Cdc13 both positively and negatively regulates telomere replication

doi:10.1101/gad.861001

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Vol. 15, No. 4, pp. 404-414, February 15, 2001

RESEARCH PAPER
Cdc13 both positively and negatively regulates telomere replication

Abha Chandra,¹ Timothy R. Hughes,²^,³ Constance I. Nugent,¹^,⁴ and Victoria Lundblad¹^,²^,⁵

¹ Department of Molecular and Human Genetics and ² Program in Cellular and Molecular Biology, Baylor College of Medicine, Houston, Texas 77030, USA

ABSTRACT

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Cdc13 is a single-strand telomeric DNA-binding protein that positively regulates yeast telomere replication by recruitingtelomerase to chromosome termini through a site on Cdc13 thatis eliminated by the cdc13-2 mutation. Here we show that Cdc13has a separate role in negative regulation of telomere replication,based on analysis of a new mutation, cdc13-5. Loss of this secondregulatory activity results in extensive elongation of the G strandof the telomere by telomerase, accompanied by a reduced abilityto coordinate synthesis of the C strand. Both the cdc13-5 mutationand DNA polymerase $alpha$ mutations (which also exhibit elongated telomeres)are suppressed by increased expression of the Cdc13-interactingprotein Stn1, indicating that Stn1 coordinates action of the laggingstrand replication complex with the regulatory activity of CDC13.However, the association between Cdc13 and Stn1 is abolished bycdc13-2, the same mutation that eliminates the interaction betweenCdc13 and telomerase. We propose that Cdc13 participates in tworegulatory steps $---$ first positive, then negative $---$ as a result ofsuccessive binding of telomerase and the negative regulator Stn1to overlapping sites on Cdc13. Thus, Cdc13 coordinates synthesisof both strands of the telomere by first recruiting telomeraseand subsequently limiting G-strand synthesis by telomerase inresponse to C-strand replication.

[Key Words: Telomere; telomerase; Cdc13; Stn1; DNA replication]

	Introduction

Top Abstract Introduction Results Discussion Materials and methods References

Telomeres are guanine-rich, simple repeat sequences that constitute the physical ends of eukaryotic chromosomes. The sequenceand structure of these specialized DNA termini permits extensionof the G strand by the enzyme telomerase, thereby counteractingsequence loss due to incomplete replication or degradative activities(Lingner et al. 1995; Greider 1996). In yeast and human cells,a telomerase deficiency leads to a progressive decline in telomerelength that inhibits the proliferative capacity of the cell andheralds replicative senescence (Lundblad and Szostak 1989; Bodnaret al. 1998). Analysis of telomerase-deficient mice has also revealedan essential role for telomere maintenance in the long-term viabilityof high-renewal organ systems (Lee et al. 1998). Furthermore,loss of telomerase in the absence of checkpoint function can alsopromote genetic instabilities and carcinogenesis, especially inhighly regenerative tissues (Chin et al. 1999; Artandi et al.2000), illustrating the importance of telomeres in maintaininggenomicstability.

Increasing attention has been directed at the importance of coordinating G-strand synthesis by telomerase with replicationof the C strand of the telomere. Following extension of the 3'terminus of the G-rich strand by telomerase, fill-in synthesisof the other strand, presumably by the machinery that normallyperforms lagging strand DNA replication, is thought to be necessaryto prevent elongated single-stranded regions at chromosome termini.Several recent studies indicate that disruption of C-strand DNAsynthesis can impair telomere length control (for review, seePrice 1997; Evans and Lundblad 2000). In the ciliate Euplotes,inhibition of DNA polymerases $alpha$ and $delta$ during de novo telomeresynthesis alters the length of the telomeric C strand and alsocauses an increase in the length and heterogeneity of the G strand(Fan and Price 1997). Similarly, propagation of S. cerevisiaestrains defective for components of the lagging strand DNA replicationmachinery cause a telomerase-dependent increase in telomere length(Carson and Hartwell 1985; Adams and Holm 1996; Adams Martin etal. 2000). In addition, de novo telomere formation at a newlycreated double-strand break requires not only telomerase but alsoDNA polymerase $alpha$ and $delta$ (Diede and Gottschling 1999). Collectively,these results indicate that in both yeast and ciliates, G-strandand C-strand synthesis are tightly coregulated, although the molecularmechanism for this coordination has not beenelucidated.

In yeast, a critical contributor to several aspects of telomere function is the protein Cdc13, which exhibits high affinitysequence-specific binding for single-stranded telomeric DNA (Linand Zakian 1996; Nugent et al. 1996; Hughes et al. 2000a). Consistentwith this substrate specificity, Cdc13 is associated with thetelomere during S phase (C.I. Nugent and V. Lundblad, in prep.),which correlates with the transient increased single-strand G-richextension observed at yeast telomeres (Wellinger et al. 1993,1996). CDC13 performs an essential activity necessary to protectchromosome termini, as loss of CDC13 function is accompanied byimmediate and extensive loss of one strand of the telomere (Garviket al. 1995; Diede and Gottschling 1999). In addition to thisend protection function, CDC13 positively regulates telomere replicationby recruiting telomerase to the telomere, an activity that isabolished by the cdc13-2 missense mutation. The cdc13-2 strain,which is normal for telomeric end protection, exhibits a telomerereplication defect similar to that of a strain that lacks telomerase(Nugent et al. 1996), although telomerase activity in cell-freecdc13-2 extracts is unaffected (Lingner et al. 1997). This defectis partially suppressed by increased expression of the telomerase-associatedEst1 protein (Nugent et al. 1996), and a complex containing bothproteins can be coimmunoprecipitated in yeast, using overexpressedrecombinant versions of Est1 and Cdc13 (Qi and Zakian 2000). Furthermore,the cdc13-2 mutation can be reciprocally suppressed by a specificmissense mutation in EST1 (Pennock et al. 2001), thereby demonstratingthat positive regulation of telomere replication by Cdc13 is dueto a direct interaction between Cdc13 and a subunit of telomerase,resulting in recruitment of the enzyme to thetelomere.

