De Novo DNA Methyltransferase DNMT3b Interacts with NEDD8-modified Proteins*

DNA methylation and histone modifications play an important role in transcription regulation. In cancer cells, many promoters become aberrantly methylated through the activity of the de novo DNA methyltransferases DNMT3a and DNMT3b and acquire repressive chromatin marks. NEDD8 is a ubiquitin-like protein modifier that is conjugated to target proteins, such as cullins, to regulate their activity, and cullin 4A (CUL4A) in its NEDD8-modified form is essential for repressive chromatin formation. We found that DNMT3b associates with NEDD8-modified proteins. Whereas DNMT3b interacts directly in vitro with NEDD8, conjugation of NEDD8 to target proteins enhances this interaction in vivo. DNMT3b immunoprecipitated two major bands of endogenously NEDDylated proteins at the size of NEDDylated cullins, and indeed DNMT3b interacted with CUL1, CUL2, CUL3, CUL4A, and CUL5. Moreover, DNMT3b preferentially immunoprecipitated the NEDDylated form of endogenous CUL4A. NEDD8 enhanced DNMT3b-dependent DNA methylation. Chromatin immunoprecipitation assays suggest that DNMT3b recruits CUL4A and NEDD8 to chromatin, whereas deletion of Dnmt3b reduces the association of CUL4A and NEDD8 at a repressed promoter in a cancer cell line.

DNA methylation plays an important role in cellular differentiation and development (for a review, see Ref. 1), parental imprinting, X chromosome inactivation, silencing of endogenous retroviruses as well as foreign DNA, and preservation of genome integrity. Changes in the DNA methylation pattern are associated with human cancers, where there is global hypomethylation and promoter-specific hypermethylation (for a review, see Ref. 2). So far, three DNA methyltransferases (DNMTs) 2 have been identified in mammalian cells: DNMT1, also known as the maintenance methylase (3,4), and DNMT3a and DNMT3b, the two de novo DNA methyltransferases (5). Purified recombinant DNMT3a and DNMT3b can methylate DNA in vitro without preference for hemimethylated DNA (6 -8). The de novo methylation activity of DNMT3a and -3b was also demonstrated in vivo, where ectopic expression leads to methylation of episomal plasmid DNA (9). Inactivation of both genes blocks de novo methylation in embryonic stem cells and early mouse embryos, and these double homozygous embryos die before embryonic day 11.5 (10).
DNMT3a and DNMT3b are highly related proteins that share a PWWP motif (highly conserved proline-tryptophantryptophan-proline motif) and an ATRX-like plant homeodomain (PHD) in the N terminus regulatory domain. Disruption of the PWWP motif prevents the association of DNMT3a and -3b with pericentric heterochromatin and abolishes their ability to methylate the major satellite repeats (11). The ATRX-like plant homeodomain in DNMT3a and -3b shares homology with a similar region found in ATRX (12) but lacks the characteristic histidine residue present in typical plant homeodomain fingers (13). The ATRX-like plant homeodomain is responsible for most of the transcriptional repression mediated by DNMT3a and 3b (14) and for interaction with HDAC1 (histone deacetylase-1) and RP58 (a putative transcriptional repressor) (15). Although there is clear evidence for the important role DNA methylation plays in development and cancer, it is still unclear what leads to promoter hypermethylation in cancer and how the enzymatic activity and localization of the DNA methyltransferases are regulated.
