Identification and Characterization of a Family of Mammalian Methyl-CpG Binding Proteins

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Molecular and Cellular Biology, November 1998, p. 6538-6547, Vol. 18, No. 11
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Identification and Characterization of a Family of Mammalian Methyl-CpG Binding Proteins

Brian Hendrich^* and Adrian Bird

Institute of Cell and Molecular Biology, University of Edinburgh, Edinburgh EH9 3JR, Scotland

Received 24 June 1998/Returned for modification 9 August 1998/Accepted 20 August 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Methylation at the DNA sequence 5'-CpG is required for mouse development. MeCP2 and MBD1 (formerly PCM1) are two known proteinsthat bind specifically to methylated DNA via a related amino acidmotif and that can repress transcription. We describe here threenovel human and mouse proteins (MBD2, MBD3, and MBD4) that containthe methyl-CpG binding domain. MBD2 and MBD4 bind specificallyto methylated DNA in vitro. Expression of MBD2 and MBD4 taggedwith green fluorescent protein in mouse cells shows that bothproteins colocalize with foci of heavily methylated satelliteDNA. Localization is disrupted in cells that have greatly reducedlevels of CpG methylation. MBD3 does not bind methylated DNA invivo or in vitro. MBD1, MBD2, MBD3, and MBD4 are expressed insomatic tissues, but MBD1 and MBD2 expression is reduced or absentin embryonic stem cells which are known to be deficient in MeCP1activity. The data demonstrate that MBD2 and MBD4 bind specificallyto methyl-CpG in vitro and in vivo and are therefore likely tobe mediators of the biological consequences of the methylationsignal.

	INTRODUCTION

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DNA methylation is the major modification of eukaryote genomes. In vertebrates, this occurs predominantly at position 5 ofcytosines when followed by guanosine (CpG). DNA methylation canrepress transcription and for this reason has been implicatedin stable alterations of gene expression in development (3).Whereas the genomes of certain invertebrates appear to contain"compartments" of either mostly methylated or mostly unmethylatedDNA (43), the somatic genomes of vertebrates are globally methylated,with the exception of so-called CpG islands (6). CpG islandsare GC-rich regions of DNA, stretching for an average of about1 kb, which are coincident with the promoters of approximately60% of human RNA polymerase II-transcribed genes (1). Methylationof CpG islands and subsequent silencing of associated transcriptionunits have been found to occur in genes located on the inactiveX chromosome (39), genes silenced by genomic imprinting (36,38), and genes silenced in transformed cell lines and tumors(2, 8, 16, 18, 40). DNA methylation is known to playan essential role in mammalian development because mice lackinga functional gene encoding the maintenance DNA methyltransferase(DNMT) are developmentally retarded and die at midgestation (29).In contrast to the situation in somatic cells, undifferentiatedembryonic stem (ES) cells lacking a functional DNMT gene apparentlygrow normally despite containing approximately 5% of the wild-typeDNA methylation level (25, 35).

One mechanism by which DNA methylation can cause transcriptional repression is by directly interfering with the binding ofsequence-specific transcription factors to DNA. Some transcriptionfactors have been shown to be unable to bind to their target sequenceswhen methylated (14, 21). The observations that DNA methylationis capable of repressing transcription at some distance (12,23) and that repression of transgenes only occurs after chromatinassembly (11) are inconsistent with the direct mechanism andindicate that a more indirect mechanism also exists. Two proteinshave been identified, MeCP1 and MeCP2, which bind specificallyto methylated DNA in any sequence context (27, 30). Both arecapable of inhibiting transcription (9, 32). It is likelythat MeCP1 and MeCP2 are important in interpreting the signalthat methylation of DNA represents.

MeCP2 consists of a single polypeptide that contains both a methyl-CpG binding domain (MBD) and transcriptional repressiondomain (TRD) (32, 33). MeCP2 is capable of binding to a singlesymmetrically methylated CpG pair and was found to bind to chromosomesat sites known to contain methylated DNA (35). On mouse chromosomes,this is visualized as prominent binding to the highly methylatedmajor satellite located just proximal to centromeres, whereason human or rat chromosomes which do not contain highly methylatedsatellite DNAs, general chromosomal binding is observed (32).MeCP2 localization is disrupted in ES cells lacking a functionalDNMT gene, demonstrating that MeCP2 is a bona fide methyl-CpGbinding protein in vivo (35). Like DNMT-deficient ES cells,MeCP2-deficient ES cells appear to grow normally in culture butare not capable of supporting embryonic development (42). Incontrast to DNMT deficiency, however, MeCP2 deficiency is compatiblewith somatic cell viability, and certain imprinted genes knownto be misexpressed in the absence of DNMT (5, 28) are notmisexpressed in MeCP2-deficient cells (17a). These observationssuggest that the effects of DNA methylation are not solely dependenton MeCP2, as the DNA methylation-dependent transcriptional silencingobserved at imprinted loci does not appear to rely upon its presence.The known characteristics of MeCP2 point to it being responsiblefor genomewide transcriptional repression or "transcriptionalnoise reduction" (7). Its involvement in the repression ofspecific genes remains unproven.

In contrast to MeCP2, MeCP1 has been shown to require >10 methyl-CpGs to bind DNA (30), making it more likely to be involvedin DNA methylation-mediated transcriptional repression of specificgenes. Indeed, Boyes and Bird have shown that MeCP1 is capableof repressing transcription of densely methylated promoters (9).Further, MeCP1 was found to be capable of repressing transcriptionfrom sparsely methylated promoters, though the interaction isweak and can be overcome by the presence of an enhancer (10).MeCP1 activity is ubiquitous in somatic cells and tissues butis notably absent in ES cells which are also tolerant of DNMTdeficiency (30). Thus, MeCP1 is likely to be important in theDNA methylation-mediated repression of genes in somatic cells.

