Poly(ADP-ribose) Polymerase-2 (PARP-2) Is Required for Efficient Base Excision DNA Repair in Association with PARP-1 and XRCC1

doi:10.1074/jbc.M202390200

Poly(ADP-ribose) Polymerase-2 (PARP-2) Is Required for Efficient Base Excision DNA Repair in Association with PARP-1 and XRCC1^*

Valérie Schreiber, Jean-Christophe Amé, Pascal Dollé^§, Inès Schultz, Bruno Rinaldi, Valérie Fraulob^§, Josiane Ménissier-de Murcia, and Gilbert de Murcia^¶

From the UPR 9003 du Centre National de la Recherche Scientifique, Laboratoire conventionné avec le Commissariat à l'Energie Atomique, Université Louis Pasteur, Ecole Supérieure de Biotechnologie de Strasbourg, boulevard Sébastien Brant, F-67400 Illkirch and the ^§ Institut de Génétique et de Biologie Moléculaire et Cellulaire, CNRS/INSERM/ULP, Collège de France, BP 163, 67404 Illkirch cedex, France

Received for publication, March 12, 2002, and in revised form, April 8, 2002

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The DNA damage dependence of poly(ADP-ribose) polymerase-2 (PARP-2) activity is suggestive of its implication in genome surveillanceand protection. Here we show that the PARP-2 gene, mainly expressedin actively dividing tissues follows, but to a smaller extent,that of PARP-1 during mouse development. We found that PARP-2and PARP-1 homo- and heterodimerize; the interacting interfaces,sites of reciprocal modification, have been mapped. PARP-2 wasalso found to interact with three other proteins involved in thebase excision repair pathway: x-ray cross complementing factor1 (XRCC1), DNA polymerase $beta$ , and DNA ligase III, already knownas partners of PARP-1. XRCC1 negatively regulates PARP-2 activity,as it does for PARP-1, while being a polymer acceptor for bothPARP-1 and PARP-2. To gain insight into the physiological roleof PARP-2 in response to genotoxic stress, we developed by genedisruption mice deficient in PARP-2. Following treatment by thealkylating agent N-nitroso-N-methylurea (MNU), PARP-2-deficientcells displayed an important delay in DNA strand breaks resealing,similar to that observed in PARP-1 deficient cells, thus confirmingthat PARP-2 is also an active player in base excision repair despiteits low capacity to synthesize ADP-ribosepolymers.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

In response to DNA interruptions, PARP-1,¹ the founding member of the poly(ADP-ribose) polymerase superfamily, catalyzes thesuccessive covalent addition of ADP-ribose units from NAD to alimited number of nuclear acceptors to form a branched anionicpolymer. PARP-1 is a nuclear enzyme involved in the detectionand signaling of DNA strand breaks introduced either directlyby ionizing radiation or indirectly following enzymatic incisionof a DNA lesion (abasic sites or oxidized or alkylated bases)repaired by the base excision repair (BER) pathway (see for reviewRef. 1). The discovery of numerous PARP-1 protein partnersand/or poly(ADP-ribose) acceptors involved in DNA architecture(histones H1 and H2B, lamin B, and high mobility group proteins)or in DNA metabolism (DNA replication factors, DNA repair proteins,i.e. XRCC1, transcription factors, topoisomerases, and PARP-1itself) has shed light onto the implication of PARP-1 in theseprocesses (see for review Ref. 1).

The function of PARP-1 in BER has long been assumed, until direct evidence demonstrated the presence of PARP-1 in the BERcomplex, associated to XRCC1 (2, 3) and DNA polymerase (pol) $beta$ (4). The polymer produced by PARP-1 upon activation by DNAbreaks triggers the recruitment of XRCC1, which shows high affinityfor oligo(ADP-ribosyl)ated PARP-1 (3-5). The requirement of PARP-1in BER was established in vivo, because PARP-1 knock-out cellsdisplayed a severe defect in strand breaks resealing followinggenotoxic treatment (6, 7). The preferential role of PARP-1in long patch BER was observed using extracts from these PARP-1knock-out cells (4). Photoaffinity labeling experiments revealedthat PARP-1 binds to BER intermediates (8). In reconstitutedin vitro systems containing purified human BER enzymes, PARP-1was shown to stimulate strand displacement DNA synthesis by DNApol $beta$ , in cooperation with FEN-1, leading to long patch BER (9).

The mouse models in which the PARP-1 gene has been knocked out (10-12) revealed the dual facets of PARP-1 function. In proliferativecells inflicted with sub-lethal doses of DNA damage, PARP-1 asa survival factor participates in DNA damage detection and signaling,leading to cell cycle arrest and DNA repair, to avoid deleteriousgenetic alterations (1). On the other hand, in post-mitoticcells, massive DNA damage as observed in pathological conditionssuch as cerebellar or cardiac ischemia or septic shock and tooveractivate PARP-1, triggering energy depletion that leads tocell death (see for review Ref. 13).

The PARP-1 knock-out mice were at the origin of the discovery of a new DNA damage-dependent PARP protein, named PARP-2, becausean unexpected residual poly(ADP-ribose) synthesis could be measuredin PARP-1-deficient cells following DNA damage (14, 15). Inaddition to PARP-2 (15-17), several other PARPs were discoveredalmost simultaneously, all having in common a conserved catalyticdomain responsible for poly(ADP-ribose) synthesis: PARP-3 (17),vPARP, a 193-kDa PARP belonging to the vault particles (18),Tankyrase 1 and 2, two proteins associated to the telomeric proteinTRF1 but also found in the Golgi or in nuclear pore complexes(19-22), and the 2,3,7,8-tetrachlorodibenzo-p-dioxin-inducibleTiPARP (23). PARP-1 and PARP-2 are the only ones reported tobe DNA damage-dependent, and in Arabidopsis thaliana both PARP-1and PARP-2 genes are induced by ionizing radiation (24). TheN-terminal part of mammalian PARP-2 contains a nuclear locationsignal and a functional DNA binding domain (15) distinct fromthat of PARP-1 (two zinc fingers). The nature of this DNA bindingdomain has yet to bedetermined.

