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Differential Processing of Leading- and Lagging-Strand Ends at Saccharomyces cerevisiae Telomeres Revealed by the Absence of Rad27p Nuclease
Julie Parenteaua and Raymund J. Wellingeraa Département de Microbiologie et Infectiologie, Faculté de Médecine, Université de Sherbooke, Sherbooke, Quebec J1H 5N4, Canada
Corresponding author: Raymund J. Wellinger, Faculté de Médecine, Université de Sherbooke, 3001 12 Ave. Nord, Sherbooke, Quebec J1H 5N4, Canada., raimund.wellinger{at}usherbrooke.ca (E-mail)
Communicating editor: L. PILLUS
 | ABSTRACT |
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Saccharomyces cerevisiae strains lacking the Rad27p nuclease, a homolog of the mammalian FEN-1 protein, display an accumulation of extensive single-stranded G-tails at telomeres. Furthermore, the lengths of telomeric repeats become very heterogeneous. These phenotypes could be the result of aberrant Okazaki fragment processing of the C-rich strand, elongation of the G-rich strand by telomerase, or an abnormally high activity of the nucleolytic activities required to process leading-strand ends. To distinguish among these possibilities, we analyzed strains carrying a deletion of the RAD27 gene and also lacking genes required for in vivo telomerase activity. The results show that double-mutant strains died more rapidly than strains lacking only telomerase components. Furthermore, in such strains there is a significant reduction in the signals for G-tails as compared to those detected in rad27
cells. The results from studies of the replication intermediates of a linear plasmid in rad27 cells are consistent with the idea that only one end of the plasmid acquires extensive G-tails, presumably the end made by lagging-strand synthesis. These data further support the notion that chromosome ends have differential requirements for end processing, depending on whether the ends were replicated by leading- or lagging-strand synthesis.
TELOMERES, the complex nucleoprotein structures at the ends of eukaryotic chromosomes, are essential for chromosome integrity: they protect chromosome ends from degradation and random fusion events (
30-base G-tail specifically during S-phase, when the telomeres are replicated (
Although there is mounting evidence that conventional DNA replication and the specialized replication to maintain telomeric repeats are interrelated, little is known about mechanistic details of how this coordination is achieved (
3' direction (reviewed in cells, an appearance of an abnormally large amount of G-tails can be detected ( cells. Alternatively, it remained possible that the generation of the excess G-tails in rad27 cells was due to an interference with the coordination of telomerase activity with the lagging-strand machinery or an abnormally high activity of the nucleolytic activities required to process leading-strand ends.
To distinguish between these possibilities and to further examine the participation of telomerase in the appearance of single-stranded DNA in rad27 cells, we have constructed several haploid yeast strains that carry a rad27 mutation and mutations in genes implicated in telomerase activity. One of the predictions was that if Rad27p functions in lagging-strand DNA synthesis alone, the combined absence of telomerase activity and Rad27p in yeast cells should result in an accelerated loss of telomeric repeats. Indeed, we observe that cells with a deletion of RAD27 and lacking telomerase components are not able to grow for the same number of generations as cells lacking only telomerase. In addition, the relative signals for G-tails on telomeres derived from the double-mutant strains were significantly higher than those from wild type or telomerase-lacking strains. These data suggest that in telomeric DNA, an absence of Rad27p results primarily in incomplete synthesis of the C-rich strands, generating an excess of G-tails. These G-tails may then be further elongated in a telomerase-dependent fashion. The analyses of replication intermediates of a linear plasmid derived from rad27 cells further corroborate this conclusion in that they suggest that excess G-tails occur on only one end of the plasmid, presumably the end replicated by lagging-strand synthesis. We interpret these data to support the notion that chromosomal ends are processed differently, depending on whether the newly synthesized strand on a particular end was generated by leading- or lagging-strand synthesis (
| MATERIALS AND METHODS |
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Strains and plasmids:
Yeast strains used in this study are listed in Table 1. UCC3535 (gift of M. Singer and D. Gottschling; ::URA3 (obtained from E. Friedberg and M. Reagan; ::URA3 (a gift from E. Friedberg and M. Reagan;
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Yeast cells were transformed by a modification (
Media, senescent phenotype, and survivors:
Indicated heterozygous diploids that have the same nonsenescent phenotype as a wild-type diploid were grown at 30° and sporulated at room temperature. After tetrad dissection, only tetratypes were selected for study by growth on SC-Leu (tlc1::LEU2), SC-His (est1::HIS3 and est3::HIS3), or SC-Ura (rad27::URA3) plates. The cdc13-2est mutant was selected by its senescence phenotype. The apparent senescence phenotype (
20 generations) onto rich growth medium (YPD) in quarter-plate sectors for single colonies (Fig 1). After this first restreak, cells were estimated to have grown for 40 generations. After 4 days of growth at the permissive temperature for rad27::URA3 cells (23°), single colonies derived from the first streak were restreaked on a second YPD plate for single colonies (60 generations). This procedure was repeated a third time to allow the population to have grown for 80 generations. At this stage, the vast majority of cells were unable to form normal colonies (senescence), but a few normal-looking colonies did emerge. Such colonies are termed survivors (160 generations after germination. Single colonies were grown in liquid media at 23° for 10 additional generations for DNA analysis.