In addition to this positive regulatory role, Cdc13 has been implicated in negative control of telomere length. The thermolabilecdc13-1 mutant exhibits greatly elongated telomeres when grownat intermediate temperatures (Grandin et al. 1997). However, thismutant strain is also severely impaired for the essential endprotection function of CDC13 (Garvik et al. 1995; Diede and Gottschling1999); therefore, analysis of the cdc13-1 mutation has not clarifiedwhether the proposed role in negative length control is distinctfrom the essential function of CDC13. An additional factor thatcontributes to negative length regulation is the Cdc13-interactingprotein Stn1. These two proteins associate in a two-hybrid assayand display a number of genetic interactions, suggesting thatStn1 and Cdc13 function together at the telomere as a complex(Grandin et al. 1997). Furthermore, a mutation in STN1 increasestelomere length by ~1 kb, leading Charbonneau and colleagues topropose that Stn1 is a negative regulator of telomere length (Grandinet al. 1997, 2000). Cdc13 is also associated with DNA polymerase $alpha$ , although mutations that disrupt this association have onlya modest (50-150 bp) increase in telomere length (Qi and Zakian2000); therefore, the contribution of the Cdc13-Pol $alpha$ associationto telomere length control isunclear.

We describe here the identification of a mutation of CDC13, cdc13-5, that exhibits a striking defect in negative regulationof telomere length, with no impact on the essential function ofCDC13. In this strain, telomere length is increased by $>=$ 1000 bpas a result of unregulated elongation of the G-rich strand bytelomerase. This is accompanied by a reduced ability to coordinatesynthesis of the C-rich strand, resulting in chromosome terminiwith greatly extended single-strand extensions of the G strand.The cdc13-5 defect is dependent on the ability to recruit telomeraseto the telomere, as cdc13-5-mediated telomere elongation is blockedby the cdc13-2 mutation. Genetic interactions between the cdc13-5mutation and DNA polymerase $alpha$ also implicate misregulation ofC-strand synthesis in this mutant phenotype. Therefore, cdc13-5defines a role for Cdc13 in coordination of the synthesis of thetwo strands of the telomere, which is distinct from the telomeraserecruitment activity defined by the cdc13-2 mutation. We proposethat these two regulatory activities of Cdc13 correspond to twodistinct steps in telomere replication that coordinate and regulatesynthesis of the two strands of the telomere. In the first step,Cdc13 initiates telomere replication by recruiting telomerase,which extends the 3' terminus of the G strand of the telomere.In the second step, fill-in synthesis of the C strand by laggingstrand synthesis machinery acts to limit extension of the G strandby telomerase, an inhibitory activity that is defective in thecdc13-5 mutant. We further suggest that these two steps are theconsequence of successive binding of the telomerase-associatedEst1 subunit and the negative regulator Stn1 to overlapping bindingsites on Cdc13. By relying on a single protein as the regulatorycenter, this proposed mechanism provides a simple means for coordinatingsynthesis of the two strands of thetelomere.

	Results

Top Abstract Introduction Results Discussion Materials and methods References

Cdc13 is a negative regulator of telomerase

As part of our investigation of the Cdc13 protein, we uncovered two alleles of CDC13, cdc13-3 and cdc13-5, that result ina pronounced defect in telomere length maintenance. The telomerictract, which is normally ~350 bp in a wild-type strain, was elongatedby ~500-1000 bp in cdc13-5 and cdc13-3 strains, along with anaccompanying increase in telomere length heterogeneity (Fig. 1A).The cdc13-3 mutation was the result of an alanine scan mutagenesisof CDC13 (Hughes 1998) and mapped to residues 695-699 at the C-terminalboundary of the Cdc13 DNA-binding domain. Western analysis, usingan N-terminally epitope-tagged version (HA3-Cdc13-3), indicatedthat the mutant Cdc13-3 protein apparently existed in two formsin yeast: the full-length 105-kD protein and a truncated versionthat migrated at ~80 kD, with both variants present in substantiallyreduced levels relative to the wild-type full-length Cdc13 protein(data not shown). We surmised that the cdc13-3 mutation resultedin an unstable protein that was readily proteolyzed to remove~20 kD from the C-terminal region of the protein. To test directlywhether removal of the C terminus of Cdc13 was responsible fortelomere elongation, an additional allele, cdc13-5, was constructedby the introduction of a stop codon following amino acid 694,which truncated the Cdc13 protein by 230 amino acids. This truncationoccurs at the boundary of the DNA-binding domain, which can beexpressed separately as a stable polypeptide (Hughes et al. 2000a).The cdc13-5 mutant yeast strain exhibited extensive telomere elongationto a degree roughly comparable to that observed with the cdc13-3strain (Fig. 1A). As described in more detail later in this article,the cdc13-5 strain also grew as well as a wild-type strain. TheCdc13-5 protein was also produced at levels comparable to wild-typeprotein (Fig. 1B) in contrast to the situation with the cdc13-3mutant strain. Therefore, unless otherwise noted, the experimentsdescribed in this article were conducted with the cdc13-5 allele.

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Figure 1. Cdc13 is a negative regulator of telomere elongation. (A) Telomere length of CDC13⁺ (lane 1), cdc13-3 (lane 2), and cdc13-5 (lane 3). The cdc13-3 and cdc13-5 haploid strains were derived from DVL233 and DVL326, respectively, by tetrad dissection; DNA was prepared after ~35 generations of growth. (B) Anti-HA immunoblot of anti-HA immunoprecipitates from equal amounts of whole cell extract prepared from a cdc13- $Delta$ strain expressing HA3-Cdc13 (lane 1; pVL841), HA3-Cdc13-5 (lane 2; pVL903) and untagged Cdc13 (lane 3; pVL440); all plasmids were single-copy CEN vectors, with CDC13 expressed from its native promoter. Arrowheads indicate the full-length Cdc13 protein (~116 kD) and the truncated Cdc13-5 protein (~80 kD). (C) Telomere length of CDC13/cdc13-5 EST1/est1- $Delta$ RAD52/rad52- $Delta$ (lane 1), CDC13⁺ (lane 2), rad52- $Delta$ (lane 3), cdc13-5 (lanes 4,5), cdc13-5 rad52- $Delta$ (lanes 6,7), est1- $Delta$ (lane 8), and cdc13-5 est1- $Delta$ (lane 9). The haploid strains shown in lanes 2-9 were obtained from DVL328 (lane 1) by tetrad dissection; DNA was prepared after ~35 generations of growth, except for lanes 5 and 7, which were grown for an additional 10 generations. (D) Telomere length of cdc13-5 (lane 1), cdc13-2,5 (lane 2), cdc13-2 (lane 3), and CDC13⁺ (lane 5); strains were generated by transforming cdc13- $Delta$ /pVL438 with pVL1033 (cdc13-5), pVL1360 (cdc13-2,5), pVL690 (cdc13-2), and pVL440 (CDC13), followed by eviction of pVL438 on 5-FOA. Although a cdc13-2,5 strain exhibits a senescence phenotype characteristic of a telomere replication defect, telomere length of the cdc13-2,5 strain is reproducibly not quite as short as the cdc13-2 strain at any given time point (cf. lanes 2 and 3). This may be caused by residual recruitment activity of the Cdc13-2 mutant protein (which is consistent with the prior demonstration that the senescence phenotype of a cdc13-2 strain is somewhat delayed relative to telomerase null mutations; Lendvay et al. 1996

), thereby allowing partial manifestation of the cdc13-5 defect.

