Telomere Folding Is Required for the Stable Maintenance of Telomere Position Effects in Yeast

doi:10.1128/MCB.20.21.7991-8000.2000

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Molecular and Cellular Biology, November 2000, p. 7991-8000, Vol. 20, No. 21
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Telomere Folding Is Required for the Stable Maintenance of Telomere Position Effects in Yeast

Derik de Bruin,¹ Sara M. Kantrow,¹^, Rachel A. Liberatore,¹ and Virginia A. Zakian²^,^*

Department of Molecular Biology, Princeton University, Princeton, New Jersey 08544,² and Laboratory of Molecular Genetics and Immunology, The Rockefeller University, New York, New York 10021¹

Received 1 June 2000/Returned for modification 18 July 2000/Accepted 8 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Yeast telomeres reversibly repress the transcription of adjacent genes, a phenomenon called telomere position effect (TPE).TPE is thought to result from Rap1 and Sir protein-mediated spreadingof heterochromatin-like structures from the telomeric DNA inwards.Because Rap1p is associated with subtelomeric chromatin as wellas with telomeric DNA, yeast telomeres are proposed to form fold-backor looped structures. TPE can be eliminated in trans by deletingSIR genes or in cis by transcribing through the C_1-3A/TG_1-3tract of a telomere. We show that the promoter of a telomere-linkedURA3 gene was inaccessible to restriction enzymes and that accessibilityincreased both in a sir3 strain and upon telomere transcription.We also show that subtelomeric chromatin was hypoacetylated athistone H3 and at each of the four acetylatable lysines in histoneH4 and that histone acetylation increased both in a sir3 strainand when the telomere was transcribed. When transcription throughthe telomeric tract occurred in G₁-arrested cells, TPE was lost,demonstrating that activation of a silenced telomeric gene canoccur in the absence of DNA replication. The loss of TPE thataccompanied telomere transcription resulted in the rapid and efficientloss of subtelomeric Rap1p. We propose that telomere transcriptiondisrupts core heterochromatin by eliminating Rap1p-mediated telomerelooping. This interpretation suggests that telomere looping iscritical for maintainingTPE.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The physical termini of linear eukaryotic chromosomes consist of DNA-protein structures called telomeres (57). In additionto their functions in promoting chromosome stability, yeast telomeresaffect the behavior of nearby DNA. Saccharomyces telomeres repressthe basal transcription of adjacent genes, a phenomenon calledtelomere position effect (TPE) (19), and they also affect boththe timing of DNA replication (13) and the rate of mitotic recombination(48). Yeast telomeres are often clustered near the nuclear periphery,and it has been suggested that this positioning is important fortranscriptional silencing (17).

Yeast telomeric DNA is assembled into a nonnucleosomal chromatin structure, the telosome, which encompasses the entire terminaltract of telomeric DNA (56). The major protein in the telosomeis the sequence-specific DNA binding protein Rap1p (11), butSir2p, Sir3p, and Sir4p, proteins required for TPE (2), alsobind telomeres in vivo (5). The Sir proteins are most likelyrecruited to the telomere by their ability to interact with Rap1p(10, 36), and their appearance there is thought to be theinitiating event in the establishment of TPE (31). Subtelomericchromatin propagates continuously from the telomere inward (41),presumably through interactions between the Sir proteins and subtelomericnucleosomes (24).

Although telomere-adjacent DNA is packaged into nucleosomes (56), these subtelomeric nucleosomes differ in several respectsfrom nucleosomes elsewhere in the genome. First, the DNA in subtelomericnucleosomes is less accessible to DNA-modifying enzymes such asEscherichia coli dam methyltransferase (20). Second, Sir proteinsassociate as a complex with subtelomeric nucleosomes (25, 49)by virtue of their ability to bind the N-terminal tails of histonesH3 and H4 (24). Third, the N-terminal tails of histones H3 andH4 in subtelomeric nucleosomes are hypoacetylated compared tothose of histones in most other regions of the genome (6, 35).These structural features are also characteristics of the yeastsilent mating type or HM loci (22). At both telomeres and theHM loci, these structural features are lost in strains with siror histone mutations that eliminate silencing, suggesting thattranscriptional repression is a consequence of their uncommonchromatin structure (6, 30, 46, 52).

There is also evidence for a higher-order organization of yeast telomeric chromatin. Chromatin immunoprecipitation experimentsreveal that Rap1p is associated in vivo not only with telomericDNA (11) but also with subtelomeric chromatin (49). SinceRap1p, unlike the Sir proteins, does not interact directly withhistones, this result led to the proposal that the yeast telomerefolds back onto the subtelomeric regions to form a ~3-kb regionof core heterochromatin (22, 49). Similarly, mammalian telomeresare known to end in large 10- to 20-kb duplex "t loops" (21).Telomere loops might play an important role in regulating TPE(39).

The transcriptional state of a telomere-linked gene is reversible, and once established both the transcribed and the repressedstates are stable for many cell generations (19, 35). Thereversibility of TPE suggests a competition between the establishmentof an active transcription complex and the assembly of the repressivechromatin structure, and this competition appears dependent oncell cycle progression. Although DNA replication is not neededfor certain yeast genes to switch from a repressed to a transcriptionallyactive state (43), reactivation of regionally silenced chromatin,which involves the reconfiguration of an entire chromosomal domain,is thought to require DNA replication. For example, the accessibilityof a repressed telomere-linked URA3 gene to its trans-activatorPpr1p occurs only during a limited interval late in the cell cycle(3) that corresponds roughly to the time when telomeric DNAis replicated (55).

