Exo1 Roles for Repair of DNA Double-Strand Breaks and Meiotic Crossing Over in Saccharomyces cerevisiae

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Vol. 11, Issue 7, 2221-2233, July 2000

Exo1 Roles for Repair of DNA Double-Strand Breaks and Meiotic Crossing Over in Saccharomyces cerevisiae

Hideo Tsubouchi,^* and Hideyuki Ogawa

Department of Biology, Graduate School of Science, Osaka University, Osaka 560-0043, Japan

Submitted January 4, 2000; Revised April 20, 2000; Accepted April 21, 2000
Monitoring Editor: Thomas D. Fox

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The MRE11, RAD50, and XRS2 genes of Saccharomyces cerevisiae are involved in the repair of DNA double-strand breaks (DSBs)produced by ionizing radiation and by radiomimetic chemicals suchas methyl methanesulfonate (MMS). In these mutants, single-strandDNA degradation in a 5' to 3' direction from DSB ends is reduced.Multiple copies of the EXO1 gene, encoding a 5' to 3' double-strandDNA exonuclease, were found to suppress the high MMS sensitivityof these mutants. The exo1 single mutant shows weak MMS sensitivity.When an exo1 mutation is combined with an mre11 mutation, bothrepair of MMS-induced damage and processing of DSBs are more severelyreduced than in either single mutant, suggesting that Exo1 andMre11 function independently in DSB processing. During meiosis,transcription of the EXO1 gene is highly induced. In meiotic cells,the exo1 mutation reduces the processing of DSBs and the frequencyof crossing over, but not the frequency of gene conversion. Theseresults suggest that Exo1 functions in the processing of DSB endsand in meiotic crossingover.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In mating-type switching and meiotic recombination in budding yeast, the formation of double-strand breaks (DSBs) is the initiatingevent. The DSB ends are subjected to 5' to 3' directed exonucleolyticprocessing to leave 3'-tailed single-strand (ss) DNA (Stahl, 1996).These ssDNA tails can be detected in vivo as intermediates duringmating-type switching (White and Haber, 1990) and during meioticrecombination (Sun et al., 1989, 1991; Cao et al., 1990). Intermediateswith ssDNA tails accumulate if the strand invasion step is blockedby a mutation in the RAD51, -52, -54, -55, or -57 gene duringmating-type switching and also in DMC1 during meiotic recombination(Bishop et al., 1992; Shinohara et al., 1992; Sugawara and Haber,1992; Ogawa et al., 1993; Sugawara et al., 1995). Several of thesegenes, RAD51, -55, -57, and DMC1, encode homologues of the Escherichiacoli RecAprotein.

One candidate for the enzyme involved in the production of 3'-tailed ssDNA is the Mre11/Rad50/Xrs2 protein complex. A lackof any one of these proteins makes cells highly sensitive to DSBs(Game and Mortimer, 1974; Ivanov et al., 1992; Ajimura et al.,1993) and reduces processing of DSB ends produced by the HO endonucleaseduring mating-type switching (Ivanov et al., 1994; Lee et al.,1998; Tsubouchi and Ogawa, 1998). As a consequence, the kineticsof recombinant formation is slow, but the amount of recombinantDNA ultimately formed is the same as in wild type (Ivanov et al.,1994; Tsubouchi and Ogawa, 1998).

The Mre11/Rad50/Xrs2 complex is implicated in several aspects of DNA metabolism, including mitotic recombination, telomeremaintenance, and nonhomologous end joining (Haber, 1998). Recentbiochemical studies show that Mre11 and its mammalian homologueshave double-strand (ds) DNA 3' to 5' exonuclease activity andssDNA endonuclease activity (Furuse et al., 1998; Paull and Gellert,1998; Trujillo et al., 1998; Usui et al., 1998; Moreau et al.,1999; reviewed by Haber, 1998). These activities are not directlyinvolved in the formation of 3'-tailed ssDNA at DSB ends, becausemre11 mutants that lack them still show the wild-type level ofDSB processing in vivo (Moreau et al., 1999).

The Exo1 protein of fission and budding yeasts has been isolated as a 5' to 3' dsDNA exonuclease (Szankasi and Smith, 1995;Fiorentini et al., 1997). This protein is conserved through highereukaryotes and is implicated in recombination and mismatch correctionin vivo (Digilio et al., 1996; Tishkoff et al., 1997, 1998; Qiuet al., 1999). In accord with the mismatch correction function,budding yeast Exo1 interacts with the Msh2 protein (Tishkoff etal., 1997). A homology search of the complete genome of buddingyeast reveals four predicted proteins that share sequence similaritywith Exo1: Rad2, Rad27, Din7, and Yen1 (Mieczkowski et al., 1997;Tishkoff et al., 1997). There could be functional redundancy amongtheseproteins.

Proper segregation of homologous chromosomes at the reductional division of meiosis requires crossing over to establish chiasmata,which physically connect homologues after disassembly of the synaptonemalcomplex. Gene conversion has no significant role in segregation(Roeder, 1997). A mutation in any one of a group of genes (ZIP1,ZIP2, MSH4, MSH5, MLH1, MLH3, and MER3) reduces crossing over(Ross and Roeder, 1994; Sym and Roeder, 1994; Hollingsworth etal., 1995; Hunter and Borts, 1997; Chua and Roeder, 1998; Nakagawaand Ogawa, 1999; Wang et al., 1999). Among these, MSH4, MSH5,MLH1, and MLH3 are homologues of the mismatch repair proteinsof E. coli, suggesting a mechanistic relationship between mismatchrepair and crossing over (Nakagawa et al., 1999).

In this study, we isolated the EXO1 gene as a high-copy suppressor of the methyl methanesulfonate (MMS) sensitivity of mre11mutants. The exo1 mutant itself is moderately sensitive to MMS.The exo1 mre11 double mutant, however, is more sensitive to MMSand shows a greater reduction in DSB processing efficiency duringmating-type switching than either single mutant. During meiosis,the exo1 mutation reduces both DSB processing and crossover frequencyand causes nondisjunction of homologous chromosomes. We suggestthat Exo1, as well as the Mre11 complex, is involved in the processingof DSB ends and that Exo1 is also involved in crossing over topromote the accurate segregation of chromosomes duringmeiosis.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Plasmids

