Accumulation of Single-Stranded DNA and Destabilization of Telomeric Repeats in Yeast Mutant Strains Carrying a Deletion of RAD27

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Molecular and Cellular Biology, June 1999, p. 4143-4152, Vol. 19, No. 6
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Accumulation of Single-Stranded DNA and Destabilization of Telomeric Repeats in Yeast Mutant Strains Carrying a Deletion of RAD27

Julie Parenteau and Raymund J. Wellinger^*

Département de Microbiologie et Infectiologie, Faculté de Médecine, Université de Sherbrooke, Sherbrooke, Quebec, J1H 5N4, Canada

Received 30 November 1998/Returned for modification 13 January 1999/Accepted 26 March 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Saccharomyces cerevisiae RAD27 gene encodes the yeast homologue of the mammalian FEN-1 nuclease, a protein that is thoughtto be involved in the processing of Okazaki fragments during DNAlagging-strand synthesis. One of the predicted DNA lesions occurringin rad27 strains is the presence of single-stranded DNA of thetemplate strand for lagging-strand synthesis. We examined thisprediction by analyzing the terminal DNA structures generatedduring telomere replication in rad27 strains. The lengths of thetelomeric repeat tracts were found to be destabilized in rad27strains, indicating that naturally occurring direct repeats aresubject to tract expansions and contractions in such strains.Furthermore, abnormally high levels of single-stranded DNA ofthe templating strand for lagging-strand synthesis were observedin rad27 cells. Overexpression of Dna2p in wild-type cells alsoyielded single-stranded DNA regions on telomeric DNA and causeda cell growth arrest phenotype virtually identical to that seenfor rad27 cells grown at the restrictive temperature. Furthermore,overexpression of the yeast exonuclease Exo1p alleviated the growtharrest induced by both conditions, overexpression of Dna2p andincubation of rad27 cells at 37°C. However, the telomere heterogeneityand the appearance of single-stranded DNA are not prevented bythe overexpression of Exo1p in these strains, suggesting thatthis nuclease is not simply redundant with Rad27p. Our data thusprovide in vivo evidence for the types of DNA lesions predictedto occur when lagging-strand synthesis is deficient and suggestthat Dna2p and Rad27p collaborate in the processing of Okazakifragments.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Due to the conserved 5'-to-3' polarity of all DNA polymerases known to date, newly synthesized DNA at the replication forkis assembled in a discontinuous (lagging) and a continuous (leading)strand. All replicative polymerases also require a primer to efficientlystart synthesizing DNA. This priming of DNA synthesis by a shortRNA molecule presumably only occurs once, at the origin of replication,for leading-strand synthesis, but priming is required throughoutthe synthesis of the lagging strand. Thus, the generation of acontinuous DNA strand for lagging-strand synthesis is dependenton the activities of a primase, DNA polymerases $alpha$ , $delta$ , and/or $varepsilon$ with accessory proteins such as PCNA and RF-C, as well as activitiesinvolved in removal of the RNA primer and resealing of the resultinggap (for reviews, see references 3 and 4).

In the yeast Saccharomyces cerevisiae, as in mammalian cells, removal of the RNA primer is thought to be mediated by an endo/exonucleolyticactivity called FEN-1 (flap endonuclease or 5'-exonuclease 1 [20,21]), presumably aided by RNase H1 (18, 24, 36, 48,50; for reviews, see references 17, 29, and 32). Recentbiochemical analyses of the FEN-1 nuclease indicate that the FEN-1protein interacts with, and its activity is stimulated by, PCNA(31, 56). The yeast homologue of the mammalian FEN-1 enzymeis encoded by the RAD27/RTH1 gene and belongs in the RAD6 epistasisgroup (37). Yeast cells lacking Rad27p are sensitive to alkylatingagents like methyl methanesulfonate but not to ionizing radiation(37). Mutant strains also display high levels of instabilityof simple repetitive DNA (14, 26, 28, 41) and a temperature-sensitivegrowth defect (37, 45). Finally, rad27 $Delta$ strains incubatedat the restrictive temperature exhibit a checkpoint-dependentcell cycle arrest in late S/G₂ (49). These phenotypes, as wellas the molecular analysis of the mutation spectra occurring inrad27 $Delta$ strains, suggest a crucial deficiency in DNA replicationand repair (28, 47). Since mutations in RAD27, when combinedwith mutations in genes belonging to the RAD52 epistasis group,yield inviable cells, it has been proposed that the lesions occurringin rad27 $Delta$ cells are predominantly repaired by a double-strandbreak repair mechanism (47). Recent studies have also shownthat an essential yeast replicative helicase, Dna2p, interactsgenetically and biochemically with Rad27p (6, 7). Cellsharboring temperature sensitivity alleles of DNA2 arrest in G₂/Mwith a 2C DNA content at the restrictive temperature and containDNA of low molecular weight (13). Taken together, these resultshave been interpreted to suggest that Rad27p and Dna2p act togetherin lagging-strand processing (3, 4). Specifically, basedalso on the fact that the Rad27p nuclease loads onto, and actsmuch more efficiently on, a displaced-5'-end single strand, ithas been proposed that Dna2p displaces the 5' ends at the RNA-DNAjunction of Okazaki fragments, resulting in a 5' flap structurethat could be removed by the endonucleolytic activity of Rad27p(36). However, direct in vivo evidence for such a mode of actionis stilllacking.

