Cdc2-cyclin B kinase activity links Crb2 and Rqh1-topoisomerase III

doi:10.1101/gad.221402

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Vol. 16, No. 10, pp. 1195-1208, May 15, 2002

RESEARCH PAPER
Cdc2-cyclin B kinase activity links Crb2 and Rqh1-topoisomerase III

Thomas Caspari,¹ Johanne M. Murray, and Antony M. Carr²

Genome Damage and Stability Centre, University of Sussex, Brighton BN1 9RQ, UK

ABSTRACT

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

The availability of a sister chromatid, and thus the cell cycle phase in which DNA double-strand breaks (DSBs) occur, influencesthe choice between homologous recombination (HR) or nonhomologousend joining (NHEJ). The sequential activation and destructionof CDK-cyclin activities controls progression through the cellcycle. Here we provide evidence that the major Schizosaccharomycespombe CDK, Cdc2-cyclin B, influences recombinational repair ofradiation-induced DSBs during the G₂ phase at two distinct stages.At an early stage in HR, a defect in Cdc2 kinase activity, whichis caused by a single amino acid change in cyclin B, affects theformation of Rhp51 (Rad51^sp) foci in response to ionizing radiation in a process that isredundant with the function of Rad50. At a late stage in HR, lowCdc2-cyclin B activity prevents the proper regulation of topoisomeraseIII (Top3) function, disrupting a recombination step that occursafter the assembly of Rhp51 foci. This effect of Cdc2-cyclin Bkinase on Top3 function is mediated by the BRCT-domain-containingcheckpoint protein Crb2, thus linking checkpoint proteins directlywith recombinational repair in G₂. Our data suggest a model inwhich CDK activity links processing of recombination intermediatesto cell cycle progression via checkpoint proteins.

[Key Words: Homologous recombination; cdc2; cyclin B; Rqh1; Top3; Crb2; checkpoint]

	Introduction

Top Abstract Introduction Results Discussion Materials and methods References

DNA double-strand breaks (DSBs) pose a considerable threat to genomic integrity and cell survival. If not repaired, a singleDSB can result in cell death (Rudin and Haber 1988). DSBs ariseboth spontaneously, for example, during DNA replication, and inresponse to exogenous agents such as ionizing radiation (IR).The two major DSB repair pathways in eukaryotic cells are nonhomologousend joining (NHEJ) and homologous recombination (HR). NHEJ resultsin the ligation of broken DNA ends irrespective of their sequenceinformation. This process is potentially error-prone and can resultin loss of genetic information. In contrast, HR uses the geneticinformation stored in the sister chromatid (or potentially thehomologous chromosome) to repair DSBs with highfidelity.

Genetic studies in Saccharomyces cerevisiae have established that HR is performed by the products of the RAD52 epistasis groupof genes (Paques and Haber 1999). Once a DSB is formed, the endsare resected by a 5'-3' exonuclease in a manner partially dependenton the Rad50-Mre11-Xrs2 protein complex (Ivanov et al. 1994).This results in 3'-ended single-strand DNA (ssDNA) tails, whichare channeled into different homology-dependent recombinationpathways. In a minor pathway, 3' tails can undergo intrachromosomalsingle-strand annealing (SSA) (Ivanov et al. 1996), which resultsin the deletion of the intervening sequence. The major pathway,however, is invasion of a homologous DNA region on a sister chromatidor on a homologous chromosome by the 3' tails. Invasion by oneof the two ssDNA tails generates a unidirectional replicationfork, which can migrate down the template chromosome, copyingthe genetic information, a process termed DNA-break induced replication(BIR) (Kraus et al. 2001). Invasion by both ssDNA tails resultsin the formation of a double Holliday Junction (HJ), which, whenresolved, results in gene conversion with or without a crossoverevent. SSA, BIR, and gene conversion are all dependent on Rad52,but only the latter pathway requires assembly of the Rad51 nucleoproteinfilament, which promotes homologous pairing and strand exchange(Paques and Haber 1999).

The availability of the sister chromatid, and therefore the cell cycle phase in which the DSB occurs, determines the choiceof the appropriate repair pathway. The molecular mechanisms underlyingthis channeling event are unknown. In G₁, DSBs are rejoined byNHEJ, SSA, or BIR (in a diploid), whereas after DNA replication,the sister chromatid serves as an information donor for HR. Thecell cycle is controlled by the sequential action of CDK-cyclincomplexes, and it would thus be logical if these were also toinfluence the channeling of DSBs into different repair pathways.However, evidence for such a function has not been reported. Thereare several ways in which CDKs could channel DSBs into specificrepair pathways. For example, CDKs could regulate the expressionof key repair enzymes, thereby influencing the choice betweenHR and NHEJ. It has been proposed that Rad52 competes with proteinsof the NHEJ pathway for binding to DSBs (Van Dyck et al. 1999).The increased expression of Rad52 in late S phase and in G₂ (whenHR is at its highest level) in human cells might thus affect thebalance of repair events (Chen et al. 1997). Alternatively, CDKscould directly phosphorylate proteins involved in the responseto DNA damage. CDK-dependent phosphorylation has been reportedfor several proteins involved in the DSB response, including single-strandbinding protein (RPA) (Dutta and Stillman 1992; Niu et al. 1997),DNA ligase I (Aoufouchi et al. 1995), Srs2 DNA helicase (Liberiet al. 2000), the tumor suppressor protein BRCA1 (Ruffner et al.1999), and the Schizosaccharomyces pombe checkpoint protein Crb2(Esashi and Yanagida 1999).

Crb2 is the S. pombe analog of the canonical S. cerevisiae Rad9 checkpoint protein and contains two C-terminal BRCT motifs(Saka et al. 1997; Wilson et al. 1997). Cdc2-cyclin B kinase hasbeen shown to phosphorylate Crb2 during metaphase, just beforedestruction of cyclin B (Esashi and Yanagida 1999). Later in thecell cycle, this modification is an essential prerequisite forthe checkpoint-dependent hyperphosphorylation of Crb2 by the Rad3protein kinase in response to DNAdamage.