MeCP1 is a large protein complex of 400 to 800 kDa. Cross et al. (15) recently identified a component of MeCP1 by searchingthe XREF database (4) for sequences homologous to the MBD ofMeCP2. A human expressed sequence tag (EST) was identified andfound to encode a novel protein containing a MBD-like motif locatedat its N terminus. This protein, called MBD1 (formerly PCM1),was shown to bind methylated DNA via its MBD-like region and torepress transcription from a methylated promoter in vitro. MBD1is a component of the MeCP1 protein complex. We now report theidentification of three novel MBD-containing proteins. We showthat two of these novel proteins specifically bind methylatedDNA in vitro and colocalize with methylated sequences in vivoand are thus candidates for mediators of the effects of DNA methylationin mammalian cells.

	MATERIALS AND METHODS

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cDNA identification and cloning. Full-length human MeCP2 and the MBD region of MBD1 protein sequences were used to search the XREF database (http://www.ncbi.nlm.nih.gov/XREFdb)or dbEST directly via BLAST (NCBI BLAST Server; http://www.ncbi.nlm.nih.gov/BLAST).The murine homologue of MBD1 was not present in the EST databaseso degenerate primers designed from the amino acid sequences ofthe cysteine-rich motifs of the human MBD1 gene (primer G235 [5'-CARACNCARGARGAYTGYGG-3']and primer D355 [5'-CCNCCRAAYTTRGGYTTRTC-3']; designed by M. Carr)were used to amplify a portion of the murine cDNA. This PCR productwas then used to screen a mouse brain cDNA library (Stratagene),and full-length clones were isolated and sequenced. Approximately2 × 10⁵ plaques were plated out and lifted onto nitrocellulose filters.Filters were hybridized in Church buffer (7% sodium dodecyl sulfate[SDS], 0.5M sodium phosphate [pH 7.2]) supplemented with 15 µgof denatured salmon sperm DNA per ml at 68°C overnight and washedto a final stringency of 0.1% SDS-0.1 × SSC (1× SSC is 0.15 MNaCl plus 0.015 M sodium citrate) at 65°C.

Mbd2 and Mbd3 were identified by database screening as ESTs (accession no. Z31258 for Mbd2 and accession nos. W81894and W91000 for Mbd3). The corresponding cDNA clones (MMTEST693,403236, and 420899, respectively) were obtained and used to screenthe mouse brain cDNA library. A number of full-length clones wereisolated and sequenced for both Mbd2 and Mbd3. Human MBD2 andMBD3 sequences were identified by subsequent screening of thedbEST database with full-length Mbd2 and Mbd3 sequences. No full-lengthMBD2 or MBD3 IMAGE clones were identified in database screensso 5' rapid amplification of cDNA ends (RACE) was used to obtainthe 5' end of MBD3 by the 5' RACE protocol of Boehringer Mannheim.To obtain the 5' end of MBD2, a gridded cosmid library (LawrenceLivermore National Laboratories cosmid library LL18NC02; providedby the United Kingdom Human Genome Mapping Project Resource Centre[HGMP], Cambridge, England) was screened with a PCR product correspondingto the 5' end of MBD2 intron 1 (PCR product of primers 5'-AAAATCTGGGCTAAGTGCTGG-3'and 5'-ACGCCTTCCACATAAGATGC-3'), using the hybridization conditionsdescribed above. Two independent cosmids (clones AD15-O10 andAD17-O6) were identified and subcloned, and the relevant regionswere sequenced.

MBD4 was identified as an EST (AA149549). The corresponding clone (588272) was sequenced and found to contain a long openreading frame. No ESTs for Mbd4 were present in the database,so the human cDNA was used as a probe against a mouse 129 genomiclambda library (a gift from A. J. H. Smith). Hybridization conditionswere as described above, but filters were washed to a final stringencyof 1% SDS-0.5 M NaCl-50 mM Tris (pH 8) at 65°C. Positive cloneswere identified which, upon subcloning and sequencing, were foundto contain the Mbd4 gene. Genomic clones were used to screen amouse brain cDNA library which resulted in the identificationof one partial cDNA containing a short poly(A) tail. This cDNAwas used as a probe on a gridded mouse cDNA library (embryonicregion cDNA library ER-IV, HGMP; 17), and another partial cDNAclone which ends in a poly(A) at the same location was identified.The full-length Mbd4 sequence was determined by sequencing ofcDNAs and by comparison of genomic sequence to that of the humanMBD4 cDNA, followed by verification by RT-PCR, 5' RACE, and sequencingof products.

All IMAGE consortium (LLNL) cDNA clones (26) described here were obtained from the HGMP, except for clones 400458, 403236,and 420899, which were obtained from Research Genetics; cloneHIBAA05 (MBD3), which was obtained from the American Type CultureCollection; and clone MMTEST (46), which was obtained from ChristerHöög, Stockholm, Sweden. Sequencing was performed with an ABIAutomated Sequencer 373A Stretch apparatus. Contig construction,sequence analysis, and comparison was performed by using the LasergeneDNA analysis software package (DNAStar).

Expression analysis. Total RNA was isolated from tissues of adult mice using acid guanidinium thiocyanate-phenol-chloroform extraction (13).Ten or 20 µg of total RNA was used per lane on Northern blots.Blots were hybridized in Church buffer as described above. Blotswere washed to a final stringency of 0.1% SDS-0.1× SSC at 68°Cfor all probes except Mbd4, which was washed to a final stringencyof 1% SDS-0.5 M NaCl-50 mM Tris (pH 8) at 65°C. Signal was detectedwith a PhosphorImager (Molecular Dynamics). For reverse transcription-PCR(RT-PCR) analysis, 5 µg of total RNA was reverse transcribed at42°C by Moloney murine leukemia virus reverse transcriptase for2 h according to the manufacturer's instructions (Life Technologies).One microliter of the reverse transcriptase reaction mixture wasthen subjected to 30 cycles of PCR.