In our attempts to further characterize PARP-2 and compare its biological implication with that of PARP-1 with respect toDNA damage surveillance, we discovered that the expression patternof PARP-2 and PARP-1 genes follows almost the same tissue distribution.The two proteins homo- and heterodimerize and poly(ADP-ribosyl)ateeach other. In addition, PARP-2 was found to interact with theBER proteins XRCC1, DNA pol $beta$ , and DNA ligase III, all being PARP-1partners as well. XRCC1 could be heteromodified by PARP-2 andwas able to negatively regulate PARP-2 activity as it does forPARP-1. The requirement for PARP-2 in BER was demonstrated invivo by the COMET assay in mouse embryonic cells lacking PARP-2.Our results showed that PARP-2 is a component of a functionalBER complex in vivo, likely through dimerization with PARP-1.This strengthens the role of PARP-2 as a survival factor followinggenotoxicstress.

EXPERIMENTAL PROCEDURES

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Plasmids-- The SmaI/NotI fragment encoding full-length murine PARP-2 (mPARP-2) cDNA was isolate from pVL-mPARP-2 (15), and sub-clonedinto HpaI/NotI sites of the pBC vector (25) in-frame with GST,allowing the expression of GST-mPARP-2 fusion protein. Truncatedforms of mPARP-2 were generated by PCR and cloned in-frame withGST in the pBC vector. The XhoI/XhoI PCR product encompassingfull-length mPARP-2 was ligated into the XhoI site of pEGFP-C3vector (CLONTECH, Palo Alto, CA), allowing the expression of GFP-mPARP-2.Complementary oligonucleotides encoding the FLAG epitope followinga methionine were linked into the EcoRV/EcoRI sites of the pIRES-eGFPvector (CLONTECH), allowing the expression of the FLAG epitope(F). The cDNA encoding full-length human XRCC1 (hXRCC1, kindlygiven by K. Caldecott) was subcloned into the EcoRI sites of pIRES-FLAGvector, allowing the expression of FLAG-tagged XRCC1 (F-hXRCC1).

In Situ Hybridization-- In situ hybridization was performed as described in Niederreither and Dollé (26) on serial sections (10 µm) of frozen embryosor mouse adult organs dissected from 2- or 16-week CD1 mice andfrozen in OCT. A XhoI/PstI fragment from a mouse PARP-1 EST clone(AA032357, Research Genetics, Huntsville, AL), encoding residues337-572, was subcloned into pBluescript SK(+), and antisense andsense mPARP-1 riboprobes were produced using T3 and T7 RNA polymerases,respectively. The murine PARP-2 probe corresponding to residues8-363 is described in Amé et al. (15). Exposure varied from4 to 6 weeks for PARP-1 and PARP-2probes.

Immunoprecipitation, GST Pull-down, and Western Blot Analyses-- For immunoprecipitation of purified proteins, 1 µg of purified hPARP-1 and/or mPARP-2 (as indicated) was incubated 2 h at4 °C with 20 µl of F1.23 monoclonal anti-PARP-1 antibody and 1µg of bovine serum albumin in 1 ml of LSB (20 mM Tris-HCl pH 8,120 mM NaCl, 0.1% Nonidet P-40, 0.5 mM phenylmethylsulfonyl fluoride)with protease inhibitors (Complete Mini, Roche Molecular Biochemicals,Mannheim, Germany). Protein G-Sepharose beads (Amersham Biosciences,Inc.) were added, and after 30-min incubation at 4 °C, bound immunecomplexes were washed three times with LSB buffer, and the pelletswere resuspended in Laemmli buffer and heated 3 min at 100 °Cbefore analysis by Western blotting. For immunoprecipitation ofendogenous PARP-1 from HeLa cells, cells were lysed in LSB buffer20 min at 4 °C, scraped, and centrifuge 20 min at 13,000 rpm at4 °C. After preclearing with protein G-Sepharose 30 min at 4 °C,20 µl of F1.23 anti-PARP-1 antibody was added, and immunoprecipitationwas carried on as describedabove.

GST-pull-down analyses were performed in HeLa S3 cells as described in Dantzer et al. (4).

For immunodetection, blots were incubated with anti-PARP-1 (Monte 1/2,500 (4)), anti-PARP2 (Yuc 1/2,500 (15)), anti-XRCC1(Roman 1/5,000 (3)), anti-DNA pol $beta$ (1/1,000 (4)), and anti-DNAligase III (1/250, kindly given by A. Tomkinson, San Antonio,TX) polyclonal antibodies or with anti-GST (1/10,000, Institutde Génétique et de Biologie Moléculaire et Cellulaire, Illkirch,France) and anti-GFP (1/1000, Roche Molecular Biochemicals, Indianapolis,IN) monoclonal antibodies. Blots where then probed with horseradishperoxidase-coupled secondary antibodies (goat anti-rabbit, 1/20,000or sheep anti-mouse, 1/20,000, Sigma Chemical Co., St. Louis,MO), and immunoreactivity was detected by enhanced chemiluminescence(PerkinElmer Life Sciences, Boston, MA). When indicated, 3-AB(1 mM) was added 2 h prior to lysis and maintained throughoutall the lysis and washingsteps.

Heteromodification of GST Fusion Proteins by PARP-2 or PARP-1-- GST pull-down assays were performed as described above, except that washes were done with HSB (20 mM Tris-HCl, pH 8, 500 mMNaCl, 0.5% Nonidet P-40, 0.5 mM phenylmethylsulfonyl fluoride).After a last wash with activity buffer (50 mM Tris-HCl, pH 8,4 mM MgCl₂, 0.3 mM dithiothreitol), each sample was split ontothree, the beads were pelleted (volume of the pellet: ± 20 µl)and resuspended in 300 µl of activity buffer containing either300 pmol of hPARP-1, 600 pmol of mPARP-2, or no PARP. Reactionwas started by the addition of 180 µl of activity buffer containingDNase I-activated calf thymus DNA, and [³²P]NAD. Final concentrations were 0.5 µg of DNA, 1 µM NAD for control,and PARP-2 and 0.1 µM for PARP-1 samples. In addition, each samplecontained 1 pmol of [³²P]NAD (1000 Ci/mmol). After 4 min at 25 °C, the reaction was stoppedby the addition of 500 µl of cold HSB on ice, and beads were washedthree times with HSB, resuspended in 12 µl of Laemmli buffer,and heated for 3 min at 100 °C before analysis by Westernblot.

