JARID2 and the PRC2 complex regulate the cell cycle in skeletal muscle

JARID2 is a noncatalytic member of the polycomb repressive complex 2 (PRC2) which methylates of histone 3 lysine 27 (H3K27). In this work, we show that JARID2 and the PRC2 complex regulate the cell cycle in skeletal muscle cells to control proliferation and mitotic exit. We found that the stable depletion of JARID2 leads to increased proliferation and cell accumulation in S phase. The regulation of the cell cycle by JARID2 is mediated by direct repression of both cyclin D1 and cyclin E1, both of which are targets of PRC2-mediated H3K27 methylation. Intriguingly, we also find that the retinoblastoma protein (RB1) is a direct target of JARID2 and the PRC2 complex. The depletion of JARID2 is not sufficient to activate RB1. However, the ectopic expression of RB1 can suppress cyclin D1 expression in JARID2-depleted cells. Transient depletion of JARID2 in skeletal muscle cells leads to a transient up-regulation of cyclin D1 that is quickly suppressed with no resulting effect on proliferation, Taken together, we show that JARID2 and the PRC2 complex regulate skeletal muscle proliferation in a precise manner that involves the repression of cyclin D1, thus restraining proliferation and repressing RB1, which is required for mitotic exit and terminal differentiation.

JARID2 is a noncatalytic member of the polycomb repressive complex 2 (PRC2) which methylates of histone 3 lysine 27 (H3K27). In this work, we show that JARID2 and the PRC2 complex regulate the cell cycle in skeletal muscle cells to control proliferation and mitotic exit. We found that the stable depletion of JARID2 leads to increased proliferation and cell accumulation in S phase. The regulation of the cell cycle by JARID2 is mediated by direct repression of both cyclin D1 and cyclin E1, both of which are targets of PRC2-mediated H3K27 methylation. Intriguingly, we also find that the retinoblastoma protein (RB1) is a direct target of JARID2 and the PRC2 complex. The depletion of JARID2 is not sufficient to activate RB1. However, the ectopic expression of RB1 can suppress cyclin D1 expression in JARID2-depleted cells. Transient depletion of JARID2 in skeletal muscle cells leads to a transient up-regulation of cyclin D1 that is quickly suppressed with no resulting effect on proliferation, Taken together, we show that JARID2 and the PRC2 complex regulate skeletal muscle proliferation in a precise manner that involves the repression of cyclin D1, thus restraining proliferation and repressing RB1, which is required for mitotic exit and terminal differentiation.
Cell proliferation and differentiation are mutually exclusive but closely coordinated and highly regulated processes. In skeletal muscle, the process is marked by a large number of gene expression changes as cell cycle genes go from highly expressed to permanently silenced while another set of genes that are normally repressed during proliferation are activated during differentiation (1).
Two essential protein families that regulate the cell cycle are cyclins and cyclin-dependent kinases (CDKs). 2 These complexes guide the transition of cells through the different phases of the cell cycle. In the mammalian system, cyclins D and E govern the progress through the G 1 /S phases whereas the mitotic cyclins A and B promote progression through the S/G 2 /M phases of the cell cycle (2). Mitogenic signaling stimulates the synthesis and assembly of the short-lived D-type cyclins with CDK4 or CDK6 (3). Cyclin D/CDK complexes are active as long as mitogenic stimulation continues. Cyclin D/CDK acts directly as a kinase to phosphorylate cellular substrates critical for cell cycle progression. D-type cyclins also act to sequester the CDK inhibitors p27 and p21 in a kinase-independent role (2). The protein level of cyclin E is maximum at the G 1 /S transition and is followed by an increase in cyclin A levels during S phase. Both cyclin A and E can form complexes with CDK2, although CDK1 can only form a complex with cyclin A. Rising levels of cyclin B result in the induction of CDK1 at the G 2 /M phase. Coordinated cell cycle progression is a result of the highly regulated fluctuation in the expression of cyclins and activation of cognate CDKs (reviewed in Ref. 1).
Skeletal muscle determination and differentiation are controlled by four highly related basic-helix-loop-helix transcription factors known as the myogenic regulatory factors (MRFs) which include Myf5 (Myf5), MyoD (Myod), myogenin (Myog), and MRF4 (Myf6) (4 -6). MyoD and Myf5 have been shown to promote the proliferation of muscle progenitor cells whereas myogenin appears to possess the intrinsic activity required to mediate cell cycle exit as the exogenous expression of myogenin in proliferating myoblast causes premature exit of myoblast from the cell cycle (7). MyoD can also promote cell cycle arrest by induction of the cyclin-dependent kinase inhibitor p21 (8,9) along with other Cip1/Kip1 family members, p57 and p27, which inhibit a wide range of CDKs essential for cell cycle progression (10). During differentiation, the induction of p21 is followed by the expression of myogenin, which marks a "point of no return" for mitotic exit. High levels of p21 are required for maintenance of the post-mitotic state in differentiated myoblasts and MyoD can also induce RB1 expression (11).
In skeletal muscle, the retinoblastoma protein (pRB, RB1) has a critical role in negative regulation of cell cycle progression by promoting exit from the cell cycle and maintaining the differentiated state (12)(13)(14). RB1 maintains cell cycle arrest, which is required for skeletal muscle differentiation, in part by regulating the activity of the E2F family of transcription factors. Pocket proteins, a family that includes RB1 as well as related p107 and p130 proteins, bind and repress E2F activity (12). Activation of cyclin D and CDK4/6 proteins by mitogen-rich conditions allows monophosphorylation of pocket proteins which releases bound activator E2F transcription factors from hypophosphorylated RB1 proteins. Thus, cyclin D/CDK expression results in activation of E2F target cell cycle genes including cyclin E. Cyclin E, in complex with CDK2, further hyperphosphorylates RB1 proteins into the hyperphosphorylated inactive form of RB1 which allows cells to progress through the G 1 /S restriction point (reviewed in Refs. 15 and 16).
Polycomb repressor proteins have an important developmental role and play essential roles in skeletal muscle. The two major polycomb complexes, Polycomb Repressive Complex-1 (PRC1) and Polycomb Repressive Complex-2 (PRC2), are responsible for the ubiquitination of lysine 119 of histone H2A (H2AK119) (17) and the methylation of lysine 27 on histone H3 tail (H3K27), respectively (18 -20). The methylation of H3K27 by PRC2 requires one of the SET domain-containing enhancer of zeste proteins, EZH1 or EZH2. Promoters and enhancers of many lineage-specific genes contain dimethylated and trimethylated H3K27, and the methylation profile of many of these genes is lost upon differentiation (reviewed in Ref. 21).
JARID2, a founding member of Jumonji family of histone demethylases, has no detectable histone demethylase activity and yet is evolutionarily conserved from Drosophila to human (Ref. 22,reviewed in Ref. 23). Recently, it has been shown to be a substoichiometric component of PRC2 which aids in targeting PRC2 and is required for embryonic stem cell differentiation (24). In mice, JARID2 was found to be essential for heart development (25). JARID2 mutant mice exhibit various neural tube, cardiac, and hematopoietic defects and die in utero because of cardiac and hematopoietic defects (26). In cardiac cells, JARID2 has been shown to control the cell cycle through regulation of cyclin D1 (25,27,28). However, the role of JARID2 in skeletal muscle development and regeneration is not well-understood.
We have recently shown that loss of JARID2 blocks differentiation in C2C12 cells through the modulation of the canonical Wnt signaling pathway (29). Here, we examined the effect of JARID2 on the proliferation of skeletal muscle cells. We found that depletion of JARID2 increased the proliferation rate and caused de-repression of positive cell cycle regulators like cyclin D1 and cyclin E1, whereas the negative cell cycle regulators like p21 and RB1 were down-regulated. JARID2 has been shown to recruit the histone methyltransferases G9a and GLP to directly regulate cyclin D1 in cardiomyocytes (30). We show here that JARID2 recruits the PRC2 complex to repress cyclin D1 and cyclin E1 in skeletal muscle and results in H3K27 methylation of target promoters. In a related study, we also have found that the modest depletion or chemical inhibition of EZH2 promotes proliferation through the JARID2-directed regulation of cyclin D1 and cyclin E1. 3 We also show that Rb1 is a direct target of JARID2 and the PRC2 complex, but loss of repression by PRC2 is not sufficient to de-repress gene expression. The differentiation block with consequential increase in proliferation could be restored by exogenous expression of JARID2. Together, we show that JARID2 regulates the cell cycle in PRC2-dependent manner in skeletal muscle cells.