Construction of expression vectors and protein expression. The coding sequences for all four genes were PCR amplified (Mbd1, 5'-AAGCATCCATGGCTGAGTCCTGGC-3' and 5'-GGGAGGGCAGTAATAAGGCCAGTCA-3';Mbd2, 5'-GGGAAGACCATGGACTGCCCG-3' and 5'-GCGGATCCTTACGCCTCATCTCCCTC-3';Mbd3, 5'-GGCGCCATGGAGCGGAAGAGGTG-3' and 5'-TCCCCCGGCACTCGCTCTGGCTCCGG-3';Mbd4, 5'-GCGCCATGGAGAGCCCAAACCTTG-3' and 5'-GCGGATCCAGGCAGCTTCAAGATAG-3';MBD4, 5'-CCTGCTCCATGGGCACGACTGGGCTG-3' and 5'-GCGGGATCCTGAGCTTGAAAGCTGCAG-3')using Pfu polymerase (Stratagene) or Pwo polymerase (BoehringerMannheim) according to the manufacturer's instructions and clonedinto the bacterial expression vector pET6H (19). Recombinantproteins were expressed in Escherichia coli BL21(DE3)/pLysS asdescribed previously (15) and purified over a nickel agarosecolumn (Ni²⁺-NTA-Superflow Agarose [Qiagen]). Extracts were loaded onto thecolumn, washed in a solution containing 60 mM imidazole, 250 mMNaCl, 20 mM Tris (pH 7.9), 10% glycerol, 0.1% Triton X-100, and10 mM 2-mercaptoethanol, and eluted in elution buffer (wash buffercontaining 0.5 M imidazole). Proteins were further purified byfractionation over Fractogel EMD SO₃--650(M) (Merck). Proteinspartially purified on the nickel-agarose column were loaded ontothe Fractogel column, washed in a solution containing 250 mM NaCl,50 mM HEPES (pH 7), 10% glycerol, 0.1% Triton X-100, and 10 mM2-mercaptoethanol, and eluted in the same buffer containing 1M NaCl. All column wash and elution buffers were supplementedwith complete protease inhibitor tablets (Boehringer Mannheim).

Constructs producing MBD1-GFP, MBD4-GFP, and MeCP2-GFP were made by PCR amplifying either cloned cDNAs (Mbd1) with Pfu polymeraseas described above or reverse-transcribed total ES cell RNA (Mbd4)or murine brain RNA (Mecp2) with Pwo polymerase as described above,digesting the PCR products with HindIII and KpnI or KpnI alone(Mecp2), and ligating into the pCMXGFP mammalian expression vector.The MBD2-GFP construct was made by cloning the coding sequences(NaeI-SspI fragment) of a full-length Mbd2 cDNA into the HindIIIsite of pCMXGFP. pCMXGFP was constructed by K. Umesono by insertionof the green fluorescent protein (GFP) cDNA (37) into Asp718-BamHI-cutpCMX vector (44). The GFP cDNA is under the control of a cytomegaloviruspromoter and both a polyomavirus enhancer and a simian virus 40enhancer. This version of GFP contains the following amino acidchanges: F64L, V163A, S175Q, I167T, and S65T. The GFP-MBD3 constructwas made by PCR amplifying an Mbd3 cDNA with Pfu polymerase, digestingwith BglII and SpeI, and ligating into the pCMXGFP2 mammalianexpression vector. pCMXGFP2 was derived from pCMXGFP by mutatingthe stop codon for the GFP from TGA to GGG by PCR mutagenesis.Primers used were as follows: for Mbd1, 5'-GCGGAAGCTTATGGCTGAGTCCTGGCAG-3'and 5'-GCGGTACCCAAAACTTCCTCCTTCAACTGC-3'; for Mbd3, 5'-GCAGATCTATGGAGCGGAAGAGGTGG-3'and 5'-GCACTAGTACACTCGCTCTGGCTCC-3'; for Mbd4, 5'-GCGAAGCTTATGGAGAGCCCAAACCTTG-3'and 5'-GCGGTACCAGGCAGCTCCAAGATAGAC-3'; for MeCP2, 5'-GCGGTACCATGGTAGCTGGGATGTTAG-3'and 5'-GCGGTACCGCTAACTCTCTCGGTCACG-3'.

Band shifts. Band shift assays were performed essentially as described previously (15) except that binding reactions were carried outat room temperature for 30 min and contained 100 ng of sonicatedE. coli DNA for MBD1, MBD2, and MBD4 or 200 ng of E. coli DNAfor MBD3. Complexes were electrophoresed through 2% agarose gelsor 6% polyacrylamide gels in 0.5× TBE (Tris-borate EDTA) at 4°C.The GAM12 and GAC probes have been described previously (27).The double-stranded Sm probe was made by A. Prokhortchouk et al.(37a). The NB probe was made by excising a 125-bp NcoI-BamHIfragment from the MBD1 cDNA clone 222390 (15). Doubly methylatedand fully methylated NB were made by methylation with HpaII andHhaI methylases or SssI methylase (New England Biolabs), respectively.The 51 probe was a gift from J. Huntriss and M. Monk (20). TheMM1 and MM2 probes were designed by H.-H. Ng. GAM12, GAM5, GAC,MeCG11, and CG11 probes have been described previously (27,30).

Cell culture, transfection, and fluorescence imaging. L, HT1080, and CHO cells were grown on coverslips in minimal essential medium alpha (Life Technologies) supplemented witheither 10% (L cells) or 5% (HT1080 and CHO cells) bovine calfserum (Hyclone). EFS2 cells were derived from an ES cell linecontaining a randomly integrated $beta$ -geo transgene (42). Embryonicfibroblasts were obtained from this line by injecting ES cellsinto blastocysts and selecting resistant cells (500 µg of Geneticinper ml and 10% bovine calf serum in minimal essential medium alpha[Life Technologies]) from dissociated embryos in culture (17b).ES cells were grown in Glasgow medium (Life Technologies) supplementedwith 10% fetal calf serum (Globepharm), 1× nonessential aminoacids (Life Technologies), 1 mM sodium pyruvate, 50 µM 2-mercaptoethanol,and soluble differentiation-inhibitory activity/leukemia-inhibitoryfactor (41) at 37°C in a 5% CO₂ atmosphere. Ten micrograms ofeach expression construct was transfected at approximately 50%confluence by using Lipofectin or Lipofectamine (Life Technologies)onto 2-cm² coverslip of cells at 50% confluence according to the manufacturer'sinstructions. Approximately 36 h after transfection, cells werefixed in 4% paraformaldehyde in phosphate-buffered saline for20 min at 37°C and then washed twice in phosphate-buffered saline.Coverslips were mounted in Vectashield (Vector Laboratories) containing1 µg of 4',6-diamidino-2-phenylindole (DAPI) per ml and visualizeddirectly. Images were obtained using a Zeiss epifluorescence microscopefitted with a charge-coupled device camera (Photometrics) andcontrolled by a Macintosh computer running the Quips mFISH software(Vysis Inc.).

