Molecular anatomy and regulation of a stable replisome at a paused eukaryotic DNA replication fork

doi:10.1101/gad.337205

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Published online before print , 10.1101/gad.337205
GENES & DEVELOPMENT 19:1905-1919, 2005
©2005 by Cold Spring Harbor Laboratory Press; ISSN 0890-9369/ $5.00

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RESEARCH PAPER

Molecular anatomy and regulation of a stable replisome at a paused eukaryotic DNA replication fork

Arturo Calzada¹^,2^,3, Ben Hodgson¹^,3, Masato Kanemaki¹, Avelino Bueno² and Karim Labib¹^,4

¹ Paterson Institute for Cancer Research, Christie Hospital NHS Trust, Manchester M20 4BX, United Kingdom; ² Cancer Research Institute, University of Salamanca/CSIC, 37007 Salamanca, Spain

Abstract

Top
Abstract
Results
Discussion
Materials and methods
Acknowledgments
References

Eukaryotic cells regulate the progression and integrity of DNAreplication forks to maintain genomic stability and couple DNAsynthesis to other processes. The budding yeast proteins Mrc1and Tof1 associate with the putative MCM–Cdc45 helicaseand limit progression of the replisome when nucleotides aredepleted, and the checkpoint kinases Mec1 and Rad53 stabilizesuch stalled forks and prevent disassembly of the replisome.Forks also pause transiently during unperturbed chromosome replication,at sites where nonnucleosomal proteins bind DNA tightly. Wedescribe a method for inducing prolonged pausing of forks atprotein barriers assembled at unique sites on a yeast chromosome,allowing us to examine for the first time the effects of pausingupon replisome integrity. We show that paused forks maintainan intact replisome that contains Mrc1, Tof1, MCM–Cdc45,GINS, and DNA polymerases ${alpha}$ and ${epsilon}$ and that recruits the Rrm3 helicase.Surprisingly, pausing does not require Mrc1, although Tof1 andCsm3 are both important. In addition, the integrity of the pausedforks does not require Mec1, Rad53, or recombination. We alsoshow that paused forks at analogous barriers in the rDNA areregulated similarly. These data indicate that paused and stalledeukaryotic replisomes resemble each other but are regulateddifferently.

[Keywords: DNA replication forks; Mrc1; Tof1; Csm3; checkpoint; recombination]

Received January 17, 2005; revised version accepted June 17, 2005.

Chromosomal DNA replication in eukaryotic cells is initiatedfrom multiple origins on each chromosome, each of which is activatedjust once during the S phase of each cell cycle, to ensure thata single copy of the genome is made (Kearsey and Cotterill 2003

;Diffley 2004

; Stillman 2005

). DNA replication forks are establishedat each origin and then move away as the parental DNA duplexis unwound by the action of DNA helicases. In order to preservegenomic stability and prevent lethal damage to the chromosomesduring mitosis, it is crucial that progression of the two convergingforks from each pair of adjacent origins continues until theforks meet each other and termination occurs. Despite this fact,individual forks can stop for a variety of reasons before termination,and eukaryotic cells have thus evolved a variety of mechanismsthat regulate both the progression and stability of DNA replicationforks.

Much of our understanding of the regulation of eukaryotic DNAreplication forks has come from studies of budding yeast cellstreated with the drug hydroxyurea (HU), which inhibits ribonucleotidereductase and thus causes forks to stall. The stalling of forkprogression is partly a consequence of the reduced availabilityof dNTPs but also requires the two replisome components Mrc1and Tof1 (Katou et al. 2003). In the absence of these proteins,the replisome progresses faster than it is able to synthesizeDNA; it thus appears that individual replisomes play an activerole in the stalling of forks in response to HU. The mechanismby which Mrc1 and Tof1 restrain the progression of forks isnot understood, but they both interact with the Cdc45–MCM2–7complex that is thought to act as the DNA helicase responsiblefor unwinding the parental DNA duplex at DNA replication forks(Katou et al. 2003; Pacek and Walter 2004; Shechter et al. 2004;Nedelcheva et al. 2005).

Mrc1 and Tof1 are also both important for the activation ofa "checkpoint" response following nucleotide depletion by HU.The budding yeast kinases Mec1 and Rad53 block mitosis and alsoinhibit initiation events at later origins of DNA replicationunder such conditions. When cells lacking either Mrc1 or Tof1are treated with HU, neither anaphase nor the firing of lateorigins of DNA replication is inhibited, showing that checkpointactivation is partially defective (Alcasabas et al. 2001; Foss2001; Katou et al. 2003). It thus appears that Mrc1 and Tof1share a similar role at HU-stalled forks.

Checkpoint activation is also essential in order to preservethe stability of HU-stalled DNA replication forks (Lopes etal. 2001) and thus prevent disassembly of the replisome (Cobbet al. 2003). In addition, both Mec1 and Rad53 are essentialto maintain the integrity of DNA replication forks that stallupon encountering DNA damage induced by the alkylating agentmethyl methanesulphonate (MMS) (Tercero and Diffley 2001); cellslacking either kinase are therefore exquisitely sensitive tothe stalling of DNA replication forks by HU or MMS (Allen etal. 1994; Desany et al. 1998; Tercero and Diffley 2001).

DNA replication forks can also pause transiently during thenormal process of chromosome replication, upon encounteringsites where nonnucleosomal proteins are bound tightly to DNA(Greenfeder and Newlon 1992; Wang et al. 2001; Ivessa et al.2002, 2003; Makovets et al. 2004). It has been estimated thatthere are >1000 such pause sites in the budding yeast genome(Ivessa et al. 2003), and they are thought to represent an importantchallenge to the maintenance of genomic stability, as thereis evidence that such paused forks may break and that theirsubsequent repair by homologous recombination may provide asource of genetic variability (Keil and McWilliams 1993; Ivessaet al. 2000, 2002, 2003; Ahn et al. 2005; Lambert et al. 2005;Prado and Aguilera 2005).

The consequences of the pausing of eukaryotic DNA replicationforks at protein–DNA barriers are much less well understoodthan is the case for HU-stalled forks, principally because forksonly pause very transiently at most sites, so that a molecularanalysis is much more complicated. Previous studies have notdetermined the kinetics of pausing at individual sites withinthe genome, and many fundamental questions remain to be answered.Most importantly, it is not known whether the replisome disassembleswhen a fork encounters a protein–DNA barrier or whetherreplisome proteins, including regulators such as Mrc1 and Tof1,remain stably associated with the fork, as is the case at HU-stalledforks. Previous work suggested that the MCM2–7 complexmust be maintained at DNA replication forks in an uninterruptedfashion between initiation and termination, as removal of MCMproteins from HU-stalled forks blocks irreversibly the recoveryof DNA synthesis (Labib et al. 2000), but it has previouslynot been possible to test whether the putative MCM helicasedoes indeed remain associated with paused forks, as would bepredicted by this model. It would also be interesting, for example,to examine whether proteins such as the primase associated withDNA polymerase ${alpha}$ remain at the paused fork, as lagging strandsynthesis is completed rapidly after pausing occurs.

