Targeting of the Yeast Ty5 Retrotransposon to Silent Chromatin Is Mediated by Interactions between Integrase and Sir4p

doi:10.1128/MCB.21.19.6606-6614.2001

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Molecular and Cellular Biology, October 2001, p. 6606-6614, Vol. 21, No. 19
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.19.6606-6614.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Targeting of the Yeast Ty5 Retrotransposon to Silent Chromatin Is Mediated by Interactions between Integrase and Sir4p

Weiwu Xie,¹ Xiaowu Gai,¹ Yunxia Zhu,¹ David C. Zappulla,² Rolf Sternglanz,² and Daniel F. Voytas¹^,^*

Department of Zoology and Genetics, Iowa State University, Ames, Iowa 50011-3260,¹ and Department of Biochemistry and Cell Biology, State University of New York, Stony Brook, New York 11794-5215²

Received 12 March 2001/Returned for modification 8 May 2001/Accepted 30 June 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Ty5 retrotransposons of Saccharomyces cerevisiae integrate preferentially into regions of silent chromatin at the telomeresand silent mating loci (HMR and HML). We define a Ty5-encodedtargeting domain that spans 6 amino acid residues near the C terminusof integrase (LXSSXP). The targeting domain establishes silentchromatin when it is tethered to a weakened HMR-E silencer, andit disrupts telomeric silencing when it is overexpressed. As determinedby both yeast two-hybrid and in vitro binding assays, the targetingdomain interacts with the C terminus of Sir4p, a structural componentof silent chromatin. This interaction is abrogated by mutationsin the targeting domain that disrupt integration into silent chromatin,suggesting that recognition of Sir4p by the targeting domain isthe primary determinant in Ty5 targetspecificity.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The long terminal repeat (LTR) retrotransposons are a large and ubiquitous class of mobile genetic elements. Like their cousinsthe retroviruses, they replicate by reverse transcribing an elementmRNA and then integrating the cDNA product into their host's chromosomes.LTR retrotransposons are typically abundant components of nucleargenomes, constituting a few percentages of the Saccharomyces cerevisiaegenome to over 50% of the genomes of some plants such as maize(31, 45). As the genome sequencing projects progress, it isapparent that most retrotransposons are not randomly distributedon chromosomes. In Drosophila melanogaster and Arabidopsis thaliana,for example, retrotransposons are highly enriched in pericentromericheterochromatin (19, 44). This nonrandom distribution maybe the result of preferential integration to these sites. It hasbeen suggested that the low gene density of heterochromatin mayoffer a safe haven for transposition, which ensures persistenceof retrotransposons by avoiding the harmful consequences of mutationsthat might occur if integration were random (5). Because repetitivesequences can form heterochromatin in some species, the accumulationof retrotransposons in certain regions of the genome may, in turn,contribute to the formation of chromatin domains (18).

How is it that retrotransposons identify certain chromosomal regions during integration? One model suggests that the integrationapparatus recognizes specific chromatin states or DNA-bound proteincomplexes (7). This interaction tethers the integration machineryto target sites and results in the observed target site biases.This model is best supported by studies of the S. cerevisiae retrotransposons.Over 90% of native Ty1, Ty2, Ty3, and Ty4 insertions are locatedupstream of genes transcribed by RNA polymerase III (RNAP III)(31). These regions are often gene poor and, like heterochromatin,may provide a safe haven for transposition within the streamlinedS. cerevisiae genome (5). For Ty1 and Ty3, the associationwith sites of RNAP III transcription is due to targeted integration.Targeting requires assembly of the RNAP III transcription complex,and promoter mutations in target genes that prevent transcriptioncomplex assembly render them inefficient targets (8, 9,13). In vitro targeted-transposition assays have been developedfor Ty3 in which binding of TFIIIB and TFIIIC to tRNA gene templatesis sufficient for targeting (32). The critical factors withinthese complexes appear to be the TATA binding protein and Brf(also called TFIIIB70) (50). These data support the model thattargeting results when the retrotransposon preintegration complexrecognizes specific DNA-boundproteins.

In contrast to the other S. cerevisiae retrotransposons, native Ty5 elements are not located at sites of RNAP III transcription.Rather, like retrotransposons in many other organisms, Ty5 insertionsare predominantly found within the heterochromatin-like domainsof the S. cerevisiae genome, such as at the telomeres and silentmating loci (HMR and HML) (57). The chromatin at these sitesis referred to as silent chromatin, because it represses transcriptionof genes located in these regions. Silent chromatin is made upof a large number of proteins that assemble at specific DNA sequences(reviewed in references 35 and 36). Several proteins or proteincomplexes bind the E and I silencers that flank HMR and HML, includingthe origin recognition complex (ORC), the transcription factorAbf1, and the repressor activator protein Rap1p. These proteinsalso bind to sequences near the telomeres: ORC and Abf1 bind tothe subtelomeric X repeat, and Rap1p binds to the telomeric repeatsequences (TG_1-3). These DNA-bound proteins recruit additionalcomponents of silent chromatin, including the well-studied Sirproteins. Sir2p is a histone deacetylase (21, 33, 47), andSir3p and Sir4p are considered structural components of silentchromatin. All three proteins interact with each other, and theynucleate at the silencers and spread outward along the chromosome(17, 40).