Nucleotide sequence accession numbers. All sequences reported here are available in Genbank under accession nos. AF072240 to AF072252. Human EST contigs forMBD2, MBD3, and MBD4 can be found as entries Hs.25674, Hs.107254,and Hs.35947, respectively, through the UniGene web page: http://www.ncbi.nlm.nih.gov/Schuler/UniGene.

	RESULTS

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A family of MBD-containing proteins. We sought to identify novel proteins containing a MBD-like motif by searching the EST database. In addition to Mecp2 and MBD1,three other genes (Mbd2, Mbd3, and Mbd4) were identified in humansand mice encoding proteins containing putative MBDs. Assignmentof the initiator AUG codons for each gene was given to the firstin-frame ATG in each case. While this location is conserved inthe human and murine Mbd1, Mbd2, and Mbd3 genes, it is not conservedin human and murine Mbd4 genes. In both the human and murine Mbd4genes, the AUG codon at which we propose translation initiatesis the only in-frame methionine codon N terminal to the MBD-likeregion. The first in-frame start codons in the Mbd2 and MBD2 openreading frames is within a CpG island, and the second is located152 codons downstream, just upstream of the MBD. These two potentialinitiator codons show 6 of 10 and 5 of 10 matches to the Kozakconsensus sequence for initiator codons, respectively (24).Conceptual translation of the region between the first two ATGcodons produces a repetitive amino acid sequence due to the highG+C content of the underlying DNA. At this point, we do not knownwhich initiator methionine is used in vivo, though the high degreeof conservation between the human and murine genes in this CpGisland is consistent with the first methionine being the trueinitiator methionine.

Alignment of the MBD-like regions from the murine MBD1 to MBD4 and MeCP2 proteins is shown in Fig. 1A. The MBD protein familycomprises two subgroups based upon the sequences of the putativeMBDs (Fig. 1A). The MBD of MBD4 is most similar to that of MeCP2in primary sequence, while the MBDs of MBD1, MBD2, and MBD3 aremore similar to each other than to those of either MBD4 or MeCP2.The MBDs within each protein appear to be related evolutionarilybased on the presence of an intron located at a conserved positionwithin all five genes (Fig. 1A).

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FIG. 1. Comparison of MBD family proteins. (A) Amino acid alignment of the MBDs from murine MBD1, MBD2, MBD3, MBD4, and MeCP2 proteins. Amino acids identical in three or more proteins are indicated by shading. The location of an intron present in all five genes is indicated. (B) Comparison of MBD protein structure. Proteins are indicated as horizontal lines, and MBDs are shown as labeled white boxes. Two forms of MBD2 are shown corresponding to initiation of translation at either the first (MBD2a) or second (MBD2b) methionine codons (see text). The cysteine-rich repeats of MBD1 are represented by two black boxes, and the repression domain of MeCP2 is indicated as a stippled box. The glycine-arginine repeat in MBD2a and the C-terminal glutamic acid repeat of MBD3 are indicated as horizontal lines beneath the respective proteins. Alternate splice events are indicated as diagonal lines above or below the line of the protein. Any novel translation termination codons introduced in alternate splice events are indicated. The brain-specific splice of MBD1 and testis-specific splice of MBD2 are labeled B and T, respectively. Predicted molecular masses (in kilodaltons) and isoelectric points of each protein are also listed. The isoelectric point of the MBD3 protein is given both for the full-length protein and, in parentheses, for the protein excluding the glutamic acid repeat. aa, amino acids.

With the exceptions of MBD2 and MBD3, sequence similarity between the proteins is limited to the MBDs themselves. MBD3 ishighly similar to MBD2 over most of its length with 71.1% overallamino acid identity (Fig. 2), diverging only at the extreme Cterminus where MBD3 has 12 consecutive glutamic acid residuesencoded by an imperfect trinucleotide repeat. This characteristicis also conserved in the rat and human MBD3 proteins, althoughthe acidic tail of the latter homologue is slightly longer andcontains aspartic acid residues as well as glutamic acid residues.MBD2 and MBD3 show high conservation between human and murinegenes (97.6 and 93.8% amino acid identity, respectively), whereasthe human and murine homologues of MBD1 and MBD4 are less wellconserved (70.9 and 65.5% amino acid identity, respectively [datanot shown but all sequences are available in GenBank]). Searchesof the protein databases revealed no significant matches for MBD1,MBD2, or MBD3 outside of the MBDs and the CxxCxxC motifs of MBD1(15). Searches with the MBD4 protein sequence produced a seriesof low-scoring hits to bacterial DNA repair enzymes (data notshown).

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FIG. 2. Amino acid alignment of murine MBD2 and MBD3. Identical residues are indicated with a vertical line between the sequences; homologous residues are indicated with a colon, and similar residues are indicated with a period. Boxed amino acids correspond to the MBD. The glutamic acid repeat of MBD3 is represented by (E₁₂). Amino acid numbering for MBD2 begins from the upstream initiator methionine (see MBD2a in Fig. 1B).

