Nucleic Acids Research

Nucleic Acids Research Advance Access originally published online on August 25, 2006
Nucleic Acids Research 2006 34(15):4138-4146; doi:10.1093/nar/gkl528

This Article Abstract Print PDF (293K) Screen PDF (296K) OA All Versions of this Article: 34/15/4138    most recent gkl528v1 Alert me when this article is cited Alert me if a correction is posted Services Email this article to a friend Similar articles in this journal Similar articles in ISI Web of Science Similar articles in PubMed Alert me to new issues of the journal Add to My Personal Archive Download to citation manager Search for citing articles in: ISI Web of Science (3) Commercial Re-use Guidelines for Open Access NAR Content Google Scholar Articles by Nedelcheva-Veleva, M. N. Articles by Stoynov, S. S. Search for Related Content PubMed PubMed Citation Articles by Nedelcheva-Veleva, M. N. Articles by Stoynov, S. S. Social Bookmarking          What's this?

Nucleic Acids Research, 2006, Vol. 34, No. 15 4138-4146
© 2006 The Author(s)
This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/2.0/uk/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Survey and Summary

Coordination of DNA synthesis and replicative unwinding by the S-phase checkpoint pathways

Marina N. Nedelcheva-Veleva, Dragomir B. Krastev and Stoyno S. Stoynov^*

Institute of Molecular Biology, Bulgarian Academy of Sciences 21 G. Bonchev Strasse Sofia 1113, Bulgaria

^*To whom correspondence should be addressed. Tel: +359 979 36 89; Fax: +359 2 72 25 077; Email: stoynov{at}obzor.bio21.bas.bg

Received May 14, 2006. Revised July 8, 2006. Accepted July 10, 2006.

	ABSTRACT

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
The process of DNA replication includes duplex unwinding, followed immediately by DNA synthesis. In eukaryotes, DNA synthesis is disturbed in damaged DNA regions, in replication slow zones, or as a result of insufficient nucleotide level. This review aims to discuss the mechanisms that coordinate DNA unwinding and synthesis, allowing replication to be completed even in the presence of genomic insults. There is a growing body of evidence which suggests that S-phase checkpoint pathways regulate both replicative unwinding and DNA synthesis, to synchronize the two processes, thus ensuring genome stability.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
Fine coordination of several individual processes during DNA replication is required for correct duplication of genetic information and maintenance of genome stability. Recent studies of the physical and functional interaction at replication forks have shed light on the synchronization between DNA synthesis and replicative unwinding.

The MCM heterohexameric helicase complex is essential for DNA unwinding during both the initiation and elongation steps of DNA replication (1). Several regulatory proteins—Cdc45 (2), Mrc1, Tof1, Csm3 (3) and GINS (4) complex interact with MCM. The binding of the DNA polymerization machinery to the origin of DNA replication requires the pre-loading of MCM complex and its associated factors Cdc45 and GINS, by the ORC/Cdc6/Cdt1 initiation apparatus (5–9), but the exact mechanism by which this is accomplished is still unclear. It was demonstrated that polymerase is the first DNA polymerase, which is bound at the origins of DNA replication and is required for polymerase /primase association with these origins (10,11). The order of polymerase loading is surprising in view of the fact that the DNA synthesis by polymerase requires synthesis of a RNA/DNA primer by polymerase /primase (12).

Several other proteins are necessary for initiation of DNA replication. Dpb11/Sld2 interaction with polymerase is involved in binding of polymerases to the origin of replication (10,13). In addition, MCM10 is required to load polymerase /primase onto the replication forks (14). After the binding of polymerase , the four subunit polymerase /primase complex creates a short RNA/DNA primer as a first step in DNA synthesis of both the leading and lagging strands (15). This primer is then utilized by the PCNA bound polymerase for processive elongation of the two strands (15,16). The loading of the sliding clamp PCNA onto the RNA/DNA primer, by the clamp loader protein complex RF-C, catalyses the switch between polymerase and the polymerase (17). In contrast to polymerase , polymerase is a highly processive polymerase without PCNA (18). Interaction of polymerase with GINS complex greatly stimulates its catalytic activity in vitro (19). Although the precise role of polymerase in vivo is still unclear, several findings suggest its catalytic role during DNA replication. Polymerase is associated with replication forks during S phase (5,11) and abolishment of its polymerase activity, displays a defect in the elongation step of chromosomal DNA replication (20). However, the catalytic activity of polymerase is not required for cell viability, which implies an other important function of this protein (21,22).

It was shown that both polymerase (23) and polymerase (24) complexes form dimers. Although the precise role of this dimerization remains to be determined, it is thought to play an essential role in the physical connection between the synthesizing machinery of both strands.

	STRUCTURAL AND FUNCTIONAL INTERACTION BETWEEN DNA UNWINDING AND POLYMERASE MACHINERY

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
It is still unclear whether DNA unwinding and polymerase machinery physically interact with each other. The essential methodological problem is that both helicase and DNA polymerases are DNA motor protein complexes therefore, co-purification of their subunits could be either an artefact of their binding to DNA, or a result of specific protein–protein interactions. The absence of co-purification after treatment of DNA with DNAse or ethidium bromide can be interpreted in two ways, either that the polymerase and helicase complexes do not interact with each other, or that their protein–protein interaction requires them to bind to DNA. Despite the difficulties in explaining the co-purification results, several findings suggest that there is a physical interaction between DNA polymerase complexes and replicative unwinding machinery. It was shown that in addition to co-precipitation with MCM helicase (4), GINS proteins form a complex with DNA polymerase epsilon holoenzyme in stoichiometric amounts in vitro (19). It has been established that Cdc45 co-precipitates not only with MCM helicase, but also polymerase (2). Finally, the MCM complex and the replicative polymerases simultaneously become uncoupled from the inhibited DNA synthesis, in Mrc1 and Tof1 deficient cells (25). However, this raises the question as to whether the protein–protein interactions between DNA polymerase and replicative helicase complexes are sufficient to ensure the coupling of DNA synthesis and replicative unwinding? The flexibility of the ssDNA makes possible the uncoupling of the replicative unwinding and the disturbed DNA synthesis even if the helicase and the polymerase are physically connected (Figure 1C). The estimated persistence length of the single stranded DNA, defined as the length at which DNA is capable of bending significantly in two independent directions, ranges from 1.5 to 3 nm (26–28). This means that beyond 5–9 bases ssDNA length of the elastic cost of ssDNA bending is totally negligible.

View larger version (49K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 1 Regulation of DNA synthesis by Mec1-checkpoint pathway. (A) Replication fork during unperturbed DNA replication. (B) Regulation of DNA synthesis and replicative unwinding when DNA synthesis is disturbed. (C) The presence of extensive single stranded loops in mrc1, csm3 and tof1 mutants impeding the passage through a cohesin ring and the establishment of sister chromatid cohesion.

