Identification of Kluyveromyces lactis Telomerase: Discontinuous Synthesis along the 30-Nucleotide-Long Templating Domain

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Molecular and Cellular Biology, September 1998, p. 4961-4970, Vol. 18, No. 9
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Identification of Kluyveromyces lactis Telomerase: Discontinuous Synthesis along the 30-Nucleotide-Long Templating Domain

Tracy Boswell Fulton and Elizabeth H. Blackburn^*

Departments of Microbiology and Immunology & Biochemistry and Biophysics, University of California, San Francisco, San Francisco, California 94143-0414

Received 30 March 1998/Returned for modification 4 May 1998/Accepted 3 June 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Telomeres in the budding yeast Kluyveromyces lactis consist of perfectly repeated 25-bp units, unlike the imprecise repeatsat Saccharomyces cerevisiae telomeres and the short (6- to 8-bp)telomeric repeats found in many other eukaryotes. Telomeric DNAis synthesized by the ribonucleoprotein telomerase, which usesa portion of its RNA moiety as a template. K. lactis telomeraseRNA, encoded by the TER1 gene, is ~1.3 kb long and contains a30-nucleotide templating domain, the largest ever examined. Toexamine the mechanism of polymerization by this enzyme, we identifiedand analyzed telomerase activity from K. lactis whole-cell extracts.In this study, we exploited the length of the template and theprecision of copying by K. lactis telomerase to examine primerelongation within one round of repeat synthesis. Under all invitro conditions tested, K. lactis telomerase catalyzed only oneround of repeat synthesis and remained bound to reaction products.We demonstrate that K. lactis telomerase polymerizes along thetemplate in a discontinuous manner and stalls at two specificregions in the template. Increasing the amount of primer DNA-templateRNA complementarity results in stalling, suggesting that the RNA-DNAhybrid is not unpaired during elongation in vitro and that lengthyduplexes hinder polymerization through particular regions of thetemplate. We suggest that these observations provide an insightinto the mechanism of telomerase and its regulation.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Telomeres, the essential protein-DNA elements at the ends of most eukaryotic chromosomes, confer chromosome stability andconstitute protective terminal caps for the genetic material ofthe cell (for a review, see reference 45). Telomeric DNA typicallyconsists of tandem arrays of a precisely repeated 5- to 8-bp sequence(for a review, see reference 17). However, the telomeric repeatunits of yeast species have greatly diverged in precision andlength (4, 26). The budding yeast Kluyveromyces lactis, witha perfectly repeated 25-bp telomeric repeat unit (27), is oneof several budding yeasts with exceptionally large telomeric repeats(26). In Saccharomyces cerevisiae and the fission yeast Schizosaccharomycespombe, the telomeric sequences are shorter, imprecisely repeatedunits (5'-TG_1-3-3' and primarily 5'-GGTTACA-3', respectively[18, 36]). Despite their variability between species, allof these telomeric sequences are specified by the enzyme telomerase.

Telomerase, a ribonucleoprotein (RNP) reverse transcriptase, facilitates the complete biosynthesis and maintenance of telomeres.Telomerase activity, as shown initially for the ciliate Tetrahymenathermophila (12) and subsequently for many other eukaryotes(3, 24, 25, 31, 35, 37, 44), is dependent on anintegral telomerase RNA component (13, 14) which containsa sequence that serves as a template for telomeric DNA synthesis(14, 43). While in T. thermophila the templating domain is5'-CAACCCCAA-3', complementary to one and a half telomeric repeats(14), in K. lactis it is a 30-nucleotide (nt) RNA sequence complementaryto one and a fifth telomere repeat units (27). Specific mutationswithin the templating domain of both T. thermophila and S. cerevisiaetelomerase RNA drastically reduce or alter telomerase activityin vitro and in vivo, suggesting that bases in the template arenot simply copied but play crucial roles in active-site functions(8, 9, 33). Active-site functions are also carried bythe reverse transcriptase protein component of telomerase (thehTERT gene product), which has been identified in Euplotes aediculatus,yeasts, and human cells (16, 23, 30, 32), confirming thattelomerase requires both reverse transcriptase protein and RNAcomponents.

Unlike the extensive RNA genome copying carried out by the more typical reverse transcriptases of viruses and retroposons,the polymerization activity of telomerase is restricted to copyingthe discrete template portion of the telomerase RNA. In vitro,telomerase elongates a telomeric DNA primer substrate, which alignswithin the templating domain via Watson-Crick base pairing (14).The sequence of the oligonucleotide primer determines the positioningof the 3' end and therefore the site of initiation. Telomerasethen extends the primer by polymerization of one nucleotide ata time along the RNA template to the 5'-end boundary. In T. thermophilaand S. cerevisiae, mutating the RNA sequence adjacent to the templatingdomain allows polymerization to proceed beyond the normal template.Hence, telomerase RNA structures or interactions outside of thetemplate also appear to prevent polymerization beyond the templateboundary (1, 33). It is not known whether during primer elongationa constant length of template RNA-product DNA hybrid is maintained(monotonic polymerization) or if the RNA-DNA duplex builds up,although it has been proposed that T. thermophila telomerase maintainsa minimal 3- to 4-bp hybrid during elongation (21). During invitro reactions, telomerases from most organisms catalyze multiplerounds of telomere repeat synthesis, and two modes of synthesis,distributive and translocative, have been distinguished. In thedistributive synthesis mode, T. thermophila telomerase dissociatesfrom its DNA product and then binds a new primer to repeat thecycle (5, 21). Translocative synthesis, catalyzed by telomerasefrom T. thermophila, E. aediculatus, Saccharomyces castellii,and human cells, involves repositioning of the 3' end of the newlyelongated primer at the beginning of the template without releaseof the product (for a review, see reference 11). Such translocationand the resulting processive synthesis of multiple repeats ona single primer in vitro are influenced by interactions of the5' end of the primer with an anchor site within a protein and/orRNA component of telomerase (5, 15, 20).

Synthesis of small repeats (such as the 6-nt repeat of T. thermophila) requires minimal relative movement within the telomeraseRNP of the built-in RNA template as it crosses the catalytic siteof the TERT protein (41). However, the templating domains ofthe yeast telomerase RNAs that have been identified, TLC1 RNAfrom S. cerevisiae and TER1 RNA from K. lactis, are considerablylarger, posing interesting mechanistic challenges to telomererepeat synthesis. TLC1 RNA contains a templating domain maximally17 nt long (39). An 11-nt portion of this domain has been shownto be copied (33), although it is rarely copied in its entiretyin vitro, resulting in a series of incomplete single-round extensionproducts (3, 23, 33, 34). Since the frequent stallingexhibited in vitro produces variable 3'-end sequences, alignmentof the partially redundant template sequence at telomeric endscan presumably take place in multiple registers and may underliethe degeneracy of the telomeric repeat sequences in vivo (3,33). The templating domain of K. lactis TER1 RNA is theoretically30 nt, longer than any examined to date, and in contrast to theirregular repeats of S. cerevisiae telomeres, the telomeric repeatunits in K. lactis are tandem arrays of perfect copies of a 25-bpsequence (27). These features suggest that K. lactis telomerasefaithfully copies its entire template.

We predicted that the properties that enable K. lactis telomerase to combine a precise mode of copying with an exceptionallylong template would be important for understanding general mechanisticfeatures of telomerase action. In particular, we anticipated thatanalysis of telomerase polymerization along a lengthy templatewould allow in-depth dissection of the steps in primer elongationoccurring within a round of repeat synthesis. In addition, K.lactis has already been established as a highly informative andexperimentally advantageous model system for studies on telomeremaintenance and length regulation (19, 27, 28).

Here we report the identification and characterization of telomerase activity from K. lactis. We show that in vitro, K. lactistelomerase catalyzes no more than a single round of repeat synthesis,remains bound to its elongated DNA products, and stalls at specificpositions along the template. Stalled complexes result from position-specificarrest and pausing; both are exacerbated by increased complementaritybetween DNA product and the RNA template. These observations providenew insights into the mechanism of polymerization by telomeraseand have implications for the in vivo functioning of the enzyme.

	MATERIALS AND METHODS

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Strain construction. The mutant telomerase RNA yeast strains used in this study (29) were constructed in a K. lactis 7B520 background, usingprocedures described previously (27).

