152
Bortvin A, Goodheart M, Liao M, Page DC (2004) Dppa3/Pgc7/stella is a maternal factor and is not required for germ cell specification in mice. BMC Dev Biol 4:2
Buecker C, Srinivasan R, Wu Z, Calo E, Acampora D, Faial T, Simeone A, Tan M, Swigut T, Wysocka J (2014) Reorganization of enhancer patterns in transition from naive to primed pluripotency. Cell Stem Cell 14:838–853
Buenrostro JD, Giresi PG, Zaba LC, Chang HY, Greenleaf WJ (2013) Transposition of native chromatin for fast and sensitive epigenomic profiling of open chromatin, DNA-binding proteins and nucleosome position. Nat Methods 10:1213–1218
Cuddapah S, Jothi R, Schones DE, Roh TY, Cui K, Zhao K (2009) Global analysis of the insulator binding protein CTCF in chromatin barrier regions reveals demarcation of active and repressive domains. Genome Res 19:24–32
Dai Q, Ren A, Westholm JO, Serganov AA, Patel DJ, Lai EC (2013) The BEN domain is a novel sequence-specific DNA-binding domain conserved in neural transcriptional repressors. Genes Dev 27:602–614
Dai Q, Ren A, Westholm JO, Duan H, Patel DJ, Lai EC (2015) Common and distinct DNA-binding and regulatory activities of the BEN-solo transcription factor family. Genes Dev 29:48–62
de Sousa Lopes SM, Roelen BA, Monteiro RM, Emmens R, Lin HY, Li E, Lawson KA, Mummery CL (2004) BMP signaling mediated by ALK2 in the visceral endoderm is necessary for the generation of primordial germ cells in the mouse embryo. Genes Dev 18:1838–1849
Dixon JR, Selvaraj S, Yue F, Kim A, Li Y, Shen Y, Hu M, Liu JS, Ren B (2012) Topological domains in mammalian genomes identified by analysis of chromatin interactions. Nature 485:376–380
Dixon JR, Gorkin DU, Ren B (2016) Chromatin domains: the unit of chromosome organization. Mol Cell 62:668–680
Duggal G, Heindryckx B, Warrier S, O’Leary T, Van der Jeught M, Lierman S, Vossaert L, Deroo T, Deforce D, Chuva de Sousa Lopes SM et al (2013) Influence of activin A supplementation during human embryonic stem cell derivation on germ cell differentiation potential. Stem Cells Dev 22:3141–3155
Duggal G, Heindryckx B, Warrier S, Taelman J, Van der Jeught M, Deforce D, de Sousa C, Lopes S, De Sutter P (2015) Exogenous supplementation of Activin A enhances germ cell differentiation of human embryonic stem cells. Mol Hum Reprod 21:410–423
Fang F, Angulo B, Xia N, Sukhwani M, Wang Z, Carey CC, Mazurie A, Cui J, Wilkinson R, Wiedenheft B et al (2018) A PAX5-OCT4-PRDM1 developmental switch specifies human primordial germ cells. Nat Cell Biol 20:655–665
Fedotova A, Clendinen C, Bonchuk A, Mogila V, Aoki T, Georgiev P, Schedl P (2019) Functional dissection of the developmentally restricted BEN domain chromatin boundary factor Insensitive. Epigenet Chromatin 12:2
Fischer G, Schmidt C, Opitz J, Cully Z, Kuhn K, Poschl E (1993) Identification of a novel sequence element in the common promoter region of human collagen type IV genes, involved in the regulation of divergent transcription. Biochem J 292(Pt 3):687–695
Gaszner M, Felsenfeld G (2006) Insulators: exploiting transcriptional and epigenetic mechanisms. Nat Rev Genet 7:703–713
Gkountela S, Zhang KX, Shafiq TA, Liao WW, Hargan-Calvopina J, Chen PY, Clark AT (2015) DNA Demethylation dynamics in the human prenatal germline. Cell 161:1425–1436
Guibert S, Forne T, Weber M (2012) Global profiling of DNA methylation erasure in mouse primordial germ cells. Genome Res 22:633–641