 
During normal replication, leading strand DNA synthesis immediately follows replicative unwinding (Figure 1A), which is visualized as a fork branch structure by two-dimensional agarose gel electrophoresis. It was observed that single-stranded DNA (ssDNA) at replication forks is 200 bp long, most probably as a result of its engagement with replisome (29). When replication forks stall at replication slow zones, damaged DNA regions, or are inhibited by hydroxyurea (HU), yeast cells activate the Mec1-dependent checkpoint pathway (30). This process stabilizes the replication complex to facilitate the re-establishment of fork progression after the stress has been removed (31,32). The best known difference between stalled and normal replication forks is an increase in the single-stranded gap. When the movement of the fork is arrested by HU, the ssDNA region becomes approximately 400 nucleotides long (29). When DNA synthesis is arrested by HU in checkpoint deficient yeast strains, much longer ssDNA regions accumulate (29). All these findings suggest that the Mec1-checkpoint pathway could cause DNA synthesis and replicative unwinding to couple in budding yeast.

	MEC1-REPLICATION CHECKPOINT PATHWAY

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
Mec1 is a member of the phosphoinositide-3-kinases (PIKKs) and is an essential component of the replication checkpoint pathway (30,33–35) in budding yeast. Mec1, in complex with Ddc2 (36,37), recognizes ssDNA coated by replication protein A (RPA) (38,39). The recruitment of Mec1-Ddc2 to the replication intermediates, containing ssDNA regions, is required to activate replication and DNA damage checkpoints.

Other essential players in these checkpoints are the Mrc1, Tof1 and Csm3 budding yeast proteins (40–44) which form a three-protein complex (3). These three proteins co-localize with both normal and stalled replication forks (25,45), all of which are required to slow down DNA replication, for full activation of Rad53 either in response to reduced levels of dNTPs, or to DNA damage (42,45–47). The phosphorylation and activation of Rad53 in a Mec1-dependent manner, leads to the stabilization of stalled replication forks, inhibition of late origin firing and a delay in S/M-phase cell cycle transition (48). The activation of Rad53, in response to inhibition of DNA synthesis by HU, requires Mrc1 phosphorylation by Mec1 (45,49).

	MEC1-CHECKPOINT PATHWAY REGULATION OF DNA UNWINDING

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
Several recent findings suggest that Tof1, Csm3 and Mrc1 are required to regulate replicative unwinding by the Mec1-checkpoint pathway.

When synthesis is inhibited by HU, deletions of Mrc1, or Tof1, lead to the uncoupling of Cdc45, MCM complex and replicative polymerases from DNA synthesis (25). Tof1, Csm3 and Mrc1 checkpoint proteins interact with different subunits of the MCM helicase complex (3). In addition, the synthetic lethality of the double mutants, carrying deletions in tof1, csm3 or mrc1 and temperature-sensitive mutations in one of the polymerase /primase subunit genes, suggests that the Mrc1/Tof1/Csm3 checkpoint complex, can prevent the lethality of cells in which DNA unwinding can proceed without synthesis (3). Recently, it was found that the metazoan Mec1 homolog, the ATR kinase, directly phosphorylates the subunits of the MCM helicase complex. It was observed that the ATR phosphorylates the Mcm2 subunit in human and Xenopus, in response to DNA damage and stalled replication forks (50,51). In addition, ATR-interacting protein ATRIP, homologous to budding yeast Ddc2, directly interacts with the Mcm7 (50). ATM, the other metazoan phosphoinositide-3-kinase, required for the activation of the replication and DNA damage checkpoint, phosphorylates Mcm3, as a result of ionizing irradiation (50). Finally, Mcm4 is extensively phosphorylated in HeLa cells when they are incubated in the presence of inhibitors of DNA synthesis or are exposed to UV irradiation (52). Apart from MCM complex, ATR/ATRIP directly interacts with the Timeless protein, human homolog of Tof1 (53). How the interactions between ATR/ATRIP, MCM and Mrc1/Tof1/Csm3 complexes and ATR/ATM phosphorylations of Mrc1 and MCM contribute to the stalling of the replication fork is still unclear. It was shown that the deletion of mrc1 or tof1 is sufficient for the uncoupling of Cdc45 and the MCM complex from DNA synthesis during HU arrest (25). In the double mec1/tel1 deletion mutant the co-factor of MCM helicase Cdc45 almost disappears from DNA during HU arrest, indicating a more profound effect of this mutant in the stalling of replication forks (25).

	MODELS FOR REGULATION OF DNA UNWINDING BY THE MEC-DEPENDANT CHECKPOINT MECHANISM

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
The above findings suggest possible mechanisms for the regulation of replicative unwinding when synthesis is disturbed. Pausing of DNA synthesis in response to a decrease in nucleotide levels, or DNA damage (thymine dimers, photo adducts, alkylated bases, etc.), leads to an accumulation of ssDNA regions as a result of the uncoupling of DNA unwinding from synthesis (Figure 1B). RPA mediates Mec1-Ddc2 binding to the single-stranded regions (39), and allows Mec1 to interact with and phosphorylate MCM complex and Mrc1/Tof1/Csm3. These interactions could change the binding of Mrc1/Tof1/Csm3 to MCM complex and inhibit the helicase activity of the latter. The ability of Mrc1 of Schizosaccharomyces pombe and claspin (the human homolog of Mrc1) to bind DNA in vitro could play an important role for inhibition of the helicase movement (54,55).

In eukaryotes, replication forks also stall at natural site-specific sequences, called ‘replication fork barriers’. These sites cause polar fork arrest, which is required for various cellular events, including mating-type switching in S.pombe (56) and extrachromosomal ribosomal circle DNA formation in eukaryotes (57,58).

It is interesting that Swi1 and Swi3 (the S.pombe's homologs of Tof1 and Csm3), but not Mrc1, are required for stalling of replication forks at five out of six yeast fission replication fork barriers (58,59). Mrc1 is also not required for the stalling of replication forks at the replication fork barriers in budding yeast (60). In this case, Mrc1 could be replaced in Tof1/Csm3 complex by another protein, such as Fob 1 in budding yeast (61) and Reb1 in S.pombe (62). These proteins bind to the replication fork barrier at the ribosomal locus, which is required for replication fork stalling at this sequence.