JARID2-depleted cells have increased proliferation
To understand the function of JARID2 in skeletal muscle proliferation, we established cell lines depleted for JARID2 with three independent shRNA constructs in C2C12 cells (29), a well-established in vitro differentiation model. mRNA and protein confirmation of one JARID2 depletion line derived from each shRNA construct is shown in Fig. S1. All described experiments were performed in two cell lines depleted with independent shRNA constructs (shJarid2-1 and shJarid2-3), and the results were consistent. For clarity, only the results for one shRNA construct (shJarid2-3) are shown. We assayed for the proliferation rate of these cells, and we found that C2C12 cells depleted for JARID2 proliferated significantly faster than cells with the scrambled control (Fig. 1A). To determine whether increased DNA synthesis was correlated with the enhanced proliferation observed, we performed an EdU incorporation assay for DNA synthesis and found that the number of actively proliferating cells marked by EdU incorporation was significantly higher in JARID2-depleted cells (Fig. 1B). To correlate the enhanced proliferation with changes in the cell cycle, the cell cycle state was assessed by flow cytometry following propidium iodide staining of the cells. We found that JARID2depleted cells were much more highly enriched in the S phase at the expense of cells in the G 1 phase than the cells with a scrambled control, indicating that JARID2 plays a role in regulating the G 1 /S transition ( Fig. 1C and Fig. S2).

