The Rad51 Paralog Rad51B Promotes Homologous Recombinational Repair

doi:10.1128/MCB.20.17.6476-6482.2000

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Molecular and Cellular Biology, September 2000, p. 6476-6482, Vol. 20, No. 17
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The Rad51 Paralog Rad51B Promotes Homologous Recombinational Repair

Minoru Takata,¹^,² Masao S. Sasaki,³ Eiichiro Sonoda,⁴ Toru Fukushima,¹ Ciaran Morrison,¹ Joanna S. Albala,⁵ Sigrid M. A. Swagemakers,⁴ Roland Kanaar,⁴ Larry H. Thompson,⁵ and Shunichi Takeda¹^,²^,^*

Bayer-Chair Department of Molecular Immunology and Allergy, Faculty of Medicine,¹ CREST, JST (Japan Science and Technology),² and Radiation Biology Center,³ Kyoto University, Sakyo-ku, Kyoto 606-8501, Japan; Medical Genetics Center, Department of Cell Biology and Genetics, Erasmus University Rotterdam, 3000 DR Rotterdam, The Netherlands⁴; and Biology and Biotechnology Research Program, Lawrence Livermore National Laboratory, Livermore, California 94551-0808⁵

Received 9 September 1999/Returned for modification 27 October 1999/Accepted 26 January 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The highly conserved Saccharomyces cerevisiae Rad51 protein plays a central role in both mitotic and meiotic homologous DNArecombination. Seven members of the Rad51 family have been identifiedin vertebrate cells, including Rad51, Dmc1, and five Rad51-relatedproteins referred to as Rad51 paralogs, which share 20 to 30%sequence identity with Rad51. In chicken B lymphocyte DT40 cells,we generated a mutant with RAD51B/RAD51L1, a member of the Rad51family, knocked out. RAD51B^/ cells are viable, although spontaneous chromosomal aberrationskill about 20% of the cells in each cell cycle. Rad51B deficiencyimpairs homologous recombinational repair (HRR), as measured bytargeted integration, sister chromatid exchange, and intragenicrecombination at the immunoglobulin locus. RAD51B^/ cells are quite sensitive to the cross-linking agents cisplatinand mitomycin C and mildly sensitive to $gamma$ -rays. The formationof damage-induced Rad51 nuclear foci is much reduced in RAD51B^/ cells, suggesting that Rad51B promotes the assembly of Rad51nucleoprotein filaments during HRR. These findings show that Rad51Bis important for repairing various types of DNA lesions and maintainingchromosomeintegrity.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Double-strand DNA breaks (DSBs) occur during DNA replication and are produced by ionizing radiation. Since DSBs are so deleteriousto the cell, it is not surprising that there are two DSB repairpathways: nonhomologous end joining (NHEJ) and homologous recombinationrepair (HRR). Repair of DSBs by HRR requires the presence of homologousduplex DNA elsewhere in the genome, i.e., either a homologouschromosome or, more likely, a sister chromatid. NHEJ simply actsto process and ligate broken ends without a requirement for extensivehomology. These pathways are conserved from the yeast Saccharomycescerevisiae to humans (5, 8, 9, 19, 49, 53, 64).While HRR is the primary mechanism of DSB repair in yeast, vertebratecells use both the NHEJ and HRR pathways extensively (28, 34,35, 44). The analysis of radiosensitive yeast mutants hasrevealed a number of genes involved in HRR, which comprise theRAD52 epistasis group (reviewed in references 4, 29, and51).

Among the members of the RAD52 epistasis group, the structure and function of Rad51 have been conserved to a remarkable degreeamong all eukaryotes. Rad51 is structurally and functionally relatedto the Escherichia coli recombination protein RecA (reviewed inreference 32). The functional forms of both RecA and Rad51 aremultimeric helical nucleoprotein filaments that form on single-strandedDNA ends produced at DSBs (41). These filaments are involvedin the search for homologous sequence, DNA pairing, and strandexchange. Recombination intermediates produced in this way arethen processed further in reactions that involve DNA synthesis,branch migration, resolution of Holliday junctions, and ligation(reviewed in reference 4). The conservation of the RAD52 epistasisgroup genes from yeast to vertebrate cells suggests that the basicmechanism of HRR is maintained during evolution. However, whileS. cerevisiae RAD51 mutants are viable, Rad51 deficiency in vertebratecells causes rapid chromosomal aberrations and cell death (54).One possible explanation for this lethality is that the largersize of the vertebrate genome requires more HRR activity for chromosomestability (22, 54).