Hackett JA, Sengupta R, Zylicz JJ, Murakami K, Lee C, Down TA, Surani MA (2013) Germline DNA demethylation dynamics and imprint erasure through 5-hydroxymethylcytosine. Science 339:448–452
Hajkova P, Erhardt S, Lane N, Haaf T, El-Maarri O, Reik W, Walter J, Surani MA (2002) Epigenetic reprogramming in mouse primordial germ cells. Mech Dev 117:15–23
Han L, Ren C, Li L, Li X, Ge J, Wang H, Miao YL, Guo X, Moley KH, Shu W et al (2018) Publisher correction: embryonic defects induced by maternal obesity in mice derive from Stella insufficiency in oocytes. Nat Genet 50:768
Han L, Ren C, Zhang J, Shu W, Wang Q (2019) Differential roles of Stella in the modulation of DNA methylation during oocyte and zygotic development. Cell Discovery 5:9
Handoko L, Xu H, Li G, Ngan CY, Chew E, Schnapp M, Lee CW, Ye C, Ping JL, Mulawadi F et al (2011) CTCF-mediated functional chromatin interactome in pluripotent cells. Nat Genet 43:630–638
Hayashi K, Ohta H, Kurimoto K, Aramaki S, Saitou M (2011) Reconstitution of the mouse germ cell specification pathway in culture by pluripotent stem cells. Cell 146:519–532
Hayashi K, Ogushi S, Kurimoto K, Shimamoto S, Ohta H, Saitou M (2012) Offspring from oocytes derived from in vitro primordial germ cell-like cells in mice. Science 338:971–975
Hayashi M, Kawaguchi T, Durcova-Hills G, Imai H (2018) Generation of germ cells from pluripotent stem cells in mammals. Reprod Med Biol 17:107–114
Hernandez-Hernandez A, Lilienthal I, Fukuda N, Galjart N, Hoog C (2016) CTCF contributes in a critical way to spermatogenesis and male fertility. Sci Rep 6:28355
Hikabe O, Hamazaki N, Nagamatsu G, Obata Y, Hirao Y, Hamada N, Shimamoto S, Imamura T, Nakashima K, Saitou M et al (2016) Reconstitution in vitro of the entire cycle of the mouse female germ line. Nature 539:299–303
Hill PWS, Leitch HG, Requena CE, Sun Z, Amouroux R, Roman-Trufero M, Borkowska M, Terragni J, Vaisvila R, Linnett S et al (2018) Epigenetic reprogramming enables the transition from primordial germ cell to gonocyte. Nature 555:392–396
Hu CD, Kerppola TK (2003) Simultaneous visualization of multiple protein interactions in living cells using multicolor fluorescence complementation analysis. Nat Biotechnol 21:539–545
Irie N, Weinberger L, Tang WW, Kobayashi T, Viukov S, Manor YS, Dietmann S, Hanna JH, Surani MA (2015) SOX17 is a critical specifier of human primordial germ cell fate. Cell 160:253–268
Ji X, Dadon DB, Powell BE, Fan ZP, Borges-Rivera D, Shachar S, Weintraub AS, Hnisz D, Pegoraro G, Lee TI et al (2016) 3D chromosome regulatory landscape of human pluripotent cells. Cell Stem Cell 18:262–275
Kagiwada S, Kurimoto K, Hirota T, Yamaji M, Saitou M (2013) Replication-coupled passive DNA demethylation for the erasure of genome imprints in mice. EMBO J 32:340–353
Kehler J, Tolkunova E, Koschorz B, Pesce M, Gentile L, Boiani M, Lomeli H, Nagy A, McLaughlin KJ, Scholer HR et al (2004) Oct4 is required for primordial germ cell survival. EMBO Rep 5:1078–1083
Kumar V, Muratani M, Rayan NA, Kraus P, Lufkin T, Ng HH, Prabhakar S (2013) Uniform, optimal signal processing of mapped deep-sequencing data. Nat Biotechnol 31:615–622
Kurimoto K, Yabuta Y, Ohinata Y, Shigeta M, Yamanaka K, Saitou M (2008a) Complex genome-wide transcription dynamics orchestrated by Blimp1 for the specification of the germ cell lineage in mice. Genes Dev 22:1617–1635
Kurimoto K, Yamaji M, Seki Y, Saitou M (2008b) Specification of the germ cell lineage in mice: a process orchestrated by the PR-domain proteins, Blimp1 and Prdm14. Cell Cycle 7:3514–3518