Plasmids were constructed by standard procedures. A 4.4-kilobase (kb) SphI fragment containing EXO1 was cloned into the SphIsite of YEplac195 (Gietz and Sugino, 1988) to make pHT131. AnEcoRI fragment in the EXO1 coding sequence was replaced with a1.1-kb EcoRI fragment containing URA3 from YEp24 to make pHT133or with a 2.2-kb HpaI fragment containing LEU2 from YEp13 to makepHT256. Plasmids pHT133 and pHT254 were used for EXO1 disruptionexperiments. pHT59 is a pUC118-based plasmid carrying a 3.4-kbNsiI-BamHI fragment of XRS2 on which a XbaI-BglII fragment wasreplaced with a 3.8-kb hisGURA3hisG fragment from pNKY51 (Alaniet al., 1987). pHT127 carries a 4.3-kb BamHI fragment containingMRE11 on YEplac195. pNKY291 contains sequences downstream of HIS4.pYtel is based on pBluescriptII SK $-$ and carries a 1.0-kb XhoIfragment of a yeast chromosomal end, which contains 120-base pairtelomere repeats and part of the Y' subtelomeric repeat (a giftfrom F. Ishikawa, Tokyo Institute of Technology, Tokyo, Japan).pYA301 carries a 3.4-kb BamHI-EcoRI fragment that includes theyeast actin gene cloned into the BamHI-EcoRI sites of pBR322 (Gallwitzand Seidel, 1980). pBTM116 (Chien et al., 1991) was used to measureplasmid end joining (Boulton and Jackson, 1996b)

Yeast Strains and Media

Strains used in this study are listed in Table 1. All gene targeting was carried out by the one-step gene disruption method(Rothstein, 1983). KJC010 contains an mre11-1 allele and is MMSsensitive at 34°C (Ajimura et al., 1993). HTY836 was made by replacinga BglII-BglII region of the THR4 coding sequence of the R167 strain(a gift from J.E. Haber, Brandeis University, Waltham, MA) witha hisGlacZ insertion. HTY525, -1076, -1104, -1106, -1214, -1215,-1330, and -1336 are SK1 derivatives that enter the meiotic cellcycle in a highly synchronous manner (Fast, 1973). HTY1212, -1213,-1326, -1328, -1434, -1436, -1442, and -1444 are congenic to SK1.HTY1212, -1213, -1214, and -1215 are identical to a pair of haploidsconsisting of MY257 and a pair of haploids consisting of MY261,respectively (Sym and Roeder, 1994), and are gifts from G.S. Roeder(Yale University, New Haven, CT). The EXO1 gene was disruptedby transforming strains with pHT133 or pHT256 after SphI digestion.The XRS2 gene was disrupted by transforming strains with pHT59after SphI and BamHI double digestion. Disruption of MRE11, RAD50,RAD52, and DMC1 was carried out as described previously (Alaniet al., 1989; Bishop et al., 1992; Johzuka and Ogawa, 1995; Tsubouchiand Ogawa, 1998).

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Table 1. Strains used

All media used in this study were detailed previously (Tsubouchi and Ogawa, 1998). YPLac contains 1% yeast extract, 2% bactopeptone, and 2% sodium lactate (pH 5.5), and YPGal is identicalexcept that it contains 2% galactose instead oflactate.

Isolation of High-Copy Suppressors for MMS Sensitivity of mre11

KJC010 was transformed with a yeast genomic library constructed in YEp24 (Botstein et al., 1979), plated on SD-URA (syntheticcomplete medium lacking uracil) plates, and incubated at 34°Cfor 3 d. Transformants were replica-plated onto YPD plates containing0.01% MMS and incubated for 3 d at 34°C. MMS-resistant Ura+ cloneswere streaked on 5-FOA plates to isolate plasmid segregants, andMMS sensitivity of mre11-1 strains with and without the suppressorcandidate plasmids was compared. The plasmids that make the mre11-1strain resistant to MMS were isolated and sequenced from bothsides of the insert fragment. The primers used are Pri 1 (cagtcctgctcgcttcgc)and Pri 2(atgtcggcgatataggcg).

Plasmid End-joining Assay

This assay was performed as described previously (Boulton and Jackson, 1996b). In brief, HTY987, -989, and -991 were transformedwith supercoiled, or linear, pBTM116 (Chien et al., 1991) digestedwith BamHI. One hundred nanograms of each DNA was used to transformeach strain. The ratio of Ura+ Trp+ transformants obtained withcut or uncut DNA was determined for each strain. The average valueof two independent assays for each strain isshown.

Detection of Mating-type Switching

Induction of HO break and detection of mating-type switch process by Southern blot analysis have been described (Tsubouchiand Ogawa, 1998). Genomic DNA samples obtained at indicated timeswere cut with StyI (Eco130I), separated on 0.7% agarose gels,and subjected to Southern blot analysis with a 1.0-kb NdeI-HindIIIfragment of pHT46 as aprobe.

Detection of Telomeres

Genomic DNA was isolated from overnight cultures of the strains indicated (see Figure 7), cut with XhoI, separated on 0.7%agarose gels, and subjected to Southern blot analysis with a 1-kbXhoI-BamHI fragment of pYtel as aprobe.

Return-to-Growth Experiment and Meiotic DSB Detection

Synchronous entry of cells into meiosis, return-to-growth experiments, and detection of meiosis-specific DSBs were performedas described previously (Cao et al., 1990; Johzuka and Ogawa,1995). Genomic DNA samples at different times during meiosis werecut with PstI, separated on 0.7% agarose gels, and subjected toSouthern blot analysis with a 1.5-kb PstI-BglII fragment of pNKY291as a probe (Cao et al., 1990).

Detection of the EXO1 Transcript during Meiosis

Total RNA was extracted from meiotically dividing cells of HTY525, a diploid SK1 derivative, as reported previously (Johzukaand Ogawa, 1995), and subjected to Northern blot analysis. Theamounts of RNA loaded to keep the amount of the ACT1 transcriptnearly constant through meiosis are as follows: 10 µg for 0 h,20 µg for 2 and 4 h, 40 µg for 6 h, and 60 µg for 8 and 10 h.As probes, a 0.9-kb EcoRI fragment of pHT130 and a 0.6-kb ClaIfragment of pYA301 were used to detect transcripts of EXO1 andACT1,respectively.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The EXO1 Gene on a Multicopy Plasmid Suppresses the Repair Defect of an mre11 Mutant

In an mre11, rad50, or xrs2 null mutant, the kinetics of recombination during mating-type switching is slow because of inefficientDSB processing. However, the wild-type amount of recombinant isformed eventually, suggesting that there are additional proteinsinvolved in this process. To identify a gene involved in the process,we screened for high-copy suppressors of the high MMS sensitivityof the mre11-1 missense mutant, which shows temperature-dependentMMS sensitivity (Ajimura et al., 1993). The mutant was transformedwith a genomic DNA library constructed in a 2-µm vector, YEp24.From transformants that grew on YPD plates containing 0.01% MMSat 34°C, plasmids were retrieved and DNA sequences from both endsof the inserts were determined. Seventeen clones were found tocontain the MRE11 gene itself, and eight contained the EXO1 gene.The 4.4-kb SphI-SphI fragment containing the EXO1 gene was clonedinto YEplac195, a 2-µm vector, and this plasmid (pHT131) was usedfor furtheranalysis.