DNA oligonucleotides. All oligonucleotides (Cruachem) were purified on denaturing polyacrylamide gels (15% polyacrylamide, 8 M urea) run in 1× Tris-borate-EDTA(TBE). DNA was eluted from excised gel fragments by overnightincubation at 30°C in distilled water with nutation. Purifiedoligonucleotides were desalted on Sep-Pak C₁₈ columns (Waters).The concentration of purified oligonucleotides was calculatedbased on (i) taking 1 OD₂₆₀ (unit of optical density at 260 nm)as representing 30 µg of DNA and (ii) the molecular weight ofthe individual oligonucleotide.

Extract preparation and fractionation. K. lactis cells were harvested at an OD₅₉₅ of 1.2 to 1.5 and resuspended in TMG buffer (10 mM Tris-HCl [pH 8], 1.2 mM MgCl₂,10% glycerol, 0.1 mM EDTA, 0.1 mM EGTA, 1.5 mM dithiothreitol[DTT], 1 µM pepstatin A, 1× EDTA-free COMPLETE protease inhibitortablet [Boehringer Mannheim]). Whole-cell extracts and S-100 supernatantswere prepared essentially as described previously (3) exceptfor extract used in the experiment shown in Fig. 1A, lanes 1 to5, which was prepared by disrupting cells with a mortar and pestleunder liquid nitrogen (7). For partial purification of telomerase,S-100 supernatants at protein concentrations of 10 to 15 mg/mlwere adjusted to 0.5 M sodium acetate (pH 8.0) and loaded onto5-ml disposable columns (Iso-Lab) packed with 2 ml of DEAE-agarose(Bio-Rad) equilibrated in the same buffer. Columns were washedwith TMG containing 0.5 M sodium acetate, and telomerase elutedwith 3 ml of TMG containing 0.7 M sodium acetate. Fractions weredesalted by dialysis (Dispo-dialysers; Spectra/Por) against TMGfor 2 h and then aliquoted and stored at $-$ 80°C. Mutant cell extractswere prepared alongside wild-type cell extracts, and equivalentamounts of protein (by Bradford assay, 10 to 15 mg/ml) were loadedonto DEAE-agarose columns. TER1 RNA levels were compared by dotblot and hybridization with a labeled TER1 probe to ensure thatextracts contained similar telomerase RNA concentrations.

In vitro telomerase reactions. Unless otherwise indicated, standard 20-µl telomerase reaction mixtures contained 50% (vol/vol) DEAE fraction, 50 mM Tris-HCl(pH 8), 1 mM spermidine, 1 mM DTT, 50 µM dTTP, 50 µM dATP, 50µM dCTP, 3.75 µM [ $alpha$ -³²P]dGTP (800 Ci/mmol), and 1 µM gel-purified oligonucleotide. Reactionswere incubated at 30°C for 20 min, stopped with the addition of2.5 µl of stop buffer (2% sodium dodecyl sulfate [SDS], 250 mMTris-HCl [pH 8], 250 mM EDTA) and 2.5 µl of proteinase K (20 mg/ml),and incubated at 65°C for 25 min. An equal amount of terminaltransferase-labeled 10-mer was added to each reaction after thestop to monitor the recovery of the products. Reaction productswere extracted with phenol-chloroform-isoamyl alcohol (25:24:1)and precipitated with 1/10 volume 3 M sodium acetate (pH 5.2),2.5 volumes of ethanol, and 10 µg of tRNA or glycogen as a carrier.For the pulse-chase and time course reactions, a nucleotide mixand a mix of the other reaction components were prewarmed separatelyat 30°C for 5 min before being mixed together, aliquots were removedat various time points, and reactions were stopped with the additionof stop buffer and proteinase K. Reaction products were resolvedon denaturing 15% acrylamide (20:1 acrylamide/bisacrylamide)-8M urea gels in 1× TBE and visualized by autoradiography. Reactionproducts were quantified either by using a Molecular DynamicsPhosphorImager and ImageQuant or by scanning and using the NIHImage program.

Sephacryl S-300 gel filtration, native gel electrophoresis, and Northern analysis. A scaled-up standard 260-µl telomerase reaction mixture with primer KL13(12) was incubated at 30°C for 7 min, mixed with aterminal transferase-labeled 30-mer (TGGGTGTGGTGTGTGGGTGTGGTGTGTGGG),and then separated on Sephacryl S-300 (Pharmacia) essentiallyas described previously (34). The reaction mixture was loadedonto a 2-ml column and eluted with TMG buffer in 150-µl fractions.A 15-µl portion of each fraction was Cerenkov counted. A 30-µlportion was further processed as described for the standard telomerasereaction. Two 30-µl aliquots from each fraction were loaded ontoseparate native gels composed of 3% acrylamide (80:1 acrylamide/bisacrylamide)and 0.6% agarose and electrophoresed in 50 mM Tris-acetate at200 V for 3 h. One gel was exposed to film immediately for 2 h.The other gel was soaked in 50% (wt/vol) urea for 20 min and transferredto a Hybond Plus membrane (Amersham) in 0.5× TBE. Since the transferredlabeled products generated considerable background signal, themembrane was set aside for approximately 2 months to allow theradioisotope to decay to a level that would not interfere withhybridization. To ensure low background levels, the membrane wasexposed to film for 2 h. The membrane was then hybridized to amixture of two ³²P-labeled probes prepared by random-prime labeling (Amersham)of PCR fragments amplified from the TER1 gene. The fragments spannt 26 to 277 and 701 to 1273 of the TER1 gene, which exclude thetemplate region. The membrane was then reexposed to film for 2h.

	RESULTS

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Identification of telomerase activity from K. lactis. To identify K. lactis telomerase in vitro, we fractionated S-100 extracts prepared from wild-type cells by ion-exchange chromatographyon a DEAE-agarose column (see Materials and Methods) and assayedfor telomerase activity. In these experiments, DEAE fractionswere incubated with one $alpha$ -³²P-radiolabeled deoxynucleoside triphosphate (dNTP), three unlabeleddNTPs, and an oligonucleotide complementary to part of the previouslyidentified K. lactis TER1 RNA templating domain (27). Afterincubation of the reaction mixture for 20 min at 30°C, reactionswere terminated and products were purified and separated on 15%denaturing polyacrylamide gels. Initially, a 17-nt-long oligonucleotide(17-mer) [KL22(17) (Fig. 1A)] was used as the DNA primer to detectpolymerization activity in extracts. ³²P-labeled products longer than the input primer by up to 8 nt(+1 to +8 products) were expected if the primer was elongatedall the way along the template. Such products were revealed, withthe majority of the labeled products appearing at +6 (Fig. 1B,lane 1, arrowhead), corresponding to a position near the presumedend of the template (Fig. 1A, arrowhead). Through the remainderof this report, we refer to these prominent products as near-terminalproducts. The high-molecular-weight products seen at the top ofthe gel were, as described previously for comparable S. cerevisiaeextracts (3, 33), independent of RNase pretreatment or telomeraseRNA as described below and were therefore not attributable totelomerase activity.