It appears, however, that the progression of paused forks isactively regulated in a somewhat analogous fashion to HU-stalledforks, as the fission yeast homolog of Tof1 is required, togetherthe associated Swi3 protein, for forks to pause at the mating-typelocus and in the rDNA (Dalgaard and Klar 2000; Krings and Bastia2004). This suggests that the progression of paused and stalledforks may be restrained by the same mechanism, although therole of Mrc1 at paused forks has not been tested directly.

It is presently unclear whether checkpoint kinases play a rolein preserving the stability of paused forks in budding yeast.Both Mec1 and Rad53 are essential for viability even in theabsence of replication stress, and cells lacking Mec1 accumulatedouble-strand breaks in DNA and are unable to complete chromosomereplication (Zhao et al. 2001; Cha and Kleckner 2002). The lethaleffects of deleting the MEC1 or RAD53 genes can be suppressedby overexpressing the large subunit of ribonucleotide reductase(Desany et al. 1998) or by additionally deleting the gene encodingthe Sml1 protein, which is an inhibitor of ribonucleotide reductase(Zhao et al. 1998; Chabes et al. 1999). Previous studies ofbudding yeast have not determined whether DNA replication forksstill pause at protein barriers under such conditions.

The rDNA in budding yeast contains an efficient replicationfork barrier sequence (RFB) that actively blocks the progressionof DNA replication forks when bound tightly by a specific proteincalled Fob1 (Fork block 1) (Brewer and Fangman 1988; Linskensand Huberman 1988; Kobayashi and Horiuchi 1996; Kobayashi 2003;Mohanty and Bastia 2004). As shown in Figure 1A (panel i), eachof the $~$ 200 rDNA repeats contains a potential origin of bidirectionalDNA replication. Initiation occurs within a limited number ofthe repeats during S phase, and the rightward fork is free toprogress into the adjacent unit, in the same direction as transcription.The leftward fork passes through a 5S rRNA gene without opposingtranscription, but then pauses at the RFB (Brewer and Fangman1988; Linskens and Huberman 1988). The barrier only blocks theprogression of leftward forks, so that replication of the rDNArepeats occurs principally in the same direction as the highlyactive transcription by RNA PolI.

The highly repetitive nature of the rDNA impedes the analysisof individual paused DNA replication forks, and each leftwardfork at the RFB is generally resolved by the arrival of a rightwardfork from the preceding repeat (Brewer and Fangman 1988; Linskensand Huberman 1988). We describe a system that exploits the efficiencyof the Fob1–RFB to allow extended but finite pausing ofspecific DNA replication forks that originate from adjacentorigins on chromosome 3 of budding yeast. By studying the compositionand regulation of such individual paused eukaryotic replisomes,we identify similarities with, but also important differencesfrom, their counterparts at HU-stalled forks.

Results

Top
Abstract
Results
Discussion
Materials and methods
Acknowledgments
References

A model system for studying paused eukaryotic replisomes

Our initial aim was to create an experimental system with whichto study the fate of eukaryotic replisomes when DNA replicationforks pause transiently at protein–DNA barriers duringthe process of chromosome replication. We wanted to study forksfrom the earliest origins so that generation of the paused forkswould not be affected if we subsequently used strains or conditionsthat activate checkpoint kinases, which inhibit the firing oflater origins. Previous studies determined the location andtiming of origins of DNA replication throughout the buddingyeast genome (Raghuraman et al. 2001), and we used this informationto design a strain in which two early forks would pause foran extended but finite period of time at unique sites, withoutbeing resolved by the arrival of forks from a neighboring replicon.The two origins ARS305 and ARS306 on chromosome 3 are separatedby 36 kb and are among the earliest and most active originsin the genome. In almost every cell cycle, a rightward forkfrom ARS305 and a leftward fork from ARS306 enter the interveningregion with similar timing and subsequently meet toward thecenter of the region (Reynolds et al. 1989; Raghuraman et al.2001). RFB sequences from the rDNA were inserted within thisregion, $~$ 10 kb from each origin, so that the forks from bothARS305 and ARS306 would pause with similar kinetics, withoutbeing resolved by a fork from elsewhere in the genome (see Fig. 1A,panel ii; Supplementary Fig. 1). We used a yeast strainin which expression of the FOB1 gene was controlled by the regulatableGAL1,10 promoter, so that we could switch-off FOB1 and thusgrow cells without activating the RFBs between ARS305 and ARS306,synchronize cells in the G1 phase of the cell cycle, and thenrapidly induce FOB1 to activate the barriers before examiningthe immediate consequences in the subsequent round of chromosomereplication.

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Figure 1. Using the Fob1–RFB system to pause specific DNA replication forks on chromosome 3. (A, panel i) Map of two consecutive repeats of the rDNA on chromosome 12 of budding yeast. The positions of the replication fork barrier (RFB), origin of DNA replication (ARS), 35S rRNA (35S), and 5S rRNA (5S) genes are indicated. (Panel ii) Insertion of RFB sequences on chromosome 3 to block the forks from ARS305 and ARS306. The distances indicated are measured from the left end of chromosome 3; "B" and "S" mark the positions of BclI and SalI restriction enzyme sites used for the two-dimensional DNA gels. See Materials and Methods and Supplementary Figure 1 for more information. (Panel iii) Using two-dimensional DNA gels to study DNA replication intermediates; see text for details. The two spots below the Y-arc in the left panel correspond to other sites in the genome that are recognized weakly by the chosen probe. (B) DNA replication forks do not pause at the RFBs on chromosome 3 in the absence of Fob1. (C, panel i) In cells expressing Fob1, the forks from ARS305 and ARS306 pause for an extended period at the two RFBs on chromosome 3. (Panel ii) The histograms show a quantification of paused forks at the indicated times (calculated as described in Materials and Methods).

We used two-dimensional (2D) "neutral-neutral" DNA gels (Brewerand Fangman 1987

) to study DNA replication intermediates isolatedfrom samples taken every 15 min after releasing cells from G1arrest. After digestion of genomic DNA with appropriate restrictionenzymes, both unreplicated and fully-replicated linear DNA fragmentscorresponding to a particular locus migrate in an identicalfashion in both dimensions, producing a prominent spot in thebottom right of the gel (Fig. 1A, panel iii). In contrast, restrictionfragments that contain replication intermediates are retardedin the first dimension by virtue of their greater size, andare also retarded in the second dimension due to their abnormalshape. Passive replication of the region produces a characteristic"Y-arc" beginning at the spot corresponding to linear DNA andending at a point equivalent to a restriction fragment thatis just less than fully replicated (Fig. 1A, panel iii, left).Pausing of the fork at a specific site produces an accumulationof molecules with the same size and shape, corresponding toa distinctive spot on the Y-arc (Fig. 1A, panel iii, middle,spot labeled RFB).