RAD51 paralogs (genes related by duplication within a single genome) have been identified in many eukaryotes and constitutethe Rad51-related gene family (63, 64). The completion ofthe S. cerevisiae genomic sequence established that four previouslyidentified proteins, Rad51, Rad55, Rad57, and Dmc1, constitutethe complete set of RecA relatives in this organism (1, 3,7, 37, 50). Thus far, seven members of the Rad51 proteinfamily have been identified in mammals. In human cells, Rad51(49), Dmc1 (23), XRCC2 (15, 28, 36), XRCC3 (36, 44,62), Rad51B (also called Rad51L1/hRec2) (2, 14, 47),Rad51C (Rad51L2) (18), and Rad51D (Rad51L3) (14, 30, 45)are highly conserved. While human Dmc1 is ~50% identical to humanRad51, the other human Rad51 paralogs are 20 to 30% identicalto human Rad51. These paralogs are less than 30% identical toeach other and to yeast Rad55 and Rad57 (reviewed in reference63). Overexpression of Rad51 in yeast partially suppresses theDNA repair defect of rad55 and rad57 mutant strains (25, 27),implying that Rad55 and Rad57 may functionally cooperate withRad51. This idea is supported by physical interactions betweenRad51 and Rad55 and between Rad55 and Rad57 (25, 27, 57).Similarly, physical interactions occur between human Rad51 andXRCC3, XRCC3 and Rad51C and between Rad51B and Rad51C (18, 36).These observations argue that Rad51 paralogs may function as Rad51accessory factors, analogous to yeast Rad55 and Rad57. Just asRad55 and Rad57 are important for HRR in yeast, in mammalian cellsthe Rad51 paralogs XRCC2 and XRCC3 have recently been shown toplay an important role in radiation resistance through HRR (28,44). Here we present evidence that the RAD51B gene is also importantforHRR.

Very recently, a RAD51B knockout mutation was made in mice but embryonic lethality prevented analysis of the cellular phenotype(52). Transcription of RAD51B was induced following UV or $gamma$ irradiation, suggesting that it has a regulated response to DNAdamage (42, 47). To investigate the role of Rad51B in vertebratecells, we generated RAD51B^/ cells from the hyperrecombinogenic chicken DT40 cell line (11,12). Comparison of the phenotype of this mutant with that ofRAD54^/ DT40 cells (5) suggests that Rad51B and Rad54 have distinctlydifferent roles in recombinationalrepair.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of targeting and expression vectors, gene targeting, and cell culture. Partial cDNA clones encoding the chicken RAD51B gene were isolated from a chicken spleen cDNA library (Clontech, Palo Alto,Calif.) by low-stringency hybridization using human RAD51B cDNAas a probe (2). A genomic fragment of the RAD51B locus wasPCR amplified from DT40 genomic DNA using a pair of RAD51B-specificprimers (5'-CCG TAA GCA TGG GAG GAC TAG ATG GGG C and 5'-CTC GATACA GAT GAA TGC TAC GGG TC). The flanking portions of the lociwere amplified from a DT40 genomic library constructed in lambdaFIX II phage vector (kindly provided by T. Nakayama and Y. Takami,Miyazaki, Japan) using the LA-PCR kit (Takara, Kyoto, Japan) witha combination of either one of the chicken RAD51B-specific primers(5'-GCC CCA TCT AGT CCT CCC ATG CTT ACG G and 5'-GAC CCG TAG CATTCA TCT GTA TCG AG) and the primer hybridizing with the T7 siteof the FIX II phage vector. Amplified fragments were subsequentlysubcloned into the TOPO-pCRII cloning vector (Invitrogen, Carlsbad,Calif.). The identity of genomic clones was confirmed by sequencingand partial mapping of theclones.