To determine whether the increase in telomere length was mediated by telomerase or recombination, telomerase-defective andrecombination-defective cdc13-5 double mutant strains were examined.In a cdc13-5 strain that lacked telomerase (cdc13-5 tlc1- $Delta$ orcdc13-5 est1- $Delta$ ), telomere elongation was abolished, and the doublemutant strain showed the senescence phenotype characteristic oftelomerase null strains (Fig. 1C; data not shown). In contrast,telomere length in the cdc13-5 strain was unaffected by loss ofthe major pathway for homologous recombination, as elongationoccurred to the same degree in cdc13-5 rad52- $Delta$ and cdc13-5 RAD52strains (Fig. 1C). Therefore, the greatly elongated telomeresobserved in the cdc13-5 strain are the result of action by telomerase.The cdc13-5 mutation was recessive to CDC13⁺, indicating that the ability to negatively regulate telomerelength is a property of the wild-type protein (Fig. 1C).

CDC13 also has a positive role in maintaining telomere length, which is eliminated by the cdc13-2 mutation (Nugent et al.1996). One model consistent with both positive and negative regulatoryroles for CDC13 proposes that the wild-type Cdc13 protein firstrecruits telomerase (an activity that is lost in the cdc13-2 mutant)and then subsequently acts to limit the degree of extension ofthe G-rich strand by telomerase (an activity that is lost in thecdc13-5 mutant). A prediction of this model is that an alleleof CDC13 that contains both mutations should fail to recruit telomeraseand, therefore, should not result in elongated telomeres. Consistentwith this prediction, a cdc13-2,5 strain, with both regulatorymutations introduced into the CDC13 gene, no longer exhibitedlong telomeres. Instead, telomeres were short (Fig. 1D), and thecdc13-2,5 strain showed a senescence phenotype (data not shown).Therefore, the loss of regulation of telomere length exhibitedby the cdc13-5 mutation depends on the telomerase recruitmentfunction of CDC13.

The cdc13-5 mutation results in greatly increased single-strand extension of the G-rich strand of the telomere

One means by which telomerase synthesis could become unregulated could be because of a loss of coordination between G-strandand C-strand synthesis. Impairment of DNA polymerase $alpha$ resultsin elongated telomeres, as well as an increase in the extent ofthe terminal single-strand extension of the G-rich strand (Carsonand Hartwell 1985; Adams and Holm 1996; Fan and Price 1997; AdamsMartin et al. 2000). To examine whether the cdc13-5 mutant similarlyaffected the extent of single-stranded G-rich DNA, nondenaturingin-gel hybridization was used to examine chromosome termini. Inwild-type yeast, the G-rich strand can only be readily detectedas single stranded in late S phase, whereas at other points inthe cell cycle, the chromosome terminus is either blunt or theoverhang is below the detection limit (<30 bases; Wellinger etal. 1993). Therefore, due to both detection limits and the transientnature of the single strandedness of the G strand during S phase,single-stranded yeast termini cannot be reliably detected in asynchronouscultures of wild-type cells. However, when unsynchronized culturesof both cdc13-3 and cdc13-5 mutant strains were examined, G-richsingle-strand telomeric signals were readily detected using astrand-specific probe (Fig. 2A). Treatment with Escherichia coliExoI, a 3' $right-arrow$ 5' single-strand exonuclease, abolished the signal,arguing for the presence of a terminal single-stranded G-richoverhang, as opposed to internal gaps or nicks. Moreover, no singlestrandedness corresponding to the C-rich strand was detected (datanot shown). Strand separation gels that measured the length ofthe C strand showed that this strand was also elongated in a cdc13-5strain, relative to the length of the C strand in a wild-typestrain (data not shown). Therefore, the increased single strandednessof the G strand does not appear to be caused by extensive resectionof the C strand. These results indicate that increased elongationof the G strand by telomerase in this mutant strain is accompaniedby a loss in coordination of the synthesis of the C strand.

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Figure 2. The cdc13-5 strain exhibits an altered end structure during S phase. (A) DNA from CDC13⁺, cdc13-3, and cdc13-5 strains were mock treated (lanes 3,5,7) or treated with ExoI (lanes 4,6,8), digested with XhoI, and analyzed by nondenaturing in-gel hybridization with a C_1-3A oligonucleotide probe (top); the same gel, denatured and rehybridized with the same oligonucleotide probe (bottom); lanes 1,2: pVL260 (with 80 bp of G_1-3T telomeric repeat DNA) heat denatured or nondenatured, respectively. Size markers: $lambda$ HindIII-digested DNA. (B) DNA from a cdc13-5 strain, prepared from time points collected every 20 min after release from an $alpha$ factor-induced G₁ arrest, was examined by native in-gel hybridization with a C_1-3A oligonucleotide probe (top, left), denaturation and rehybridization with the same probe (bottom, left), and FACS analysis (right); lanes 1,2: pVL260, denatured or nondenatured, respectively.

The elongated terminal extensions detected in a cdc13-5 strain could reflect a defect during S phase, when telomere synthesisby telomerase occurs (Marcand et al. 2000). The alternative possibilityis that the altered G tails in the cdc13-5 mutant are the consequenceof an alteration in end structure that persists throughout thecell cycle, such as that observed in yku70 and yku80 mutants (Gravel et al. 1998; Polotnianka et al. 1998), possiblyas a consequence of exposure of telomeres to unregulated activitiesother than telomerase. To distinguish between these two possibilities,we determined whether extensive elongation of the G-rich strandcould be detected at different periods of the cell cycle, usingsynchronized cultures of the cdc13-5 mutant strain. Cells werearrested with $alpha$ factor in G₁ and subsequently released, and theG-rich strand of the telomere was examined on native gels usinga strand-specific probe (Fig. 2B). When cells were arrested inG₁, no telomeric single strandedness could be detected. However,40-60 min after release, when FACS analysis indicated that themajority of cells had entered S phase, the cdc13-5 mutant exhibiteda peak of single-stranded G-rich telomeric DNA. This signal declinedas the cells exited S phase and increased again during the nextcell cycle, although the peak of the signal became less pronouncedas the culture became more asynchronous. These results indicatethat the single-stranded G tail is a substrate for extended synthesisby telomerase during S phase, resulting in the telomere lengthdefect observed in the cdc13-5 mutantstrain.