In this work, we provide evidence showing that a functional Cdc2-cyclin B kinase complex is required for successful HR. Apoint mutation in cdc13, encoding the major G₂-cyclin in S. pombe,reduces CDK activity and renders cells sensitive to IR. The increasein sensitivity is not caused by a checkpoint defect, but relatesprimarily to an impaired function of topoisomerase III (Top3).Loss of Top3 activity, which acts downstream of, or in parallelwith, the Rqh1 DNA helicase, permits the use of an alternativeRqh1-dependent mechanism that results in hyperrecombination andcell death following IR. Our data suggest that CDK targets Top3indirectly, via the checkpoint protein Crb2. Although Crb2, Rqh1,and Top3 all act at a late stage in HR after formation of Rhp51(Rad51 homolog) foci, we also find that CDK activity plays a secondrole at an early stage. CDK activity positively regulates a functionthat is required for the assembly of Rhp51 foci in a redundantmanner with Rad50. Our findings show that a functional Cdc2-cyclinB kinase complex is necessary to protect cells from the genotoxicconsequences of IR and suggest a mechanism by which Crb2 actsat the interface between cell cycle regulation, checkpoint function,and DSBrepair.

	Results

Top Abstract Introduction Results Discussion Materials and methods References

A point mutation in cdc13 renders S. pombe cells sensitive to IR

To identify S. pombe proteins involved in the response to DNA damage that are also essential for cell growth, we screeneda collection of temperature-sensitive mutants for sensitivityto a variety of DNA-damaging agents. Under permissive conditions,one mutant (TC-245) was highly sensitive to ionizing radiation(IR), mildly sensitive to UV light, and insensitive to DNA replicationblocks caused by nucleotide depletion (Fig. 1A-C). The mutationmapped to the cdc13 gene (cdc13-245), which encodes the majorG₂-cyclin in S. pombe (Booher and Beach 1988; Hagan et al. 1988).Sequence analysis shows that the phenotype results from a singleamino acid replacement at position 255 (E255R) within the cyclinbox (data not shown). Because loss-of-function mutants in cdc13undergo DNA re-replication (Hayles et al. 1994) , we analyzedthe DNA content of an asynchronous cdc13-245 culture under permissiveconditions. FACS analysis revealed a 2C DNA content identicalto wild-type controls, showing that cdc13-245 cells do not re-replicateunder these conditions and that the IR sensitivity is not a resultof an increase in G₁ cells (data not shown).

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Figure 1. Low Cdc2-cyclin B kinase activity renders S. pombe cells sensitive to IR without affecting the DNA damage checkpoint. (A-C) The sensitivity of cdc13-245 mutant cells to IR, to UV-induced DNA damage, and to S-phase arrests caused by nucleotide depletion. The rad3-d strain is checkpoint-deficient and was used as a control. (D) G₂-synchronized cells were exposed to 0 Gy, 250 Gy, or 500 Gy of IR, and progression through mitosis was analyzed under permissive conditions. A checkpoint-deficient mutant (rad3-d) was used as a negative control (data not shown). (E) An example of a cdc13-245 cell undergoing aberrant mitosis after IR. (F, left panels) Immunoprecipitation. Cdc2 kinase was precipitated from soluble extracts (prepared from untreated cells) using either an anti-Cdc13 antibody or an unrelated control antibody. (B) Before addition of the antibodies, 50 µg of soluble protein; (A) after precipitation, 50 µg of soluble protein; (P) pellet. The asterisk marks a nonspecific band. (Right panel) In vitro kinase assay. The anti-Cdc13 antibody was used to precipitate Cdc2-cyclin B kinase from untreated extracts and from extracts prepared after irradiation with a dose of 500 Gy. The precipitated material was incubated with histone H1 and ATP.

Cdc13 is known to regulate mitotic progression, and it is possible that the sensitivity of cdc13-245 cells is a result ofcheckpoint failure. To investigate this, we irradiated wild-typecells and cdc13-245 cells that had been synchronized in G₂ bylactose gradient centrifugation and analyzed their subsequentcell cycle progression. Like wild-type cells, cdc13-245 cellstransiently arrested entry into mitosis, showing that checkpointfailure is not responsible for the IR sensitivity (Fig. 1D). Interestingly,unlike wild-type cells, ~40% of cdc13-245 cells entered a catastrophicmitosis upon recovery from the G₂/M arrest, as indicated by nuclearabnormalities (Fig. 1E). This mitotic failure, despite normalG₂ delay, is indicative of a defect in DNArepair.

The E255R substitution reduces Cdc2 kinase activity in vivo and in vitro

Under permissive conditions, cdc13-245 cells are slightly more elongated than wild-type cells (data not shown), which is indicativeof a moderate delay over entry into mitosis. Because mitotic entryrequires high Cdc2-Cdc13 kinase activity, this delay suggeststhat the E255R mutation reduces CDK activity in vivo. To characterizethe effect of the E255R substitution under in vitro conditions,we coimmunoprecipitated Cdc2 from soluble wild-type and cdc13-245extracts (prepared under permissive conditions from asynchronouscells) using a polyclonal anti-Cdc13 antibody. The efficient coprecipitationof Cdc2 from cdc13-245 extracts indicates that the E255R substitutiondid not affect the interaction between Cdc2 and Cdc13. However,the loss of histone H1 phosphorylation by Cdc2 in this in vitroassay (Fig. 1F) further suggests that the mutation in cyclin Bimpairs CDKactivity.

The E255R substitution compromises homologous recombination

Given that Rad51 is essential for the repair of DSBs by HR (Muris et al. 1993; Paques and Haber 1999), we constructed a cdc13-245rhp51-d double mutant. The double mutant displayed the same sensitivityas the rhp51-d single mutant (Fig. 2A), suggesting that low CDKactivity affects the Rhp51-dependent DSB repair pathway. However,compared to rhp51-d mutants, which are completely deficient inHR, cdc13-245 cells are significantly less sensitive, especiallyto doses below 200 Gy (Fig. 2A). To verify the epistatic relationshipbetween cdc13-245 and rhp51-d, we repeated our genetic analysisusing UV light. S. pombe cells use two pathways to repair UV damage.Photoproducts are either removed by nucleotide excision repair(NER) or channeled into an Rhp51-dependent pathway after beingremoved by the UVDE enzyme (Murray et al. 1997; McCready et al.2000). The cdc13-245 rhp51-d double mutant showed an identicalUV sensitivity to that of the rhp51-d single mutant (Fig. 2B).In contrast, loss of NER (rad13 deletion) in a cdc13-245 backgroundresulted in a double mutant that was significantly more UV sensitivethan either of the two single mutants (Fig. 2C). These data areconsistent with the involvement of HR in UV repair in fissionyeast (McCready et al. 2000) and confirm the conclusion that lowCDK activity compromises Rhp51-dependent HR.

