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Central Role for the XRCC1 BRCT I Domain in Mammalian DNA Single-Strand Break Repair

School of Biological Sciences, University of Manchester, Manchester M13 9PT, United Kingdom

Received 30 October 2001/ Returned for modification 28 December 2001/ Accepted 16 January 2001

	ABSTRACT

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The DNA single-strand break repair (SSBR) protein XRCC1 is required for genetic stability and for embryonic viability. XRCC1 possesses two BRCA1 carboxyl-terminal (BRCT) protein interaction domains, denoted BRCT I and II. BRCT II is required for SSBR during G₁ but is dispensable for this process during S/G₂ and consequently for cell survival following DNA alkylation. Little is known about BRCT I, but this domain has attracted considerable interest because it is the site of a genetic polymorphism that epidemiological studies have associated with altered cancer risk. We report that the BRCT I domain comprises the evolutionarily conserved core of XRCC1 and that this domain is required for efficient SSBR during both G₁ and S/G₂ cell cycle phases and for cell survival following treatment with methyl methanesulfonate. However, the naturally occurring human polymorphism in BRCT I supported XRCC1-dependent SSBR and cell survival after DNA alkylation equally well. We conclude that while the BRCT I domain is critical for XRCC1 to maintain genetic integrity and cell survival, the polymorphism does not impact significantly on this function and therefore is unlikely to impact significantly on susceptibility to cancer.

	INTRODUCTION

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Thousands of DNA single-strand breaks (SSBs) arise in cells each day both directly by the disintegration of damaged sugars and indirectly as intermediates of base excision repair (BER) (4, 29). If not repaired, SSBs pose a threat to both genetic stability and cell survival, resulting in an increased frequency of mutations and chromosome aberrations (15, 23, 38, 50, 53, 56). The threat posed by unrepaired SSBs most likely reflects their ability to become double-strand breaks during chromosome replication (27). The enzymatic pathways adopted by cells for DNA SSB repair (SSBR) can be divided into four basic steps, involving damage detection, end processing, gap filling, and DNA ligation (see reference 8 for a review). For example, in the case of direct SSBs arising from sugar damage or spontaneous cleavage at abasic sites, the breaks are most likely detected by poly(ADP-ribose) polymerase 1 (PARP-1) or poly(ADP-ribose) polymerase 2 (PARP-2) (3, 18-20, 52). Next, damaged 3' or 5' termini present at the breaks are converted to conventional 3'-hydroxyl and 5'-phosphate chemistries by AP endonuclease (APE1/HAP1), DNA polymerase ß (Polß), or polynucleotide kinase (PNK). Finally, SSBR is completed by gap filling by Polß or Pol/ and DNA ligation by DNA ligase I (Lig1) or DNA ligase III (Lig3).

A feature of mammalian SSBR appears to be the employment of protein-protein interactions to stimulate individual component steps and/or the overall repair reaction. Arguably the most intriguing SSBR protein in this respect is XRCC1 (X-ray repair cross-complementing group 1), a polypeptide that interacts with PARP-1 (9, 33), PNK (54), Polß (9, 26), and Lig3 (10, 11) (reviewed in references 8 and 51). The interaction of XRCC1 with PNK stimulates both the 5'-kinase and 3'-phosphatase activities of this enzyme (54), and the interaction with Lig3 increases the intracellular stability of the ligase (11, 46). Studies have demonstrated a role for XRCC1 both in vitro and in vivo during the repair of either direct SSBs or those arising indirectly during BER (13, 14, 16, 17, 21, 48, 49, 54). Consistent with this, rodent cells lacking XRCC1 are hypersensitive to a broad range of genotoxins (7, 13, 15-17, 49, 56). Loss of XRCC1 also results in decreased genetic stability, including increased frequencies of spontaneous and/or induced chromosome translocations and deletions (15, 23, 49, 53, 56).