JARID2 represses the positive cell cycle genes cyclin D1 and cyclin E1 to regulate the G 1 /S transition
To understand how JARID2 was regulating the G 1 /S transition, we examined the expression of factors that mediate this transition, including the gene encoding cyclin D1 (Ccnd1). Ccnd1 is methylated at histone H3 lysine 27 in C2C12 cells in a PRC2-dependent manner upon differentiation (13). We found that Ccnd1 mRNA was up-regulated in cells depleted for JARID2 ( Fig. 2A), and this result was confirmed at the protein level as well (Fig. 2B). We next examined cyclin E1 (Ccne1), which functions in concert with cyclin D1 for the cells transition from G 1 to S phase. We found that cyclin E1, like cyclin D1, was also up-regulated at the level of mRNA (Fig. 2C) and protein (Fig. 2D). CDK4/6 and CDK2 are the CDKs that partner with cyclin D1 and cyclin E1, respectively, to phosphorylate various cellular substrates including the retinoblastoma protein (RB1) to regulate cell cycle progression. Thus, we also examined the expression of CDK2 and CDK4 and found that they were up-regulated at the mRNA level (Fig. 2, E and G) as well as the protein level (Fig. 2F).

Stable loss of JARID2 results in repression of negative cell cycle regulators
The cyclin-dependent kinase inhibitor p21 and retinoblastoma proteins (RB1) are known negative regulators of cell cycle progression (G 1 /S transition) and are key regulators of cell cycle exit. Thus, we assayed for the expression of RB1 (Rb1) and found that Rb1 was severely down-regulated at the level of both mRNA (Fig. 3A) and protein (Fig. 3B). We also examined the expression of p21 (Cdkn1a), which is also required for cell cycle exit. We found that Cdkn1a expression was inhibited at the mRNA level upon JARID2 depletion (Fig. 3C). The protein level was less severely affected, but the results show that Cdkn1a is not up-regulated upon the depletion of JARID2 (Fig. 3D).

Exogenous expression of JARID2 restores cell proliferation defect in JARID2-depleted C2C12 cells
To confirm the dependence on JARID2, we asked if restoration of JARID2 could rescue the observed effects on the cell cycle regulators. Scr control and JARID2-depleted cells were transfected with an expression construct for JARID2 (pEF-Ja-rid2) or vector control (pEF). The expression of JARID2 was confirmed by mRNA ( Fig. 4A) and protein (Fig. 4B) analysis. We found that restoration of JARID2 rescued the increased proliferation defect observed on the JARID2 depletion (Fig.  4C). We also found that restoration of JARID2 down-regulated cyclin D1 at the mRNA (Fig. 4D), and protein ( Fig. 4E) level, thus confirming that JARID2 controls the expression of cyclin D1 in skeletal muscle cells. Restoration of JARID2 also suppressed the expression of Ccne1 (Fig. 4F). Cdk4 and Cdk2 mRNA expression were restored by JARID2 expression as well (Fig. 4, G and H). This effect could also be observed at the protein level (Fig. 4I). Interestingly, expression of the negative cell cycle regulators, RB1 and p21, were also rescued, resulting in an up-regulation of expression (Fig. 4J).

JARID2 directly represses cyclin D1 in PRC2-dependent manner
In cardiac cells, JARID2 represses Ccnd1 though alterations in histone H3 lysine 9 (H3K9) methylation (30). To determine whether JARID2 directly repressed Ccnd1 in skeletal muscle, chromatin immunoprecipitation (ChIP) assays were used to probe JARID2 recruitment to the Ccnd1 promoter. We found that JARID2 was present on the Ccnd1 promoter and that depletion of JARID2 reduced this association (Fig. 5A). We next examined the methylation of H3K9 (H3K9me) in cells with or without JARID2 and found no change in the H3K9me profile (Fig. 5B). The antibody used in these experiments was panmethyl H3K9 that recognizes all three states of H3K9 methylation. We next examined the methylation of H3K27 as JARID2 has been shown to direct the PRC2 complex to target genes (31,32) and found that depletion of JARID2 led to a significant depletion of this modification (Fig. 5C). To confirm that this reduction was not because of a loss of total histone 3 (H3) at this promoter, we also examined H3 levels in this region and found that H3 levels were unaltered (Fig. 5C). We also assayed for the presence of the catalytic subunit of the PRC2 complex, EZH2, and we found that EZH2 was associated with the Ccnd1 promoter and that the association was reduced when JARID2 was depleted (Fig. 5D). EZH2 has previously been shown to bind to the Ccnd1 promoter in myotubes (13), but we show here that this can also be detected in myoblasts and importantly, the recruitment of EZH2 depends on JARID2. As a positive control