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FIG. 1. Identification of K. lactis telomerase activity in vitro. (A) Schematic of K. lactis telomerase RNA (TER1) template region and the expected alignment of the primers KL22(17) and KL12(17). Arrowhead indicates the 3' end position of correspondingly marked products in panels B and C. The boxed template residue corresponds to the site of the C-to-A mutation in the Ter1-SnaBI strain examined in panel C. (B) Telomerase reactions were carried out with primers KL22(17) (lanes 1 to 5) and KL12(17) (lanes 6 to 8) as described in Materials and Methods, with the following changes: lane 2, pretreatment of extract with proteinase K (PK; 0.5 mg/ml) for 5 min at 25°C; lanes 3 and 7, pretreatment of extract with RNase A (10 µg/ml) at 25°C for 5 min (lane 3), followed by an additional 5-min incubation with 50 U of RNasin and 1 mM DTT; lane 4, pretreatment of extract with 50 U of RNasin and 1 mM DTT at 25°C for 5 min, followed by RNase A (10 µg/ml) for an additional 5 min; lane 5, no input primer; lane 8, ddATP substituted for dATP, with chain termination product marked. Reactions in lanes 6 to 8 were performed with 7.5 µM [ $alpha$ -³²P]dTTP (400 Ci/mmol) as the radioactive label. The primer +1 position for terminal transferase-labeled KL22(17) is shown on the lower left side of lane 1. Product positions up to +8 are marked, but +8 products were visible only on longer gel exposures. Terminal transferase-labeled KL12(17) primer is in the lane marked M. Product positions up to +18 are marked, but +18 products were visible only on longer gel exposures. The high-molecular-weight products at the top of the gel were, as described previously for comparable S. cerevisiae extracts (3, 33), independent of RNase pretreatment or telomerase RNA as described below and were therefore not attributable to telomerase activity. Also, the diffuse band between +1 and +2 in lanes 1 to 5 was not produced by telomerase, as it formed independent of primer and was insensitive to RNase A and proteinase K. Std rxn, standard reaction. (C) Reactions with DEAE-fractionated extracts from wild-type (wt; lanes 1 to 7) and Ter1-SnaBI (lanes 8 to 14) strains were carried out with primer KL22(17) as described in Materials and Methods, with the following changes: lanes 1 and 8, pretreatment with RNase A as described above; lanes 3 and 10, no input primer; lanes 4 to 6 and 11 to 13, substitution of each indicated ddNTP for its partner dNTP; lanes 7 and 14, [ $alpha$ -³²P]dGTP as the sole dNTP substrate. Shaded lanes highlight nucleotide incorporation differences between the wild-type and mutant extracts. Terminal transferase-labeled KL22(17) primer (lane M) marks the primer +1 position. The nucleotides predicted to be incorporated by wild-type and Ter1-SnaBI telomerase are marked on the left and right, respectively. (D) Reactions with DEAE-fractionated extracts from wild-type (lanes 1, 2, and 5) and ter1- $Delta$ 7 (lanes 3, 4, and 6) were carried out with primer KL22(17) (lanes 1 to 4) and primer KL12(12) (lanes 5 and 6). Extract in lanes 2 and 4 was pretreated with RNase A as described above.

Telomerase activity requires input of a DNA primer and is dependent on both protein and RNA components. K. lactis polymerizationactivity fulfilled these essential criteria, as no products weredetected in the absence of a primer (Fig. 1B, lane 5), and theactivity was abolished by preincubation of the extract with eitherproteinase K or RNase A (Fig. 1B, lanes 2 and 3). RNase-pretreatedextracts sometimes produced bands (Fig. 1B, lane 3), but thesewere often variable in appearance and have never been attributableto telomerase activity. Specific polymerization still occurredwhen the telomerase preparation was incubated with RNase inhibitor(RNasin) before pretreatment with RNase A (Fig. 1B, lane 4). Hence,RNase inhibition of the activity was due to RNA digestion ratherthan other aspects of the preincubation conditions.

Further evidence that this activity was telomerase came from testing its ability to prime synthesis from another telomericoligonucleotide, KL12(17). This 17-mer was designed to align onthe template 10 nt 3' of KL22(17) (Fig. 1A). The longest majornear-terminal product produced in assays with KL12(17) (Fig. 1B,lane 6, +16 product, arrowhead) was 10 nt longer than the majorproduct from KL22(17) (Fig. 1B, lane 1, +6 product). This resultis in agreement with the predicted alignment of the primers onthe TER1 RNA template. The RNase-sensitive products seen withKL12(17) included both the near-terminal products and a set ofshorter products (Fig. 1B, lane 7). The shorter products, whichwe will refer to as mid-template products, are further characterizedbelow.

To test the prediction for TER1 RNA template-directed synthesis, we performed assays in which each unlabeled dNTP was substitutedby its ddNTP analog. With both primers, this resulted in prematurechain termination at positions predicted from the template sequence(Fig. 1B, lane 8; Fig. 1C, lanes 4 to 6). In addition, omissionof unlabeled dNTPs from the KL22(17)-primed reaction resultedin the expected strong stop at +2, after the addition of two [³²P]dG residues to the input primer (Fig. 1C, lane 7).

As a direct test for dependence on the telomerase RNA template, extracts were prepared from strains in which the telomeraseRNA gene was mutated. First, extracts were assayed from the ter1- $Delta$ 7strain (27), in which a 300-bp fragment of the TER1 gene, includingthe template, is deleted. As predicted, these extracts had noRNase-sensitive polymerization activity with either primer, demonstratingthat the template region is required for synthesis of both mid-templateand near-terminal products (Fig. 1D, lanes 3 and 6, and data notshown). Confirmation of template-directed synthesis came frommutations introduced in the template region. The Ter1-SnaBI strain(29) was engineered to contain a C-to-A mutation within theTER1 RNA template (boxed residue in Fig. 1A). Fractionated extractsprepared from this strain produced the predicted patterns of incorporation:specifically, in assays with KL22(17), chain termination due toincorporation of ddTTP occurred at +2 instead of +4 (Fig. 1C;compare lanes 5 and 12), and polymerization ended at +1 insteadof +2 in [³²P]dGTP-only reactions (Fig. 1C; compare lanes 7 and 14). Thus,the SnaBI mutation, which is incorporated into telomeres in vivo,produced the expected changes in dNTP incorporation in vitro.In addition, polymerization was specifically altered in extractsprepared from both the Ter1-SnaBI mutant and another templatemutant, Ter1-TaqI (data not shown) (29). Together, these resultsshowed that telomerase is responsible for the K. lactis polymerizationactivity.

K. lactis telomerase catalyzes a single round of telomere repeat synthesis in vitro. Under a variety of in vitro conditions, S. cerevisiae telomerase remains bound to its DNA reaction products in a manner thatprevents further elongation (34). With many different primers,polymerization by K. lactis telomerase in vitro was also foundto be confined to one round of synthesis across the template,which was often incomplete (Fig. 1B and reference 7). To addresswhether these properties of the K. lactis telomerase reactionhave a basis similar to that of S. cerevisiae telomerase, we firstcharacterized the kinetics of K. lactis telomerase by varyingthe amounts of extract and primer [KL22(17)] under standard assayconditions. Product yield increased linearly with increasing enzymeconcentration, indicating that telomerase was limiting (Fig. 2A).Reactions with various primer concentrations demonstrated thatthe 1 µM concentration used in standard assays was well abovethe apparent K_m for the reaction (Fig. 2B). In fact, maximal telomeraseactivity was observed at primer concentrations as low as 0.04µM, with no change in product distribution (data not shown). At1 µM primer, despite the large excess of primer and dNTP substratesused in all of the experiments described (see below), productyield reached a plateau by ~3 min (Fig. 2C; quantitation shownin Fig. 2D), which would not be expected if repeated cycles ofextension occurred. For example, in similar experiments with T.thermophila telomerase, total product yield increases over a periodof up to 60 min (10, 20). In a pulse-chase experiment, excessunlabeled dGTP was added to a standard reaction after 45 s andincubated for a total of 25 min. The shorter (+1 to +5) productswere chased into longer (+6 and +7) products (Fig. 2C; compare45 sec lane to P/C lane), consistent with telomerase remainingbound to the +1 to +5 products during elongation. Notably, thechase did not stimulate synthesis of multiple consecutive 25-bprepeats (Fig. 2C, in which second-round products would have beenvisible in the top quarter of the autoradiogram portion shown).These results suggested that K. lactis telomerase consistentlycatalyzes only a single round of synthesis.

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FIG. 2. Kinetics of K. lactis telomerase activity. Reactions were performed with wild-type DEAE-fractionated extract and primer KL22(17). (A) Plot of product yield from reactions containing 0, 2, 4, 8, or 10 µl of wild-type DEAE-fractionated cell extract. The sums of the +1 to +7 products for each reaction were quantified and are presented as percentages of the yield with 10 µl of extract. (B) Plot of product yield from reactions containing 0, 0.125, 0.25, 0.5, and 1 µM primer. Product yield was quantified as in panel A. (C) Reaction with 10 µl of extract and 1 µM primer incubated for various time periods. Products from a 45-s reaction followed by a 24-min chase with 100 µM unlabeled dGTP are shown in lane P/C. Any products resulting from translocative synthesis would have appeared in the top quarter of the gel region shown. (D) Plot of product yield from reactions shown in panel C. The sums of the +5 and +6 (marked by arrowhead) products were quantified from a scanned autoradiogram, using the program NIH Image, and the results are presented as percentages of the yield at 3 min.