Apart from the uncoupling of Cdc45, MCM and DNA polymerases from disturbed DNA synthesis, deletion mutants of MRC1 or TOF1 express two additional phenotypes. Mrc1, csm3 and tof1 mutants exhibit mild defects in sister chromatid cohesion (63–65) and slow down the unperturbed DNA replication in Tof1 and Mrc1 deletion cells (45,66,67). It is still unknown, whether these phenotypes are due to the separate function of Tof1/Csm3/Mrc1 or are a consequence of the uncoupling of DNA synthesis and replicative unwinding. The relationship between the processes of replication and sister chromatid cohesion provides possible explanation for these two phenotypes. If the helicase and the polymerase complexes physically interact with each other, then, uncoupling of DNA synthesis and unwinding in Tof1/Csm3/Mrc1 deficient cells will generate single-stranded loops (Figure 1C). Generation of such loops would hinder sister chromatid cohesion. According to one of the proposed models, supported by Nasmyth's results, cohesion is established by the cohesin rings (68), which encircle the two sister chromatids (69). These rings are loaded onto DNA during S phase. The passage of the replication fork through a cohesion ring is supposed to ensure the cohesion of the two newly synthesized DNA strands. In our opinion the presence of extensive single stranded loops, in mrc1, csm3 and tof1 mutants, would impede the passage through a cohesin ring and the establishment of sister chromatid cohesion (Figure 1C). Difficulties in passing through these loops could also explain slower DNA replication in Tof1 and Mrc1 deletion cells (45,66,67).

	REGULATION OF DNA SYNTHESIS BY THE MEC1-CHECKPOINT PATHWAY

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
The Mec1-checkpoint pathway not only regulates the activity of the MCM helicase, but also controls DNA synthesis. It has been shown that the Mec1/Rad53-pathway increases the level of nucleotides during S-phase and in response to DNA damage (70). Cells deficient in Mec1 activity exhibit a 25% reduction in the level of dNTPs. The ribonucleotide reductase (RNR) catalyzes the synthesis of dNDPs from NDPs (71). In response to DNA damage, Mec1 activates the Dun1 kinase, that leads to the transcriptional induction of RNR (72,73) and the inhibition of its repressor Sml1 (74), thus increasing dNTP level. It appears that higher levels of dNTPs help the polymerase machinery to replicate replication slow zones and damaged DNA regions faster and more effectively.

All these results suggest that when synthesis is delayed by DNA lesions, the S phase checkpoint pathways both stall replicative unwinding and increase level of DNA synthesis, synchronizing the two processes. Synchronization of DNA synthesis and unwinding by the Mec1 pathway could explain the Mec1 mutant phenomena. Mec1-deficient cells die as a result of generation of double-stranded breaks in the replication slow zones (75). This lethality is suppressed by additional deletion of sml1, which increases nucleotide level. Both, the slowing of DNA synthesis and the uncoupling of the MCM helicase in Mec1-deficient cells, lead to generation of ssDNA at the replication slow zones. The instability of ssDNA leads to generation of double-stranded breaks and cell death.

	UNWINDING OF DNA, CONTAINING SINGLE-STRANDED REGIONS, ACCORDING TO THE VARIOUS MECHANISMS FOR HELICASE ACTION

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
What happens when the replicative helicase unwinds DNA containing a single-stranded gap or nick? Such sites are frequently generated during both nucleotide and base excision repair or ionizing radiation. The continued replication of such a DNA template would lead to the generation of a double-stranded break in one of the newly synthesized DNA molecules, which is the worst possible scenario for the cell. It is interesting to know how the replicative DNA helicases unwind DNA containing a single-stranded break, according to the different suggested models for helicase action.

In the ‘wedge model’, also referred as to the ‘steric-exclusion model’ (Figure 2A), one of the separated strands tightly binds to the central helicase channel. The helicase moves unidirectionally along the strand bound to its central channel, and the movement provides sufficient force to enable the helicase to destabilize the base pairs at the DNA duplex junction (76). When a helicase, functioning in this way, encounters a single-stranded break, the break is transformed into a double-stranded break, in one of the daughter DNA molecules (Figure 2B and C). When the ssDNA break has occurred on the strand where the helicase is moving, the helicase is unloaded from DNA (Figure 2B).

View larger version (50K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 2 Unwinding of DNA containing ssDNA break according to the ‘wedge’ and ‘ploughshare’ model. (A) DNA unwinding, according to the ‘wedge’ model. (B) Unwinding of DNA, containing ssDNA break at strand where the helicase is moving, according to the ‘wedge’ model. (C) Unwinding of DNA, containing single-stranded break at the opposite DNA strand according to the ‘wedge’ model. (D) Mechanism for DNA unwinding based on the ‘ploughshare’ model.

 
Recently a variant of the wedge model was proposed, that was referred to as the ‘ploughshare model’ (77). It was postulated that the MCM complex translocates along duplex DNA and that strand separation is achieved by a protein that sterically separates the two strands after they exit from the helicase (Figure 2D). When a ‘ploughshare’ type helicase encounters a single-stranded break, this break will be transformed into a double-stranded break in one of the daughter DNA molecules; however, the helicase will not be unloaded from DNA.

In the ‘torsional model’, the two strands are tightly bound to the central helicase channel (76). By rotating the two strands with respect to each other, the helicase generates negative superhelical stress that destabilizes the duplex DNA (Figure 3A). The passage of helicase through a single-stranded break would lead to relaxation of the negative superhelical stress behind the ssDNA region. Therefore, the DNA helix cannot be unwound (Figure 3B), and the replication fork would stall without generation of a double-stranded break in the daughter DNA and unloading of the MCM helicase. The maintenance of the MCM helicase on DNA is important since, until now, the re-loading mechanism of MCM onto DNA during S-phase has not been detected.

View larger version (51K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 3 Unwinding of DNA containing ssDNA break according to the ‘torsional’ model. (A) Mechanism for DNA unwinding based on the ‘torsional’ model. (B) DNA unwinding when there is an ssDNA break, according to the ‘torsional’ model. (C and D) Origin DNA unwinding and loading of polymerase /primase according to the ‘torsional’ model.

 
The torsional model of DNA unwinding requires superhelical tension to be preserved in the region, between the replicative helicase and the polymerase complexes. The dimerization of the leading and lagging strand polymerase (or polymerase ) complex and its binding to the MCM via GINS (4,19) and Cdc45 (2,4) can ensure a topologically independent DNA region between them, for the preservation of negative supercoiling (Figure 3A). Several findings indirectly support such a structural role of the polymerase . The C-terminal part of the catalytic subunit of polymerase , which is responsible for its dimerization but not for polymerase activity, is essential for cell viability (21,22). Polymerase loading at the origins of DNA replication is required for polymerase /primase association with these fragments (10,11), which suggests its role in the unwinding at the origin of DNA, to ensure a template for synthesis of RNA/DNA primer (Figure 3C and D).