To determine if multiple copies of the EXO1 gene can suppress the defect of the mre11 null mutant, the mutant was transformedwith vector alone (YEplac195), a plasmid containing EXO1 (pHT131),or a plasmid containing MRE11 (pHT127). Suppression of MMS sensitivitywas clearly observed for the mutant with a high dosage of theEXO1 gene (Figure 1). Because the phenotypes of mre11, rad50,and xrs2 mutants are indistinguishable (Alani et al., 1990; Ivanovet al., 1992; Johzuka and Ogawa, 1995) and the Mre11 protein formsa complex with the Rad50 and Xrs2 proteins (Johzuka and Ogawa,1995; Usui et al., 1998), the EXO1 gene was tested for its abilityto suppress the MMS sensitivity of rad50 and xrs2 mutants as well.As expected, suppression was observed in these null mutants tothe same extent as in the mre11 mutant (Figure 1). High dosageof EXO1 increased resistance to MMS >1000-fold at 0.005% MMS (Figure2 A). However, EXO1 overexpression did not suppress the repairdefect of the rad52 mutant (Figure 2 A), indicating that the suppressioneffect is specific to the mre11, rad50, and xrs2 mutants.

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Figure 1. Suppression of the MMS sensitivity of the mre11 null mutant by high-copy EXO1. Wild-type (HTY836), mre11 (HTY837), rad50 (HTY838), and xrs2 (HTY839) null mutants containing YEplac195 or YEpEXO1 (pHT131) were streaked on YPD containing 0.005% MMS.

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Figure 2. (A) Quantitative analysis of the suppression efficiency of a high dosage of EXO1. Mutant mre11 (HTY837), rad50 (HTY838), and rad52 (HTY975) strains containing YEplac195, YEpEXO1 (pHT131), or YEpMRE11 (pHT127) were cultured and plated on SD-URA plates containing various concentrations of MMS. Colonies were counted after 5 d at 30°C and normalized to the number of colonies formed in the absence of MMS. (B) MMS sensitivity of the exo1 null mutant. (C) MMS sensitivity of double mutants. (B and C) Wild-type (HTY836), exo1 (HTY1013), mre11 (HTY837), rad50 (HTY838), mre11 exo1 (HTY1015), and rad50 exo1 (HTY1017) were cultured and plated on YPD plates containing various concentrations of MMS. Survival fractions were calculated as in A. Each experiment was performed at least twice for each strain; the results of single representative experiments are shown here.

Mating-type Switching Is Extremely Retarded in the Absence of Both Exo1 and Mre11

To test whether EXO1 is involved in DSB repair, the phenotype of an EXO1 deletion mutant was examined. The mutant is moresensitive to MMS than wild type, particularly in the presenceof >0.0125% MMS (Figure 2B). Furthermore, exo1 mre11 and exo1rad50 double mutants demonstrate more pronounced repair defectsthan the mre11 and rad50 single mutants (Figure 2C). Therefore,the EXO1 gene is involved in a damage repair pathway that is independentof MRE11, RAD50, and XRS2. However, its contribution to repairis not as great as that of MRE11/RAD50/XRS2.

The process of mating-type switching is well characterized and provides a good model system for analyzing the effect of theexo1 mutation on homologous recombination. DSBs were formed atthe MAT locus by the HO endonuclease, whose expression was controlledby a galactose-inducible promoter. When wild-type cells are incubatedin medium containing galactose for 1 h, a 1.8-kb MAT $alpha$ band, whichcontains an HO target site, is reduced in amount and a 0.7-kbfragment corresponding to an HO-cut fragment appears (Figure 3,A, B, F, and G). When cells are shifted to glucose medium for1 h, most of the 0.7-kb HO-cut fragment disappears and a 0.9-kbMATa band, the product of mating-type switching, appears.The 0.7-kb band completely disappears with an additional 1 h ofincubation (Figure 3, B, F, and G). In the exo1 mutant, the kineticsof MAT switching is indistinguishable from that of wild type (Figure3, D, F, and G). In the mre11 mutant, however, the 0.7-kb bandpersists after 3 h in glucose medium, and the appearance of the0.9-kb MATa band is delayed about 2 h (Tsubouchi and Ogawa,1998) (Figure 3, C, F, and G). In the exo1 mre11 double mutant,~10% of the 0.7-kb HO-cut fragment still remains at 9 h, and theappearance of the 0.9-kb MATa band is further delayed comparedwith the mre11 single mutant (Figure 3, E, F, and G). The relativeintensity of HO-cut fragments in the mre11 exo1 double mutantincreases even after shutting off the expression of HO, presumablybecause the remaining HO endonuclease is active while DSB processingis very slow, resulting in further accumulation of HO-cut fragments.These results indicate that recombination is retarded, but stilloccurs, even in the absence of both Exo1 and Mre11.

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Figure 3. Mating-type switching. (A) Physical map of the MAT locus. (B-E) Cells were preincubated in YPLac, then transferred into YPGal for 1 h, to induce a DSB at the Y/Z junction by HO endonuclease. Transcription was then repressed by changing the culture medium to YPD. Cells were harvested at the indicated times, and genomic DNA was extracted and subjected to Southern blot analysis with a probe shown in A. (B) Wild type (HTY1332); (C) mre11 (HTY1333); (D) exo1 (HTY1334); (E) mre11 exo1 (HTY1335). (F and G) Densitometric analyses of HO-cut fragments (F) and recombinant fragments (G) in Southern blot data from B-E. The band intensities of HO-cut fragments (in F) or recombinant fragments (in G) were divided by the combined intensities of bands corresponding to MAT distal, MAT $alpha$ , MATa, and HO cut fragment to obtain the relative intensities.

EXO1 Does Not Suppress the Reduction in Nonhomologous End Joining in mre11

MRE11 is involved in the nonhomologous end joining (NHEJ) pathway as well as the homologous recombination pathway of DSB repair.To test whether EXO1 can suppress the mre11 defect in NHEJ, aplasmid recircularization assay was used (see MATERIALS AND METHODS).The mre11 null mutant containing vector alone (HTY987), a plasmidcarrying EXO1 (HTY989), or a plasmid carrying MRE11 (HTY991) wastransformed with pBTM116 linearized by BamHI or with a supercoiledplasmid control. Because the linearized plasmid must be recircularizedto be propagated, the ratio of the number of transformants obtainedwith the linear plasmid tested relative to the number obtainedwith the supercoiled plasmid reflects the ability of the strainsto repair DSBs. In pBTM116, there is no yeast-derived sequencearound the restriction enzyme cleavage site; therefore, repairoccurs predominantly by NHEJ. The proportion of transformantsrecovered with cut plasmid relative to uncut plasmid in mre11carrying a vector alone is almost identical to that of mre11 carryingmulticopy EXO1 (2.5 and 1.9%, respectively), and both of thesevalues are ~10-fold lower than the value obtained with mre11 carryingthe MRE11 gene (18.8%) (Figure 4). We also tested the recoveryof a plasmid linearized with a restriction enzyme that createsblunt ends; there was no difference in the plasmid recircularizationratio regardless of whether or not mre11 carried multicopy EXO1(our unpublished result). These results indicate that EXO1 doesnot suppress the NHEJ defect of mre11.