Overexpression of STN1 suppresses cdc13-5 and pol $alpha$ telomere length defects

The similarity in phenotypes of the cdc13-5 and DNA polymerase $alpha$ mutant strains suggests that the same step in telomere replicationmay be affected, which is also consistent with the recent demonstrationthat Cdc13 and DNA Pol $alpha$ can be coimmunoprecipitated (Qi and Zakian2000). To provide further support for a functional relationshipbetween these two proteins, we asked whether alterations in thelevel of the Cdc13-interacting protein, Stn1, could influencethe phenotypes of either pol1 or cdc13-5 mutants. Notably, increasedexpression of STN1 suppressed the telomere phenotypes of mutationsin both genes, implicating the cdc13-5 defect in a step in telomerereplication that depends on DNA polymerase $alpha$ function. STN1 expression,driven by the GAL promoter and on a high-copy plasmid, reducedtelomere length in a cdc13-5 strain to nearly wild-type length(Fig. 3A) whereas overexpression of STN1 had little or no effecton telomere length in a wild-type strain. In addition, single-strandedG-rich DNA was not detectable in asynchronous cultures of a cdc13-5strain overexpressing STN1 (Fig. 3B), as would be predicted ifthe alterations in telomere length and the terminal G strand overhangare the result of the same defect. Increased expression of STN1similarly influenced the telomere replication defect of DNA polymerase $alpha$ mutants. The telomere elongation phenotype observed when pol1-12,pol1-16, and pol1-17 mutant strains were grown at semipermissivetemperatures was substantially suppressed when STN1 was overexpressed(Fig. 3C; data not shown). Suppression was specific to the telomerereplication phenotype of the pol1 mutant strains, as overexpressionof STN1 did not suppress the temperature sensitivity of thesepol1 mutant alleles (data not shown).

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Figure 3. Overexpression of STN1 suppresses the telomere elongation phenotypes of cdc13-5 and pol1 mutant strains. (A) Telomere length of a cdc13- $Delta$ strain covered by a CDC13⁺ plasmid (pVL440; lanes 1-4) or a cdc13-5 plasmid (pVL1033; lanes 5-8) plus a plasmid overexpressing STN1 (pVL1035) or a control vector (pVL1036). (B) DNA prepared from a cdc13- $Delta$ strain covered by a CDC13⁺ plasmid (pVL440; lanes 3,4) or a cdc13-5 plasmid (pVL1033; lanes 5,6) plus a plasmid overexpressing STN1 (pVL1035; lanes 4,6) or a control vector (pVL1036; lanes 3,5) was analyzed by nondenaturing in-gel hybridization with a C_1-3A oligonucleotide probe (left); denatured and rehybridized with a Y' probe (middle); and denatured and rehybridized with a C_1-3A oligonucleotide probe (right); lanes 1,2: pVL260 heat denatured or nondenatured, respectively; lane 7: pJH354, containing a region of Y' sequence. (C) Telomere length of the indicated pol1 mutant strains or the isogenic POL1⁺ strain (indicated as wt) transformed with either a plasmid overexpressing STN1 (pVL1034) or vector (YEplac112). (D) CDC13 (UCC3505, Singer and Gottschling 1994

), cdc13-5 (TVL422) and sir3- $Delta$ (TV318), each containing a telomere-proximal URA3 gene, were grown in rich media, and 10-fold serial dilutions were plated on rich media, on media lacking uracil, and on media containing 5-FOA and incubated for 48 h at 30°C.

Duplex telomeric chromatin is not altered in the cdc13-5 strain

One mechanism for telomere length control proposes that telomeric chromatin equilibrates between an open conformation thatpermits telomerase access and a higher-order closed conformationthat inhibits access of the telomerase enzyme through sequestrationof the chromosome terminus (for review, see Evans and Lundblad2000). This length-determining conformational switch is determinedby binding of negative regulatory proteins to duplex telomericDNA. Therefore, the increased telomere length of pol1 strainscould be due to reduced assembly of inhibitory proteins on duplextelomeric DNA, possibly as a consequence of altered rates of laggingstrand synthesis (Diede and Gottschling 1999; Adams Martin etal. 2000). Alterations in telomeric chromatin are often assessedby monitoring the metastable repression of transcription of reportergenes placed adjacent to the telomeric G_1-3T telomeric tract,referred to as telomeric silencing (Gottschling et al. 1990).In a pol1-17 mutant strain, telomeric silencing is greatly reduced,even under growth conditions where telomeres have not yet undergoneextensive elongation (Adams Martin et al. 2000). In contrast,telomeric silencing is unaltered in the cdc13-5 strain (Fig. 3D),indicating that the structure of duplex telomeric chromatin isunaffected in this mutant. This suggests that the telomere elongationobserved in the cdc13-5 mutant strain is a consequence of eventsthat are restricted to the veryterminus.

Stn1 interaction with Cdc13 is abolished by the cdc13-2 mutation

Increased expression of STN1 suppressed the telomere length phenotypes of the cdc13-5 strain (Fig. 3) but did not suppressthe cdc13-2 defect; in fact, the senescence phenotype of a cdc13-2strain was enhanced when the negative regulator STN1 was overexpressed(data not shown). In contrast, the cdc13-2 phenotype is partiallysuppressed when the positive regulator EST1 is overexpressed (Nugentet al. 1996), which is also consistent with recent work indicatingthat Est1 binds to a site on Cdc13 that is abolished by the cdc13-2mutation (Pennock et al., 2001). Since two-hybrid analysis hadpreviously shown that Stn1 and Cdc13 also interact (Grandin etal. 1997), we tested whether Stn1 performs its negative regulatoryrole by binding to a similar domain on Cdc13 as is bound by Est1.Figure 4 shows that Stn1 and Cdc13 exhibit a strong two-hybridinteraction, as previously observed. Strikingly, the cdc13-2 mutationabrogates this Stn1-Cdc13 interaction. This effect is specificto this mutation, as association between Stn1 and Cdc13 is stillobserved when either the cdc13-1 or cdc13-3 mutations are introduced(Fig. 4; data not shown).

