The N-terminal Region of Chromodomain Helicase DNA-binding Protein 4 (CHD4) Is Essential for Activity and Contains a High Mobility Group (HMG) Box-like-domain That Can Bind Poly(ADP-ribose)*

Chromodomain Helicase DNA-binding protein 4 (CHD4) is a chromatin-remodeling enzyme that has been reported to regulate DNA-damage responses through its N-terminal region in a poly(ADP-ribose) polymerase-dependent manner. We have identified and determined the structure of a stable domain (CHD4-N) in this N-terminal region. The-fold consists of a four-α-helix bundle with structural similarity to the high mobility group box, a domain that is well known as a DNA binding module. We show that the CHD4-N domain binds with higher affinity to poly(ADP-ribose) than to DNA. We also show that the N-terminal region of CHD4, although not CHD4-N alone, is essential for full nucleosome remodeling activity and is important for localizing CHD4 to sites of DNA damage. Overall, these data build on our understanding of how CHD4-NuRD acts to regulate gene expression and participates in the DNA-damage response.

The nucleosome remodeling and deacetylase (NuRD) 3 complex is a conserved transcription co-regulatory complex that is found in all complex animals. It is unique in that it contains both nucleosome remodeling and deacetylase activity (1)(2)(3)(4)(5)(6); other co-regulator complexes such as Sin3 (7), Rpd3S (8), and PRC2 (9) only carry a single enzymatic activity. The NuRD complex has been shown to have essential roles in both activation and repression of gene transcription and has links to stem cell renewal and differentiation (10), cell cycle control (11), cancer (for review see Ref. 12), and the DNA-damage response, including DNA double strand break (DSB) repair (13). DSBs are highly cytotoxic; if repaired erroneously or left unrepaired, they can lead to cancer, neurodegeneration, and immunodeficiency (14).
One of the defining components of the NuRD complex is chromodomain helicase DNA-binding protein 4 (CHD4). CHD4 mediates the chromatin remodeling activity of the NuRD complex via a SNF2-type DNA translocase domain (15), and evidence has accumulated that CHD4 is important for an effective DNA-damage response and for the maintenance of genomic integrity. For example, the expression level of CHD4 has been shown to increase upon UV irradiation (16). CHD4 has been also reported to be a target of the DNA-damage response apical kinases ATM and ATR (17)(18)(19) and to be recruited to DSB sites as part of the NuRD complex (20). This recruitment occurs in a poly(ADP-ribose) polymerase (PARP)dependent manner. It has been shown that a 750-residue N-terminal fragment of CHD4 (residues 1-758) was sufficient for its recruitment and that this region binds poly(ADP-ribose) (PAR) polymers with the same apparent affinity as full-length CHD4 (20), suggesting that the N-terminal portion of CHD4 contains one or more PAR binding motifs. Similarly, the Drosophila homologue of CHD4 (dMi-2) has been shown to be recruited to active heat shock genes in a PARP-dependent manner (21). Proteomic studies have also indicated that CHD4 and other proteins of the CHD family can undergo poly-ADP-ribosylation; however, the biological effects of this modification are still unknown (22,23).
Poly(ADP-ribose) molecules are linear or multibranched chains of ADP-ribose. These polymers are synthesized by PARPs using NAD ϩ as a substrate and are attached covalently to proteins as a post-translational modification (for review see Ref. 24). Although still somewhat mysterious, PARylation has been shown to inhibit protein-protein and protein-DNA interactions, promote or alter protein localization, and regulate protein modifications such as ubiquitylation (for review see Ref. 25). As signaling molecules, PARylated proteins have roles in a number of cellular processes, including DNA repair and programmed cell death. In recent years, several PAR binding domains have been identified and their structures determined. For example, the DNA repair factor aprataxin polynucleotide kinase-like (APLF) has been shown to interact with PAR through its two PAR-binding zinc finger (PBZ) domains (26). The structure of the PAR binding macrodomain, a module present in histone macroH2A1.1, has been determined in complex with ADP-ribose (27). The apoptosis-inducing factor (AIF), which has a critical role in PARP1-mediated cell death (28), has also been shown to bind PAR with high affinity; however, there is no structural information on this interaction. These data suggest that several distinct modes of PAR recognition exist and that interactions occur either through stacking between tyrosine/phenylalanine residues and the adenine rings or through electrostatic interactions between basic residues and the phosphate moiety of ADP-ribose.
In addition to its SNF2 DNA translocase domain, CHD4 possesses two conserved chromodomains that are a feature of all CHD proteins and that are known to regulate the activity of the SNF2 domain (29) (Fig. 1a). Two additional plant homeodomains (PHDs) are present upstream of the chromodomains and are also found in the paralogues CHD3 and CHD5. The CHD4 PHDs bind the N-terminal tail of histone H3, exhibiting a preference for trimethylated or acetylated Lys-9 (30,31) and potentially conferring some substrate specificity to the CHD4-NuRD complex. Unlike CHD1 (32)(33)(34), which carries a DNA binding SANT-SLIDE domains in the C-terminal region, CHD4 has not yet been shown to contain any C-terminal DNA binding domains. The N-terminal region of CHD4, which we define here as the ϳ360 residues upstream of the PHD domains, is conserved in CHD3/4 orthologues but absent in other members of the CHD family. This sequence lacks appreciable similarity to known domains and is rich in stretches of basic and acidic residues.
The focus of this study was to probe the role of the N-terminal region in the function of human CHD4. We identified a conserved domain in the N-terminal region of CHD4 (CHD4-N) and determined its three-dimensional structure by solution NMR spectroscopy. CHD4-N displays structural similarity to the high mobility group (HMG)-box fold, a known DNA binding module that has roles in a wide variety of nuclear processes (for review see Ref. 35) but no known affinity for PAR. We performed microscale thermophoresis (MST) assays and NMR experiments to assess the nucleic acid binding properties of CHD4-N and carried out chromatin remodeling assays and transient transfections coupled with laser micro-irradiation to assess whether the N-terminal region of CHD4 plays a role in localizing CHD4 to DSB sites. Our data show that the CHD4-N domain can recognize PAR and that the remainder of the N-terminal region of CHD4 enhances the chromatin remodeling activity of CHD4 and is important for directing CHD4 to DSB sites.