In earlier studies on telomeric heterochromatin, loss of silencing was achieved using mutations in SIR or histone genes. However,these mutations affect all telomeres (24, 52) and also influencebasal transcription (29), recombination (18), and chromosomestability (38). In this paper, we use a system in which TPEcan be eliminated in cis at a single telomere by inducing transcriptionthrough the telomeric tract of C_1-3A/TG_1-3 DNA. Thistelomeric transcription has no effect on the stability of theaffected chromosome (42). We show that switching this conditionaltelomere from a repressed to a transcribed state was accompaniedby all of the chromatin changes previously associated with transcriptionalactivation, such as increased accessibility to the dam methyltransferaseand a conversion from hypo- to hyperacetylated histones. The chromatinchanges that accompany the switch from a repressed to a transcribedstate in a telomere-linked gene, as well as transcription itself,occurred in G₁-arrested cells. Although by nearly all criteriathe chromatin structure of the transcribed telomere was indistinguishablefrom that of a telomere in a sir3 strain, telomere transcriptiondid not result in the complete loss of subtelomeric Sir3p. However,telomere transcription rapidly and efficiently disrupted subtelomericRap1p interactions, suggesting that it caused loss of the coreheterochromatin fold-back telomericstructure.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

All experiments were done with Saccharomyces cerevisiae yeast strains derived from either YPH499 (MATa ura3-52 lys2-801ade2-101 trp1- $Delta$ 63 his3- $Delta$ 200 leu2- $Delta$ ) or YPH500 (a MAT $alpha$ versionof YPH499) (45). Strains containing the UT, PT, and XT telomeremodifications were made by transforming with EcoRI- and SalI-cleavedpADH4UCA, ADH4UGT, and pADH4UGT-TATA, respectively (19, 42).E. coli dam methyltransferase was inserted at LYS2 by transformingYPH499 with XhoI-digested pDP6-dam to create YPH499LD (20).UTLD, PTLD, and XTLD were derived from YPH499LD by transformationas described above. With the exception of the dam methyltransferase-expressingstrains, yeast strains carried ura3::LEU2 and had an 845-bp deletionin the ura3 transcription unit generated by transforming withHindIII-digested pULA (19). UTsir3 (sir3::LYS2) was made bytransforming UT with EcoRI-digested pJR317 (28). The UINT strainwas constructed by inserting URA3 at lys2 using AatII-cleavedpCF116 (15). The ura3 $Delta$ EB minigene was made by first deletingthe 78-bp EcoRV-BstBI fragment from pVZURA3-1 (1.1-kb URA3 HindIIIfragment in pVZ1 (J. Stavenhagen, unpublished) and then recircularizingthe plasmid to generate pVZura3 $Delta$ EB. The ~1-kb XbaI ura3 $Delta$ EB minigenefragment was recovered from pVZura3 $Delta$ EB, the ends were blunted,and then the fragment was ligated into SmaI-digested pDP6 (14).The resulting plasmid, pDPura3 $Delta$ EB, was digested with XhoI andtransformed into ura3 $Delta$ yeast to generate DdB5 $Delta$ EB, thus integratingura3 $Delta$ EB at the LYS2 locus. UT $Delta$ EB, PT $Delta$ EB, and XT $Delta$ EB were made bytransforming DdB5 $Delta$ EB as described above. UTsir3 $Delta$ EB was derivedfrom UT $Delta$ EB by transformation with EcoRI-digested pKL3sir3::HIS3(J. Stavenhagen, unpublished). For the G₁ arrest experiments,strain aDdB6PTb was used. This strain carried bar1::HIS3and was constructed by transforming a MATa version of PTwith PvuII-digested pUCB14HIS3 (from D.Pederson).

Yeast complete synthetic medium (YC), 5-fluoro-orotic acid (FOA) medium, and rich medium (yeast extract-peptone [YEP]) wereprepared and supplemented with either 2% glucose, 3% raffinose,or 3% galactose (Ultrapure; Sigma) as described previously (4,19). For TPE analyses, 10-fold serial dilutions from each offour to six colonies from a YEP-peptone-dextrose plate were plated(~300 cells per plate) on YC, YC-uracil, and YC plus FOA medium(47). Colonies were counted after 4 days of growth at 30°C.Methods for dam methylation protection assays (35) were describedpreviously. Nuclei were prepared for in vivo restriction enzymemapping from spheroplasts by Ficoll lysis as described previously(56), except that phenylmethylsulfonyl fluoride (PMSF) and iodoaceticacid were replaced with Complete, EDTA-free protease inhibitors(Boehringer Mannheim) plus 0.7 µg of pepstatin/ml. Nuclei werewashed and resuspended in 1 ml of reaction buffer (10 mM Tris[pH 7.5], 50 mM NaCl, 10 mM MgCl₂, 0.1 mM EDTA [pH 8.0], 0.2 mMEGTA [pH 8.0], 1 mM dithiothreitol, 0.1 mM PMSF) for every 7.5× 10⁹ starting cells. Enzyme digestion was carried out essentiallyas described previously (1). Aliquots of nuclei (200 µl) wereremoved, 100 to 200 U of enzyme was added, and the reaction mixturewas incubated at 37°C for 30 min. Reactions were stopped by theaddition of 1/10 volume of stop buffer (2% Sarkosyl, 0.4 M EDTA[pH 8], 10 mg of proteinase K/ml), and the DNA was recovered andanalyzed by Southern blotting (56). The URA3 Southern hybridizationprobe was the 248-bp EcoRV-StuI fragment from pVZURA3-1.

ChIP experiments were carried out essentially as detailed elsewhere (12, 25). Antibodies against either tetra-acetylatedhistone H4, diacetylated histone H3, unacetylated histone H3 (giftsfrom David Allis or purchased from Upstate Biotechnology), orspecific monoacetylated histone H4 lysine residues (H4KAc5, H4KAc8,H4KAc12, and H4KAc16; Serotec) were used. Production of antihistoneantibodies, their specificities and their efficacies in chromatinimmunoprecipitation (ChIP) have been described elsewhere (6,9). The anti-Sir3p and anti-Rap1p antisera were previouslydescribed (11, 38). Recovered DNA was analyzed by PCR (94°Cfor 3 min followed by 25 cycles of 45 s at 94°C, 45 s at 55°C,and 75 s at 72°C), and the amount of template DNA for PCRs wasdetermined empirically. PCR primers were URA3 5' (URA3F1, GGAAAC GAA GAT AAA TCA TGT C; URA3R1, AGG CCT CTA GGT TCC TTT GTTAC), URA3 3' (URA3F2, GTC CCA AAA TTT GTT TAC TAA AAA C; URA3R2,CTA CCT TAG CAT CCC TTC CC), AND TEL VI (TEL-300.fwd and TEL-300.rev)(34). PCR products were separated on 2% MetaPhor agarose (FMC)Tris-borate-EDTA-buffered gels, stained with ethidium bromide,and quantified by image analysis (Bio-Rad Molecular Analystsoftware).