NEDD8 (neural precursor cell-expressed developmentally down-regulated 8) or RUB1 (related to ubiquitin 1) is the closest homolog to ubiquitin, with 60% identity and 80% homology (16). NEDD8, similar to ubiquitin and ubiquitin-like proteins, can be covalently attached to other proteins in a process called NEDDylation. NEDDylation is essential for the viability of most model organisms, including Schizosaccharomyces pombe, Caenorhabditis elegans, Drosophila, Arabidopsis, and mice (17)(18)(19)(20)(21)(22). NEDD8 is conjugated to target proteins in order to regulate their activity, through modulation of protein-protein interactions. The most abundant substrates of NEDD8 are a family of scaffold proteins, called cullins. Cullins are essential for the assembly of several multiprotein E3 ubiquitin ligase complexes that are active only when the cullins are modified by NEDD8 (23)(24)(25)(26). Immunocytochemical analysis showed that NEDD8conjugated proteins are highly enriched in the nucleus, suggesting nuclear functions for NEDD8. Recent papers have revealed essential roles for NEDD8 modification of CUL4A in heterochromatin formation in yeast (27) and heterochromatin formation as well as DNA methylation in Neurospora (28). In both cases, deletion of Cul4 disrupts heterochromatin formation, and the mutant strains can be complemented with Cul4 but not with Cul4 that cannot be NEDDylated. The mammalian homolog of Cul4, CUL4A, was shown to be associated with repressed chromatin, and its suppression by small interfering RNA (siRNA) reduced histone 3 Lys 9 and Lys 27 methylation, which are markers of heterochromatin (29).
Here we describe the association of DNMT3b with NEDDylated proteins. We have found that DNMT3b is associated with endogenous NEDD8-modified proteins at a size between 85 and 90 kDa, the size of NEDDylated cullins, and indeed DNMT3b interacts with CUL1, CUL2, CUL3, CUL4A, and CUL5. We confirmed that DNMT3b interacts with endogenous CUL4A and mapped the interaction to the C terminus of CUL4A. Moreover, DNMT3b interacts preferentially with the NEDDylated form of CUL4A. Expression of DNMT3b increased the recruitment of CUL4A and NEDD8 to chromatin. Chromatin immunoprecipitation assays in cells with knock-out of Dnmt3b showed reduced association of CUL4A and NEDD8 with a repressed promoter. Furthermore, by modulating the NEDDylation pathway, we were able to regulate de novo methylation. These results support a connection between DNA methylation and protein NEDDylation.
DNA Methyltransferase Assays-Assays in transfected HEK 293T cells were performed as described previously (37). For experiments involving siRNA, cells were transfected with siRNA control or siRNA against NAE1/APPBP1 (SMARTpool, DHARMACON Inc.) by Effectene reagent (Qiagen). After 7 h, transfected cells were replated and cultured overnight. The next day, cells were transfected again with siRNAs plus pREP8-RTA and plasmid expressing DNMT3b. At 24 h post-transfection, cells were replated onto 10-cm plates and cultured for another 3 days. DNA was purified by Hirt extraction and digested by HhaI prior to Southern blotting or real-time PCR with primers (sense, AGCGTATGCTTCAGGACCAC; antisense, ACAGATTGTGGCATTCGGTA) overlapping the HhaI restriction site in plasmid pREP8-RTA.
Chromatin Immunoprecipitation Assays-ChIP assays with HCT cell lines were performed on HCT 116 or HCT 116 with a deletion of both alleles of Dnmt3b (3b KO). ChIP assays with HEK 293T cells were performed on cells that were transfected with a plasmid that contains 5xGAL4 UAS (5xGAL4TKCAT) with or without GAL4-DNMT3b expression vector. Antibodies against NEDD8 and CUL4A were used to immunoprecipitate endogenously expressed proteins. ChIP assays were performed essentially as described previously (40), except that after proteinase K, the DNA was purified with a PCR purification kit (Ultra Clean PCR clean-up kit, MO BIO Laboratories, Inc.). ChIP DNA was analyzed by real-time PCR (iCycler, Bio-Rad) on products generated with SYBR Green PCR master mix (Applied Biosystems) and primers for PCDH10 promoter (sense, GCTCGGTGTCCTTCATCTTC; antisense, ATCGC-TGGCCAGACAAGTAT) (41) or 5xGAL4 UAS (sense, CTC-TAGAGTCGAGCTAGAGT; antisense, CCCCTGAAG-CTTGCATGCC).