Experimental Procedures
Sequence Analysis-Analysis of the N-terminal sequence of CHD4-(1-364) was performed using a combination of multiple sequence alignments, secondary structure prediction in Jpred (36), and disorder predictions (37,38).
Cloning, Expression, and Purification of CHD4-N in Bacteria-Residues 145-225 (CHD4-N) of human CHD4 were cloned into a pGEX-6P vector to produce an N-terminal GST fusion protein. CHD4-N was expressed in Escherichia coli Rosetta 2 cells grown for 20 h at 25°C in rich medium or, for isotope labeling, in minimal medium prepared as described previously (39). Cells were harvested and lysed and CHD4-N purified as described previously (39). CHD4-N has the additional sequence GPLGS on the N-terminal end, a remnant from the protease cleavage site. Purified CHD4-N was assessed by SDS-PAGE and size-exclusion chromatography coupled to a multiangle laser light scattering detector. For NMR experiments, the protein was concentrated to 0.3-1 mM in a buffer composed of 20 mM sodium phosphate, pH 7.5, and 150 mM NaCl. D 2 O (5% v/v) and 2,2-dimethyl-2-silapentane-5-sulfonic acid (170 M, as a chemical shift reference) were added to the solution.
NMR Assignments and Structure Calculations-NMR spectra were recorded at 25°C on 600 or 800 MHz Bruker Avance spectrometers equipped with TCI cryoprobes, processed using TopSpin TM (Bruker, Karlsruhe), and analyzed with SPARKY (T. D. Goddard and D. G. Kneller, University of California at San Francisco). 1 H, 15 N, and 13 C assignments were made using standard triple resonance spectra, and backbone dihedral angles were calculated with TALOSϩ (40), as described previously (39). Two-dimensional, 15 N-separated and 13 C-separated NOESY spectra were analyzed to obtain distance constraints, and initial structure calculations were performed using CYANA (41). From a family of 500 structures, the 100 lowest energy structures were subjected to water refinement using the RECOORD protocol (42). The 20 lowest energy water-refined structures were analyzed by PROCHECK NMR (43). Protein coordinates have been deposited in the Protein Data Bank under the accession code 2n5n. 15 N HSQC Titrations-All 15 N HSQC spectra were recorded at 25°C. 15 N-Labeled CHD4-N was used at 50 M (170 M in the case of adenosine 5Ј-diphosphate (ADP, Sigma) titration) in buffer containing 20 mM sodium phosphate, pH 7.5, 50 mM NaCl, 5% D 2 O, and 0.17 mM 2,2-dimethyl-2-silapentane-5-sulfonic as a chemical shift reference. Titrations were performed with ADP, an ADP-ribose dinucleotide (Sigma), or poly(A) (single-stranded DNA ssA 15 , Integrated DNA Technologies) dissolved in the same buffer as CHD4-N. Spectra were recorded for CHD4-N alone and after each addition of ADP, ADP-ribose dinucleotide, or poly(A). Molar ratios of CHD4-N:ligand for which spectra were collected were 1:0, 1:0.5, 1:1, 1:2, 1:5, 1:10. 15 N HSQC spectra were also recorded for 20 M 15 N-labeled CHD4-N in a buffer composed of 10 mM Tris, pH 8, and 1 mM EDTA in the presence or absence of poly(ADP-ribose) (Trevigen); the poly(ADP-ribose) was added to a concentration of 6 M in ADP-ribose subunits. All spectra were processed using TopSpin TM (Bruker).
Microscale Thermophoresis-MST experiments were performed on a Monolith NT.115 (Nanotemper Technologies, Munich, Germany). Each titration curve consisted of 12 points prepared from a serial dilution of CHD4-N and a constant con-centration of the fluorescein-labeled ligand. Experiments were carried out using 50 nM fluorescein-labeled DNA (Integrated DNA Technologies); sequences tested were: (i) 15 nucleotides of single stranded poly(A) (ssA 15 ), (ii) 15-nucleotide poly(T) (ssT 15 ), and (iii) 15 base pairs of double-stranded poly(AT) (prepared from ssT 15 and fluorescein-labeled ssA 15 hybridized in-house and purified by size exclusion chromatography). Titrations with poly(ADP-ribose) were performed using a mixture of 200 nM fluorescein-labeled streptavidin (Vector Laboratories) and 1 nM biotinylated PAR (Trevigen). Commercially available PAR consists of a mixture of polymers that range from 2 to 300 subunits; the average of subunits per polymer was considered to be 150 for the purpose of concentration determination. MST assays were performed with 20, 50, or 100% LED power using a blue filter and a 20 or 50% MST power. The normalized fluorescence readings were plotted as a function of CHD4-N concentration and fitted to a standard Langmuir binding isotherm, as implemented in the Nanotemper software.