JARID2 regulates the cell cycle in skeletal muscle
for these experiments, we also examined the H3K27me3 status of the Hoxb7 promoter, a well-established target of the PRC2 complex (33). H3K27me3 was highly enriched on the Hoxb7 promoter and the depletion of JARID2 did not significantly disrupt this modification (Fig. 5E). Total H3 levels were also unaltered (Fig. 5E). The percentage input calculation shows that the Hoxb7 promoter is more highly enriched for H3K27me3 than Ccnd1, which may explain how the methylation of the Ccnd1 and Ccne1 promoters could have been overlooked in previous genome-wide studies. As a negative control, we also examined a promoter proximal region of Tnni2 which we have previously shown is not a target of the PRC2 complex in proliferating cells  panel). B, right panel, blots were quantified and plotted. Plots were normalized to GAPDH loading control. C and D, JARID2 also represses cyclin E1. As in A, cells were assayed for cyclin E1 by qRT-PCR (C) and Western blotting (D, left panel). D, right panel, blots in C were quantified and plotted. Plots were normalized to GAPDH loading control. E-G, JARID2 also represses cyclin-dependent kinases. Cells in A were assayed for Cdk2 and Cdk4 by qRT-PCR (E and G) and Western blotting (F, left panel). D and F were performed simultaneously and the same GAPDH blot was used. Blots in F were quantified and plotted. Plots were normalized to GAPDH (F, right panel). Error bars, mean Ϯ S.E. (Student t test; *, p Ͻ 0.05 and ***, p Ͻ 0.001; n ϭ 3-6 (qRT-PCR) and 3 (Western blots) biological replicates.) JARID2 regulates the cell cycle in skeletal muscle (32). We found that JARID2 and EZH2 were not recruited to this region and H3K27me3 and H3K9me were not altered upon JARID2 depletion (Fig. 5F).
Cyclin D1 is an essential cell cycle regulator and is activated by several factors, including ␤-catenin, the effector of the canonical Wnt pathway. We have recently found that JARID2 directly represses an antagonist of the canonical Wnt signaling pathway, Sfrp1, which leads to an inhibition of the nuclear translocation of ␤-catenin in JARID2-depleted cells (29). To determine whether an alteration in ␤-catenin recruitment contributed to the activation of cyclin D1, we performed ChIP assays for ␤-catenin on the Ccnd1 promoter. We found that ␤-catenin levels were reduced on the Ccnd1 promoter upon JARID2 depletion (Fig. 5G). This result is consistent with our study showing the JARID2-dependent reduction in the nuclear translocation of ␤-catenin (29). This result also shows that the up-regulation of cyclin D1 observed is because of the loss of the JARID2/PRC2-dependent H3K27 methylation and not an enhanced recruitment of the activator ␤-catenin.
We next asked if Ccne1 was also a direct target of JARID2 and the PRC2 complex. JARID2 was found to be associated with the Ccne1 promoter, and JARID2 depletion reduced this association (Fig. 5H). Like Ccnd1, we found that H3K9 methylation on the Ccne1 promoter was unchanged upon JARID2 depletion (Fig. 5I). We found that H3K27 methylation at the Ccne1 promoter was reduced upon JARID2 depletion and again, total H3 levels were unaltered (Fig. 5J). The H3K27me3 enrichment in the JARID2-depleted cells was below the IgG control signal; therefore, the value was zeroed. We also observed a decrease in EZH2 enrichment on the Ccne1 promoter upon JARID2 depletion (Fig. 5K), showing that JARID2 is required to recruit PRC2 to the Ccne1 promoter. Together, these data establish that Ccnd1 and Ccne1 are direct targets of the PRC2 complex and that JARID2 directs the PRC2 complex to these target genes.

RB1 is also a direct target of JARID2 and the PRC2 complex
Cyclin D1 and cyclin E1 function to prevent cell cycle exit by inhibiting the function of the RB1. RB1 is required for the irreversible cell cycle exit associated with the arrest of myoblasts and myogenic differentiation (13,14). We showed that RB1 was down-regulated upon JARID2 depletion (Fig. 3, A and B), but RB1 has also been shown to cooperate with PRC2 in the methylation of cell cycle genes (13). To understand if Rb1 itself was a target of H3K27me3, we asked if the Rb1 gene was a direct target of JARID2 and the PRC2 complex. We found that JARID2 was recruited to the Rb1 promoter and depletion of JARID2 reduced this association (Fig. 6A). We next examined the histone methylation of the Rb1 promoter. We found that the H3K9 methylation profile was significantly low and was not altered upon JARID2 depletion (Fig. 6B), but H3K27 methylation was significantly reduced (Fig. 6C). Total H3 was not reduced and, in fact, was modestly enhanced upon JARID2 depletion (Fig. 6C). We also examined the association of EZH2 and found that EZH2 was associated with the Rb1 promoter and the depletion of JARID2 reduced this binding (Fig. 6D). Thus, Rb1 is a direct target of a JARID2-guided PRC2 complex. However, our data clearly show that the relief of H3K27me inhibition is not sufficient to overcome the cyclin D1-mediated repression of Rb1.
We next asked if the Cdkn1a was directly regulated by JARID2. ChIP assays were performed for JARID2, EZH2, H3K27me3, and H3K9me. However, we did not see any signif-