DNMT3b and DNMT3a
Associate with NEDD8-modified Proteins-Because the cellular DNMTs can lead to promoter hypermethylation and transcription silencing, their activity and recruitment to different promoters must be tightly regulated. Previously, it was shown that DNMT3a (42,43), DNMT3b (44), and recently DNMT1 (45) are modified by the ubiquitin-like protein SUMO-1. We investigated whether the DNMTs (DNMT1, DNMT3a, and DNMT3b) are subjected to regulation by other small ubiquitin modifiers and discovered an interaction with NEDD8-modified proteins. Cells were transfected with FLAG-NEDD8 and HA-DNMTs, and cell extracts were immunoprecipitated with anti-FLAG-conjugated beads to immunoprecipitate NEDD8 and NEDD8-associated proteins.
Both DNMT3a and DNMT3b were immunoprecipitated with NEDD8 ( Fig. 1, top), whereas DNMT1 was not efficiently immunoprecipitated under these conditions. The co-immunoprecipitation of DNMT3b with NEDD8 can be explained by either interaction or modification of DNMT3b by NEDD8. To distinguish between these two possibilities, we performed a reciprocal immunoprecipitation. Extracts from cells transfected with HA-Dnmt3b were immunoprecipitated with anti-HA-conjugated beads to immunoprecipitate DNMT3b and associated endogenous NEDD8 and NEDD8conjugated proteins. We observed that DNMT3b co-immunoprecipitated with NEDD8-modified proteins of ϳ85-90 kDa (Fig. 2, top). These NEDDylated bands are smaller than the size of HA-tagged DNMT3b (ϳ130 kDa), making it unlikely that NEDDylated DNMT3b is being detected. These experiments suggest that DNMT3b associates with NEDD8-modified proteins.
DNMT3b Preferentially Interacts with Conjugated NEDD8-If NEDD8 modification regulates the interaction of DNMT3b with different proteins, DNMT3b should preferentially interact with conjugated NEDD8 over unconjugated free NEDD8. We performed immunoprecipitations to examine whether a mutant NEDD8 that cannot be conjugated is able to co-immunoprecipitate DNMT3b. Because the diglycine in NEDD8 (as well as in ubiquitin and ubiquitin-like proteins) is essential for conju-gation, we introduced a deletion of the diglycine (NEDD8⌬ GG). Although DNMT3b co-immunoprecipitated efficiently with wild type NEDD8, it was not efficiently co-immunoprecipitated with the ⌬GG mutant (Fig. 3A, top). This result indicates that DNMT3b preferentially interacts with conjugated NEDD8.
The above results demonstrate that DNMT3b is associated with NEDD8 in mammalian cells. Because proteins are often are found in multisubunit protein complexes and are immunoprecipitated with their protein complex, the interaction that we observed could be mediated through additional proteins. In order to test whether DNMT3b and NEDD8 interact directly, we performed a series of pull-down assays. Bacterially expressed and purified recombinant His 6 -NEDD8 was incubated with GST-DNMT3b or GST that were immobilized on glutathione beads. Bound proteins were eluted and analyzed by Western blotting (Fig. 3B). Recombinant NEDD8 was bound to GST-DNMT3b and not GST alone, suggesting that direct interaction between NEDD8 and DNMT3b can occur.
Protein NEDDylation is a balance between NEDDylation and de-NEDDylation processes. In a DEN1 (NEDD8 de-NEDDylating enzyme, also known as NEDP1 and SENP8) null mutant in Drosophila, many cellular proteins become highly NEDDylated (46), suggesting that many more proteins are NEDDylated in the cell than are currently recognized. In order to push the balance toward protein NEDDylation, we overexpressed FLAG-NEDD8. Cells were co-transfected with HA-DNMT3b and FLAG-NEDD8, and cell extracts were immunoprecipitated with anti-HA-conjugated beads. We observed that DNMT3b co-immunoprecipitated with multiple NEDD8-modified proteins when the blots were probed with anti-FLAG for FLAG-NEDD8-conjugated proteins (Fig. 3C, top). CULLIN-5 (CUL5), a known NEDD8-modified protein, served as a control (Fig.  3D). In contrast to the many NEDDylated proteins associated with DNMT3b, CUL5 immunoprecipitated as a single NEDDylated band (Fig. 3D, top), as expected for a NEDDylated protein.