To construct RAD51B targeting vectors, ~1.8-kb and ~2.4-kb fragments at the RAD51B locus were cloned in the pBS vector (Stratagene,La Jolla, Calif.). A unique BamHI site was generated artificiallybetween the fragments. The bsr or puro drug resistance cassette(56) was inserted into this BamHI site. Gene targeting of theseconstructs was expected to disrupt two exons and delete the interveningintron, resulting in deletion of the coding sequence correspondingto published human Rad51B amino acids 137 to 173 (2). Cellculture and transfection were done as previously described (12).Before transfection, targeting vectors Rad51B-bsr and Rad51B-purowere linearized by NotI and SacI, respectively. Transfectantswere selected in the presence of blastocidin-S (Calbiochem, LaJolla, Calif.) at 25 µg/ml or puromycin (Sigma, St. Louis, Mo.)at 0.5 µg/ml.

To determine gene targeting frequencies, KU70-his (58), XRCC2-his (unpublished), and OVA-his (55) vectors were linearizedand transfected into wild-type and mutant cells. Genomic DNA wasextracted from each selected clone and analyzed for targetingevents by genomic Southern blot analysis. To construct the expressionvectors, hRAD51 (49) or hRAD51B (2) cDNA was inserted intothe EcoRI site of pAneo (56).

Western and Northern blot analysis. Cells were harvested and resuspended in lysis buffer (20 mM Tris-HCl [pH 7.5], 140 mM NaCl, 1 mM EDTA, 1 mM dithiothreitol,20 µg of aprotinin per ml, 20 µg of leupeptin per ml, 1 mM phenylmethylsulfonylfluoride, 1% NP-40). After 30 min of incubation on ice, the celllysates were centrifuged for 15 min at 4°C. The protein concentrationof the lysates was determined by the bicinchoninic acid proteinassay (Pierce, Rockford, Ill.). The lysates (10 µg/lane) wereseparated by sodium dodecyl sulfate-12.5% polyacrylamide gel electrophoresis,transferred to a nitrocellulose membrane, and probed with anti-Rad51antibody. The membrane was developed using horseradish peroxidase-conjugatedanti-rabbit immunoglobulin G (IgG) antibody and Super Signal chemiluminescentsubstrate (Pierce). Total RNA was extracted using TRIZOL (Gibco-BRL,Grand Island, N.Y.) following the manufacturer's instructions.Total RNA (20 µg/lane) was separated in a formaldehyde-1.2% agarosegel, transferred to a nylon membrane, and then hybridized witha ³²P-labeled RAD51B cDNA probe corresponding to the amino acid sequencesshown in Fig. 1A.

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FIG. 1. Gene targeting of RAD51B loci. (A) Amino acid (aa) sequence comparison between human and chicken Rad51B cDNAs. The Walker A and B motifs for nucleotide binding are overlined, and the sequence deleted by gene targeting is indicated. Letters in gray boxes represent identical amino acids in the two species, whereas those in open boxes represent similar (P, A, G, S, and T; E, D, N, and Q; V, I, L, and M; F, W, and Y; R, K, and H) amino acids. Numbers denote amino acid positions. (B) Schematic representation of part of the RAD51B locus, the gene disruption constructs, and the configuration of the targeted alleles. B, BamHI site; E, EcoRI site. Solid boxes indicate the positions of the exons. Only disrupted exons are indicated. (C) Southern blot analysis of BamHI-digested genomic DNA from cells with the indicated genotypes of the RAD51B gene with the probe shown in panel B. The positions and sizes of the hybridizing fragments of the wild-type and targeted loci are indicated. (D) Northern blot analysis of total RNA with a chicken RAD51B cDNA fragment as a probe. The same membrane was reprobed with the chicken $beta$ -actin fragment (12).

Flow cytometric analysis of cell viability, cell counting, and rate of Ig gene conversion. To determine cell viability, cells were resuspended in phosphate-buffered saline containing propidium iodide at 5 µg/ml andanalyzed by FACScaliber (Becton Dickinson, Mountain View, Calif.).Cells were counted in triplicate cultures using a fixed numberof plastic microbeads and a FACScaliber as previously described(58). The rate of Ig gene conversion was examined as previouslydescribed (11, 59).