Initially we grew cells in the absence of Fob1 throughout theexperiment and examined replication of the two barrier sitestogether with an intervening locus (Fig. 1B). We observed simpleY-arcs at all three sites, peaking between 30 and 45 min afterrelease from G1 arrest. This shows that the two forks from ARS305and ARS306 replicate the region without pausing significantlyat the RFB sequences in the absence of the Fob1 protein.

We then released cells from G1 arrest after first switching-onexpression of Fob1. As shown in Figure 1C, a strong spot appearedon the Y-arc for each of the two forks, at a position correspondingto the RFB sequence within the restriction fragment (Fig. 1C,panel i, top and bottom). The rightward fork from ARS305 andthe leftward fork from ARS306 arrive at the corresponding RFBwith very similar kinetics and then pause for an extended periodrelative to the time required to replicate the rest of the genome(Fig. 1C, panel ii; Supplementary Fig. 2). Pausing of the twoforks delays replication of the site between the two barriers,although Y-arcs are eventually observed at later times (Fig. 1C,panel i, middle), indicating that DNA synthesis does subsequentlyresume at the paused forks, and cells are thus able to growwell in the continued presence of active barriers on chromosome3 (Supplementary Fig. 3).

Pausing of forks at the Fob1–RFB does not cause replisome disassembly

The preceding experiments show that the introduction of twoRFBs between ARS305 and ARS306 generates an ideal system withwhich to study the protein composition and stability of pausedeukaryotic replisomes, as the two forks pause for an extendedbut finite period at unique sites. We could thus examine thekinetics with which the replisome arrives at the RFB and iseither maintained or disassembled, by using cultures of cellsthat are replicating their chromosomes synchronously. We usedchromatin immunoprecipitation (ChIP) to examine the compositionof the replisome under such conditions, by treating cells withformaldehyde before preparing an extract that was sonicatedto shear chromosomal DNA into fragments of several hundred basepairs; we then isolated the protein of interest by immunoprecipitation.We used a "real-time" version of the polymerase chain reaction(PCR) to determine quantitatively the association of replisomeproteins with specific DNA sequences in vivo (see Materialsand Methods), and initially examined five sites on chromosome3: ARS305, a site very close to where the first RFB was inserted,a site between the two barriers, a site very close to the secondRFB, and ARS306 (sites 1–5 in Fig. 2A; Supplementary Fig.4). In all the subsequent experiments, cells were grown underidentical conditions to those described above for the experimentshown in Figure 1C.

To confirm that we were indeed able to detect proteins presentat the RFB sites on chromosome 3, we used ChIP to examine theputative association of the Fob1 protein at the five sites mentionedabove, and observed a strong enrichment in the Fob1 immunoprecipitatesof the DNA sequences close to each of the two RFBs introducedon chromosome 3 (Fig. 2B, sites 2 and 4). Although the resolutionof ChIP is limited to several hundred nucleotides, this experimentconfirmed that we could use our assay to detect proteins thataccumulate at the RFB sites on chromosome 3, where DNA replicationforks pause during the process of chromosome replication.

We thus proceeded to examine the association of replisome proteinswith the same sites at different points during the S phase ofthe cell cycle. We started by examining Pol2, the catalyticsubunit of DNA polymerase ${epsilon}$ , which has previously been shownto remain associated with the stalled replisome at DNA replicationforks when cells are treated with HU (Aparicio et al. 1997,1999; Tanaka and Nasmyth 1998; Masumoto et al. 2000; Cobb etal. 2003). In a strain lacking RFB sequences on chromosome 3,Pol2 was strongly enriched at ARS305 and ARS306 30 min afterrelease from G1 arrest (Fig. 2C, panel i, –RFBs, sites1 and 5) and could also be observed $~$ 10 kb from each origin (sites2 and 4), consistent with its presence at active DNA replicationforks. Fifteen minutes later, association of Pol2 with the abovesites was greatly reduced, and instead, the protein could bedetected toward the middle of the region (site 3), as replicationwas completed.

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Figure 2. Pausing of forks at the RFBs does not cause the replisome to disassemble. (A) ChIP was used to study the localization of proteins at the five sites indicated. Further details can be found in Supplementary Figure 4. (B) Cells were synchronized in the G1 phase of the cell cycle before expressing GAL-FOB1-9MYC for 45 min, maintaining the G1 arrest throughout. The Fob1-9Myc protein was detected specifically at the two RFBs introduced on chromosome 3. (C [panel i], D) The localization of Pol2-9Myc or Psf2/Cdc102-9Myc was examined at the same five sites, as cells entered synchronously into the S phase of the cell cycle in the presence (+RFBs) or absence (–RFBs) of the Fob1–RFBs on chromosome 3; see text for details. (C, panel ii) The region between ARS305 and the corresponding RFB was also examined with higher resolution.

We then examined Pol2 in a strain with active RFBs on chromosome3. Thirty minutes after release from G1 arrest, the associationof Pol2 with ARS305 and ARS306 was similar to that seen in theprevious experiment (Fig. 2C, panel i, +RFBs, sites 1 and 5).Strikingly, however, enrichment of the RFB-proximal sequenceswas greatly increased in the Pol2 immunoprecipitates (sites2 and 4). Moreover, we observed that these sequences were stillstrongly enriched in the Pol2 immunoprecipitates after 45 min,in contrast to the strain lacking RFBs. By 60 min, the associationof Pol2 with the RFB-proximal sequences was largely but notcompletely diminished.

We also examined with higher resolution the 10-kb region tothe right of ARS305 (Fig. 2C, panel ii). At 30 min after releasefrom G1 arrest, Pol2 was detected throughout this region regardlessof the presence or absence of RFBs on chromosome 3; 15 min later,however, only the sequence next to the RFB insertion site wasstrongly associated with Pol2, and this was dependent upon presenceof the RFB. Taken together, these experiments indicate thatPol2 remains associated with the forks from ARS305 and ARS306that pause at the two RFBs on chromosome 3.