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DNA isolation:
For Fig 2 and Fig 3, yeast cultures were grown in YPD at the permissive temperature for rad27::URA3 strains to midlogarithmic phase [optical density at 660 nm (OD660) = 0.4–0.6] and then shifted to semipermissive temperature (30°) or to restrictive temperature (37°) for 12 hr. Total genomic DNA from these cells was isolated using a modified glass bead procedure (::URA3 cells containing YLpFAT10 were grown in SC-Trp medium at 23° to midlogarithmic phase and shifted to restrictive temperature (37°) for 8 hr. DNA was isolated by a "Hirt" extraction that enriched for low-molecular-weight DNA (
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Southern blot analysis, in-gel hybridization, and two-dimensional agarose gel:
Agarose gel techniques, Southern blot transfers to nylon membranes, and hybridization conditions were as described previously (42 hr in 0.37% agarose. For the second dimension, lanes were excised from the first dimension gel, rotated 90°, imbedded in 1.1% agarose containing 1 µg/ml ethidium bromide, and run at 10 V/cm for 4 hr in the presence of 1 µg/ml of ethidium bromide at 4°. DNA used as probes were pVZ1 (
Quantification for all signals was obtained by storage phosphorimaging with a Storm and ImageQuant software. In the native gel, the integrated volume used comprised the entire lane, background values derived from an area lacking a signal were subtracted, and the resulting value was divided by the corrected volume integrated of the same lane in the denatured gel. For 2D gels, the area described for each experiment was integrated, a background was subtracted, and the resulting value was divided by an internal standard value as indicated. The values obtained for the wild-type strains were set as 1; values of the indicated mutant strains are expressed relative to this wild-type value. Care was taken to ensure that the signals never exceeded the capacity of the storage phosphor plates.
| RESULTS |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Enhancement of senescence phenotype in rad27 telomerase-minus strains:
In vivo telomerase activity in yeast requires at least five genes: TLC1, encoding the RNA component of telomerase, as well as EST1, EST2, EST3, and CDC13 (for review see 80 generations (, the wild type and rad27 segregants grow normally without any senescence phenotype. However, cultures derived from spores with mutations in the genes encoding telomerase components (i.e., tlc1, est1, est3, or cdc13-2est) died at an average of 70–85 generations after germination. The double-mutant strains (i.e., strains harboring rad27 and one of the above mutations affecting telomerase components) died more rapidly than strains carrying only the mutations in telomerase: our analysis determined senescence to occur in these strains between 35 and 50 generations after germination (Table 2). For example, rad27 est1 double-mutant cells already yielded colonies of variable sizes with predominantly small colonies upon the first streaking (40G) after the dissection plate (Fig 1A). These small rad27 est1 colonies did not grow further whereas est1 single mutants began to lose viability after only 60 divisions (Fig 1A). We obtained essentially the same results for the rad27 cdc13-2est double-mutant strain (Fig 1B), as well as for the rad27 est3 and rad27 tlc1 strains (Table 2 and data not shown). As anticipated, even in the single telomerase mutants, the number of generations required for the senescence phenotype to appear is variable within a certain range (see the ranges in Table 2). While we find a similar variation for the occurrence of senescence in the double mutants, it is clear that overall senescence onset is earlier. Thus, the rad27 mutation caused an accelerated senescence phenotype in strains also lacking components required for in vivo telomerase activity.