JARID2 regulates the cell cycle in skeletal muscle
icant change in the enrichment of H3K9me, H3K27me3, JARID2, and EZH2 for the Cdkn1a promoter upon JARID2 depletion (Fig. S3), suggesting that Cdkn1a is not a direct target of the JARID2-guided PRC2 complex. We do, however, note that H3K27me3 was enriched on the Cdkn1A promoter and this association was lost upon EZH2 depletion, indicating that JARID2 regulates the cell cycle in skeletal muscle EZH2 does directly regulate the Cdkn1a locus. 3 Our results indicate that this regulation may be independent of JARID2.
To understand how the suppression of Rb1 contributed to the effects observed in JARID2-depleted cells, we used expression construct for RB1-WT and a constitutively active form of RB1 which contains 14 mutated phosphorylation sites (RB-NPC) (34). These constructs were transiently transfected in scr and JARID2-depleted cells. Cells were harvested both before and after differentiation conditions. The known up-regulation of RB1 upon differentiation and the loss of RB1 expression in JARID2-depleted cells could be observed in this experiment (Fig. 6E). We found that RB1-WT could efficiently silence cyclin D1 expression in JARID2-depleted cells (Fig. 6E). The nonphosphorylatable form of RB1 (NPC) did not effectively suppress cyclin D1 (Fig. 6E). Phosphorylation of RB1 releases E2F and our data suggest that phosphorylation of RB1 is required for cyclin D1 repression. We have also shown that the depletion of JARID2 inhibits the expression of myogenin through the loss of ␤-catenin-mediated expression of MyoD (29). Although RB1 could effectively suppress cyclin D1, it could not restore myogenin expression (Fig. 6E). Thus, the effects of JARID2 on the cell cycle and Wnt pathway signaling are independent and show that JARID2 and the PRC2 complex regulate myogenesis through multiple pathways.

Transient loss of JARID2 transiently up-regulates cyclin D1
Our results showing that JARID2 is required to restrain proliferation through the PRC2 complex were surprising given that ablation of EZH2 has been shown to lead to reductions in the muscle stem cell pool (35). In our companion manuscript with EZH2, 3 we show that EZH2 restrains cell proliferation through precise regulation of both positive and negative cell cycle genes in skeletal muscle and that the resulting phenotype of enhanced proliferation or cell death correlated to the level of EZH2 depletion or inhibition. To understand if JARID2 had similar effects, we asked if we could observe enhanced proliferation and the up-regulation of cyclin D1 using a transient depletion approach. JARID2 was transiently depleted in C2C12 cells using the same shRNAs used to generate the stable cell lines, and cells were harvested 24 and 48 h following the transfection. Quantification of JARID2 mRNA following the depletion is shown in Fig. 7A. Unlike EZH2 depletion or loss, we did not see any discernible difference in cell proliferation (Fig. 7B). However, we also did not observe enhanced proliferation, indicating that stable depletion of JARID2 is required to see this effect. Myogenin is a known target of the PRC2 complex in skeletal muscle (33) and we found that an immediate up-regulation of Myog could be observed in the transient approach (Fig. 7C). However, the expression quickly returned to normal levels by 48 h post transfection (Fig. 7C). We next asked how cyclin D1 expression was affected in a transient depletion of JARID2. Like myogenin, we saw an immediate burst of mRNA expression 24 h post transfection. However, by 48 h post transfection the expression was lower than the scrambled control (Fig. 7D). At the protein level, no up-regulation of cyclin D1 could be detected (Fig. 7E). To confirm that JARID2 was depleted in this approach, protein expression of JARID2 was examined as well, and we saw that JARID2 was down-regulated, consistent with the mRNA analysis (Fig. 7E). The depletion efficiency of JARID2 correlated closely with the burst of Ccnd1 mRNA expression detected in this approach.
C2C12 cells are known to have mutated p16/p19 locus (36), and it was not clear what impact the mutated locus had on the results we observed with C2C12 cells. To answer this question, we next used freshly isolated primary myoblasts to determine whether we could recapitulate the results we saw with C2C12 cells. JARID2 was transiently depleted in primary myoblasts using the shRNA constructs used for stable depletion and cells harvested 24 or 48 h post transfection. We found that JARID2 was depleted at both time points (Fig. 8A), but as we saw in C2C12 cells, an up-regulation of cyclin D1 expression could be observed at 24 h post transfection, but cyclin D1 levels quickly returned to baseline 48 h post transfection (Fig. 8B). Again similar to what we observed in C2C12 cells using a transient approach, we observed no changes in cell cycle progression upon on the transient loss of JARID2 in primary myoblasts (Fig.  8C). We also saw no significant increase in DNA synthesis as assayed by an EdU incorporation assay (Fig. 8D). At the 48 h time point, all positive cell cycle genes assayed were down-regulated including Ccne1 (Fig. 8E), Cdk4 (Fig. 8F), and Cdk2 (Fig.  8G). Down-regulation of CYCLIN D1, CDK4, and CDK2 were observed at the protein level as well (Fig. 8H). As we observed with a transient EZH2 depletion, 3 the negative cell cycle regulator Cdkn1a (p21) was up-regulated (Fig. 8I), and this effect could also be seen at the protein level (Fig. 8H). The Cdkn2a (p16/p19) locus was down-regulated (Fig. 8J), indicating that the loss of this locus is not implicated in the proliferation defect observed in C2C12 cells upon stable depletion of JARID2. Intriguingly, although a significant effect on cell viability was not observed upon transient JARID2 depletion, we did observe increased mRNA expression of the pro-apoptotic gene Bax (Fig. 8K) and decreased expression of the anti-apoptotic factor Bcl2 (Fig. 8L)

JARID2 regulates the cell cycle in skeletal muscle
Together, our results confirm that JARID2 directly regulates cyclin D1 through the PRC2 complex, but because of the complex effects on both positive and negative cell cycle genes, sustained depletion is required to see a sustained activation of cyclin D1 and enhanced proliferation.

