Recruitment of Histone Methyltransferase G9a Mediates Transcriptional Repression of Fgf21 Gene by E4BP4 Protein*

Background: The epigenetic mechanism underlying E4BP4-dependent repression of hepatic Fgf21 during refeeding is unknown. Results: E4BP4 interacts with G9a, and knockdown of G9a by shRNA abolishes suppression of Fgf21 by refeeding in vivo. Conclusion: G9a is a co-repressor required for E4BP4-dependent repression of Fgf21 expression. Significance: G9a is a critical histone methyltransferase in E4BP4-dependent repression of Fgf21 during refeeding. The liver responds to fasting-refeeding cycles by reprogramming expression of metabolic genes. Fasting potently induces one of the key hepatic hormones, fibroblast growth factor 21 (FGF21), to promote lipolysis, fatty acid oxidation, and ketogenesis, whereas refeeding suppresses its expression. We previously reported that the basic leucine zipper transcription factor E4BP4 (E4 binding protein 4) represses Fgf21 expression and disrupts its circadian oscillations in cultured hepatocytes. However, the epigenetic mechanism for E4BP4-dependent suppression of Fgf21 has not yet been addressed. Here we present evidence that histone methyltransferase G9a mediates E4BP4-dependent repression of Fgf21 during refeeding by promoting repressive histone modification. We find that Fgf21 expression is up-regulated in E4bp4 knock-out mouse liver. We demonstrate that the G9a-specific inhibitor BIX01294 abolishes suppression of the Fgf21 promoter activity by E4BP4, whereas overexpression of E4bp4 leads to increased levels of dimethylation of histone 3 lysine 9 (H3K9me2) around the Fgf21 promoter region. Furthermore, we also show that E4BP4 interacts with G9a, and knockdown of G9a blocks repression of Fgf21 promoter activity and expression in cells overexpressing E4bp4. A G9a mutant lacking catalytic activity, due to deletion of the SET domain, fails to inhibit the Fgf21 promoter activity. Importantly, acute hepatic knockdown by adenoviral shRNA targeting G9a abolishes Fgf21 repression by refeeding, concomitant with decreased levels of H3K9me2 around the Fgf21 promoter region. In summary, we show that G9a mediates E4BP4-dependent suppression of hepatic Fgf21 by enhancing histone methylation (H3K9me2) of the Fgf21 promoter.

The liver responds to fasting-refeeding cycles by reprogramming expression of metabolic genes. Fasting potently induces one of the key hepatic hormones, fibroblast growth factor 21 (FGF21), to promote lipolysis, fatty acid oxidation, and ketogenesis, whereas refeeding suppresses its expression. We previously reported that the basic leucine zipper transcription factor E4BP4 (E4 binding protein 4) represses Fgf21 expression and disrupts its circadian oscillations in cultured hepatocytes. However, the epigenetic mechanism for E4BP4-dependent suppression of Fgf21 has not yet been addressed. Here we present evidence that histone methyltransferase G9a mediates E4BP4dependent repression of Fgf21 during refeeding by promoting repressive histone modification. We find that Fgf21 expression is up-regulated in E4bp4 knock-out mouse liver. We demonstrate that the G9a-specific inhibitor BIX01294 abolishes suppression of the Fgf21 promoter activity by E4BP4, whereas overexpression of E4bp4 leads to increased levels of dimethylation of histone 3 lysine 9 (H3K9me2) around the Fgf21 promoter region. Furthermore, we also show that E4BP4 interacts with G9a, and knockdown of G9a blocks repression of Fgf21 promoter activity and expression in cells overexpressing E4bp4. A G9a mutant lacking catalytic activity, due to deletion of the SET domain, fails to inhibit the Fgf21 promoter activity. Importantly, acute hepatic knockdown by adenoviral shRNA targeting G9a abolishes Fgf21 repression by refeeding, concomitant with decreased levels of H3K9me2 around the Fgf21 promoter region. In summary, we show that G9a mediates E4BP4-dependent suppression of hepatic Fgf21 by enhancing histone methylation (H3K9me2) of the Fgf21 promoter.