Cloning of the murine Mbd1 gene revealed the presence of three exons with a potential to encode cysteine-rich domains (CxxCxxC[Fig. 1B]), whereas the human gene was reported to encode onlytwo of these domains (15). RT-PCR analysis of various murinetissues detected an alternately spliced RNA form in which theexon encoding the third CxxCxxC motif is excluded from the maturemessage (Fig. 1B). Further investigation of ESTs present in thedatabases allowed us to identify human MBD1 ESTs in which an exonencoding a third CxxCxxC motif is present (accession nos. U55972and R14016). Whereas the 3' CxxCxxC-encoding exon is alternatelyspliced in mice, the 5'-most CxxCxxC-encoding exon is alternatelyspliced in the human gene. Thus, both the human and murine Mbd1genes can generate proteins containing two or three such motifsdepending upon alternate splicing. An additional alternate splicingevent was also detected in cDNA derived from mouse brain in whichthe third exon (encoding the C-terminal half of the MBD) is removed(Fig. 1B, splice labeled B). This splicing event does not maintainthe correct reading frame in subsequent exons, and any resultingRNAs would not be expected to encode a functional protein. A thirdalternate splice would result in the replacement of the C-terminal29 amino acids with an alternate 44-amino-acid C-terminal tail.This splice variant was found in cDNAs from both brain and embryoniccDNA libraries (this study and IMAGE clone 400458, accession no.W77338) but was not detectable by RT-PCR and is therefore predictedto occur with very low frequency.

A number of cDNAs isolated for the Mbd3 gene contain an in-frame deletion of the first exon which would result in a transcriptlacking the coding sequence for the N-terminal half of the MBD(Fig. 1B). This appears to be due to the use of an alternate splicedonor site within the first exon. This protein would be only slightlysmaller than the full-length protein, but the MBD would be destroyed.Both spliced and unspliced forms of the message are readily detectablein many somatic tissues by RT-PCR, indicating that the shortermessage makes up a significant fraction of total Mbd3 message(Fig. 1B and data not shown). The Mbd2 gene is also capable ofusing alternate splicing to produce potentially nonsense transcripts:a rare, larger form of the transcript includes an alternate fourthexon (4' [Fig. 1B]) which contains an in-frame stop codon. Thetestis-specific form seen in Fig. 3B results from the inclusionof an alternate third exon which again results in early terminationof the reading frame and truncation of the message (T [Fig. 1B]).This testis-specific exon was found in both the human and murinegenes, though the level of sequence conservation in this exonis much lower than that seen for the rest of the coding region.Evidence of alternate splicing was also found for the human andmurine Mbd4 transcripts. None of the identified alternately splicedforms affect the coding sequence of the MBD-like region, thoughone form of the human message found in the EST database wouldresult in a truncated protein lacking the C-terminal 42 aminoacids which are completely conserved between the human and murinegenes. The significance of these alternately spliced variantsis not known but may reflect a common method for the regulationof the MBD protein family members.

Expression of Mbd genes. MeCP1 activity has been detected in numerous somatic cell types but is notably absent in ES cells and germ cells (30). Inorder to determine the expression pattern of the Mbd genes, thecorresponding cDNA clones were hybridized to Northern blots containingRNA from various murine tissues including testis and ES cells(Fig. 3). The Mbd genes were expressed in all somatic tissuestested. No Mbd1 transcripts were detectable in ES cells, consistentwith the absence of MeCP1 activity in these cells. Similarly,Mbd2 transcript levels were significantly reduced in ES cells,while an alternately spliced transcript of reduced size is detectedin testis (see above). DNA methylation is known to be dispensablein ES cells (25) so it would not be surprising for methyl-CpGbinding proteins to be reduced or absent in this cell type. Mbd2expression was detected as a doublet RNA band in somatic tissues,which may reflect alternate polyadenylation site usage. Mbd3 transcriptswere detectable in all tissues tested, including testis and EScells. Mbd4 expression was undetectable on Northern blots exceptat very low levels in ES cells, though expression was detectablein all tissues by RT-PCR (data not shown). Expression of MBD4was detectable in RNA from numerous human somatic tissues as wellas ovary and testis (data not shown).

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FIG. 3. Expression of MBD1 to MBD3. cDNAs corresponding to Mbd1 (A), Mbd2 (B), and Mbd3 (C) were hybridized to Northern blots containing 10 µg of total RNA per lane from various murine tissues and ES cells. Size markers (in kilobases) are shown to the left of each blot. Blots were stripped and rehybridized to a probe corresponding to mouse ribosomal protein 26 cDNA (S26) to act as an RNA loading control. Sk. Muscle, skeletal muscle.

MBD proteins bind methylated DNA in vitro. The MBD protein family members were identified due to the presence in each of a MBD-like region. We tested recombinant formsof each protein for the ability to bind to methylated and unmethylatedDNA probes in a gel retardation assay. As shown in Fig. 4, MBD1,MBD2, and MBD4 all produce a specific complex with a methylatedprobe but not with the unmethylated version of the same probe(Fig. 4, compare lanes 3 and 4, 7 and 8, and 15 and 16). The bipartiteshift observed with MBD1 is likely due to the presence of a 36-kDadegradation product within the recombinant MBD1 preparation, aswas also seen with the human protein (15). The methyl-CpG-specificcomplexes formed by MBD1, MBD2, and MBD4 are effectively competedaway upon addition of 100-fold excess unlabeled probe but notupon addition of the same amount of the unmethylated version ofthis probe (Fig. 4, compare lanes 5 and 6, 9 and 10, and 17 and18). While MBD3 forms a complex with the methylated probe andnot the unmethylated probe (Fig. 4, lanes 11 and 12), this shiftis not competed with either methylated or unmethylated probe (lanes13 and 14) and thus is not a specific shift. Both MBD1 and MBD2are capable of binding to a probe containing two symmetricallymethylated CpGs located 25 bp apart, though MBD4 failed to bindthis probe (NB-HH probe [Table 1]). MBD1, MBD2, and MBD4 allwere capable of specifically binding a probe containing one symmetricallymethylated CpG (MM2 [Table 1]). Additionally, MBD1 and MBD4 bindingcan be competed by 100-fold excess hemimethylated oligonucleotide[(GAM)₁₂/(GTC)₁₂] though significantly less well than with a symmetricallymethylated version of the same probe (data not shown). The MBD2shift is not affected by this hemimethylated oligonucleotide.None of these proteins bind single-stranded DNA whether methylatedor not, and they do not bind a double-stranded oligonucleotidecontaining repeats of the sequence TpG (thymine being similarto 5-methylcytosine in that both are pyrimidines with a methylgroup at position 5). Thus MBD1, MBD2, and MBD4 proteins specificallybind methylated DNA in vitro and preferably double-stranded, symmetricallymethylated DNA, although MBD1 and MBD4 complexes are also competedto a lesser extent by hemimethylated oligonucleotides. The bindingof MBD1, -2, and -4 to methyl-CpGs appears to be independent ofsequence context in that they bind methylated versions of a numberof different oligonucleotide probes (Table 1).