We next examined the GINS complex, which plays an essentialthough poorly characterized role during chromosome replicationand has been shown to associate with stalled forks after HUtreatment (Kanemaki et al. 2003; Kubota et al. 2003; Takayamaet al. 2003). We used ChIP to determine the association of theGINS subunit Psf2/Cdc102 with the region between ARS305 andARS306 during S phase. As shown in Figure 2D, GINS behaves ina very similar fashion to Pol2, associating 30 min after releasefrom G1 arrest with both of the origins and also with DNA replicationforks (Fig. 2D, –RFBs and +RFBs), and then remaining associatedwith the two paused DNA replication forks (Fig. 2D, +RFBs 45min), until replication of the region resumes and is completed(Fig. 2D, +RFBs 60 min). We conclude, therefore, that GINS remainsassociated with paused DNA replication forks.

Previous studies of forks that stall after depletion of nucleotidesshowed that the putative MCM–Cdc45 helicase complex remainspart of the stalled replisome together with the two associatedproteins, Mrc1 and Tof1 (Aparicio et al. 1997; Katou et al.2003; Osborn and Elledge 2003). As shown in Figure 3A, panelsi,ii, Mcm4, Cdc45, Mrc1, and Tof1 are all retained at the siteof the paused forks originating from ARS305 and ARS306. We alsoexamined the Pri1 protein that forms part of the DNA polymerase ${alpha}$ -primase complex, and we found that this also associates withthe paused DNA replication forks (Fig. 3A, panel ii), just aspreviously shown for HU-stalled forks (Tanaka and Nasmyth 1998;Aparicio et al. 1999; Masumoto et al. 2000; Cobb et al. 2003;Lucca et al. 2004), despite the rapid completion of lagging-strandsynthesis behind the pause site (Lucchini and Sogo 1994; Gruberet al. 2000).

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Figure 3. Other components of the paused replisome. (A, panel i) Cdc45 accumulates during S phase at the sites of the paused forks (+RFBs) but is more transiently associated with the same sites in the absence of pausing (–RFBs). (Panel ii) Mcm4, Mrc1, Tof1, and Pri1 all remain associated with the forks that pause at the Fob1–RFBs on chromosome 3. (B) The localization of Pri1-9Myc and Cdc102-5Flag was determined in the same cells at the indicated times. The change in the specific enrichment of the RFB sequences is shown from 30 min (100%) to 40 min. (C) Rrm3 is specifically recruited to paused replisomes (panel i), and is not a stable component of active forks established at origins of replication (panel ii).

To provide stronger evidence that the various proteins describedabove all associate in a similar manner with the paused forks(despite small differences in kinetics seen from one experimentto another), we examined two different replisome componentsin the same cells. In the experiment shown in Figure 3B, bothPri1 and Psf2/Cdc102 associated in a similar manner with thetwo RFB sites 30 min after release from G1 arrest (Fig. 3B,30 min, sites 2 and 4). Ten minutes later, the enrichment ofthe ARS305-proximal barrier in the Pri1 immunoprecipitate hadreduced slightly to 86% of the value at 30 min, whereas theenrichment of the ARS306-proximal barrier had increased to 142%of the value at 30 min. For Psf2/Cdc102, the enrichment of theARS305-proximal barrier at 40 min decreased to 84% of the valueat 30 min, whereas the enrichment of the ARS306-proximal barrierincreased to 143% of the value at 30 min. This experiment showsthat the behavior of Pri1 and Psf2/Cdc102 at the RFBs was extremelysimilar. Overall, therefore, these experiments lead us to concludethat the replisome does not disassemble when a eukaryotic DNAreplication fork pauses upon encountering a protein–DNAbarrier. Instead, the paused fork retains an intact replisome,analogous to the replisome that is maintained at HU-stalledforks.

The Rrm3 helicase is specifically recruited to paused eukaryotic replisomes

It is possible that some proteins that function at DNA replicationforks do not normally form part of the active replisome butinstead are recruited specifically to paused or stalled replisomes.The Rrm3 DNA helicase plays an important role in helping forksprogress past protein–DNA barriers at many sites acrossthe budding yeast genome (Ivessa et al. 2003), including theFob1–RFB in the rDNA, but it is not clear if Rrm3 assemblesas part of the replisome at origins during the initiation ofchromosome replication or instead is specifically recruitedto paused DNA replication forks. We therefore examined the Rrm3helicase in a strain with RFBs on chromosome 3, and saw thatthe protein accumulates specifically at the sites of the pausedforks, with similar kinetics to other components of the pausedreplisome (Fig. 3C). Importantly, however, we could not detectsignificant association of Rrm3 with the two origins ARS305and ARS306 (Fig. 3C, panel i), or with other sites between ARS305and the corresponding RFB (Fig. 3C, panel ii). This suggeststhat Rrm3 is not normally a stable component of DNA replicationforks but instead is principally recruited to paused replisomes.

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Figure 4. Mrc1 is not essential for DNA replication forks from ARS305 and ARS306 to pause at the RFBs on chromosome 3, but Tof1 and Csm3 are both important. Fork progression was examined as above in cells lacking Tof1 (A), Mrc1 (B), or Csm3 (C). (D) Larger versions of the data from the 60-min time point. (E) Fob1 still associates with the RFBs on chromosome 3 in the absence of Tof1 or Csm3. Cells were synchronized in G1 phase, and expression of Fob1-9Myc was then induced for 45 min.

Mrc1 is not essential for the replisome to pause at the Fob1–RFB

At HU-stalled forks, both Mrc1 and Tof1 play a similarly importantrole in restraining progression of the stalled replisome (Katouet al. 2003). We have shown that both proteins are also componentsof the paused replisome at the Fob1–RFB (Fig. 3), andit might be expected therefore that both Mrc1 and Tof1 are equallyimportant for pausing, particularly as the fission yeast homologof Tof1 has already been shown to be important for forks topause within the mating-type locus and in the rDNA (Dalgaardand Klar 2000; Krings and Bastia 2004). We therefore used 2DDNA gels as above to examine the progression of forks from ARS305and ARS306 in the absence of either Tof1 or Mrc1. As shown inFigure 4A, both forks pass the corresponding RFB sites withvery little sign of pausing in a strain lacking the Tof1 protein.In striking contrast, forks from ARS305 and ARS306 are stillable to pause at the RFBs in the absence of Mrc1 (Fig. 4B),thereby identifying an important difference in regulation betweenforks that pause at a protein–DNA barrier and HU-stalledforks.

Work with fission yeast has shown that another protein, Swi3,is also required in addition to the homolog of Tof1 for forksto pause in the mating locus and in the rDNA (Dalgaard and Klar2000; Krings and Bastia 2004). The budding yeast protein Csm3(Rabitsch et al. 2001) is similar in sequence to Swi3, and previouswork has shown that Tof1 and Csm3 interact with each other (Mayeret al. 2004). We thus examined the progression of forks fromARS305 and ARS306 in cells lacking Csm3, and saw once againthat pausing at the RFB sites was greatly reduced (Fig. 4C).