Analysis of chromosome aberrations and SCEs. Chromosome and sister chromatid exchange (SCE) analysis was carried out as previously described (54, 55). To analyze mitomycinC (MMC)-induced SCEs, cells were incubated in medium containingMMC at 0.05 µg/ml for 12 h (the length of a single cell cycleof DT40 cells is ~8 h). Colcemid at 0.1 µg/ml was added for thelast 1.5 h of this incubation beforeharvest.

Measurement of cells surviving $gamma$ irradiation or treatment with cisplatin or MMC. Clonogenic survival was monitored by colony formation assay as previously described (58). Briefly, following various genotoxictreatments, appropriate numbers of cells were plated into six-wellcluster plates containing complete medium supplemented with 1.5%methylcellulose (Aldrich, Milwaukee, Wis.). Colony numbers werecounted after 7 to 10 days, and percent survival was determinedrelative to numbers of colonies of untreated cells. To measuresensitivities to cisplatin (Nihon-Kayaku, Tokyo, Japan) and MMC(Kyowa-Hakkou, Tokyo, Japan), cells were incubated at 39.5°C incomplete medium containing these drugs for 1 h and then washedthree times with warm medium. ¹³⁷Cs $gamma$ irradiation (Gammacell 40E; Nordion International, Kanata,Ontario, Canada) was done after cells were plated on six-wellclusterplates.

Visualization of Rad51 foci. Cells were harvested at the indicated time points after $gamma$ irradiation or MMC treatment. Cytospin slides were prepared usingCytospin 3 (Shandon, Pittsburgh, Pa.). Staining and visualizationof Rad51 foci were performed as previously described (65).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Generation of RAD51B^/ mutant cells and their proliferative properties. To construct RAD51B disruption vectors, we isolated a partial cDNA encoding chicken RAD51B (Fig. 1A). The sequence surroundingthe putative ATP binding sites is highly conserved between thechicken and human Rad51B proteins (10) (Fig. 1A). However, theextremely well-conserved GXXXXGKTQ motif in the Walker A box ischanged to SXXXXGKTQ in the chicken sequence in both cDNA andgenomic isolates. Two RAD51B disruption constructs, RAD51B-puroand RAD51B-bsr (Fig. 1B), were expected to replace the chickenRAD51B coding sequence for amino acids 137 to 173 with the selectionmarkers. The disruption of both RAD51B alleles in two independentlyisolated clones was verified by Southern and Northern blot analyses(Fig. 1C andD).

The proliferative properties of RAD51B^/ cells were monitored by growth curves and by cell cycle analysis. The growth rate ofRAD51B^/ clones was significantly lower than that of wild-type cells.High expression of human Rad51B in RAD51B^/ clones restored their growth rate to a wild-type level (Fig.2A). A pulse-chase experiment with bromodeoxyuridine showed thatthe length of a single cell cycle is comparable between wild-typeand RAD51B^/ cells (data not shown). On the other hand, flow cytometric analysisshowed that more dead cells were present in RAD51B^/ cultures than in wild-type cultures (Fig. 2B). Thus, the lowerproliferation rate of RAD51B^/ cell cultures is likely caused by an elevated rate of cell death.The fraction of RAD51B^/ cells dying spontaneously during a single cell cycle was calculatedto be 20% (58), which is not significantly different from thepercentage of metaphase cell having chromosomal aberrations (Table1). The plating efficiencies of cells in methylcellulose plateswere 100% for wild-type cells and ~50% for RAD51B^/ cells.

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FIG. 2. Growth rate and viability of RAD51B^/ cells. (A) Growth curves of cells of the indicated genotypes. Means ± standard deviations of triplicate cultures are shown. (B) The level of spontaneous cell death was assessed by flow cytometric analysis of propidium iodide uptake and forward scatter representing cell size. The values shown are percentages of dead (propidium iodide-bright and propidium iodide-dim) cells.