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FIG. 4. Binding of recombinant MBD proteins to methylated DNA in vitro. One hundred picograms of radiolabeled, double-stranded GAC (lanes 1, 3, 7, 11, and 15) or GAM12 (lanes 2, 4 to 6, 8 to 10, 12 to 14, and 16 to 18) DNA (Table 1) was incubated with recombinant MBD proteins in the presence (+) or absence ( $-$ ) of 200 ng of unlabeled methylated or unmethylated competitor DNA and then electrophoresed through a 2% agarose gel. The location of the free probe is indicated, and protein-DNA interactions are evidenced as slower-migrating DNA. Approximate amounts of recombinant protein used were as follows: MBD1, 20 ng; MBD2b, 10 ng; MBD3, 100 ng; MBD4, 100 ng. All proteins form a slower-migrating complex with methylated probe but not with the unmethylated probe. The shifts of MBD1, MBD2b, and MBD4 are prevented by the presence of excess, unlabeled, methylated DNA during incubation (M⁺ Competitor), but not by the addition of excess unmethylated DNA (M Competitor). The full-length MBD2 protein also produces a methyl-specific shift (data not shown). The shift produced by MBD3 is competed by neither methylated nor unmethylated DNA and is therefore considered to be nonspecific.

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TABLE 1. Binding of MBD proteins to methylated DNA in gel shift experiments

MBD1, -2, and -4 proteins are targeted to methylated DNA in vivo. Approximately 50% of all 5-methylcytosine is concentrated in major satellite in murine cells; subsequently MeCP2 protein hasbeen found to be concentrated at this repetitive sequence (35).Mouse major satellite is organized in foci of constitutive heterochromatinand corresponds to regions of the nucleus that stain brightlywith Hoechst 33258 and DAPI (31). The specific localizationof MeCP2 is no longer seen in cells with <5% of normal DNA methylation(25), demonstrating that appropriate cellular localization isdependent upon DNA methylation (35). Having shown that the MBDproteins specifically bind methylated DNA in vitro, we wantedto determine whether the cellular localization of the MBD proteinsis consistent with them binding methylated DNA in vivo. To dothis, we examined their localization in normal murine cells andin cells lacking >95% of normal DNA methylation (Fig. 5A). Constructsdesigned to express GFP-tagged versions of each of the MBD proteinsunder the control of a cytomegalovirus promoter were transfectedinto either wild-type or DNMT-deficient ES cells. As is shownin Fig. 5 and 6, ectopically expressed MBD proteins were predominantlynuclear in murine cells. Nuclear localization was also seen inhuman (HT1080) and hamster (CHO) cells (data not shown). OverexpressedMBD1-GFP, MBD2-GFP, and MBD4-GFP preferentially localized to regionsof the genome known to be highly methylated, as evidenced by colocalizationof protein signals with DAPI-bright areas (Fig. 5B to D).

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FIG. 5. Binding of MBD proteins to methylated and hypomethylated genomes in vivo. (A) DNA from wild-type ES cells (lanes 1 and 4), DNMT mutant ES cells (lanes 2 and 5), and murine somatic cells (lanes 3 and 6) was digested with the methylation-sensitive restriction enzyme MaeII (Boehringer Mannheim) and electrophoresed on a 1% agarose gel. Lanes 1 to 3 show the ethidium bromide-stained gel, and lanes 4 to 6 show the gel blotted and probed with the 234-bp major satellite repeat monomer. (B to D) Localization of MBD-GFP fusion proteins in nuclei of ES cells. Either wild-type (WT) or DNMT-deficient (DNMT) ES cells were transiently transfected with MBD1-GFP (B), MBD2-GFP (C), or MBD4-GFP (D) expression constructs. GFP fluorescence (upper panels) indicates the location of the MBD-fusion protein. DNA is visualized in the same nuclei by DAPI staining (lower panels), and major satellite is visible as intense spots of DAPI fluorescence. All fusion proteins are predominantly nuclear in all cells. MBD1-GFP colocalizes with major satellite in wild-type and mutant cells. MBD2-GFP and MBD4-GFP colocalize with major satellite in wild-type ES cells but fail to localize to major satellite in DNMT-deficient ES cell nuclei. Localization of MBD4-GFP to the nucleolus in DNMT-deficient ES cell nuclei was not observed consistently.

MBD1-GFP, MBD2-GFP, and MBD4-GFP all localized to major satellite in transfected wild-type murine cells, consistent with theirability to bind methylated DNA in band shift assays. Whereas MBD1-GFPshowed heterochromatic localization in all transfected cells,in cells expressing low levels of MBD2-GFP and MBD4-GFP, unlocalizednuclear staining was often observed. This pattern was seen insomatic murine cells (primary mouse cells and L cells [data notshown]) as well as ES cells. In order to determine whether MBD2-GFPand MBD4-GFP localization was disrupted in DNMT-deficient ES cells,the following screening protocol was used. Coverslips were scannedunder ×20 magnification, and cells containing a visible amountof GFP signal at this level of magnification were then analyzedunder ×100 magnification and scored for subnuclear localization.Using this selection criterion, 100% of wild-type ES cells analyzedshowed localization of MBD2-GFP or MBD4-GFP signal with majorsatellite. In contrast, DNMT-deficient ES cells expressing MBD2-GFPor MBD4-GFP displayed an overall nuclear localization of the GFPsignal (Fig. 5C and D), indicating that the association of MBD2-GFPand MBD4-GFP with major satellite is dependent upon DNA methylation.MBD1-GFP localized to major satellite in all wild-type murinecells analyzed, irrespective of the amount of fluorescence seen.In DNMT-deficient ES cells, MBD1-GFP localized to DAPI-brightregions in most, but not all, nuclei (Fig. 5B). This is in starkcontrast with the patterns seen for MBD2-GFP and MBD3-GFP, aswell as that reported for MeCP2-LacZ which localized to majorsatellite in a minority of DNMT-deficient ES cells (35). Thepossibility of contamination of the DNMT-deficient ES cell culturesby wild-type ES cells was ruled out by verifying the undermethylationof the DNMT-deficient ES cells by digestion of total DNA withthe methylation-sensitive restriction enzyme MaeII (Fig. 5A).While normal ES cell DNA and somatic cell DNA is highly resistantto MaeII digestion, the DNMT-deficient ES cell DNA is readilydigested with MaeII, which is able to digest the sequence ACGTonly when the cytosine is unmethylated (Fig. 5A, compare lane2 to lanes 1 and 3). Blotting and probing of this gel with majorsatellite DNA illustrate the high degree of undermethylation ofthis repetitive sequence in the DNMT-deficient ES cells comparedto that of wild-type ES cells or somatic cell DNA (Fig. 5A, comparelane 5 to lanes 4 and 6). This observation may mean that the residualmethylation known to exist in the DNMT-deficient ES cells is sufficientto direct MBD1-GFP to the major satellite. An alternate interpretationof these results is that MBD1-GFP is tethered to major satellitevia some other protein factor and that this association is independentof DNA methylation.