During the normal fasting-refeeding cycles, the liver responds to nutrient influx and deprivation by turning on and off corresponding metabolic gene expression (1). Fasting activates catabolic events, such as lipolysis, fatty acid oxidation, and proteolysis, whereas feeding promotes anabolic pathways, including lipogenesis and glycogenesis. FGF21 is a hepatic hormone highly induced by food starvation or ketogenic diet and suppressed by refeeding (2). As an adaptive response to fasting, elevated levels of FGF21 promote lipolysis in the white fat tissue and ketogenesis in the liver (3). Several nuclear receptors, including peroxisome proliferator-activated receptor ␣ (PPAR␣), 2 thyroid hormone receptor ␤, retinoid X receptor, and RAR-related orphan receptor ␣ have been identified as transcription activators for Fgf21 in the liver (2)(3)(4)(5)(6). The critical role of PPAR␣ has been highlighted by abolishment of Fgf21 induction in the liver PPAR␣ knockout mice after prolonged fasting or bezofibrate (PPAR␣ agonist) treatment (7,8). So far, few repressors of Fgf21 gene expression are known. Our laboratory previously reported that the basic leucine zipper transcription factor E4BP4 represses Fgf21 upon insulin stimulation and is critical for circadian oscillations of Fgf21 (9). However, the epigenetic program underlying the E4BP4-dependent repression of Fgf21 remains unknown.
E4BP4 is a basic leucine zipper transcription factor initially identified as adenoviral E4 promoter-binding repressor and an IL3-induced factor in B-lymphocytes (10,11). In E4bp4 knockout mice, it has been shown that E4BP4 is critical for NK cell development and IgE expression in B cells (12)(13)(14). In addition to its role in the immune system, E4bp4 is also highly expressed in the liver, adipose tissue, and the suprachiasmatic nuclei of the hypothalamus (15). Hepatic E4bp4 mRNA displays a potent cycling in the liver with peak expression at circadian time 0 and trough expression at circadian time 12 h (15). As a circadian output oscillator, E4BP4 may regulate circadian oscillations of a subset of circadian out genes, such as Mdr1 (multidrug-resistant gene 1) (16), PPAR␥ (17), and Cyp7a (18). In Drosophila, the E4bp4 homologue vrille functions as a key negative regulator of * This work was supported, in whole or in part, by National Institutes of Health Grant K99/R00 DK 077449 (to L. Y.). Part of this work was also supported by a pilot grants (to L. Y.) from the Michigan Diabetes Research Center (P600K020572) and Michigan Obesity and Nutrition Research Center (DK089503). 1 To whom correspondence should be addressed. the fly circadian clock (19,20). E4BP4 actively represses target gene expression primarily through its binding to the D-box elements of target promoters (21). The TATA box-binding protein (TBP)-binding protein D1 was postulated as a potential repression cofactor of E4BP4 based upon its interaction with E4BP4 (22). Despite the potent repression of targets by E4BP4, epigenetic changes and histone-modifying enzymes involved in its transcriptional silencing remain largely unknown. A subset of transcriptional repression is characterized by a repressive mark, dimethylation at lysine 9 of histone H3 (H3K9me2), around the promoter region of target genes (23). H3K9me2 is catalyzed by a group of histone methyltransferases, including G9a and G9a-like protein (GLP), members of the highly conserved SET (Su (var) 3-9-enhancer of zestetrithorax) domain family (24). G9a and GLP exist predominantly in a heterodimeric complex to function as a functional H3K9 methyltransferase in vivo (25). Global deletion of G9a in mice drastically reduced levels of H3K9me2 and resulted in embryonic lethality, highlighting the consequences of global perturbation of gene repression during embryogenesis (26). G9a-associated transcription repression might be also involved in the postdevelopmental stage and participate in a short term gene regulation. Indeed, G9a-dependent methyltransferase activity has been found to be involved in the expression of Th2associated cytokines (27), terminal differentiation of B-lymphocytes (28), bile acid metabolism (29), cocaine-induced neuronal plasticity (30), tumor growth and metastasis (31)(32)(33), and the interferon response (34). No previous studies have reported the role of G9a in lipid metabolism in the liver.