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Figure 2. The cdc13-245 mutation affects homologous recombination. (A) cdc13-245 does not increase IR sensitivity of an rhp51-d mutant. (B) The cdc13-245 mutant is epistatic with rhp51 in recombinational repair of photoproducts. (C) Loss of NER renders cdc13-245 cells more sensitive to UV-induced DNA damage.

Low CDK activity impairs Rhp51 (Rad51 homolog) foci formation

To map the function of Cdc2-cyclin B within the HR pathway, we combined the cdc13-245 allele with different mutants deficientin recombinational repair. The Rad50-Mre11-Xrs2 protein complexfunctions upstream of Rad51 and links processing of DNA ends withthe availability of the sister chromatid (Hartsuiker et al. 2001).rad50-d cells are more radiation resistant than rhp51-d cells(Hartsuiker et al. 2001), indicating that the early functionsin HR can be performed by redundant pathways. Interestingly, therad50-d cdc13-245 double mutant is more sensitive to IR than therad50-d single mutant (Fig. 3A). This increase implies that lowCDK activity impairs HR at an early stage (such as end processing)in a manner redundant with the Rad50 function.

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Figure 3. The cdc13-245 mutation impairs an end-processing pathway that is redundant with Rad50. (A) The cdc13-245 mutation increases the IR sensitivity of rad50-d cells. (B) Indirect immunofluorescence microscopy of wild-type cells and the indicated mutant strains at 1 h postirradiation (500 Gy). A cross-reacting human anti-Rad51 antibody was used to detect Rhp51. Note that rad54-d cdc13-245 cells are proficient in the formation of Rhp51 foci, but a rad50-d cdc13-245 double mutant is impaired. (C) Mean percentage of various mutant cells showing Rhp51 foci at 1 h postirradiation.

To seek further evidence supporting this hypothesis at the cellular level, we used a cross-reacting anti-human Rad51 antibodyto analyze the formation of Rhp51 foci in irradiated S. pombecells. Human Rad51 accumulates at sites of DNA damage in postreplicativechromatin (Tashiro et al. 2000). Treatment of wild-type S. pombecells with 500 Gy of IR resulted in the assembly of Rhp51 in brightnuclear foci within 1 h postirradiation (Fig. 3B). Irradiationof synchronized cells confirmed that foci formation occurred inG₂ (data not shown; see below). Next, we visualized Rhp51 fociin different mutants to characterize the role of other recombinationproteins. The formation of foci was dependent on the mediatorprotein Rhp55, which is thought to facilitate the formation ofthe Rad51 nucleoprotein filament, whereas it was independent ofthe synaptic factor Rad54, which functions later in HR to permitstrand invasion. Cells deleted for rad50 showed only a moderatereduction in the focal assembly of Rhp51 (Fig. 3B). Although almost100% of wild-type cells possessed Rhp51 foci 1 h postirradiation,only 53% ± 10% of rad50-d cells developed bright foci (Fig. 3C)and 17% ± 8% of rad50-d cells failed to produce any foci. Thediminished ability of rad50-d cells to assemble Rhp51 foci isconsistent with the higher radiation resistance of these cellswhen compared with an rhp51-d strain. Interestingly, in a rad50-dbackground, the ability to produce Rhp51 foci was largely dependenton an intact Cdc2-cyclin B kinase complex. At 1 h postirradiation,only 7% ± 4% of rad50-d cdc13-245 cells assembled bright wild-type-likefoci and 53% ± 5% of cells were without foci (Fig. 3B,C). Westernblot analysis confirmed that all mutants contained similar levelsof Rhp51 protein (data not shown). These data provide evidencethat CDK activity positively controls an early recombination functionthat is redundant with Rad50 and required for IR-induced focalassembly ofRhp51.

Loss of Rqh1 DNA helicase restores IR resistance in a cdc13-245 mutant

Rqh1 is the only RecQ-like DNA helicase in S. pombe (Murray et al. 1997; Stewart et al. 1997). During S phase, Rqh1 is thoughtto act at stalled replication forks during recombination-basedrepair (Murray et al. 1997). The link between Rqh1 and HR promptedus to test whether Rqh1 is also required for the response to IRin G₂ cells. Survival analysis following IR revealed that rqh1-dcells are sensitive to IR and showed that Rqh1 acts in the samepathway as Rhp51 (Fig. 4A). Thus, both Rqh1 and Cdc13 contributeto successful recombinational repair of IR-induced DSBs via anRhp51-dependent pathway. Surprisingly, deletion of rqh1 in a cdc13-245background resulted in a significant restoration of IR resistance(Fig. 4B) compared with either the rqh1-d or cdc13-245 singlemutants.

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Figure 4. Analysis of both Rqh1 foci and Top3 foci. (A) Rqh1 and Rhp51 act in the same recombination repair pathway. (B) Loss of Rqh1 DNA helicase restores IR resistance of a cdc13-245 mutant. Note the mutual rescue, which suggests that the cdc13-245 mutation can also prevent cell death in an rqh1-d background. This rescue could relate to the involvement of Cdc2-Cdc13 in an early recombination step such as end-processing. (C) Deletion of rqh1 in an rad50-d background does not affect assembly of Rhp51 in foci at 1 h postirradiation (500 Gy). (D, left) Kinetic analysis of cell cycle progression either untreated or with a dose of 500 Gy in the second G₂ phase. (Right) Untreated (0 Gy) or irradiated (500 Gy) wild-type G₂ cells from the same experiment. Rqh1 was visualized with an Rqh1-specific antibody. The arrow marks damage-induced Rqh1 foci at 1 h postirradiation. (E, left) DAPI, anti-Rqh1 antibody staining, and merge images showing representative cells irradiated in G₂. Arrows indicate cells with foci. (Right) Single G₂ cells either before ( $-$ IR) or 1 h after irradiation (+IR). In these merged images, chromatin is stained with DAPI (green) and Rqh1 is visualized by the anti-Rqh1 antibody (red). (F) Mean percentage of synchronized G₂ cells showing Rhp51 foci, Rqh1 foci, or MYC-Top3 foci at the indicated periods of time after 500 Gy of IR. (G) Staining of the indicated asynchronous cells with the anti-MYC antibody at 140 min postirradiation (500 Gy). The arrow marks damage-induced MYC-Top3 foci.