These experiments indicate that Tof1-Csm3 and Mrc1 are functionallydistinct, at least in the context of a paused DNA replicationfork (an enlarged version of the 60-min time point is shownin Figure 4D to illustrate the point more clearly). It was importantto confirm that the barrier was still intact in the absenceof Tof1 and Csm3, and we therefore used ChIP to show that Fob1still associated with the two RFB sites on chromosome 3 in thesestrains, just as in the control (Fig. 4E).

Previous work showed that progression of the replisome is uncoupledfrom DNA synthesis at HU-stalled forks in cells lacking Mrc1or Tof1 (Katou et al. 2003). It was possible, therefore, thatDNA synthesis might indeed be arrested at the RFB in cells lackingMrc1, as indicated by the 2D gels, but the replisome (or componentssuch as the MCM–Cdc45 helicase) may still progress beyondthe RFB. In this case, both Mrc1 and Tof1 would be importantto restrain progression of the replisome at a paused fork, justas at HU-stalled forks, but Tof1 (and Csm3) would have an additionalrole in restraining DNA synthesis, for example, by inhibitingprogression of a DNA polymerase. To test this possibility, weused ChIP to determine the behavior of Cdc45 in cells lackingeither Mrc1 or Tof1, and to aid the analysis we grew both strainsin parallel in the same experiment (Fig. 5). Thirty minutesafter release from G1 arrest, Cdc45 associated principally withARS305 and ARS306 but also associated with the sites $~$ 10 kb fromeach origin, and the observed pattern of localization was verysimilar in cells lacking either Mrc1 or Tof1. Fifteen minuteslater, however, the situation was very different in the twostrains: In cells lacking Mrc1, the sites close to the two RFBswere strongly enriched in the immunoprecipitate of Cdc45 (Fig. 5,mrc1 ${Delta}$ , sites 2 and 4); in the absence of Tof1, however, Cdc45did not accumulate at the RFB sites, and instead the site towardthe middle of the region was strongly enriched in the Cdc45immunoprecipitate (Fig. 5, tof1 ${Delta}$ , site 3). This experiment, togetherwith the 2D data described above, shows that progression ofthe replisome is still coupled to DNA synthesis in the mrc1 ${Delta}$ strain. Mrc1 is not essential, therefore, for the replisometo pause at the Fob1–RFB, in striking contrast to theimportant role played by Tof1.

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Figure 5. Pausing of the replisome at the RFBs on chromosome 3 is independent of Mrc1 but requires Tof1. The association of Cdc45 with the region between ARS305 and ARS306 was examined by ChIP at 30 min or 45 min after release of cells from G1 arrest.

We wanted to test whether the observations made at the RFBson chromosome 3 were also true for the endogenous RFB in therDNA repeats on chromosome 12. We therefore examined replicationof the rDNA repeats in the same experiments described above(the region of interest and the expected products in the 2Dgels are shown in Fig. 1A, panels i,iii [right]; SupplementaryFig. 1C). As shown in Figure 6, a strong spot on the Y-arc isobserved at the site of the RFB during replication of the rDNArepeats (Fig. 6A, panel i, Control), together with a "bubblearc" representing activation of the rDNA origin of replication.One or two vertical lines emerge from the RFB spot in the 2Dgels; such structures probably represent reversed forks or "chickenfeet" (Vengrova and Dalgaard 2004

) at each of the two adjacentpause sites within the RFB (Brewer et al. 1992

; Gruber et al.2000

). These structures are not detected at the RFB in vivo(Lucchini and Sogo 1994

) and may thus form in vitro during theisolation of genomic DNA containing DNA replication forks. Theyform in the absence of recombination (see Fig. 9C, below), andthe accumulation of forks at the unique RFB site within themultiple rDNA repeats may simply aid their detection.

In cells lacking Mrc1 or Tof1, replication of the rDNA occursover a shorter period, perhaps reflecting changes in originefficiency or copy number within the rDNA repeats; a similarthough milder effect is observed in the absence of Csm3 (Fig. 6A).The behavior of DNA replication forks at the RFB is strikinglydifferent, however, in the three strains. Forks still pausestrongly at the RFB within the rDNA in the absence of Mrc1 (Fig. 6A,panel i), as shown above for chromosome 3. Pausing at theRFB is greatly reduced in the absence of Tof1 or Csm3 and isassociated with weak pausing at a point beyond the normal RFBsite (Fig. 6B). This latter pause site is independent of Fob1(Supplementary Fig. 5), and may correspond to forks that clashwith 3' end of the 35S rRNA gene when pausing at the RFB isprevented, as reported previously (Takeuchi et al. 2003). Thebehavior of forks at the RFB within the rDNA repeats is thusstrikingly different in cells lacking either Mrc1 or Tof1-Csm3,consistent with our observations of individual forks that pauseat the RFBs on chromosome 3.

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Figure 6. (A) Mrc1 is not essential for DNA replication forks to pause at the endogenous RFB within the rDNA, but Tof1 and Csm3 are both important for pausing. (B) Larger versions of the data from the 45-min time point. The arrows mark the site where forks normally pause at the RFB (1), as well as a region beyond this point where weak pausing can be seen in the absence of Tof1 or Csm3 (2).

Pausing and recovery of eukaryotic forks without checkpoint kinases

When DNA replication forks stall in response to the depletionof nucleotides, checkpoint kinases such as the budding yeastproteins Mec1 and Rad53 are essential to preserve the integrityof the stalled fork, and thus ensure that replication can resumesubsequently (Lopes et al. 2001). As both Mec1 and Rad53 arealso essential for cell viability even in the absence of replicationstress, we examined cells lacking either kinase in additionto the Sml1 protein that inhibits ribonucleotide reductase (seeIntroduction). We first assayed the progression of forks fromARS305 and ARS306 in cells lacking Sml1. As shown in Figure 7A,both forks still paused at the corresponding RFB, just asin a wild-type strain. We then performed a similar experimentusing cells lacking both Mec1 and Sml1. Strikingly, replicationof the region between ARS305 and ARS306 was very similar tothe sml1 ${Delta}$ control: The forks from each origin paused at the correspondingbarrier as before, and DNA synthesis then resumed subsequently,so that replication of the region was completed (Fig. 7B, paneli). We also showed that the forks from ARS305 and ARS306 pauseand recover in a similar manner in cells lacking both Rad53and Sml1 (Fig. 7B, panel ii; note that the onset of S phaseis slightly advanced in this strain); moreover, neither Mec1nor Rad53 is essential for pausing or recovery of forks at theendogenous RFB within the rDNA (Fig. 8). We thus conclude thatthe integrity of forks that pause at the Fob1–RFB is independentof checkpoint kinases, contrasting once again with the regulationof HU-stalled forks.