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Figure 4. Multicopy EXO1 does not suppress the reduced NHEJ efficiency of mre11. The NHEJ assay is described in MATERIALS AND METHODS.

EXO1 Suppresses Neither Telomere Shortening nor Spore Inviability in mre11

Telomeres become shortened in the mre11, rad50, and xrs2 mutants (Kironmai and Muniyappa, 1997; Boulton and Jackson, 1998;Nugent et al., 1998). Because a high dosage of the EXO1 gene suppressesthe DSB repair defect of the mre11 mutant, we examined the effectsof EXO1 on telomere shortening in mre11. In the exo1 mutant, telomeresare not shortened (Figure 5, lane 3), and shortening is not enhancedin the exo1 mre11 double mutant compared with mre11 alone (Figure5, lane 4). Furthermore, high dosage of the EXO1 gene does notsuppress the telomere shortening of mre11 (Figure 5, lane 6).Thus, unlike Mre11, Exo1 does not appear to be involved in telomeremaintenance.

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Figure 5. Telomere length in mutant strains. Genomic DNAs were extracted, cut with XhoI, and subjected to electrophoresis, followed by Southern blot analysis to detect telomere sequences (see MATERIALS AND METHODS). Lane 1, wild-type (HTY836); lane 2, mre11 (HTY837); lane 3, exo1 (HTY1013); lane 4, mre11 exo1 (HTY1015); lane 5, mre11 with YEplac195 (HTY987); lane 6, mre11 with YEpEXO1 (HTY989); lane 7, mre11 with YEpMRE11 (HTY991).

mre11 produces inviable spores during meiosis. To determine if a high dosage of EXO1 suppresses this defect, spore viabilitywas compared between an mre11 strain carrying multicopy EXO1 anda control mre11 strain carrying vector alone. In both cases, noviable spores were generated (44 tetrads dissected foreach).

Meiotic Phenotypes of the exo1 Mutant

Transcription of EXO1 Is Induced during Meiosis The EXO1 gene of the fission yeast was reported to be induced during meiotic prophase and implicated to have functions inmismatch correction (Szankasi and Smith, 1995). The Exo1 homologueof Drosophila, named Tosca, is also induced during meiosis (Digilioet al., 1996). We tried to determine if transcription of the EXO1gene of budding yeast is induced during meiosis. Cells progressingsynchronously through meiosis were harvested, and total RNA wasextracted and subjected to Northern blot analysis. The amountof RNA loaded at each time point was normalized to the amountof ACT1 mRNA. In the strain used, premeiotic DNA synthesis iscompleted by 4 h, the DSB level reaches a maximum at around 5h, and the fraction of cells that are binucleate is maximal ataround 6 h. EXO1 transcripts are present at a low level duringmitosis but increase drastically between 4 and 6 h after entryinto meiosis, as has been shown before (Chu et al., 1998a,b) (Figure6). The maximum increase of 36-fold is reached by 6 h; by 10 h,transcript levels begin to decline, suggesting its role by meiosisI.

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Figure 6. Meiotic induction of EXO1 transcription. Total RNA from a wild-type diploid (HTY525) was isolated at the indicated times during meiosis, fractionated on formaldehyde agarose gels (0.7%), and subjected to Northern blot analysis. (A) Transcription of the EXO1 and ACT1 genes was monitored with EXO1 (0.9-kb EcoRI fragment from pHT130) and ACT1 (0.6-kb ClaI fragment from pYA301) coding sequences as probes. The ACT1 transcript, which is expressed at a constant level during meiosis, was used as an internal control (McKee and Kleckner, 1997

). (B) Relative intensity of the EXO1 transcript compared with that of ACT1. At each time, the intensities of the EXO1 and ACT1 bands were measured and the amount of EXO1 transcript was divided by the amount of ACT1 transcript.

DSB Processing Is Impaired in the exo1 Mutant Almost all meiotic recombination is initiated by DSBs formed at recombination hot spots (Haber, 1997). The effect of the exo1mutation on meiotic recombination was monitored at one of thesehot spots, the HIS4::LEU2 locus (Cao et al., 1990) (Figure 7A).DSB products appeared at 3 h and reached a maximal level at 5h in both wild type and exo1, but their disappearance was delayedby 1-2 h in exo1 (Figure 7B). Progression through the meioticcell cycle was monitored at the same time. In exo1, the fractionof cells that had passed the first meiotic division reached amaximum at 7 h after entry into meiosis, which is 1 h later thanin wild type (our unpublished result). To understand the effectof the exo1 mutation on DSB processing more clearly, we took advantageof the dmc1 mutant, in which the recombination reaction is blockedat the strand-transfer stage and DSBs with ssDNA tails accumulate(Bishop et al., 1992). In the exo1 dmc1 double mutant, meioticDSBs were formed as in a wild-type time course, but the DNA fragmentappeared more discrete (Figure 7C), indicating a defect in exonucleolyticprocessing to expose ssDNA tails. This reduction in processingwas first evident at 3 h and became more pronounced at later times(Figure 7C).

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Figure 7. Processing of meiotic DSBs is reduced in exo1. (A) Restriction map of the HIS4::LEU2 construct. DSBs are formed at sites I and II. Fragments diagnostic of DSBs at sites I and II and the unbroken parental fragment (parental) are shown. (B) Detection of meiotic DSBs in wild type (HTY525) and exo1 (HTY1076). (C) Detection of meiotic DSBs in dmc1 (HTY1104) and dmc1 exo1 (HTY1106). DNA was extracted from cultures of each strain at the indicated times during meiosis. After digestion with PstI and electrophoresis, DSBs were detected by Southern blot analysis with an appropriate probe (1.5-kb PstI-EcoRI band from pNKY291).

The exo1 Mutation Reduces Meiotic Crossing Over To examine the effect of the exo1 mutation on recombination, gene conversion frequencies were measured with two sets of heteroalleles,his4X/his4B and arg4-bgl/arg4-nsp (Sherman and Roman, 1963; Espositoand Esposito, 1974). At both of these loci, recombination wasinduced almost to the same extent as in the wild type at 24 hafter entry into meiosis (Table 2). Crossing over was measuredin four intervals (CEN3-HIS4, CAN1-URA3, URA3-HOM3, and HOM3-TRP2)by tetrad analysis (Sym and Roeder, 1994). In each interval, mapdistance was reduced 1.5- to 2.0-fold in the exo1 mutant (Table3); this reduction is statistically significant (CEN3-HIS4, p< 0.02; CAN1-URA3, p 0.0001; URA3-HOM3, p 0.0001; HOM3-TRP2,p < 0.004).