This mutual rescue indicates that Cdc2-Cdc13 activity influences at least two distinct stages of HR. Because the cdc13-245mutation suppresses loss of Rqh1, Cdc13 activity appears to controlan early step that channels DNA structures into the Rqh1-dependentpathway. That Cdc13 activity is required for a second step laterin HR becomes evident from the observation that inactivation ofRqh1 restores IR resistance in a cdc13-245 background. This rescuestrongly suggests that Cdc13 activity is necessary to deal withrecombination intermediates that are generated by Rqh1 DNA helicase.The fact that this late function is not blocked by the early defectindicates that the pathway is not linear and that Rqh1 receivesDNA substrates from two parallel pathways, and only one of theseis dependent onCdc13.

This interpretation is consistent with our observation that Cdc13 activity is necessary to allow focal assembly of Rhp51 ina rad50-d background. To test whether Rqh1 shares this early functionwith Cdc13, we analyzed focal assembly of Rhp51 in a rad50-d rqh1-ddouble mutant. Deletion of rqh1 did not affect the appearanceof Rhp51 foci in rad50-d cells 1 h postirradiation (Fig. 4C).This result implies that Rqh1 does not participate in the earlystep, but acts close to the late recombination function. Takentogether, these data indicate that the pathways that provide DNAstructures for Rqh1 are under control of Cdc13 and Rad50, respectively.This suggestion is supported by the observation that deletionof rad50 in a cdc13-245 rqh1-d background (the rqh1-d cdc13-245rad50-d triple mutant) renders cells as IR sensitive as cdc13-245rad50-d double-mutant cells (data notshown).

Impaired CDK activity stabilizes both Rqh1 foci and Top3 foci

The genetic interaction between cdc13-245 and rqh1-d indicates a function for Rqh1 not only during S phase but also in G₂.To test this idea, we irradiated wild-type cells that were synchronizedin G₂ and analyzed the response of Rqh1. Neither protein levelsnor electrophoretic mobility of Rqh1 changed upon IR (data notshown), but, in a proportion of cells, Rqh1 relocalized from apredominantly nucleolar distribution to discrete foci in the chromatincompartment 1 h postirradiation (Fig. 4D,E). This relocalizationoccurred in 5% ± 1% of wild-type cells after 60 min and increasedto 20% ± 2% by 140 min postirradiation. To dissect the relationshipbetween Rhp51 and Rqh1 foci, we monitored the kinetics of Rhp51,Rqh1, and Top3 assembly in nuclear foci upon irradiation of G₂-synchronizedcells (Fig. 4F). We included Top3 in our analysis, because theassociation between RecQ-like DNA helicases and Top3 is highlyconserved (Harmon et al. 1999; Bennett and Wang 2001). The N-terminallyMYC-tagged Top3 protein (L.V. Laursen, A.H. Andersen, and J.M.Murray, unpubl.), which we used in our study, had no obvious phenotypein either wild-type cells or in a cdc13-245 mutantbackground.

At 1 h postirradiation, almost 100% of wild-type cells possessed Rhp51 foci. The percentage of cell with Rhp51 foci declinedsteadily during the G₂/M arrest period and dispersed as cellsre-entered the cell cycle between 180 min and 200 min postirradiation(Fig. 4F; data not shown). In contrast, foci containing eitherRqh1 or MCY-Top3 appeared toward the end of the arrest period,reaching a maximum at ~140 min postirradiation (Fig. 4F). Thislate response to IR is consistent with the idea that both Rqh1and Top3 function at a late stage in HR after formation of Rhp51foci. Moreover, it suggests that both enzymes deal with recombinationintermediates, which appear only in a limited number of cellsshortly before the end of thearrest.

We repeated this analysis using G₂-synchronized cdc13-245 cells and found that the number of cells assembling either Rqh1or MYC-Top3 in nuclear foci upon IR increased significantly comparedwith wild-type cells. At 140 min postirradiation, the percentageof cells possessing Rqh1 foci rose from 20% ± 2% seen in wild-typecells to 48% ± 1%. Similarly, the number of cells showing MYC-Top3foci increased from 5% ± 2% in wild-type cells to 35% ± 2% incdc13-245 cells (Fig. 4F). The protein levels of both Rqh1 andMYC-Top3 did not change during the experiment (data not shown),and the kinetic of Rhp51 foci formation and subsequent dispersalwas not affected by the cdc13-245 mutation.

To test whether the stabilization of these foci relates to our model that Cdc13 activity is required to process recombinationintermediates that are generated by Rqh1, we analyzed formationof Top3 foci in an rqh1-d cdc13-245 background. Loss of Rqh1 preventedthe focal assembly of Top3 in the double mutant (Fig. 4G), showingthat assembly of Top3 foci is dependent on Rqh1 function and thatlow Cdc2-Cdc13 kinase activity stabilizes Top3 foci only whenRqh1 generatesintermediates.

The checkpoint protein Crb2 acts in the same recombination pathway as cyclin B

The checkpoint protein Crb2 becomes phosphorylated at threonine 215 by Cdc2-cyclin B kinase during mid-mitosis. Phosphorylationof T215 is a prerequisite for subsequent Rad3-dependent hyperphosphorylationof Crb2 in response to DNA damage (Esashi and Yanagida 1999).The link between Crb2 and Cdc2-cyclin B prompted us to createthe crb2-T215A allele at the endogenous crb2 locus in both a wild-typebackground and a cdc13-245 background. We observed that crb2-T215Acells are more IR sensitive than cdc13-245 cells and that thedouble crb2-T215A cdc13-245 mutant had the same IR sensitivityas the crb2-T215A single mutant, showing that both proteins actin the same pathway for IR survival (Fig. 5A).