Laser Micro-irradiation and Live Imaging-U2OS cells were cultured at 37°C in a humidified atmosphere containing 5% CO 2 in Dulbecco's modified Eagle's medium (DMEM; Sigma) supplemented with 10% (v/v) fetal bovine serum (FBS) from BioSera. Plasmid transfections were performed using TransIT-LT1 (Mirus Bio) following the manufacturer's guidelines. Localized lines of DNA damage were induced by laser microirradiation essentially as described previously (46,47). Briefly, U2OS cells were plated on glass-bottomed dishes (Willco-Wells) pre-sensitized with 10 M BrdU (Sigma) in phenol redfree medium (Invitrogen) for ϳ48 h at 37°C. Subsequent exposure to a laser beam was performed using a FluoView 1000 confocal microscope (Olympus) equipped with a 37°C heating stage (Ibidi) and a 405-nm laser diode (6 milliwatt) focused through a 60ϫ UPlanSApo/1.35 oil objective and resulting in a spot size of 0.5-1 m. Laser beam exposure times of 250 ms (fast scanning mode) were used at a setting of 0.4-milliwatt output (50 scans) to yield pre-sensitization-dependent DNA damage, restricted to laser tracks without detectable cytotoxicity. Images of live cells were acquired using the same microscope, objective, and software as described above. For live-intensity quantifications of GFP-CHD4 laser lines, average GFP-CHD4 intensities along laser tracks were measured, and ratios of GFP-CHD4 average line intensities over average nucleoplasm intensities were calculated and compared using FV-10 software (Olympus). Approximately 10 cells were quantified per GFP-CHD4 variant per time point. Normalized average intensities (1 for the GFP-CHD4-WT) are presented.
Expression and Purification of FLAG-CHD4 in Mammalian Cells-HEK293 cells were cultured at 37°C in a humidified atmosphere containing 5% CO 2 in DMEM supplemented with 10% (v/v) FBS, 2 mM L-glutamine, 1ϫ minimum essential media non-essential amino acids, 1 mM sodium pyruvate, 50 units/ml penicillin, and 50 g/ml streptomycin (all ingredients from Gibco TM ). pcDNA3 plasmids encoding for FLAG-CHD4 constructs were transfected into HEK293 cells at 70% confluence, and CHD4 proteins were expressed for 48 -72 h at 37°C and 5% CO 2 . Cells were harvested and resuspended in 50 mM HEPES, pH 7.5, 1.5 mM MgCl 2 , 10 mM KCl, 1 mM DTT, 1 mM PMSF, and 1ϫ cOmplete EDTA-free protease inhibitor mixture (Roche Applied Science). Cells were incubated on ice for 30 min, vortexed, and spun down for 5 min at 3300 ϫ g. The supernatant, which corresponds to the cytoplasmic fraction, was removed. The pellet was resuspended in 50 mM Tris, pH 8, 0.5 M NaCl, 1 mM EDTA, 1% Triton-X, 1.5 mM MgCl 2 , 1 mM DTT, 1 mM PMSF, and 1ϫ EDTA-free protease inhibitors. The nuclear fraction was then lysed by sonication on ice, incubated on ice for 30 min to allow chromatin to precipitate, and cleared by centrifugation for 20 min at 16,000 ϫ g at 4°C. The resulting nuclear extract was then incubated with ␣-FLAG M2 Affinity Gel beads (Sigma) overnight on a rocker at 4°C. The next day the protein was eluted with 300 g/ml 3X-FLAG-peptide (ApexBio) in 20 mM HEPES, pH 7.5, 150 mM NaCl, 1 mM DTT, and 10% v/v glycerol. Protein samples were analyzed by SDS-PAGE and visualized using SYPRO-Ruby and Coomassie stains.
Nucleosome Reconstitutions-Nucleosomes were assembled on DNA fragments derived from the 601 nucleosome positioning sequence (48) and purified recombinant Xenopus laevis histone octamers to give a typical final nucleosome concentration of 1-2 M. Assembly was performed by salt gradient dialysis using a double-dialysis method (48) as follows. Reactions were placed in microdialysis buttons, which were placed inside a dialysis bag containing 30 ml of 1ϫ Tris-EDTA (TE) and 2 M NaCl; the dialysis bag was then dialyzed overnight against 2 liters of 1ϫ TE at room temperature and then against a further 1 liter of 1ϫ TE for 3-6 h.
DNA fragments were produced by PCR using MyTaq DNA polymerase (Bioline) and fluorophore/quencher-labeled primers purchased from Sigma or ATDBio. The PCR products were purified via 0.5ϫ Tris borate-EDTA 5% polyacrylamide gel electrophoresis and electroelution. The notation xWy denotes the 147-bp 601 sequence with flanking DNA of x and y bp on the upstream and downstream side, respectively.
ATP-driven Nucleosome Remodeling Reactions-Nucleosomes were assembled on Cy3 or BHQ1-labeled 0W47 DNA to generate asymmetric end-positioned nucleosomes for gelbased and real-time remodeling reactions, respectively. All remodeling reactions were performed at 30°C. Gel-based remodeling reactions were carried out essentially as described in Ryan et al. (32). Real-time quenched FRET remodeling reactions were performed under similar conditions but monitored in a FluoStar Optima plate reader using Corning black nonbinding surface half-area 96-well plates and 485P and 520P excitation and emission filters, respectively. The reactions contained 50 nM BHQ1-0W47 AlexaFluor488-labeled nucleosomes, 50 mM Tris, pH 7.5, 50 mM NaCl, 3 mM MgCl 2 , and the enzyme concentrations indicated in the figures. Reactions were monitored for 1 min before the addition of 1 mM ATP to ensure fluorescence changes were ATP-dependent and then monitored for a further 5-10 min. The following single exponential function was fit to each individual remodeling data set.
where a is the asymptote, b is the total response (i.e. a minus the starting value), and c is a constant. The initial reaction rates were then calculated using the solution of the first derivative of f(x) when x ϭ 0, as follows.
Relative rates were calculated against the nominated control sample (e.g. wild-type CHD4 or control treatment nucleosomes).
Nucleosome/DNA-stimulated PARylation Reactions-PARylation and control reactions were performed at room temperature for 35 min. BHQ1-0W47 AlexaFluor488-labeled nucleosomes (0.5 M) or an equimolar amount of free BHQ1-0W47 DNA were incubated in 50 mM Tris, pH 7.5, 50 mM NaCl, 3 mM MgCl 2 in the presence of 1 unit/l of high-specific activity PARP1 (Trevigen) and 250 M NAD ϩ . Reactions were stopped via the addition of the PARP inhibitor 3-aminobenzamide (3-AB) to 1 mM either before or after the addition of PARP1. Control treatment reactions contained NAD ϩ and 3-AB but not PARP1.