Telomeres, the ends of eukaryotic chromosomes, are essential for chromosome integrity: they protect chromosome ends from degradationand random fusion events (34, 40), and they ensure the completereplication of the chromosome (19, 51, 57). Chromosomesin S. cerevisiae end in 300 bp of short, heterogeneous sequencerepeats, commonly abbreviated as C_1-3A or TG_1-3 (42).These yeast telomeric sequence repeats are similar to those ofmost other eukaryotes in having clusters of G residues in thestrand running 5' to 3' from the center toward the end of theDNA molecule (the G-rich strand) (53). Due to the base disparitybetween the two strands and the polarity of DNA synthesis, theG-rich strand will always be synthesized by leading-strand synthesisand the C-rich strand will always be synthesized by lagging-strandsynthesis (Fig. 1). Analyzing the DNA replication intermediatesoccurring during telomere replication, we have previously shownthat chromosome ends in yeast acquire transient $>=$ 30-base single-strandedextensions of the G-rich strand (G tails) (52, 54). Furthermore,these G tails could be detected in cells that were devoid of telomerase,suggesting that the bulk of the G tails are generated in a telomerase-independentfashion (11).

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FIG. 1. Nucleotide composition of templating and newly synthesized strands on telomeric repeats. Due to the conserved polarity of the telomeric repeats on all telomeres, the templating strand for lagging-strand synthesis is always the G-rich strand and the templating strand for leading-strand synthesis is the C-rich strand. Thick lines with nucleotides in boldface, templating strands; thin lines, newly synthesized strands. Note that the identity of the last nucleotide at the end of each strand is unknown; the designation drawn out here is given for simplicity.

In order to understand all the activities required for telomere processing, we are interested in determining how the single-strandedG tails occurring during telomere replication are generated andprocessed. Since the Rad27p/Dna2p proteins have been proposedto process the 5' ends of newly generated Okazaki fragments, weinvestigated the involvement of these proteins in the generationof telomere replication intermediates. If these proteins wereinvolved in lagging-strand synthesis in vivo, we expected aberranttelomere processing and/or a deficiency in synthesizing the newC-rich strands on telomeres in rad27 $Delta$ strains. Indeed, terminalsingle-stranded G-rich strands do occur at abnormally high levelson terminal restriction fragments (TRFs) derived from rad27 $Delta$ cellsincubated at the restrictive temperature. Conversely, single-strandedDNA of the C-rich strand, which would be indicative of failingleading-strand synthesis, remained undetectable as in wild-typecells. In the same DNA samples, there were no detectable single-strandedY' sequences for either strand. The appearance of the single-strandedG tails correlated with an expansion of the heterogeneity of thelengths of the terminal repeat tracts, indicative of abnormalrepeat lengthening and shortening in rad27 $Delta$ cells. Overexpressionof a full-length Dna2p resulted in cell cycle arrest. This arrestin cell growth can be suppressed by cooverexpressing Rad27p inthe same cells, supporting the notion of a functional interactionbetween Rad27p and Dna2p. Most significantly, by analysis of thechromosomal termini derived from cells in which Dna2p was overexpressed,a transient increase in single-stranded G strands was detected.We also show that while overexpression of the yeast exonucleaseExo1p can suppress the temperature sensitivity and mutator phenotypesof rad27 $Delta$ cells (47), it does not suppress the appearance ofsingle-stranded DNA in these cells. Our results thus provide invivo physical evidence for the types of lesions generated by anabsence of Rad27p and suggest that Rad27p and Dna2p collaboratein proper Okazaki fragmentprocessing.

	MATERIALS AND METHODS

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Strains and plasmids. Yeast strains used were SX46A (MATa RAD27 ade2 his3-532 trp1-289 ura3-52), SX46A rad27 $Delta$ ::URA3 (MATa rad27 $Delta$ ::URA3ade2 his3-532 trp1-289 ura3-52) (37), 7399-3-1 (MAT $alpha$ trp1 leu2ura3 his3) (obtained by J. Aron and T. Formosa), and MW35a (MATaade2 ade5 can^r 1 cyh^r 2 lys5 ura3 trp1 leu2-3,112 his3- $Delta$ 200 Gal⁺⁺).