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Figure 7. Stability of forks that pause at the RFBs on chromosome 3 does not require checkpoint kinases. Progression of forks was examined as before in sml1 ${Delta}$ (A), mec1 ${Delta}$ sml1 ${Delta}$ (B, panel i) or rad53 ${Delta}$ sml1 ${Delta}$ (B, panel ii) strains.

Recovery of paused forks at the Fob1–RFB without recombination

It has often been suggested that the pausing of DNA replicationforks may lead to breakage that is then repaired by homologousrecombination (Keil and McWilliams 1993; Ivessa et al. 2000,2002, 2003; Weitao et al. 2003; Ahn et al. 2005; Lambert etal. 2005; Prado and Aguilera 2005), but previous studies havenot established whether such events represent an important mechanismby which DNA synthesis normally resumes at paused forks in eukaryoticcells, or else result from rare failures to achieve recoveryby other means. By studying the kinetics of replication of individualreplicons that contain specific pause sites, we have shown thatforks from ARS305 and ARS306 pause for an extended period withan intact replisome at the RFB sites between the two origins,before DNA synthesis resumes at each fork and replication ofthe region is rapidly completed. Our data suggest, therefore,that DNA synthesis normally resumes without breakage or recombinationat the RFBs, and we have not observed recombination intermediatesat the paused forks on chromosome 3 (X-shaped molecules withdouble the DNA content of the unreplicated restriction fragment,which would have been seen in the 2D gels as a vertical lineemerging from the bottom-left corner of the Y-arc).

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Figure 8. Stability of paused forks at the RFB in the rDNA is independent of checkpoint kinases. (A) Progression of forks was examined as before in sml1 ${Delta}$ , mec1 ${Delta}$ sml1 ${Delta}$ , or rad53 ${Delta}$ sml1 ${Delta}$ strains. (B) Larger versions of individual time points are shown for the three strains.

The Rad52 protein is essential for practically all forms ofhomologous recombination in eukaryotic cells, including recombinationbetween the rDNA repeats (Gangloff et al. 1996

; Park et al.1999

; Ivessa et al. 2000

). Budding yeast cells lacking Rad52frequently become arrested at the G2/M phase of the cell cycleand are highly sensitive to the drug HU that causes DNA replicationforks to stall (Bennett et al. 2001

; Chang et al. 2002

; Shoret al. 2002

), probably reflecting a failure to repair double-strandbreaks in DNA that occur during chromosome replication. To examinethe importance of recombination in the resumption of DNA synthesisafter extended pausing of DNA replication forks at the RFBson chromosome 3, we measured the viability of cells lackingRad52 as they entered the cell cycle synchronously and replicatedtheir chromosomes, either in the presence or absence of extendedpausing of forks at the RFBs on chromosome 3.

As shown in Figure 9A, panel i, we only detected minor changesin the viability of rad52 ${Delta}$ cells throughout the experiment, regardlessof the presence or absence of RFBs on chromosome 3. Moreover,cells lacking Rad52 were able to form colonies just as wellin the presence of active barriers on chromosome 3 as in theirabsence (Fig. 9A, panel ii). We used 2D gels to confirm thatthe barriers were indeed active in the absence of Rad52, andas before, we saw that the forks from ARS305 and ARS306 pausedfor an extended period at the corresponding RFBs, before theresumption of DNA synthesis allowed replication of the interveningregion to be completed (Fig. 9B). We also examined the endogenousRFB in the rDNA in the same experiment, and found that the pausedforks behaved as in previous experiments (Fig. 9C; note thepresence of the "pointers" emerging from the RFB, which arethus formed independently of recombination). We therefore concludefrom these experiments that DNA synthesis at the paused forkscan normally resume without recombination, consistent with ourobservation of a stable replisome at the RFBs.

Discussion

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Discussion
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References

By introducing RFBs on chromosome 3 of budding yeast, we havegenerated a system that is ideal for studying the compositionand regulation of the replisome at individual paused eukaryoticDNA replication forks. The forks from ARS305 and ARS306 arriveat the corresponding RFBs with similar kinetics in each cellcycle and then pause for a greatly extended period, relativeto most other pause sites in the genome. Eventually, DNA synthesisresumes from each of the two paused forks, allowing us to studyboth the stability and recovery of paused replisomes, withoutthe arrival of a neighboring fork that would induce termination.Within the endogenous rDNA, however, origins tend to be activatedin small clusters of adjacent repeats, so that most forks thatpause at the RFBs are resolved after a relatively short periodby forks from neighboring repeats. The RFB system on chromosome3 is therefore ideally suited to the study of individual pausedreplisomes, in contrast to the highly repetitive rDNA, wherechanges in the copy number or frequency of origin activationcan also produce further complications.

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Figure 9. Recovery of DNA synthesis from forks paused at the Fob1–RFB does not require recombination. (A, panel i) Viability of the indicated strains was measured as cells were released from G1 phase in the presence of Fob1, as in previous experiments. DNA content was measured by flow cytometry. (Panel ii) Growth of cells lacking Rad52 is not affected by extended pausing of DNA replication forks at the RFBs on chromosome 3. Serial dilutions of cells were plated on YPD medium (inactive RFBs) and YPGal medium (active RFBs) and photographed after 48 h growth at 25°C. Note that yeast cells grow more slowly on YPGal medium. (B) Progression of DNA replication forks through the region between ARS305 and ARS306 was examined as before. (C) Replication of the rDNA repeats was examined in the same experiment.

Our study identifies both similarities and also important differencesbetween the replisomes associated with paused and stalled eukaryoticDNA replication forks. Our data indicate that many componentsof the replisome remain associated with the paused fork, justas when forks stall in response to the depletion of nucleotidesby HU treatment. We do not know whether the various componentsof the paused replisome associate with the fork in an uninterruptedfashion, or repeatedly disassociate and then rapidly reassociate,but it is clear that the replisome does not disassemble whena fork pauses at the Fob1–RFB. It is interesting thatDNA polymerase ${alpha}$ -primase remains associated with the paused fork,despite the fact that synthesis of the lagging-strand is likelyto be completed rapidly upon pausing (Gruber et al. 2000

). Itis also notable that the paused replisome retains the putativeMCM–Cdc45 helicase, as it has previously been shown thatthe removal of MCM2–7 proteins from HU-stalled DNA replicationforks blocks irreversibly the subsequent resumption of DNA synthesis(Labib et al. 2000

), suggesting that the MCM complex must bemaintained continuously at forks from initiation to termination;our observations of paused replisomes are consistent with thisidea. We note that our data also suggest that the MCM–Cdc45complex does indeed travel with DNA replication forks as partof the replisome, rather than functioning at a significant distanceaway from forks as recently suggested (Laskey and Madine 2003