Previously, we identified Fgf21 as a direct circadian target of E4BP4 in hepatocytes (9). In the present study, we demonstrate that E4BP4 is an in vivo repressor of Fgf21 transcription during fasting-refeeding cycles. At the molecular level, we provide evidence that E4BP4 interacts with histone methyltransferase G9a to repress Fgf21 expression. Manipulation of G9a expression or inhibition of its enzymatic activity alters Fgf21 transcription in cultured hepatocytes. Crucially, depletion of G9a expression by shRNA knockdown in the mouse liver abolishes the hepatic Fgf21 oscillations during fasting-refeeding cycles.

EXPERIMENTAL PROCEDURES
Plasmids and Adenovirus Generation-Both E4BP4 overexpression and shRNA vectors were reported before (9). The adenovirus for Ad-E4bp4 (overexpression), Ad-shE4bp4 (knockdown), and Ad-shG9a (knockdown) were generated using the pAdEasy system (Agilent) and pAd-Block-it system (Invitrogen). The shRNA targeting sequence for mouse E4bp4 is 5Јggaattcattccggacgagaa. The shRNA targeting sequence for mouse G9a is 5Ј-gcctgtactatgatgctgact. The HA-G9a expression vector is a generous gift from Dr. Kenneth Wright (Moffitt Cancer Center, University of South Florida). The HA-G9a-⌬SET mutant (⌬995-1159aa) was generated via QuikChange mutagenesis (Agilent) and confirmed by sequencing.
Animal Experiments-All animal care and use procedures were in accordance with guidelines of the University of Michigan Institutional Animal Care and Use Committee. All mice used in this study were of the C57 Bl/6 strain. Both male wildtype (WT) and E4bp4 Ϫ/Ϫ mice age 8 -10 weeks were main-tained on 12-h/12-h light/dark with free access to food and water. Both WT and E4bp4 Ϫ/Ϫ mice (n ϭ 4 -5 mice/group) were then sacrificed at Zeitgeber time 6 h, and both serum and liver tissues were collected for analysis. Serum FGF21 was measured by ELISA according to the manufacturer's instructions (R&D Systems). Serum level of ␤-hydroxybutyrate (ketone body) was measured by a commercial kit (Pointe Scientific).
Adenoviral Injection-WT C57BL/6J male mice (between 8 and 10 weeks old) were maintained on a 12-h/12-h light/dark cycle with free access to standard diet and water. For adenoviral injections, 1 ϫ 10 12 plaque-forming units (pfu)/recombinant adenovirus were administrated via tail vein injection. For each virus (Ad-shLacz or Ad-shG9a), a group of 4 -5 mice were injected with the same dose treatment. 14 days after injection, mice were sacrificed around Zeitgeber time 8 h following either overnight fasting or refeeding for 16 h. Both serum and liver tissues were harvested for protein analysis.
Primary Hepatocyte Isolation-Primary mouse hepatocytes (PMHs) were isolated by a two-step collagenase digestion with 100 units/ml collagenase in HBSS at pH 7.4. After dissection, the liver was placed in DMEM and carefully pulled apart to release hepatocytes. Hepatocytes in DMEM were passed through a 100 m cell strainer and then spun at 50 ϫ g for 1 min. The pellet was resuspended in DMEM and then spun at 50 ϫ g for 10 min in a Percoll gradient to remove dead hepatocytes. The viable cells were washed with DMEM at 50 ϫ g for 10 min and checked by trypan blue staining. PMHs were cultured on collagen-coated plates in 5% FBS and DMEM. The adenoviral transduction was performed within 6 h after seeding. After overnight incubation, cells were switched to fresh serum-free medium and incubated for another 24 h before harvest.
Cell Culture and Cell Synchronization-Both 293T and mouse hepatoma Hepa1c1c-7 cell lines were maintained in minimum essential medium supplemented with 10% fetal bovine serum at 37°C under 5% CO 2 . The protocol for in vitro synchronization study was described previously. Briefly, the freshly seeded Hepa1c1c-7 cells were firstly transduced with Ad-shLacz or Ad-shG9a for 16 h. 50% horse serum shock was performed 24 h later. Cells then were collected for mRNA analysis at 4-h intervals between the 24 and 60 h time points postsynchronization.
Luciferase Reporter Assay-Cells were plated in a 24-well plate overnight before transfection with mFgf21-WT or -D-box deletion mutant promoter luciferase reporter alongside either overexpression or shRNA vectors using Lipofectamine 2000 (Invitrogen). 48 h post-transfection, cells were lysed for luciferase activity assay measurement on a BioTek Synergy 2 microplate reader. The ␤-galactosidase construct was also co-transfected in each well for normalizing luciferase activity.