CHD4 Contains a Conserved Domain at the N Terminus-
Sequence analysis of CHD4 (residues 1-364) revealed the presence of an 80-residue region (145-225) that is highly conserved across complex animals (Fig. 1b). For example, sequence identity between human and zebrafish CHD4 is ϳ90% in this region, whereas orthologues of CHD4 in plants lack this N-terminal region. The conserved sequence is predicted to encode a stable structure according to secondary structure and disorder prediction software, suggesting that it might constitute a functional domain. We expressed and purified a polypeptide comprising human CHD4(145-225), which we termed CHD4-N, and used standard solution NMR approaches to determine its three-dimensional structure. The solution structure obtained is of high precision, with a root mean square deviation over the backbone atoms of ordered residues (residues 150 -217) of 0.40 Å and, for all heavy atoms, 0.9 Å when the 20 lowest energy structures are superposed (Fig. 2a). Experimental restraints and structural statistics are reported in Table 1. The CHD4-N geometry has no outliers according to the Ramachandran plot generated by PROCHECK NMR (43), suggesting that the CHD4-N structure is of high quality.
CHD4-N Forms a Helical Bundle-The structure of CHD4-N consists of a four-helix bundle (Fig. 2a). Helices 1 and 2 are on opposite sides of the domain and are separated by a long linker, whereas helices 2 and 3 and helices 3 and 4 are linked by short turns. Helix 1 packs against helix 4, which in turn packs against helix 3. At the helix 2 end, CHD4-N presents a hydrophobic core comprising His-165 and Phe-167 of the long linker, Tyr-172 of helix 2, Tyr-178, Phe-181, and Phe-184 of helix 3, and Trp-209 and Phe-212 of helix 4 (Fig. 2b). Electrostatic surface charge analysis reveals the presence of two charged regions on opposite faces of the protein: a basic region along helices 3 and 4 and an acidic region along the long linker (Fig. 2c). Although in principle this observation could indicate dimerization or oligomerization of CHD4-N, size-exclusion chromatography-multiangle laser light scattering detector data show that CHD4-N is monomeric in solution (Fig. 2d). On the other hand, the combination of basic and acidic surfaces could suggest a possible interaction with chromatin in which the basic surface contacts DNA, whereas the acidic region simultaneously makes interactions with the highly basic histone proteins.
CHD4-N Is an HMG Box-like Domain-Structure matching of CHD4-N, performed by the structure search engine PDBe-Fold, identifies the fold as similar to that of HMG-box domains. The HMG-box is a versatile protein module that in general binds preferentially to distorted DNA structures (for review see Ref. 35). This domain is found in both HMG-only-containing proteins or as part of multi-domain proteins, such as transcription factors or chromatin remodeling factors.
The three most similar HMG-box structures displayed 26% sequence similarity with CHD4-N, and structural comparisons give root mean square deviation values of between 1.2-1.5 Å over 38 -39 C␣ atoms (Fig. 3a). All structural superpositions and sequence similarity occurred between the DNA binding region of the HMG-box and helices 3 and 4 of CHD4-N ( Fig. 3, b-d), the helices that form a positively charged surface. These observations are consistent with the idea that the helix 3/4 region might mediate binding to DNA. At the same time our structural data demonstrate that there is no homology between CHD4-N and structurally characterized PAR binding domains.

CHD4-N Can
Bind DNA-In light of the structural similarity with the HMG-box domain and the reported PAR binding activity of the N-terminal portion of CHD4, 15 N HSQC titrations were performed to assess the binding of CHD4-N to nucleic acids. 15 N HSQC titrations using a single-stranded DNA oligonucleotide revealed that CHD4-N can bind to a 15-nucleotide poly(A) homopolymer (ssA 15 , Fig. 4a). We then used MST to measure the affinity of CHD4-N for ssA 15 . In MST experiments the diffusion of a fluorescently labeled macromolecule in a temperature gradient is measured in the presence of increasing concentrations of a binding partner (51). Changes in diffusion are plotted to create a binding isotherm. Titration of fluorescein-labeled ssAA 15 with CHD4-N confirmed that the two species form a 1:1 complex with a dissociation constant, K D , of 32 Ϯ 3 M (Fig. 4b). Similarly, MST experiments performed using single-stranded poly(T) (ssT 15 ) showed 1:1 binding that fitted with a K D of 11 Ϯ 1 M (Fig. 4c). These data suggest that CHD4-N recognizes the DNA backbone structure rather than making specific interactions with the bases. To further assess DNA binding specificity, MST assays were per-     formed with the corresponding double-stranded DNA (d(A⅐T) 15 ). The calculated K D in these assays was 13 Ϯ 1 M (Fig. 4d), indicating that CHD4-N does not distinguish singlestranded from double-stranded DNA. To explore whether sequences N-or C-terminal to the core CHD4-N domain influenced DNA binding affinity, we expressed and purified eight polypeptides spanning different fractions of residues 1-355 of CHD4 (Fig. 5). Two could not be expressed (1-310 and 1-355). Affinities for the interaction of each of the others with ssA15 (measured by MST) are shown in Fig. 5. Overall, proteins with C-terminal extensions displayed ϳ10-fold higher affinity for ssA 15 than CHD4-N. We selected the polypeptide with the highest affinity, CHD4-(145-310) and also measured its binding to ssT 15 . Binding of CHD4-(145-310) to ssT 15 was also higher than for CHD4-N (2.7 M compared with 11 M, respectively). This indicates that the additional C-terminal sequence that is rich in basic amino acids improved binding to single-stranded DNA in a nonspecific manner.