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Figure 5. High levels of Top3 protein restore IR resistance in both the crb2-T215A mutant and the cdc13-245 mutant. (A) The inability to phosphorylate Crb2 at threonine 215 renders cells sensitive to IR. The crb2-T215A mutation is epistatic with the cdc13-245 mutation. (B) Mean percentage of the indicated asynchronous cells showing Rhp51 foci at 1 h postirradiation (500 Gy). (C) Deletion of rqh1 restores IR resistance in a crb2-T215A mutant. Note that, unlike the case seen for the rqh1-d cdc13-245 double mutant, the mutation in crb2 fails to improve survival of rqh1-d cells. This is consistent with the fact that Crb2 is not involved in an early step in recombination. (D) Mean percentage of asynchronous wild-type and crb2-T215A cells showing Rqh1 foci at the indicated periods of time upon 500 Gy of IR. (E) Overexpression of HIS₆-top3 from a pREP1 plasmid restores IR resistance in a crb2-T215A mutant. (F) Overexpression of HIS₆-top3 restores IR resistance of cdc13-245 cells.

Given that the mutation in cdc13 affects two steps in HR, we asked which of these steps might be compromised in the crb2-T215Amutant. For this purpose, we constructed a rad50-d crb2-T215Adouble mutant and an rqh1-d crb2-T215A double mutant. Upon IR,the rad50-d crb2-T215A double mutant assembled Rhp51 foci in amanner that was quite similar to that of the rad50-d single mutant(Fig. 5B), suggesting that the early Cdc13-dependent functionis not affected by the crb2-T215A mutation. Interestingly, deletionof rqh1 suppressed the IR sensitivity of the crb2-T215A mutant,but, unlike in the case of the rqh1-d cdc13-245 double mutant,IR resistance was only restored to a level that is characteristicfor the rqh1-d single mutant (Fig. 5C). This limited increasein IR resistance suggests that Crb2 function is restricted tothe late step in HR that requires Rqh1 activity. Consistent withthis suggestion, we found that the percentage of crb2-T215A cellscontaining Rqh1 foci rose from the wild-type level of 23% ± 3%to 72% ± 8% at 140 min postirradiation (Fig. 5D).

Top3 is an efficient multicopy suppressor of both cdc13-245 and crb2-T215A

During our strain construction, we noticed that MYC-top3 crb2-T215A double-mutant cells are inviable (data not shown). Althoughthe MYC-top3 allele appears fully functional (cell morphologyand damage resistance assays) in other genetic backgrounds, theN-terminal tag appears to impair a function that becomes essentialin crb2-T215A cells. This genetic interaction prompted us to testwhether overexpression of top3 could restore IR resistance incrb2-T215A cells. Indeed, high protein levels of Top3 proved veryefficient in suppressing the sensitivity to IR (Fig. 5E). BecauseCrb2 and cyclin B appear to act in the same pathway, downstreamof Rqh1, we repeated this experiment in cdc13-245 cells and obtaineda similar result (Fig. 5F). This efficient rescue implies thatboth the cdc13-245 and crb2-T215A mutations impair Top3 activity.However, there is a potential alternative explanation for thisrescue effect: as in the case of the deletion of rqh1, high Top3protein levels could contribute to the increase in IR survivalby impairing Rqh1 helicase function. To exclude this possibility,we overexpressed top3 in wild-type cells and found that high proteinlevels of Top3 did not increase the sensitivity of wild-type cellsto IR (data notshown).

An obvious link between Cdc13 and Crb2 is the Cdc2-dependent phosphorylation of Crb2 at T215. Because the mutation in cdc13impairs Cdc2 kinase activity, a reduced phosphorylation stateof T215 could explain the observed genetic relationship. However,the use of an antibody ( $alpha$ -T125-P) that recognizes Crb2 only inits CDK-phosphorylated form revealed that the phosphorylationstatus of T215 was not significantly altered in a cdc13-245 backgroundunder permissive conditions (data not shown). Thus, the relationshipbetween Crb2 and Cdc13 appears to be more indirect (seeDiscussion).

Mutations in cdc13 and crb2 cause Rqh1-dependent hyperrecombination

As a consequence of impaired Top3 activity in cdc13-245 and crb2-T215A mutants, Rqh1 DNA helicase could become hyperactive.Because such an increase in uncontrolled activity could resultin more recombination events, we integrated a recombination substrateinto wild-type, crb2-T215A, and cdc13-245 cells to measure spontaneousand IR-induced HR. The recombination substrate consists of twoade6 heteroalleles that are separated by 4.5 kb of DNA containinga ura4⁺ marker (Schuchert and Kohli 1988). Recombination between theheteroalleles restores a functional ade6 gene and allows growthon medium lacking adenine. Two types of event can be distinguished,gene conversion and crossover recombination, which results inloss of ura4⁺.

The spontaneous recombination frequency in a wild-type background was 2.8 ± 0.5 × 10³ (0.7 × 10³/2.1 × 10³ conversion/crossover), and exposure to increasing doses of IRdid not change this rate significantly (Fig. 6A,C). A similarrate of spontaneous recombination was observed in a crb2-T215Abackground, 2.2 ± 0.4 × 10³ (0.6 × 10³/1.6 × 10³ conversion/crossover). However, in contrast to wild-type cells,the rate of recombination increased up to 50-fold when crb2-T215Acells were treated with increasing doses of IR (Fig. 6A). In agreementwith the functional link between Cdc13 and Crb2, cells harboringthe cdc13-245 allele showed a similar phenotypic trait, althoughIR-induced recombination increased only fivefold (Fig. 6C). Interestingly,the mutation in cdc13 deceased the spontaneous rate approximatelyfourfold, 0.8 ± 0.3 × 10³ (0.5 × 10³/0.3 × 10³ conversion/crossover), when compared with the other two strains.This decrease in spontaneous recombination might be caused bythe early defect in HR. In no case was there a significant differencein the ratio of conversion to crossover events in response toIR (data not shown).

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Figure 6. Both crb2-T215A cells and cdc13-245 cells show Rqh1-dependent hyperrecombination in response to IR. (A,C) Relative induction of the recombination rate between two ade6 heteroalleles in response to increasing doses of IR. (B,D) Cell survival during the recombination experiment. All data shown are the average of three independent experiments.