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Figure 4. Cdc13, but not Cdc13-2, interacts with Stn1, by a two-hybrid test. Activation of a lacZ two-hybrid reporter gene was evaluated using X-gal overlay assays to detect $beta$ -galactosidase activity. Results are shown for three independent transformants each of CDC13 and STN1 (pVL705 and pVL859), cdc13-1 and STN1 (pVL667 and pVL859), cdc13-2 and STN1 (pVL854 and pVL859), and CDC13 and vector (pVL705 and pACT2). The ADE2 and HIS3 reporter genes present in this strain (pJ69-4A; James et al. 1996

) gave results similar to the lacZ reporter (data not shown).

The increased single-stranded telomeric DNA present in a cdc13-5 strain does not invoke a DNA damage response

Cdc13 has an essential function in protecting the chromosome termini from degradation, as loss of CDC13 function (using thethermolabile cdc13-1 allele characterized previously) resultsin substantial resection of the C strand of the telomere and aresulting RAD9-mediated G₂/M arrest (Weinert and Hartwell 1993;Garvik et al. 1995; Diede and Gottschling 1999). This indicatesthat Cdc13 has an essential function in protecting the chromosometermini from degradation (Garvik et al. 1995; Nugent et al. 1996).The cdc13-5 strain, in contrast, does not appear to be defectivefor this essential function of CDC13 because it does not exhibiteither growth defects or a DNA damage response. The growth ofa cdc13-5 strain was comparable to that of a wild-type strainat both 30°C and 36°C, temperatures that are not permissive forgrowth of the thermolabile cdc13-1 strain (Fig. 5A). Both FACSdata (Fig. 2B) and bud index analysis (data not shown) showedthat the cdc13-5 strain exhibited the same cell cycle distributionas a wild-type strain at 30°C. In addition, the kinetics of microcolonyformation for a cdc13-5 strain was comparable to that of wildtype, whereas a cdc13-1 strain arrested as large budded cellsat 30°C (Fig. 5B). Thus, the cdc13-5 mutant does not show a noticeablegrowth defect or an alteration in cell cycle progression, showingthat the activity of CDC13 that is responsible for negative regulationof telomere length is distinct from the essential end protectionfunction of CDC13. Furthermore, expression of the RNR genes, whichare normally induced in response to DNA damage or replicationblocks (Elledge et al. 1993), was comparable in the cdc13-5 andCDC13 strains, in contrast to the robust induction of RNR expressionthat was observed either in a cdc13-1 strain at a nonpermissivetemperature (30°C) or in a CDC13 strain treated with HU (Fig.5C). In addition, genome-wide expression analysis of a cdc13-3strain did not reveal any characteristic expression patterns suggestinga response to DNA damage, clearly distinguishing it from cdc13-1(T.R. Hughes et al., in prep.). Therefore, the substantial increasein the amount of single-stranded DNA at the telomere that is observedin cdc13-3 and cdc13-5 strains is not sufficient to invoke a DNAdamage response.

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Figure 5. The cdc13-5 mutation is not compromised for the essential role of CDC13. (A) 10-fold serial dilutions of CDC13⁺, cdc13-5, and cdc13-1 strains were plated on rich media and incubated at 26°C, 30°C, and 36°C. (B) Progression of individual cells to microcolonies, for CDC13, cdc13-1, and cdc13-5 strains, measured as described by Weinert and Hartwell 1993

. Strains were grown to early log growth phase at 23°C and plated for individual cells on prewarmed plates at 30°C (a nonpermissive temperature for the cdc13-1 strain); for each genotype, $>=$ 100 cells were monitored at 0, 4, and 8 h for the proportion of large budded cells. (C) Northern analysis monitoring the expression level of RNR genes. CDC13⁺ and cdc13-5 strains were grown to an OD₆₀₀ of 0.4 at 30°C, and an aliquot of CDC13⁺ cells was incubated in the presence of 200 mM hydroxyurea for 3 h; the cdc13-1 strain was grown at 23°C and an aliquot shifted to 30°C for 3 h. Relative RNR transcript levels are shown, normalized to the fold difference between the level of the RNR transcript relative to the U1 transcript levels in the wild-type strain.

This suggests that the DNA damage response of the cdc13-1 mutant strain may be the combined consequence of the simultaneousincrease in single-stranded DNA and the loss of the unstable Cdc13-1protein from chromosome ends. The lack of a DNA damage responseevoked by the cdc13-5 mutant could be explained if the extendedsingle-stranded G tails are transient and/or are still bound (andhence protected) by the Cdc13 protein. The latter suggestion isalso compatible with the previous demonstration that a single-strandedtelomeric oligomer is capable of binding multiple Cdc13 molecules(Hughes et al. 2000a). Consistent with such a model, the bindingaffinity of the truncated 80-kD version of the Cdc13-3 proteinto a 24-base oligonucleotide was almost identical to that of wild-typeCdc13 protein (Fig. 6; data not shown). We therefore propose thatthe extended single-stranded DNA present at telomeres in cdc13-3and cdc13-5 strains is still bound by Cdc13 (and presumably otherfactors) and is incapable of sending a DNA damage signal.

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Figure 6. The 80-kD truncated Cdc13 protein retains DNA binding activity. DNA binding ability of wild-type Cdc13 (lanes 2,3) and the 80-kD truncated derivative of Cdc13-3 (lanes 4,5), as assessed by DNA gel shift assays with 5' end-labeled d(TGT GTGGG)₃ oligomer at 1 nM and protein concentration at 10 or 1 nM, as indicated; lane 1, no protein added.

	Discussion

Top Abstract Introduction Results Discussion Materials and methods References

Several previous studies, in both ciliates and budding yeast, indicate that coordinated synthesis of the two strands of thetelomere is required for telomere length maintenance. Disruptionof the activity of the lagging strand DNA replication machinery,by either mutation or pharmacological intervention, leads to unregulatedelongation of the G-rich strand, accompanied by an impaired inabilityto regulate synthesis of the C-rich strand. However, the specificmechanism that coordinates G-strand synthesis by telomerase withC-strand synthesis by the lagging strand synthesis machinery hasnot beenelucidated.