Poly ADP-ribosylation of PARP-2 and XRCC1-- Purified mPARP-2 (200 pmol) was incubated with 1- to 8-fold purified hXRCC1 (3) for 2 min at 25 °C in 40 µl of activitybuffer containing 300 ng of bovine serum albumin, 5 µM [³²P]NAD (1000 Ci/mmol), and 100 ng of DNase I activated calf thymusDNA. Reaction was stopped by addition of 15 µl of Laemmli bufferon ice, and reaction products were analyzed by gel electrophoresison 8% SDS-PAGE and autoradiography of the Coomassie Blue-stainedand driedgel.

Generation and Culture of Mouse Embryonic Fibroblasts-- Mouse embryonic fibroblasts (MEFs) were isolated by micro-dissection of embryos at day 13.5 of gestation resulting from intercrossesbetween PARP-2^+/ heterozygous mice. Each embryo was genotyped by PCR to screenfor the disruption of the PARP-2 allele. The generation of thesemice and the genotyping PCR procedure will be described elsewhere.MEFs were maintained in Dulbecco's modified Eagle's medium, 4.5g/liter glucose medium supplemented with 10% fetal bovine serumand 0.5% gentamicin. For Western blot analysis, 10⁵ cells were resuspended in Laemmli buffer and sonicated, and proteinswere analyzed by Western blot as described above, using anti-PARP-2(Yuc) and anti-PARP-1 (Monte) polyclonal antibodies. The evaluationof residual poly(ADP-ribose) synthesis in MEF cell extracts wasperformed as described by Amé et al. (15).

Single Cell Gel Electrophoresis (COMET) Assay-- Passage 3 MEFs were thawed 48 h prior to harvesting on 60-mm Petri dishes. The following day, cells were either mock treatedor exposed for 30 min to N-nitroso-N-methylurea (MNU) as indicated.COMET assay was performed as described in Trucco et al. (6).Slides were dried in cold ethanol, and DNA was stained prior toscoring with 2 µg/ml ethidium bromide. Fifty COMET per slide wereobserved using a Zeiss Axioplan microscope equipped with a DP50camera (Olympus) and analyzed using the VisCOMET software (ImpulsBildanalyse GmbH, Gilsching, Germany) to calculate the tail momentas defined by Olive et al. (27).

RESULTS

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Tissue Distribution of PARP-1 and PARP-2 Transcripts during Embryogenesis and in Mouse Adult Tissues-- In situ hybridization experiments were performed to compare the expression patterns of the PARP-1 and PARP-2 genes at variousstages of mouse development and in adult tissues. Antisense probesfor PARP-1 and PARP-2 yielded specific labeling patterns thatappeared similar although not perfectly identical. During earlydevelopmental stages, both genes were expressed throughout theembryo (data not shown). Differential labeling patterns becameapparent by E12.5. At that stage, both genes were expressed athigh levels in the developing liver and kidney (Fig. 1, A-C).Only PARP-1, however, was found to be expressed at higher levelsin the genital ridge and the spinal ganglia. The signals observedthroughout other embryonic regions for both PARP-1 and PARP-2antisense probes were higher than for the corresponding senseprobes (data not shown), indicating a ubiquitous moderate expressionof both enzymes.

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Fig. 1. Comparative in situ analysis of PARP-1 and PARP-2 transcript distributions in mouse embryos and adults organs. Each row consists of dark-field views of PARP-1 (middle) and PARP-2 (right) in situ hybridization signals (white dots) on adjacent sections, and one of the corresponding bright-field views (left) to show histological details. Sagittal sections through the trunk region of an E12.5 embryo (A-C), the head and neck of an E18.5 fetus (D-F), and the abdominal cavity of an E18.5 fetus (G-I). The insets show an enlargement of one of the intestinal loops. Frontal sections of an adult (16-week-old) mouse brain (J-L). Sections through the testis of a 16-week-old male (M-O). ad, adrenal gland; cb, cerebellum; cg, cranial ganglia; cx, cortex; dg, dentate gyrus; gr, genital ridge; hp, hippocampus; ht, heart; in, intestinal epithelium (G) or interstitial tissue (M); ki, kidney; li, liver; lu, lung; ob, olfactory bulb; sg, spinal ganglia; st, seminiferous tubules; te, testis; th, thymus.

At E18.5 (Fig. 1, D-I), PARP-1 and to a lesser extent PARP-2 were preferentially expressed in the thymus and in regions ofthe nervous system (see below). Within the developing trunk, preferentialexpression of PARP-1 and PARP-2 persisted in the liver and becamerestricted to the cortical region of the kidney, the spleen, adrenalgland, and in stomach and intestinal epithelia (Fig. 1, G-I, anddata not shown). Note that PARP-1 transcripts appeared more restrictedthan those of PARP-2 toward the base of the intestinal crypts(G-I, insets).

From E14.5 to E18.5, as well as in the adult mouse, both genes were expressed at the highest levels in the thymus (Fig. 1,D-F and data not shown). In the adult mouse, PARP-1 and -2 expressionwas particularly high in the subcapsular zone of the thymus (datanot shown), where immature lymphocytes proliferate. Expressiondecreased as lymphocytes mature and was also found in the medulla.PARP-1, and to a lesser extend, PARP-2 transcripts were detectedin the white pulp of the spleen, especially in the germinal centersand in Peyer's patches in the intestine wall (data not shown)suggesting that high levels of PARP-1 and -2 expression are relatedto proliferation of immaturelymphocytes.

At E18.5, PARP-1 was preferentially expressed in specific brain regions (see the olfactory bulb, cerebellar, and cerebralcortex in Fig. 1, D-F) and in the olfactory epithelia. Expressionwas also higher in the cranial and spinal ganglia. PARP-2 expressionappeared more homogeneous in craniofacial tissues, although itwas slightly up-regulated in brain and cranial/spinal ganglia.In the adult brain (Fig. 1, J-L), both PARP-1 (28) and PARP-2genes showed high expression in neuronal cells forming the stratumgranulosum of the dentate gyrus and the stratum pyramidale ofthe hippocampus (CA 1-3). Weaker expression was detected in cellsof the cerebral cortex. Only PARP-1, however, was expressed athigh levels in the Purkinje cell layer of the cerebellum (datanotshown).