Kurimoto K, Yabuta Y, Hayashi K, Ohta H, Kiyonari H, Mitani T, Moritoki Y, Kohri K, Kimura H, Yamamoto T et al (2015) Quantitative dynamics of chromatin remodeling during germ cell specification from mouse embryonic stem cells. Cell Stem Cell 16:517–532
Lee J, Inoue K, Ono R, Ogonuki N, Kohda T, Kaneko-Ishino T, Ogura A, Ishino F (2002) Erasing genomic imprinting memory in mouse clone embryos produced from day 11.5 primordial germ cells. Development 129:1807–1817
Lee OH, Kim H, He Q, Baek HJ, Yang D, Chen LY, Liang J, Chae HK, Safari A, Liu D et al (2011) Genome-wide YFP fluorescence complementation screen identifies new regulators for telomere signaling in human cells. Mol Cell Proteom: MCP 10:M110 001628
Li Y, Zhang Z, Chen J, Liu W, Lai W, Liu B, Li X, Liu L, Xu S, Dong Q et al (2018) Stella safeguards the oocyte methylome by preventing de novo methylation mediated by DNMT1. Nature 564:136–140
Liu L, Mao SQ, Ray C, Zhang Y, Bell FT, Ng SF, Xu GL, Li X (2015) Differential regulation of genomic imprinting by TET proteins in embryonic stem cells. Stem Cell Res 15:435–443
Liu X, Wang C, Liu W, Li J, Li C, Kou X, Chen J, Zhao Y, Gao H, Wang H et al (2016) Distinct features of H3K4me3 and H3K27me3 chromatin domains in pre-implantation embryos. Nature 537:558–562
Lobanenkov VV, Nicolas RH, Adler VV, Paterson H, Klenova EM, Polotskaja AV, Goodwin GH (1990) A novel sequence-specific DNA binding protein which interacts with three regularly spaced direct repeats of the CCCTC-motif in the 5’-flanking sequence of the chicken c-myc gene. Oncogene 5:1743–1753
Loh YH, Wu Q, Chew JL, Vega VB, Zhang W, Chen X, Bourque G, George J, Leong B, Liu J et al (2006) The Oct4 and Nanog transcription network regulates pluripotency in mouse embryonic stem cells. Nat Genet 38:431–440
Lucifero D, Mertineit C, Clarke HJ, Bestor TH, Trasler JM (2002) Methylation dynamics of imprinted genes in mouse germ cells. Genomics 79:530–538
Magaraki A, van der Heijden G, Sleddens-Linkels E, Magarakis L, van Cappellen WA, Peters A, Gribnau J, Baarends WM, Eijpe M (2017) Silencing markers are retained on pericentric heterochromatin during murine primordial germ cell development. Epigenet Chromatin 10:11
Miyoshi N, Stel JM, Shioda K, Qu N, Odajima J, Mitsunaga S, Zhang X, Nagano M, Hochedlinger K, Isselbacher KJ et al (2016) Erasure of DNA methylation, genomic imprints, and epimutations in a primordial germ-cell model derived from mouse pluripotent stem cells. Proc Natl Acad Sci USA 113:9545–9550
Moore JM, Rabaia NA, Smith LE, Fagerlie S, Gurley K, Loukinov D, Disteche CM, Collins SJ, Kemp CJ, Lobanenkov VV et al (2012) Loss of maternal CTCF is associated with peri-implantation lethality of Ctcf null embryos. PLoS ONE 7:e34915
Mulholland CB, Nishiyama A, Ryan J, Nakamura R, Yigit M, Gluck IM, Trummer C, Qin W, Bartoschek MD, Traube FR et al (2020) Recent evolution of a TET-controlled and DPPA3/STELLA-driven pathway of passive DNA demethylation in mammals. Nat Commun 11:5972
Murakami K, Gunesdogan U, Zylicz JJ, Tang WWC, Sengupta R, Kobayashi T, Kim S, Butler R, Dietmann S, Surani MA (2016) NANOG alone induces germ cells in primed epiblast in vitro by activation of enhancers. Nature 529:403–407
Nakaki F, Hayashi K, Ohta H, Kurimoto K, Yabuta Y, Saitou M (2013) Induction of mouse germ-cell fate by transcription factors in vitro. Nature 501:222–226