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TABLE 1. Spontaneous chromosomal aberrations per 100 cells^a

Given the possible role of Rad51B in HRR of DSBs, cell death in RAD51B^/ cultures may be caused by a defect in the removal of DSBs thatnormally arise during DNA replication (reviewed in references17, 22, and 31). To test this hypothesis, we performed chromosomeanalysis of metaphase-arrested cells (54). RAD51B^/ cells displayed a significantly increased level of spontaneouschromosome breaks (Table 1), which likely lead to cell death,and the mutant cells exhibited more chromosomal aberrations thandid RAD54^/ cells. This difference is consistent with the slower growth rateand higher level of death of RAD51B^/ cells compared to RAD54^/cells.

Defective homologous recombination in RAD51B^/ cells. The spontaneous chromosomal aberrations in RAD51B^/ cells may be caused by defective HRR of replication-associated DSBs. Toestimate the HR capacity of RAD51B^/ cells, we examined the rate of intragenic homologous recombinationat the Ig light-chain (IgL) locus (i.e., Ig gene conversion),the efficiency of targeted integration of transfected genomicDNA constructs, and the frequency ofSCE.

In a manner similar to the process of B-cell diversification in the bursa of Fabricius, DT40 cells continue to diversify theirIg loci by gene conversion with pseudogenes serving as donors.To measure gene conversion, RAD51B^/ clones were generated from a surface IgM-negative (sIgM) variant called clone 18. This clone contains a frameshift inthe rearranged V segment of its IgL locus (11, 59). Sinceoverlapping gene conversion events leading to re-expression ofsIgM can repair this mutation, we measured the percentage of sIgM⁺ revertants among 40 subclones of wild-type, RAD51B^/, and RAD54^/ cells. The calculated Ig gene conversion rate was 8.3 × 10⁴ for wild-type cells and 1.70 × 10⁴ for HRR-deficient RAD54^/ control cells (5). Like RAD54^/ cells, RAD51B^/ cells also exhibited a significant reduction in intragenic HRR,i.e., to 3.5 × 10⁴. We next measured the frequencies of targeted integration atthe KU70, OVALBUMIN, and XRCC2 loci and found no targeting eventsin RAD51B^/ cells (Table 2). The complementation of RAD51B^/ cells with human RAD51B cDNA restored the targeting frequency,showing that Rad51B is indeed involved in HRR.

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TABLE 2. Targeted integration frequencies^a

We previously showed that at least a portion of SCEs reflects postreplicational HRR of spontaneous DNA lesions and involvescrossing over between sister duplexes (55). RAD51B^/ cells, together with control RAD54^/ cells, exhibited a significant reduction in the spontaneous levelof SCEs (Fig. 3). A similar reduction in SCE levels was observedafter treatment of the RAD51B^/ cells with MMC, which is known to stimulate SCE.

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FIG. 3. Level of SCE per cell. Cells were incubated with or without MMC (0.05 µg/ml) for 12 h and treated with colcemid during the last 1.5 h of this incubation to enrich mitotic cells. One hundred fifty cells were analyzed in each preparation. Error bars represent standard errors calculated as previously described (58).

Rad51B promotes the formation of Rad51 foci after genotoxic treatment. To further assess the role of Rad51B in recombinational repair, we analyzed Rad51 focus formation. Immunostaining of vertebratecell nuclei has shown that they form visible complexes of Rad51during meiotic recombination and mitotic DNA repair (6, 16,21, 33, 38, 61, 66). It is believed that Rad51 focirepresent nucleoprotein filaments engaged in recombinational repair(46). We exposed cycling wild-type and RAD51B^/ DT40 clones to $gamma$ rays and MMC and then immunostained the cellswith anti-Rad51 serum. We found that the formation of Rad51 fociwas severely impaired in RAD51B^/ cells following $gamma$ irradiation and MMC treatment (Fig. 4 and 5A).Western blot analysis of the Rad51 protein revealed normal steady-statelevels of Rad51 in RAD51B^/ DT40 cells after the genotoxic treatments (Fig. 5B). Thus, RAD51B^/ cells are defective in the damage-induced redistribution of Rad51within the nucleus.

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FIG. 4. Immunofluorescent visualization of Rad51 subnuclear foci. Wild-type (A to C), RAD54^/ (D to F), and RAD51B^/ (G to I) cells were analyzed 5 h after genotoxic treatments. Cells were treated with either 8 Gy of $gamma$ radiation (IR) (B, E, and H) or 500 ng of MMC per ml (for 1 h) (C, F, and I).