CHD4-N and HMG-box Domains Have Similar Binding
Surfaces-The DNA binding properties of CHD4-N were further examined in a 15 N HSQC titration with ssA 15 ; up to 10 mol eq of ssA 15 was added. The interaction was in fast exchange on the chemical shift timescale, and residues that had the largest chemical shift changes after the addition of DNA were Lys-200, Met-201, Met-202, Val-204, Leu-205, Gly-206, Ala-207, Trp-209, and Arg-210 (Fig. 4, e and f). This set of residues lies essentially on one surface of helix 4 of CHD4-N, the same surface that was predicted to interact with nucleic acids due to its basic surface charge and structural homology with other HMG-box domains.
CHD4-N Binds PAR with Higher Affinity Than DNA-Given the published observation that the N-terminal portion of CHD4 has PAR binding activity, we performed binding experiments to determine if CHD4-N would bind to substrates that could mimic poly(ADP-ribose) molecules. Previously, PBZ (PAR-binding zinc finger) domains of the APLF (polynucleotide kinase-like) protein have been shown to bind similarly to ADP and ADP-ribose but not to adenine alone (26), suggesting that the substrate recognition occurs at the ribose-phosphate moiety. However, 15 N HSQC titrations of 15 N-CHD4-N with either ADP alone or a dinucleotide of ADP-ribose (up to 10 mol eq) did not give rise to any chemical shift changes. It is possible that ADP-ribose dinucleotide is too short to effectively mimic PAR, so we, therefore, tested the binding of CHD4-N to polymers of ADP-ribose. Commercially available PAR consists of a heterogeneous mixture of oligomers and polymers of different lengths and branched architectures, ranging from an estimated 2 to 300 subunits. This heterogeneity prevents accurate determination of a molar concentration. We estimated the average size of PAR molecules to be 150 subunits and calculated concentrations on that basis. Biotinylated PAR was incubated with fluorescein-tagged streptavidin, and this complex was used as   (Fig. 6a), ϳ50 times tighter than the affinity for DNA. Note that because PAR was the titrand, the calculated K D does not differ significantly for different estimated polymer lengths between 2 and 300 subunits. Furthermore, the shape of the binding curve did not indicate the presence of cooperativity even though multiple CHD4-N monomers could likely bind to a single PAR polymer. In contrast to the situation for DNA binding, the affinity of the longer CHD4-(145-310) polypeptide for PAR was ϳ7-fold lower (2.0 M) than was the affinity of CHD4-N. This effect could be due to the additional C-terminal residues preventing access to the PAR-binding site. Thus, these residues did not make a contribution to the interaction with PAR, suggesting that the minimal PAR binding region is the CHD4-N domain.
To confirm the binding of CHD4-N to PAR, we ran 15 N HSQC spectra of CHD4-N in the absence and presence of PAR (Fig. 6b). The addition of PAR (the molar ratio of protein:PAR was 1:0.3; only this quantity was available) gave rise to a range of selective changes in the CHD4-N spectrum. In this case the timescale for binding to PAR appeared to be slower than for binding to DNA, consistent with the higher affinity. Additional line broadening might also arise from the high molecular weight of the PAR ligand, although carbohydrates typically display very fast internal dynamics compared with proteins, which would serve to mitigate this effect. The majority of the peaks that suffered chemical shift changes upon binding lie on the linker between helices 1 and 2 and the surrounding surface (Fig. 6, c and d), suggesting that the surface in CHD4-N involved in PAR binding is not the same as the surface that binds DNA.
The CHD4-N Domain Is Not Essential to Recruit CHD4 to DSB Sites-To evaluate the effect of CHD4-N on CHD4 recruitment to DNA damage sites, we performed laser micro-irradiation experiments in a similar manner to those described previously (20). It has been shown that, when laser micro-irradiation is used to generate localized DNA damage in human U2OS cells, CHD4 co-localizes with ␥H2AX, a well established marker of DNA DSBs in a PARP-dependent manner. We tested several GFP-tagged mutants of CHD4 in these experiments. CHD4-WT corresponds to the full-length wild-type protein, CHD4-⌬N lacks the CHD4-N domain, CHD4-␣4A is a fulllength protein with five mutations to alanine on the DNA-binding surface of helix 4 of CHD4-N, and CHD4-⌬364 lacks the whole N-terminal region upstream of the PHD domains (Fig.  7a). As shown in Fig. 7b, GFP-tagged-CHD4-WT, -CHD4-⌬N, and -CHD4-␣4A are effectively localized to the nucleus and accumulate at DSB sites with similar kinetics (Fig. 7c). In contrast, GFP-CHD4-⌬364, which lacks both CHD4-N and the surrounding sequence that is predicted to be disordered, was present in both the nucleus and cytoplasm and was unable to accumulate at DSB sites.