Nakamura T, Arai Y, Umehara H, Masuhara M, Kimura T, Taniguchi H, Sekimoto T, Ikawa M, Yoneda Y, Okabe M et al (2007) PGC7/Stella protects against DNA demethylation in early embryogenesis. Nat Cell Biol 9:64–71
Ohinata Y, Payer B, O’Carroll D, Ancelin K, Ono Y, Sano M, Barton SC, Obukhanych T, Nussenzweig M, Tarakhovsky A et al (2005) Blimp1 is a critical determinant of the germ cell lineage in mice. Nature 436:207–213
Okamura D, Tokitake Y, Niwa H, Matsui Y (2008) Requirement of Oct3/4 function for germ cell specification. Dev Biol 317:576–584
Okashita N, Kumaki Y, Ebi K, Nishi M, Okamoto Y, Nakayama M, Hashimoto S, Nakamura T, Sugasawa K, Kojima N et al (2014) PRDM14 promotes active DNA demethylation through the ten-eleven translocation (TET)-mediated base excision repair pathway in embryonic stem cells. Development 141:269–280
Pastor WA, Aravind L, Rao A (2013) TETonic shift: biological roles of TET proteins in DNA demethylation and transcription. Nat Rev Mol Cell Biol 14:341–356
Payer B, Saitou M, Barton SC, Thresher R, Dixon JP, Zahn D, Colledge WH, Carlton MB, Nakano T, Surani MA (2003) Stella is a maternal effect gene required for normal early development in mice. Curr Biol: CB 13:2110–2117
Payer B, de Sousa C, Lopes SM, Barton SC, Lee C, Saitou M, Surani MA (2006) Generation of stella-GFP transgenic mice: a novel tool to study germ cell development. Genesis 44:75–83
Plasschaert RN, Vigneau S, Tempera I, Gupta R, Maksimoska J, Everett L, Davuluri R, Mamorstein R, Lieberman PM, Schultz D et al (2014) CTCF binding site sequence differences are associated with unique regulatory and functional trends during embryonic stem cell differentiation. Nucleic Acids Res 42:774–789
Pope BD, Ryba T, Dileep V, Yue F, Wu W, Denas O, Vera DL, Wang Y, Hansen RS, Canfield TK et al (2014) Topologically associating domains are stable units of replication-timing regulation. Nature 515:402–405
Radzisheuskaya A, Chia Gle B, dos Santos RL, Theunissen TW, Castro LF, Nichols J, Silva JC (2013) A defined Oct4 level governs cell state transitions of pluripotency entry and differentiation into all embryonic lineages. Nat Cell Biol 15:579–590
Saitou M, Yamaji M (2010) Germ cell specification in mice: signaling, transcription regulation, and epigenetic consequences. Reproduction 139:931–942
Saitou M, Kagiwada S, Kurimoto K (2012) Epigenetic reprogramming in mouse pre-implantation development and primordial germ cells. Development 139:15–31
Senft AD, Bikoff EK, Robertson EJ, Costello I (2019) Genetic dissection of Nodal and Bmp signalling requirements during primordial germ cell development in mouse. Nat Commun 10:1089
Smith ZD, Meissner A (2013) DNA methylation: roles in mammalian development. Nat Rev Genet 14:204–220
Takahashi K, Yamanaka S (2006) Induction of pluripotent stem cells from mouse embryonic and adult fibroblast cultures by defined factors. Cell 126:663–676
Tang WW, Kobayashi T, Irie N, Dietmann S, Surani MA (2016) Specification and epigenetic programming of the human germ line. Nat Rev Genet 17:585–600
van den Berg DL, Zhang W, Yates A, Engelen E, Takacs K, Bezstarosti K, Demmers J, Chambers I, Poot RA (2008) Estrogen-related receptor beta interacts with Oct4 to positively regulate Nanog gene expression. Mol Cell Biol 28:5986–5995
van den Berg DL, Snoek T, Mullin NP, Yates A, Bezstarosti K, Demmers J, Chambers I, Poot RA (2010) An Oct4-centered protein interaction network in embryonic stem cells. Cell Stem Cell 6:369–381