For the G₁ arrest experiments, aDdB6PTb cells were grown in YEP-3% raffinose media to an optical density at 660 nmof 0.4. Next, $alpha$ -factor (Sigma) was added to 20 nM and potassiumhydrate phthalate (pH 5.5) was added to 50 mM, and the culturewas incubated at 30°C for 3 h to induce cell cycle arrest, asindicated by the presence of <2% budded cells (3, 8). Uponarrest, cultures were split into aliquots and either were allowedto continue growth with $alpha$ -factor in YEP-raffinose or were harvestedby centrifugation and suspended in an equal volume of warmed YEP-3%galactose medium either with or without $alpha$ -factor and potassiumhydrate phthalate. To the cultures without $alpha$ -factor 1 mg of pronase/mlwas added to degrade residual mating pheromone (8). Throughoutthis experiment the cells with $alpha$ -factor remained at <2% buds,whereas the cells without $alpha$ -factor lost the arrested phenotypeand the bud indexincreased.

RNA (20 µg of DNase I-treated total yeast RNA) was transferred by slot blotting onto 0.2-µm Nytran+ nylon membranes (Schleicher& Schuell) as described previously (4). The ACT1 probe wasthe 282-bp KpnI-PstI DNA fragment from pYST122 (6), the SWI5probe was a 2.1-kb labeled PCR product of the full-length geneamplified from YPH499 genomic DNA using the primers SWI5FF (TGGATA CAT CAA ACT CTT GGT T) and SWI5R (CCT TTG ATT AGT TTT CATTGG C), and the URA3 probe was a full-length antisense transcriptfrom BamHI-cut pVZURA3-1 transcribed in vitro by T3 RNApolymerase.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Chromatin structural changes in a telomeric URA3 gene without loss of TPE. Yeast cells expressing Ura3p die on media containing FOA. A telomeric URA3 gene is a convenient reporter for TPE, as the fractionof cells in which the telomeric URA3 is repressed can be measuredby determining the fraction of cells that grow on FOA media (19).Three previously described URA3-based reporter constructs (42)were used in the present study. In each construct, URA3 was positionednear the left telomere of yeast chromosome VII (Fig. 1A). In theUT construct, the 5' end of the URA3 transcription unit is ~1.1kb from the chromosome end (19). To make the XT construct, theGAL1,10 upstream activation sequence (UAS_G) was inserted betweenURA3 and the telomere (42). UAS_G is located immediately downstreamof URA3 and contains four wild-type Gal4p binding sites but lacksendogenous TATA sequences. When UAS_G is positioned downstreamof a gene, as at the XT telomere, it does not activate transcription(23, 50). The PT construct is similar to XT but contains theCYC1 TATA between UAS_G and the telomere. Because the CYC1 TATA-UAS_Gis located 3' of URA3 in the PT strain and because all of thestrains carried PPR1, URA3 remains under the transcriptional controlof its own promoter and trans-activator, Ppr1p. Previous studiesdemonstrated that growth of PT cells in galactose media resultsin Gal4p-mediated transcription through the telomeric tract ofC_1-3A/TG_1-3 DNA and loss of TPE (42) but that TPEat other telomeres (W. H. Tham and V. A. Zakian, unpublished)and the chromosome stability of the transcribed telomere (42)were not affected. Thus, in this system, TPE at a single telomerecan be controlled in cis without affecting other aspects of chromosomebehavior.

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FIG. 1. Chromatin from galactose-grown PT and XT cells is accessible to dam methyltransferase. (A) A conditional telomere alleviates TPE in cis. Shown is a schematic of the UT, XT, and PT telomere modifications at the ADH4 locus on the left arm of chromosome VII (42). Quantitative TPE data (percentages of FOA-resistant cells) are means ± standard deviations. The URA3 promoter is located ~1.1, 1.4, and 1.7 kb from the end of the chromosome in UT, XT, and PT cells, respectively. $left-arrow$ , C_1-3A/TG_1-3 telomeric repeat tract. Relevant restriction enzyme recognition sites are marked (D, DpnI; H, HindIII; B, BamHI). *, telomeric GATC sites (D) in URA3 that were protected from in vivo dam methylation. (B) Yeast cells expressing E. coli dam DNA methyltransferase (499LD, UTLD, XTLD, and PTLD) were grown in YEP media supplemented as shown. Purified DNA was digested with BamHI and HindIII, and some was also digested with DpnI (+), while the rest was not ( $-$ ). The DNA was analyzed by Southern blotting using a URA3 probe (19). The XT and PT strains contain two DpnI sites near the telomere. The DpnI site closest to the telomere was within the nuclease-sensitive region that is fully accessible to dam methyltransferase (56). In this experiment the accessibility of the more-internal DpnI site is monitored. Lanes 499, internal control.

The UT, XT, and PT constructs were placed in the YPH499 strain background. In raffinose media, Gal4p binds UAS_G but cannotactivate transcription, whereas in galactose media the bound Gal4pactivates transcription. As predicted from previous results (42),the three strains had equivalently high TPE when grown in FOA-raffinosemedium. Although TPE was lost in galactose-grown PT cells, TPEremained high in the galactose-grown UT and XT strains (Fig. 1A).

The E. coli dam DNA methyltransferase gene can be expressed in yeast, and the accessibility of a given GATC sequence to dammethylation in vivo is thought to reflect the degree of opennessin the surrounding chromatin structure (46). For example, asmeasured by the degree of methylation-sensitive DpnI cleavage,the single GATC site within the UT URA3 open reading frame (ORF)is inaccessible to dam methyltransferase in wild-type UT cellsbut is wholly accessible in TPE-negative UTsir2 or UTsir4 cells(20). We determined if the transcriptional state of the telomericURA3 gene in XT and PT cells also correlated with access to invivo dam methyltransferase (20). The ura3-52 allele in thesestrains, which is near the centromere of chromosome V, was usedas an internal control for full dam methyltransferase accessibility(Fig. 1B, lanes 499). DNA isolated from raffinose- and galactose-growncells was analyzed by Southern hybridization either with or withoutcleavage by DpnI (Fig. 1B).