Immunoprecipitation (IP) and Immunoblotting (IB)-The standard immunoprecipitation method has been described previously (35). For detecting the protein interaction between FLAG-E4BP4 and HA-G9a, 293T cells were first transfected with both expression plasmids at a 1:1 ratio and then lysed in FLAG-IP buffer 48 h later. Cell lysates were then incubated with FLAG-M2-agarose beads (Sigma) overnight at 4°C. The beads were washed five times in FLAG-IP buffer and eluted in 30 l of 2ϫ SDS loading buffer. For IP of endogenous proteins, liver tissues or cell pellets were lysed in ice-cold radioimmune precipitation assay buffer supplemented with 1ϫ protease inhibitor and 50 mM NaF and incubated on ice for 20 min. Protein lysates were cleared by centrifugation at 14,000 rpm at 4°C for 10 min. The supernatants were collected and quantified using the Bio-Rad protein assay kit. Cell lysates were then incubated with specific antibodies overnight at 4°C. The protein complex was captured by adding 30 l of Protein A-Sepharose beads and incubating at 4°C for 1 h. The beads were washed five times in radioimmune precipitation assay buffer and eluted in 30 l of 2ϫ SDS loading buffer. Western blotting was performed to detect the presence of targeted proteins.
Statistical Analysis-All of the luciferase assays were done in triplicates. Luciferase readings were normalized to ␤-galactosidase activity for each well. Three individual replicates were performed for each treatment in FGF21 ELISA. The results were indicated as mean Ϯ S.E. To compare two groups, p Ͻ 0.05 was considered statistically significant for Student's t test.

E4BP4 Represses Hepatic Fgf21 Expression in Vivo-
We previously established that E4BP4 represses Fgf21 via directly binding to a D-box cis element of its promoter in the mouse hepatoma Hepa1c1c-7 cells (9). In the mouse liver, we similarly detected direct binding of E4BP4 protein to the promoter of Fgf21 by ChIP assay, suggesting E4BP4 might regulate Fgf21 transcription in whole animals. To assess the in vivo role of E4BP4 in Fgf21 regulation, we examined the Fgf21 expression in E4bp4 Ϫ/Ϫ mice. The loss of E4BP4 expression was confirmed by the lack of E4BP4 protein in the liver (Fig. 1A). In comparison with 3-month-old WT male mice on regular chow, serum FGF21 levels in male E4bp4 Ϫ/Ϫ mice were significantly higher (Fig. 1B), consistent with the higher levels of Fgf21 mRNA in the liver (Fig. 1C). Therefore, we established E4BP4 as a physiological regulator of Fgf21 expression in the liver.
Because it was reported that circadian transcription repressors, including REV-ERB␣ and PER1, function by recruiting histone deacetylases (HDACs) as co-repressors (39,40), we hypothesized that E4BP4-mediated repression of Fgf21 also requires a corepressor protein or a repression complex to achieve the optimal effect. To that end, we first examined the role of HDACs in E4BP4-mediated FGF21 repression. To our surprise, neither trichostatin A (inhibitor of class I and II HDACs) nor nicotinamide (inhibitor of class III HDACs) could  FEBRUARY 22, 2013 • VOLUME 288 • NUMBER 8 block the E4BP4-dependent repression of the Fgf21 promoterdriven luciferase construct (Fgf21-luc) activity (Fig. 2, A and B), suggesting that HDACs may not be required for E4BP4 repression function. In contrast, a histone methyltransferase inhibitor, BIX01294 (41), completely reversed E4BP4-dependent repression on Fgf21-luc (Fig. 2C). BIX01294 is a reversible specific inhibitor of G9a, which creates a repressive milieu for transcription by enhancing H3K9me2 of target promoters. We therefore examined the level of H3K9me2 on the Fgf21 promoter when E4BP4 level is elevated. 48 h post-transduction with either Ad-E4bp4 or Ad-GFP control, we assayed the histone modification level of the Fgf21 promoter in Hepa1 cells by ChIP using anti-H3K9me2 antibody. Compared with Ad-GFP control, Ad-E4bp4-transduced cells showed a drastic increase in the level of H3K9 dimethylation around the 5Ј-untranslated region (UTR) of the Fgf21 promoter (19-fold) and transcription start site (TSS) (5-fold). In contrast, there was no change in the H3K9me2 level around the 3Ј-UTR region (Fig. 2D). Together, our results suggest that histone methyltransferase G9a is a potential corepressor protein involved in E4BP4-dependent suppression of Fgf21.