Ty5 integrates preferentially into regions of silent chromatin. Over 95% of de novo Ty5 transposition events occur withina 3-kb window on either side of the HM silencers or the subtelomericX repeat (54, 55). Silent chromatin is required for this targetchoice, because mutations in HMR-E that prevent its assembly abolishtargeting to this locus (56). Targeting decreases by approximately50% in sir2 $Delta$ strains, whereas it is virtually abolished in sir3 $Delta$ and sir4 $Delta$ strains (53). An allele of SIR4 (sir4-42) causes adramatic change in the chromosomal distribution of the Sir complex(29). In sir4-42 strains, Sir3p and Sir4p move from the telomeresand silent mating loci to the ribosomal DNA (rDNA) (30). Thischange in Sir protein distribution is related to mother cell aging,and sir4-42 strains are long-lived (29). Ty5 target specificitychanges with the chromosomal distribution of the Sir complex insir4-42 strains, and over 25% of the insertions occur within therDNA (53). These results suggest that the Sir complex, particularlySir3p and Sir4p, determines Ty5 targetchoice.

Ty5-encoded proteins are also important for target site selection. A Ty5 missense mutation decreases targeting more than 20-foldand provides the first direct evidence that retroelements encodetheir own targeting determinants (14). In this paper, we furtherdefine Ty5-encoded factors required for targeting and describea short targeting domain (TD) near the integrase C terminus (INC).This TD interacts with silent chromatin because, when tetheredto a defective HMR-E silencer, reporter genes at HMR are transcriptionallysilenced in a Sir-dependent fashion. Overexpression of the TDdisrupts telomeric silencing, likely by titrating away criticalsilencing components. We show that the TD interacts with Sir4pin both yeast two-hybrid and in vitro binding assays. Sir4p, therefore,appears to be the primary host determinant mediating Ty5 targetspecificity, and the interaction between the Ty5-encoded TD andSir4p appears to determine targetchoice.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Mutagenesis of Ty5 elements. A BspEI-PflMI fragment of Ty5 (Fig. 1) was mutagenized by PCR, using two different protocols to minimize mutation biases.The first used the nucleoside triphosphate analogue dPTP, whichpairs with both A and G and thereby increases the mutation spectrum(51). A typical 20-µl reaction mixture included 5 ng of templateDNA (pXW27, a plasmid containing the BspEI-PflMI fragment), 2.5U of Taq polymerase, 2 µl of 10× buffer, 0.5 µl of the universaland reverse primers (20 pM), 1.6 µl of 25 mM MgCl₂, 4 µl of deoxynucleosidetriphosphates (dNTPs) (2.5 mM each), and 2.5 µl of dPTP (400 µM).The PCR was carried out for five cycles as follows: 92°C for 1min, 50°C for 1.5 min, and 72°C for 5 min. An aliquot of the reactionmixture (0.5 µl) was then used for PCR amplification without dPTP(3). The second mutagenesis method used Mn²⁺ (rather than Mg²⁺) and biased amounts of dNTPs (46). A typical 50-µl reactionmixture included 5 ng of template DNA, 2.5 U of Taq polymerase,5 µl of 10× buffer, 0.5 µl of each primer (20 pM), 14 µl of 25mM MgCl₂, 0.75 µl of 10 mM MnCl₂, 4 µl of dNTPs (2.5 mM each),4 µ l of dCTP (10 mM), and 4 µl of dTTP (10 mM). The PCR was carriedout for 13 cycles as follows: 94°C for 30 s, 50°C for 45 s, and72°C for 3 min. An aliquot of the reaction mixture (0.5 µl) wasused as a template in a standard PCR amplification (3). Themutant Ty5 library was constructed by replacing the mutagenizedBspEI-PflMI fragment with the corresponding fragment in a wild-typeTy5 element on pNK254 (27).

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FIG. 1. The Ty5 TD is located at the C terminus of integrase. (A) Ty5 is 5,375 bp in length. It expresses a full-length protein of 182 kDa, which is processed by protease (PR) into Gag, IN, and RT (22). The cleavage sites, based on the mobilities of mature proteins by SDS-PAGE, are shown by dashed lines. The black bar marks the position of TD. The BspEI and PflMI sites define the region of IN used in the mutagenesis experiment. pIP19, pWW32, and pWW59 carry Ty5 elements that were modified by an RGS-H₆ tag. The tag replaced TD (pWW59) or was inserted either into the middle of IN (pWW32) or at the end of RT (pIP19) (22). (B) The modified Ty5 elements were expressed in yeast, and an anti-RGS-H₆ antibody was used to identify IN or RT on immunoblots. The partially processed and mature protein species are indicated. (C) The Ty5 IN fragments used throughout this paper are shown. INC and inc are 258 aa long (the small letters indicate the version with the S1094L mutation). TD and td represent the wild-type and mutant TD plus 3 flanking aa from Ty5. (D) Western blots demonstrating that the wild-type and mutant GBD fusion proteins are expressed at comparable levels in the test strains (YSB2 and UCC3505). GBD-INC and GBD-TD have molecular masses of approximately 47 and 19 kDa, respectively.