The internal GATC site in telomeric URA3 genes was largely inaccessible to modification by dam methyltransferase in raffinose-grownUT, PT, and XT cells and in galactose-grown UT cells (Fig. 1B).However, in both PT and XT galactose-grown cells, the GATC sitewas completely accessible to the dam methyltransferase. The levelof accessibility of PT and XT in galactose medium was comparableto that of the same site in a UTsir3 strain (Fig. 1B). These resultsdemonstrate that URA3 transcription is not necessary for the chromatinalterations that allow dam methyltransferase access, as this sitewas methylated efficiently in FOA-resistant (Fig. 1A) galactose-grownXT cells (Fig. 1B). Additionally, chromatin immunoprecipitationanalysis revealed that Gal4p bound the downstream UAS_G in bothraffinose and galactose media but not in glucose medium (datanot shown). Thus, the chromatin remodeling seen in XT galactose-growncells was dependent on Gal4p activation rather than Gal4p binding.These data suggest that accessibility to the dam methyltransferasereflects an intermediate state in chromatin remodeling that isnot itself sufficient for transcriptionalactivation.

Restriction enzyme accessibility reveals promoter blocking in a repressed, telomere-linked URA3. To obtain a more detailed description of the chromatin structure of repressed and transcribed telomeric URA3 genes, we developeda restriction enzyme accessibility assay to monitor the opennessof specific DNA sequences. Purified yeast nuclei from UT and UTsir3cells were incubated with five different restriction enzymes withrecognition sites throughout the ORF or within the promoter regionof URA3 (Fig. 2A). DNA was then purified, digested with restrictionenzymes to release the telomeric fragments, and analyzed by Southernblotting using a URA3 probe (Fig. 2A). In UT nuclei, the telomericURA3 gene was largely inaccessible to digestion by all restrictionenzymes tested (Fig. 2B). A similar pattern was seen for UTsir3nuclei, except that the NdeI and DdeI restriction sites flankingthe URA3 TATA were much more accessible to restriction enzymecleavage (Fig. 2B). The increased accessibility of the NdeI andDdeI sites was not due to a loss of a neighboring nucleosome,as the nucleosome immediately adjacent to the URA3 TATA containsa recognition site for PstI (Fig. 2A) and this site was inaccessibleto cleavage in both sir3 and wild-type UT cells (Fig. 2B).

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FIG. 2. The URA3 TATA region is nuclease accessible when a telomeric gene is transcribed. (A) Cartoon of URA3 transcription unit showing six positioned nucleosomes (ovals) (51). The URA3 ORF (hatched box), URA3 TATA (gray box), relevant restriction enzyme recognition sites (H, HindIII; D, DdeI; N, NdeI; P, PstI; E, EcoRV; S, StuI; Sa, Sau3A; B, BamHI), probe, and C_1-3A/TG_1-3 telomeric repeat tract ( $left-arrow$ ) are shown. The Sau3A (DpnI) site is 203 bp from the BamHI site on the edge of the penultimate nucleosome. Vertical arrows denote restriction enzymes with recognition sites throughout the ORF or within the promoter region of URA3. (B) Restriction enzyme mapping of telomeric URA3 loci. For these experiments, the internal ura3-52 locus was deleted, so that the only URA3 sequences in the strain came from the telomere-linked gene. Isolated nuclei from UT and UTsir3 cells were incubated with either DdeI (D), NdeI (N), EcoRV (E), Sau3A (Sa), or PstI (P). Recovered DNA was digested with HindIII and StuI (lanes $-$ , D, N, P, and E) or with BamHI and HindIII (lane Sa) prior to Southern analysis using the URA3 probe. The Southern blots were quantitated by image analysis. The experiment was performed twice, and representative data are shown. (C) In vivo restriction enzyme mapping of UT, PT, and XT cells. Prior to nucleus isolation, cells were grown overnight in either raffinose or galactose media. Chromatin was analyzed as described for panel B. This experiment was performed twice, and representative data are shown.

To determine if transcription through the telomere had the same effects on restriction enzyme susceptibility as mutating sir3,raffinose- and galactose-grown UT, XT, and PT cells were examinedusing the same methods. For all three strains, the URA3 TATA wasnot accessible to either DdeI or NdeI cleavage in raffinose-growncells or in galactose-grown UT cells (Fig. 2C). However, galactose-grownPT cells were accessible to cleavage by both enzymes to an extentcomparable to that for UTsir3 cells (86 and 37% accessibilityfor the DdeI and NdeI sites, respectively, in galactose-grownPT cells versus 90 and 22%, respectively at the same sites forUTsir3 cells). In the XT strain, there was a small but reproducibleincrease in the level of DdeI accessibility in galactose-growncells (Fig. 2C). It has been proposed that proximity to a telomerediminishes the accessibility of the promoter of a telomeric gene(3). Our data provide the first evidence for this model, aswell as a new monitor for the chromatin structure of a telomere-linkedgene. On the basis of promoter accessibility, telomeric transcriptionand deletion of SIR3 had similar effects on telomericchromatin.

Telomeric chromatin is hypoacetylated at each acetylatable histone H4 lysine residue as well as in histone H3. Previous studies examining histone acetylation patterns in yeast showed that the silent HM loci are associated with hypoacetylatedhistones H3 and H4 (6, 7). However, at the HM loci, histoneH4 K12 appears hyperacetylated relative to the other lysine residuesbut hypoacetylated with respect to a sir2 mutant (7). Whenantiserum that recognizes a tetra-acetylated histone H4 is used,subtelomeric chromatin is hypoacetylated and this hypoacetylationis SIR dependent (6, 35). Here we used a quantitative ChIPto examine the acetylation status at specific lysine residuesin telomeric histone H4 as well as the general acetylation stateof histoneH3.