Discussion
In this work, we show that JARID2, along with the PRC2 complex, restrains proliferation by repressing the pro-proliferative cell cycle regulators cyclin D1 and cyclin E1. When expressed, these factors then phosphorylate RB1, thus releasing activator E2F transcription factors that further up-regulate various cell cycle genes including cyclin E1. This feed-forward loop forms a switch that decides whether the cell proceeds to S phase surpassing the G 1 /S restriction point or exits the cell cycle in a RB1-dependent manner.
Our finding that JARID2 regulates cell proliferation is in agreement with the previous finding in heart muscle which showed that JARID2 regulates cell proliferation through repression of the Ccnd1 gene (25,27). However, unlike in cardiomyocytes where JARID2 has been shown repress Ccnd1 by H3K9 methyltransferases (30), we show that JARID2 represses

JARID2 regulates the cell cycle in skeletal muscle
Ccnd1 by recruiting a H3K27 methyltransferase, the PRC2 complex, in skeletal muscle. This finding is in agreement with previous findings that showed no significant contribution of H3K9 methylation during skeletal muscle differentiation (33). JARID2 has also been shown to regulate various target genes in a PRC2-dependent manner during cardiac development as well (38). Clearly, the role of JARID2, an inactive histone demethylase, and its regulatory partner complexes is evolutionarily diverse depending on cell type. It is interesting that JARID2/PRC2 directly regulates both cyclin D1 and cyclin E1 to maintain control of the cell cycle. The dual regulation serves to maintain control of two central regulators of the G 1 /S transition phase. Our results also suggest that the PRC2 complex has many divergent roles in skeletal muscle cells that require a fine balance of JARID2 and EZH2 expression.
Intriguingly, JARID2 and the PRC2 complex also methylate Rb1 in proliferating cells, the repression of which prevents mitotic exit and terminal differentiation. Thus, the normal function of JARID2 and the PRC2 complex in skeletal muscle appears to be restraining the rate of proliferation while also preventing mitotic exit. In the JARID2 depletions characterized here, the loss of inhibition of cyclin D1 dominates the potential de-repression of Rb1. However, when JARID2 expression was restored, it was interesting that the normal expression of both negative and positive cell cycle regulators was restored. In this case, the repression of cyclin D1 is clearly sufficient to restore RB1 expression, irrespective of H3K27 methylation. Figure 6. Rb1 is directly regulated by JARID2 but not Cdkn1a (p21). A-D, RB1 is a direct target of JARID2 and the PRC2 complex. ChIP assays were performed on proliferating scr and JARID2-depleted (shJarid2) C2C12 cells with antibodies against JARID2 (A), H3K9me (B), H3K27me3 and H3 (C) EZH2 (D), and primers spanning the Rb1 promoter. IgG background signals were subtracted from immunoprecipitation signals. E, restoration of RB1 can inhibit cyclin D1, but not activate myogenin. C2C12 cells with scrambled (scr) and JARID2 depletion (shJarid2) were transiently transfected with expression constructs for RB1 (RB1-WT), and RB1 mutated at phosphorylation sites (RB1-NPC). UD represents the proliferative, undifferentiated time point and D2Ј represents 2 days in differentiation media. Cells were analyzed for total RB1, cyclin D1, and myogenin. GAPDH was used as a loading control. # represents the band of interest for RB1 protein as determined by molecular weight standards. Error bars, mean Ϯ S.E. (Student's t test; ns represents not significant, *, p value Ͻ 0.05; **, p value Ͻ 0.01; ***, p value Ͻ 0.001; n ϭ 3 biological replicates.)

JARID2 regulates the cell cycle in skeletal muscle
JARID2 has also been shown to regulate cell proliferation through repression of Ccnd1 in leukemia (28). JARID2 has been identified as an oncogene that is often overexpressed in multiple cancers including rhabdomyosarcoma (39). In rhabdomyosarcoma, JARID2 is essential for cell viability and loss of JARID2 rescues partial differentiation in rhabdomyosarcoma (39). However, JARID2 has recently been shown to act as tumor sup-pressor in myeloid neoplasm through restriction of hematopoietic progenitor cells self-renewal (40).
Importantly, in our study we found that JARID2 could be efficiently depleted in C2C12 cells without a significant impact on viability, unlike EZH2. We did observe changes in apoptotic cell marker expression upon transient JARID2 depletion in primary myoblasts, so it remains to be determined if JARID2 could Recent studies have shown that the expression Cdk4/cyclin D1 expands neural stem cells and increases neurogenesis (41). It has also been shown that regulation of the cell cycle through reintroduction of cyclin D1 and CDK4 in cardiac cells can increase cardiac cell regeneration and repair post injury (42). Our work suggests that inhibiting the function of JARID2 could potentially be used to expand the muscle stem cell pool and enhance muscle repair and regeneration. Clearly, the roles of JARID2 and the PRC2 complex are complex in skeletal muscle and serve to both inhibit and activate several steps of the myogenic program. Characterization of each of these roles aid in the understanding of how these factors are involved in normal myogenesis, repair, and disease.