The work presented here shows that Cdc13 negatively regulates elongation of the G strand and that this activity is a key componentin the coordination between G-strand and C-strand synthesis. Amodel to explain this negative regulatory role must also takeinto account the fact that Cdc13 positively regulates telomerereplication as well. One simple proposal, presented in Figure7, is derived from a model presented by Fan and Price (1997),based on their studies of de novo telomere replication in theciliate Euplotes crassus. These authors proposed that followingelongation of the G strand by telomerase, fill-in synthesis ofthe C strand could limit further addition of telomeric repeats,possibly by displacement or inhibition of telomerase by the pol $alpha$ /primase complex. In Figure 7, we expand their model by proposingthat the two regulatory activities of Cdc13, defined by the cdc13-2and cdc13-5 defects, correspond to two distinct steps in telomerereplication that coordinate and regulate synthesis of the twostrands of the telomere. Binding of Cdc13 to the transiently exposedsingle-strand G tails present in S phase initiates telomere replicationby recruiting telomerase, which can then extend the 3' terminusof the G-rich strand. Subsequent fill-in synthesis of the C strandgenerates a terminus that no longer exhibits an extended single-strandedend structure. We propose that synthesis of the C strand by laggingstrand synthesis machinery acts to limit extension of the G strandby telomerase, and it is this inhibitory second regulatory stepthat is defective in the cdc13-5 mutant. Thus, the first step(telomerase recruitment) occurs normally in the cdc13-5 strain,but the subsequent response to the initiation of C-strand DNAreplication is impaired or delayed, allowing telomerase to continueunchecked in its synthesis of the G strand.

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Figure 7. Cdc13 plays a dual role in regulation of G-strand synthesis by telomerase. The extended G strand, which is generated by a telomerase-independent mechanism (Wellinger et al. 1996

), provides a substrate for binding by Cdc13. Once bound to the telomere, Cdc13 initiates synthesis of the G strand by recruiting telomerase through an interaction with the Est1 telomerase subunit. Binding of Est1 to Cdc13, and hence enzyme recruitment, is blocked by the cdc13-2 mutation. Elongation of the G strand by telomerase is subsequently followed by fill-in synthesis of the C strand by lagging strand synthesis machinery, which inhibits further synthesis of the G strand by telomerase. This inhibitory step is defective in the cdc13-5 mutant, allowing telomerase to further extend the G strand. We propose that binding of Stn1 to Cdc13, thereby displacing telomerase, is the mechanism by which unchecked telomerase synthesis is inhibited.

This model is supported by several observations. First, the telomere elongation defect of the cdc13-5 mutant is dependenton an intact telomerase complex, as well as the recruitment activityof Cdc13. In addition, the enhanced single-strand extension ofthe G strand observed in the cdc13-5 mutant is also restrictedto the same period of the cell cycle when telomeres are normallyelongated (Marcand et al. 2000). Two experiments indicate thatregulation of C-strand synthesis is also an important componentof the phenotype of the cdc13-5 mutant. The telomere length defectsof both cdc13-5 and pol1 mutant strains are suppressed by overexpressionof the Stn1 protein, indicating that Stn1 helps coordinate theaction of the lagging strand replication complex with the regulatoryactivity of CDC13. Furthermore, the cdc13-5 strain displays anextreme enhancement of the telomere defect in response to altereddosage of one subunit of the lagging strand DNA replication machinery,arguing that the cdc13-5 defect is correlated with the abilityto synthesize the C strand (data not shown). Finally, the lackof a silencing defect in the cdc13-5 strain argues that the telomereelongation phenotype is not a secondary consequence of a moregeneral disruption of duplex telomeric chromatinstructure.

Several lines of evidence indicate that both Stn1 and Est1 bind to the Cdc13 protein. Therefore, we suggest that the two stepsin regulation of G-strand synthesis may be the consequence ofthe binding of two successive complexes to Cdc13. Work presentedelsewhere demonstrates that the telomerase-associated Est1 proteinpromotes the positive regulatory step in telomere replicationby binding to the recruitment domain of Cdc13, an interactionthat is eliminated by the cdc13-2 mutation (Nugent et al. 1996;Qi and Zakian 2000; Pennock et al., 2001). In this work, we showthat interaction of the negative regulator Stn1 with Cdc13 isalso abolished by the same mutation. Thus, binding of Stn1 toCdc13, occurring in response to C-strand synthesis, could limitthe extent of G-strand synthesis by displacing telomerase fromCdc13. This proposed mechanism predicts that Est1 and Stn1 shouldcompete for binding to overlapping binding sites on Cdc13 (definedby the cdc13-2 missense mutation), a possibility that is currentlyunderinvestigation.

The cdc13-5 mutation, which is caused by the loss of the 230 terminal amino acids of Cdc13, still retains the site definedby the cdc13-2 mutation. Based on the above model, loss of theC-terminal region presumably impairs the ability of the Cdc13-5protein to interact with Stn1. This is consistent with rescueof the cdc13-5 defect by overexpression of STN1, indicating thatincreased Stn1 protein levels can restore an interaction betweenStn1 and the truncated Cdc13-5 protein. Therefore, the presenceof the C-terminal 230 amino acids of Cdc13, although not essentialfor interaction with Stn1, may help stabilize or facilitate theStn1-Cdc13 association. It is possible that the C terminus ofCdc13 interacts with yet another protein that could modulate theproposed competition for binding between Est1 andStn1.

We have previously described another means by which the limit on telomere length homeostasis can be overcome, by fusing asubunit of telomerase to Cdc13 or to the DNA binding domain ofCdc13, DBD_Cdc13 (Evans and Lundblad 1999; Hughes et al. 2000b).These telomerase fusions result in greatly elongated telomeres,presumably because the first step in telomere length regulation $---$ therecruitment step $---$ has been greatly enhanced. This contrasts withthe proposal, above, that telomere elongation caused by the cdc13-5mutation is due to a defect subsequent to the recruitment step.Comparison of the properties of these two perturbations of telomerelength control supports the idea that two different regulatorysteps in telomere replication are altered. First, telomere elongationby DBD_Cdc13-telomerase or Cdc13-telomerase fusions is the resultof a gain-of-function property, whereas the cdc13-5 defect isa recessive mutation. Second, elongation by the Cdc13-telomerasefusions is not dependent on the activity defined by the cdc13-2mutation (Evans and Lundblad 1999; Hughes et al. 2000b), whereastelomerase elongation by the cdc13-5 mutation cannot occur inthe presence of the recruitment-defective cdc13-2 allele. Finally,the Cdc13-5 mutant protein does not exhibit a detectable associationwith telomerase (S.K. Evans, A. Chandra, and V. Lundblad, unpubl.),whereas the Cdc13-Est1 and Cdc13-Est2 fusions both retain tightassociation with an active enzyme complex (Evans and Lundblad1999).