The strains used for ChIP analysis contained, in addition to the telomeric URA3 gene, a ura3 minigene called ura3 $Delta$ EB thatwas inserted at the nontelomeric LYS2 locus. The ura3 $Delta$ EB genehad a 78-bp deletion within the URA3 ORF. After formaldehyde fixation,a soluble chromatin fraction was prepared from UT $Delta$ EB and UTsir3 $Delta$ EBcells. Antibodies specific for various acetylated and unacetylatedforms of histones H3 and H4 were used to immunoprecipitate chromatinfragments (6, 25). The DNA in the immunoprecipitate was purifiedand subjected to quantitative competitive PCR (12) to determinethe relative levels of URA3 and ura3 $Delta$ EB present in the immunoprecipitatedchromatin.

Representative PCR results as well as the quantitation of these and other experiments obtained using URA3-specific primersare shown in Fig. 3A. The antisera specific for tetra-acetylatedhistone H4 (Fig. 3A) showed that telomeric URA3 chromatin is hypoacetylatedcompared to the internal ura3 $Delta$ EB chromatin) in wild-type cellsbut not in sir3 cells. In addition, telomeric chromatin was hypoacetylatedat histone H3, and this hypoacetylation was SIR3 dependent (Fig.3A, lanes 3+ and 3 $-$ ). By using antisera specific for each of themonoacetylated forms of histone H4 (anti-H4KAc16, anti-H4KAc12,anti-H4KAc8, and anti-H4KAc5), telomeric chromatin was shown tobe hypoacetylated at each H4 acetylatable lysine residue, includingH4 K12, and that at each residue hypoacetylation was SIR3 dependent(Fig. 3A). As a control for the telomere ChIP experiments, weexamined the histone acetylation state of the HMR locus. We foundthat histone H4 at HMR was hypoacetylated relative to ACT1 ina SIR3-dependent manner and that there was slight enrichment inH4 monoacetylated at lysine 12 at HMR chromatin compared to thelevel of acetylation of other H4 lysines (data not shown).

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FIG. 3. Histone acetylation analysis of UT $Delta$ EB and UTsir3 $Delta$ EB cells. Antibodies specific for acetylated and unacetylated histones were used to immunoprecipitate chromatin. The recovered DNA was analyzed by PCR using primers from either the 5' or 3' end of URA3. PCR products were quantitated by image analysis. To determine the relative level of histone acetylation, the URA3/ura3 $Delta$ EB ratio was calculated from an aliquot of the soluble chromatin extract and this value was used to normalize the URA3/ura3 $Delta$ EB ratios of the specific immunoprecipitates. This correction accounts for the relative immunoprecipitation efficiency of each antiserum (12). (A) (Top) Inverse of an ethidium bromide-stained agarose gel showing representative ChIP PCRs using the URA3 5' primers. T, total soluble chromatin aliquot; 4+, anti-tetra-acetylated histone H4; 3+, anti-di-acetylated histone H3; H3 $-$ , anti-unacetylated histone H3; 16+, 12+, 8+, 5+, antibodies specific for specific acetylated N-terminal lysine residues of histone H4. (Bottom) Quantitated ChIP data for subtelomeric chromatin. URA3/ura3 $Delta$ EB ratios are mean values ± standard deviations (SD) from three experiments using the 5' URA3 primers. (B) Quantitated ChIP analysis of histone acetylation state in raffinose- and galactose-grown UT $Delta$ EB, PT $Delta$ EB, and XT $Delta$ EB cells. Yeast cells were grown in the indicated media and analyzed by ChIP as described for panel A using either the anti-tetra-acetylated histone H4 antibody (anti-H4+) or the anti-unacetylated histone (anti-H3 $-$ ) antisera. URA3/ura3 $Delta$ EB ratios are the mean values ± SD from three independent assays using either the 5' URA3 or 3' URA3 primer pairs.

To determine if Gal4p binding alone and/or telomeric transcription promoted changes in histone acetylation, we examined the3' and 5' regions of the telomeric URA3 gene in UT $Delta$ EB, PT $Delta$ EB,and XT $Delta$ EB strains using quantitative ChIP and either the tetra-acetylatedhistone H4 antisera or the unacetylated histone H3 antisera (Fig.3B). In UTsir3 and PT galactose-grown cells, URA3 activation correlatedwith a 4- to 5-fold increase in histone H4 acetylation in the5' region and a 11- to 14-fold increase in the 3' region of thegene. In contrast, in UT and XT cells shifted from raffinose togalactose, histone H4 acetylation was relatively unchanged. Likewise,the acetylation of histone H3 increased 3- to 12-fold in PT galactose-grownand UTsir3 cells, whereas galactose-grown UT and XT cells showedlittle change. Thus, telomere transcription and sir3 mutationhad similar effects on histone acetylation. However, the bindingof activated Gal4p in XT galactose-grown cells was not sufficientto promote histone acetylation of subtelomericchromatin.

A switch from repressed to active transcriptional states does not require DNA replication. Earlier experiments suggested that DNA replication is necessary for a telomere-linked gene to switch from a repressed to atranscribed state (3). In particular, if ppr1 cells with atelomeric URA3 gene are arrested in G₁ and Ppr1p expression isthen induced from a plasmid, then the telomeric URA3 gene remainssilenced. In contrast, Ppr1p can induce URA3 expression in G₂/M-arrestedcells (3). We reconsidered this observation by asking if therepressed URA3 gene in galactose-grown PT cells could be reactivatedduring G₁arrest.

PT cells were grown in raffinose media to which $alpha$ -factor was added to arrest cells in late G₁ phase (26). Two criteria wereused to verify that cells remained in G₁ phase, a bud index of<2% (data not shown) and a lack of SWI5 RNA (Fig. 4A) (SWI5 isexpressed only from S through M phases) (3, 37). Once cellswere arrested, a time zero aliquot was removed for RNA analysis(Fig. 4A, sample 1). The rest of the culture was washed, resuspendedin medium containing 3% galactose, and then split in two. Oneculture was maintained in G₁ by addition of more $alpha$ -factor. Inthe second, $alpha$ -factor was removed and the cells allowed to progressthrough the cell cycle (Fig. 4A). Aliquots of cells were takenfor RNA analysis at 1-h intervals (Fig. 4A).