Given the number of protein-protein interactions involving XRCC1 it is important to identify the contribution made by each to genetic stability. To achieve this we are systematically mutating the individual protein binding domains within XRCC1. A striking feature of XRCC1 is the presence of two BRCA1 carboxyl-terminal (BRCT) domains, denoted BRCT I and BRCT II, that are located centrally and at the C terminus of this polypeptide, respectively (5, 12). The C-terminal domain is responsible for binding and stabilizing Lig3 (31, 37, 47) and is required for SSBR specifically during the G₀/G₁ phase of the cell cycle (36, 46). In contrast, little is known about the role of the central BRCT I domain. However, this domain has become the focus of considerable interest since it was identified as the site of a common human genetic polymorphism (R399Q) that appears from a large number of epidemiological studies to impact significantly on cancer risk (1, 2, 6, 22, 24, 28, 34, 41-45). This polymorphism has been reported to both increase and decrease cancer frequencies, depending on the type and location of the cancer. In addition, a correlation has been reported between the presence of the 399Q allele and levels of DNA damage, mutation, and ionizing radiation-induced mitotic delay (25, 30, 35). Although provocative, these epidemiological studies are difficult to interpret because little is known about the role and importance of the BRCT I domain and because of the variation in genetic background that is intrinsic to such studies. Here, we have directly examined the importance of the BRCT I domain to cell survival and SSBR in an isogenic cellular background and examined the impact of the common R399Q polymorphism on these processes.

	MATERIALS AND METHODS

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Expression constructs and Arabidopsis thaliana XRCC1. The mammalian cell expression vector pcD2E and the derivative pcD2EXH, which encodes C-terminally histidine-tagged XRCC1 (XRCC1-His), have been described previously (10). Derivatives of pcD2EXH harboring mutations within the BRCT I domain were created by site-directed mutagenesis using the QuikChange protocol (Stratagene). The sequence of all resulting open reading frames was confirmed by sequencing. The sequence of the A. thaliana XRCC1 was obtained by direct sequencing of the lambda PRL2 clone, 210J9T7, obtained from the Arabidopsis Biological Research Center (Ohio State University).

Cell culture. CHO cells were cultured as monolayers or in suspension as appropriate in alpha-minimal essential medium supplemented with 10% fetal bovine serum (GibcoBRL). Expression constructs were introduced into EM9 cells by calcium phosphate coprecipitation, and stable clones were selected in the presence of G418 (1.5 mg/ml) for 10 to 14 days.

Cell extracts and affinity purification of histidine-tagged XRCC1 protein complexes. Whole-cell extracts were prepared from frozen pellets of transfected EM9 cells (1 x 10⁷ to 3 x 10⁷) by resuspension in 1.5 ml of lysis buffer (50 mM Tris-Cl [pH 7.5], 130 mM NaCl, 0.5% Triton X-100, 10% glycerol, 1 mM dithiothreitol, 1/20 dilution of protease inhibitor cocktail [Sigma P8340]) and incubation on ice for 30 min. High-molecular-weight DNA was sheared by passage through a narrow-gauge needle several times, and insoluble material was removed by centrifugation in a microcentrifuge for 5 min at 4°C. To affinity-purify histidine-tagged XRCC1 complexes, clarified protein extracts (1.5 ml) from the different EM9 transfectants were incubated in parallel with 0.5 ml (bed volume) of nickel-nitrilotriacetic acid (NTA)-agarose (Qiagen) prewashed in lysis buffer and incubated with gentle agitation on ice for 30 min. The resulting suspensions were added to disposable 5-ml chromatography columns (Polyprep; Bio-Rad), and the protein-agarose beads were washed with 10 column volumes of lysis buffer containing 20 mM imidazole. Histidine-tagged XRCC1 protein complexes were eluted with 10 column volumes of lysis buffer containing 250 mM imidazole, with 0.25- to 0.5-ml fractions collected dropwise.

Indirect immunofluorescence. Immunofluorescence was conducted as described previously (46). Images were captured at x400 magnification.

SSBR assays. Single cell agarose gel electrophoresis was conducted on asynchronous or synchronized populations of CHO cells as described previously (36, 46).

Survival curves. Survival curves describing the resistance of transfected CHO cells to methyl methanesulfonate (MMS) were obtained as described previously, for ethyl methanesulfonate (46).

Nucleotide sequence accession number. The sequence of the open reading frame of A. thaliana XRCC1 was placed in GenBank (accession number AJ276506).