It is in testis that the expression pattern of PARP-1 and PARP-2 is the most distinct. PARP-1 is expressed at high levelsin the seminiferous tubules of the developing testis (Fig. 1,G-I). Expression was particularly strong in the basal layers ofthe seminiferous epithelium (Fig. 1, M-N, and Ref. 29), whereasno signal was detected in the luminal layers of the seminiferousepithelium indicating a down-regulation of PARP-1 expression atthe haploid stage of meiosis. In contrast, the PARP-2 signal wasweak and rather homogeneous, throughout the seminiferous tubulesand the interstitial tissue (Fig. 1O).

Apart from testis, the expression pattern of PARP-2 resembles that of PARP-1 except that the level of expression of PARP-2isweaker.

PARP-2 and PARP-1 Homo- and Heterodimerize-- PARP-1 is known to act as a catalytic dimer (30, 31). To investigate possible homodimerization of PARP-2, extracts fromHeLa cells transfected with a plasmid allowing the overexpressionof murine PARP-2 (mPARP-2) in fusion with GST were mixed withextracts from HeLa cells transfected with a plasmid allowing theexpression of either mPARP-2 fused to GFP, or GFP alone (Fig.2, lanes 2 and 6, respectively). GST fusion proteins were alsogenerated expressing truncated versions of mPARP-2 (see Fig. 2):amino acids 1-69 (Nt, the DNA binding domain), amino acids 63-202(domain E), and amino acids 203-559 (F, the catalytic domain).GST-fused proteins were trapped on glutathione-Sepharose beads,and copurifying GFP-tagged mPARP-2 was assessed by Western blotanalysis using anti-GFP antibody. Fig. 2 shows that PARP-2 isable to homodimerize (lane 2) through its E domain (lane 4).

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Fig. 2. PARP-2 homodimerizes. Top: schematic representation of mPARP-2. DBD, DNA binding domain. Bottom: Extracts from HeLa cells expressing GST (lane 1) and GST-tagged mPARP-2 (lanes 2 and 6) or deletion mutants of mPARP-2 (lanes 3-5) were mixed with extracts from HeLa cells expressing GFP (lane 6) or GFP-mPARP-2 (lanes 1-5). Interacting proteins were analyzed by GST-pull-down and Western blot with anti-GFP antibody (top). Blot was subsequently probed with anti-GST antibody (bottom). Lane 7 (input): 1/50 of the total cell extract of HeLa cells transfected with GFP-mPARP-2.

To further investigate the possibility that PARP-2 forms heterodimers with PARP-1 and to prevent any cross-reaction with PARP-2,we immunoprecipitated PARP-1 from HeLa cell extracts using theF1.23-specific monoclonal antibody raised against the N-terminalpart of PARP-1 (32). PARP-2 was coimmunoprecipitated with PARP-1(Fig. 3A, lane 3). A negative control using an unrelated antibodydid not trap either of these two proteins (lane 2). The interactionbetween PARP-2 and PARP-1 was also observed (lane 4 and see Fig.5B below) in the presence of the PARP inhibitor 3-aminobenzamide(3-AB), indicating that it occurs independently of their polymerizingactivity.

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Fig. 3. PARP-2 interacts with PARP-1 in vitro and in vivo. A, co-immunoprecipitation of PARP-2 with PARP-1 in HeLa cell extracts. Extracts from untreated (lanes 2 and 3) or 1 mM 3-AB treated (lane 4) HeLa cells were incubated with the F1.23 mouse monoclonal anti-PARP-1 antibody (lanes 3 and 4) or with anti $beta$ -galactosidase antibody (lane 2). Bound immune complexes were analyzed by Western blot with a mixture of anti-PARP-1 and anti-PARP-2 polyclonal antibodies. Lane 1, control immunoprecipitation without HeLa extract. B, coimmunoprecipitation of purified mPARP-2 with purified hPARP-1. 1 µg of hPARP-1 (lanes 1, 2, and 4) was incubated without (lanes 2 and 3) or with 1 µg of mPARP-2 (lanes 1 and 4) and with either F1.23 anti PARP-1 (lanes 2, 3, and 4) or with anti-lamin (lane 1) monoclonal antibodies. Bound immune complexes were analyzed by Western blot as in A. Inputs: hPARP-1 (40 ng) and mPARP-2 (20 ng).

The complex between PARP-1 and PARP-2 was reconstituted in vitro using purified proteins: mPARP-2 was coimmunoprecipitatedwith human PARP-1 (hPARP-1) using the F1.23 antibody (Fig. 3B,lane 4) demonstrating a direct interaction between PARP-2 andPARP-1.

Identification of the Domains Involved in the Association of PARP-2 with PARP-1-- To map the interaction domain within PARP-1, GST fusion proteins were generated expressing truncated versions of hPARP-1 (Fig.4A): amino acids 1-371 (A-C, the DNA binding domain), amino acids174-366 (B and C), amino acids 384-524 (D, encompassing the BRCTdomain), amino acids 572-1014 (F, encompassing the catalytic domain),and amino acids 525-655 (region E). These fusion proteins wereoverexpressed in HeLa cells, and GST pull-down experiments wereperformed followed by Western blot analyses. Copurification ofendogenous PARP-2 was efficient with constructs containing eitherthe DNA binding domain (lane 2) or the BRCT domain (lane 4). Thesedomains are those involved in the homodimerization of PARP-1 (Fig.4A and Ref. 30), as well as in the binding to several partnerssuch as XRCC1 (3), DNA pol $beta$ (4), DNA ligase III (Fig. 4A),histones, hUbc9, and transcription factors such as E47, TEF-1,RXR $alpha$ , Oct-1, and YY1 (see for review Ref. 1), suggesting thatthe DNA binding and the BRCT domains of PARP-1 are interfacesfor protein-protein association.