The 2µm DNA2 plasmid, pTN3, was made by inserting a 5,709-bp EcoRI-PstI fragment containing the DNA2 gene into YEplac195 (16).The pGal-DNA2 plasmid was constructed by using a ScaI-PstI fragmentcontaining the complete DNA2 open reading frame. The ScaI siteupstream of DNA2 was converted to a BamHI site, and this fragmentwas inserted into the Gal-inducible pJS227 vector. pJS227 is YEplac195(16) containing the Gal1-10 promoter (27). Plasmids pTN3 andpGAL-DNA2 were kindly provided by J. Aron and T. Formosa. pGAL-vectoris pGAL-DNA2 from which a 5.9-kb BamHI-PstI fragment was removedand the vector was religated. The 2µm RAD27 plasmid, pR2, wasconstructed by inserting the 2,500-bp SphI-EcoRI fragment of pMR92393(37) into EcoRI-SmaI-digested pRS424 (10). The 2µm EXO1 plasmid,pE1, was made by inserting a 2,470-bp NotI-XhoI fragment of pRW200into NotI-XhoI-digested pRS423 DNA (10). In order to amplifythe yeast EXO1 gene from wild-type genomic DNA, we used the followingprimers for PCR: DF 5'-CTCCTCGAGTCTTTATAGGGCATTATTTGTAC-3' (theunderlined bases are complementary to positions $-$ 288 to $-$ 265 relativeto the EXO1 translational start site, and the 5' extension containsan XhoI site) and DR 5'-CTCTCTAGATCTTGTCTTGAGGCATTTCG-3' (theunderlined bases are complementary to positions +2585 to +2566relative to the EXO1 translational start site, and the 5' extensioncontains an XbaI site). We used 30 cycles of PCR at 94°C for 1min, 56°C for 1 min, and 72°C for 3 min, followed by a 15-min72°C soaking period. The PCR product was digested with XhoI andXbaI and cloned into pRS316 (43) to generate plasmidpRW200.

All plasmids were propagated in bacteria by using standard Escherichia coli strains and growth conditions (39). Yeast cellswere transformed by a modification (15) of the lithium acetatemethod (25) and grown in standard yeast media (38, 58).

DNA isolation and analysis. For Fig. 2 to 5 and 8, yeast strains were grown in synthetic complete (SC) medium at the permissive temperature for SX46Arad27 $Delta$ ::URA3 (23°C) to mid-logarithmic phase (optical densityat 660 nm [OD₆₆₀] = 0.6), then shifted to a semipermissive temperature(30°C) or to the restrictive temperature (37°C) for the indicatedtimes. For Fig. 7, the MW35a cells containing pGAL-DNA2 were grownin SC-Ura medium containing glycerol (2%) and lactate (2%) at30°C to mid-logarithmic phase. Galactose (final concentration,2%) was then added to induce expression of DNA2, and the cellswere incubated for the indicated times. Total genomic DNA fromcells was isolated by a modified glass bead procedure (23, 54).Treatment of genomic DNA with E. coli exonuclease I and mung beannuclease was carried out as described elsewhere (54).

Agarose gel techniques, Southern blot transfer to a nylon membrane, and hybridization conditions were as described previously(54). The nondenaturing in-gel hybridizations were carried outas described in reference 11. DNAs used as probes were a 300-bpfragment containing 280 bp of telomeric repeats derived from pYLPV(54), a 1.4-kb XhoI-XhoI fragment derived from yeast chromosomalCEN4 sequences (55), a 22-mer of the sequence 5'-CCCACCACACACACCCACACCC-3'(referred to as the CA oligonucleotide [11]), a 22-mer of thesequence 5'-GGGTGTGGGTGTGTGTGGTGGG-3' (referred to as the GT oligonucleotide),and a 30-mer of the sequence 5'-CCCTCGTGTTATCTGCAGCGAGAACTTCAA-3'(referred to as the Y' oligonucleotide). A heat-denatured 0.6-kbKpnI-KpnI fragment of Y' sequences (33) cloned in the KpnI siteof pVZ1 (22) was used as a Y' control. Single-stranded DNA frompCA75 and pGT75 (54) were obtained by standard procedures usinga helper phage (39) to produce CA and GT controls, respectively.The double-stranded control was obtained by the linearizationof pMW55 with BamHI. The pMW55 plasmid was made by inserting 55bp of duplex telomeric repeat DNA into the EcoRV site of pRS303(43).

	RESULTS

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Increased heterogeneity of telomeric repeats in rad27 $Delta$ cells at the restrictive temperature. Previous work showed an elevated instability of di- and trinucleotide repeats in yeast strains deficient for Rad27p (14,26, 28, 41). Telomeres, the ends of the chromosomes, representone genomic locus that naturally consists of short direct repeatsin many eukaryotes. We were therefore interested to know whethertelomeric repeat maintenance was affected by an absence of Rad27p.Telomeric repeat length in yeast can be assessed by digestinggenomic DNA with XhoI, which generates diagnostic TRFs of approximately1.3 kb due to the conservation of such a site in the subtelomericY' element that is present on most telomeres (Y' TRFs) (9).However, about one-third of the telomeres do not harbor a Y' element,and the TRFs derived from these telomeres (non-Y' TRFs) will belarger. When the TRFs of RAD27 strains grown at 23°C and shiftedto 37°C were analyzed, no apparent change in the TRF lengths couldbe discerned, as expected (Fig. 2A). However, after rad27 $Delta$ strainswere shifted to the nonpermissive temperature, the TRFs displayedvery heterogeneous sizes: Y' TRFs ranged from 0.9 to 1.6 kb, andthe bands for non-Y' TRFs were similarly broadened (Fig. 2A).This increase in size heterogeneity did not require extensiveoutgrowth, as these cells, when incubated at 37°C, arrested aslarge-budded cells after 2 to 3 generations and did not grow further(data not shown). As a control, the Southern blot shown in Fig.2A was stripped of the probe and rehybridized to a probe specificfor the CEN4 region (see Materials and Methods). This rehybridizationyielded the expected distinct band at approximately 1.4 kb forall DNAs, including the DNA derived from rad27 $Delta$ cells incubatedat the restrictive temperature (Fig. 2B). At 30°C, cells witha deletion of RAD27 grow slowly and display a TRF heterogeneitythat is intermediate between those of wild-type and rad27 $Delta$ cellsincubated at 37°C. However, this intermediate heterogeneity didnot change significantly upon further outgrowth of the cells at30°C for at least 100 generations (Fig. 2C). Thus, in rad27 $Delta$ cellsincubated at the semipermissive and restrictive temperatures,telomeric repeat length is destabilized, resulting in very heterogeneousTRFs. These results suggest that in rad27 $Delta$ cells, the naturalyeast telomeric repeats are subject to tract expansions and contractionssimilar to those reported for artificially inserted short repeatedelements in the yeast genome (14, 26, 28, 41).