	RESULTS

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To examine the biological importance of the BRCT I domain, mutations were created that were analogous to those previously shown to disrupt the folding (57) and activity (36, 46, 47) of the BRCT II domain (Fig. 1A). These mutations lie within the ß3 sheet (LI360/361DD) and the highly conserved 3 helix (W385D) (Fig. 1B). The mutation in the 3 helix is particularly noteworthy, since it removes the tryptophan residue that is present in almost all BRCT domains (5, 12). Empty pcD2E expression vector or pcD2E constructs encoding wild-type (pcD2EXH) or mutant (pcD2EXH^LI360/361DD or pcD2EXH^W385D) histidine-tagged XRCC1 were transfected into XRCC1 mutant EM9 cells by calcium phosphate coprecipitation. For further analysis we attempted to isolate single clones that possessed similar levels of wild-type or mutant XRCC1, as measured by indirect immunofluorescence and immunoblotting. In the clones selected, the level of mutant XRCC1^W385D was essentially the same as the level of wild-type XRCC1, whereas the level of XRCC1^LI360/361DD was approximately half this amount (Fig. 2A and B). A hallmark phenotype of XRCC1 mutant cells is hypersensitivity to MMS (49). Whereas pcD2EXH was able to restore wild-type levels of resistance to MMS, neither pcD2EXH^LI360/361DD nor pcD2EXH^W385D increased survival much above that observed in EM9 cells expressing empty pcD2E vector (Fig. 2C). In agreement with these data, EM9 cells harboring either pcD2EXH^LI360/361DD or pcD2EXH^W385D were also unable to survive culture conditions in which 20% of genomic thymine base is replaced with chlorouracil during cell division, conditions that are lethal to cells lacking XRCC1 but which do not affect the survival of cells expressing wild-type XRCC1 (data not shown). The inability of pcD2EXH^LI360/361DD and pcD2EXH^W385D to complement the MMS sensitivity of EM9 cells did not reflect the use of single clones, since similar results were observed with pooled populations of >100 clones (data not shown). The lack of cellular complementation by pcD2EXH^LI360/361DD similarly did not simply reflect the lower level of expression of XRCC1^LI360/361DD, since wild-type XRCC1 or XRCC1 harboring the analogous mutation in the BRCT II domain fully restores resistance to the alkylating agent even at protein levels that are undetectable by immunoblotting (36; unpublished observations).These data suggest that mutation of the BRCT I domain disrupts the ability of XRCC1 to promote cell survival following MMS treatment. This contrasts dramatically with the BRCT II domain, which is largely dispensable for MMS resistance in cycling CHO cells (36, 46).

View larger version (51K): [in this window] [in a new window]   FIG. 1. (A) XRCC1 protein-protein interaction domains. The location of the NTD and the two BRCT domains within XRCC1 are indicated. The location of mutations in BRCT II previously employed (36, 46, 47) to disrupt activity of this domain, and the analogous BRCT I mutations employed in this study, are shown. Also shown is the location of the common human genetic polymorphism in BRCT I, R399Q. (B) CD alignment (NCBI) of the pfam00533 consensus BRCT domain with BRCT domains present in XRCC1, Lig3, and BRCA1. Boxed residues denote regions of hydrophobicity (with hydrophobic residues in boldface) that are conserved in the BRCT family, with those in dark grey denoting those that are most conserved. The position of secondary structure, based on the crystal structure of the BRCT II domain of XRCC1 (57), is shown at the top and bottom. The amino acids mutated to aspartate (D) in this study, and the position of the common human polymorphism (Q) is also indicated.

View larger version (31K): [in this window] [in a new window]   FIG. 2. Characterization of EM9 cells expressing wild-type or mutant XRCC1. (A) XRCC1 protein was examined in the indicated cell lines by indirect immunofluorescence, using the primary anti-XRCC1 MAb 33-2-5 and a fluorescein isothiocyanate-conjugated rabbit antimouse secondary antibody (DAKO). Nuclei were visualized with the DNA stain 4',6'-diamidino-2-phenylindole. Photographs were taken under x400 magnification. (B) XRCC1 protein levels were examined in cell extracts (20 µg of total protein) from the indicated cell lines (XH, EM9-XH; 360/361, EM9-XHLI360/361DD; 385, EM9-XHW385D; V, EM9-V) by immunoblotting, using the anti-XRCC1 MAb 33-2-5. (C) The cell lines indicated (see panel A for an explanation of symbols) were plated in six-well dishes (200 cells/well) and treated with the indicated concentrations of MMS for 1 h. After a wash, cells were incubated in drug-free medium for 7 to 10 days to allow formation of macroscopic colonies. The fraction of cells surviving MMS treatment was calculated by dividing the number of colonies in treated wells by the number in untreated wells. Results are the mean ± 1 standard deviation of three independent experiments.