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Fig. 4. Interaction between PARP-2 and PARP-1: mapping of the interface domains. A, schematic representation of hPARP-1. GST (A and B, lane 1) and GST-tagged deletion mutants of hPARP-1 (A, lanes 2-6) or mPARP-2 (B, lanes 2-5) were expressed in HeLa cells and interacting endogenous proteins were extracted by GST-pull-down and analyzed by Western blot, using the indicated antibodies. Blots were subsequently probed with anti-GST antibody (A and B, bottom: one representative GST immunodetection). A, lane 7 and B, lane 6: crude extract of 4 × 10⁵ HeLa cells. In panel A, the stars show the immunodetection of PARP-2 that was carried out before GST immunodetection.

In reciprocal experiments, full-length and truncated versions of mPARP-2 fused to GST were expressed in HeLa cells and affinity-purifiedon glutathione-Sepharose beads. Copurification of endogenous PARP-1was efficient with full-length mPARP-2 and with its E domain (Fig.4B, lanes 2 and 4, respectively). These results showed that theE domain of PARP-2 is involved in both the homodimerization ofPARP-2 (Fig. 2) and the heterodimerization with PARP-1 (Fig. 4B).

PARP-2 and PARP-1 Poly(ADP-ribosyl)ate Each Other in Vitro-- The ability of PARP-1 to poly(ADP-ribosyl)ate PARP-2 was evaluated. Truncated versions of mPARP-2 fused to GST and expressedin HeLa cells were isolated on glutathione-Sepharose beads asdescribed above for Fig. 4B, except that the washing buffer usedcontained 0.5 M NaCl and 0.5% Nonidet P-40 to prevent the interactionbetween endogenous PARP-1 and mPARP-2 (data not shown). Trappedproteins on the beads were incubated for 4 min with either hPARP-1or mPARP-2 or neither, in the presence of [³²P]NAD (0.1 µM for hPARP-1 and 1 µM for mPARP-2 or control) andDNase I activated calf thymus DNA. Autoradiography revealed thathPARP-1 was able to poly-(ADP-ribosyl)ate the E domain of mPARP-2(Fig. 5A, panel 3), and to a lesser extent the DNA binding domain(panel 2). Automodification of mPARP-2 was weakly detected onlyon the E domain (panel 3). In the presence of 3-AB, no auto-/heteromodificationof the E domain of mPARP-2 was observed (panel 5), confirmingthat the radioactive labeling detected was due to polymer synthesis.

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Fig. 5. Heteromodification of PARP-1 and PARP-2. The GST-tagged deletion mutants of mPARP-2 (A) or hPARP-1 (B) were expressed in HeLa cells, extracted by GST pull-down, and incubated 4 min at 25 °C in activity buffer with or without purified hPARP-1 or mPARP-2 as indicated in the presence of [³²P]NAD (1 µM for control and mPARP-2, 0.1 µM for hPARP-1) and DNase I activated DNA. Samples were analyzed by Western blot with anti-GST antibody (left panels) and autoradiography (18-h exposure at $-$ 80 °C, right panels). A, bottom panel: 1 mM 3-AB was present throughout the experiment.

The reciprocal experiment showed that, in the presence of 1 µM [³²P]NAD, mPARP-2 poly(ADP-ribosyl)ates the DNA binding domain andthe BRCT domain of hPARP-1 (Fig. 5B, panels 1 and 3, respectively).These domains contain most of the polymer acceptor sites in theautomodification reaction of PARP-1 (Fig. 5B).

These results show that PARP-1 and PARP-2 can associate to form homo- or heterodimers and can be reciprocally poly(ADP-ribosyl)ated.

PARP-2 Belongs to a BER Complex Containing XRCC1, PARP-1, DNA pol $beta$ , and DNA Ligase III-- Given that PARP-1 is involved in base excision repair through its association with the scaffold protein XRCC1 (2-4), we examinedwhether PARP-2 and XRCC1 could also interact. The Western blotused to delineate the region of PARP-2 interacting with PARP-1(described in Fig. 4B) was probed with the anti-XRCC1 antibody.Results showed that full-length mPARP-2 (Fig. 4B, lane 2) andits E-domain (lane 4) interacted with endogenous XRCC1, demonstratingthat PARP-2 belongs to the BER complex through its interactionwith XRCC1. A similar approach was used to identify the regionof human XRCC1 (hXRCC1) interacting with PARP-2. Fig. 6A showsthat only the GST fusion proteins harboring the central BRCT domain(BRCT1) of human XRCC1 (lanes 3 and 4) could interact with endogenousPARP-2. Neither the second BRCT of hXRCC1 (BRCT2) nor the N-terminalpart of hXRCC1 known to interact with DNA pol $beta$ were found associatedto PARP-2 (lanes 2 and 5, respectively). Therefore, XRCC1 interactswith both PARP-1 and PARP-2 through the same region, the BRCT1module. The association between PARP-2 and XRCC1 resists stringentconditions (500 mM NaCl), indicating a high affinity of one proteinfor the other (data not shown).

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Fig. 6. PARP-2 interacts with XRCC1. A, proteins interacting with GST (lane 1) or GST-tagged deletion mutants of hXRCC1 (lanes 2-5) were extracted from HeLa cells by GST-pull-down and analyzed by Western blot with anti-PARP-2 and anti-PARP-1 antibodies (top: overlay of the two immunodetection signals. The star indicates a cross-reaction of anti-PARP-2 antibody with the GST-XRCC_1170-428 fusion protein). Blot was subsequently probed with anti-GST antibody (bottom). Lane 6, Crude extract of 2 × 10⁵ HeLa cells and lane 7, 10 ng of purified mPARP-2. B, GST (lanes 1 and 4) or GST-mPARP-2 (lanes 2, 3, 5, and 6) was expressed in HeLa cells, and interacting proteins were selectively extracted by GST-pull-down and analyzed by Western blot, using successively the indicated antibodies. Blot was subsequently probed with anti-GST antibody (boldface). Lanes 3 and 6, 1 mM 3-AB was present throughout the experiment. Input corresponds to 1/50 of the total cell extract used for the GST pull-down experiment. C, control FLAG (lanes 1 and 4) or FLAG-hXRCC1 (lanes 2, 3, 5, and 6) was expressed in HeLa cells and immunoprecipitated with anti-FLAG antibody. Interacting proteins were analyzed by Western blot using successively the indicated antibodies. Blot was subsequently probed with anti-XRCC1 antibody (boldface) to detect the immunoprecipitated FLAG-hXRCC1 protein. Lanes 3 and 6, 1 mM 3-AB was present throughout the experiment. Input corresponds to 1/50 of the total cell extract used for the immunoprecipitation.