In a third model, named the ‘rotary pump model’, two MCM complexes, located at a distance from each other, pump DNA in opposite directions (78). According to this model, the generated superhelical stress would unwind DNA between the two MCM hexamers (Figure 4A). The MCM helicase has to be immobilized, to induce enough torsional stress to unwind the DNA. Introduction of a single-stranded break in that region could lead to a relaxation of the negative superhelical stress, thus preventing DNA unwinding and the generation of a double-stranded break (Figure 4B). Recently, it was shown that the helicase complexes in vertebrates are detected at the replication fork (79), which is not easily explained by rotary pump unwinding at a distance. In a variant of the ‘rotary pump model’, two hexamer helicases are not located on distance but are bound to each other to pump DNA in opposite directions (80). This model is supported by the double hexameric structure of SV40 T-antigen replicative helicase (81,82). Archaeal MCM complex also forms a double hexamer (83,84). The binding of the two hexamers, could induce sufficient torsional stress for DNA unwinding (Figure 4C and D). In contrast to SV40, T-antigen and archaeal MCM complex, recent experiments suggest that metazoan MCM complex is a monomer on the replication fork (4). It is interesting that the capability of SV40 T-antigen to maintain torsional tension by its double hexamer organization makes the structural role of polymerase unnecessary. In fact, polymerase is not required for SV40 T-antigen dependent DNA replication (85,86).

View larger version (40K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 4 Unwinding of DNA containing ssDNA break according to the ‘rotary pump’ model. (A). DNA unwinding, according to the ‘rotary pump’ model. (B) Unwinding of DNA, containing ssDNA break based on the ‘rotary pump’ model. (C) Mechanism for DNA unwinding based on the ‘SV40’ model. (D) Unwinding of DNA, containing single-stranded DNA break based on the ‘SV40’ model.

 
Currently, there are no efficient experimental systems for the investigation of the unwinding of DNA containing a single stranded break. The inhibition of topoisomerase I leads to an accumulation of single-stranded breaks in DNA (87). However, in this case the end of the single-stranded break becomes covalently linked to the Topoisomerase I (87) molecule. This makes it impossible to determine whether the experimental results are a consequence of the single-stranded break or of the covalently bound protein. A promising model for ascertaining the true mechanism of DNA unwinding, is the mating-type switching in S.pombe. Mating-type switching occurs when the mat1 allele is replaced with the opposite mating-type allele by recombination with one of the two transcriptionally silent donor cassettes mat2P or mat3M (88,89). Mating-type switching is a process that requires two rounds of DNA replication. During the first round, a stable single-stranded imprint is made at the mat1 locus that remains in the DNA throughout the next cell cycle. During the following round of DNA replication, the replisome encounters the imprint, which leads to recombination and mating-type switching. Recent studies suggest that the imprint at mat1 is either a ssDNA break (90,91) or an alkali–labile DNA modification (92–94). Using the mating-type switching for investigation of the DNA unwinding mechanism requires clarification as to whether the imprint is a single stranded DNA break.

	REPLICATIVE DNA UNWINDING IN XENOPUS EMBRYONIC CELLS

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 
Whether the ATR- (Mec1-) checkpoint pathway coordinates the replicative unwinding and DNA synthesis in all eukaryotic cells is still unclear. It is known that SV40 T-antigen unwinds DNA in vivo when DNA synthesis is inhibited (95). This could be explained by the fact that SV40 virus T-antigen helicase is not under the control of the host Mec-1 checkpoint pathway. This is not the case with Xenopus and sea urchin embryos. In their cells, few if, any replication forks were observed (96,97). Instead, unbranched DNA that was suggested to be single-stranded, was abundant during the S-phase (96,97). This phenomenon is difficult to explain in terms of coupling of replicative unwinding and DNA synthesis. In the Xenopus egg extract, plasmid DNA was completely unwound when DNA synthesis was inhibited either by aphidicolin (98) and cis-platinum treatment or by UV irradiation (99); however, the replicative checkpoint in this extract seems to be at least partially active. Claspin and Chk1 proteins are phosphorylated by ATR, when DNA synthesis is inhibited (47,100). The phosphorylation of Chk1 requires DNA to be unwound to allow ATR-ATRIR to bind ssDNA via the RPA proteins (99). In addition, as indicated above, ATR directly phosphorylates the MCM helicase as a result of checkpoint activation (50,51). Why the ATR phosphorylation of MCM, claspin and Chk1 delays mitosis, but does not slow down the replicative unwinding in Xenopus embryos is still unclear. One possible reason could be in Tof1 and Csm3 homologs which have not been identified at the replication forks in the Xenopus egg extract.

Finally, we can conclude that coordination of unwinding and DNA synthesis by the S-phase checkpoint pathway is required for correct DNA replication and the maintenance of genome stability. Future investigations will reveal in detail the intimate mechanisms that lead to regulation of the MCM replication fork stalling activity.

	ACKNOWLEDGEMENTS

 
The authors would like to thank Atanas Gospodinov, Anna Ivanova and Rayna Kraeva for critical reading of the manuscript. The research of S.S.S. has been supported by an Alexander von Humboldt Foundation Return Fellowship and HATO Grant EAP.RIG.981642. This work was also funded by the National Science Fund of the Bulgarian Ministry of Education and Science under contracts K 1306/03 and MY- 1507. The Open Access publication charges for this article were waived by Oxford University Press.

Conflict of interest statement. None declared.

	REFERENCES

TOP ABSTRACT INTRODUCTION STRUCTURAL AND FUNCTIONAL... MEC1-REPLICATION CHECKPOINT... MEC1-CHECKPOINT PATHWAY... MODELS FOR REGULATION OF... REGULATION OF DNA SYNTHESIS... UNWINDING OF DNA, CONTAINING... REPLICATIVE DNA UNWINDING IN... REFERENCES

 

1. Tye, B.K. (1999) MCM proteins in DNA replication Annu. Rev. Biochem, . 68, 649–686[CrossRef][Web of Science][Medline] .

2. Zou, L. and Stillman, B. (2000) Assembly of a complex containing Cdc45p, replication protein A, and Mcm2p at replication origins controlled by S-phase cyclin-dependent kinases and Cdc7p-Dbf4p kinase Mol. Cell. Biol, . 20, 3086–3096[Abstract/Free Full Text] .

3. Nedelcheva, M.N., Roguev, A., Dolapchiev, L.B., Shevchenko, A., Taskov, H.B., Francis Stewart, A., Stoynov, S.S. (2005) Uncoupling of unwinding from DNA synthesis implies regulation of MCM helicase by Tof1/Mrc1/Csm3 checkpoint complex J. Mol. Biol, . 347, 509–521[CrossRef][Web of Science][Medline] .

4. Gambus, A., Jones, R.C., Sanchez-Diaz, A., Kanemaki, M., van Deursen, F., Edmondson, R.D., Labib, K. (2006) GINS maintains association of Cdc45 with MCM in replisome progression complexes at eukaryotic DNA replication forks Nature Cell. Biol, .

5. Aparicio, O.M., Weinstein, D.M., Bell, S.P. (1997) Components and dynamics of DNA replication complexes in S. cerevisiae: redistribution of MCM proteins and Cdc45p during S phase Cell, 91, 59–69[CrossRef][Web of Science][Medline] .