K. lactis telomerase remains bound to reaction products. The early plateau in product yield seen in Fig. 2 was similar to that previously observed with S. cerevisiae telomerase (34)and could have been attributed to (i) dissociation and inactivationof telomerase at the completion of the reaction or (ii) telomeraseremaining bound to its reaction products, thus precluding bindingand extension of the excess free primer present in the reaction.To test directly whether telomerase enzyme remains bound to itsproducts, we used size-exclusion chromatography to determine whetherK. lactis telomerase products coeluted with the large telomeraseRNP complex, as has been shown for S. cerevisiae telomerase (34).Reactions were primed with the 12-mer oligonucleotide KL13(12),which produces a product profile similar to KL12(17), includingboth mid-template and near-terminal products. After a 7-min incubation,the reaction was size fractionated on a Sephacryl S-300 column.A portion of each fraction was electrophoresed on a native gel,transferred to a membrane, and hybridized with a radiolabeledprobe for the TER1 RNA subunit of telomerase to determine theelution profile of the telomerase complex (Fig. 3A). The hybridizationwas performed after the ³²P label incorporated into the products had decayed for 2 months,to prevent interference from any signal resulting from productsof the telomerase reaction bound to telomerase complexes. The³²P-labeled DNA products of the telomerase reaction, purified froma second aliquot of each fraction from the sizing column (seeMaterials and Methods), were separated by denaturing polyacrylamidegel electrophoresis (Fig. 3B). The remainder of each fractionwas also electrophoresed on a separate native gel and exposedto film directly, to visualize large complexes carrying ³²P label after the telomerase reaction. Although a large ³²P-labeled complex in this directly exposed native gel cofractionatedand comigrated with the TER1 RNA (data not shown), it was partiallyobscured by a background of the high-molecular-weight, non-telomerase-generated,³²P-labeled products shown in Fig. 1B. However, quantitation ofthe results shown in Fig. 3A and B clearly showed that after SephacrylS-300 chromatography, both mid-template and near-terminal productscofractionated with the TER1 RNA, peaking in fractions 4 and 5(Fig. 3C). Reaction products that had dissociated from the telomeraseRNP would have eluted in a peak following the TER1 RNA-telomeraseproduct peak. This was demonstrated by loading a marker 30-mer(previously ³²P labeled by terminal transferase) together with the telomerasereaction mix onto the Sephacryl S-300 column; the 30-mer elutedafter the telomerase product-TER1 RNA peak (Fig. 3B, top panel).A small population of telomerase products eluted after the peak(Fig. 3B and C), which may be attributable to the stability ofthe enzyme-product complex. These results indicated that K. lactistelomerase remained bound to the majority of both near-terminaland mid-template products of the extension reaction and suggestedthat each telomerase-active site carries out only one round ofextension on a given primer molecule.

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FIG. 3. Association of K. lactis telomerase with elongation products. An in vitro telomerase reaction with primer KL13(12) was performed, and then the mixture was size fractionated on Sephacryl S-300 as described in Materials and Methods. (A) Aliquots of each fraction were separated on a native gel composed of 3% polyacrylamide (80:1 acrylamide/bisacrylamide) and 0.6% agarose (lanes 1 to 10; numbers correspond to fraction numbers), along with a portion of the nonfractionated telomerase reaction (Load lane) and 10 µl of the partially purified K. lactis extract that was used in the reaction (Extract lane). The gel was transferred to a Hybond Plus membrane (Amersham) and hybridized to a mixture of two ³²P-labeled fragments of the TER1 gene that exclude the template region. (B) Aliquots of each fraction were separated on a denaturing 15% polyacrylamide (20:1 acrylamide/bisacrylamide)-8 M urea gel (lanes 1 to 10), along with a portion of the nonfractionated telomerase reaction (Load lane). Arrowhead corresponds to products described in Fig. 1B, and positions of mid-template and near-terminal products are bracketed. The upper portion of the panel shows the fractionation pattern of a telomeric 30-mer, ³²P labeled by terminal transferase and loaded on the S-300 column with the completed telomerase reaction. This portion of the panel is from an exposure of the gel 30-fold longer than that used to show telomerase products. (C) Plot of the relative amounts of TER1 RNA (A) and telomerase products (B) recovered in each fraction. Products in each fraction were quantified and are represented as a percentage of the total collected.

Telomerase stalls at specific template regions in arrested and paused conformations. As described above, the majority of the products of K. lactis telomerase were shorter than would be expected if polymerizationreached the end of the template (Fig. 1 to 3). To investigatethe influence of the primer on the progression of polymerizationalong the template, we primed telomerase reactions with a seriesof template-complementary 12-mers which align stepwise acrossthe template (Fig. 4A). Each primer was designed to anneal completelywithin the templating domain, with 3' ends at template positions12 through 3R (numbering as in Fig. 4A). Two distinct regionsof product accumulation emerged from this data set: region M (mid-template)at positions 18 through 22, and region NT (near-terminal) at positions2R through 4R (Fig. 4). A somewhat altered set of mid-templateproducts was also seen with Ter1-SnaBI mutant extracts (data notshown), again confirming that the mid-template products as wellas the near-terminal products were generated by telomerase activity.As shown in Fig. 4B for the wild-type enzyme, as primers alignedcloser to the 3' end of the template, the amount of products endingin the M region increased (compare bands in Fig. 4B marked withasterisks in lanes 12 and 17), while the amount of products endingin the NT region decreased proportionally (Fig. 4B; compare bandsmarked with arrowheads in lanes 12 and 20). Quantitation of theindividual products and correction for the number of labeled incorporatednucleotides substantiated this trend and also confirmed that theamounts of total products formed were similar for all primers.These results suggest that mid-template products accumulate atthe expense of near-terminal products. Because, as shown above,K. lactis telomerase remains bound to the majority of its extensionproducts (Fig. 3), we hypothesized that product accumulation inthe M and NT regions represents stalled telomerase-DNA complexes.Interestingly, stalling was not uniform along the template butinstead occurred specifically at these two preferred regions.

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FIG. 4. Primer-dependent stalling by K. lactis telomerase. (A) Schematic of results from assays using 12-mer oligonucleotides aligning at different positions along the template. Numbers next to primers reflect the positions of the primers' 3' end on the template, as indicated by numbers above the template. Product bands are denoted at their appropriate template positions with black dots. The size of each dot represents the relative intensity of signal from products stalled at each position, and shaded columns of dots indicate the two preferred regions of stalling. Asterisks above positions 18 through 22 and the arrowheads above positions 3R and 4R mark 3'-end positions of products shown in panel B. (B) Reactions using primers 12 to 20, as depicted in panel A. Since all primers are the same length but align stepwise across the template, elongation of primers to the same position resulted in products varied by 1 nt in length (compare positions of arrowheads and asterisks).

At limiting dNTP concentrations, telomerases from other species pause at template positions just prior to incorporation ofthat particular dNTP (20, 31, 38). Similarly, a subset ofthe stalls in the K. lactis telomerase reactions resulted fromthe low [³²P]dGTP concentration used in standard in vitro reactions, as shownby titrating unlabeled dGTP into telomerase reactions with primerKL12(12) and monitoring product formation (Fig. 5A and B). Alongwith the expected quantitative decrease in total incorporated³²P label as the unlabeled dGTP concentration was increased, thedistribution of products also changed, suggesting that stallingwas overcome at some positions along the template. However, strikingly,products at template positions 19, 20, and 21 (M stalls) remainedvisible even at 50 µM dGTP (Fig. 5A, boxed asterisks). This resultis in agreement with the accumulation of products at these sametemplate positions in the experiment shown in Fig. 1B, in whichdTTP was the limiting radiolabeled nucleotide and dGTP was notlimiting (Fig. 1B, lane 6, +7 to +9 products). After correctionfor both the decreasing specific activity and the number of radiolabeleddG residues incorporated into each product, total product formationwas similar at all dGTP concentrations, confirming that higherdGTP does not stimulate turnover. Product yields at 18 (data notshown) and 22 (Fig. 5B, small open circles) dropped as the dGTPconcentration was increased, as expected for positions precedingincorporation of dG (pre-G positions). This finding suggests thattelomerase stalled in the M region at positions 18 and 22 waspaused, awaiting incorporation of a dG residue. Yields of thelonger products at 3R and 4R in the NT region increased as thedGTP concentration was raised (Fig. 5B, filled and open triangles,respectively). However, high dGTP did not promote their extensionto the extreme terminus of the template (Fig. 5A, 5R position).Strikingly, the high dGTP concentrations only slightly affectedthe product yields for positions 19, 20, and 21 (Fig. 5B, largecircles), with the observed minor increase being attributableto depletion of smaller intermediates. Hence we conclude thatthe strong stalls at positions 19 through 21 in the M region and3R and 4R in the NT region are functionally distinct from thepauses at pre-G positions 18 and 22. As we have shown that K.lactis telomerase remains associated with its products, we willrefer to the stalls which are not elongated in response to highdGTP concentrations (at positions 19, 20, 21, 3R, and 4R) as arrestedtelomerase-product complexes.