As predicted, the IR-induced hyperrecombination observed in crb2-T215A and cdc13-245 mutants was largely dependent on Rqh1activity (Fig. 6A,C). Deletion of rqh1 significantly reduced thenumber of ade6⁺ recombinants in both mutant backgrounds at the same time as itsuppressed the IR sensitivity (Fig. 6B,D). This increase in thesurvival rate indicates that Rqh1-dependent hyperrecombinationmay reflect the primary cause of IR sensitivity in both cdc13-245cells and crb2-T215Acells.

	Discussion

Top Abstract Introduction Results Discussion Materials and methods References

Our findings allow us to propose a model suggesting a functional link between Cdc2-cyclin B kinase activity and recombinationalrepair of DSB induced in G₂ by IR (Fig. 7). In this model, Rqh1,in association with Top3, processes recombination intermediatesthat are channeled into this pathway by at least two differentevents. One of these early recombination steps is dependent onCdc2-Cdc13 kinase activity, whereas the other step requires Rad50.In addition, Cdc2-Cdc13 kinase activity exerts a second functionlater in HR by facilitating the processing of recombination intermediatesby Rqh1 and Top3. Interestingly, this late step also requiresa functional Crb2 protein. Because Crb2 was so far only attributedto the checkpoint response and not to the repair response (Wilsonet al. 1997; Esashi and Yanagida 1999), these data provide a newlink between both pathways.

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Figure 7. A model indicating two functions for Cdc2-cyclin B kinase in HR. (Left panel) Cdc2-cyclin B kinase activity positively regulates an early step in HR that is redundant with Rad50. Both steps generate recombination intermediates that are processed by Rqh1 DNA helicase in association with topoisomerase III. Cdc2-cyclin B kinase activity exerts a second function together with Crb2 at a late step in HR. Both proteins are required to maintain Top3 activity until all recombination intermediates are processed. Cdc2-Cdc13 kinase activity may prevent premature dephosphorylation of Crb2, thereby supporting Top3 function. In the absence of Top3 activity, Rqh1 uses an alternative pathway resulting in hyperrecombination. (Right panel) Probable defects associated with the cdc13-245 mutation.

Is there an independent function for cyclin B?

In S. pombe, there is no evidence suggesting that cyclin B can function independently of Cdc2 kinase. Cdc13 appears to targetCdc2 to its nuclear destinations, and Cdc13 has to dissociatefrom Cdc2 to be degraded at the metaphase-anaphase transition(Decottignies et al. 2001). There are two plausible explanationsfor the IR sensitivity of cdc13-245 cells, which are not mutuallyexclusive. The mutation in cyclin B could either interfere withthe localization of Cdc2 to structures within the nucleus, orit could reduce the kinase activity of the protein complex. Ourdata support the second explanation. Under permissive conditions,cdc13-245 cells slightly delay entry into mitosis (data not shown),which requires high Cdc2-cyclin B kinase activity. Such a decreasein Cdc2 activity would be consistent with the result of our invitro kinase assay. The E255R substitution within the cyclin boxof Cdc13 did not affect the interaction with Cdc2, but it dramaticallydecreased the phosphorylation of histone H1 (Fig. 1F). These invitro data are in agreement with a previously published reportshowing that mutations of invariant residues in the cyclin box,which included an E255Q substitution, result in the accumulationof Cdc2-cyclin B kinase complexes with impaired activity (Zhengand Ruderman 1993).

A role for cyclins in the response to DNA damage in other systems

To our knowledge, there is only one report in the literature showing a role for cyclins in the response to DNA damage. Lossof the S-phase cyclins Clb5 and Clb6 renders Saccharomyces cerevisiaecells sensitive to MMS, UV-light, and IR (Meyn and Holloway 2000).In contrast to the normal checkpoint response of cdc13-245 cells(Fig. 1D), a clb5-d clb6-d double mutant bypasses the checkpointarrest in metaphase and arrests instead with separated sisterchromatids. Because sister chromatid cohesion is established whencells are passing through S phase (Uhlmann and Nasmyth 1998),loss of Clb5 and Clb6 could indirectly affect cell cyclearrest.

The repair defect caused by cdc13-245 is G₂-specific

HR is not only required to repair DSBs in G₂ but also during S phase to restart stalled replication forks (Michel et al. 2001).This dual function explains why mutants deficient in HR are sensitiveto nucleotide depletion by HU treatment and lose viability whenOkazaki fragment processing is defective (Muris et al. 1996).In this context, cdc13-245 is not a typical recombination mutant.cdc13-245 cells are not HU sensitive (Fig. 1C), and loss of Rad2endonuclease, which is required for the processing of Okazakifragments, is not synthetically lethal (data not shown). Hence,the repair defect in cdc13-245 mutant cells appears to be restrictedto postreplicative stages in the cell cycle. A G₂-specific functionof Cdc13 is consistent with its expression profile, which risesduring S phase and peaks in G₂ (Moreno et al. 1989). A G₂-specificrole in recombination repair is also compatible with our observation(Fig. 1E) that ~40% of cdc13-245 cells, when irradiated in G₂,enter a catastrophic mitosis upon exit from the G₂/Marrest.

Rqh1 DNA helicase is required to repair DSBs in G₂

Rqh1 belongs to the highly conserved RecQ family of DNA helicases, which includes S. cerevisiae Sgs1 and the human BLM andWRN proteins, which are mutated in patients suffering from Bloom'sand Werner's syndromes, respectively (Mohaghegh and Hickson 2001).A body of evidence suggests that these helicases function in Sphase to prepare blocked replication forks for the recombinationalrepair machinery (Murray et al. 1997; Stewart et al. 1997; Doeet al. 2000). The data we present here show a further functionfor Rqh1 in the repair of DSBs in G₂. Rqh1 relocalizes from apredominantly nucleolar distribution to foci in the chromatincompartment of the nucleus upon irradiation in G₂ (Fig. 4E,F).In addition, loss of rqh1 improves the survival rate of cdc13-245cells (Fig. 4B), strongly suggesting that Rqh1 acts upstream of,or parallel to, the recombination step dependent on Cdc2-cyclinB kinase activity. Several published observations support thissuggestion: First, BLM is most highly expressed in late S phaseand G₂, when HR occurs. Second, BLM and Sgs1 both associate withRad51. And, finally, BLM colocalizes with human Rad51 and bindsto regions of ssDNA, when cells are irradiated in G₂ (Bischofet al. 2001; Wu et al. 2001).