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FIG. 4. RNA slot blot analysis and in vivo restriction enzyme mapping of $alpha$ -factor-arrested PT cells. (A) PT cells (aDdB6PTb) were grown in raffinose media to which $alpha$ -factor was added to arrest cells in late G₁ phase. An aliquot of cells was removed (sample 1) for RNA isolation. The remainder of the culture was resuspended in galactose medium and then split into two; $alpha$ -factor was added to one culture (+), and pronase was added to the other ( $-$ ). Aliquots were removed at 1-h intervals for RNA preparation (time values are hours in galactose media for samples 2 to 11). Total RNA slot blots were hybridized with URA3, ACT1, and SWI5 probes. (B) (Top) Cells were grown in raffinose media and arrested in late G₁ with $alpha$ -factor mating pheromone. An aliquot of arrested cells (R0) was removed, and nuclei were prepared for restriction enzyme mapping. The rest of the culture was split into two parts; galactose was added to one culture, and fresh $alpha$ -factor was added to both. Aliquots were removed for preparation of the nuclei from the cultures at the indicated number of minutes. Nuclei were prepared and then either incubated without restriction enzyme ( $-$ ) or with either DdeI (D) or NdeI (N). DNA was recovered and analyzed by Southern blotting. (Bottom) Total RNA was prepared from PT cells harvested from an $alpha$ -factor arrest experiment identical to the one described above. In addition to the raffinose- or galactose-grown cultures containing $alpha$ -factor (RAF+ $alpha$ or GAL+ $alpha$ , respectively), a culture with galactose but without $alpha$ -factor (GAL- $alpha$ ) was examined. The amounts of URA3, SWI5, and ACT1 RNA were determined by slot blot analysis. The URA3 and SWI5 values were normalized to those for ACT1, and these values were plotted.

Within 1 h of galactose addition, RNA slot blot analysis showed that the telomeric URA3 gene was transcribed in both G₁-arrested(with $alpha$ -factor) and cycling (without $alpha$ -factor) cells. By the criteriaof SWI5 expression and budding index, the culture without $alpha$ -factorprogressed through the cell cycle while the cells with $alpha$ -factorremained in G₁ (Fig. 4A). These data suggest that a repressedtelomere-linked gene can be reactivated without undergoing DNAreplication.

An alternative explanation for these data is that the telomeric URA3 gene was transcribed in only a small fraction of cells.To test this possibility, we examined the chromatin structureof the telomeric URA3 gene in G₁-arrested PT cells after additionof galactose. If only a small fraction of telomeric genes weretranscribed, then we would not expect to see the changes in chromatinstructure that characterized the switch from a repressed to atranscribed state. However, by the criterion of promoter accessibility,the chromatin structure of URA3 was that of a transcribed geneby 45 min after galactose addition (Fig. 4B). Furthermore, usingthe anti-tetra-acetylated histone H4 antibody to immunoprecipitatechromatin, we found that the acetylation state of histone H4 inboth G₁-arrested and cycling galactose-grown PT cells increased(data not shown). These results indicate that transcriptionalactivation of a telomeric gene does not require cell cycleprogression.

Subtelomeric Rap1p interactions are lost upon telomere transcription. By the experimental criteria used so far, the chromatin structure of galactose-grown PT cells was indistinguishable from thatof a strain lacking Sir3p (Fig. 1 to 3). Overproduction of Sir3p,furthermore, could partially restore silencing in galactose-grownPT cells (data not shown). Moreover, earlier work showed thatthe HM loci are transcribed in the absence of DNA replicationwhen cells are depleted of Sir3p (33). These data suggestedthat the loss of silencing in galactose-grown PT cells might bedue to the loss of Sir3p from subtelomeric chromatin. ChIP analysiswas used to test directly if Sir3p was lost from subtelomericchromatin in galactose-grown PTcells.

PT $Delta$ EB cells were grown for 16 h (~10 cell divisions) in either raffinose or galactose media; UTsir3 $Delta$ EB cells were grown for16 h in raffinose media. Soluble chromatin was precipitated usingantisera for tetra-acetylated histone H4, Sir3p (anti-Sir3p),or Rap1p (anti-Rap1p). Precipitated DNA was analyzed by multiplexPCR using primers for URA3 and a unique subtelomeric region onchromosome VI (34). The URA3/ura3 $Delta$ EB ratio was calculated todetermine changes in histone acetylation relative to that of theura3 minigene. The URA3/TEL VI ratio was calculated to determineloss of Sir3p or Rap1p at the transcribed telomere relative tothe level of Sir3p or Rap1p at an unmodified subtelomeric regionon chromosome VI (Fig. 5A). For presentation purposes, the absoluteratios have been normalized to show the percentage of change.

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FIG. 5. ChIP analysis of subtelomeric Sir3p and Rap1p in PT and UTsir3 yeast. ChIP analysis was done using either an anti-tetra-acetylated histone H4 antiserum (anti-H4+), an anti-Sir3p antiserum (anti-Sir3p), or an anti-Rap1p antiserum (anti-Rap1p) as described for Fig. 3. (A) PT $Delta$ EB and UTsir3 $Delta$ EB yeast cells were grown overnight (16 h) in either raffinose (PT + RAF and UTsir3) or galactose (PT + GAL) media prior to analysis. (Left) Inverse of ethidium bromide-stained gel showing representative multiplex PCRs using the URA3 5' primers (URA3 and ura3 $Delta$ EB) and the unique chromosome VI subtelomeric primers (TEL VI). Lanes: T, total; 4+, anti-H4+; S, anti-Sir3p; R, anti-Rap1p. (Right) Quantitated ChIP data. The mean values of the URA3/ura3 $Delta$ EB and URA3/TEL VI ratios from three independent assays were calculated. These ratios were divided by either the UTsir3 value for anti-H4+ (3.2) or by the PT + RAF values for anti-Rap1p (1.1) and anti-Sir3p (1.2), and the normalized ratios were plotted. (B) Time course ChIP analysis of PT $Delta$ EB cells. Cells were grown in raffinose media and then switched to galactose media. Aliquots of cells were removed at the indicated time points and analyzed by ChIP as described for panel A.