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FIG. 5. Dependence of K. lactis telomerase stalling on nucleotide concentration. (A) Reactions using the primer KL13(12) and dGTP concentrations equaling 3.75, 5.63, 7.50, 9.38, 11.25, 18.75, 35.63, and 52.50 µM (each reaction mixture contains 50 µCi of [ $alpha$ -³²P]dGTP and a variable amount of unlabeled dGTP). Products of particular interest are marked on the left side by their 3'-end positions. Asterisks and arrowheads mark products corresponding to those shown in Fig. 4. (B) Plot of telomerase products at various dGTP concentrations. At each concentration, products stalled at template positions 18, 19, 20, 21, 22, 3R, and 4R were quantified, corrected for specific activity differences, and divided by the number of dG residues incorporated into each product. Results for position 18 were omitted due to interference of the diffuse background band visible in the last two lanes, which corresponds to the non-telomerase-generated product seen in Fig. 1B, lanes 1 to 5. (C) A scaled-up reaction mixture with 3.75 µM [ $alpha$ -³²P]dGTP was incubated for 1.5 min and then divided into three aliquots; one part was stopped (short pulse lane) with proteinase K and SDS (see Materials and Methods), the second aliquot was mixed with 100 µM unlabeled dGTP and incubated for an additional 23.5 min (long chase lane), and the third was incubated for a total of 25 min with no chase (long pulse lane). Asterisks and arrowheads mark mid-template and near-terminal products, respectively, and boxed asterisks show unchaseable products.

The assignment of stalled complexes as either paused or arrested was confirmed by a pulse-chase experiment with the same primer.Excess unlabeled dGTP was added to a reaction mixture at 45 s,and then the incubation continued for a total of 25 min (Fig.5C). Consistent with the findings from the dGTP titration, mid-templatepre-G intermediates at positions 18 and 22 that had accumulatedby 45 s (Fig. 5C, nonboxed asterisks) were chased into 3R and4R (NT region) products (Fig. 5C, arrowheads). In contrast, productyield at positions 19 through 21 was unaffected by the unlabeleddGTP chase (Fig. 5C, bands marked with asterisks), confirminga steady-state level of arrested complexes. The lack of elongationto 5R during the chase provided further evidence that most 3Rand 4R products were also arrested.

Increased primer-template complementarity exacerbates stalling. The frequency of telomerase stalling in the M region increased as primers annealed further toward the 3' end of the template(Fig. 4A and B). This could have resulted from the increased lengthof (i) just the DNA added to the primer by the enzyme, (ii) totalpotential RNA-DNA duplex created during polymerization, or (iii)the DNA product itself (primer plus added nucleotides) when polymerizationreaches the stall region, regardless of its degree of pairingto the template. To test which of these parameters influencedstalling, we performed telomerase reactions using two sets ofprimers, each set having a common 3' end but variable 5' ends.The 3' end of the first set of primers was at template position16, and with such a 12-mer primer little stalling occurred inthe M region (Fig. 4B, lane 16; Fig. 6, lane 1). However, extendingthe amount of primer-template complementarity with extra nucleotideson the 5' end of the primer dramatically increased the ratio ofmid-template products (Fig. 6, bands marked with asterisks) tonear-terminal products (lanes 1 to 5, arrowheads). In contrast,extra noncomplementary 5' nucleotides did not exacerbate stalling(lanes 6 and 7). In additional experiments, M region stallingwas also alleviated when the length of potential RNA-DNA duplexof a 12-mer ending at position 15 was reduced to 11 nt, by changingthe 5' nucleotide from the complementary dG to a dA, dT, or dCresidue (data not shown). Comparable results were seen with asecond set of primers with a common 3' end at position 22, designedto examine stalling in the NT region. Stalling at position 3Rrelative to 4R was exacerbated when the 5' end of a 12-mer wasextended with five template-complementary nucleotides (lanes 8and 9) and alleviated when the 5' end was made noncomplementary(lanes 10 and 11).

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FIG. 6. Dependence of telomerase stalling on primer-template complementarity. Lanes 1 to 7, products from reactions with primers 1 to 7 as illustrated above (lane numbers correspond to the numbers at the left of the primers). All primers have 3' ends aligning at template position 16. Primers' amounts of template complementarity increase by 1 nt at a time from 12 to 16 nt (number above each primer). Note that the overall length of the primers also increases, and therefore the +1 position changes on the gel correspondingly. Primers numbered 6 and 7 are both 16 nt long, with 12 nt of complementarity to the template. The 4 nt at the 5' end of primer 6 are the same as those of primer 5 but scrambled so that none of them are complementary to the template. The nucleotide composition of the 5' end of primer 7 is nontelomeric (ATAT). Lanes 8 to 11, products from reactions with primers, as illustrated. Primers in this set share 3' ends that align at position 22. Again, the numbers above each primer reflect their degree of complementarity to the template. Primers 10 and 11 are both 17 nt long, and both have 12 nt of complementarity to the template. The 5 nt at the 5' end of primer 10 are as in primer 9 but scrambled (as with primer 6). The 5' end of primer 11 is nontelomeric (ATATA). Asterisks and arrowheads correspond to products previously discussed.

These results demonstrated that stalling by K. lactis telomerase in vitro is not determined by the total length per se ofthe product or by the length of only the newly synthesized stretchof DNA. Instead, in the M and NT regions of the template, stallingis exacerbated by increasing the length of the potential DNA-RNAtemplate duplex. Interestingly, the class of stalled complexesinfluenced by limiting dGTP concentrations (at positions 18 and22; top and bottom bands marked with asterisks) also accumulatedin response to increased primer-template complementarity (Fig.6), suggesting an interplay between dGTP concentration and complementarityin contributing to stalling.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The telomerases described heretofore use a short template to synthesize either short, precise repeats or irregular repeats(3, 24, 25, 31, 35, 37, 44). However, K. lactistelomerase synthesizes 25-bp repeats from a 30-nt templating domain,the largest described to date (27). Here we have reported theidentification and characterization of in vitro telomerase activityfrom this budding yeast. This study reveals intriguing propertiesof K. lactis telomerase, including stalling at specific regionsof the template and the dependence of stalling on increased primer-templatecomplementarity. The establishment of an in vitro K. lactis telomerasesystem will allow other questions about telomere biology to beaddressed. For example, certain previously characterized templatemutations in K. lactis cause major effects on telomere lengthand maintenance in vivo (19, 27). It will now be possibleto distinguish whether these effects result from altered bindingof telomere-associated proteins (for example, Rap1p) or alteredtelomerase activity.

We found that K. lactis telomerase catalyzes only a single round of primer elongation in vitro, like telomerase from S. cerevisiae(3, 23, 33, 34). In K. lactis and S. cerevisiae cellslacking intact telomerase RNA, telomeres shorten by an averageof only 5 bp per cell division (27, 39). Hence in wild-typeK. lactis cells, the copying of even one-fifth of a telomericrepeat per cell division on average would be sufficient to maintaintelomere length equilibrium. Thus, single-round repeat synthesisby K. lactis telomerase could maintain telomeres in vivo. Thein vitro behavior of K. lactis telomerase reported here is consistentwith a model in which telomerase acts in each cell cycle to synthesizea small amount of telomeric DNA. Synthesis of only small incrementsper cell cycle was proposed previously for S. cerevisiae, basedon analysis of the observed small-length fluctuations of its telomeresin vivo (36). Another property of K. lactis telomerase activityreported here, its nondissociativity from reaction products, mayindicate a structural role for telomerase in a telomere-cappingcomplex, as suggested previously for S. cerevisiae telomerase(34).