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FIG. 2. Telomeric repeat instability in rad27 $Delta$ strains. (A) Genomic DNA isolated from RAD27 (WT) or rad27 $Delta$ cells that were incubated at 23 or 37°C for the indicated times was digested with the restriction endonuclease XhoI and analyzed by Southern blotting. The probe used was randomly labeled telomeric repeat DNA. Y' TRFs migrate at about 1.3 kb, and some of the other bands correspond to non-Y' TRFs. M, end-labeled 1-kb ladder DNA serving as a size standard. (B) The same blot as in panel A, rehybridized to a probe specific for CEN4 sequences. (C) The same experiment as in panel A, except that the strains were grown at 30°C. Note that rad27 $Delta$ cells do grow at this temperature. Every day, an aliquot of the cultures was diluted into fresh medium and the cells were regrown to stationary phase (days of culturing are indicated on top of the gel). From cell density measurements, it was calculated that the cultures had grown for approximately 100 generations on day 8 (data not shown).

Accumulation of single-stranded DNA of the G-rich telomeric repeats is detected in rad27 $Delta$ cells incubated at 37°C. The specific types of mutations observed in rad27 $Delta$ cells are most easily rationalized if the Rad27p is involved in processingthe 5' ends of Okazaki fragments (28, 47). The homologousenzyme from mammalian cells will cleave a displaced 5' strand(flap) in vitro, which is thought to be necessary to allow theligation of two adjoining Okazaki fragments. The displaced 5'end of the downstream Okazaki fragment could be generated by stranddisplacement synthesis from the upstream Okazaki fragment or couldbe the product of a helicase-mediated strand separation (3,4). However, the 5' end of the most distal Okazaki fragmentinitiated on telomeric repeat DNA cannot be displaced by stranddisplacement synthesis, as by definition there is no upstreamOkazaki fragment that could initiate this process (see Fig. 1).If a helicase displaces the 5' ends of Okazaki fragments for Rad27pcleavage, the most distal Okazaki fragment could be processedin the same way as the internal ones. In order to establish whethercells lacking Rad27p had a deficiency in telomeric repeat replication,TRFs derived from rad27 $Delta$ cells were analyzed for the appearanceof single-stranded DNA. In wild-type cells, telomeres acquiresingle-stranded DNA of the G-rich strand (G tails) late in S phasebut have no detectable single-stranded DNA during the rest ofthe cell cycle (52, 54). Moreover, single-stranded DNA ofthe C-rich strand always remained undetectable. Thus, when theTRFs derived from asynchronous wild-type cells were analyzed forG tails, only a very faint signal was detected (Fig. 3A). Similarly,rad27 $Delta$ cells grown at 23°C and shifted to 37°C for a short time( $<=$ 6 h) displayed only minor G tails (Fig. 3A). However, TRFs derivedfrom rad27 $Delta$ cells incubated at 37°C for more than 6 h had single-strandedG-rich DNA that was easily detectable in our assay (Fig. 3A).The appearance of this single-stranded DNA correlated in timewith the appearance of the repeat heterogeneity (Fig. 2 and 3B)and with the arrest of cell growth (data not shown). The single-strandedDNA detected in Fig. 3A could reflect gaps or could be a terminalG tail, as occurs on telomeres derived from wild-type cells. Todistinguish between these possibilities, genomic DNA derived fromrad27 $Delta$ cells that were incubated at the restrictive temperaturewas digested with E. coli exonuclease I, a 3'-end-specific single-strandedexonuclease (30), prior to TRF analysis. This treatment abolishedthe signal for the single-stranded DNA, as did a pretreatmentwith mung bean nuclease, a single-stranded-specific endonuclease(Fig. 4B). Neither of these treatments caused a general DNA degradation,and approximately the same amount of DNA was loaded in all lanes(Fig. 4C). Moreover, on this same DNA, no single-stranded DNAof the C-rich strand was detectable (Fig. 4A). Finally, a probespecific for Y' sequences and located about 500 bp proximal tothe Y'-to-telomeric repeat transition did not reveal any single-strandedDNA in this region (Fig. 5A). The probe used in Fig. 5A woulddetect the strand making the 3' ends of the chromosomes (the G-richstrand on the telomeric repeats), but an analogous probing witha probe from the opposing strand did not detect any single-strandedDNA either (data not shown). Once again, however, the accumulationof single-stranded DNA of the G-rich strand was detected on theDNA derived from rad27 $Delta$ cells incubated at 37°C, when this gelwas rehybridized to a telomeric C-strand probe (Fig. 5B), andall lanes contained approximately the same amount of DNA (Fig.5C). Thus, the single-stranded DNA detected on the TRFs derivedfrom rad27 $Delta$ cells incubated at the restrictive temperature isspecific for the G-rich telomeric repeats and consists of terminalextensions. These results indicate that in rad27 $Delta$ cells incubatedat the restrictive temperature, excessive telomeric G tails aregenerated and cannot be processed to normal chromosomal ends.