6. Nishitani, H., Lygerou, Z., Nishimoto, T., Nurse, P. (2000) The Cdt1 protein is required to license DNA for replication in fission yeast Nature, 404, 625–628[CrossRef][Medline] .

7. Bell, S.P. and Dutta, A. (2002) DNA replication in eukaryotic cells Annu. Rev. Biochem, . 71, 333–374[CrossRef][Web of Science][Medline] .

8. Bowers, J.L., Randell, J.C., Chen, S., Bell, S.P. (2004) ATP hydrolysis by ORC catalyzes reiterative Mcm2-7 assembly at a defined origin of replication Mol. Cell, 16, 967–978[CrossRef][Web of Science][Medline] .

9. Randell, J.C., Bowers, J.L., Rodriguez, H.K., Bell, S.P. (2006) Sequential ATP hydrolysis by Cdc6 and ORC directs loading of the Mcm2-7 helicase Mol. Cell, 21, 29–39[CrossRef][Web of Science][Medline] .

10. Masumoto, H., Sugino, A., Araki, H. (2000) Dpb11 controls the association between DNA polymerases alpha and epsilon and the autonomously replicating sequence region of budding yeast Mol. Cell. Biol, . 20, 2809–2817[Abstract/Free Full Text] .

11. Hiraga, S., Hagihara-Hayashi, A., Ohya, T., Sugino, A. (2005) DNA polymerases alpha, delta, and epsilon localize and function together at replication forks in Saccharomyces cerevisiae Genes Cells, 10, 297–309[Abstract/Free Full Text] .

12. Hubscher, U., Nasheuer, H.P., Syvaoja, J.E. (2000) Eukaryotic DNA polymerases, a growing family Trends Biochem. Sci, 25, 143–147[CrossRef][Web of Science][Medline] .

13. Kamimura, Y., Masumoto, H., Sugino, A., Araki, H. (1998) Sld2, which interacts with Dpb11 in Saccharomyces cerevisiae, is required for chromosomal DNA replication Mol. Cell Biol, . 18, 6102–6109[Abstract/Free Full Text] .

14. Ricke, R.M. and Bielinsky, A.K. (2004) Mcm10 regulates the stability and chromatin association of DNA polymerase-alpha Mol. Cell, 16, 173–185[CrossRef][Web of Science][Medline] .

15. Hubscher, U., Maga, G., Spadari, S. (2002) Eukaryotic DNA polymerases Annu. Rev. Biochem, . 71, 133–163[CrossRef][Web of Science][Medline] .

16. Tsurimoto, T. and Stillman, B. (1991) Replication factors required for SV40 DNA replication in vitro II. Switching of DNA polymerase alpha and delta during initiation of leading and lagging strand synthesis J. Biol. Chem, . 266, 1961–1968[Abstract/Free Full Text] .

17. Maga, G., Stucki, M., Spadari, S., Hubscher, U. (2000) DNA polymerase switching: I. Replication factor C displaces DNA polymerase alpha. prior to PCNA loading J. Mol. Biol, . 295, 791–801[CrossRef][Web of Science][Medline] .

18. Hamatake, R.K., Hasegawa, H., Clark, A.B., Bebenek, K., Kunkel, T.A., Sugino, A. (1990) Purification and characterization of DNA polymerase II from the yeast Saccharomyces cerevisiae. Identification of the catalytic core and a possible holoenzyme form of the enzyme J. Biol. Chem, . 265, 4072–4083[Abstract/Free Full Text] .

19. Seki, T., Akita, M., Kamimura, Y., Muramatsu, S., Araki, H., Sugino, A. (2006) Gins is a DNA polymerase epsilon accessory factor during chromosomal DNA replication in budding yeast J. Biol. Chem, . [Epub ahead of print] .

20. Ohya, T., Kawasaki, Y., Hiraga, S., Kanbara, S., Nakajo, K., Nakashima, N., Suzuki, A., Sugino, A. (2002) The DNA polymerase domain of pol(epsilon) is required for rapid, efficient, and highly accurate chromosomal DNA replication, telomere length maintenance, and normal cell senescence in Saccharomyces cerevisiae J. Biol. Chem, . 277, 28099–28108[Abstract/Free Full Text] .

21. Kesti, T., Flick, K., Keranen, S., Syvaoja, J.E., Wittenberg, C. (1999) DNA polymerase epsilon catalytic domains are dispensable for DNA replication, DNA repair, and cell viability Mol. Cell, 3, 679–685[CrossRef][Web of Science][Medline] .

22. Dua, R., Levy, D.L., Campbell, J.L. (1999) Analysis of the essential functions of the C-terminal protein/protein interaction domain of Saccharomyces cerevisiae pol epsilon and its unexpected ability to support growth in the absence of the DNA polymerase domain J. Biol. Chem, . 274, 22283–22288[Abstract/Free Full Text] .

23. Burgers, P.M. and Gerik, K.J. (1998) Structure and processivity of two forms of Saccharomyces cerevisiae DNA polymerase delta J. Biol. Chem, . 273, 19756–19762[Abstract/Free Full Text] .

24. Dua, R., Edwards, S., Levy, D.L., Campbell, J.L. (2000) Subunit interactions within the Saccharomyces cerevisiae DNA polymerase epsilon (pol epsilon ) complex. Demonstration of a dimeric pol epsilon J. Biol. Chem, . 275, 28816–28825[Abstract/Free Full Text] .

25. Katou, Y., Kanoh, Y., Bando, M., Noguchi, H., Tanaka, H., Ashikari, T., Sugimoto, K., Shirahige, K. (2003) S-phase checkpoint proteins Tof1 and Mrc1 form a stable replication-pausing complex Nature, 424, 1078–1083[CrossRef][Medline] .

26. Mills, J.B., Vacano, E., Hagerman, P.J. (1999) Flexibility of single-stranded DNA: use of gapped duplex helices to determine the persistence lengths of poly(dT) and poly(dA) J. Mol. Biol, . 285, 245–257[CrossRef][Web of Science][Medline] .

27. Kuznetsov, S.V., Shen, Y., Benight, A.S., Ansari, A. (2001) A semiflexible polymer model applied to loop formation in DNA hairpins Biophys. J, . 81, 2864–2875[Web of Science][Medline] .

28. Murphy, M.C., Rasnik, I., Cheng, W., Lohman, T.M., Ha, T. (2004) Probing single-stranded DNA conformational flexibility using fluorescence spectroscopy Biophys. J, . 86, 2530–2537[Web of Science][Medline] .

29. Sogo, J.M., Lopes, M., Foiani, M. (2002) Fork reversal and ssDNA accumulation at stalled replication forks owing to checkpoint defects Science, 297, 599–602[Abstract/Free Full Text] .