Deletion of the N-terminal of CHD4 Reduces Nucleosome Remodeling Activity-We next assessed the role of the N-terminal region of CHD4 in the nucleosome remodeling activity of CHD4. First, we purified full-length FLAG-tagged recombinant CHD4 from HEK293 cells using anti-FLAG-Sepharose beads. Then we established that the purified protein was able to reposition nucleosomes in an ATP-dependent manner in a standard gel-based nucleosome repositioning assay. The addition of CHD4 and ATP to an asymmetric end-positioned nucleosome results in the appearance of a second band on a native DNA gel (Fig. 8a), consistent with CHD4 centering the nucleosome  through its intrinsic remodeling activity. To obtain a more quantitative estimate of CHD4 activity, we established a realtime FRET-based nucleosome repositioning. This assay is similar to that described by Yang et al. (52) except that the FRET dye pair has been modified to simplify measurements, increase throughput, and improve sensitivity. 4 Briefly, asymmetric endpositioned nucleosomes with 0-and 47-bp linker DNA on each side were assembled in which the DNA was labeled on the 0-bp linker with the dark quencher BHQ1. AlexaFluor488 was con-  S145  K146  E147  P148  K149  S150  S151  A152  Q153  Q153sc  Q153sc  L154  L155  E156  D157  W158sc  W158sc  G159  M160  E161  D162  I163  D164  H165  V166  F167  S168  E169  E170  D171  Y172  R173  T174  L175  T176  N177  Y178  K179  A180  F181  S182  Q183  Q183sc  Q183sc  F184  V185  R186  P187  L188  I189  A190  A191  K192  N193  N193sc  N193sc  P194  K195  I196  A197  V198  S199  K200  M201  M202  M203  V204  L205  G206  A207  K208  W209  W209sc  R210  E211  F212  S213  T214  N215  N215sc  N215sc  N216  N216sc  N216sc  P217  F218  K219  G220  S221  S222  G223  A224  S225 CHD4-N residue   Constructs that were designed to encode longer segments of the N-terminal part of CHD4 as shown were designed, expressed, and purified. Their affinity for ssA15 was measured by MST. K D values from two independent measurements (one carried out with the corresponding cleaved protein or with the GST-fusion protein, respectively) are shown.

R P M N A F M V W S R G Q R R K M A Q E N P K M H N S E I S K R L G A E W K V M S E A E K S D H I K R P M N A F M V W S R G Q R R K M A Q E N P K M H N S E I S K R L G A E W K L L S E A E K L E K V K R P M N A F M V W S S A Q R R Q M A Q Q N P K M H N S E I S K R L G A Q W K L L D E D E K V D H V K R P M N A F M V W S R A Q R R K M A Q E N P K M H N S E I S K R L G A E W K L L T E S E K
jugated to a cysteine mutant (T120C) of histone H2A; this residue is close to the exit point of the DNA in the nucleosome (Fig. 8, b  and c). The proximity of the BHQ1 moiety to the AlexaFluor488 in these nucleosomes results in strong quenching of AlexaFluor488 fluorescence. Any movement of the BHQ1 away from the Alex-aFluor488 dye, such as during ATP-dependent repositioning by a remodeling enzyme, results in a robust increase in fluorescence that can be monitored in real time (Fig. 8d).
PARylation of Nucleosomes/PARP1 Inhibits the Nucleosome Remodeling Activity of CHD4 -Given the interaction between CHD4 and PAR and that PARylation is a common nucleosomal modification (53)(54)(55)(56), we next tested if PARylation has any effect on CHD4 remodeling activity. Real-time nucleosome repositioning assays were performed as above, except that the nucleosomes were treated with PARP1, NAD ϩ , and the PARP1 inhibitor 3-AB as outlined in Fig. 9a. Repositioning assays were performed with wild-type CHD4 using either standard untreated nucleosomes or nucleosomes treated with NAD ϩ and 3-AB alone (control treatment) or with NAD ϩ and PARP1 that was inhibited by 3-AB at the start of the treatment (inhibited PARP). Fig. 9b shows that neither NAD ϩ /3-AB nor inhibited PARP1 have a discernible effect on the rate of nucleosome repositioning by CHD4. In comparison, nucleosome repositioning by CHD4 is greatly reduced when nucleosomes have been pretreated with active PARP1. These results indicate that PARylation, either of nucleosomes or PARP1 itself, inhibits the remodeling activity of CHD4. PARylation of CHD4 cannot account for the observed effect as PARP1 is inhibited by 3-AB before encountering CHD4 in the repositioning assay. Furthermore, these effects are not due to major disruption of the substrate nucleosomes, which look essentially identical in all cases by native PAGE.
Next, we assessed the activity of our N-terminal mutants in these assays. Fig. 9c shows that the relative rates of repositioning by the mutant proteins on control-treated nucleosomes mirrors the pattern seen with untreated nucleosomes in Fig. 8d, indicating NAD ϩ and 3-AB do not affect the activity of the mutants. Treatment of nucleosomes with inhibited PARP1 also does not lead to any significant changes in the rates of repositioning (Fig. 9d, gray bars). In contrast, nucleosomes treated with active PARP1 are repositioned much more slowly by either wildtype CHD4 or by any of the mutants (Fig. 9d, white bars). CHD4-⌬364 appears to be slightly less affected than the other mutants. However, it should be noted that the activity of CHD4-⌬364 is already significantly reduced compared with wild type (Fig. 9c); the reduction shown in Fig. 9d is in addition to that change and equates to Ͻ10% of normal wild-type activity. Given that the trend is similar across all CHD4 mutants, these data suggest that the N-terminal region of CHD4 does not specifically drive the PARylation-dependent reduction of CHD4 activity.
The inhibition of remodeling we observe after treatment of nucleosomes with active PARP1 could result from PARylation of the nucleosomes, PARP1 itself, or both. To investigate this issue, we set up PARylation reactions targeting PARP1 only. It is known that PARP1 activity is stimulated by nucleic acids (54), and so PARylation reactions were performed essentially as described in Fig. 9a, except that the nucleosomes were substituted with free BHQ1-0W47 DNA. This treatment maintains stimulation of PARP1 activity but means that PARP1 itself is the only available substrate. Subsequently, PARP1 was inhibited with 3-AB and the material mixed with nucleosomes in preparation for real-time repositioning experiments. The final reaction mixture contained equimolar amounts of nucleosomes, free DNA, and PARP1 at an equivalent concentration to previous experiments. Fig. 9e shows that in the absence of PARylation all repositioning reactions proceed at essentially the same rate. Note that the presence of the free DNA itself partially inhibits CHD4 activity (compare the black dashed line with ϩDNA treatments), most likely by simple competition with nucleosomal DNA for CHD4 binding. In contrast, the presence of auto-PARylated PARP1 (red curve) results in a marked decrease in the rate of nucleosome repositioning by CHD4 (compare the red with blue curves). However, the level of inhibition achieved under these conditions is not as great as when both PARP1 and nucleosomes are available as PARP1 substrates (compare the red line and dashed gray line).