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Table 2. Gene conversion

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Table 3. Crossing over

There is a modest but significant reduction of spore viability in the exo1 mutant (84%, 216 tetrads dissected, p

0.0001),as reported previously (Fiorentini et al., 1997

). Furthermore,the number of viable spores per ascus is not random: fractionsof asci that contain zero, two, or four viable spores per ascus(7, 12, and 74%, respectively) are more frequent than asci containingone or three viable spores per ascus (2 and 4%, respectively)(Figure 8). This suggests that a large fraction of the nondisjunctionevents is due to pairs of homologues segregating to the same poleat the first meiotic division. To examine the segregation of homologouschromosomes directly, a diploid strain was used in which the centromereon one chromosome III was marked with TRP1 and the other withURA3 (Sym and Roeder, 1994

). In a cross between CENIII-TRP1 andCENIII-URA3 strains, spores that are disomic for chromosome IIIresult from nondisjunction at the first meiotic division and canbe identified as both Ura+ and Trp+. Among 63 two-spore-viabletetrads, 8 resulted from nondisjunction of chromosome III. Amongthem, no recombinant was found in CEN3-HIS4. In 45 of the remaining55 tetrads containing two viable spores, the two spores were sisters(i.e., both spores were Ura+ or Trp+), suggesting that they resultedfrom meiosis nondisjunction of another pair of chromosomes. Theseresults indicate that crossing over is reduced and nondisjunctionis increased in exo1.

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Figure 8. Distribution of tetrad types. The distribution of 216 asci with four (4+), three (3+), two (2+), one (1+), or no (0+) viable spores is shown for the wild type (HTY525) and the exo1 strain (HTY1076).

It was shown previously that the meiosis-specific mismatch repair homologues MSH4 and MSH5 are involved in meiotic crossingover (Ross and Roeder, 1994

; Hollingsworth et al., 1995

). Thesetwo gene products form a complex and act in the same pathway.In the msh4 mutant, crossing over is less than (in CAN1-HOM3,p

0.0001) or similar to (in HOM3-TRP2, the difference of thetwo values at this interval is statistically insignificant [p> 0.4]) that in the exo1 mutant (Table 3). To understand therelationship between the MSH4-dependent pathway and EXO1, a msh4exo1 double mutant was constructed and crossing over was measuredin the CAN1-HOM3 and HOM3-TRP2 intervals. The reduction of crossingover in msh4 was not much affected by the additional exo1 mutation(Table 3) (the differences of genetic distances in each intervalare statistically insignificant [p > 0.5 and p > 0.9, respectively]).Unexpectedly, however, spore viability in msh4 exo1 (28%, 870tetrads dissected) is lower than that in msh4 (43%, 570 tetradsdissected). The difference is statistically significant (p < 0.0001)

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Exo1 and Mre11 Are Involved in DSB Processing

We isolated the EXO1 gene as a high-copy suppressor of the MMS sensitivity of the mre11-1 mutant. The EXO1 gene also suppressesthe MMS sensitivity of the mre11, rad50, and xrs2 null mutantsbut not the rad52 mutant. These results suggest that the functionof Exo1 can compensate for the defect of the mre11, rad50, andxrs2 mutants in MMS-induced DNA damage repair. The exo1 mutantshows moderate MMS sensitivity, and in combination with the mre11mutation, MMS sensitivity is more pronounced. These results suggestthat Exo1 and the Mre11/Rad50/Xrs2 complex act independently inMMS-induced DNA damagerepair.

MMS, a radiomimetic agent, is assumed to cause DSBs, and the MMS sensitivity of the mre11 mutant is attributed to its inabilityto repair DSBs (Tavassoli et al., 1995; Bressan et al., 1998).DSBs are predominantly repaired by homologous recombination inyeast (Friedberg et al., 1995), and the process of mating-typeswitching serves as a model system for analyzing the recombinationprocess (Haber, 1995). In this system, the mre11 and rad50 nullmutations reduce 5' to 3' exonucleolytic processing from DSB ends,which delays the formation of mature recombinants (Sugawara andHaber, 1992; Lee et al., 1998; Tsubouchi and Ogawa, 1998). AlthoughDSB processing at the MAT locus appears normal in the exo1 mutant,processing in the exo1 mre11 double mutant is delayed comparedwith that in the mre11 singlemutant.

Because EXO1 encodes a dsDNA 5' to 3' exonuclease (Fiorentini et al., 1997; Tishkoff et al., 1997), promotion of ssDNA formationat DSB ends by EXO1 overexpression could explain the suppressionof the repair defect of mre11. Although MRE11 is involved in theNHEJ pathway as well, EXO1 overproduction does not suppress thereduction of NHEJ, suggesting that EXO1 suppression is independentof the NHEJpathway.

These results argue that Exo1 and Mre11 are involved in DSB processing to create 3'-tailed ssDNA. It is likely that Exo1 isinvolved directly in this process, whereas recent biochemicalstudies have demonstrated that Mre11 (and human Mre11 complex,consisting of hMre11, hRad50, and p95) displays 3' to 5' dsDNAexonuclease activity as well as ssDNA endonuclease activity invitro, and that these activities are not important for the creationof 3'-tailed ssDNA in vivo (Furuse et al., 1998; Paull and Gellert,1998; Trujillo et al., 1998; Usui et al., 1998; Moreau et al.,1999). Thus, it is not likely that Mre11 plays a major role inDSB processing as a nuclease. A second possibility is that therole of the Mre11 complex in DSB processing is to facilitate ssDNAformation indirectly, e.g., the complex may recruit other enzyme(s)and help them to process DSBends.

DSB Processing and DSB Repair

We have observed a correlation between MMS sensitivity and the efficiency of DSB processing during mating-type switching:no reduction in DSB processing and moderate MMS sensitivity inexo1; reduced processing and more severe MMS sensitivity in mre11;and even greater reduction in processing and sensitivity to MMSin the mre11 exo1 double mutant. The fact that the exo1 mutationdoes not affect mating-type switching, although the mutant isslightly sensitive to MMS, might be due to a difference in thenumber of DSBs induced. In mating-type switching, only one DSBis created per cell, whereas multiple DSBs are produced at highdoses ofMMS.

Functional Redundancy in DSB Processing

Although delayed, recombination still occurs in the absence of both Mre11 and Exo1, suggesting the existence of other protein(s)with exonuclease activity. There are four genes (RAD2, RAD27,DIN7, and YEN1) that encode putative proteins sharing homologywith Exo1. DIN7 was recently shown to function specifically inmitochondria (Fikus et al., 2000), so it is unlikely that DIN7and EXO1 function redundantly. In particular, RAD27 may sharecommon functions with EXO1, because exo1 rad27 double mutantsexhibit a synthetic lethal phenotype, and the EXO1 gene is a high-copysuppressor of the temperature-sensitive and mutator phenotypesof a rad27 mutant (Tishkoff et al., 1997). There may be otherenzymes with exonuclease activity invivo.