E4BP4-G9a Complex Represses Fgf21 Expression
As a major histone methyltransferase targeting H3K9, G9a has mainly been studied for its epigenetic effects on stem cell differentiation, cell fate determination, and heterochromatin formation (24). Very little is known about its function in metabolic regulation. Previous work has shown that G9a acts as a corepressor protein for the nuclear receptor SHP (small heterodimer protein) to repress Cyp7a expression in the bile acid biosynthesis pathway (29). To test whether G9a is involved in E4BP4-dependent repression, we first tested whether these two proteins form a protein complex by overexpressing both G9a and E4BP4 in 293T cells and performing IP with antibodies. Indeed, we detected a strong interaction between FLAG-tagged E4BP4 and HA-tagged G9a (Fig. 3A). In contrast, no specific interaction was detected between E4BP4 and LSD1 (lysine demethylase 1) (Fig. 3B). To map the region of E4BP4 that interacts with G9a, we generated an E4BP4 truncation mutant without its C-terminal repression domain R-del (⌬-R). Such a mutant no longer interacts with G9a protein, indicating that the C-terminal region is required for interaction of E4BP4 with G9a  The potential interaction between FLAG-E4BP4 and HA-LSD1 was similarly assayed in transiently transfected 293T cells. IP was performed with anti-FLAG antibody. The presence of HA-LSD1 was detected by immunoblotting with anti-HA antibody. NS, nonspecific signal. C, the C-terminal repression domain of E4BP4 is required for interaction with G9a. The HA-G9a expression vector was co-transfected with GFP, FLAG-E4bp4-WT, or FLAG-E4bp4-⌬-R (amino acids 1-380) expression vector. IP was performed as usual with anti-FLAG antibody. The presence of HA-G9a was detected by immunoblotting with anti-HA antibody. D, insulin has no effect on interaction between E4BP4 and G9a. Interactions between FLAG-E4BP4 and HA-G9a were tested in the presence of insulin treatment. 293T cells were first transfected with FLAG-E4bp4 and HA-G9a vectors. 24 h later, cells were switched to serum-free medium and treated with 100 nM insulin for 16 h before IP with anti-FLAG antibody. The presence of HA-G9a was detected by immunoblotting with anti-HA. (Fig. 3C). Based upon our previous finding that E4BP4 is required for insulin-mediated repression of Fgf21 (9), we asked whether insulin could stimulate interaction of E4BP4 with G9a. When both proteins were transiently overexpressed in 293T cells via transfection, treatment of insulin did not impact the E4BP4-G9a complex formation, indicating that insulin signaling is not required for E4BP4-G9a interaction (Fig. 3D). To determine whether these two proteins interact with each other in vivo, we tested both Hepa1 cells and PMHs but failed to detect protein-protein interaction between the endogenous E4BP4 and G9a proteins (data not shown), possibly due to relative low abundance of G9a.