30. Muzi-Falconi, M., Liberi, G., Lucca, C., Foiani, M. (2003) Mechanisms controlling the integrity of replicating chromosomes in budding yeast Cell Cycle, 2, 564–567[Medline] .

31. Lopes, M., Cotta-Ramusino, C., Pellicioli, A., Liberi, G., Plevani, P., Muzi-Falconi, M., Newlon, C.S., Foiani, M. (2001) The DNA replication checkpoint response stabilizes stalled replication forks Nature, 412, 557–561[CrossRef][Medline] .

32. Tercero, J.A. and Diffley, J.F. (2001) Regulation of DNA replication fork progression through damaged DNA by the Mec1/Rad53 checkpoint Nature, 412, 553–557[CrossRef][Medline] .

33. Weinert, T.A., Kiser, G.L., Hartwell, L.H. (1994) Mitotic checkpoint genes in budding yeast and the dependence of mitosis on DNA replication and repair Genes. Dev, . 6, 652–665 .

34. Paulovich, A.G. and Hartwell, L.H. (1995) A checkpoint regulates the rate of progression through S phase in S. cerevisiae in response to DNA damage Cell, 82, 841–847[CrossRef][Web of Science][Medline] .

35. McGowan, C.H. and Russell, P. (2004) The DNA damage response: sensing and signaling Curr. Opin. Cell Biol, . 16, 629–633[CrossRef][Web of Science][Medline] .

36. Rouse, J. and Jackson, S.P. (2002) Lcd1p recruits Mec1p to DNA lesions in vitro and in vivo Mol. Cell, 9, 857–869[CrossRef][Web of Science][Medline] .

37. Melo, J.A., Cohen, J., Toczyski, D.P. (2001) Two checkpoint complexes are independently recruited to sites of DNA damage in vivo Genes. Dev, 15, 2809–2821[Abstract/Free Full Text] .

38. Zou, L. and Elledge, S.J. (2003) Sensing DNA damage through ATRIP recognition of RPA-ssDNA complexes Science, 300, 1542–1548[Abstract/Free Full Text] .

39. Namiki, Y. and Zou, L. (2006) ATRIP associates with replication protein A-coated ssDNA through multiple interactions Proc. Natl Acad. Sci. USA, 103, 580–585[Abstract/Free Full Text] .

40. Kumagai, A. and Dunphy, W.G. (2000) Claspin, a novel protein required for the activation of Chk1 during a DNA replication checkpoint response in Xenopus egg extracts Mol. Cell, 6, 839–849[CrossRef][Web of Science][Medline] .

41. Alcasabas, A.A., Osborn, A.J., Bachant, J., Hu, F., Werler, P.J., Bousset, K., Furuya, K., Diffley, J.F., Carr, A.M., Elledge, S.J. (2001) Mrc1 transduces signals of DNA replication stress to activate Rad53 Nature Cell Biol, . 3, 958–965[CrossRef][Web of Science][Medline] .

42. Foss, E.J. (2001) Tof1p regulates DNA damage responses during S phase in Saccharomyces cerevisiae Genetics, 157, 567–577[Abstract/Free Full Text] .

43. Mayer, M.L., Pot, I., Chang, M., Xu, H., Aneliunas, V., Kwok, T., Newitt, R., Aebersold, R., Boone, C., Brown, G.W., et al. (2004) Identification of protein complexes required for efficient sister chromatid cohesion Mol. Biol. Cell, 15, 1736–1745[Abstract/Free Full Text] .

44. Noguchi, E., Noguchi, C., McDonald, W.H., Yates, J.R., 3rd, Russell, P. (2004) Swi1 and Swi3 are components of a replication fork protection complex in fission yeast Mol. Cell Biol, . 24, 8342–8355[Abstract/Free Full Text] .

45. Osborn, A.J. and Elledge, S.J. (2003) Mrc1 is a replication fork component whose phosphorylation in response to DNA replication stress activates Rad53 Genes. Dev, 17, 1755–1767[Abstract/Free Full Text] .

46. Tong, A.H., Lesage, G., Bader, G.D., Ding, H., Xu, H., Xin, X., Young, J., Berriz, G.F., Brost, R.L., Chang, M., et al. (2004) Global mapping of the yeast genetic interaction network Science, 303, 808–813[Abstract/Free Full Text] .

47. Kumagai, A. and Dunphy, W.G. (2003) Repeated phosphopeptide motifs in Claspin mediate the regulated binding of Chk1 Nature Cell Biol, . 5, 161–165[CrossRef][Web of Science][Medline] .

48. Longhese, M.P., Clerici, M., Lucchini, G. (2003) The S-phase checkpoint and its regulation in Saccharomyces cerevisiae Mutat. Res, . 532, 41–58[Web of Science][Medline] .

49. Zhao, H., Tanaka, K., Nogochi, E., Nogochi, C., Russell, P. (2003) Replication checkpoint protein Mrc1 is regulated by Rad3 and Tel1 in fission yeast Mol. Cell Biol, . 23, 8395–8403[Abstract/Free Full Text] .

50. Cortez, D., Glick, G., Elledge, S.J. (2004) Minichromosome maintenance proteins are direct targets of the ATM and ATR checkpoint kinases Proc. Natl Acad. Sci. USA, 101, 10078–10083[Abstract/Free Full Text] .

51. Yoo, H.Y., Shevchenko, A., Dunphy, W.G. (2004) Mcm2 is a direct substrate of ATM and ATR during DNA damage and DNA replication checkpoint responses J. Biol. Chem, . 279, 53353–53364[Abstract/Free Full Text] .

52. Ishimi, Y., Komamura-Kohno, Y., Kwon, H.J., Yamada, K., Nakanishi, M. (2003) Identification of MCM4 as a target of the DNA replication block checkpoint system J. Biol. Chem, . 278, 24644–24650[Abstract/Free Full Text] .

53. Unsal-Kacmaz, K., Mullen, T.E., Kaufmann, W.K., Sancar, A. (2005) Coupling of human circadian and cell cycles by the timeless protein Mol. Cell Biol, . 25, 3109–3116[Abstract/Free Full Text] .

54. Zhao, H. and Russell, P. (2004) DNA binding domain in the replication checkpoint protein Mrc1 of Schizosaccharomyces pombe J. Biol. Chem, . 279, 53023–53027[Abstract/Free Full Text] .

55. Sar, F., Lindsey-Boltz, L.A., Subramanian, D., Croteau, D.L., Hutsell, S.Q., Griffith, J.D., Sancar, A. (2004) Human claspin is a ring-shaped DNA-binding protein with high affinity to branched DNA structures J. Biol. Chem, . 279, 39289–39295[Abstract/Free Full Text] .