Overexpression of NEDD8 leads to the appearance of the   NOVEMBER 19, 2010 • VOLUME 285 • NUMBER 47 expected higher molecular weight band of CUL5 (Fig. 3D, bottom). The difference in behavior of DNMT3b and CUL5 supports the notion that DNMT3b interacts with NEDD8-conjugated proteins.

DNMT3b Associates with NEDDylated Proteins
DNMT3b Interacts with NEDDylated Proteins through a Region between Its ATRX-like PHD and DNA Methyltransferase Domains-To further validate interaction of DNMT3b with NEDDylated proteins, we performed a series of immunoprecipitations with several different DNMT3b deletion mutants. HEK 293T cells were transfected with FLAG-NEDD8 together with GAL4-DNMT3b or the N terminus of DNMT3b (GAL4-DNMT3b) (aa 1-515), and protein extracts were subjected to immunoprecipitation with anti-FLAG-conjugated beads (Fig.  4A). Although GAL4-DNMT3b was co-immunoprecipitated with NEDD8, GAL4-DNMT3b 1-515 was not. This result shows that there is no interaction domain within the N terminus of DNMT3b. In order to narrow down the interaction domain, we next used a series of mouse DNMT3b mutants (Fig.  4B). Full-length (FL) DNMT3b as well as DNMT3b 1-583 and DNMT3b deleted for the ATRX-like PHD domain (⌬433-532) were able to interact with NEDD8 in a co-immunoprecipitation assay, but the mutant DNMT3b 1-433 failed to interact with NEDD8. This experiment shows that mouse DNMT3b has the ability to associate with NEDD8-modified proteins and that a small region between 532 and 583 of mouse DNMT3b is required for interaction. This set of assays maps the region between the ATRX-like PHD domain and the catalytic domain of DNMT3b as the interaction domain for NEDDylated proteins (Fig. 4C).
Because conjugation of NEDD8 is typically on a lysine residue, we mutated the two lysines K540R and K562R present in the aa 532-583 region of DNMT3b. Both mutants retained their ability to associate with NEDD8 (Fig. 4D), further strengthening the concept that DNMT3b interacts with NEDD8-modified proteins and is not modified by NEDD8.
NEDD8 Increases DNMT3b-dependent DNA Methylation-After confirming the interaction between DNMT3b and NEDD8-conjugated proteins, we sought to test the role of NEDD8-modified proteins in DNA methylation. We performed an in vivo methylation assay (9), using HEK 293T cells transfected with an episomal target plasmid DNA containing a known methylation-regulated herpesvirus promoter (37,47). We co-transfected NEDD8 in combination with DNMT3b and the target plasmid (pREP8-RTA). Five days after transfection, DNA was isolated from the cells and subjected to methylationsensitive restriction enzyme digestion (HhaI), and the digested DNA was analyzed by Southern blotting (Fig. 5A) or by real-time PCR using primers surrounding the HhaI restriction site (Fig. 5B). Exogenous expression of NEDD8 alone did not lead to any detectable methylation because the assay is dependent on co-expression of de novo methyltransferase in these cells. As expected, expression of DNMT3b resulted in detectable DNA methylation. Interestingly, co-expression of NEDD8 and DNMT3b resulted in a more profound DNA methylation, suggesting that NEDD8-conjugated proteins play a role in DNMT3b-dependent DNA methylation. An in vivo DNA methylation assay was also performed where the first enzyme (E1) in the NEDDylation pathway, NAE1, was suppressed by siRNA. Suppression of NAE1 levels by siRNA was confirmed by reverse transcription followed by real-time PCR (Fig. 5C). Suppression of NAE1 inhibited DNMT3b-dependent DNA methylation (Fig. 5D), as compared with siControl. Interestingly, the level of DNA methylation was inhibited to the same level that NAE1 was suppressed. These experiments suggest that NEDDylation can control DNA methylation; higher levels of NEDDylation enhance DNA methylation, whereas lower levels of NEDDylation attenuate DNA methylation.