View larger version (17K): [in this window] [in a new window]   FIG. 3. Measurement of MMS-induced SSBs in asynchronous populations of transfected EM9 cells. (A) EM9-V cells were treated for 15 min with the indicated concentrations of MMS, and the level of SSBs was quantified by alkaline agarose gel electrophoresis (comet assay). SSB levels are expressed as the tail moment, an arbitrary unit reflecting the product of the amount of DNA present in the "comet" tail and the tail length, after electrophoresis. (B) SSBs were quantified in the indicated EM9 transfectants before treatment for 15 min with 0.3 mg of MMS/ml (U, untreated), immediately after MMS treatment (T, treated), or after a subsequent repair incubation in drug-free medium for 20 min (R20) or 3 h (R180). Results are the average from four independent experiments (±1 standard deviation). The asterisk denotes the absence of a data point for a 20-min repair incubation in EM9-XHLI360/361DD cells.

View larger version (40K): [in this window] [in a new window]   FIG. 4. Measurement of MMS-induced SSBs in synchronized populations of EM9 transfectants. (A) DNA content of EM9-V cells synchronized in G1 (top panel) or S/G2 (bottom panel) by serum starvation and mimosine as described previously (36, 39, 46). Similar synchrony was observed with other EM9 transfectants (data not shown). The respective arrows denote peak positions of cells with G1 and G2 DNA content. (B) SSBs were quantified in the indicated EM9 transfectants in G1 (top panel) or S/G2 (bottom panel) before treatment for 15 min with 0.3 mg of MMS/ml (U, untreated), immediately after MMS treatment (T, treated), or after a subsequent repair incubation in drug-free medium for 3 h (R180). Results are the mean (±1 standard deviation) from three independent experiments.

View larger version (47K): [in this window] [in a new window]   FIG. 5. Presence of Lig3 and Polß in affinity-purified XRCC1 protein complexes. Total cellular protein (20 µg) from the cell lines indicated on the left was subjected to metal chelate affinity chromatography (nickel agarose; Qiagen) to purify histidine-tagged XRCC1 protein complexes. Aliquots of the recovered complexes were subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis and immunoblotted with anti-XRCC1 MAb (33-2-5), anti-Lig3 Pab (TL-25), or anti-Polß MAb (Clone 18S; Lab Vision).

View larger version (30K): [in this window] [in a new window]   FIG. 6. MMS sensitivity and SSBR capacity of EM9 cells harboring the human genetic polymorphism XRCC1R399Q. (A) The indicated cell lines (pooled populations of >100 independent transfectants) were plated in six-well dishes (200 cells/plate) and treated with the indicated concentration of MMS for 1 h. After a wash, cells were incubated in drug-free medium for 7 to 10 days to allow formation of macroscopic colonies, and the fraction of surviving cells was calculated as described in the legend for Fig. 2. (B) Total cellular protein (20 µg) from the indicated cell lines was fractionated by SDS-PAGE and immunoblotted with the anti-XRCC1 MAb, 33-2-5. (C) SSBs (expressed as tail moments) were quantified in the indicated EM9 transfectants before (-MMS) or immediately after (+MMS) treatment with 0.3 mg of MMS/ml. (D) The percentage of the MMS-induced SSBs shown in panel C remaining after a 3-h repair incubation in drug-free medium (calculated from the tail moment present after the repair incubation). Symbols are as in panel C. Results are the mean ± 1 standard deviation for three independent experiments.

	DISCUSSION

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It seems unlikely that the BRCT I mutations ablate XRCC1-dependent SSBR through an indirect effect on regions located outside of this domain. This is because these mutations did not disrupt binding of XRCC1 to either Polß or Lig3, two interactions known to occur within XRCC1 domains that flank the BRCT I domain. Rather, these data suggest a direct requirement for the BRCT I domain for SSBR in G₁ and S/G₂ and for cellular resistance to MMS.