Experimental procedures
Cell culture C2C12 cells (ATCC) were grown in DMEM, supplemented with 10% FBS (HyClone Laboratories) according to standard protocols. Proliferating C2C12 myoblasts were grown in DMEM supplemented with 10% FBS (HyClone Laboratories), and 2% horse serum (Gibco Laboratories) in DMEM was used to induce differentiation. Primary myoblasts were isolated according to standard protocols (43). Briefly, hind limb muscles of neonatal mice were isolated and digested with Collagenase Type II (Worthington Biochemical Corp.). Cells were filtered through a sterile 70-micron filter, plated on gelatin-coated plates in 20% FBS in F-10 basal media with 1ϫ penicillin-streptomycin (Corning) and 2.5 ng/ml bFGF (gift of D. Cornelison, University of Missouri). Primary myoblasts were enriched by pre-plating cells onto uncoated plates for 30 min before transferring myoblast suspensions to collagen-coated plates and repeating until the majority of the cells were myoblasts. Myoblast identity was confirmed by expression analysis of MRFs, differentiation assays, and myosin heavy chain immunofluorescence. All mouse procedures were approved by the Southern Illinois University Institutional Animal Care and Use Committee.

Plasmid constructs
JARID2 was depleted with shRNA constructs designed by the RNAi Consortium in the pLOK.1 plasmid (Open Biosystems) as described (29). Three constructs targeting murine Jarid2 and one scrambled control were linearized using the ScaI restriction enzyme (New England Biolabs), transfected into C2C12 cells using TurboFect (Thermo Scientific) following manufacturer's protocol, and selected with puromycin (2 g/ml). Individual clones were selected, propagated, and confirmed by mRNA and protein analysis. For transient transfections, circu-lar (uncut) plasmids were transfected using TurboFect. mRNA and protein were extracted at indicated time points. Drug selection was not used for transient transfection experiments.
The coding sequence of murine Jarid2 was PCR amplified from cDNA reverse transcribed from the total RNA extracted from proliferating C2C12 cells. The PCR amplified Jarid2 insert was cloned into the pEF6/V5 His TOPO TA expression vector according to manufacturer's protocol (Invitrogen). The clones were confirmed by sequencing. For rescue of JARID2 expression, pEF6-Jarid2 plasmid was stably transfected in C2C12 cells previously depleted of JARID2 using shRNA construct (mature antisense sequence: 5Ј-AAATTGCACATGGATGACAGG-3Ј) that targets 3Ј-untranslated region (UTR) of Jarid2 mRNA. The stable clones were selected with blasticidin (10 g/ml), confirmed by mRNA and protein analysis.
Expression plasmids for WT and a nonphosphorylatable form (NPC) of retinoblastoma protein (RB1) were generated in the lab of Sibylle Mittnacht (University College London Cancer Institute) (34). Colin Goding (University of Oxford Ludwig Cancer Research) used these constructs to characterize the interaction of Mitf and RB1 (37) and generously gifted these constructs to our laboratory. The constructs were confirmed by restriction enzyme mapping and sequencing. The plasmids were transfected using TurboFect as described previously.

Western blot analysis
Cell extracts were made by lysing PBS washed cell pellets in radioimmune precipitation assay buffer (RIPA) supplemented with protease inhibitors (cOmplete Protease Inhibitor, Roche Diagnostics). Following incubation on ice, clear lysates were obtained by centrifugation. Protein concentrations were determined by Bradford's assay (Bio-Rad). For each sample, 30 g of protein was loaded on each gel unless otherwise specified. Proteins were transferred onto a PVDF membrane using a tank blotter (Bio-Rad). The membranes were then blocked with 5% milk in 1ϫ Tris-buffered saline plus Tween 20 (TBST) and incubated with primary antibody overnight at 4°C. Membranes were then washed with 1ϫ TBST and incubated with the corresponding secondary antibody. Membranes were again washed with 1ϫ TBST, incubated with chemiluminescent substrate according to manufacturer's protocol (SuperSignal, Pierce) and visualized by an iBright Imaging System or developed by autoradiography. The antibodies used include anti-JARID2 (ABclonal), anti-cyclinD1 (DCS-6, Invitrogen), anticyclin E1 (Santa Cruz Biotechnology), anti-CDK2 (ABclonal), anti-CDK4 (ABclonal), anti-pRB1 (LabVision) (Fig. 4I), anti-pRB1(Cell Signaling Technology) (Figs. 3B and 6E), anti-p21 (ABclonal), anti-tubulin (E7, Developmental Studies Hybridoma Figure 8. Transient loss of Jarid2 does not decrease cell viability in primary myoblasts. A, freshly isolated primary myoblasts were transiently transfected with scrambled (scr) control or shRNA against Jarid2 (shJarid2) without drug selection. Jarid2 expression was assayed by qRT-PCR at the indicated time points. B, cells in A were assayed for cyclin D1 expression by qRT-PCR. C, transient loss of Jarid2 in primary myoblast does not have significant change cell cycle progression. Cells in A were ethanol fixed, propidium iodide stained, and analyzed for cell cycle phase distribution using flow cytometry. D, transient loss of Jarid2 did not result in a significant increase in DNA synthesis in primary myoblasts. Cells in A were assayed for DNA synthesis by EdU incorporation assay (left panel). Five random fields were counted for EdU ϩ nuclei and plotted (right panel). DAPI was used to stain nuclei. Scale bar, 50 m; n ϭ 2 biological replicates. E-J, cell cycle genes are deregulated upon transient loss of Jarid2 in primary myoblasts. Cells as in A were analyzed for the expression of cyclin E1 (Ccne1) (E), Cdk4 (F), Cdk2 (G), p21 (Cdkn1a) (I), and Cdkn2a (p16/19) (J) by qRT-PCR and Western blotting (H). GAPDH was used as a loading control. # represents the band of interest for CDK2 based on molecular weight standards. K and L, Jarid2 depletion increased apoptotic marker expression in primary myoblasts. Cells in A were assayed for the pro-apoptotic marker Bax (K) and anti-apoptotic marker Bcl2 (L) by qRT-PCR. Error bars, mean Ϯ S.E. (Student's t test; ns represents not significant; ***, p Ͻ 0.001; n ϭ 3 biological replicates.) Bank), and anti-GAPDH (Millipore). Protein expression levels were quantified using iBright analysis software or ImageJ (National Institutes of Health) software on at least three independent experiments unless otherwise mentioned. Representative images are shown.