An unusual property of the K. lactis telomerase activity is that it stalls during the synthesis of a telomeric repeat in atleast two specific regions of the template. The mechanistic basisfor this stalling is unknown, but it may be influenced by theconstrained nature of the template combined with the potentialto create a long RNA-DNA hybrid during polymerization. In Tetrahymenatelomerase, the regions of telomerase RNA outside the templateregion are apparently buried in the RNP (14). Therefore, themovement of the templating domain across the catalytic centerof telomerase at each polymerization step is necessarily constrainedby the anchoring of the template in the RNP by RNA-protein associations.The exacerbation of stalling that we observed upon increasingthe DNA-template RNA complementarity supports the idea that basepairing between template RNA and DNA contributes to stalling.Building up a long, presumably rigid RNA-DNA hybrid duplex duringelongation in vitro is likely to interfere with the constrainedmovement of the template through the catalytic center. Furthermore,such a duplex may also prevent the active site of the RNP fromassuming the correct conformation necessary for polymerization.Hence, as the hybrid lengthens, steric restriction may becomesufficient to prevent further polymerization.

The formation of lengthy template RNA-primer or product DNA hybrids during polymerization in vitro would imply that telomeraselacks the ability to unpair the duplex, which, as discussed above,may contribute to stalling. Other telomerases analyzed to date,including those from ciliated protozoa, human cells, and the buddingyeast S. castellii, catalyze multiple cycles of synthesis in vitro(3, 10, 15, 31), which requires unpairing of the productDNA-RNA template hybrid. Telomerase activity reconstituted froma human telomerase protein (hTERT) and the telomerase RNA component(hTR), as well as extensively purified Tetrahymena and Euplotestelomerase preparations are able to carry out translocative synthesis,indicating that such unpairing ability is intrinsic to these telomeraseenzymes and does not require other factors in vitro (6, 22,42). It has been proposed that Tetrahymena telomerase unpairsthe recently made DNA from the template through the energy ofbinding to another site in the RNP and that this site is analogousto that shown to bind the nascent transcript of RNA polymerase(21). The K. lactis telomerase preparations used in this studymay lack telomeric binding proteins, other components of the telomerasecomplex, or accessory factors such as a helicase that could alleviatestalling in vitro. Alternatively, the buildup of an RNA-DNA hybridand stalling may be inherent to the in vivo action of telomerase.

The available information is compatible with some occurrence of stalling in vivo. S. cerevisiae telomerase has been suggestedto stall frequently in vitro as copying proceeds along its template,and in this yeast, degenerate repeats are found in vivo in a patternconsistent with the in vitro properties of this enzyme (3,33). Stalling by other polymerases appears to be exploited invivo. For example, pausing by RNA polymerase in bacterial cellscoordinates transcription and other processes including translation,possibly the loading of regulatory proteins important for antiterminationand the formation of appropriate RNA structure during rRNA transcription(for a review, see reference 40). The stalling that we havereported here for K. lactis telomerase, which often results inonly partial synthesis of a repeat in vitro, is compatible withsynthesis of the perfectly repeated telomeric sequence of thisspecies in vivo as long as primer alignment on the template iscorrect before the next round of synthesis. Since the templatelacks internal redundancy, primers with 3' ends in the M or NTregion can align in a unique register, and thus incomplete extensioncould be tolerated in vivo. Hence stalling by telomerase is apotential step at which telomerase action could be regulated invivo.

The diversity of telomeric repeat lengths and sequences in budding yeasts suggests differences among the polymerization propertiesand, potentially, the evolutionary stages of their telomerases.Long-template telomerases may have been derived sporadically inbudding yeasts, arising from short template telomerases copyingbeyond their normal template boundaries. In this case, it is conceivablethat the K. lactis telomerase template positions where stallingoccurs represent the ancient boundaries of a shorter template.It has been suggested that the ancestor to telomerase was a catalyticself-replicating RNA. This ancestor is proposed to have acquireda reverse transcriptase protein component but to have retainedRNA, with at least a portion still functioning as a template (2).By this model, the long-template telomerases of budding yeastsmay represent an intermediate stage in the evolution from a ribozymethat completely copied itself to the typical short-template telomeraseswhich copy a small discrete region of RNA. Indeed, stalling bythe more primitive telomerases is one possible means that mayhave helped initiate the eventual evolution into copying progressivelyshorter regions of telomerase RNA. Further analysis of telomerasesfrom budding yeasts will be valuable for our understanding theorigins of their diverse telomere repeats and the general mechanismof telomerase.

	ACKNOWLEDGMENTS

We are grateful to M. McEachern for the strains used in this study. We thank Y. Tzfati, T. Ware, A. Krauskopf, and C. Grossfor critical reading of the manuscript, and we thank members ofthe Blackburn laboratory for helpful discussions and support.

This work was supported by NIH grants GM26259 and DE11356 to E.H.B. and NIH training grant T32 CA09270 to T.B.F.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, University of California San Francisco,San Francisco, CA 94143-0414. Phone: (415) 476-4912. Fax: (415)476-8201. E-mail: porter{at}itsa.ucsf.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Autexier, C., and C. W. Greider. 1995. Boundary elements of the Tetrahymena telomerase RNA template and alignment domains. Genes Dev. 9:2227-2239[Abstract/Free Full Text].

2. Blackburn, E. H. Telomerase. In R. F. Gesteland and J. F. Atkins (ed.), The RNA world II, in press. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

3. Cohn, M., and E. H. Blackburn. 1995. Telomerase in yeast. Science 269:396-400[Abstract/Free Full Text].

4. Cohn, M., M. J. McEachern, and E. H. Blackburn. 1998. Telomeric sequence diversity within the genus Saccharomyces. Curr. Genet. 33:83-91[Medline].

5. Collins, K., and C. W. Greider. 1993. Tetrahymena telomerase catalyzes nucleolytic cleavage and nonprocessive elongation. Genes Dev. 7:1364-76[Abstract/Free Full Text].

6. Collins, K., R. Kobayashi, and C. W. Greider. 1995. Purification of Tetrahymena telomerase and cloning of genes encoding the two protein components of the enzyme. Cell 81:677-686[Medline].

7. Fulton, T. B., and E. H. Blackburn. Unpublished data.

8. Gilley, D., and E. H. Blackburn. 1996. Specific RNA residue interactions required for enzymatic functions of Tetrahymena telomerase. Mol. Cell. Biol. 16:66-75[Abstract].

9. Gilley, D., M. S. Lee, and E. H. Blackburn. 1995. Altering specific telomerase RNA template residues affects active site function. Genes Dev. 9:2214-2226[Abstract/Free Full Text].

10. Greider, C. W. 1991. Telomerase is processive. Mol. Cell. Biol. 11:4572-4580[Abstract/Free Full Text].

11. Greider, C. W. 1995. Telomerase biochemistry and regulation, p. 35-68. In E. H. Blackburn, and C. W. Greider (ed.), Telomeres. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

12. Greider, C. W., and E. H. Blackburn. 1985. Identification of a specific telomere terminal transferase activity in Tetrahymena extracts. Cell 43:405-413[Medline].

13. Greider, C. W., and E. H. Blackburn. 1987. The telomere terminal transferase of Tetrahymena is a ribonucleoprotein enzyme with two kinds of primer specificity. Cell 51:887-898[Medline].

14. Greider, C. W., and E. H. Blackburn. 1989. A telomeric sequence in the RNA of Tetrahymena telomerase required for telomere repeat synthesis. Nature 337:331-337[Medline].

15. Hammond, P. W., T. N. Lively, and T. R. Cech. 1997. The anchor site of telomerase from Euplotes aediculatus revealed by photo-cross-linking to single- and double-stranded DNA primers. Mol. Cell. Biol. 17:296-308[Abstract].

16. Harrington, L., W. Zhou, T. McPhail, R. Oulton, D. S. Yeung, V. Mar, M. B. Bass, and M. O. Robinson. 1997. Human telomerase contains evolutionarily conserved catalytic and structural subunits. Genes Dev. 11:3109-3115[Abstract/Free Full Text].

17. Henderson, E. 1995. Telomere DNA structure, p. 11-34. In E. Blackburn, and C. W. Greider (ed.), Telomeres. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

18. Hiraoka, Y., E. Henderson, and E. H. Blackburn. 1998. Not so peculiar: fission yeast telomere repeats. Trends Biochem. Sci. 23:126[Medline].