As expected, PT cells grown in galactose for 16 h showed increased histone H4 acetylation at the PT telomere (Fig. 5A) butnot at the VI R telomere (data not shown) whereas the sir3 strainshowed increased acetylation at both (Fig. 5A and data not shown).Although the level of subtelomeric Sir3p was reduced in galactose-grownPT cells, the level of subtelomeric Sir3p at 16 h was still ~35%of the preinduction level (Fig. 5A, lanes S). In contrast, thelevel of subtelomeric Rap1p was <20% of that seen in raffinose-growncells (Fig. 5A, lanesR).

To assess the relative rates of Rap1p and Sir3p loss, the amounts of subtelomeric Rap1p and Sir3p as well as the extent ofhistone H4 acetylation were monitored shortly after the switchof PT cells to galactose medium. Within 20 min of galactose addition,the level of subtelomeric Rap1p dropped to <50% of the preinductionlevel, whereas the levels of Sir3p and histone H4 acetylationwere unchanged (Fig. 5B). Although the amount of Sir3p graduallydecreased between 20 min and 2.5 h, at 2.5 h Sir3p was still at~65% of the preinduction level. By 1 h, URA3 RNA was at high levels(Fig. 4A), even though Sir3p was still at the telomere (Fig. 5B).In contrast, at 2.5 h, the amount of subtelomeric Rap1p was reducedto background levels (Fig. 5B, 16 h). Thus, telomere transcriptionrapidly and efficiently eliminates subtelomeric Rap1p but onlypartially and more slowly removes subtelomericSir3p.

Induction of telomeric URA3 is not sufficient to disrupt subtelomeric Rap1p and Sir3p. Since telomere transcription resulted in the efficient loss of subtelomeric Rap1p, we asked if this loss was a general featureof the transcriptional reactivation of a telomeric URA3 gene.Using ChIP analysis, UT cells growing in complete medium, whereTPE is high (Fig. 1A), were compared to UT cells growing in mediumlacking uracil, where TPE is eliminated (19). RNA slot blotanalysis confirmed that the amounts of steady-state URA3 mRNAin UT cells lacking uracil and galactose-grown PT cells were similar(Fig. 6A). However, URA3 induction in the UT strain did not resultin loss of either Rap1p or Sir3p from subtelomeric chromatin,although, as expected, histone H4 acetylation increased (Fig.6B). Thus, transcriptional activation of a telomeric gene canoccur without loss of either subtelomeric Rap1p or Sir3p.

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FIG. 6. RNA and ChIP analysis of an activated telomeric URA3 gene. (A) RNA slot blot analysis of steady-state URA3 transcripts. Total yeast RNA was isolated from yeast strains with the endogenous ura3-52 sequences deleted and grown in the indicated media. The UINT strain contains a nontelomeric URA3 gene. DNase I-treated RNA was probed with either ACT1 or URA3 probes. The URA3/ACT1 ratios are means ± standard deviations obtained from three independent experiments. (B) ChIP analysis of subtelomeric histone H4, Sir3p, and Rap1p in repressed and activated UT $Delta$ EB cells. UT $Delta$ EB cells were grown overnight in the indicated media, and the chromatin was immunoprecipitated as described for Fig. 3. (Left) Inverse of ethidium bromide-stained gel showing multiplex PCRs using the URA3 5' primers (URA3 and ura3 $Delta$ EB) and the unique chromosome VI subtelomeric primers (TEL VI). Lanes, T, total; 4+, anti-H4+; S, anti-Sir3p; R, anti-Rap1p. (Right) Quantitated ChIP data. The URA3/ura3 $Delta$ EB and URA3/TEL VI ratios were calculated, and the average ratios from two independent experiments were plotted.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

It has been suggested that the transcriptional silencing of telomere-linked genes occurs because telomeric heterochromatinoccludes the promoter, thereby preventing access to transcriptionfactors (3). This paper provides the first direct evidencefor this hypothesis. Using restriction enzyme accessibility, weshow that the promoter of a telomere-linked URA3 gene was inaccessibleto restriction enzymes and that this effect was SIR3 dependent(Fig. 2). When URA3 was repressed, restriction enzyme sites flankingthe URA3 TATA sequence were inaccessible to in vivo cleavage (~5%access for repressed UT cells), whereas these sites were ~90%accessible in a UTsir3strain.

We also examined changes in the chromatin structure of a telomere-linked URA3 gene using a system wherein TPE is controlledin cis at a single telomere by transcription through the C_1-3A/TG_1-3telomere repeat tract. Telomere transcription resulted in changesin chromatin structure at the PT telomere similar to those resultingfrom deletion of SIR3: we observed enhanced access of subtelomericDNA to both dam methyltransferase (Fig. 1) and to restrictionenzymes (Fig. 2). In contrast, the XT telomere in galactose-growncells appeared to have a chromatin state intermediate betweenrepressed and transcribed states. In galactose medium, the XTtelomere was repressed (Fig. 1A), yet accessibility to the dammethyltransferase was as high as that for a transcribed telomericgene (Fig. 1B). These data show that an inaccessible chromatinstructure at the 3' end of a telomere-linked gene is not essentialfor maintaining transcriptional repression. The URA3 promoterin galactose-grown XT cells also appeared to be in an intermediatestate, as monitored via its accessibility at the DdeI site (Fig.2). Yet despite the changes in dam methyltransferase and promoteraccessibility, the acetylation of histones H3 and H4 did not increasein galactose-grown XT cells (Fig. 3B). The 5' and 3' URA3 chromatinchanges could represent preliminary steps in URA3 reactivation,such as the Gal4p-mediated recruitment of a preinitiation complexto the URA3 TATA (40). Once the complex is recruited to theURA3 TATA, elongation of the assembled transcription complex pastthe NdeI site may be blocked either by the core heterochromatinstructure (44) or by telomere-telomere or telomere-nuclear envelopeinteractions. These data suggest that certain changes in telomericchromatin structure, such as the reorganization that allows accessibilityto the dam methyltransferase, are induced prior to transcriptionbut that others, such as histone acetylation, are consequencesoftranscription.