Despite the association of both Mrc1 and Tof1 with paused DNAreplication forks, our data show that Mrc1 is dispensable forpausing to occur, whereas Tof1 is crucially important for efficientpausing of the replisome at a protein–DNA barrier, asis the associated protein Csm3. Previous studies showed thatboth Mrc1 and Tof1 are equally important to restrain the progressionof HU-stalled forks (Katou et al. 2003). The homolog of Mrc1in vertebrate cells, Claspin, is required for checkpoint activationto occur in response to the stalling of DNA replication forks(Kumagai and Dunphy 2000), and in budding yeast, it appearsthat both Mrc1 and Tof1 are important for checkpoint activationin response to HU-stalled DNA replication forks (Alcasabas etal. 2001; Foss 2001; Katou et al. 2003). It therefore seemsthat Mrc1 and Tof1 play a similar role in the regulation ofHU-stalled DNA replication forks. Our data identify an importantfunctional distinction between these proteins when DNA replicationforks pause at protein–DNA barriers. Although we cannotexclude that Mrc1 contributes to pausing in a manner that isredundant with Tof1-Csm3, the reverse is not true, and it isclear that Tof1 and Csm3 are both crucial for the efficientpausing of DNA replication forks at the Fob1–RFB, in contrastto Mrc1.

We have also shown that individual paused eukaryotic DNA replicationforks can recruit a protein that is not normally part of thereplisome. The Rrm3 helicase is important throughout the genometo help forks progress past protein–DNA barriers (Ivessaet al. 2003) and was shown previously by ChIP to associate withthe rDNA in asynchronous cultures of budding yeast cells (Ivessaet al. 2000), though the timing and site of recruitment werenot determined. By studying the kinetics of individual repliconscontaining RFBs, we have shown that Rrm3 is recruited specificallyto the individual paused replisomes on chromosome 3, and doesnot associate significantly with newly established forks atARS305 and ARS306. It is known that Rrm3 can interact with PCNA(Schmidt et al. 2002), which is loaded onto the lagging strandas a "sliding clamp" for DNA polymerase ${delta}$ during the synthesisof each Okazaki fragment. When synthesis of the lagging-strandis completed soon after pausing of a DNA replication fork ata protein–DNA barrier, PCNA on the newly completed laggingstrand may become available for interaction with other proteinssuch as Rrm3, which can thus gain access to the paused fork.It is interesting to note that the Rrm3 helicase moves alongDNA with a 5'–3' polarity (Ivessa et al. 2002), contrastingwith the 3'–5' polarity proposed for the MCM helicase(Ishimi 1997; Kelman et al. 1999; Chong et al. 2000; Shechteret al. 2000; Lee and Hurwitz 2001; Kaplan et al. 2003). Althoughthe mechanism of the putative MCM–Cdc45 helicase has yetto be resolved, one attractive possibility would be that theMCM–Cdc45 helicase moves 3'–5' along the templateof the leading strand and then pauses upon encountering theFob1–RFB, until Rrm3 loads onto the template of the laggingstrand and unwinds the RFB 5'–3', thus displacing Fob1transiently and allowing progression of MCM–Cdc45 to continue(Fig. 10).

It is also clear that HU-stalled forks recruit specific proteinsthat are not normally part of the replisome, analogous to ourfinding that Rrm3 is specifically recruited to paused forksat the Fob1–RFB. These include the checkpoint kinase complexMec1–Ddc2 (Katou et al. 2003; Osborn and Elledge 2003;Lucca et al. 2004), which together with Rad53 is essential tomaintain the integrity of the stalled fork and prevent disassemblyof the stalled replisome (Lopes et al. 2001; Cobb et al. 2004).We have shown that these checkpoint kinases are not requiredto preserve the integrity of forks that pause for prolongedperiods at the Fob1–RFB, further highlighting the differencesin regulation between paused and stalled forks. Although themechanism by which Mec1 and Rad53 stabilize stalled forks isnot understood, it has been suggested that these kinases arerequired to prevent breakage occurring due to the exposure oflong regions of single-strand DNA at DNA replication forks (Lopeset al. 2001; Sogo et al. 2002). As a paused fork will rapidlybecome double stranded except at the junction with the parentalduplex, the fork and its associated replisome may simply beinherently stable and thus would not require checkpoint kinasesto preserve their integrity. Alternatively, the stability ofpaused forks may be maintained by another mechanism that remainsto be identified.

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Figure 10. A model for the pausing and recovery of DNA replication forks at a protein–DNA barrier; see text for details.

When forks pause for an extended period at the Fob1–RFB,we have shown that the resumption of DNA synthesis does notnormally require recombination, indicating that breakage ofsuch paused forks does not occur commonly. It has been shownpreviously, however, that recombination levels are increasedin the absence of the Rrm3 helicase (Keil and McWilliams 1993

;Ivessa et al. 2000

, 2002

, 2003

), indicating that increased pausingof DNA replication forks may provide an important source ofgenomic instability. Recent studies have demonstrated that pausingof forks at specific loci does indeed promote an increased rateof Rad52-dependent recombination events (Ahn et al. 2005

; Lambertet al. 2005

; Prado and Aguilera 2005

), again supporting theidea that the pausing of forks may contribute to breakage andrecombination. Our data do not contradict this possibility butinstead indicate that DNA synthesis normally resumes from pausedforks without breakage and recombination, as the replisome atthe Fob1–RFB is generally stable even after extended pausing,so that breakage events are likely to be relatively rare. TheFob1 protein can indeed promote recombination between sequencesthat are derived from the rDNA, but it is interesting to notethat this requires RNA PolI transcription (Keil and Roeder 1984

;Voelkel-Meiman et al. 1987

; Stewart and Roeder 1989

; Huang andKeil 1995

). Stimulation of recombination under such conditionsdoes not correlate with the pausing of DNA replication forksat the RFB (Ward et al. 2000

), and it is not known whether clashesbetween RNA PolI transcription and DNA replication forks arethe key to increased recombination in this case. It will beinteresting to determine in the future whether the majorityof paused eukaryotic replisomes resume synthesis subsequentlywithout breakage of the fork and so without recombination, assuggested by our analysis of the Fob1–RFB, or whethercertain kinds of barriers to the progression of DNA replicationforks are more likely to cause breakage than others.

It appears that active pausing of DNA replication forks at protein–DNAbarriers allows cells to couple DNA synthesis to other cellularprocesses. For example, mating type switching in fission yeastrequires the homologs of Tof1 and Csm3, in order for a specificDNA replication fork to pause at a particular site and allowthe establishment of a genomic imprint (Dalgaard and Klar 1999,2000; Kaykov and Arcangioli 2004; Vengrova and Dalgaard 2004).It is interesting to note that the fission yeast mrc1 gene wasnot isolated in the original screen for mutations causing defectsin mating type switching, despite the isolation of several allelesof swi1 and swi3 (Egel et al. 1984), consistent with our findingthat Mrc1 is not essential for the pausing of DNA replicationforks at a protein–DNA barrier in budding yeast. It willbe interesting in the future to investigate the roles of homologsof Mrc1, Tof1, and Csm3 in the pausing of DNA replication forksat protein–DNA barriers in higher eukaryotes.