Verma N, Pan H, Dore LC, Shukla A, Li QV, Pelham-Webb B, Teijeiro V, Gonzalez F, Krivtsov A, Chang CJ et al (2018) TET proteins safeguard bivalent promoters from de novo methylation in human embryonic stem cells. Nat Genet 50:83–95
Vincent SD, Dunn NR, Sciammas R, Shapiro-Shalef M, Davis MM, Calame K, Bikoff EK, Robertson EJ (2005) The zinc finger transcriptional repressor Blimp1/Prdm1 is dispensable for early axis formation but is required for specification of primordial germ cells in the mouse. Development 132:1315–1325
Vincent JJ, Huang Y, Chen PY, Feng S, Calvopina JH, Nee K, Lee SA, Le T, Yoon AJ, Faull K et al (2013) Stage-specific roles for tet1 and tet2 in DNA demethylation in primordial germ cells. Cell Stem Cell 12:470–478
von Meyenn F, Berrens RV, Andrews S, Santos F, Collier AJ, Krueger F, Osorno R, Dean W, Rugg-Gunn PJ, Reik W (2016) Comparative principles of DNA methylation reprogramming during human and mouse in vitro primordial germ cell specification. Dev Cell 39:104–115
Wan LB, Pan H, Hannenhalli S, Cheng Y, Ma J, Fedoriw A, Lobanenkov V, Latham KE, Schultz RM, Bartolomei MS (2008) Maternal depletion of CTCF reveals multiple functions during oocyte and preimplantation embryo development. Development 135:2729–2738
Wei W, Qing T, Ye X, Liu H, Zhang D, Yang W, Deng H (2008) Primordial germ cell specification from embryonic stem cells. PLoS ONE 3:e4013
Wendt KS, Yoshida K, Itoh T, Bando M, Koch B, Schirghuber E, Tsutsumi S, Nagae G, Ishihara K, Mishiro T et al (2008) Cohesin mediates transcriptional insulation by CCCTC-binding factor. Nature 451:796–801
Williams K, Christensen J, Pedersen MT, Johansen JV, Cloos PA, Rappsilber J, Helin K (2011) TET1 and hydroxymethylcytosine in transcription and DNA methylation fidelity. Nature 473:343–348
Wongtrakoongate P, Jones M, Gokhale PJ, Andrews PW (2013) STELLA facilitates differentiation of germ cell and endodermal lineages of human embryonic stem cells. PLoS ONE 8:e56893
Wu X, Zhang Y (2017) TET-mediated active DNA demethylation: mechanism, function and beyond. Nat Rev Genet 18:517–534
Yakhkeshi S, Rahimi S, Sharafi M, Hassani SN, Taleahmad S, Shahverdi A, Baharvand H (2018) In vitro improvement of quail primordial germ cell expansion through activation of TGF-beta signaling pathway. J Cell Biochem 119:4309–4319
Yamaguchi S, Shen L, Liu Y, Sendler D, Zhang Y (2013) Role of Tet1 in erasure of genomic imprinting. Nature 504:460–464
Yamaji M, Seki Y, Kurimoto K, Yabuta Y, Yuasa M, Shigeta M, Yamanaka K, Ohinata Y, Saitou M (2008) Critical function of Prdm14 for the establishment of the germ cell lineage in mice. Nat Genet 40:1016–1022
Yao M, Zhou X, Zhou J, Gong S, Hu G, Li J, Huang K, Lai P, Shi G, Hutchins AP et al (2018) PCGF5 is required for neural differentiation of embryonic stem cells. Nat Commun 9:1463
Zhang Y, Feng XH, Derynck R (1998) Smad3 and Smad4 cooperate with c-Jun/c-Fos to mediate TGF-beta-induced transcription. Nature 394:909–913
Zhang H, Zhang X, Clark E, Mulcahey M, Huang S, Shi YG (2010) TET1 is a DNA-binding protein that modulates DNA methylation and gene transcription via hydroxylation of 5-methylcytosine. Cell Res 20:1390–1393
Zhang W, Xia W, Wang Q, Towers AJ, Chen J, Gao R, Zhang Y, Yen CA, Lee AY, Li Y et al (2016) Isoform switch of TET1 regulates DNA demethylation and mouse development. Mol Cell 64:1062–1073
Acknowledgements
We thank Dr. Dan Liu from Baylor College of Medicine for critical reading of this manuscript. We thank Dr. Jian Ren and Dr. Qi Zhao from Sun Yat-sen University for bioinformatics analysis.