Quantitative real-time PCR
RNA was isolated from cells by TRIzol extractions (Invitrogen). Following treatment with DNase (Promega), 2 g of total RNA was reversed transcribed with MultiScribe™ MuLV Reverse Transcriptase (Applied Biosystems). cDNA equivalent to 40 ng was used for quantitative PCR amplification (Applied Biosystems) with SYBR green PCR master mix (Applied Biosystems). Samples in which no reverse transcriptase was added (no RT) were included for each RNA sample. Quantitative PCR data were calculated using the comparative Ct method (Applied Biosystems). Standard deviations from the mean of the [⌬] Ct values were calculated from three independent RNA samples. Primers are described in Table  S1. Where possible, intron-spanning primers were used. All quantitative PCR was performed in triplicate, and three independent RNA samples were assayed for each time point. For measurements of relative gene expression, a -fold change was calculated for each sample pair and then normalized to the -fold change observed at hypoxanthine guanine phosphoribosyl transferase (HPRT) and/or 18S rRNA.

ChIP assays
ChIP assays were performed as described previously (37). The following antibodies were used: anti-Jarid2 (Cell Signaling Technology), anti-Ezh2 (Cell Signaling Technology), anti-H3K27me3 (Cell Signaling Technology), anti-H3K9me (pan) (Cell Signaling Technology), anti-H3 (Cell Signaling Technology) and anti-␤-Catenin (Santa Cruz Biotechnology). Rabbit IgG (Santa Cruz Biotechnology) was used as a nonspecific control. Primers are described in Table S1. The real-time PCR was performed in triplicate. The results were represented as the percentage of immunoprecipitation over input signal (% Input) with IgG background signal subtracted. All ChIP assays shown are representative of at least three individual experiments unless otherwise stated. Standard error from the mean was calculated and plotted as the error bar.

EdU incorporation assay
Cells were assayed using a Click-iT EdU Alexa Fluor 488 Imaging Kit according to the manufacturer's protocol (Life Technologies). C2C12 and primary myoblast cells were grown in the presence of EdU for 2 and 3 h, respectively. EdU positive nuclei were counted in at least five random fields on microscopic images taken at 200ϫ and 400ϫ magnification using a Leica microscope.

Proliferation assay
An equal number of cells were seeded, and on the indicated days, cells were harvested using trypsin, resuspended and counted under a light microscope using a hemocytometer. Cell viability was determined by Trypan Blue staining. Cell counting was performed in duplicate for at least three blinded biological replicates.

Cell cycle analysis by flow cytometry
Cells were split in 100-mm diameter plates at 1:5 dilution, grown for 48 h in duplicates in 10% FBS in 5% CO 2 incubator. The cell plates were washed twice with sterile 1ϫ PBS, pH 7.4, harvested using trypsin, and resuspended in 1ϫ PBS, pH 7.4. Cells were pelleted down at 600 ϫ g for 5 min at room temperature, washed twice with 1ϫ PBS and were fixed in chilled 70% ethanol overnight at Ϫ20°C. Cells were washed with 1ϫ PBS, pH 7.4, treated with RNase (10 g/ml), and stained with propidium iodide (50 g/ml) for 2 h at room temperature before running through a BD Accuri C6 flow cytometer (BD Biosciences). Data were analyzed using FlowJo (FlowJo LLC) software.

Statistics
Data are presented as mean Ϯ S.E. Statistical comparisons were performed using the unpaired two-tailed Student's t tests and analysis of variance (ANOVA) test followed by Tukey's multiple comparison test. A probability value of Ͻ 0.05 was taken to indicate significance. All statistical analyses and graphs were made in GraphPad Prism 8.0 software.