Mre11 and Regulation of Telomere Length

Although MRE11/RAD50 are implicated in the telomerase-mediated pathway for telomere replication, it remains unclear how theyfunction (Haber, 1998; Nugent et al., 1998). We have confirmedthat telomere shortening occurs in the mre11 null mutant, as expectedfrom the earlier report for the rad50 mutant (Kironmai and Muniyappa,1997; Boulton and Jackson, 1998; Nugent et al., 1998). The exo1null mutation, however, does not affect the telomere length, andhigh copies of the EXO1 gene do not affect the telomere shorteningseen in the mre11 null mutant. Therefore, the reduction in DSBprocessing observed in the mre11 mutant is not likely to be relatedto telomere shortening. Mutations in yeast Ku homologues abolishNHEJ and reduce telomere length (Boulton and Jackson, 1996a,b,1998; Milne et al., 1996; Porter et al., 1996). Both yeast Kuhomologues and MRE11, RAD50, and XRS2 are implicated in the samepathway of NHEJ (Milne et al., 1996; Boulton and Jackson, 1998);therefore, the NHEJ activity of the Mre11 complex could contributeto telomere maintenance. This is consistent with our finding thathigh-copy EXO1 does not suppress the NHEJ defect of the mre11mutant.

Exo1 and Crossing Over during Meiosis

In the present investigation, we observed increased fractions of tetrads exhibiting zero, two, and four viable spores in exo1mutants, reminiscent of conditions that cause defects in meiosisI. Crossing over is reduced to ~50% of the wild-type level andincreased levels of chromosome nondisjunction are observed, suggestingthat Exo1 is important for homologous chromosome segregation byensuring crossing over. Consistent with this view, none of theeight chromosome III disomes was recombinant. In the absence ofMlh1, Mlh3, Msh4, Msh5, Zip1, Zip2, and Mer3, crossing over isreduced twofold to threefold during meiosis, leading to abnormalreductional division (Ross and Roeder, 1994; Sym and Roeder, 1994;Hollingsworth et al., 1995; Hunter and Borts, 1997; Chua and Roeder,1998; Nakagawa and Ogawa, 1999; Wang et al., 1999). Mlh1, Mlh3,Msh4, and Msh5 are homologues of mismatch repair proteins, andboth Mlh1 and Mlh3, like Exo1, are also required for mismatchcorrection; thus, a close mechanistic correlation between mismatchrepair and crossing over is suggested. Our genetic data show thatcrossing over in the exo1 msh4 double mutant is no more reducedthan in msh4, arguing that Exo1 and Msh4 work in a common pathway.There is a strong interaction between EXO1 and MSH2; MSH2 encodesa homologue of the MutS protein of E. coli and plays a centralpart in recognition of mismatch base pairing (Tishkoff et al.,1997), but it does not play a role in crossing over (Hunter andBorts, 1997). Exo1 physically interacts with Msh2, and EXO1 actsin the MSH2-dependent mismatch repair pathway. Because Msh2 andMsh4 are two homologues of the bacterial MutS protein, Exo1 functionin mismatch repair may be mechanistically related to its rolein crossingover.

Although the rate of meiotic crossing over in msh4 is not affected by the exo1 mutation, fewer spores are viable in the exo1msh4 double mutant than in the msh4 single mutant, suggestingthat Exo1 and Msh4 have additional roles during meiosis otherthan crossing over. Crossing over interference is severely reducedin msh4 strains, and the distribution of crossing over among chromosomesis random (Roeder, 1997). The greater spore viability of exo1strains, despite a similar reduction in crossing over, suggeststhat interference is unaffected by the exo1 mutation. On the otherhand, we have observed a reduction in the processing of meiosisDSBs in exo1. The greater reduction in spore viability in msh4exo1 strains, compared with the corresponding single mutants,might be due to the combination of a defect in interference anda failure to repair someDSBs.

	ACKNOWLEDGMENTS

We thank G.S. Roeder, L. Symington, J.E. Haber, and A. Shinohara for helpful discussions and critical reading of the manuscript,T. Tsubouchi for helpful discussions, R. Nobuki for technicalassistance, and other members of the Ogawa laboratory for theirstimulating comments. We also are indebted to J.E. Haber, F. Ishikawa,G.S. Roeder, and N. Kleckner for providing yeast strains and plasmids.This work was supported by Grants-in-Aid for Specially PromotedResearch from the Ministry of Education, Science, Sports, andCulture of Japan, by the Howard Hughes Medical Institute, andby CREST of JST (Japan Science andTechnology).

	FOOTNOTES

^* Present addresses: Department of Biology, Yale University, P.O. Box 208103, New Haven, CT 06520-8103;

Iwate College of Nursing, 14-1 Sengakubo, Ohgama, Takizawa, Iwate 020-0151,Japan.