56. Dalgaard, J.Z. and Klar, A.J. (1999) Orientation of DNA replication establishes mating-type switching pattern in S. pombe Nature, 400, 181–184[CrossRef][Medline] .

57. Brewer, B.J., Lockshon, D., Fangman, W.L. (1992) The arrest of replication forks in the rDNA of yeast occurs independently of transcription Cell, 71, 267–276[CrossRef][Web of Science][Medline] .

58. Krings, G. and Bastia, D. (2004) swi1- and swi3-dependent and independent replication fork arrest at the ribosomal DNA of Schizosaccharomyces pombe Proc. Natl. Acad Sci. USA, 101, 14085–14090[Abstract/Free Full Text] .

59. Dalgaard, J.Z. and Klar, A.J. (2000) swi1 and swi3 perform imprinting, pausing, and termination of DNA replication in S. pombe Cell, 102, 745–751[CrossRef][Web of Science][Medline] .

60. Calzada, A., Hodgson, B., Kanemaki, M., Bueno, A., Labib, K. (2005) Molecular anatomy and regulation of a stable replisome at a paused eukaryotic DNA replication fork Genes. Dev, 19, 1905–1919[Abstract/Free Full Text] .

61. Mohanty, B.K. and Bastia, D. (2004) Binding of the replication terminator protein Fob1p to the Ter sites of yeast causes polar fork arrest J. Biol. Chem, . 279, 1932–1941[Abstract/Free Full Text] .

62. Sanchez-Gorostiaga, A., Lopez-Estrano, C., Krimer, D.B., Schvartzman, J.B., Hernandez, P. (2004) Transcription termination factor reb1p causes two replication fork barriers at its cognate sites in fission yeast ribosomal DNA in vivo Mol. Cell Biol, . 24, 398–406[Abstract/Free Full Text] .

63. Rabitsch, K.P., Toth, A., Galova, M., Schleiffer, A., Schaffner, G., Aigner, E., Rupp, C., Penkner, A.M., Moreno-Borchart, A.C., Primig, M., et al. (2001) A screen for genes required for meiosis and spore formation based on whole-genome expression Curr. Biol, . 11, 1001–1009[CrossRef][Web of Science][Medline] .

64. Tong, A. and Boone, C. (2004) Global mapping of the yeast genetic interaction network Science, 303, 808–814[Abstract/Free Full Text] .

65. Xu, H., Boone, C., Klein, H.L. (2004) Mrc1 is required for sister chromatid cohesion to aid in recombination repair of spontaneous damage Mol. Cell Biol, . 24, 7082–7090[Abstract/Free Full Text] .

66. Szyjka, S.J., Viggiani, C.J., Aparicio, O.M. (2005) Mrc1 is required for normal progression of replication forks throughout chromatin in S. cerevisiae Mol. Cell, 19, 691–697[CrossRef][Web of Science][Medline] .

67. Tourriere, H., Versini, G., Cordon-Preciado, V., Alabert, C., Pasero, P. (2005) Mrc1 and Tof1 promote replication fork progression and recovery independently of Rad53 Mol. Cell, 19, 699–706[CrossRef][Web of Science][Medline] .

68. Gruber, S., Haering, C.H., Nasmyth, K. (2003) Chromosomal cohesin forms a ring Cell, 112, 765–777[CrossRef][Web of Science][Medline] .

69. Ivanov, D. and Nasmyth, K. (2005) A topological interaction between cohesin rings and a circular minichromosome Cell, 122, 849–860[CrossRef][Web of Science][Medline] .

70. Zhao, X., Chabes, A., Domkin, V., Thelander, L., Rothstein, R. (2001) The ribonucleotide reductase inhibitor Sml1 is a new target of the Mec1/Rad53 kinase cascade during growth and in response to DNA damage Embo. J, . 20, 3544–3553[CrossRef][Web of Science][Medline] .

71. Reichard, P. (1988) Interactions between deoxyribonucleotide and DNA synthesis Annu. Rev. BioChem, . 57, 349–374[CrossRef][Web of Science][Medline] .

72. Zhou, Z. and Elledge, S.J. (1993) DUN1 encodes a protein kinase that controls the DNA damage response in yeast Cell, 75, 1119–1127[CrossRef][Web of Science][Medline] .

73. Elledge, S.J., Zhou, Z., Allen, J.B., Navas, T.A. (1993) DNA damage and cell cycle regulation of ribonucleotide reductase Bioessays, 15, 333–339[CrossRef][Web of Science][Medline] .

74. Zhao, X. and Rothstein, R. (2002) The Dun1 checkpoint kinase phosphorylates and regulates the ribonucleotide reductase inhibitor Sml1 Proc. Natl Acad. Sci. USA, 99, 3746–3751[Abstract/Free Full Text] .

75. Cha, R.S. and Kleckner, N. (2002) ATR homolog Mec1 promotes fork progression, thus averting breaks in replication slow zones Science, 297, 602–606[Abstract/Free Full Text] .

76. Patel, S.S. and Picha, K.M. (2000) Structure and function of hexameric helicases Annu. Rev. BioChem, . 69, 651–697[CrossRef][Web of Science][Medline] .

77. Takahashi, T.S., Wigley, D.B., Walter, J.C. (2005) Pumps, paradoxes and ploughshares: mechanism of the MCM2-7 DNA helicase Trends Biochem. Sci, 30, 437–444[CrossRef][Web of Science][Medline] .

78. Laskey, R.A. and Madine, M.A. (2003) A rotary pumping model for helicase function of MCM proteins at a distance from replication forks EMBO. Rep, . 4, 26–30[CrossRef][Web of Science][Medline] .

79. Pacek, M., Tutter, A.V., Kubota, Y., Takisawa, H., Walter, J.C. (2006) Localization of MCM2-7, Cdc45, and GINS to the site of DNA unwinding during eukaryotic DNA replication Mol. Cell, 21, 581–587[CrossRef][Web of Science][Medline] .

80. Mendez, J. and Stillman, B. (2003) Perpetuating the double helix: molecular machines at eukaryotic DNA replication origins Bioessays, 25, 1158–1167[CrossRef][Web of Science][Medline] .

81. Fanning, E. and Knippers, R. (1992) Structure and function of simian virus 40 large tumor antigen Annu. Rev. BioChem, . 61, 55–85[CrossRef][Web of Science][Medline] .

82. Li, D., Zhao, R., Lilyestrom, W., Gai, D., Zhang, R., DeCaprio, J.A., Fanning, E., Jochimiak, A., Szakonyi, G., Chen, X.S. (2003) Structure of the replicative helicase of the oncoprotein SV40 large tumour antigen Nature, 423, 512–518[CrossRef][Medline] .

83. Fletcher, R.J., Bishop, B.E., Leon, R.P., Sclafani, R.A., Ogata, C.M., Chen, X.S. (2003) The structure and function of MCM from archaeal M. Thermoautotrophicum Nature Struct. Biol, . 10, 160–167[CrossRef][Web of Science][Medline] .