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from cells transfected with HA-DNMT3b were immunoprecipitated with anti-HA-conjugated beads, and endogenously co-immunoprecipitated proteins were detected with anti-NEDD8, anti-CUL5, and anti-CUL4A antibodies. We found that DNMT3b interacts with endogenous CUL5 and CUL4A as well as with NEDD8 (Fig. 6A).
To examine whether other cullin family members are able to interact with DNMT3b, cells were co-transfected with FLAGtagged DNMT3b and HA-tagged CUL1, CUL2, CUL3, and CUL5 (Fig. 6B). Cell extracts were immunoprecipitated with anti-FLAG-conjugated beads and blotted with anti-HA antibody. CUL1, CUL2, CUL3, and CUL5 were detected in the immunoprecipitates. These data demonstrate that DNMT3b has the ability to interact with multiple cullins, the most abundant targets for NEDDylation in the cell.
DNMT3b Preferentially Interacts with NEDDylated CUL4A-In order to check the role of NEDD8 modification on DNMT3b and CUL4A interaction, cell lysis and immunoprecipitation procedures were performed with or without NEM (N-ethylmaleimide). NEM is a cysteine protease inhibitor that inhibits deconjugation of ubiquitin and ubiquitin-like proteins and therefore is used routinely to maintain NEDD8 modification.
Cells were transfected with HA-DNMT3b, and 2 days after transfection, the cells were collected into two tubes; in one tube, protein extract was prepared and immunoprecipitated with NEM, and in the second tube, immunoprecipitation was done without NEM. Anti-CUL4A was used to detect endogenous CUL4A that was co-immunoprecipitated with DNMT3b. Two protein bands of CUL4A were detected in the input in the presence of NEM, but the slow migrating band corresponding to NEDDylated CUL4A was markedly reduced without NEM (Fig. 7A, top, lanes 3  and 4). Interestingly, DNMT3b was associated specifically with NEDDylated CUL4A and only in the presence of NEM (Fig. 7A, top,  lanes 1 and 2). The immunoprecipitation was also blotted with anti-NEDD8 antibody (Fig. 7A, middle) to confirm that the modification is NEDDylation. This result indicates that DNMT3b interacts preferentially with the NEDDylated form of endogenous CUL4A.
An Inactive CUL4A Mutant Impairs DNMT3b-dependent DNA Methylation-Deletion of aa 1-100 from the N terminus of CUL4A abolishes its ability to bind to DDB1 and to ubiquitinate substrates such as CDT1 (48). DNMT3b interacts with this mutant (Fig. 7C); therefore, this mutant may act as a dominant negative. We used this mutant to examine the importance of CUL4A in DNMT3b DNA methylation in vivo. Cells were transfected with DNMT3b and CUL4A ⌬ N100 together with the target plasmid, and methylation of the target DNA was analyzed by HhaI digestion followed by real-time PCR (Fig. 7E). The expression of CUL4A ⌬ N100 indeed impaired DNMT3bdependent DNA methylation. This suggests a role for active CUL4A in DNA methylation by DNMT3b. . NEDD8 enhances DNMT3b-dependent DNA methylation. A, pREP8-RTA target DNA was transfected into HEK 293T cells with or without NEDD8 or DNMT3b. Plasmid DNA was isolated by Hirt extraction 5 days after transfection and digested with the methylation-sensitive restriction enzyme HhaI, and the DNA was examined by Southern blotting. M, methylation-induced bands; U, unmethylated bands. B, analysis of the HhaI-digested DNA (from A) by real-time PCR using primers surrounding an HhaI restriction site in the RTA promoter. The data are expressed as a ratio of the signal obtained from HhaI-digested versus undigested DNA. C, cells were transfected with siRNA control or siRNA against NAE1. After 72 h, RNA was isolated, and reverse transcription real-time PCR was performed. The ratio of NAE1 level relative to actin is presented. D, in vivo methylation assay was performed as in A, except that cells were also transfected with siRNA control or siRNA against NAE1. Error bars, S.D.