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FIG. 3. Appearance of single-stranded DNA on telomeres derived from rad27 $Delta$ cells. (A) Genomic DNA isolated from RAD27 (WT) or rad27 $Delta$ cells incubated at 37°C for the indicated times was digested with XhoI and analyzed by a nondenaturing in-gel hybridization procedure (11) with an end-labeled CA oligonucleotide as a probe. Double-stranded and linearized pMW55 served as a negative control (labeled ds), and single-stranded phagemid DNA containing yeast telomeric repeats of the G-rich strands served as a positive control (labeled GT) (see Materials and Methods). Molecular size standards are as in Fig. 2. (B) The DNA in the gel shown in panel A was denatured, and the same gel was rehybridized to the probe to show all the telomeric repeat-containing fragments.

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FIG. 4. The single-stranded telomeric repeats observed on TRFs derived from rad27 $Delta$ cells are specific for the G-rich strand and are terminal extensions. RAD27 (WT) or rad27 $Delta$ cells were pregrown at 23°C, then incubated overnight at 37°C, and DNA was isolated from both cultures. This DNA was then digested with mung bean nuclease (lanes labeled + for MB) or E. coli exonuclease I (lanes labeled + for Exo) or was mock treated (no enzyme; indicated with a minus sign). All the DNAs were then digested with XhoI and analyzed by nondenaturing in-gel hybridization as in Fig. 3. For the designation of the control DNAs, see Fig. 3 and Materials and Methods. (A) The gel was hybridized to the end-labeled GT oligonucleotide. (B) The gel shown in panel A was then rehybridized to the end-labeled CA oligonucleotide. Note that due to the fact that the gel was not denatured between the two probings, both the CA and GT single-stranded controls show positive signals after the second probing. (C) A photograph of the ethidium bromide-stained gel prior to the first hybridization is shown to demonstrate approximately equal loading of DNA in all lanes.

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FIG. 5. The single strandedness of the telomeric G-rich strand does not extend into neighboring Y' sequences. DNAs derived from RAD27 (WT) or rad27 $Delta$ cells incubated overnight at the indicated temperatures were digested with XhoI and analyzed as in Fig. 3 and 4. (A) The probe consisted of an end-labeled Y' oligonucleotide, detecting the same strand as the G-rich telomeric repeat strand, and the sequences are about 500 bp from the Y'-telomeric repeat sequences boundary. (B) The same gel as in panel A, rehybridized to the telomeric CA probe. Since the gel was not denatured between probings, both single-stranded controls are visible. (C) The gel shown in panels A and B was then denatured and rehybridized to the telomeric CA oligonucleotide. During the repeated hybridizations and washings, some of the smaller DNA fragments (below 1.2 kb) had diffused out of the gel (note the losses of the DNA size standard bands of 1 kb and less). Thus, the signal for the 1.3-kb Y' TRFs is somewhat weaker than expected for this gel. Controls and DNA size standards are as in Fig. 3 and 4.