84. Fletcher, R.J., Shen, J., Gomez-Llorente, Y., Martin, C.S., Carazo, J.M., Chen, X.S. (2005) Double hexamer disruption and biochemical activities of Methanobacterium thermoautotrophicum MCM J. Biol. Chem, . 280, 42405–42410[Abstract/Free Full Text] .

85. Waga, S. and Stillman, B. (1994) Anatomy of a DNA replication fork revealed by reconstitution of SV40 DNA replication in vitro Nature, 369, 207–212[CrossRef][Medline] .

86. Zlotkin, T., Kaufmann, G., Jiang, Y., Lee, M.Y., Uitto, L., Syvaoja, J., Dornreiter, I., Fanning, E., Nethanel, T. (1996) DNA polymerase epsilon may be dispensable for SV40- but not cellular-DNA replication Embo. J, . 15, 2298–2305[Web of Science][Medline] .

87. Pommier, Y., Redon, C., Rao, V.A., Seiler, J.A., Sordet, O., Takemura, H., Antony, S., Meng, L., Liao, Z., Kohlhagen, G., et al. (2003) Repair of and checkpoint response to topoisomerase I-mediated DNA damage Mutat. Res, 532, 173–203[Web of Science][Medline] .

88. Egel, R. (2005) Fission yeast mating-type switching: programmed damage and repair DNA. Repair. (Amst.), 4, 525–536[CrossRef][Medline] .

89. Holmes, A.M., Kaykov, A., Arcangioli, B. (2005) Molecular and cellular dissection of mating-type switching steps in Schizosaccharomyces pombe Mol. Cell Biol, . 25, 303–311[Abstract/Free Full Text] .

90. Kaykov, A. and Arcangioli, B. (2004) A programmed strand-specific and modified nick in S. pombe constitutes a novel type of chromosomal imprint Curr. Biol, . 14, 1924–1928[CrossRef][Web of Science][Medline] .

91. Kaykov, A., Holmes, A.M., Arcangioli, B. (2004) Formation, maintenance and consequences of the imprint at the mating-type locus in fission yeast Embo. J, 23, 930–938[CrossRef][Web of Science][Medline] .

92. Vengrova, S. and Dalgaard, J.Z. (2004) RNase-sensitive DNA modification(s) initiates S. pombe mating-type switching Genes. Dev, 18, 794–804[Abstract/Free Full Text] .

93. Vengrova, S. and Dalgaard, J.Z. (2005) The Schizosaccharomyces pombe imprint—nick or ribonucleotide(s)? Curr. Biol, . 15, R326–327 author reply R327[CrossRef][Web of Science][Medline] .

94. Vengrova, S. and Dalgaard, J.Z. (2006) The wild-type Schizosaccharomyces pombe mat1 imprint consists of two ribonucleotides EMBO. Rep, 7, 59–65[CrossRef][Web of Science][Medline] .

95. Droge, P., Sogo, J.M., Stahl, H. (1985) Inhibition of DNA synthesis by aphidicolin induces supercoiling in simian virus 40 replicative intermediates Embo. J, . 4, 3241–3246[Web of Science][Medline] .

96. Baldari, C.T., Amaldi, F., Buongiorno-Nardelli, M. (1978) Electron microscopic analysis of replicating DNA of sea urchin embryos Cell, 15, 1095–1107[CrossRef][Web of Science][Medline] .

97. Gaudette, M.F. and Benbow, R.M. (1986) Replication forks are underrepresented in chromosomal DNA of Xenopus laevis embryos Proc. Natl Acad. Sci. USA, 83, 5953–5957[Abstract/Free Full Text] .

98. Walter, J. and Newport, J. (2000) Initiation of eukaryotic DNA replication: origin unwinding and sequential chromatin association of Cdc45, RP A, and DNA polymerase alpha Mol. Cell, 5, 617–627[CrossRef][Web of Science][Medline] .

99. Byun, T.S., Pacek, M., Yee, M.C., Walter, J.C., Cimprich, K.A. (2005) Functional uncoupling of MCM helicase and DNA polymerase activities activates the ATR-dependent checkpoint Genes. Dev, 19, 1040–1052[Abstract/Free Full Text] .

100. Jeong, S.Y., Kumagai, A., Lee, J., Dunphy, W.G. (2003) Phosphorylated claspin interacts with a phosphate-binding site in the kinase domain of Chk1 during ATR-mediated activation J. Biol. Chem, . 278, 46782–46788[Abstract/Free Full Text] .

CiteULike    Connotea    Del.icio.us    What's this?

This article has been cited by other articles:

				K. A. Urtishak, K. D. Smith, R. A. Chanoux, R. A. Greenberg, F. B. Johnson, and E. J. Brown Timeless Maintains Genomic Stability and Suppresses Sister Chromatid Exchange during Unperturbed DNA Replication J. Biol. Chem., March 27, 2009; 284(13): 8777 - 8785. [Abstract] [Full Text] [PDF]

				D. Biswas, S. Takahata, H. Xin, R. Dutta-Biswas, Y. Yu, T. Formosa, and D. J. Stillman A Role for Chd1 and Set2 in Negatively Regulating DNA Replication in Saccharomyces cerevisiae Genetics, February 1, 2008; 178(2): 649 - 659. [Abstract] [Full Text] [PDF]

This Article Abstract Print PDF (293K) Screen PDF (296K) OA All Versions of this Article: 34/15/4138    most recent gkl528v1 Alert me when this article is cited Alert me if a correction is posted Services Email this article to a friend Similar articles in this journal Similar articles in ISI Web of Science Similar articles in PubMed Alert me to new issues of the journal Add to My Personal Archive Download to citation manager Search for citing articles in: ISI Web of Science (3) Commercial Re-use Guidelines for Open Access NAR Content Google Scholar Articles by Nedelcheva-Veleva, M. N. Articles by Stoynov, S. S. Search for Related Content PubMed PubMed Citation Articles by Nedelcheva-Veleva, M. N. Articles by Stoynov, S. S. Social Bookmarking          What's this?

Online ISSN 1362-4962 - Print ISSN 0305-1048

Copyright © 2009 Oxford University Press

Oxford Journals Oxford University Press

• Site Map
• Privacy Policy
• Frequently Asked Questions

Other Oxford University Press sites: Oxford University Press Oxford Journals China Oxford Journals Japan American National Biography Booksellers' Information Service Children's Fiction and Poetry Children's Reference Corporate & Special Sales Dictionaries Dictionary of National Biography Digital Reference English Language Teaching Higher Education Textbooks Humanities International Education Unit Law Medicine Music Online Products Oxford English Dictionary Reference Rights and Permissions Science School Books Social Sciences Very Short Introductions World's Classics