One potentially surprising consequence of this study is the observation that the extensive single-stranded regions presentduring S phase in a cdc13-5 strain can be tolerated without obviouseffects on cell cycle progression or genomic stability. A cdc13-5strain does not exhibit a DNA damage response (Fig. 5), nor ischromosome loss elevated in this strain (data not shown). Thiscontrasts with previous studies of the cdc13-1 mutant strain,which exhibits increased mitotic recombination and chromosomeloss at semipermissive temperatures (Carson and Hartwell 1985;Hartwell and Smith 1985) and a severe DNA damage response andextensive loss of C-strand DNA under nonpermissive conditions(Weinert and Hartwell 1993; Garvik et al. 1995). Diede and Gottschling(1999) have proposed that tight coupling between telomerase synthesisand the activity of DNA polymerases $alpha$ and $delta$ is necessary to preventinappropriately elongated G-tails, which could elicit the samedetrimental consequences similar to those observed in a cdc13-1mutant. One explanation for the behavior of the cdc13-5 strainthat would still be consistent with their proposal is that thecdc13-5 mutation may not be a complete coupling defect, as theelongated G tails are only observed in S phase in this strain.Because telomeres appear to be primarily duplex at other stagesof the cell cycle in the cdc13-5 strain, most of the C strandmust be eventually synthesized during each cell cycle in thismutant. This indicates that there is a delay, rather than a completeblock, in coupling between synthesis of the two strands. However,if the proposed coupling function is essential for cell cycleprogression, it is notable that the cdc13-5 strain displays noapparent cell cycle delay. This suggests that tight coupling maynot be essential and that the cell may be able to maintain genomicintegrity even in the presence of elongated single-stranded tractsat the telomere (at least during one period of the cell cycle),as long as these single-stranded regions are bound and protectedbyCdc13.

In this article, we have described a role for Cdc13 in the negative regulation of telomere length by coordinating G-strandand C-strand synthesis. This mechanism appears to be distinctfrom that promoted by duplex telomere DNA binding proteins, whichmediate a conformational switch that affects the accessibilityof the chromosome end to telomerase (for review, see Evans andLundblad 2000). Notably, like CDC13, the mammalian telomere bindingprotein TRF2 is required for both negative regulation of telomerelength (Smogorzewska et al. 2000) and an essential role in chromosomeend protection (van Steensel et al. 1998). Both end protectionand length regulation of human telomeres may rely on the regulatedformation of a unique DNA structure, dubbed the t-loop, in whichthe G-rich 3' overhang invades the duplex telomeric tract (Griffithet al. 1999). Whether such a structure forms at yeast telomeres,and is regulated by the Cdc13 protein, is an interesting experimentalquestion.

	Materials and methods

Top Abstract Introduction Results Discussion Materials and methods References

Strains and plasmids

All strains used in this study are isogenic, derived from previously published strains by introduction of the relevant deletionmutations or cdc13 mutations by standard molecular techniques,with the exception of the strains used in Figure 3C and 3D. DVL233(MATa/ $alpha$ ura3-52/ura3-52 ade2-101/ade2-101 trp1 $Delta$ -1/trp1 $Delta$ -1his3- $Delta$ 200/his3- $Delta$ 200 leu2- $Delta$ 1/leu2- $Delta$ 1 TLC1/tlc1 $Delta$ ::LEU2 RAD52/rad52- $Delta$ ::LEU2CDC13/cdc13-3 CF-SUP11-TRP1) and DVL326 (MATa/ $alpha$ ura3-52/ura3-52ade2-101/ade2-101 trp1 $Delta$ -1/trp1 $Delta$ -1 his3- $Delta$ 200/his3- $Delta$ 200 leu2- $Delta$ 1/leu2- $Delta$ 1TLC1/tlc1- $Delta$ ::LEU2 CDC13/cdc13-5 CF-SUP11-TRP1) were derived fromDVL131 as described (Lendvay et al. 1996), DVL328 (MATa/ $alpha$ ura3-52/ura3-52 ade2-101/ade2-101, trp1 $Delta$ -1/trp1 $Delta$ -1 his3- $Delta$ 200/his3- $Delta$ 200leu2- $Delta$ 1/leu2- $Delta$ 1 EST1/est1- $Delta$ 3::HIS3 RAD52/rad52- $Delta$ ::LEU2 CDC13/cdc13-5CF-SUP11-TRP1) was derived from TVL140 as described previously(Lundblad and Blackburn 1993), and DVL162 (MATa/ $alpha$ ura3-52/ura3-52ade2-101/ade2-101, trp1 $Delta$ -1/trp1 $Delta$ -1 his3- $Delta$ 200/his3- $Delta$ 200 leu2- $Delta$ 1/leu2- $Delta$ 1CDC13/cdc13- $Delta$ ::LYS2 CF-SUP11-TRP1/pVL 438) from YPH275 (Lundbladand Szostak 1989). Haploid cdc13-1, cdc13-3, cdc13-5, or cdc13-2,5strains were derived by either dissecting the relevant diploidor by introducing the relevant plasmids into a cdc13- $Delta$ /pVL438haploid strain (derived from dissection of DVL162), followed byeviction of pVL438 on selective media containing 5-FOA.