Overexpression of Dna2p leads to formation of G tails. One possible interpretation of the above results could be that in the absence of the Rad27p nuclease, a DNA helicase responsiblefor the dissociation of the 5' ends of newly generated Okazakifragments inappropriately dissociates Okazaki fragments. Giventhe genetic and biochemical interactions of the Dna2p helicasewith Rad27p, it was previously proposed that Dna2p could be thehelicase performing this function (3, 4). However, DNA2has been shown to be an essential gene, and a temperature sensitivityallele of DNA2, dna2-1, is synthetically lethal with a rad27 $Delta$ mutation (6). Thus, we were unable to test whether the defectscaused by a rad27 $Delta$ mutation could be alleviated by mutations inDNA2. Alternatively, one might predict that overexpression ofDna2p in otherwise wild-type cells should yield the same phenotypesas an absence of Rad27p at high temperatures. To test this prediction,the entire coding sequence for Dna2p was inserted downstream ofa galactose-inducible promoter and transformed into yeast grownon glucose media. While transformed cells form colonies on platescontaining glucose, no growth is discernible on plates containinggalactose (Fig. 6), indicating that overexpression of Dna2p yieldsinviable cells. In addition, a high-copy-number vector harboringthe DNA2 gene did not yield any transformants, while control transformationswith the empty vector did (Table 1). More significantly, however,cotransformation of the high-copy-number plasmid containing theDNA2 gene with one that contained the RAD27 gene resulted in viabletransformants (Table 1). We conclude that overexpression of theDna2p helicase induces growth arrest and that this arrest canbe suppressed by a concomitant overexpression of Rad27p. It wastherefore possible that the actual lesions to the chromosomesin cells overexpressing Dna2p were similar to those observed inrad27 $Delta$ cells grown at elevated temperatures. To test this hypothesis,DNA was isolated from cells in which DNA2 expression was inducedfrom the pGAL-DNA2 plasmid. This DNA was then analyzed for telomericend structure (Fig. 7). After 1 h of galactose-induced Dna2p expression,only a slight signal for single-stranded G strands was detectable(Fig. 7). However, after 5 h of induction, signals for single-strandedG strands were readily detectable. In cultures in which Dna2pwas induced for longer than 5 h, cells stopped growing, with aconcomitant decrease in the signal for single-stranded DNA (Fig.7). After 24 h of induction, single-stranded DNA was barely detectable,even though somewhat more DNA was loaded in this lane than inthe other lanes (Fig. 7). Although we do not know the reasonswhy the signals decrease upon prolonged Dna2p expression, single-strandedtelomeric G-strand DNA is generated at elevated levels when Dna2pis overexpressed for a brief period, and the cells are still ableto return to growth on glucose-containing plates. We concludethat induction of Dna2p overexpression results in increased amountsof telomeric G-strand single-stranded DNA, a feature that is alsodisplayed in rad27 $Delta$ cells at elevated temperatures. We also examinedthe chromosomal end structure on DNA derived from cells that containeda temperature sensitivity allele of the DNA2 gene, dna2-1 (5),at the permissive and restrictive temperatures. Contrary to resultsobtained with DNA derived from the rad27 $Delta$ cells, no aberrant single-strandedDNA was detectable at any temperature, but the overall telomericrepeat length appeared slightly increased in these strains (datanot shown).

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FIG. 6. Overexpression of DNA2 leads to nongrowing cells. WT, nontransformed MW35a cells grown on SC media; WT+pGAL-vector, MW35a cells containing the empty vector and grown on SC-Ura plates; WT+pGAL-DNA2, MW35a cells transformed with a plasmid that contained the DNA2 gene under the control of a galactose-inducible promoter (see Materials and Methods for construction of the plasmids). The plates contained glucose (left) or galactose (right) as a carbon source.

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TABLE 1. Rescue of Dna2p-induced mortality by Rad27p and Exo1p^a

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FIG. 7. Induction of DNA2 expression leads to a transient increase of single-stranded telomeric G-rich DNA. MW35a cells containing pGAL-DNA2 were pregrown in SC-Ura media containing glycerol and lactate. Expression of DNA2 was then induced by the addition of galactose, and DNA was prepared from the culture at the indicated times after galactose addition. These DNAs were then digested with XhoI and analyzed by nondenaturing in-gel hybridization (left) using an end-labeled CA oligonucleotide as a probe. After denaturation of the DNA, the gel was rehybridized to the same probe as a control (right). Controls and molecular size standards are as in Fig. 2 through 5.

Overexpression of Exo1p does not suppress all the phenotypes observed for rad27 $Delta$ cells. The characterization of the EXO1 gene, encoding a 5'-3' exonuclease, has shown that Exo1p, when overexpressed, can suppressthe temperature sensitivity and mutator phenotypes of cells carryingmutations in RAD27 (46). In addition, mutations in EXO1 arelethal when combined with RAD27 mutations (46). Thus, it hasbeen speculated that either EXO1 and RAD27 may encode redundantfunctions or that the actual lesions occurring in rad27 $Delta$ cellsneed Exo1p for repair (46). Since our physical analysis of theDNA derived from rad27 $Delta$ cells uncovered the existence of single-strandedG tails at the telomeres, we investigated whether overexpressionof Exo1p would also reverse this effect in rad27 $Delta$ cells (Fig.8). Overexpression of Exo1p from a high-copy-number vector inwild-type cells or deletion of the EXO1 gene had no effect ontelomeric end structure or telomere length (Fig. 8 and data notshown). However, while introducing the same plasmid into rad27 $Delta$ cells suppressed their temperature sensitivity (46) (data notshown), it did not alleviate the appearance of the terminal single-strandedDNA after rad27 $Delta$ cells were shifted to 37°C (Fig. 8A). Furthermore,the length heterogeneity of the TRFs in this strain is very similarto that observed in rad27 $Delta$ cells without overexpression of Exo1p(compare the last two lanes in Fig. 8B with those in Fig. 2A).Thus, overexpression of Exo1p does not suppress all the phenotypesobserved for rad27 $Delta$ cells, suggesting that the EXO1 gene productis not redundant with RAD27 but rather is required for an efficientrepair of the lesions induced by the absence of Rad27p.