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FIG. 5. Induction of Rad51 focus-positive cells after genotoxic treatments. (A) Cells with the indicated genotypes were analyzed at the indicated time points after either $gamma$ irradiation (IR; 8 Gy) or MMC treatment (500 ng/ml, 1 h). A cell containing more than four distinct foci was scored as positive. Each bar represents the result of scoring at least 100 cells. (B) Rad51 protein expression before and after exposure to 8 Gy of $gamma$ irradiation. At the indicated time points, total cell lysates were prepared and the same amount of protein was loaded into each lane. WT, wild type.

As a control, Rad51 focus formation was assayed in RAD54^/ cells. Interestingly, we observed clear differences between RAD51B^/ and RAD54^/ cells with respect to Rad51 focus formation. First, the percentageof RAD54^/ cells containing spontaneous Rad51 foci was about fivefold higherthan for wild-type and RAD51B^/ cells (Fig. 4 and 5A). Second, the absence of the Rad54 proteindid not abrogate the induction of Rad51 foci; in fact, more Rad51foci were detected in RAD54^/ cells than in wild-type cells (Fig. 4 and 5A). A simple explanationfor these findings is that in the absence of Rad54, HRR is arrestedimmediately after the formation of nucleoprotein filaments, resultingin their accumulation. This explanation is consistent with a rolefor Rad54 protein in the synaptic phase of the homologous DNApairing reaction (43) and is also supported by the presenceof Rad51 foci during meiosis in Rad54-deficient yeast (20).In contrast, Rad54 is required for Rad51 focus formation in murineembryonic stem cells (60). Thus, the role of Rad54 in Rad51focus formation may differ among species and/or among celllines.

Increased sensitivities of RAD51B^/ cells to various genotoxic treatments. The DNA repair capacity of RAD51B^/ cells was analyzed in colony survival assays. As a control for these experiments, we includedHRR-deficient RAD54^/ DT40 cells (5). We examined the cellular sensitivity to ionizingradiation and to the DNA cross-linking agents MMC and cisplatin.RAD51B^/ and RAD54^/ cells were comparable in radiosensitivity (Fig. 6A), whereasRAD51B^/ cells showed higher sensitivity to both MMC and cisplatin comparedwith RAD54^/ or wild-type cells (Fig. 6B and C). The elevated level of chromatidbreaks induced by $gamma$ irradiation in RAD51B^/ cells suggests that their defective DSB repair (Table 3) causestheir elevated radiosensitivity. Human Rad51B expression in RAD51B^/ cells substantially increased resistance to the three agents(Fig. 6A to C).

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FIG. 6. Sensitivity of clones of the indicated genotypes to DNA-damaging agents. The fractions of the surviving colonies after the indicated treatment of cells compared to nontreated controls of the same genotype are shown on the y axis on a logarithmic scale. Panels: A, $gamma$ irradiation; B, MMC; C, cisplatin (CDDP). The dose of radiation treatment and concentrations (conc) of MMC and cisplatin are displayed on the x axis on a linear scale in each graph. The data shown are means ± standard deviations of at least three separate experiments. The cisplatin sensitivity data of RAD54^/ cells are not shown here but were previously described (65). (D) Western blot analysis with rabbit anti-Rad51 serum showing the amounts of endogenous chicken Rad51 and human Rad51 proteins derived from the transgene. Lanes: 1, wild-type (WT) DT40; 2, RAD51B^/ cells; 3, hRad51-expressing RAD51B^/ cells.

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TABLE 3. Ionizing radiation-induced chromosomal aberrations per 100 mitotic cells^a

In yeast, the overexpression of Rad51 partially suppresses the $gamma$ -ray sensitivity of rad55 and rad57 mutant strains (25,27). Therefore, we overexpressed human Rad51 in RAD51B^/ cells and examined various phenotypes. Remarkably, although theexpression level of the human Rad51 transgene was comparable tothat of endogenous chicken Rad51 (Fig. 6D), the sensitivity ofthe RAD51B^/ cells to $gamma$ rays and MMC was restored to near wild-type levels(Fig. 6A and B). Similarly, human Rad51 expression partially suppressedcisplatin sensitivity (Fig. 6C). Interestingly, expression ofhuman Rad51 ameliorated the chromosomal aberrations (Table 1)and cell death in the mutant (data not shown) but the defect ingene targeting efficiency was not suppressed (Table 2).