DNMT3b Associates with NEDDylated Proteins
Recruitment of CUL4A and NEDD8 to Chromatin by DNMT3b-One possible outcome of the interaction between DNMT3b and CUL4A is that DNMT3b has a role in the recruitment of CUL4A to repressed promoters. In order to test a direct role for DNMT3b in the recruitment of NEDD8 and CUL4A to chromatin, we performed ChIP assays on cells that were transfected with DNMT3b fused to the GAL4 DNA binding domain together with a plasmid that contains GAL4 consensus binding sites. Endogenous NEDD8 and CUL4A were immunoprecipitated, and their association with the plasmid DNA with or without GAL4-DNMT3b was analyzed by real-time PCR (Fig. 8, A-C). The association of both NEDD8 and CUL4A with the plasmid DNA was increased in the presence of GAL4-DNMT3b. These results indicate a specific role for DNMT3b in the recruitment of CUL4A and NEDD8 to chromatin.
Deletion of Dnmt3b Reduced the Association of CUL4A and NEDD8 at a Repressed Promoter-To examine whether CUL4A recruitment to a repressed promoter in cancer cells is also dependent on DNMT3b, we performed the ChIP assay in two cell lines, HCT 116 (human colon carcinoma) or HCT 116 with a knock-out of Dnmt3b Ϫ/Ϫ (3b KO). We found reduced association of both NEDD8 and CUL4A to a known repressed promoter (PCDH10) in the Dnmt3b Ϫ/Ϫ cells as compared with the parental cells (Fig. 8D). These results indicate that DNMT3b has a role in the recruitment of CUL4A and NEDD8 to a repressed promoter in cancer cells.

DISCUSSION
Here we describe the interaction of the de novo DNA methyltransferase DNMT3b with NEDD8-modified proteins. DNMT3b immunoprecipitates two major bands of endogenously NEDDylated proteins at the size of NEDDylated cullins, and indeed DNMT3b was found to interact with CUL1, CUL2, CUL3, CUL4A, and CUL5. Protein NEDDylation is a balance between NEDDylation and de-NEDDylation processes. When this balance is disrupted, as in the DEN1 (NEDD8 de-NEDDylating enzyme) null mutant in Drosophila, many cellular proteins become highly NEDDylated (46). We found that many NEDDylated proteins associated with DNMT3b when the balance toward NEDDylation was biased by NEDD8 ectopic expression. Although DNMT3b can interact directly with NEDD8 in vitro, the interaction is enhanced upon NEDD8 conjugation because DNMT3b immunoprecipitates less efficiently with a NEDD8 mutant that cannot be conjugated. We speculate that upon conjugation, NEDD8 changes its conformation to have higher affinity for DNMT3b.