Corresponding author. E-mail address: hogawa{at}iwate-nurse.ac.jp.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ajimura, M., Leem, S.H., and Ogawa, H. (1993). Identification of new genes required for meiotic recombination in Saccharomyces cerevisiae. Genetics 133, 51-66[Abstract].
Alani, E., Cao, L., and Kleckner, N. (1987). A method for gene disruption that allows repeated use of URA3 selection in the construction of multiply disrupted yeast strains. Genetics 116, 541-545[Abstract/Free Full Text].
Alani, E., Padmore, R., and Kleckner, N. (1990). Analysis of wild-type and rad50 mutants of yeast suggests an intimate relationship between meiotic chromosome synapsis and recombination. Cell 61, 419-436[Medline].
Alani, E., Subbiah, S., and Kleckner, N. (1989). The yeast RAD50 gene encodes a predicted 153-kD protein containing a purine nucleotide-binding domain and two large heptad-repeat regions. Genetics 122, 47-57[Abstract/Free Full Text].
Bishop, D.K., Park, D., Xu, L., and Kleckner, N. (1992). DMC1: a meiosis-specific yeast homolog of E. coli recA required for recombination, synaptonemal complex formation, and cell cycle progression. Cell 69, 439-456[Medline].
Botstein, D., Falco, S.C., Stewart, S.E., Brennan, M., Scherer, S., Stinchomb, D.T., Struhl, K., and Davis, R.W. (1979). Sterile host yeasts (SHY): a eukaryotic system of biological containment for recombinant DNA experiments. Gene 8, 17-24[Medline].
Boulton, S.J., and Jackson, S.P. (1996a). Identification of a Saccharomyces cerevisiae Ku80 homologue: roles in DNA double strand break rejoining and in telomeric maintenance. Nucleic Acids Res. 24, 4639-4648[Abstract/Free Full Text].
Boulton, S.J., and Jackson, S.P. (1996b). Saccharomyces cerevisiae Ku70 potentiates illegitimate DNA double-strand break repair and serves as a barrier to error-prone DNA repair pathways. EMBO J. 15, 5093-5103[Medline].
Boulton, S.J., and Jackson, S.P. (1998). Components of the Ku-dependent non-homologous end-joining pathway are involved in telomeric length maintenance and telomeric silencing. EMBO J. 17, 1819-1828[Medline].
Bressan, D.A., Olivares, H.A., Nelms, B.E., and Petrini, J.H. (1998). Alteration of N-terminal phosphoesterase signature motifs inactivates Saccharomyces cerevisiae mre11. Genetics 150, 591-600[Abstract/Free Full Text].
Cao, L., Alani, E., and Kleckner, N. (1990). A pathway for generation and processing of double-strand breaks during meiotic recombination in S. cerevisiae. Cell 61, 1089-1101[Medline].
Chien, C.T., Bartel, P.L., Sternglanz, R., and Fields, S. (1991). The two-hybrid system: a method to identify and clone genes for proteins that interact with a protein of interest. Proc. Natl. Acad. Sci. USA 88, 9578-9582[Abstract/Free Full Text].
Chu, S., DeRisi, J., Eisen, M., Mulholland, J., Botstein, D., Brown, P.O., and Herskowitz, I. (1998a). The transcriptional program of sporulation in budding yeast. Science 282, 699-705[Abstract/Free Full Text].
Chu, S., DeRisi, J., Eisen, M., Mulholland, J., Botstein, D., Brown, P.O., and Herskowitz, I. (1998b). The transcriptional program of sporulation in budding yeast. Science 282, 1421 (Errata).
Chua, P.R., and Roeder, G.S. (1998). Zip2, a meiosis-specific protein required for the initiation of chromosome synapsis. Cell 93, 349-359[Medline].
Digilio, F.A., Pannuti, A., Lucchesi, J.C., Furia, M., and Polito, L.C. (1996). Tosca: a Drosophila gene encoding a nuclease specifically expressed in the female germline. Dev. Biol. 178, 90-100[Medline].
Esposito, R.E., and Esposito, M.S. (1974). Genetic recombination and commitment to meiosis in Saccharomyces. Proc. Natl. Acad. Sci. USA 71, 3172-3176[Abstract/Free Full Text].
Fast, D. (1973). Sporulation synchrony of Saccharomyces cerevisiae grown in various carbon sources. J. Bacteriol. 116, 925-930[Abstract/Free Full Text].
Fikus, M.U., Mieczkowski, P.A., Koprowski, P., Rytka, J., Sledziewska, G.E., and Ciesla, Z. (2000). The product of the DNA damage-inducible gene of Saccharomyces cerevisiae, DIN7, specifically functions in mitochondria. Genetics 154, 73-81[Abstract/Free Full Text].
Fiorentini, P., Huang, K.N., Tishkoff, D.X., Kolodner, R.D., and Symington, L.S. (1997). Exonuclease I of Saccharomyces cerevisiae functions in mitotic recombination in vivo and in vitro. Mol. Cell. Biol. 17, 2764-2773[Abstract].
Friedberg, E.C., Walker, G.C., and Siede, W. (1995). DNA Repair and Mutagenesis, Washington, DC: American Society of Microbiology Press.
Furuse, M., Nagase, Y., Tsubouchi, H., Murakami, M.K., Shibata, T., and Ohta, K. (1998). Distinct roles of two separable in vitro activities of yeast mre11 in mitotic and meiotic recombination. EMBO J. 17, 6412-6425[Medline].
Gallwitz, D., and Seidel, R. (1980). Molecular cloning of the actin gene from yeast Saccharomyces cerevisiae. Nucleic Acids Res. 8, 1043-1059[Abstract/Free Full Text].
Game, J.C., and Mortimer, R.K. (1974). A genetic study of X-ray sensitive mutants in yeast. Mutat. Res. 24, 281-292[Medline].
Gietz, R.D., and Sugino, A. (1988). New yeast-Escherichia coli shuttle vectors constructed with in vitro mutagenized yeast genes lacking six-base pair restriction sites. Gene 74, 527-534[Medline].
Haber, J.E. (1995). In vivo biochemistry: physical monitoring of recombination induced by site-specific endonucleases. Bioessays 17, 609-620[Medline].
Haber, J.E. (1997). A super new twist on the initiation of meiotic recombination. Cell 89, 163-166[Medline].
Haber, J.E. (1998). The many interfaces of Mre11. Cell 95, 583-586[Medline].
Hollingsworth, N.M., Ponte, L., and Halsey, C. (1995). MSH5, a novel MutS homolog, facilitates meiotic reciprocal recombination between homologs in Saccharomyces cerevisiae but not mismatch repair. Genes Dev. 9, 1728-1739[Abstract/Free Full Text].
Hunter, N., and Borts, R.H. (1997). Mlh1 is unique among mismatch repair proteins in its ability to promote crossing-over during meiosis. Genes Dev. 11, 1573-1582[Abstract/Free Full Text].
Ivanov, E.L., Korolev, V.G., and Fabre, F. (1992). XRS2, a DNA repair gene of Saccharomyces cerevisiae, is needed for meiotic recombination. Genetics 132, 651-664[Abstract].
Ivanov, E.L., Sugawara, N., White, C.I., Fabre, F., and Haber, J.E. (1994). Mutations in XRS2 and RAD50 delay but do not prevent mating-type switching in Saccharomyces cerevisiae. Mol. Cell. Biol. 14, 3414-3425[Abstract/Free Full Text].
Johzuka, K., and Ogawa, H. (1995). Interaction of Mre11 and Rad50: two proteins required for DNA repair and meiosis-specific double-strand break formation in Saccharomyces cerevisiae. Genetics 139, 1521-1532[Abstract].