Our kinetic analysis of Rqh1 foci indicates that Rqh1 helicase acts late during the G₂/M arrest. Such a late function is consistentwith the finding that loss of Rqh1 did not affect focal assemblyof Rhp51 in a rad50-d background (Fig. 4C). In vitro data obtainedfor Sgs1 and BLM helicases indicate that Rqh1 could process Hollidayjunctions. Both Sgs1 and BLM catalyze branch migration and unwindfour-way junctions in vitro (Bennett et al. 1999; Karow et al.2000).

What is the repair defect in a cdc13-245 mutant?

The correlation between DNA-damage-induced hyperrecombination and cell viability suggests that inappropriate recombinationmay be primarily responsible for the loss of IR resistance whenCdc2-cyclin B kinase activity is impaired. cdc13-245 cells showa fivefold induction in the recombination rate between two ade6heteroalleles after a dose of 500 Gy (Fig. 6C). Based on the observationsthat loss of rqh1 both suppresses these recombination events (Fig.6C) and restores IR resistance of cdc13-245 mutant cells (Fig.6D), we can speculate that Rqh1 activity might be a target eitherdirectly or indirectly of Cdc2-Cdc13 kinase and is consequentlyderegulated in cdc13-245 cells. It has been suspected for sometime that mutations in DNA topoisomerases stimulate recombinationthrough a mechanism that involves RecQ-like DNA helicases (Walliset al. 1989; Gangloff et al. 1994). In several systems, it hasbeen proposed that helicases generate an intermediate that becomesrecombinogenic if not processed by topoisomerases (Gangloff etal. 1999; Goodwin et al. 1999; Harmon et al. 1999).

Top3 is therefore a good candidate for such a function because of its interaction with RecQ-like DNA helicases and the factthat this is highly conserved (Bennett and Wang 2001). Our findingthat overexpression of top3 efficiently restores radiation resistancein the cdc13-245 mutant (Fig. 5F) implies that Rqh1 DNA helicasebecomes deregulated through a defect in Top3 function, and thatexcess Top3 can substitute for this loss of function. An alternativeexplanation would be that Top3 physically dissociates from Rqh1in cdc13-245 cells, a possibility hard to test directly becausethe majority of Rqh1 and a proportion of Top3 proteins are insolublein S. pombe G₂ cells (data not shown). In S. cerevisiae, mutationsin the N terminus of Sgs1, which promotes the interaction withTop3, are known to result in hyperrecombination (Mullen et al.2001). Our unpublished experiments are not, however, consistentwith the possibility that Cdc2-Cdc13 regulates Top3-Rqh1 interactionsdirectly: we mutated the two highly conserved Cdc2 phosphorylationmotifs in the N-terminal domain of Rqh1 without observing anyobvious phenotypes. Furthermore, we were able to immunoprecipitateRqh1 and Top3 from both soluble wild-type and cdc13-245 extractsbefore and after IR (data not shown). Such experiments, however,do not address the status of the insoluble Rqh1 and Top3, whichmay reflect the activecomponent.

The role of Crb2 in the repair of DSBs

Support for the idea that checkpoint-dependent hyperphosphorylation of Crb2 is required for efficient Top3 activity comesfrom several experiments: Loss of rqh1 restores IR resistancein a crb2-T215A mutant (Fig. 5C), which cannot be hyperphosphorylated(data not shown; Esashi and Yanagida 1999), strongly indicatingthat Rqh1 DNA helicase generates harmful intermediates in thesecells after IR treatment. At 140 min postirradiation, the numberof crb2-T215A cells assembling Rqh1 foci increased from 23% ±3% observed in wild-type cells to 72% ± 8% (Fig. 5D). Finally,overexpression of top3 very efficiently increased the survivalrate of crb2-T215A cells in an rqh1-dependent manner (Fig. 5E;data notshown).

Although these results mirror the data obtained for cdc13-245 cells, our observation that the state of Cdc2-dependent phosphorylationof Crb2 at T215 was not significantly changed in a cdc13-245 backgroundunder permissive conditions (data not shown) suggests an indirectlink between both proteins. We noticed repeatedly that, in responseto IR, the Rad3-dependent modifications of Crb2 disappeared prematurely,although cells were still arrested in G₂ (data not shown). Thissuggests that Cdc2-Cdc13 kinase activity exerts a regulatory role,thereby controlling either a phosphatase that dephosphorylatesCrb2 or a kinase that modifies Crb2 upon IR. We speculate thatpremature loss of the IR-induced hyperphosphorylation of Crb2terminates Top3 function before all recombination intermediatesareprocessed.

Crb2 shares several features with the tumor suppressor protein BRCA1. Each protein contains two BRCT domains at the C terminus,both proteins are modified by CDKs, and, finally, both proteinsbecome hyperphosphorylated in a checkpoint-dependent manner uponIR (Scully et al. 1997; Ruffner et al. 1999). BRCA1 seems to actas a scaffold protein to allow assembly of both checkpoint proteinsand repair enzymes (Paull et al. 2000; Wang et al. 2000). Interestingly,among the proteins that bind to BRCA1 is the BLM DNA helicase(Wang et al. 2000). We suggest a similar scaffold role for Crb2.In response to IR, checkpoint-dependent hyperphosphorylation ofCrb2 might promote an interaction with Top3 that is essentialfor Top3 activity. Consistent with this view, Crb2 interacts inthe two-hybrid system with the BRCT domain of Cut5 (Saka et al.1997) and the human homolog of Cut5, TopBP1, binds to topoisomeraseII (Makiniemi et al. 2001).

The recent finding that BRCA1 binds directly to branched DNA structures and four-way junctions (Paull et al. 2001), the sameDNA structures recognized by BLM and Sgs1 helicases, suggestsan alternative, but not mutually exclusive, explanation for thefunction of Crb2: Crb2 could directly participate in the processingof recombination intermediates. Such a function would be consistentwith the observation that the S. cerevisiae homolog of Crb2, Rad9,is involved in the formation of ssDNA following DNA damage neartelomeres (Lydall and Weinert 1995; Booth et al. 2001).