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FIG. 8. Overexpression of Exo1p does not prevent the formation of single-stranded DNA in rad27 $Delta$ cells. RAD27 (WT) or rad27 $Delta$ cells were transformed with either pRS423 (empty vector) or pE1 (labeled pExo1-2µm), grown in selective media, and incubated overnight at the indicated temperatures. DNA was isolated, digested with XhoI, and analyzed as in Fig. 3 through 5. (A) Nondenatured gel probed with the CA oligonucleotide. (B) The DNA in the gel shown in panel A was denatured and rehybridized to the same probe. Controls and molecular size standards are as in Fig. 7.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Instability of telomeric repeats in rad27 $Delta$ cells. Previous genetic analyses of yeast cells carrying a deletion of the RAD27 gene and biochemical analyses of the homologousmammalian FEN-1 protein in vitro suggested that Rad27p was involvedin the processing of Okazaki fragments during lagging-strand synthesis(see references 3 and 4 for reviews). A particular characteristicof yeast strains harboring a rad27 deletion is the destabilizationof micro- and minisatellite sequences (14, 26, 28, 41).This repeat tract destabilization appeared to worsen with increasedtract lengths (14, 41). Since the chromosome ends constituteone natural locus in which relatively long tracts of simple, directrepeats occur in many organisms, including yeast, we investigatedwhether the repeat instability observed in rad27 $Delta$ strains alsooccurred on telomeric repeats. As shown in Fig. 2 and 8, thisis indeed the case: telomeric repeat tract lengths display a severeincrease in their heterogeneity when rad27 $Delta$ cells are grown atelevated temperatures. This increased heterogeneity, indicatingtract contractions and expansions, appears to be in contrast tosome results that suggested a strong bias for repeat expansionsin rad27 $Delta$ cells (26, 28). However, this bias was found onlyfor relatively short tracts ( $<=$ 50 bp) of mono- and dinucleotiderepeats, and in larger tracts ( $>=$ 100 bp) of trinucleotide repeats,such a bias was not observed. In such long tracts, which moreclosely resemble the telomeric repeat tracts (average length ofabout 300 bp), there was an approximately equal distribution ofrepeat contractions and expansions in rad27 $Delta$ cells (14, 41).Thus, an absence of Rad27p not only affects the stability of artificiallyintroduced short repeats in the yeast genome or on plasmids butalso has a severe effect on the stability of the natural telomericrepeats at chromosome ends. Given that the telomeric repeats areessential for chromosomal stability, it is possible that thistract instability may contribute significantly to the growth arrestobserved in rad27 $Delta$ strains grown at elevatedtemperatures.

Single-stranded template DNA of the lagging strand occurs in rad27 $Delta$ cells and in cells in which Dna2p is overexpressed. Several mechanisms have been proposed to explain the generation of repeat tract heterogeneity in rad27 $Delta$ cells (17, 26,28, 47). Most of them rely on the assumption that Rad27p indeedplays an important role in Okazaki fragment processing in vivo,a role that was suggested from the relatively well characterizedactivities that the mammalian homologue of this enzyme displaysin vitro (see reference 32 for a review). Some particularitiesoccurring during the replication of telomeric repeats allowedan examination of this prediction, at least at a qualitative level.First, due to the conserved polarity of the repeats at all telomeres,the G-rich strands will always be synthesized by leading-strandsynthesis and the C-rich strands by lagging-strand synthesis (seeFig. 1). Thus, by analyzing and comparing C-rich strand versusG-rich strand synthesis on telomeric repeats, one can gain insightsinto strand-specific effects of the gene product investigated.Second, after the last primer is synthesized on the most distallocation on telomeric repeats, there is no upstream primer thatmay mask the processing occurring on the 5' end of the downstreamprimer. Thus, inappropriate Okazaki fragment processing eventsthat are predicted to yield single-stranded regions on the templatestrand are detectable on telomeric repeats due to an absence offill-in synthesis from an upstream Okazaki fragment. We used anondenaturing in-gel hybridization technique (11) to examinethe occurrence of such predicted DNA intermediates on telomericrepeat DNA in strains lacking Rad27p (Fig. 3 through 5). Whilesingle-stranded regions on the C-rich strands, which serve astemplates for the leading-strand synthesis, were not detectablein any cells (Fig. 4A), a strong increase in single-stranded DNAof the G-rich strand is observed in rad27 $Delta$ cells compared to wild-typecells. Control experiments using a strand-specific, single-strandexonuclease demonstrated that this single-stranded DNA consistedof terminal overhangs as opposed to gaps (Fig. 4B). Consistentwith this finding, single-stranded DNA of either strand remainsundetectable at an internal location that is just about 500 bpproximal to the Y'-to-terminal-repeat junction (Fig. 5A). We interpretthese results to suggest that there is no detectable delay betweenparental-strand separation and new-strand synthesis on leading-strandsynthesis either in wild-type or in rad27 $Delta$ cells. On the otherhand, there appears to be a deficiency in lagging-strand synthesisin rad27 $Delta$ cells grown at elevated temperatures, since we observean accumulation of terminal single-stranded DNA of the G-richstrands in suchcells.