Kironmai, K.M., and Muniyappa, K. (1997). Alteration of telomeric sequences and senescence caused by mutations in RAD50 of Saccharomyces cerevisiae. Genes Cells 2, 443-455[Abstract].
Lee, S.E., Moor, J.K., Holmes, A., Umezu, K., Kolodner, R.D., and Haber, J.E. (1998). Saccharomyces Ku70, Mre11/Rad50, and RPA proteins regulate adaptation to G2/M arrest after DNA damage. Cell 94, 399-409[Medline].
McKee, A.H., and Kleckner, N. (1997). Mutations in Saccharomyces cerevisiae that block meiotic prophase chromosome metabolism and confer cell cycle arrest at pachytene identify two new meiosis-specific genes SAE1 and SAE3. Genetics 146, 817-834[Abstract].
Mieczkowski, P.A., Fikus, M.U., and Ciesla, Z. (1997). Characterization of a novel DNA damage-inducible gene of Saccharomyces cerevisiae, DIN7, which is a structural homolog of the RAD2 and RAD27 DNA repair genes. Mol. Gen. Genet. 253, 655-665[Medline].
Milne, G.T., Jin, S., Shannon, K.B., and Weaver, D.T. (1996). Mutations in two Ku homologs define a DNA end-joining repair pathway in Saccharomyces cerevisiae. Mol. Cell. Biol. 16, 4189-4198[Abstract].
Moreau, S., Ferguson, J.R., and Symington, L.S. (1999). The nuclease activity of Mre11 is required for meiosis but not for mating type switching, end joining, or telomere maintenance. Mol. Cell. Biol. 19, 556-566[Abstract/Free Full Text].
Nakagawa, T., Datta, A., and Kolodner, R.D. (1999). Multiple functions of MutS- and MutL-related heterocomplexes. Proc. Natl. Acad. Sci. USA 96, 14186-14188[Free Full Text].
Nakagawa, T., and Ogawa, H. (1999). The Saccharomyces cerevisiae MER3 gene, encoding a novel helicase-like protein, is required for crossover control in meiosis. EMBO J. 18, 5714-5723[Medline].
Nugent, C.I., Bosco, G., Ross, L.O., Evans, S.K., Salinger, A.P., Moore, J.K., Haber, J.E., and Lundblad, V. (1998). Telomere maintenance is dependent on activities required for end repair of double-strand breaks. Curr. Biol. 8, 657-660[Medline].
Ogawa, T., Shinohara, A., Nabetani, A., Ikeya, T., Yu, X., Egelman, E.H., and Ogawa, H. (1993). RecA-like recombination proteins in eukaryotes: functions and structures of RAD51 genes. Cold Spring Harbor Symp. Quant. Biol. 58, 567-576[Medline].
Paull, T.T., and Gellert, M. (1998). The 3' to 5' exonuclease activity of Mre 11 facilitates repair of DNA double-strand breaks. Mol. Cell. 1, 969-979[Medline].
Porter, S.E., Greenwell, P.W., Ritchie, K.B., and Petes, T.D. (1996). The DNA-binding protein Hdf1p (a putative Ku homologue) is required for maintaining normal telomere length in Saccharomyces cerevisiae. Nucleic Acids Res. 24, 582-585[Abstract/Free Full Text].
Qiu, J., Qian, Y., Chen, V., Guan, M.X., and Shen, B. (1999). Human exonuclease 1 functionally complements its yeast homologues in DNA recombination, RNA primer removal, and mutation avoidance. J. Biol. Chem. 274, 17893-17900[Abstract/Free Full Text].
Roeder, G.S. (1997). Meiotic chromosomes: it takes two to tango. Genes Dev. 11, 2600-2621[Free Full Text].
Ross, M.P., and Roeder, G.S. (1994). Mutation of a meiosis-specific MutS homolog decreases crossing over but not mismatch correction. Cell 79, 1069-1080[Medline].
Rothstein, R.J. (1983). One-step gene disruption in yeast. Methods Enzymol. 101, 202-211[Medline].
Sherman, F., and Roman, H. (1963). Evidence for two types of allelic recombination in yeast. Genetics 48, 255-261[Free Full Text].
Shinohara, A., Ogawa, H., and Ogawa, T. (1992). Rad51 protein involved in repair and recombination in S. cerevisiae is a RecA-like protein. Cell 69, 457-470[Medline].
Stahl, F. (1996). Meiotic recombination in yeast: coronation of the double-strand-break repair model. Cell 87, 965-968[Medline].
Sugawara, N., and Haber, J.E. (1992). Characterization of double-strand break-induced recombination: homology requirements and single-stranded DNA formation. Mol. Cell. Biol. 12, 563-575[Abstract/Free Full Text].
Sugawara, N., Ivanov, E.L., Fishman, L.J., Ray, B.L., Wu, X., and Haber, J.E. (1995). DNA structure-dependent requirements for yeast RAD genes in gene conversion. Nature 373, 84-86[Medline].
Sun, H., Treco, D., Schultes, N.P., and Szostak, J.W. (1989). Double-strand breaks at an initiation site for meiotic gene conversion. Nature 338, 87-90[Medline].
Sun, H., Treco, D., and Szostak, J.W. (1991). Extensive 3'-overhanging, single-stranded DNA associated with the meiosis-specific double-strand breaks at the ARG4 recombination initiation site. Cell 64, 1155-1161[Medline].
Sym, M., and Roeder, G.S. (1994). Crossover interference is abolished in the absence of a synaptonemal complex protein. Cell 79, 283-292[Medline].
Szankasi, P., and Smith, G.R. (1995). A role for exonuclease I from S. pombe in mutation avoidance and mismatch correction. Science 267, 1166-1169[Abstract/Free Full Text].
Tavassoli, M., Shayeghi, M., Nasim, A., and Watts, F.Z. (1995). Cloning and characterization of the Schizosaccharomyces pombe rad32 gene: a gene required for repair of double strand breaks and recombination. Nucleic Acids Res. 23, 383-388[Abstract/Free Full Text].
Tishkoff, D.X., Amin, N.S., Viars, C.S., Arden, K.C., and Kolodner, R.D. (1998). Identification of a human gene encoding a homologue of Saccharomyces cerevisiae EXO1, an exonuclease implicated in mismatch repair and recombination. Cancer Res. 58, 5027-5031[Abstract/Free Full Text].
Tishkoff, D.X., Boerger, A.L., Bertrand, P., Filosi, N., Gaida, G.M., Kane, M.F., and Kolodner, R.D. (1997). Identification and characterization of Saccharomyces cerevisiae EXO1, a gene encoding an exonuclease that interacts with MSH2. Proc. Natl. Acad. Sci. USA 94, 7487-7492[Abstract/Free Full Text].
Trujillo, K.M., Yuan, S.S., Lee, E.Y., and Sung, P. (1998). Nuclease activities in a complex of human recombination and DNA repair factors Rad50, Mre11, and p95. J. Biol. Chem. 273, 21447-21450[Abstract/Free Full Text].
Tsubouchi, H., and Ogawa, H. (1998). A novel mre11 mutation impairs processing of double-strand breaks of DNA during both mitosis and meiosis. Mol. Cell. Biol. 18, 260-268[Abstract/Free Full Text].
Usui, T., Ohta, T., Oshiumi, H., Tomizawa, J., Ogawa, H., and Ogawa, T. (1998). Complex formation and functional versatility of Mre11 of budding yeast in recombination. Cell 95, 705-716[Medline].
Wang, T.F., Kleckner, N., and Hunter, N. (1999). Functional specificity of MutL homologs in yeast: evidence for three Mlh1-based heterocomplexes with distinct roles during meiosis in recombination and mismatch correction. Proc. Natl. Acad. Sci. USA 96, 13914-13919[Abstract/Free Full Text].
White, C.I., and Haber, J.E. (1990). Intermediates of recombination during mating type switching in Saccharomyces cerevisiae. EMBO J. 9, 663-673[Medline].

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