Materials and methods

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Yeast growth

All our budding yeast strains are based on the "W303" geneticbackground. Cells were grown at 24°C in YP medium (1% yeastextract [Difco], 2% peptone [Oxoid]) supplemented with 2% glucose(YPD), 2% raffinose (YPRaff), or 2% galactose (YPGal). To synchronizecells in the G1 phase of the cell cycle, ${alpha}$ -factor mating pheromonewas added to a final concentration of 7.5 µg/mL for onegeneration time. To induce expression from the GAL1,10 promoter,cells were grown in YPRaff medium and then centrifuged beforeresuspending in YPGal medium for 45 min.

Construction of a yeast strain with RFBs on chromosome 3

We used PCR to amplify from yeast genomic DNA a 450-bp fragmentcontaining the RFB from the rDNA repeats, corresponding to nucleotides460470–460919 of chromosome 12, preceded by a BamHI siteand followed by a SmaI site. We then generated the plasmid pBH3by inserting the SmaI–BamHI RFB fragment into the plasmidpRS306 (Sikorski and Hieter 1989), adjacent to an XhoI–SmaIfragment containing the budding yeast LEU2 gene. We made theplasmid pBH7 in an analogous fashion by inserting the SmaI–BamHIRFB fragment into the plasmid pRS305 (Sikorski and Hieter 1989),adjacent to an XhoI–SmaI fragment containing the buddingyeast URA3 gene. We used pBH7 and pBH3 to replace nucleotides48540–48608 of chromosome 3 with RFB-URA3 and nucleotides64547–64642 with LEU2-RFB, as described in the legendfor Supplementary Figure 1. We used PCR and Southern blottingto confirm that the correct integrations had indeed occurredin the resultant yeast strain, YBH17.

Two-dimensional DNA gels

DNA samples for 2D neutral-neutral gel electrophoresis wereprepared and analyzed as described previously (Friedman andBrewer 1995; Lopes et al. 2001); DNA was digested with the restrictionenzymes BclI and SalI and detected using the probes indicatedin Supplementary Figure 1B. Gels for the first dimension hadan agarose concentration of 0.4% and were run for 38 h at 0.7V/cm; gels for the second dimension had an agarose concentrationof 1% and were run for 8 h at 5 V/cm. To quantify the pausingof forks at the RFBs in our experiments, we measured the signalcorresponding to the "RFB spot" and the "linear spot" (see Fig. 1)using a Storm 860 PhosphorImager (Molecular Dynamics) andImageQuant 5.1 software; the RFB signal was then expressed asa proportion of the linear signal, and the ratio denoted "pausedforks/relative units".

Tagging yeast proteins with multiple copies of the c-myc epitope

We used a "one-step PCR" approach (Knop et al. 1999) to introducemultiple copies of the c-myc or Flag epitopes at the C terminusof yeast proteins in the diploid strain W303-1. The correctintegrations were confirmed by PCR and by immunoblotting withthe anti-myc antibody 9E11 (Neomarkers "c-myc Ab-1") or theanti-Flag antibody M2 (Sigma), and diploid colonies were thensporulated and tetrad analysis performed in order to isolatethe corresponding haploids.

ChIP

We performed ChIP experiments as described previously (Kamimuraet al. 2001), except that the immunoprecipitated DNA was purifiedusing the Qiagen PCR purification kit instead of Phenol/Chloroform/Iso-amylalcohol. In all experiments except that described in Figure 3B,we performed two immunoprecipitations for each cell extract:one using the mouse monoclonal antibodies 9E11 or M2 that recognizethe c-myc or Flag epitopes attached to the target protein, anda second using an equivalent mouse monoclonal antibody, 12CA5,which served as a negative control. For the experiment in Figure 3B,we used 9E11, M2, and 12CA5 to perform three immunoprecipitations.We used real-time PCR to quantify for each immunoprecipitatethe amount of DNA corresponding to the specific genomic locishown in Supplementary Figure 5. We set up 25 µL PCR reactionscontaining 1 µL purified DNA from a particular immunoprecipitate,1.125 µL 10 µM 5' oligonucleotide primer, 1.125µL 10 µM 3' oligonucleotide primer, 1 µL 5µM FAM-TAMRA Taqman probe (synthesised by ABI), 12.5 µL2x Taqman reaction mix (ABI), and 8 µL dH₂0. Reactionswere analyzed using an ABI 7900 thermal cycler according tothe manufacturer's instructions. We performed two independentduplicates of each PCR reaction and calculated the mean "thresholdcycle number" (or Ct value). The specific enrichment of thetarget protein for a particular sample was calculated usingthe following formula: specific enrichment = 2^{(Ct12CA5 –Ct 9E11/M2)}, where Ct 12CA5 is the Ct value for the controlimmunoprecipitate, and Ct 9E11/M2 is the Ct value for the 9E11or M2 immunoprecipitate. The specific enrichments for each timepoint were then normalized relative to the lowest backgroundvalue observed in G1-arrested cells for nonorigin sequences,which was determined in each experiment (except those in Figs.3B, 5, where the number of samples precluded analysis of G1cells—we thus did not normalize these data). On each occasion,we also performed two control PCR reactions: a negative controlwithout input DNA and a positive control using genomic DNA purifiedfrom the corresponding cell extract.

Acknowledgments

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We thank members of our groups for helpful discussions, MarcoFoiani for his 2D gel protocol, and Aloys Schepers for adviceconcerningreal-time PCR. This work was funded by Cancer Research U.K.,from whom K.L. receives a Senior Cancer Research Fellowship,and by the Instituto de Salud Carlos III (F.I.S. grant no. 03-1255),together with a PGC grant awarded to A.B. by the Spanish scienceministry. K.L. is supported by the EMBO Young Investigator program,and A.C. received a short-term fellowship from EMBO and is supportedby the Sistema Nacional de Salud (grant no. 02-3059). M.K. isfunded by a JSPS Post-Doctoral Fellowship for Research Abroad.

Footnotes

Supplemental material is available at http://www.genesdev.org.

Article and publication are at http://www.genesdev.org/cgi/doi/10.1101/gad.337205.

³ These authors contributed equally to this work.

⁴ Corresponding author.

E-MAIL klabib{at}picr.man.ac.uk; FAX 44-161-446-3109.

References

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Materials and methods
Acknowledgments
References

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