G9a Represses Fgf21 Expression in Hepatocytes-So far, our results suggest that the C-terminal region of E4BP4 can interact with G9a in cells, prompting us to ask whether G9a is involved in E4BP4-mediated repression. We first asked whether manipulation of G9a expression affects the Fgf21 promoter activity and mRNA expression. Overexpression of G9a-WT via transient transfection suppressed the Fgf21 promoter as efficiently as overexpression of E4bp4 (Fig. 4A). Moreover, G9a repression is dependent on its enzymatic activity because we did not detect any repression of the Fgf21 promoter activity in cells expressing the G9a-⌬SET enzyme-dead mutant with deletion of its SET domain, which has been shown to be critical for G9a-mediated H3K9 dimethylation (42)(43)(44) (Fig. 4B). The expression of both G9a-WT and -⌬SET mutant was confirmed by immunoblotting with HA antibody (data not shown). In addition, suppression of G9a enzymatic activity by BIX01294 led to a dose-dependent activation of the Fgf21-luc reporter in 293T cells (Fig.  4C). To test the role of G9a on the endogenous Fgf21 expression, we used adenoviral shG9a to knock down expression of G9a in freshly isolated PMHs. In Ad-shG9a-transduced PMHs, mRNA G9a expression was reduced by about 80% in comparison with control shLacz, whereas Fgf21 mRNA was elevated by 7-fold, indicating that G9a plays a significant repressive role on Fgf21 transcription (Fig. 4D). We previously showed that depletion of E4bp4 expression leads to dysregulated circadian oscillations of Fgf21 mRNA in synchronized Hepa1 cells (9). To examine the role of G9a in Fgf21 oscillations, we used Ad-shG9a to deplete G9a and synchronized Hepa1 cells for mRNA measurement. Between 24 and 48 h, Ad-Lacz-transduced control cells displayed normal oscillations of Fgf21 mRNA. However, in the case of G9a shRNA knockdown, the Fgf21 mRNA oscillated at higher amplitude and peaked at both 32 and 44 h (Fig. 4E). To test whether G9a is present on the endogenous Fgf21 promoter, we performed a ChIP assay with anti-G9a in mouse liver tissues from refed mice. Indeed, we detected clear G9a binding to the Fgf21 promoter during refeeding (Fig. 4F). Taken together, our data support a direct role of G9a in down-regulating the promoter activity and mRNA expression of Fgf21 in hepatocytes.
G9a Is Required for Refeeding-induced Repression of Fgf21 in the Liver-Finally, we sought to test whether G9a regulates Fgf21 expression in vivo. We injected mice with Ad-shG9a control and studied its effect on metabolic parameters and hepatic  (n ϭ 3). F, occupancy of G9a on the Fgf21 promoter in the liver. G9a binding to the Fgf21 promoter in the refed mouse livers was detected by a ChIP assay with anti-G9a antibody. FEBRUARY 22, 2013 • VOLUME 288 • NUMBER 8

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Fgf21 expression during a fasting-refeeding cycle. Knockdown of G9a in the liver was confirmed by QPCR analysis (Fig. 6A). G9a knockdown had no effect on body weight and plasma glucose levels (data not shown) but significantly increased ␤-hydroxybutyrate, a ketone body, during refeeding (Fig. 6B). More importantly, G9a knockdown abolished the refeeding-induced down-regulation of Fgf21 (Fig. 6C) in comparison with Ad-sh-Lacz control. Because G9a is necessary for maintaining H3K9me2, a repressive histone mark on the chromatin, we determined how acute knockdown of G9a alters the levels of H3K9me2 around the Fgf21 promoter during refeeding. Indeed, we observed a significant decrease in H3K9me2 around the 5Ј-UTR region and TSS of the Fgf21 promoter in the refed liver tissues after G9a shRNA knockdown (Fig. 6D), in parallel with elevation of Fgf21 expression. However, a similar H3K9me2 level was found around the exon 2 region of the Fgf21 gene. In summary, we concluded that G9a depletion leads to increased Fgf21 expression and reduced dimethylation of H3K9 of its promoter in the liver during refeeding.

DISCUSSION
In this report, we uncovered the novel role of histone methyltransferase G9a in regulating the expression of Fgf21, an important metabolic regulator. In response to refeeding and insulin stimulation, E4BP4 recruits G9a to dimethylate the promoter region of the Fgf21 gene and represses its transcription in the mouse liver, whereas loss of G9a-dependent H3K9me2 facilitates transcription of Fgf21 by PPAR␣ during fasting (Fig. 7).