Cullins are the most abundant NEDD8-conjugated proteins in the cell. Cullins are scaffolds for the assembly of multisubunit ubiquitin E3s that ubiquitinate numerous proteins. All cullins are NEDDylated on a conserved lysine in their C terminus domain, and modification by NEDD8 is necessary for cullin activity. Recently, several reports in yeast, Neurospora, and mammalian cells have suggested an essential role for CUL4A and its NEDDylation dependent activity in heterochromatin formation (27,29). In S. pombe, Cul4 interacts with the histone methyltransferase Clr4 that is responsible for histone 3 lysine 9 methylation across all heterochromatin domains (49). Mutations in Cul4 result in defective localization of Clr4 and a loss of silencing at heterochromatin loci. The heterochromatin defects in Cul4 mutants could not be rescued by expression of a Cul4 protein lacking NEDD8 modification, suggesting a role for a NEDDylated Cul4 in histone 3 lysine 9 methylation and heterochromatin formation (27). Recently, it was shown that Cul4 is essential for DNA methylation in Neurospora (28). Knockout of Cul4 resulted in a loss of DNA methylation, and the mutant strains were complemented by Cul4 but not by Cul4 that could not be NEDDylated. In mammalian cells, CUL4-DDB1 binds the polycomb group protein EED, a WD40 repeat  3 and 4) and in the immunoprecipitates (lanes 1 and 2). The presence of HA-DNMT3b in the immunoprecipitates was detected with anti-DNMT3b antibody (bottom panel). B, DNMT3b interacts with CUL1, CUL2, CUL3, and CUL5. FLAG-DNMT3b and HA-tagged CUL1, CUL2, CUL3, and CUL5 were cotransfected into HEK 293T cells, and cell extracts were immunoprecipitated with anti-FLAG-conjugated beads. Cullins were detected in the immunoprecipitates (panel) and the input (middle) using anti-HA antibody. Expression of FLAG-DNMT3b was detected with anti-FLAG antibody (bottom). NOVEMBER 19, 2010 • VOLUME 285 • NUMBER 47 subunit of EZH2 histone methyltransferase complex (29). The EED-EZH2-SUZ12 methyltransferase directs histone H3 methylation at Lys 9 and Lys 27 , leading to X chromosome inactivation, genomic imprinting, heterochromatin formation, and gene silencing. CUL4-DDB1 associates specifically with trimethylated histone 3 Lys 9 and histone 3 Lys 27 mononucleosomes, and inactivation of CUL4 or DDB1 significantly abolishes trimethylation at histone 3 Lys 9 and Lys 27 (29).

DNMT3b Associates with NEDDylated Proteins
The results presented here suggest that CUL4A interacts with DNA methyltransferase DNMT3b. ChIP assays revealed that expression of DNMT3b led to enhanced association of CUL4A and NEDD8 on the chromatin. The HCT-116 gastric carcinoma cell line has been extensively studied in the field of DNA methylation because of the availability of Dnmt3b and Dnmt3a knock-out derivatives (30,50). When we analyzed a known repressed and methylated promoter, PCDH10 (41), in HCT-116 cells, we found that CUL4A and NEDD8 are readily detected in association with this promoter and that knock-out of Dnmt3b reduced these associations, reinforcing the concept that DNMT3b recruits CUL4A and NEDD8 to endogenous repressed promoters. Thus, in addition to its interactions with histone methyltransferase, CUL4A also interacts with DNA methyltransferase. Although we have shown that CUL4A is recruited to chromatin by DNMT3b, this does not exclude the possibility that DNMT3b can be recruited to repressed promoters by CUL4A in different experimental systems. There is a strong correlation between histone methylation that leads to repressed chromatin and DNA methylation. Therefore, our finding that CUL4A interacts with a DNA methyltransferase is consistent with current models and extends our understanding of the complex interactions that lead to repressed methylated promoters in cancer cells.