At least two possibilities could contribute to the generation of these single-stranded DNA overhangs: either priming itselfis inefficient during fork movement, creating at the very endsof the chromosomes single-stranded tails of the templating strand,or primer processing is aberrant in these cells. For instance,priming may actually occur to the very ends of the chromosome,but these newly synthesized Okazaki fragments may be dissociatedor degraded in an inappropriate way. Since Dna2p, an essentialhelicase and/or nuclease (2, 5, 7), interacts geneticallyand biochemically with Rad27p (6), we examined whether thisprotein was involved in such a process. Indeed, an increase ofsingle-stranded G-strand DNA can be observed in cells in whichDna2p was overexpressed (Fig. 7). The results also show that overexpressionof a full-length Dna2p caused arrest of cell growth (Table 1;Fig. 6), an effect that is not observed when a truncated Dna2protein lacking the N-terminal 105 amino acids was overexpressed(6). On the other hand, overexpression of an N-terminal portionof Dna2p causes a significant derepression of genes located neara telomere in yeast (44), supporting the notion that the N-terminalpart of Dna2p may play a significant regulatory role (2).

Our results are thus consistent with a model in which Rad27p and Dna2p work together to remove the 5' ribonucleotides fromnewly generated Okazaki fragments. In the absence of Rad27p, orwhen Dna2p is overexpressed, there may be excessive primer dissociationor degradation leading to single-stranded DNA of the templatingstrand. If this model was correct, one might expect that the actuallesions on the DNA in these two experimental settings were similarin nature, triggering growth arrest via similar pathways. Consistentwith this idea, rad27 $Delta$ cells incubated at 37°C, or cells in whichDna2p was overexpressed, displayed an identical arrest phenotypewith predominantly large, dumbbell-shaped cells (data not shown)(37, 45).

The exonuclease Exo1p is not redundant to Rad27p. Overexpression of Exo1p, a yeast 5'-3' exonuclease, has been reported to be able to suppress the temperature sensitivity andmutator phenotypes of rad27 $Delta$ cells (46). However, overexpressionof Exo1p from a high-copy-number vector had no diminishing effecton the appearance of the single-stranded G tails or on the lengthheterogeneity of the TRFs in rad27 $Delta$ cells (Fig. 8). Moreover,there was no detectable increase in such G tails when EXO1 wasdeleted or overexpressed in wild-type cells (Fig. 8) (12). Theseresults suggest that Exo1p and Rad27p are not simply redundantproteins for Okazaki fragment maturation but rather that the kindsof DNA lesions occurring in the absence of Rad27p require Exo1pfor repair (46). Overexpression of Exo1p also suppresses thegrowth defect of cells in which Dna2p is overexpressed (Table1). This is consistent with our model that overexpression ofDna2p induces similar lesions as an absence of Rad27p: Exo1p maybe required for the repair of the lesions in bothsituations.

These data thus provide direct in vivo evidence of single-stranded regions that occur on the templating strand when lagging-strandsynthesis is impaired. While in our experiments such single-strandedDNA was detectable only on the terminal repeats of the chromosome,we suppose that such single-stranded areas of the template strandalso occur in internal locations, as previously proposed (17,29, 47). Due to continued fill-in synthesis from an upstreamprimer, these internal lesions may be very transient and thereforenot detectable with the techniques used here. Consistent withthis idea, newly synthesized DNA isolated from rad27 $Delta$ cells containsa large proportion of relatively small DNA molecules, corroboratingthe evidence that Okazaki fragment maturation is impaired in thesecells (35). Chromosome ends in wild-type yeast cells acquirevery transient single-stranded G-strand extensions only late inS phase (54). We have previously shown that the generation ofat least some of these G tails is independent of an active telomeraseactivity but that it does require the passage of a replicationfork (11, 12). It is thus possible that in normal cells, thereis a short delay between the separation of the two parental strandsand the time when lagging-strand synthesis reaches the very endsof the template strands. This would create single-stranded G tailswhich could serve as templates for telomerase-mediated strandelongation. If lagging-strand synthesis is compromised, thoseG tails could persist and/or become even more extensive due toprimer dissociation (see above), leading to the effects reportedhere.

Thus, our results also emphasize the importance of lagging-strand synthesis in telomeric repeat maintenance. Recently, wereported that chromosome end processing events require the passageof a replication fork (12). Furthermore, deficiencies in theregulation of telomeric repeat lengths in yeast mutants affectedin DNA replication have been documented previously (1, 8),but the mechanisms involved remained unclear. Analyzing the specifictypes of DNA lesions found in those mutants may lead to insightsas to how telomeric tract length is regulated and more-detailedinsights into the coordination of the conventional replicationmachinery with telomeremaintenance.

	ACKNOWLEDGMENTS

We thank T. Formosa, J. Aron, M. Reagan, and E. Friedberg for generous gifts of plasmids and yeast strains. The members ofthe Wellinger lab are thanked for valuable discussions duringthisproject.

This work was supported by Canadian Medical Research Council grant MT 12616. J.P. received a studentship from the Fonds pourla Formation des Chercheurs et l'Aide à la Recherche (FCAR),and R.J.W. is a Chercheur-Boursier Senior of the Fonds de la Rechercheen Santé du Québec(FRSQ).

	FOOTNOTES

^* Corresponding author. Mailing address: Département de Microbiologie et Infectiologie, Faculté de Médecine, Universitéde Sherbrooke, 3001 12 Ave. Nord, Sherbrooke, Quebec, J1H 5N4,Canada. Phone: (819) 564-2514. Fax: (819) 564-5392. E-mail: rwelli01{at}courrier.usherb.ca.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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