CHD4 Contains an HMG-box-like Domain That Can Bind
PAR-The CHD4-NuRD complex has been shown to be important in the DNA-damage response. In particular, the N-terminal ϳ750-residue region of CHD4 has been reported to be sufficient to recruit the NuRD complex to sites of damage (20). This same region was also able to bind PAR in immunoprecipitation experiments, suggesting that it would contain a PAR binding motif. In addition, Drosophila melanogaster CHD4, which shares 30% similarity with human CHD4 in the corresponding region, was shown to interact in vitro with PAR through basic motifs in this region (21). We have identified a conserved and ordered domain at the N-terminal region of CHD4. This domain, CHD4-N, does not resemble other PAR binding domains for which structures are known but is instead related to HMG-box domains. In vitro binding assays show that CHD4-N binds single-stranded and double-stranded DNA with similar affinities, suggesting that interactions with such "standard" nucleic acids are probably not sequence-specific and most likely occur at the phosphate backbone. When compared with HMG-box-DNA complex structures, CHD4-N helices 3 and 4 superpose with the helices of HMG-box domains that are commonly involved in DNA binding. Our NMR data showed that this surface in CHD4-N was involved in DNA binding, suggesting that CHD4-N and HMG-box domains interact with nucleic acids in a similar way.
In contrast, even though CHD4-N bears no resemblance to known PAR binding domains, we have demonstrated that CHD4-N can bind PAR in vitro. Despite the substantial heterogeneity of the PAR preparation used in these experiments, we can infer unequivocally both that the binding is direct and that it is non-cooperative. We can also infer that CHD4-N binds PAR with a higher affinity than it binds DNA. Our NMR data indicate that residues from the acidic linker between helices 1 and 2 of CHD4-N are most involved in the interaction with f ) e) FIGURE 8. Deletion of the CHD4 N-terminal region reduces nucleosome repositioning activity. a, native PAGE (0.5ϫ Tris borate-EDTA, 5% acrylamide) analysis of nucleosome repositioning assays using recombinant human CHD4. End-positioned Cy3-labeled 0W47 nucleosomes (50 nM) were incubated for 30 min with different amounts of enzyme (1 or 10 nM) with or without ATP. The gel was scanned for Cy3 fluorescence. b, structure of the nucleosome core particle (PDB code 1kx5) showing dye attachment sites used in real-time repositioning experiments (H2A is shown in blue; H2B, H3, and H4 in gray; DNA in orange). The dark quencher BHQ1 (purple) is attached to the 5Ј-end of the DNA, and AlexaFluor488 (green) is attached via maleimide linkage to Cys120 in H2AT120C. c, schematic representation of the ATP-and remodeler-dependent movement of the BHQ1 dye relative to AlexaFluor488. In the starting asymmetric (0W47) nucleosomes, the proximity of BHQ1 to the Alex-aFluor488 moiety resulted in strong quenching of AlexaFluor488 fluorescence. The movement of BHQ1 away from the AlexaFluo488 during remodeling released quenching, and AlexaFluor488 fluorescence emission consequently increased. Coloring is the same as in b. d, nucleosome remodeling activity is dependent on the concentration of CHD4. Real-time fluorescence repositioning traces (520 nm) for 50 nM BHQ1-0W47 AlexaFluor488-H2A nucleosomes were recorded in the presence of increasing CHD4 concentrations. e, real-time repositioning traces of BHQ1-0W47 AlexaFluor488-H2A nucleosomes (50 nM) recorded in the presence of 10 nM wild-type CHD4 or the indicated CHD4 mutants. f, relative rates of repositioning of 50 nM BHQ1-0W47 AlexaFluor488-H2A nucleosomes by CHD4 mutant proteins in comparison to wild-type CHD4. Data are the average of four experiments using 10 nM enzyme. Error bars represent the S.E. Large errors for K757A are due to the model inadequately fitting the essentially null data and not large fluctuations in the data itself.
PAR, suggesting that the PAR binding surface is distinct from the DNA binding surface discussed above.
The observation that CHD4-N did not bind to either monomeric or dimeric ADP-ribose suggests that recognition involves a structural element of PAR that is not present in these two moieties. The most likely candidate is the branch structure that is characteristic of PAR, in which the terminal ribose of an ADP-ribose unit connects to two additional units through both its C1Ј and C2Ј carbons. At this stage, however, the nature of the interaction cannot be deduced. Further analysis will require the chemical synthesis of specific PAR substructures and the purification of homogeneous preparations of PAR species, both processes that are technically challenging. Surprisingly, the corresponding HMG-box-like region of Drosophila CHD4 did not show any interaction with PAR (21), but instead the basic sequences upstream and downstream of the HMG-box-like domain were sufficient to mediate PAR binding, suggesting that PAR binding activity might be partitioned among several N-terminal regions in CHD family members.
HMG Boxes Are Known for Their Ability to Recognize Unusual Nucleic Acid Structures-The HMG-box is one of the most abundant chromatin binding domains in metazoans (57). Typically, these domains bind kinked or bent DNA structures such as those found at entry or exit points to the nucleosome (57,58). HMG-box domains have not, however, previously been shown to bind poly(ADP-ribose).
Although we have shown that CHD4-N binds more tightly to PAR than to DNA, we cannot rule out that CHD4-N could be responsible for recognizing particular DNA structures in an analogous fashion to HMG1/2. In addition, the sequence around CHD4-N harbors stretches of basic and acidic residues that could improve binding to DNA. Basic extensions at either the N or C terminus of the HMG domain have been reported to increase the DNA binding affinity and stabilize the bent conformation of DNA, as seen in the transcription factor LEF-1, the yeast chromatin-associated NHP6A protein, and the D. melanogaster non-histone chromosomal HMG-D protein (59 -61).