Previously, it has been shown that DNMT1 interacts with an E3 ubiquitin ligase, UHRF1 (ubiquitin-like, containing plant homeodomain and RING finger domains 1), also known as NP95 in mice and ICBP90 in humans (51,52). This ubiquitin ligase binds histones and ubiquitinates histone 3 (53) and, through its binding to hemimethylated DNA, is essential for the recruitment of DNMT1 to chromatin during replication and to maintain DNA methylation (51,52). Here we describe an interaction between CUL4A and DNMT3b. The CUL4A ubiquitin ligase complex, consisting of CUL4A-CUL4B-DDB1-DDB2-ROC1, is responsible for H3 and H4 ubiquitination (54). This complex is also responsible for the enhanced ubiquitination of FIGURE 7. DNMT3b associates preferentially with NEDDylated CUL4A and inactive CUL4A attenuates DNA methylation. A, DNMT3b interacts preferentially with NEDDylated CUL4A. HEK 293T cells were transfected with HA-DNMT3b, and 2 days after transfection, cells were collected into two tubes; in one tube protein extract was prepared and immunoprecipitated (IP) with NEM, and the second immunoprecipitation was done without NEM. Anti-CUL4A and Anti-NEDD8 antibodies were used to detect endogenous CUL4A and NEDDylated proteins that were co-immunoprecipitated with DNMT3b, respectively. WB, Western blot. B, HEK 293T cells were transfected with FLAG-DNMT3b and Myc-CUL4A, and immunoprecipitations were performed with anti-FLAG-conjugated beads. CUL4A was detected in the immunoprecipitates (top) and the input (middle) using anti-Myc antibody. The presence of DNMT3b in the immunoprecipitation was detected with anti-FLAG antibody (bottom). C, as in B but with transfected Myc-CUL4A ⌬ N100 (deletion of aa 1-100). D, HEK 293T cells were transfected with HA-DNMT3b and CUL4A or CUL4A-DN (aa 1-440, deletion of the C terminus), and immunoprecipitations were performed with anti-HAconjugated beads. CUL4A and CUL4A-DN were detected in the immunoprecipitates (top) and the input (bottom) using anti-CUL4A antibody. E, an inactive CUL4A mutant attenuates DNMT3b-dependent DNA methylation. pREP8-RTA target DNA was transfected into HEK 293T cells with or without CUL4A ⌬ N100 or DNMT3b. Methylation of the plasmid DNA was analyzed as in Fig. 5B. H3 and H4 induced by UV irradiation. The fact that DNMT1 and now DNMT3b interact with histone ubiquitin ligase complexes may be relevant to the cellular DNA damage response. It has been shown that both SIRT1 and DNMT3b are recruited to the chromatin after DNA damage (55). Because the CUL4A complex is recruited to DNA damage though DDB1 (56), our work raises the possibility that after DNA damage, the recruitment of both SIRT1 and DNMT3b is through a NEDDylated CUL4A complex. Determination of whether histone ubiquitination also has a role in DNMT-mediated transcription repression and DNA methylation awaits further study.
In cancer cells, many promoters become aberrantly methylated through the activity of the de novo DNA methyltransferases DNMT3a and DNMT3b and acquire repressive chromatin marks. Because DNMT3a and DNMT3b have the ability to de novo methylate DNA, their activity and recruitment to different promoters must be tightly regulated. The DNMT3L protein is essential for de novo DNA methylation at maternal genomic imprints (57) and regulates the activity of DNMT3a (58) and DNMT3b (59) through chromatin recruitment (60).
De novo DNA methylation is also regulated by the recruitment of DNMT3a and DNMT3b to chromatin by Lsh (61), Myc (62), PU.1 (63) EZH2 (64) and by the Kaposi's sarcoma-associated herpesvirus latency protein, LANA (37). Here we found that expression of NEDD8 led to enhanced DNA methylation, whereas suppression of NEDDylation inhibited DNA methylation. Because this assay is dependent on DNMT3b methyltransferase activity, we can conclude that NEDD8 collaborates with DNMT3b in DNA methylation and that NEDD8 has a positive role in de novo DNA methylation. Furthermore, we have shown that this is at least partially mediated by CUL4A because a CUL4A inactive mutant that maintained its ability to bind DNMT3b had a dominant negative effect on DNMT3b-dependent DNA methylation.
The connection between protein NEDDylation and DNA methylation, revealed in this study, may also have consequences in carcinogenesis. Overexpression of CUL4A by gene amplification is found in both breast cancer and hepatocellular carcinoma (65,66). NEDD8 conjugation is increased in all highly proliferating cells tested, including several human carcinoma cell lines, as compared with normal human fibroblasts (67). It has been suggested that higher levels of NEDD8 conjugation are necessary for the high proliferative property of many, if not all, carcinoma cell lines (67). A recent report found that DNMT3b overexpression correlates with higher DNA methyltransferase activity in breast cancer cell lines (68). It will be interesting to test a possible link between DNA methylation and NEDD8 expression in different tumor types to see if both are concurrently up-regulated.