Cdc2-cyclin B performs another function at an early stage in HR

The first step to be observed after DSB formation is a resection of the DNA ends resulting in 3' ssDNA tails. Whether thisresection is by a 5'-3' exonuclease or by an endonuclease associatedwith a helicase is not known. However, loss of the Rad50-Mre11-Xrs2protein complex retards the rate of 5'-3' exonuclease activityin vivo (Ivanov et al. 1994). The fact that rad50-d cells stillshow end-processing suggests the existence of redundant pathways.This is consistent with our observation that deletion of rad50only reduces, but does not abolish Rhp51 foci formation upon IR(Fig. 3B,C). Interestingly, in these cells assembly of Rhp51 fociis highly dependent on a functional Cdc2-cyclin B kinase (Fig.3B,C), indicating that CDK activity controls an early step inHR that is redundant with Rad50. In S. cerevisiae, one endonucleasethat appears to act as a backup system for Rad50 is Exo1 (Tsubouchiand Ogawa 2000). Given this information, we explored the roleof Exo1 in S. pombe. Like cdc13-245 rad50-d cells, an exo1-d rad50-ddouble mutant was unable to assemble Rhp51 foci 1 h postirradiation(data not shown). However, we have been unable to find furtherevidence for a functional link between Exo1 and Cdc2-cyclin Bkinase.

Conclusion

Our data provide a link between Cdc2-cyclin B activity, the BRCT-domain-containing checkpoint protein Crb2, and the controlof DNA repair in G₂. Intriguingly, the closest analog to Crb2in mammalian cells is BRCA1, which is also known to be CDK-phosphorylated(Ruffner et al. 1999) and which has been implicated in channelingDSBs into different repair pathways (Moynahan et al. 1999). Itis tempting to speculate that the control of recombinational repairby CDK complexes reflects a fundamental mechanism whereby thechromatin's replication status, and therefore the repair processesmost appropriate for DSB repair, are `hard wired` into the chromatin.Mechanistically, we have implicated the BRCT-domain protein Crb2in this process, where it appears to control a late stage of recombinationby influencing the activity of Top3 and its associated RecQ-likeDNA helicase,Rqh1.

	Materials and methods

Top Abstract Introduction Results Discussion Materials and methods References

Genetics and cell biology techniques

Strains were constructed by standard genetic techniques. The protocols for checkpoint measurements, cell scoring, irradiation,lactose gradient centrifugation, centrifugal elutriation, andfluorescence-activated cell sorter (FACS) analysis are all describedin Edwards and Carr (1997). Indirect immunofluorescence microscopywas performed according to the protocol previously published inCaspari et al. (2000), with the following changes: Both the anti-MYCantibody and the anti-hRad51 (Santa Cruz H-92) were diluted 1:100,whereas the anti-Rqh1 antibody was diluted 1:400. To determinethe percentage of cells showing nuclear foci, we visually scored1000 cells for eachsample.

Isolation of the cdc13-245 mutant

Wild-type cells (leu1-32 ura4-D18 ade6-704 h) were subjected to EMS (ethylmethane sulfonate) mutagenesis as described in Lawrence(1991). Mutants were grown on rich medium plates at 27°C and replica-platedonto two sets of plates, which were incubated at 27°C and at 36°C.Temperature-sensitive strains were isolated and tested for theirsensitivity to various DNA-damaging agents. Sensitive strainswere crossed three times with the wild-type strain to determinewhether the sensitivity relates to a single mutation. The restrictivetemperature for the cdc13-245 strain is 33°C. All experimentspresented here were performed at the permissive temperature of27°C.

Construction of the crb2-T215A mutant

Strain construction was based on the method described in Edwards et al. (1999). The crb2-T215A mutant was constructed as follows:The sequence between S43 and T215 (including both codons) wasreplaced by ura4⁺ in a wild-type background. The deletion mutant was transformedwith an NdeI fragment containing the T215A single mutation. Strainsthat had replaced the ura4⁺ gene with the mutated crb2 fragment were counterselected on YEAplates containing 1 mg/mL 5-FOA (5-fluorooroticacid).

Cell extracts, immunoprecipitation, and in vitro kinase assay

The protocols for total cell extracts, soluble extracts, and immunoprecipitation experiments are all described in Caspariet al. (2000). Insoluble extracts were prepared with the followingchanges: In buffer B, sodium phosphate was substituted by 100mM HEPES (pH 7.0; called buffer D). Cells were broken with glassbeads in a Ribolyser (Hybaid); 400 µL of buffer D was added afterhomogenization, and the cell homogenate was spun (Heraeus, 4K)into a new test tube. The protocol for the in vitro Cdc2 kinaseassay is published in Moreno et al. (1989).

Recombination assay

Mitotic recombination was assayed by the recovery of Ade6⁺ recombinants from strains containing the recombination substratedescribed in Schuchert and Kohli (1988). The assay was performedaccording to the protocol published in Paulovich et al. (1998).To assay the recombination frequency in response to IR, cellswere treated with the indicated doses of IR before being platedonto selectivemedium.

	Acknowledgments

We thank Fumiko Esashi and Mitsuhiro Yanagida for providing the crb2 alleles used for integration and their help with thephospho-specific antibody. We are grateful to Stefania Francesconifor sending us the MYC-crb2 strain and to Edgar Hartsuiker forproviding the rqh1-d rad50-d double mutant. Finally, we wouldlike to thank Jacky Hales for the anti-Cdc13 antibodies. Thiswork was funded by grants from the MRC to T.C. and A.M.C. (E160/121-4668),the Cancer Research Campaign to J.M.M.(SP2396/0201), and the HFSPto A.M.C. (RGO-178/2000-M).

The publication costs of this article were defrayed in part by payment of page charges. This article must therefore be herebymarked "advertisement" in accordance with 18 USC section 1734solely to indicate thisfact.

	Footnotes

Received November 28, 2001; revised version accepted March 26, 2002.

¹ Present address: Pieris ProteoLab AG, Lise-Meitner-Straße 30, D-85354 Freising,Germany.

² Correspondingauthor.

E-MAIL A.M.Carr{at}sussex.ac.uk; FAX 44-1273-678-121.

Article and publication are at http://www.genesdev.org/cgi/doi/10.1101/gad.221402.

References

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Abstract
Introduction
Results
Discussion
Materials and methods
References

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RESEARCH PAPER Cdc2-cyclin B kinase activity links Crb2 and Rqh1-topoisomerase III

RESEARCH PAPER
Cdc2-cyclin B kinase activity links Crb2 and Rqh1-topoisomerase III