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Additive contribution to the generation of G-tails by Rad27p and telomerase:
To establish the contribution of telomerase in the abnormally high levels of G-tails detected in rad27 cells grown at the restrictive temperature (1.3 kb is due to a conserved site in the subtelomeric Y' element that is present on most telomeres (Y' TRFs; EST1/est1 heterozygous diploid is shown in Fig 2. Spore cultures of the indicated genotype were pregrown at 23° and then split and incubated at the indicated temperatures (see MATERIALS AND METHODS). Note that rad27 strains will grow only a few generations at 37° and then will stop growing ( cells is vastly enhanced when cells are grown at 37°, allowing for a more quantitative determination of the amount of G-tails occurring (Fig 2C). On the native gel (Fig 2A), only a very faint signal for single-stranded telomeric G-strands was detected for the wild type (Fig 2A, lanes 2–4) and the est1 strains (Fig 2A, lanes 8–10) as expected and shown previously ( cells grown at 23°, and these signals are vastly augmented when the cells are grown at 37° (Fig 2A, compare lanes 5 and 7; est1 double-mutant cells (Fig 2A, lanes 11–13) a similar effect was observed, yet the signals for the G-tails did not reach the same level as those observed for the rad27 cells at the same temperatures. Rehybridization of the very same gel after DNA denaturation showed about equal amounts of DNA in each lane. In addition and as expected, telomere shortening could be seen in est1 strains: the length of Y' TRFs was 1 kb in strains lacking Est1p, whereas it was 1.3 kb in the wild type and rad27 cells (Fig 2B, arrows). Finally, as reported previously, TRFs became very heterogeneous in both strains lacking Rad27p and incubated at 37° (Fig 2B, lanes 7 and 13;
The relative signals for single-stranded DNA observed on DNA derived from cells incubated at 23° and 37° in the native gels (Fig 2A) were quantified using a PhosphorImager and corrected for DNA loading using the denatured gel (Fig 2B; see MATERIALS AND METHODS). Compared to the values obtained for the wild-type strain at the same temperature, it is clear that there is significantly more single-stranded G-rich telomeric DNA in rad27 strains (Fig 2C). However, we consistently observed 1.7-fold less signal for G-tails in the rad27 est1 double-mutant cells as compared to the rad27 strains (Fig 2C). For example, the mean values for rad27 cells were 12.2 (23°) and 58 (37°), whereas those for rad27 est1 cells were 7.3 (23°) and 32.1 (37°). DNA derived from cells with a deletion of EST1 alone scored indistinguishably from wild type at all temperatures. Virtually identical results were obtained with individual spore cultures of a tetratype derived from the RAD27/rad27 TLC1/tlc1 heterozygous diploid (data not shown). These data suggest that telomerase and the defects of lagging-strand DNA synthesis occurring in yeast cells carrying a deletion of RAD27 each contribute a significant portion to the induction of the extensive G-tails.
Rad27p is not required to produce survivors in telomerase-minus cells:
The accelerated death phenotype observed in the rad27 telomerase-minus double-mutant strains is reminiscent of the situation observed for rad52 telomerase-minus double-mutant cells (80 generations. However, RAD52-dependent rearrangements and amplifications of telomere regions can result in the generation of cells that maintain functional telomeres (survivors, Fig 3A; telomerase-minus mutant cells had the same accelerated death phenotype as rad52 telomerase-minus cells, we wanted to know whether Rad27p is also required for the mechanisms to generate survivors. Thus, RAD27 TLC1, rad27 TLC1, RAD27 tlc1, and rad27 tlc1 cells were streaked onto solid media past the senescence point (80 generations; Fig 1 and Fig 3A), and after 160 generations, single colonies were grown in liquid media at 23° for 10 additional generations for DNA analysis. Genomic DNA was extracted and telomeric DNA pattern was assessed by digesting DNA with XhoI. Occasional occurrence of healthy looking colonies (survivors) was very similar in streaks of tlc1 and rad27 tlc1 cells (Fig 3A). Moreover, type I as well as type II survivors can arise in strains lacking Rad27p and telomerase (Fig 3B, lane 8: type I; lane 9: type II). Consequently, Rad27p is not required to produce survivors in yeast cells lacking telomerase activity.