19. Krauskopf, A., and E. H. Blackburn. 1996. Control of telomere growth by interactions of RAP1 with the most distal telomeric repeats. Nature 383:354-357[Medline].

20. Lee, M. S., and E. H. Blackburn. 1993. Sequence-specific DNA primer effects on telomerase polymerization activity. Mol. Cell. Biol. 13:6586-6599[Abstract/Free Full Text].

21. Lee, M. S., R. C. Gallagher, J. Bradley, and E. H. Blackburn. 1993. In vivo and in vitro studies of telomeres and telomerase. Cold Spring Harbor Symp. Quant. Biol. 58:707-718[Abstract/Free Full Text].

22. Lingner, J., and T. R. Cech. 1996. Purification of telomerase from Euplotes aediculatus: requirement of a primer 3' overhang. Proc. Natl. Acad. Sci. USA 93:10712-10717[Abstract/Free Full Text].

23. Lingner, J., T. R. Hughes, A. Shevchenko, M. Mann, V. Lundblad, and T. R. Cech. 1997. Reverse transcriptase motifs in the catalytic subunit of telomerase. Science 276:561-567[Abstract/Free Full Text].

24. Mantell, L. L., and C. W. Greider. 1994. Telomerase activity in germline and embryonic cells of Xenopus. EMBO J. 13:3211-3217[Medline].

25. McCormick-Graham, M., and D. P. Romero. 1996. A single telomerase RNA is sufficient for the synthesis of variable telomeric DNA repeats in ciliates of the genus Paramecium. Mol. Cell. Biol. 16:1871-1879[Abstract].

26. McEachern, M. J., and E. H. Blackburn. 1994. A conserved sequence motif within the exceptionally diverse telomeric sequences of budding yeasts. Proc. Natl. Acad. Sci. USA 91:3453-3457[Abstract/Free Full Text].

27. McEachern, M. J., and E. H. Blackburn. 1995. Runaway telomere elongation caused by telomerase RNA gene mutations. Nature 376:403-409[Medline].

28. McEachern, M. J., and E. H. Blackburn. 1996. Cap-prevented recombination between terminal telomeric repeat arrays (telomere CPR) maintains telomeres in Kluyveromyces lactis lacking telomerase. Genes Dev. 10:1822-1834[Abstract/Free Full Text].

29. McEachern, M. J., and E. H. Blackburn. Unpublished data.

30. Meyerson, M., C. M. Counter, E. N. Eaton, L. W. Ellisen, P. Steiner, S. D. Caddle, L. Ziaugra, R. L. Beijersbergen, M. J. Davidoff, Q. Liu, S. Bacchetti, D. A. Haber, and R. A. Weinberg. 1997. hEST2, the putative human telomerase catalytic subunit gene, is up-regulated in tumor cells and during immortalization. Cell 90:785-795[Medline].

31. Morin, G. B. 1989. The human telomere terminal transferase enzyme is a ribonucleoprotein that synthesizes TTAGGG repeats. Cell 59:521-529[Medline].

32. Nakamura, T. M., G. B. Morin, K. B. Chapman, S. L. Weinrich, W. H. Andrews, J. Lingner, C. B. Harley, and T. R. Cech. 1997. Telomerase catalytic subunit homologs from fission yeast and human. Science 277:955-959[Abstract/Free Full Text].

33. Prescott, J., and E. H. Blackburn. 1997. Telomerase RNA mutations in Saccharomyces cerevisiae alter telomerase action and reveal nonprocessivity in vivo and in vitro. Genes Dev. 11:528-540[Abstract/Free Full Text].

34. Prescott, J., and E. H. Blackburn. 1997. Functionally interacting telomerase RNAs in the yeast telomerase complex. Genes Dev. 11:2790-2800[Abstract/Free Full Text].

35. Prowse, K. R., A. A. Avilion, and C. W. Greider. 1993. Identification of a nonprocessive telomerase activity from mouse cells. Proc. Natl. Acad. Sci. USA 90:1493-1497[Abstract/Free Full Text].

36. Shampay, J., and E. H. Blackburn. 1988. Generation of telomere-length heterogeneity in Saccharomyces cerevisiae. Proc. Natl. Acad. Sci. USA 85:534-538[Abstract/Free Full Text].

37. Shippen-Lentz, D., and E. H. Blackburn. 1989. Telomere terminal transferase activity from Euplotes crassus adds large numbers of TTTTGGGG repeats onto telomeric primers. Mol. Cell. Biol. 9:2761-2764[Abstract/Free Full Text].

38. Shippen-Lentz, D., and E. H. Blackburn. 1990. Functional evidence for an RNA template in telomerase. Science 247:546-552[Abstract/Free Full Text].

39. Singer, M. S., and D. E. Gottschling. 1994. TLC1: template RNA component of Saccharomyces cerevisiae telomerase. Science 266:404-409[Abstract/Free Full Text].

40. Uptain, S. M., C. M. Kane, and M. J. Chamberlin. 1997. Basic mechanisms of transcript elongation and its regulation. Annu. Rev. Biochem. 66:117-172[Medline].

41. Wang, H., D. Gilley, and E. H. Blackburn. 1998. A novel specificity for the primer-template pairing requirement in Tetrahymena telomerase. EMBO J. 17:1152-1160[Medline].

42. Weinrich, S. L., R. Pruzan, L. Ma, M. Ouellette, V. M. Tesmer, S. E. Holt, A. G. Bodnar, S. Lichtsteiner, N. W. Kim, J. B. Trager, R. D. Taylor, R. Carlos, W. H. Andrews, W. E. Wright, J. W. Shay, C. B. Harley, and G. B. Morin. 1997. Reconstitution of human telomerase with the template RNA component hTR and the catalytic protein subunit hTRT. Nat. Genet. 17:498-502[Medline].

43. Yu, G. L., J. D. Bradley, L. D. Attardi, and E. H. Blackburn. 1990. In vivo alteration of telomere sequences and senescence caused by mutated Tetrahymena telomerase RNAs. Nature 344:126-132[Medline].

44. Zahler, A. M., and D. M. Prescott. 1988. Telomere terminal transferase activity in the hypotrichous ciliate Oxytricha nova and a model for replication of the ends of linear DNA molecules. Nucleic Acids Res. 16:6953-6972[Abstract/Free Full Text].

45. Zakian, V. 1995. Saccharomyces telomeres: function, structure, and replication, p. 107-138. In E. Blackburn, and C. Greider (ed.), Telomeres. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

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McEachern, M. J., Iyer, S., Fulton, T. B., Blackburn, E. H. (2000). Telomere fusions caused by mutating the terminal region of telomeric DNA. Proc. Natl. Acad. Sci. USA 97: 11409-11414 [Abstract] [Full Text]