DNA pol $beta$ (4) and DNA ligase III (Fig. 4A) are other BER partners that interact with PARP-1. We tested whether these BERfactors were associated with mPARP-2 by probing the Western blotdescribed in Fig. 4B with anti-DNA ligase III and anti-DNA pol $beta$ antibodies. Results showed that both DNA ligase III and DNA pol $beta$ were trapped with full-length mPARP-2 and with its E domain, implyingthat PARP-2 belongs to a multiprotein BER complex containing atleast PARP-1, XRCC1, DNA pol $beta$ , and DNA ligaseIII.

To examine whether the interactions between all these repair factors are regulated by poly(ADP-ribosyl)ation, we performeda GST pull-down analysis with mPARP-2 fused to GST expressed inHeLa cells in the presence or absence of 1 mM 3-AB (Fig. 6B).The interaction between mPARP-2 and either PARP-1 or DNA ligaseIII was independent of poly(ADP-ribose) synthesis. PARP's inhibitionled to a slight decrease in PARP-2/DNA pol $beta$ interaction and toa significant inhibition of PARP-2/XRCC1 interaction (Fig. 6B,compare lanes 5 and 6). A reciprocal experiment was performed,with the expression of the FLAG-tagged full-length hXRCC1 in HeLacells and immunoprecipitation of this recombinant protein in thepresence or absence of 1 mM 3-AB (Fig. 6C). Results showed thatthe association between hXRCC1 and DNA ligase III or DNA pol $beta$ was not significantly affected by PARPs inhibition, whereas theinteraction between hXRCC1 and both PARP-1 and PARP-2 was abolishedby PARP's inhibition (Fig. 6C, compare lanes 5 and 6 and 4) indicatingthat polymer synthesis is a prerequisite for XRCC1 binding toPARP-2 as well as to PARP-1.

XRCC1 Negatively Regulates PARP-2 Activity-- XRCC1 was shown both in vitro and in vivo to negatively regulate PARP-1 activity, by limiting PARP-1 automodification (3),forcing it to reside on the damaged DNA. The same effect was observedfor PARP-2 in an in vitro poly(ADP-ribosyl)ation assay containingmPARP-2, DNase I-activated DNA, and [³²P]NAD (Fig. 7A). Increasing the concentration of purified recombinantHis-tagged hXRCC1 (3) leads to the inhibition of mPARP-2 activity.This inhibition occurs even though hXRCC1 is a polymer acceptorof mPARP-2, as shown by the radioactive labeling correspondingto poly(ADP-ribosyl)ated hXRCC1. Thus, as for PARP-1, XRCC1 limitsPARP-2 automodification.

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Fig. 7. Poly(ADP-ribosyl)ation of XRCC1 and negative regulation of PARP-2. A, purified mPARP-2 (200 pmol, lanes 1-5) were incubated with 0 (lane 1), 200 (lane 2), 400 (lane 3), 800 (lane 4), or 1600 (lanes 5 and 6) pmol of purified hXRCC1 for 2 min at 25 °C as described under "Experimental Procedures." Reaction products were analyzed by 8% gel electrophoresis and autoradiography of the Coomassie Blue-stained and dried gel. B, the GST-tagged deletion mutants of hXRCC1 were expressed in HeLa cells and analyzed as described in Fig. 5.

To determine the polymer binding sites on XRCC1, truncated versions of hXRCC1 fused to GST were expressed in HeLa cells andpurified on glutathione-Sepharose beads at high stringency andin the presence of 3-AB, to avoid copurification of endogenousPARP-1 and PARP-2 (see Fig. 5B and Ref. 3). The beads wereincubated for 4 min with either hPARP-1 or mPARP-2 or neitherPARP, in the presence of [³²P]NAD (1 µM for control and mPARP-2, 0.1 µM for hPARP-1) and DNaseI-activated calf thymus DNA. The autoradiography shown in Fig.7B revealed that polymer binding sites were present in the C-terminalpart, lying between residues 314 and 428 (corresponding to theBRCT1 domain, panels 3 and 4) and to a lesser extend between residues427 and 633 (encompassing the BRCT2 domain, panel 5). These polymerbinding sites are functional for both mPARP-2 and hPARP-1. Theseresults indicate that hXRCC1 is mainly poly(ADP-ribosyl)ated onthe BRCT domain that interacts with PARP-1 and PARP-2. The C-terminalregion of hXRCC1 encompassing the BRCT2 domain that interactswith DNA ligase III could also be poly(ADP-ribosyl)ated, in contrastto the N-terminal part that showed no polymer binding sites (panel2). These results suggest that poly(ADP-ribosyl)ation of hXRCC1regulates its interaction with PARP-1 and PARP-2. The interactionbetween hXRCC1 and DNA ligase III was not affected by the inhibitionof PARP activity (see Fig. 6C), therefore the function of thepoly(ADP-ribosyl)ation of the C-terminal part of hXRCC1 is stillunclear. In addition to PARP-1, PARP-2, DNA pol $beta$ , and DNA ligaseIII, XRCC1 has been shown to associate other partners in BER suchas APE1 (33) and PNK (34). We hypothesize that poly(ADP-ribosyl)ationof the C-terminal part of XRCC1 may regulate its association withone (or more) ofthese.