To further investigate the role of Rad51B in recombinational repair, we analyzed chromosomal aberrations following genotoxictreatments (Table 3). RAD51B^/ cells exhibited higher levels of chromosomal aberrations thanwild-type cells after ionizing radiation, as did RAD54^/ cells (58). Thus, the HRR pathway(s) involving Rad51B and Rad54plays an important role in repairing radiation-inducedDSBs.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Requirement for Rad51B in HRR and Rad51 focus formation. Our data show that Rad51B is involved in recombinational repair of diverse types of DNA lesions, including spontaneous DSBsthat produce chromosome aberrations. Three types of recombinationalprocesses were impaired by Rad51B deficiency: intrachromosomalgene conversion, gene targeting, and SCE. The involvement of twoother Rad51 paralogs, XRCC2 and XRCC3, in HRR was suggested bythe increased radiosensitivity of hamster xrcc2/3 mutants (36,62), the absence of Rad51 focus formation in XRCC3-deficientcells (6), and the interaction between XRCC3 and Rad51 (36).More recently, this involvement was demonstrated directly usingassays that detect intrachromosomal HRR (28, 44). By analogy,we predicted that the Rad51B, Rad51C, and Rad51D proteins shouldhave similar roles. Our findings constitute the first direct geneticevidence for a role of the Rad51B protein in HRR in vertebratecells.

The appearance of Rad51 nuclear foci is strongly correlated with active DNA repair and likely reflects Rad51 nucleoproteinfilament formation (6, 16, 21, 33, 46). In keepingwith RAD51B participation in HRR, we have shown that Rad51B isrequired for Rad51 focus formation in response to ionizing radiationor MMC treatment. However, it should be noted that the absenceof Rad51 foci does not necessarily imply the absence of Rad51nucleoprotein filaments. A minimum nucleoprotein filament sizeis necessary for visualization of a focus (46), so presumablysufficient Rad51 might still be assembled to repair some spontaneousDNA lesions without producing obviousfoci.

Role of Rad51B in HRR and gene targeting. Protein-protein interactions between Rad51 and Rad55 and between Rad55 and Rad57 suggest that these molecules act in multiproteincomplexes (25, 27, 57). The repair defects of rad55/57 mutantsare partially suppressed by the overexpression of RAD51 but notvice versa (25, 27). Also, biochemical analysis suggests thatthe Rad55/57 heterodimer acts as a cofactor to promote Rad51-single-strandedDNA nucleoprotein filament assembly in the presence of replicationprotein A (57). While direct physical interaction of Rad51Bwith human Rad51 has not been detected, Rad51B could still cooperatewith human Rad51, through its association with Rad51C and XRCC3(18), to form nucleoprotein filaments. This idea is consistentwith the defective Rad51 focus formation in RAD51B^/ cells. A similar situation applies in yeast, where mutationsin RAD55 and RAD57 prevent the appearance of Rad51 foci duringmeiosis (20). These observations suggest that the Rad51 paralogseither help assemble Rad51 into oligomeric complexes or stabilizethe complexes once formed. Likewise, in vertebrates, Rad51B maylead to more extensive nucleoprotein filament formation by Rad51and, as a result, more efficient homologysearching.

Although our RAD51B^/ cells expressing human Rad51 were able to cope well with DNA lesions from genotoxic agents, the modestincrease in the level of Rad51 (chicken plus human) expressionin this transformant (Fig. 6D) was insufficient to fully restoregene targeting efficiency in these cells (Table 2). Perhaps targetedintegration requires longer nucleoprotein filaments than can beformed in this transformant. In this case, the repair of damagemay be more efficient than gene targeting because sister chromatidsare in close proximity whereas gene targeting requires a searchfor homology throughout thenucleus.