Although yeast HM, Schizosaccharomyces pombe centromeric, and Drosophila melanogaster heterochromatins are generally hypoacetylated,there is a significant level of histone H4 lysine 12-specificacetylation (H4KAc12) present in all three (7, 12, 53).Subtelomeric chromatin had previously been shown to have low levelsof acetylated histone H4 (35). We extend this result, showingthat subtelomeric histone H4 was hypoacetylated at each acetylatablelysine, including H4KAc12, as well as at histone H3 (Fig. 3).Like the deletion of SIR3, telomere transcription in galactose-grownPT cells resulted in a 4- to 11-fold increase in subtelomerichistone acetylation relative to that for raffinose-grown cells(Fig. 3). Thus, the effects of telomere transcription on telomericchromatin structure mimic those caused by the deletion of SIR3,demonstrating that the conditional telomere was a legitimate systemfor the study ofTPE.

Telomere position effects are reversible (19). Since telomeric chromatin blocked a telomere-linked promoter (Fig. 2), DNAreplication may provide an opportunity for an activator to finda newly exposed promoter, explaining why switching from a repressedto a transcribed state is limited to a discrete part of the cellcycle (3). However, this paper demonstrated that TPE was lostin G₁-arrested PT cells when these cells were switched from raffinoseto galactose medium. Both URA3 expression (Fig. 4A) and chromatinremodeling (Fig. 4B) occurred in the absence of DNA replication.This switch was accompanied by rapid and efficient loss of subtelomericRap1p and a slower and less-complete loss of Sir3p (Fig. 5A).After ~10 generations of continuous telomere transcription, about35% of the wild-type level of subtelomeric Sir3p was still associatedwith the PT telomere, whereas the level of subtelomeric Rap1pwas ~15% of the preinduction level (Fig. 5A). Additional ChIPexperiments revealed that 20 min of telomere transcription wassufficient to remove about 60% of the subtelomeric Rap1p fromthe PT telomere, but in contrast the level of subtelomeric Sir3pwas essentially unchanged at this time point (Fig. 5B). This lossof subtelomeric Rap1p was not seen in two other situations whereTPE was disrupted, i.e., deletion of sir3 (Fig. 5A) and URA3 inductionby growth of UT cells in uracil-deficient medium (Fig. 6), noris subtelomeric Rap1p lost in galactose-grown XT cells (data notshown).

We interpret these data as indicating that telomere transcription alters the higher-order structure of telomeric chromatin,eliminating the loop postulated to form by the telomere foldingback onto subtelomeric nucleosomes (49) (Fig. 7). We proposethat DNA replication also causes telomere unfolding, and thatthis unfolding, not DNA replication per se (3), is a prerequisitefor a switch from a repressed to a transcribed state. In addition,we further suggest that, when looping is disrupted by telomeretranscription, the telomere is dislocated away from the nuclearperiphery (32, 38).

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FIG. 7. Model of how telomere transcription eliminates TPE. Growth of PT cells in galactose media eliminates telomere looping. Rap1p, in addition to being bound at the telosome, is also associated with subtelomeric chromatin for a distance of 3 to 4 kb from the telomere (49). This observation led to the model that yeast telomeres form fold-back or looped structures (22). In addition, it has been suggested that subtelomeric Rap1p may result from the spreading of Rap1p from the telomere through interactions with SIR protein complexes (16). We suggest that the rapid and efficient loss of Rap1p from the subtelomeric region of galactose-grown PT cells reflects the loss of telomere folding, which in turn eliminates Rap1p spreading and silencing at URA3.

Telomere looping may help explain the observed increase in accessibility of the URA3 promoter to restriction enzymes in galactose-grownXT cells. Since UAS_G does not function when positioned downstreamof the promoter of a nontelomeric gene (23, 50), telomerefolding could bring UAS_G-bound Gal4p to the URA3 promoter. Indeedin the absence of the GAL4-negative regulator GAL80, Gal4p canactivate URA3 from downstream and eliminate TPE in XT cells (D.de Bruin, Z. Zaman, R. A. Lieratore, and M. Ptashne, submittedfor publication), thus supporting the existence of yeast telomereloops invivo.

The analysis of mammalian telomeres suggests that looping may be a general property of eukaryotic telomeres (21). However,mammalian telomere loops appear to be critical for chromosomestability, as conditions that disrupt these loops in vivo promoteend-to-end fusions (27, 54). In contrast, in yeast, telomeretranscription disrupts looping but does not decrease chromosomestability (42). However, yeast telomere looping may still serveimportant functions. For example, telomere looping might be criticalfor telomeric silencing as well as for other telomeric positioneffects, such as blocking undesirable telomere-telomere recombinationevents (48).

	ACKNOWLEDGMENTS

We thank D. Allis for antihistone antisera, L. Pillus for the anti-Sir3p antiserum, and D. Peterson for the pUCB14HIS3 plasmid.We also thank M. A. Osley, J. Broach, E. Monson, and X. Bi fortheir helpful comments on the manuscript and P. Kaloudis for helpwith the figures. Finally, we are grateful to J. Ravetch, TheRockefeller University, for his extremely generous support ofD.D.B., S.M.K., and R.A.L.

This work was supported in part by National Institutes of Health grant GM43265 to V.A.Z. and by American Cancer Society grantPF-4236 to D.D.B.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Biology, Princeton University, Princeton, NJ 08544. Phone:(609) 258-6770. Fax: (609) 258-1701. E-mail: vzakian{at}molbio.princeton.edu.

Present address: Vanderbilt University, School of Medicine, Nashville, TN37232.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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57. Zakian, V. A. 1996. Structure, function, and replication of Saccharomyces cerevisiae telomeres. Annu. Rev. Genet. 30:141-172[CrossRef][Medline].

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