ABBREVIATIONS
ATAC-seq, assay transposase-accessible chromatin with high-throughput sequencing; BEND5, BEN domain-containing protein 5; BiFC, bi-molecular fluorescence complementation; BV, Blimp1-mVenus; SC, Stella-ECFP; BVSC+ cells, Blimp1-mVenus and Stella-ECFP positive cells; SG+ or GFP+ cells, Stella-GFP positive cells; ChIP, chromatin immunoprecipitation; ChIP-seq, chromatin immunoprecipitation followed by sequencing; co-IP, co-immunoprecipitate; CTCF, CCCTC-binding factor; C4ORF27, chromosome 4 open reading frame 27; Dppa3/Stella, developmental pluripotency-associated 3; DMRs, differentially methylated regions; EpiLCs, epiblast-like cells; mESCs, mouse embryonic stem cells; EB, embryoid body; EMSA, electrophoretic gel-mobility shift; FACS, flow cytometry analysis and cell sorting; FPKM, fragment per kilobase per million mapped fragments; HOXA3, homeobox A3; KO, knockout; KLF4, kruppel like factor 4; 5mC, 5-methylcytosine; PGCs, primordial germ cells; NME7, NME/NM23 family member; Nanog, nanog homeobox; PGCLCs, PGC-like cells; qPCR, real-time polymerase chain reaction; Prdm1, PR/SET domain 1; Prdm14, PR/SET domain 14; POU5F1 or OCT4, human POU class 5 homeobox 1; Tfap2c, transcription factor AP-2 gamma; TSS, transcription start site; SOX2, SRY-box transcription factor 2; Sox3, SRY-box transcription factor 3; SSCs, spermatogonial stem cells; Tet, ten-eleven translocation; Tet1, Tet methylcytosine dioxygenase 1; Tet2, Tet methylcytosine dioxygenase 2; Thy1, Thy-1 cell surface antigen; Usp26, ubiquitin specific peptidase 26; YFP, yellow fluorescent protein; YFPN, YFP N terminal; YFPC, YFP C terminal
DECLARATIONS
This work was supported by the National Key R&D Program of China (2017YFA0102801). The National Natural Science Foundation of China (Grant Nos. 31930058, 31671540, 32170802, and 31301082). Natural Science Foundation of Guangdong Province (2015B020228002, 2017A030313093). Guangdong Basic and Applied Basic Research Foundation (2019A1515011422, 2021A1515010759).
Guang Shi, Yaofu Bai, Xiya Zhang, Junfeng Su, Junjie Pang, Quanyuan He, Pengguihang Zeng, Junjun Ding, Yuanyan Xiong, Jingran Zhang, Jingwen Wang, Dan Liu, Wenbin Ma, Junjiu Huang, and Zhou Songyang declare that they have no conflict of interest.
All institutional and national guidelines for the care and use of laboratory animals were followed.
All the high-throughput sequencing data generated in this study are available from the corresponding authors upon request. Oct4 ChIP-seq data were download from the GEO database (GSE56098, GSM1355154, GSM1355155, GSM1355167). All the experimental materials generated in this study are available from the corresponding authors upon reasonable request.
Z.S., J.H., and G.S. designed the experiments. G.S., Y.B., X.Z., and J.S. performed the experiments and analyzed the data. G.S. and Z.S. wrote the manuscript. J.H. and Z.S. supervised the research. All authors discussed the results and commented on the manuscript.
Author information
Authors and Affiliations
Corresponding authors
Supplementary Information
Below is the link to the electronic supplementary material.
Rights and permissions
Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons licence, and indicate if changes were made. The images or other third party material in this article are included in the article's Creative Commons licence, unless indicated otherwise in a credit line to the material. If material is not included in the article's Creative Commons licence and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this licence, visit http://creativecommons.org/licenses/by/4.0/.
About this article
Cite this article
Shi, G., Bai, Y., Zhang, X. et al. Bend family proteins mark chromatin boundaries and synergistically promote early germ cell differentiation. Protein Cell 13, 721–741 (2022). https://doi.org/10.1007/s13238-021-00884-1
Received:
Accepted:
Published:
Issue Date:
DOI: https://doi.org/10.1007/s13238-021-00884-1