Regulation of Fgf21 Expression during Normal and Diseased States-Given the multiple effects of FGF21 on carbohydrate and lipid metabolism, elucidation of regulation pathways of Fgf21 induction is important for identifying novel therapeutic targets during pathogenesis of obesity and diabetes. In transgenic mice, overexpression of Fgf21 improves insulin sensitivity and lowers glucose concentration (45). However, Fgf21 global knockout did not show a diabetic phenotype, although mice displayed a defect in lipid metabolism upon ketogenic diet treatment (46). In diabetic and obese conditions, both Fgf21 mRNA and serum FGF21 levels are paradoxically elevated, indicative of development of peripheral FGF21 resistance in the context of obesity (47)(48)(49). Nuclear receptors, including

E4BP4-G9a Complex Represses Fgf21 Expression
PPAR␣ and farnesoid X receptor, are important activators of Fgf21 in response to increased levels of fatty acids and bile acid during high fat and low carbohydrate feeding (50). ATF4 induces Fgf21 expression upon amino acid deprivation (51), whereas liver X receptor represses Fgf21 expression during a cholesterol-rich diet (52). Our work demonstrates that, by inhibiting G9a enzyme via either shRNA or a small chemical compound (BIX01294), Fgf21 expression is potently induced in hepatocytes, indicating G9a as a novel epigenetic modifying enzyme for Fgf21 expression. Although so far there is no study directly showing that G9a contributes to obesity or diabetes, loss of JHDM2a, a demethylase of H3K9me2, promotes obesity and metabolic syndrome in mice (53,54), suggesting that this particular histone modification and associated modifying enzymes are involved in the pathogenesis of obesity. FGF21, like other insulin-responsive genes, might undergo a dynamic epigenetic modification during fasting-feeding cycles in order to achieve a robust amplification. It can be envisioned that the promoter of Fgf21 is capable of being turned off or on efficiently in response to hormone action. We hypothesize that such control requires concerted activities of transcription factors, histone-modifying enzymes, and chromatin-remodeling enzymes. Our future work will use epigenetic approaches to discover specific components and their activities on the Fgf21 promoter during the switch between fasting and feeding cycles.
E4BP4 Couples Food Intake with Suppression of Metabolic Genes-As an IL3-inducible factor initially identified in lymphocytes, E4BP4 is also a first degree circadian output oscillator and controls circadian cycling of a number of circadian target genes (55). In cultured hepatocytes, E4bp4 mRNA expression is diurnal and anti-phase to that of Fgf21 and is highly induced by insulin treatment (9), raising the possibility that E4BP4 may combine both circadian and nutritional signals to control metabolism. It would be interesting to test whether circadian regulation of E4BP4 in the liver is impaired in the insulin-deficient condition, such as in liver-specific insulin receptor knockout mice. Induction of Fgf21 is associated with fatty acid oxidation, lipolysis, and ketogenesis during fasting. During refeeding, E4BP4 might repress Fgf21 expression as a circadian regulator to coordinate lipid metabolism with food intake during the dark phase of circadian night. During fasting, we suspect that disruption of the E4BP4-G9a complex and dissociation from the Fgf21 promoter is also required for elevated Fgf21 expression besides PPAR␣-mediated transactivation. It is likely that E4BP4 is suppressed during fasting via either transcriptional repression or enhanced protein degradation.
Histone Modifiers in Circadian Regulation and Cycles of Fasting and Refeeding-Epigenetic modification has emerged as a novel regulatory mechanism in circadian-dependent transcription. The NAD-dependent histone deacetylase SIRT1 interacts with not only the BMAL1-CLOCK complex but also the PER2 protein, suggesting that SIRT1 is an integral part of the molecular clock (56,57). SIRT1 in fact plays a positive role in regulating Fgf21 gene expression by enhancing PPAR␣ activity in hepatocytes (58). However, we did not detect any effects of SIRT1 inhibition by nicotinamide on the E4BP4-dependent repression of Fgf21, indicating that E4BP4 represses Fgf21 independently of SIRT1. Several studies have already explored the role of histone methylation in circadian-associated transcription. For example, MLL (mixed lineage leukemia 1) and EZH2 (enhancer of zeste 2), two enzymes targeting histone methylation, have been identified to interact with the core clock proteins and modulate circadian transcription (59,60). Throughout the literature, the epigenetic function of G9a has been associated with maintaining stem cell differentiation and heterochromatin formation. Very little is known about the biological function of G9a in the postdifferentiation state. Our report is the first to report that G9a regulates gene oscillations of a metabolic regulator in the liver via interaction with a known circadian protein. The widely available small molecule inhibitors of G9a with high specificity make G9a an ideal target for treating circadian-relevant or metabolic diseases. Because FGF21 has been shown to have diverse functions in white adipose tissue, brown adipose tissue, and the central nervous system (61-63), it will be of great interest to determine whether G9a suppresses Fgf21 expression in a similar fashion in other tissues in future studies.  FEBRUARY 22, 2013 • VOLUME 288 • NUMBER 8