The MBD3-GFP fusion protein shows diffuse nuclear staining in low-expressing cells and accumulates in many nuclear foci incells expressing large amounts of the fusion protein. These focido not coincide with major satellite (Fig. 6). Thus, MBD3 doesnot prefer to associate with the highly methylated major satelliteDNA in mouse cells. To determine whether the failure of MBD3-GFPto localize to methylated DNA in vivo is due to the presence ofits acidic C-terminal tail, an MBD3 deletion protein (GFP-MBD3Nh[Fig. 6]), which is truncated at amino acid 248, was expressedin murine cells. This protein also localized to the nucleus ininterphase mouse cells but was excluded from the DAPI-bright regions,indicating that it is not the acidic tail which is preventingGFP-MBD3 from associating with methylated DNA in vivo. We nextwanted to determine whether the localization of MBD3 was influencedby its MBD-like region. A version of MBD3 (GFP-MBD3Sp [Fig. 6])lacking amino acids 4 to 36 (the amino-terminal half of the MBD-likeregion) and corresponding to the common alternately spliced variantof Mbd3 message (Fig. 1B), was expressed as a GFP fusion in murinecells. The localization of this deleted MBD3-GFP protein was indistinguishablefrom that of the full-length protein, leading us to conclude thatthe integrity of the MBD-like region is not important for thelocalization seen in this assay.

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FIG. 6. Localization of GFP-MBD3 fusion proteins in nuclei of somatic cells. The mouse embryonic fibroblast cell line EFS2 was transiently transfected with GFP-MBD3 fusion protein expression constructs. The top panels show GFP fluorescence, while the lower panels show DAPI staining of the same cells. The constructs used are diagrammed at the bottom, with MBD depicted as a gray box and the glutamic acid repeat depicted as a black box. In all cases, GFP is located at the N terminus. (A) The full-length MBD3 fusion protein localizes to the nucleus and occasionally forms bright foci of GFP fluorescence, but these spots do not correspond to the major satellite. (B) Removal of the glutamic acid repeat (GFP-MBD3Nh) does not alter subnuclear localization, nor does removal of the N-terminal half of the MBD (GFP-MBD3Sp [C]). A fourth construct in which GFP is located at the C terminus of full-length MBD3 showed a localization pattern indistinguishable from that of GFP-MBD3 (data not shown).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Searching the EST database with the amino acid sequence of the MeCP2 MBD has revealed the presence of a family of mammalianMBD-containing proteins. The absence of any other known sequencemotifs within MBD2 or MBD3 provides no clues as to the activitiesof these two proteins. In contrast, homology between MBD4 andbacterial DNA repair enzymes is consistent with a DNA repair activityfor MBD4 and may indicate a link between DNA repair and methylationin mammals, but this remains to be proven. Both the sequence andgenomic organization of the MBDs within each of the MBD proteinsmakes it clear that these motifs are related evolutionarily, butthe lack of similarity between these proteins outside of the MBD(excluding MBD2 and MBD3) may indicate that each protein carriesout a different function within the cell.

Both MeCP2 and MBD1 are capable of transcriptional repression at methylated promoters (15, 32), though there is no sequencein MBD1 (or any of the other MBD proteins) which bears any recognizablesequence homology to the TRD of MeCP2. The recent finding thatMeCP2 TRD binds to the Sin3-histone deacetylase complex (22,34) provides an attractive molecular picture of the potentialmechanism of action of MeCP2: MeCP2 binds to methylated DNA viaits MBD and attracts the Sin3-histone deacetylase complex viaits TRD, resulting in the deacetylation of methylated chromatinand subsequent transcriptional silencing. The absence of any TRD-likesequence in MBD1 may mean that the mechanism by which MBD1 repressestranscription is different from that used by MeCP2. AlternatelyMBD1 may use the same mechanism as MeCP2 but contain a novel Sin3binding domain or may bind deacetylases directly.

All of the MBD proteins, including MeCP2, are ubiquitously expressed in somatic tissues, but only Mbd3 and Mbd4 transcriptsare readily detectable in ES cells. Although ES cells generallyhave highly methylated genomes, this methylation is not necessaryfor viability (25). MeCP2 is very weakly expressed in ES cellsand is also not needed for viability (42). Thus, DNA methylationand the presence of MeCP2 do not appear to be important in EScells, and therefore, the finding that Mbd1 and Mbd2 transcriptlevels are significantly reduced in this cell type is not surprising.Mbd3 and Mbd4 are both well expressed in ES cells, but whetherthe corresponding proteins are present or important for ES cellviability is not known.