All CDC13 plasmids used in this study were derived from pVL438 (CEN URA3 CDC13; YCplac33-based) or pVL440 (CEN LEU2 CDC13;YCplac111-based); both contained the same 4.5-kb genomic insertwith the wild-type CDC13 gene. pVL690 (CEN LEU2 cdc13-2), pVL762(CEN LEU2 cdc13-1), and pVL1360 (CEN LEU2 cdc13-2,5) were derivedfrom pVL440 by introducing the relevant CDC13 mutant alleles.The cdc13-3 mutation (K695A, R697A, D698A, E699A) was constructedby site-directed mutagenesis in the E. coli expression plasmidpVL427 (Hughes et al. 2000a) and subsequently subcloned to generatepVL821 (CEN LEU2 cdc13-3). The cdc13-5 mutation was constructedby PCR to introduce a stop codon following amino acid 694 to generatepVL1033 (CEN LEU2 cdc13-5). The cdc13-3 and cdc13-5 mutationswere integrated into the genome of appropriate strains using pVL780(YIp URA3 cdc13-3) or pVL1215 (YIp URA3 cdc13-5), using a pop-in/pop-outstrategy. pVL841 and pVL903, which encode HA3-Cdc13p and HA3-Cdc13-5p,respectively, are derived from pVL440; the HA3 epitope tag introducedinto the N terminus of Cdc13 was described previously (pVL842;Hughes et al. 2000b).

Plasmids used for high copy expression of STN1 were derived from YEplac112. pVL1034 (2 µ TRP1 STN1, with expression of STN1driven by its native promoter) contains a 2.9-kb genomic insertthat includes the STN1 gene. pVL1035 (2 µ TRP1 GAL-STN1) was derivedfrom pVL1036 (YEplac112 containing the ~0.8-kb GAL1 promoter)by insertion of a PCR-amplified copy of STN1 behind the GAL1 promoter.The plasmids used for two-hybrid analysis were derived from pAS1and pACT1. pVL705 was constructed by insertion of a full-lengthfragment of CDC13 bearing an in-frame deletion of amino acids585-677 (within the DNA binding domain of Cdc13; Hughes et al.2000a) into the NdeI site of pAS1 to generate a fusion to theGal4 DNA-binding domain; deletion of a portion of the DNA-bindingdomain was necessary to prevent overexpression lethality (C. Nugent,unpubl.). pVL854 is identical to pVL705 except for the presenceof the cdc13-2 missense mutation. pVL667 contains the full-lengthcdc13-1 gene inserted into pAS1. pVL859 was recovered from a libraryscreen as a Cdc13-interacting clone and contains amino acids 5-495of the Stn1 protein fused in frame with the Gal4 activation domainof pACT1. pVL260 contains 80 bp of G_1-3T DNA cloned intothe polylinker of pDS67 (a pBluescript plasmid that also containsARG4).

Molecular methods

Standard denaturing Southern gel conditions were used for determining telomere length (Lendvay et al. 1996). Single-strandchromosome termini were analyzed by nondenaturing in-gel hybridizationwith a 22-mer CA-rich oligonucleotide as described previously(Dionne and Wellinger 1996). To assay chromosome end structureduring the cell cycle, the cdc13-5 strain was grown in YPD toOD₆₀₀ 0.2, followed by the addition of 3 µM $alpha$ factor. Additional $alpha$ factor (at a concentration of 3 µM) was added every hour until~90% of the cells appeared unbudded (for ~3-4 h). The $alpha$ factorwas removed by centrifugation and cells released into YPD at OD₆₀₀0.4. Cells for FACS analysis were fixed in 70% ethanol, washedin 50 mM Na citrate (pH 7.0), digested with RNase overnight, washedagain and stained with propidium iodide (15 µg/mL), and analyzedby flowcytometry.

For Northern blot analysis, total RNA was isolated by a phenol-freeze method (Schmitt et al. 1990), resolved on formaldehyde-1%agarose, and probed with the 1.7-kb BglII-EcoRI RNR1 fragmentfrom pSE738, the 1.1-kb HindIII RNR2 fragment from pSE310, the1-kb BamHI-EcoRI RNR3 fragment from pSE734, the 1.4-kb StuI-SwaIRNR4 fragment from pMH120, or a 600-bp fragment of the U1 gene(recovered by PCR of yeast genomicDNA).

Biochemical methods

For detection of the HA-tagged Cdc13 and Cdc13-5 proteins, cdc13- $Delta$ /pVL440 (Cdc13), cdc13- $Delta$ /pVL841 (HA3-Cdc13), and cdc13- $Delta$ /pVL903(HA3-Cdc13-5) were grown in selective media to an OD₆₀₀ 0.6. Extractpreparation and Western analyses were done as described in Hugheset al. (2000b), except that TMG 300+ (10 mM Tris-HCl at pH 8.0,1 mM MgCl₂, 5% glycerol, 1 mM PMSF, 1 mM DTT, 300 mM NaCl) wasused for immunoprecipitations andwashes.

His₆-tagged proteins (Cdc13 or Cdc13-3) were expressed in SF9 cells as described previously (Hughes et al. 2000a). For proteinproduction, cells were pelleted, washed, and resuspended in SB300 10% + (50 mM Na phosphate at pH 8.0, 300 mM NaCl, 10% glycerol,0.5% Tween-20, 10 mM imidazole, 1 mM PMSF), and sonicated for3-4 repetitions of 10-30 sec; the degree of sonication requiredwas monitored by visual inspection.Extracts were clarified bycentrifugation for 10 min, and His₆-tagged proteins were purifiedon Ni-NTA agarose at 4° (QIAGEN) by batch method, according tothe manufacturer's instructions. Protein concentration was determinedby comparison to BSA standards on Coomassie-stained SDS-PAGE gels.Binding reactions were performed as described in Nugent et al.(1996).

	Acknowledgments

We thank the members of the Lundblad laboratory for many helpful discussions and also thank the Flow Cytometry Core Lab, TexasChildren's Hospital. We gratefully acknowledge the generous giftsof strains or plasmids from Connie Holm, Oscar Aparicio, StephenBell, Judith Campbell, Steve Elledge, Tim Formosa, and Peter Burgers.This work was supported by NIH grant GM55867 (to V.L.) and a postdoctoralfellowship from the U.S. Army and Materiel Command (to C.N.).

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

	Footnotes

Received October 20, 2000; revised version accepted December 27, 2000.

Present addresses: ³Rosetta Inpharmatics, Kirkland, WA 98034,USA. ⁴Department of Cell Biology and Neuroscience, University of California, Riverside, CA 92521,USA.

⁵ Correspondingauthor.

E-MAIL lundblad{at}bcm.tmc.edu; FAX (713) 798-5931.

Article and publication are at www.genesdev.org/cgi/doi/10.1101/gad.861001.

References

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Abstract
Introduction
Results
Discussion
Materials and methods
References

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RESEARCH PAPER Cdc13 both positively and negatively regulates telomere replication

RESEARCH PAPER
Cdc13 both positively and negatively regulates telomere replication