PARP-2 Is Required for Efficient DNA Repair of Alkylated DNA in Vivo-- The presence of PARP-2 in a BER complex containing at least PARP-1, XRCC1, DNA pol $beta$ , and DNA ligase III strongly supportsa role of PARP-2 in this DNA repair pathway. We have generatedmice deficient in PARP-2 by inactivation of exon 9 of the PARP-2gene by homologous recombination.² Mouse embryonic fibroblasts (MEFs) were prepared from 13.5 d.p.c.embryos. Western blot analyses of crude extracts from these MEFsat passage 2 were performed using several polyclonal anti-PARP-2antibodies raised against full-length mPARP-2 or its catalyticdomain. These antibodies recognized PARP-2 in PARP-2^+/+ and PARP-2^+/ cells, but failed to detect any PARP-2 or truncated fragmentof it in PARP-2^/ cells (Fig. 8A, lower panel and data not shown). The same blotwas probed with the anti-PARP-1 antibody (Fig. 8A, upper panel),showing the presence of PARP-1 at comparable levels in MEFs fromany genotype, indicating no deregulation of PARP-1 expressionin the PARP-2 deficient cells.

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Fig. 8. DNA repair capacity of PARP-2^+/+, PARP-2^/, PARP-1^+/+, and PARP-1^/ MEFs treated with MNU as assessed by the COMET assay. A, Western blot analysis of total cell extract from passage 2 primary MEFs derived from 13.5 d.p.c. embryos resulting from intercrosses between PARP-2^+/ mice. The blot was sequentially probed with anti-PARP-2 (lower panel) and anti-PARP-1 (upper panel) polyclonal antibodies. B, relative PARP activity in PARP-2^+/+, PARP-2^/, and PARP-1^/ passage 3 primary MEFs. Cell extracts were incubated in standard conditions with [³²P]NAD and DNase I-activated DNA for 10 min at 25 °C. Activity is expressed as the percentage of the radioactivity of acid-insoluble material produced by cell extracts compared with PARP-2^+/+ cell extract. C, kinetic of re-ligation of DNA breaks induced by treatment of passage 4 MEFs cells (PARP-1^+/+, squares; PARP-2^+/+, circles; PARP-2^/, triangles; and PARP-1^/, diamonds) with 1 mM MNU for 30 min. The distribution of the tail moment as a function of repair time is indicated. The results shown are representative of one out of three experiments.

To evaluate the contribution of PARP-2 to PARP activity, we measured the polymer formation in whole cell extracts from PARP-2^+/+, PARP-2^/, and PARP-1^/ passage 3 MEFs (Fig. 8B). Results showed that in vitro poly(ADP-ribose)synthesis stimulated by DNA strand breaks was only moderatelyaffected in PARP-2^/ cells compared with PARP-2^+/+ cells, as opposed to the severe inhibition of polymer synthesisin PARP-1^/ cells (15). Immunofluorescence analyzes using the 10H monoclonalantibody raised against poly(ADP-ribose) showed no evident decreasein polymer synthesis in PARP-2^/ cells treated with 1 mM H₂O₂ or 2 mM MNU compare with PARP-2^+/+ cells (data not shown). These observations demonstrate that theabsence of PARP-2 has only a weak effect on the total PARP activitystimulated by DNAbreaks.

The capacity of PARP-2^/ cells to repair DNA lesions induced by alkylating agents was evaluated in vivo using the single-cellgel electrophoresis assay (COMET assay) and compared with thatof PARP-2^+/+, PARP-1^+/+, and PARP-1^/ cells. Passage 3 MEFs of the four genotypes were exposed to MNUfor 30 min as indicated in Fig. 8C, or mock treated. Measurementof the COMET tail moment reflecting the level of DNA fragmentation(27) revealed that DNA breakage varied in a linear manner withincreasing doses of MNU in the range of 0-1 mM for each genotype(data not shown). A repair assay performed with 1 mM MNU showedthat PARP-2^/ cells displayed a considerably slower rejoining kinetic (a 2-hdelay in DNA strand breaks resealing) compared with PARP-2^+/+ and PARP-1^+/+ cells, but similar to that observed for PARP-1^/ cells (Fig. 8C). These results unambiguously show that, despitethe presence of PARP-1, PARP-2^/ cells are defective in BER, demonstrating the requirement ofPARP-2 for efficient DNA strand breakresealing.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Similar Expression Pattern of PARP-1 and PARP2 Genes-- In this study, we showed that the expression of the PARP-1 and PARP-2 genes were almost similar, both being ubiquitously expressedat all stages of mouse development and in adult tissues, withvariable levels and with a generally weaker intensity for PARP-2compared with PARP-1. Expression of both transcripts seemed tobe correlated with proliferation, with higher levels occurringduring early fetal development and organogenesis and in the highlyproliferative cell compartments of adult mice. It is conceivablethat cells undergoing intensive division need functional DNA damagesensing and repair factors to avoid inherited genomic alterations.Interestingly, we observed that murine tumors also displayed highexpression of both PARP-1 and PARP-2 compared with normal tissue(data not shown). PARP-1 and -2 cannot be exclusively consideredas genes expressed in highly proliferating cells, because highexpression of both genes was also detected in the post-mitoticneurons of cranial and spinal ganglia, in hippocampal pyramidalcell layers, and in the dentate gyrus of the brain, although thetwo latter are known to contain progenitor neuronal cells (35).Several genes involved in DNA damage sensing and repair have beenreported to be expressed in neuronal cell lines, such as ATM (36),p53 (37), T:G mismatch-specific thymidine-DNA glycosylase (38),and APE1 (39), because these cells need to be efficiently protectedfrom DNAinjury.

PARP-1 and PARP-2 Heterodimerize-- The almost similar tissue distribution of PARP-1 and PARP-2 raises the question of why eukaryotic cells need simultaneouslytwo DNA damage-dependent PARPs. The requirement of a functionalPARP-1/PARP-2 heterodimer could be a plausible hypothesis. Inthis study, we demonstrated that PARP-2 and PARP-1 homo- or heterodimerizeand heteromodify each other. The PARP-2 E domain appears to actas a protein/protein interface regulated by auto- or heteromodification.Interestingly this domain is enriched in glutamate residues thatare potential automodification sites. Despite a significant aminoacid sequence conservation (38% identity, 47% similarity), thePARP-1 E domain displays none of these properties, unlike theneighboring BRCT motif. It seems likely that the E domain of PARP-2combines the properties of the D and E domains of PARP-1.

At the cellular level, both enzymes reside in the nucleus and colocalize partially into the nucleolus (40).³ This distribution suggests the need for heterodimers in the nucleolarcompartment where repetitive sequences (rDNA) need to be particularlyprotected.