The suggestion that the BRCT I domain is a fundamental component of XRCC1 function is supported by the comparison of XRCC1 homologues in different species. Whereas the BRCT II domain is present in human and other mammalian species, it is absent from both Drosophila melanogaster and A. thaliana XRCC1 (Fig. 7). In contrast, the BRCT I domain is present in all XRCC1 homologues so far identified.

View larger version (17K): [in this window] [in a new window]   FIG. 7. Evolutionary conservation of XRCC1 protein domains. Human (Hu), D. melanogaster (Dm), and A. thaliana (At) XRCC1 homologues were aligned using MACAW software, with vertical bars denoting conserved residues and enlarged boxes denoting regions of extensive conservation. The dotted box denotes the position of the BRCT II domain present in mammalian XRCC1 (represented here by the human protein). The domains identified by this alignment are the NTD, which contains the binding site for Polß, and the two BRCT domains, which contain the binding sites for PARP-1, poly(ADP-ribose), and Lig3. The Hu and Dm BRCT I domains, and the Hu and At BRCT I domains, share 54.5 and 52.8% identity, respectively.

It is also possible that the BRCT I domain mediates the recently identified interaction of XRCC1 with PNK (54). This interaction stimulates the activity of PNK at SSB termini, thereby enabling restoration of the conventional 3'-hydroxyl and 5'-phosphate chemistry required for completion of SSBR by gap filling and DNA ligation. Finally, it is possible that BRCT I also interacts with an as yet unidentified polypeptide or that it fulfills some other role. For example, it has been reported that BRCT domains can bind DNA directly, though the physiological significance of this is unclear (55). Clearly, given the importance of the BRCT I domain to XRCC1 function and genetic integrity, it is important to identify the role/s fulfilled by this structure.

A human polymorphism within BRCT I. One class of genetic factors that are likely to contribute to cancer predisposition is genetic polymorphisms. The XRCC1 BRCT I domain has recently attracted considerable interest because of the identification of a common genetic polymorphism (R399Q) at the C terminus of the BRCT I domain (43). Intriguingly, a large number of studies have reported an overrepresentation of one allele over the other among groups of individuals with a variety of cancers, including those of the lung, breast, bladder, and esophagus (1, 2, 6, 22, 24, 28, 34, 41-45). The explanation suggested for overrepresentation of one or another of the XRCC1 alleles among cancer groupings has been that the polymorphism impacts upon the activity of XRCC1 and consequently on SSBR efficiency and genetic stability. Consistent with this, a correlation has also been reported between the presence of the 399Q allele and levels of DNA damage, mutation, and ionizing radiation-induced mitotic delay (25, 30, 35).

Although provocative, such epidemiological studies are difficult to interpret in lieu of functional data concerning the impact of the polymorphism on protein function. Moreover, there is currently no clear consensus among the epidemiological studies as to which of the alleles is detrimental. A further complication with respect to XRCC1 is the additional location of several other DNA repair genes within the region of chromosome 19q13.2-13.3, such as ERCC1, ERCC2, DNA ligase I, and polynucleotide kinase, that could harbor polymorphisms that contribute to the apparent impact of the XRCC1 polymorphism. To circumvent these problems, in this study we compared directly for the first time the two XRCC1 isoforms for their ability to conduct SSBR and mediate cell survival in an isogenic background. In these experiments the two alleles were equally able to complement both the SSBR defect and sensitivity to MMS observed in XRCC1-deficient EM9 cells. Given that the BRCT I domain is critical to these functions, these experiments suggest that the polymorphism has little effect on the BRCT I domain or XRCC1 function.

In summary, we report that the BRCT I domain comprises the evolutionarily conserved core motif of XRCC1 and that this domain is critical for efficient SSBR and cell survival. However, the common human polymorphism located within this domain does not appear to significantly affect the ability of the BRCT I domain to support either of these processes following DNA alkylation, suggesting that it is unlikely to impact significantly on susceptibility to cancer.

	ACKNOWLEDGMENTS

 
R.M.T. was funded by Medical Research Council grants to K.W.C. (grants G9809326, G0001259, and G9821041).

	FOOTNOTES

 
* Corresponding author. Present address: Genome Damage and Stability Centre, University of Sussex, Falmer, Brighton BN1 9RR, United Kingdom. Phone: 01273 678123. Fax: 01273 678121. E-mail: k.w.caldecott{at}sussex.ac.uk.

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