Accumulation of single-stranded DNA in rad27 occurs at only one end of a linear plasmid:
Rad27p was proposed to be among the candidate exonucleases responsible for the processing of the blunt-ended telomeres left after leading-strand DNA synthesis. Using two-dimensional agarose gel electrophoresis, it was previously shown that the linear plasmid YLpFAT10 can form telomere-telomere interactions that are dependent on the presence of G-rich tails on both ends of the plasmid (100 nucleotides, the fraction of DNA molecules with telomere-telomere interactions depends on the length of the TG1–3-tails: the longer the G-tails are, the higher the signal of circular plasmids ( cells. However, quantitation of the signals for CFP with respect to either the signals for replication intermediates (RI1 and RI2 in Fig 4) or the linear form of the plasmid (1N in Fig 4) showed no significant difference in CFP formation, even if the rad27 cells were incubated at 37° and extensive G-tails were observed on telomeres (Table 3). This result suggests that in rad27 cells, the generation of G-tails was confined to one end of the plasmid, which we presume is the lagging-strand end. In addition, if Rad27p was the exonuclease processing the leading-strand ends, its absence could have created a situation in which the leading-strand ends remained blunt ended after replication. In this case, we expected a decrease in the signal for CFP in rad27 cells as compared to wild-type cells, since G-tailed ends will not interact with a double-stranded and blunt-ended tract of telomeric repeats, at least in vitro ( cells are normally processed at one end, presumably the one synthesized by leading-strand DNA synthesis, and abnormally processed at the other end, the one made by lagging-strand DNA synthesis. Hence, Rad27p would not be the 5'–3' exonuclease responsible for the processing of the blunt end at leading-strand telomeres.
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| DISCUSSION |
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| TOPABSTRACTMATERIALS AND METHODSRESULTSDISCUSSIONLITERATURE CITED |
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Some components of the replication machinery appear to be involved in the control of telomere length. For example, cells carrying temperature-sensitive (Ts) alleles of DNA polymerase 
(CDC17/POL1) harbor very long telomeres (
We have previously shown that, like a strain harboring Ts alleles of the CDC17 gene (pol1-17), strains with a RAD27 deletion display an accumulation of G-tails when grown at a semipermissive temperature ( as well as DNA polymerase 
are required in vivo for telomerase-mediated elongation of the 3' TG1–3 strand ( appears to at least temporarily interact with components of telomerase (
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Consistent with our model described above, the overall length of the telomeric-repeat tracts in rad27 cells becomes very heterogeneous (35–50 generations after germination, while telomerase-lacking cells die after 70–85 generations (see also Table 2). However, this accelerated death phenotype is not specific for rad27 telomerase-minus cells. rad52 telomerase-minus double mutants display a comparable accelerated senescence ( telomerase-minus cells have the additional property of being unable to generate survivors, that is, cells that can maintain telomeric repeats in the absence of telomerase ( rad52 cells display a synthetic lethality ( telomerase-minus cells (Fig 3A) and after analysis of the chromosome terminal restriction fragments recovered from such survivors, patterns typical for both type I and type II events can be documented (Fig 3B). We conclude that Rad27p is not required for the establishment of survivors in telomerase-lacking cells and that the reasons for the accelerated senescence in rad27 telomerase-minus cells may be different from those for rad52 telomerase-minus cells.
All the data are most consistent with a defect in rad27 cells of the generation and/or processing of lagging strands on telomeric repeats, as described above. On any linear DNA molecule, only one telomere, the one replicated by lagging-strand synthesis, would thus be predicted to be affected by this defect. To test this hypothesis, the replication intermediates (RIs) of a short linear plasmid called YLpFAT10 were analyzed by two-dimensional gel electrophoresis. Extensive analyses of the RIs of this linear plasmid isolated from wild-type cells have shown that replication initiated in the predicted area of the plasmid and that its telomeres acquired long G-tails in late S-phase, as chromosomal telomeres do (
The study presented here thus underscores the differential requirements for telomere maintenance on ends replicated by leading- vs. lagging-strand synthesis. The data demonstrate that interfering with components of the lagging-strand machinery causes defects in telomeric DNA end structures, which can result in increased losses of telomeric repeats. Furthermore, the results suggest that in the particular case of Rad27p, only the ends replicated by lagging-strand synthesis are affected. This implies that the leading-strand ends may be processed normally in the absence of Rad27p and suggests that Rad27p is not part of the nucleases that act on such ends to generate short G-tails. The enzymatic activities responsible for this processing remain enigmatic, even if in one case the MRE11/RAD50/XRS2 complex has been proposed to fulfill this function (
| ACKNOWLEDGMENTS |
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We thank V. Lundblad, M. Singer, D. Gottschling, E. Friedberg, and M. Reagan for providing strains and plasmids used in these studies. The members of the Wellinger lab are thanked for helpful discussions throughout this project. This research was supported by a grant (no. MOP 12616) from the Canadian Institutes of Health Research (CIHR) to R.J.W. J.P. was a recipient of a studentship of the Fonds pour la Formation des Chercheurs et l'Aide à la Recherche (FCAR) and R.J.W. is a Chercheur National supported by the Fonds de la Recherche en Santé du Québec (FRSQ).
Manuscript received May 28, 2002; Accepted for publication September 16, 2002.
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