Role of HRR in removing DNA cross-links. The cross-linking agents cisplatin and MMC form covalent adducts with many biological molecules, but their principal targetis DNA. They form a variety of DNA adducts: intrastrand cross-links,interstrand cross-links, and protein-DNA cross-links (67). Yeastmutants deficient in nucleotide excision repair, HRR, or the postreplicationrepair pathway show increased sensitivity to cisplatin, indicatingthat these repair pathways are involved in removal of the DNAlesions it causes (24). The phenotype of sensitivity to cross-linkingagents, displayed by our Rad51B-deficient cells, shows that sometypes of DNA lesions induced by cross-linking agents are repairedby HRR involving Rad51B. Since Rad54-deficient DT40 cells showless MMC sensitivity than Rad51B-deficient cells (Fig. 6) (5),it is possible that Rad54 is required for removal of only a subsetof the damage that is removed by Rad51B. Alternatively, a recentlyidentified relative of Rad54, Rad54B (26), might have a rolethat overlaps that ofRad54.

Chromosome instability and cancer. The occurrence of HRR during the vertebrate mitotic cell cycle is suggested by the appearance of Rad51 foci in S phase (61)and by spontaneous SCE. SCEs are mediated at least partially byHRR (55) and occur at a frequency of about three exchanges percell cycle in mammalian cells. Additionally, the presence of excessivechromosome breaks in RAD51^/ (54) and RAD54^/ (5) chicken cells indicates that HRR plays an essential rolein the repair of potentially lethal chromosomal breaks that likelyoccur during DNA replication (54). Here we show that Rad51Bdeficiency causes elevated frequencies of spontaneous chromosomalaberrations, indicating that Rad51B also plays a major role inthe maintenance of genomic stability. Our cell survival data (Fig.6) suggest that Rad51B acts by promoting Rad51's function. Theproperties of the xrcc2 and xrcc3 hamster mutants (36, 42)suggest that the XRCC2 and XRCC3 proteins have roles similar tothat of Rad51B. These mutants show most of the phenotypes of rad51b,including chromosome instability. RAD51B was recently knockedout in mice, but no cellular phenotype has yet been describedsince embryogenesis was arrested at about day 5 and embryoniccells in culture did not proliferate (52).

Every human genetic disorder that features chromosomal breakage is associated with an increased incidence of cancer (40).Rapidly accumulating evidence suggests that defects in HRR playa significant role in promoting tumorigenesis through genomicinstability. For example, chromosomal translocations involvingRAD51B are frequently observed in uterine leiomyoma (48). Mutationsof RAD54, or its homolog RAD54B, are observed in lymphoma, coloncancer, and breast cancer (26, 39). The breast cancer-linkedBrca2 protein interacts with Rad51 in vivo (16) and is requiredfor the formation of visible Rad51 focus formation (66). SinceRAD51B-deficient cells exhibit elevated chromosomal breakage,it will be of interest to screen tumors for mutations in the RAD51Blocus.

	ACKNOWLEDGMENTS

We thank M. Hashishin, Y. Sato, O. Koga, and M. Hirao for excellent technical assistance and H. Kurumizaka and T. Shibata(Riken, Wako, Japan), S. C. West (Imperial Cancer Research Fund,South Mimms, United Kingdom), and D. Schild (Lawrence BerkeleyNational Laboratory, Berkeley, Calif.) for discussion and criticalreading of themanuscript.

C. M. is the recipient of a JSPS postdoctoral fellowship. The Bayer-Chair Department of Molecular Immunology and Allergy issupported by Bayer Yakuhin, Kyoto, Japan. This work was supportedin part by CREST, JST (Saitama, Japan); a Grant-in-Aid for ScientificResearch on Priority Areas from the Ministry of Education, Scienceand Culture of Japan; and grants from The Mochida Memorial Foundationfor Medical and Pharmaceutical Research and from The Uehara MemorialFoundation. A portion of this work was prepared under the auspicesof the U.S. Department of Energy under contract W-7405-ENG-48(L.H.T.).

	FOOTNOTES

^* Corresponding author. Present address: CREST Research Project, Radiation Genetics, Faculty of Medicine, Kyoto University,Konoe Yoshida, Sakyo-ku, Kyoto 606-8501, Japan. Phone: 81-75-753-4410.Fax: 81-75-753-4419. E-mail: stakeda{at}rg1.rg.med.kyoto-u.ac.jp.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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