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1.	Autexier, C., and C. W. Greider. 1995. Boundary elements of the Tetrahymena telomerase RNA template and alignment domains. Genes Dev. 9:2227-2239[Abstract/Free Full Text].
2.	Blackburn, E. H. Telomerase. In R. F. Gesteland and J. F. Atkins (ed.), The RNA world II, in press. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
3.	Cohn, M., and E. H. Blackburn. 1995. Telomerase in yeast. Science 269:396-400[Abstract/Free Full Text].
4.	Cohn, M., M. J. McEachern, and E. H. Blackburn. 1998. Telomeric sequence diversity within the genus Saccharomyces. Curr. Genet. 33:83-91[Medline].
5.	Collins, K., and C. W. Greider. 1993. Tetrahymena telomerase catalyzes nucleolytic cleavage and nonprocessive elongation. Genes Dev. 7:1364-76[Abstract/Free Full Text].
6.	Collins, K., R. Kobayashi, and C. W. Greider. 1995. Purification of Tetrahymena telomerase and cloning of genes encoding the two protein components of the enzyme. Cell 81:677-686[Medline].
7.	Fulton, T. B., and E. H. Blackburn. Unpublished data.
8.	Gilley, D., and E. H. Blackburn. 1996. Specific RNA residue interactions required for enzymatic functions of Tetrahymena telomerase. Mol. Cell. Biol. 16:66-75[Abstract].
9.	Gilley, D., M. S. Lee, and E. H. Blackburn. 1995. Altering specific telomerase RNA template residues affects active site function. Genes Dev. 9:2214-2226[Abstract/Free Full Text].
10.	Greider, C. W. 1991. Telomerase is processive. Mol. Cell. Biol. 11:4572-4580[Abstract/Free Full Text].
11.	Greider, C. W. 1995. Telomerase biochemistry and regulation, p. 35-68. In E. H. Blackburn, and C. W. Greider (ed.), Telomeres. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
12.	Greider, C. W., and E. H. Blackburn. 1985. Identification of a specific telomere terminal transferase activity in Tetrahymena extracts. Cell 43:405-413[Medline].
13.	Greider, C. W., and E. H. Blackburn. 1987. The telomere terminal transferase of Tetrahymena is a ribonucleoprotein enzyme with two kinds of primer specificity. Cell 51:887-898[Medline].
14.	Greider, C. W., and E. H. Blackburn. 1989. A telomeric sequence in the RNA of Tetrahymena telomerase required for telomere repeat synthesis. Nature 337:331-337[Medline].
15.	Hammond, P. W., T. N. Lively, and T. R. Cech. 1997. The anchor site of telomerase from Euplotes aediculatus revealed by photo-cross-linking to single- and double-stranded DNA primers. Mol. Cell. Biol. 17:296-308[Abstract].
16.	Harrington, L., W. Zhou, T. McPhail, R. Oulton, D. S. Yeung, V. Mar, M. B. Bass, and M. O. Robinson. 1997. Human telomerase contains evolutionarily conserved catalytic and structural subunits. Genes Dev. 11:3109-3115[Abstract/Free Full Text].
17.	Henderson, E. 1995. Telomere DNA structure, p. 11-34. In E. Blackburn, and C. W. Greider (ed.), Telomeres. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
18.	Hiraoka, Y., E. Henderson, and E. H. Blackburn. 1998. Not so peculiar: fission yeast telomere repeats. Trends Biochem. Sci. 23:126[Medline].
19.	Krauskopf, A., and E. H. Blackburn. 1996. Control of telomere growth by interactions of RAP1 with the most distal telomeric repeats. Nature 383:354-357[Medline].
20.	Lee, M. S., and E. H. Blackburn. 1993. Sequence-specific DNA primer effects on telomerase polymerization activity. Mol. Cell. Biol. 13:6586-6599[Abstract/Free Full Text].
21.	Lee, M. S., R. C. Gallagher, J. Bradley, and E. H. Blackburn. 1993. In vivo and in vitro studies of telomeres and telomerase. Cold Spring Harbor Symp. Quant. Biol. 58:707-718[Abstract/Free Full Text].
22.	Lingner, J., and T. R. Cech. 1996. Purification of telomerase from Euplotes aediculatus: requirement of a primer 3' overhang. Proc. Natl. Acad. Sci. USA 93:10712-10717[Abstract/Free Full Text].
23.	Lingner, J., T. R. Hughes, A. Shevchenko, M. Mann, V. Lundblad, and T. R. Cech. 1997. Reverse transcriptase motifs in the catalytic subunit of telomerase. Science 276:561-567[Abstract/Free Full Text].
24.	Mantell, L. L., and C. W. Greider. 1994. Telomerase activity in germline and embryonic cells of Xenopus. EMBO J. 13:3211-3217[Medline].
25.	McCormick-Graham, M., and D. P. Romero. 1996. A single telomerase RNA is sufficient for the synthesis of variable telomeric DNA repeats in ciliates of the genus Paramecium. Mol. Cell. Biol. 16:1871-1879[Abstract].
26.	McEachern, M. J., and E. H. Blackburn. 1994. A conserved sequence motif within the exceptionally diverse telomeric sequences of budding yeasts. Proc. Natl. Acad. Sci. USA 91:3453-3457[Abstract/Free Full Text].
27.	McEachern, M. J., and E. H. Blackburn. 1995. Runaway telomere elongation caused by telomerase RNA gene mutations. Nature 376:403-409[Medline].
28.	McEachern, M. J., and E. H. Blackburn. 1996. Cap-prevented recombination between terminal telomeric repeat arrays (telomere CPR) maintains telomeres in Kluyveromyces lactis lacking telomerase. Genes Dev. 10:1822-1834[Abstract/Free Full Text].
29.	McEachern, M. J., and E. H. Blackburn. Unpublished data.
30.	Meyerson, M., C. M. Counter, E. N. Eaton, L. W. Ellisen, P. Steiner, S. D. Caddle, L. Ziaugra, R. L. Beijersbergen, M. J. Davidoff, Q. Liu, S. Bacchetti, D. A. Haber, and R. A. Weinberg. 1997. hEST2, the putative human telomerase catalytic subunit gene, is up-regulated in tumor cells and during immortalization. Cell 90:785-795[Medline].
31.	Morin, G. B. 1989. The human telomere terminal transferase enzyme is a ribonucleoprotein that synthesizes TTAGGG repeats. Cell 59:521-529[Medline].
32.	Nakamura, T. M., G. B. Morin, K. B. Chapman, S. L. Weinrich, W. H. Andrews, J. Lingner, C. B. Harley, and T. R. Cech. 1997. Telomerase catalytic subunit homologs from fission yeast and human. Science 277:955-959[Abstract/Free Full Text].
33.	Prescott, J., and E. H. Blackburn. 1997. Telomerase RNA mutations in Saccharomyces cerevisiae alter telomerase action and reveal nonprocessivity in vivo and in vitro. Genes Dev. 11:528-540[Abstract/Free Full Text].
34.	Prescott, J., and E. H. Blackburn. 1997. Functionally interacting telomerase RNAs in the yeast telomerase complex. Genes Dev. 11:2790-2800[Abstract/Free Full Text].
35.	Prowse, K. R., A. A. Avilion, and C. W. Greider. 1993. Identification of a nonprocessive telomerase activity from mouse cells. Proc. Natl. Acad. Sci. USA 90:1493-1497[Abstract/Free Full Text].
36.	Shampay, J., and E. H. Blackburn. 1988. Generation of telomere-length heterogeneity in Saccharomyces cerevisiae. Proc. Natl. Acad. Sci. USA 85:534-538[Abstract/Free Full Text].
37.	Shippen-Lentz, D., and E. H. Blackburn. 1989. Telomere terminal transferase activity from Euplotes crassus adds large numbers of TTTTGGGG repeats onto telomeric primers. Mol. Cell. Biol. 9:2761-2764[Abstract/Free Full Text].
38.	Shippen-Lentz, D., and E. H. Blackburn. 1990. Functional evidence for an RNA template in telomerase. Science 247:546-552[Abstract/Free Full Text].
39.	Singer, M. S., and D. E. Gottschling. 1994. TLC1: template RNA component of Saccharomyces cerevisiae telomerase. Science 266:404-409[Abstract/Free Full Text].
40.	Uptain, S. M., C. M. Kane, and M. J. Chamberlin. 1997. Basic mechanisms of transcript elongation and its regulation. Annu. Rev. Biochem. 66:117-172[Medline].
41.	Wang, H., D. Gilley, and E. H. Blackburn. 1998. A novel specificity for the primer-template pairing requirement in Tetrahymena telomerase. EMBO J. 17:1152-1160[Medline].
42.	Weinrich, S. L., R. Pruzan, L. Ma, M. Ouellette, V. M. Tesmer, S. E. Holt, A. G. Bodnar, S. Lichtsteiner, N. W. Kim, J. B. Trager, R. D. Taylor, R. Carlos, W. H. Andrews, W. E. Wright, J. W. Shay, C. B. Harley, and G. B. Morin. 1997. Reconstitution of human telomerase with the template RNA component hTR and the catalytic protein subunit hTRT. Nat. Genet. 17:498-502[Medline].
43.	Yu, G. L., J. D. Bradley, L. D. Attardi, and E. H. Blackburn. 1990. In vivo alteration of telomere sequences and senescence caused by mutated Tetrahymena telomerase RNAs. Nature 344:126-132[Medline].
44.	Zahler, A. M., and D. M. Prescott. 1988. Telomere terminal transferase activity in the hypotrichous ciliate Oxytricha nova and a model for replication of the ends of linear DNA molecules. Nucleic Acids Res. 16:6953-6972[Abstract/Free Full Text].
45.	Zakian, V. 1995. Saccharomyces telomeres: function, structure, and replication, p. 107-138. In E. Blackburn, and C. Greider (ed.), Telomeres. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.