Furthermore, several other ATP-dependent chromatin-remodeling complexes either contain or associate with HMG-box proteins (62)(63)(64)(65)(66). In these cases, however, the nature of the nucleic acid targets of the HMG-box domains is not known. Sequence identity between these HMG domains and CHD4-N is ϳ20 -25% around the DNA binding helices 3 and 4, not sufficient to infer that these HMG domains could also bind PAR.
CHD4, PAR, and Chromatin Remodeling-In addition to its well established connection with DNA repair, PARylation has also been shown to have effects in nucleosome remodeling; indeed, it is likely that these represent two faces of the same biochemical function. When ISWI is a target of poly-ADP-ribosylation, both ISWI ATPase activity and binding to DNA and nucleosomes are impaired (67). In contrast, the ATPase and chromatin remodeling activities of ALC1 are activated upon PARylation of PARP1 (68,69). This activation is a result of cooperative binding of PARylated PARP1 and ALC1 to nucleosomes. The interplay between PARylation and CHD4 appears to be different again. Our data show that the remodeling activity of CHD4 is strongly inhibited in the presence of PARylation. Yet, unlike ISWI, it is not the remodeler that is PARylated but rather nucleosomes and/or PARP1 itself. PARylated PARP1 is sufficient to elicit some inhibition, but the effect is enhanced when nucleosomes are also exposed to active PARP1, a situation that could result either from direct PARylation of nucleosomes or from nucleosomes acting as a greater stimulus of PARP1 activity (compared with free DNA). Further work is required to deconvolute these two possibilities. WT ΔN Δ364 α4A PARylation takes place FIGURE 9. PARylation of PARP1/nucleosomes inhibits nucleosome repositioning by CHD4. a, scheme outlining the treatment of nucleosomes with "active" or "inhibited" PARP1 used to generate PARylated and control substrates for real-time nucleosome repositioning assays. b, real-time nucleosome repositioning data for 10 nM wild-type CHD4 and 50 nM BHQ1-0W47-and Alex-aFluor488-H2A-labeled nucleosomes derived from untreated stock or pretreated as described in a. Only nucleosomes incubated with active PARP1 give rise to reduce nucleosome repositioning activity by CHD4. Note that data for the "untreated" and "control treatment" samples are directly underneath the inhibited PARP1Ј curve and, therefore, not visible. c, rates of repositioning of control treatment nucleosomes by CHD4 N-terminal mutant proteins relative to that of wild-type CHD4. Data are the average of three experiments and are recorded using the same conditions as in b. d, relative rates of repositioning of nucleosomes treated with active or inhibited PARP1 expressed as a fraction of the rate of repositioning of control-treated nucleosomes (shown in c)) using the same mutant. Data are the average of three experiments. All error bars represent the S.E. e, PARylated PARP1 inhibits CHD4 remodeling activity. DNA was used to stimulate PARP1 activity under active or inhibited conditions, essentially following the scheme described for nucleosomes in a and added to real-time fluorescence repositioning traces for 50 nM BHQ1-0W47 AlexaFluor488-H2A nucleosomes recorded in the presence of 10 nM CHD4 and 1 M PAR. The black and gray dashed curves correspond to the green and red curves in b, respectively. The magenta line shows that nucleosome repositioning is inhibited only to a small degree by free PAR (1 M).
Given our observation that the isolated CHD4-N domain binds PAR with submicromolar affinity, it was surprising that mutants targeting CHD4-N behaved largely like wild type in response to PARylation in nucleosome-repositioning assays. In addition, these mutants also had wild-type-like behavior in the laser-induced DNA damage experiments. Thus, CHD4-N appears not to be necessary for the recruitment of CHD4 to DSB sites and the PARylation-dependent inhibition of its nucleosome remodeling activity (at least on single nucleosomes). On the other hand, a larger region encompassing CHD4-N (CHD4-(1-364)) is required for the efficient accumulation of CHD4 at DSB sites and is also critical for the in vitro nucleosome repositioning activity of CHD4.
How does PARylated PARP1 inhibit CHD4 remodeling activity? One possibility is that binding of this species to CHD4 prevents it from binding nucleosomes, acting as a simple competitor in the same way free DNA also reduces CHD4 remodeling activity. Alternatively, binding to PARylated PARP1 might interfere directly with the catalytic cycle of CHD4, perhaps preventing a conformational change within the enzyme that is required for remodeling. Conversely, a direct PARP1-nucleosome interaction (PARylated PARP1 is known to bind nucleosomes; Ref. 70) might reduce the efficacy of CHD4 as a remodeler.
Finally, what is the biological context for this PARP1-mediated inhibition of CHD4 activity? We offer two possible models. First, in the context of DNA-damage repair, the presence of PARylated PARP1 at specific loci (e.g. broken DNA ends) might demarcate sites at which CHD4 should not act. In this scenario CHD4 would be recruited to damaged chromatin via PARylated PARP1 but be unable to directly remodel that chromatin. Instead, CHD4 action would be directed to areas up-and downstream of this site, either through interactions with other NuRD subunits or by subsequently being repositioned for action via the binding of its N-terminal region to other PARylated proteins. In addition, post-translational modification of CHD4 might also have a role to play in regulating its activity in this context. CHD4 has already been shown to be phosphorylated in a DNA-damage-dependent manner (20). Second, it might be that the CHD4-PARP1 interaction instead plays a role in the regulation of chromatin structure and gene transcription. PARP1 has been shown both to compact and to decondense chromatin under different circumstances and also to both stimulate and inhibit the transcription of specific genes (71). Thus, PARP1 might act to antagonize CHD4 activity in certain contexts. Choosing between these (or other) models will require a deeper understanding of the biochemical mechanisms through which both PARP1 and CHD4 act.