Clearly, the biological significance of PARP-1/PARP-2 heterodimerization needs to be further elucidated. Does PARP-2 (endowedwith a low specific activity) need PARP-1 (the most active memberof the family) at a DNA lesion to amplify the cellular responseto DNA damage? Interestingly, a direct interaction between PARP-1and PARP-3, in the centrosome compartment, has also recently beenfound,⁴ suggesting a possible generalization of this observation to otherPARP homologues. This type of organization of PARPs in physiologicalcomplexes would increase the number of possible partners, whichin turn may adapt the responses of the cell to the nature of theinjury and to the localenvironment.

What Is the Function of PARP-2 in BER?-- It is more likely that both PARPs are required simultaneously to act in the same macromolecular base excision DNA repair complex.We and others have demonstrated the requirement of XRCC1, PARP-1,and DNA pol $beta$ for both short patch (SPR) and long patch (LPR) BERpathways (2, 4, 9, 41-45). This new link between XRCC1and PARP-2, observed only in the presence of polymer synthesis(as for the PARP-1/XRCC1 interaction) strongly suggests a concertedrole of the PARP-1/PARP-2 heterodimer during base excision repair,most probably at the recruitment step of XRCC1 at damaged sites.The phenotype of embryonic fibroblasts derived from PARP-2 knockoutmice displaying a severe delay in strand breaks resealing afterMNU treatment, supports this point of view. Interestingly, theabsence of PARP-2 is as dramatic as the absence of PARP-1. Thisobservation was quite unexpected, because PARP-2 activity in responseto DNA damage is about 10 times less than PARP-1 activity. However,if we assume that PARP-1 and PARP-2 have to act as a heterodimerin base excision repair, then the absence of one of each wouldhave the same consequence on repairefficiency.

Although more work is necessary to unravel the relative function of PARP-1 and PARP-2 in BER, the implication of the formerin this pathway is becoming more evident. Two characteristic propertiesof PARP-1 place this enzyme at early steps of the repair process,most probably downstream from the action of DNA glycosylases and/orAPE1: (i) detection and binding to the sugar-phosphate backboneinterruption; (ii) bending of the nicked substrate by 100° (46)that generates a distorted structure, in turn, recognized by thenext enzyme in the pathway (47). Both the ability of XRCC1 tobind the inside bend of DNA (48) and its increased affinityfor oligo(ADP-ribosyl)ated PARP-1 and/or PARP-2 or polymers (thisstudy and Refs. 3, 5) may contribute to organize a proteinplatform at the DNA break for additional BER enzymes: PNK, DNApol $beta$ , and finally DNA ligase III (see for review Ref. 49). Additionally,we have shown that the polymerization step of LPR was mainly affectedin PARP-1-deficient cells (4). Lavrik et al. (8) showedthat PARP-1, associated to DNA pol $beta$ , efficiently binds to therepair intermediates containing a flap 5'-abasic site that areformed before sub-pathway choice leading to either SPR or LPR.The same group demonstrated that PARP-1, together with FEN-1,stimulates strand displacement synthesis by DNA pol $beta$ (9) leadingto LPR. The authors proposed that the dRP group might serve asa sensor for the recruitment of PARP-1 onto BER intermediates,then PARP-1 would activate long patch BER by recruiting otherlong patch repair proteins. It remains an open question whetherPARP-2 is also bound to this dRP-containing repair intermediatealong with PARP-1. It is also possible that PARP-2, either aloneor together with PARP-1, is involved in a distinct step of therepair process. Because PARP-1 and PARP-2 DNA binding domainsdiffer totally, we can assume that they may have distinct DNAtargets. The elucidation of the specific DNA structures (repairintermediates) recognized by PARP-2 will undoubtedly help to elucidateat which step(s) of BER it isinvolved.

ACKNOWLEDGEMENTS

We thank Dr. Shanti Natarajan-Amé for critical reading of the manuscript. We are grateful to Prof. Pierre Chambon, Institutde Génétique et de Biologie Moléculaire et Cellulaire, Illkirch,France, for continualsupport.

	FOOTNOTES

^* This work was supported by Association pour la Recherche Contre le Cancer, Ligue Nationale contre le Cancer et Comité Régional,Electricité de France, Commissariat à l'Energie Atomique andCentre National de la Recherche Scientifique.The costs of publicationof this article were defrayed in part by the payment of page charges.The article must therefore be hereby marked "advertisement" inaccordance with 18 U.S.C. Section 1734 solely to indicate thisfact.

^¶ To whom correspondence should be addressed. Tel.: 33-390-24-47-07; Fax: 33-390-24-46-86; E-mail: demurcia@esbs.u-strasbg.fr.

Published, JBC Papers in Press, April 10, 2002, DOI 10.1074/jbc.M202390200

² J. Ménissier-de Murcia et al., manuscript inpreparation.

³ J.-C. Amé and V. Schreiber, manuscript inpreparation.

⁴ A. Augustin and C. Spenlehauer, manuscript inpreparation.

ABBREVIATIONS

The abbreviations used are: PARP, poly(ADP-ribose) polymerase; 3-AB, 3-aminobenzamide; APE1, apurinic/apyrimidinic endonuclease 1; BER, base excision repair; BRCT, BRCA1 C-terminus; d.p.c., days post-coitum; dRP, deoxyribose phosphate; EST, expressed sequence tags; FEN-1, flap endonuclease-1; GFP, green fluorescence protein; GST, glutathione S-transferase; h, human; m, mouse; SPR, short patch repair; LPR, long patch repair; MEF(s), mouse embryonicfibroblast(s); MNU, N-nitroso-N-methylurea; PNK, polynucleotide kinase; pol, polymerase; XRCC1, x-ray cross complementing factor 1; E, embryonic day.

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Poly(ADP-ribose) Polymerase-2 (PARP-2) Is Required for Efficient Base Excision DNA Repair in Association with PARP-1 and XRCC1*

Poly(ADP-ribose) Polymerase-2 (PARP-2) Is Required for Efficient Base Excision DNA Repair in Association with PARP-1 and XRCC1^*