All of the MBD proteins except MBD3 bind to methylated oligonucleotide probes in vitro but do not bind to the unmethylatedversions of these oligonucleotides under our conditions. Recently,the chicken homologue of MeCP2 was proposed to be a componentof the nuclear matrix and was shown to be capable of binding toa TG-rich "matrix attachment region" sequence in gel shift assays(45). Though low-affinity TG binding has been detected for ratMeCP2 in vitro (35a), we detected no affinity of MBD1, MBD2,MBD3, or MBD4 for TG-containing probes in gel shift assays (datanot shown).

We have taken advantage of the fact that approximately half of all 5-methylcytosine in mouse cells is located at the pericentromericheterochromatin (31) in order to investigate the ability ofthe MBD proteins to localize to methylated DNA in vivo. Ectopicallyexpressed GFP-fusions of MBD1, MBD2, and MBD4 colocalized withmajor satellite in mouse cells, but localization of MBD2 and MBD4was disrupted in cells lacking a functional DNMT gene (Fig. 5).This suggests that MBD2 and MBD4 are capable of binding methylatedDNA in vivo as well as in vitro. MBD1 is also capable of associatingwith methylated DNA in vivo but binds to the same heterochromaticsites in DNMT-deficient ES cells. It is not clear whether MBD1is binding to low levels of DNA methylation in DNMT-deficientcells or to some other heterochromatin binding protein. Similarly,we cannot formally rule out the possibility that the localizationof MBD2 and MBD4 to murine heterochromatin is due to their interactionwith some other methylation-sensitive heterochromatin bindingprotein. It is unlikely that MeCP2 is responsible, as proteinactivity is undetectable in ES cells (30) and localization ofMBD1-, MBD2-, or MBD4-GFP fusion proteins is not disrupted inMeCP2-deficient somatic cells (17a).

MBD3 behaves differently than the other MBD proteins, failing to specifically bind methylated DNA in vitro (Fig. 4C) or colocalizewith major satellite in vivo (Fig. 6). The difference in specificitybetween the highly similar MBD2 and MBD3 proteins cannot be attributableto their divergent C termini, as a truncated version of MBD3 whichlacks the C-terminal 37 amino acids, including the glutamic acidrepeat, also fails to localize to DAPI-bright regions in mousenuclei (Fig. 6). Nor can it be attributable to the additional150 amino acids N-terminal to the MBD of MBD2, since a shorterMBD2-GFP protein which lacks this region also localizes to majorsatellite in murine cells (data not shown). Thus, the DNA bindingspecificities are most likely attributable to differences in theMBDs of the two proteins (Fig. 1A and 2). It is possible thatthe MBD of MBD3 is nonfunctional, since a GFP fusion of an MBD3variant resulting from the product of the common alternately splicedRNA species (Fig. 1B) which lacks the N-terminal half of the MBD-likesequence shows an in vivo localization pattern indistinguishablefrom that of the full-length protein (Fig. 6). Despite the highdegree of sequence similarity between MBD2 and MBD3, these twoproteins display completely different DNA binding activities andin vivo localization patterns. The very high degree of conservationbetween the murine and human homologues of these two proteins(97.6% amino acid identity for MBD2 and 93.8% for MBD3) indicatesthat both proteins are functional. One possible explanation forthese observations is that Mbd3 arose by gene duplication of Mbd2,but has acquired a novel DNA binding specificity which our ectopicoverexpression techniques have not detected. Whether MBD2 andMBD3 perform similar functions despite having different DNA bindingabilities remains to be determined.

MeCP2 localizes to major satellite at a very low frequency in DNMT-deficient cells (35). This may be attributable to thenonspecific DNA binding activity of MeCP2 which, in the absenceof methyl-CpGs, may allow it to bind to the TG-rich major satellite(27). We have found no in vitro evidence that any of the proteinsdescribed here has any sequence specificity other than the absoluterequirement for the presence of methylated CpGs. Nevertheless,there are hints of different binding specificities in vivo. WhereasMBD1-GFP location is coincident with DAPI-bright regions in alltransfected murine cells, MBD2-GFP and MBD4-GFP fail to bind majorsatellite in murine cells expressing very small amounts of thefusion protein (data not shown). This observation may indicatea DNA binding preference of MBD2 and MBD4 for methylated euchromaticsites over those found in major satellite. Similarly, the differentfrequencies with which the MBD proteins are found to localizeto major satellite in ES cells lacking >95% of normal methylationlevels may reflect the density of methylation required in a givensequence for each protein to bind. For example, MBD1 may be capableof binding to DNA containing low methylation levels, MeCP2 mayrequire a somewhat higher level of methylation, and MBD2 and MBD4may bind only heavily methylated DNA. This possibility will requirequantitative DNA binding assays to be tested rigorously.

DNA methylation is absolutely required for mammalian development (29). The signal that DNA methylation represents is interpretedby methylated DNA binding proteins, and until now only two ofthese $---$ MeCP2 and MBD1 $---$ had been defined molecularly (15, 27).The identification of MBD2 and MBD4 as specific methyl-CpG bindingproteins provides two more candidates for proteins that mediatethe effects of DNA methylation.

	ACKNOWLEDGMENTS

We thank En Li for the DNMT-deficient ES cells, Andrew Smith for the 129 genomic library, Jonathan Pines for the pCMXGFP vector,Christer Höög for the MMTEST clone, John Huntriss and MarilynMonk for sending oligonucleotide probes, and the HGMP for providingnumerous clones and libraries. We also thank members of the Birdlab; Cathy Abbott and Beth Sullivan for advice; Kevin Hardwickfor use of the imaging system; Vicky Clark for sequencing; AileenGreig and Joan Davidson for technical assistance; and Beth Sullivan,Cathy Abbott, Susan Tweedie, Sally Cross, and Huck-Hui Ng forcritical reading of the manuscript.

B. H. was the recipient of a Long Term Postdoctoral Fellowship from the Human Frontiers Science Program. The work was alsosupported by a program grant to A.B. from the Wellcome Trust.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Cell and Molecular Biology, University of Edinburgh, Darwin Building,King's Buildings, Edinburgh EH9 3JR, Scotland, United Kingdom.Phone: 44-(0)131-650-8695. Fax: 44-(0)131-650-5379. E-mail: Brian.Hendrich{at}ed.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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