Mutations were made by PCR-based site-directed mutagenesis to define the TD. pNK254 was PCR amplified using the reverse primerand a mutagenic primer. The amplification product was digestedwith EcoRI and then inserted into the EcoRI site of pWW37, a Ty5subclone containing an HpaI-SacI fragment. The BspEI-PflMI fragmentof the recombinant plasmid was used to replace the correspondingfragment in pNK254. The mutagenic primers were as following: DVO754for mutant pWW39 (5'-GGA-ATT-CAA-TCG-AAT-CTC-CTC-CAT-CGG-TGG-ATT-CAT-C),DVO755 for mutant pWW40 (5'-GGA-ATT-CAA-TCG-AAT-CTC-CTC-CAT-CGT-TGG-CTT-CAT-CGC-C),DVO756 for mutant pWW41 (5'-GGA-ATT-CAA-TCG-AAT-CTC-CTC-CAT-CGT-TGG-ATT-CAT-CGG-CTC-CAA-ATA-C),DVO757 for mutant pWW42 (5'-GGA - ATT - CAA - TCG - AAT - CTC- CTC - CAT - CGT - TGG - ATT - CAT - CGC - CTC - CAG-CTA-CCT-CAT-TT),DVO631 for mutant pXW198 [5'-GGA-ATT-CAA-TCG-AA(T/G)-CTC-CTC-CA(T/G)-CGT-TGG-AT],DVO632 for mutants pXW199, pXW200, and pXW201 [5'-GGA-ATT-CAA-TCG-AAT-CT(C/G)-CT(C/G)-CAT-CGT-TG],and DVO634 for mutant pXW202 [5'-GGA-ATT-CGG - TCG - AAT - CTC- CTC - CAT - CGT - TGG - ATT - CAT - CGC - CTC - CAA - AT(A/G)-CC(T/G)-CAT-TTA-AC].

The Ty5 mutants rut3, rut15, rut31, rut38, rut41, and rut46 were constructed by replacing an EcoRI-PflMI fragment of the wild-typeTy5 element on pNK254 with the corresponding fragment from mutantsut3, ut15, ut31, ut38, ut41, and ut46. Because of the multipleEcoRI sites in Ty5, this was accomplished in two steps: first,an EcoRI-EcoRI fragment from the original mutant element was insertedinto the EcoRI site of plasmid pWW37, which contains an HpaI-SacIfragment of Ty5; second, the BspEI-PflMI fragment of the resultingplasmid was used to replace the corresponding fragment of pNK254.For all mutant elements tested in this study, targeting was measuredusing our plasmid-based targeting assay described in detail inour previous study (14).

Tethered silencing. Gal4p DNA binding domain (GBD) fusion proteins were generated using pGBD plasmids, which contain the GAL4 DNA binding domainunder the control of the ADH1 promoter (24). The plasmid expressingGBD-INC (pXW140) contains amino acids (aa) 879 to 1136 of Ty5inserted between the BamHI and PstI sites of pGBDU; the GBD-incconstruct (pXW158) is identical, except that it carries the S1094Lmutation (14). The plasmid expressing TD fused to GBD (GBD-TD)(pXW205) was generated by inserting into the EcoRI and BglII sitesof pGBDU a short DNA fragment created from two complementary oligonucleotides,DVO690 (5'-AAT-TCT-TGG-ATT-CAT-CGC-CTC-CAA-ATA-CCT-CA) and DVO691(5'-GAT-CTG-AGG-TAT-TTG-GAG-GCG-ATG-AAT-CCA-AG); the GBD-td construct(pXW213) is identical, except that it has the S1094L mutation.We generated versions of these plasmids (pWW48, GBD; pWW49, GBD-TD;pWW50, GBD-td) in which the TRP1 marker gene of pGBD was replacedwith HIS3. This was accomplished by replacing the EcoRV-XbaI fragmentwith a HIS3-containing NruI-XbaI fragment. LEU2-based expressionplasmids (pWW44, GBD; pWW45, GBD-TD; pWW46, GBD-td) were generatedby swapping the Gal4p activation domain (GAD)-encoding SphI fragmentfrom pGAD (which has the LEU2 marker [24]) with an SphI fragmentencoding the various GBD fusionproteins.

To test silencing of the HMR reporter gene, the above-described expression plasmids were transformed into strains with differentHMR-E mutations (10). These strains include YSB1 (aeB but noUASg), YSB2 (aeB::3×UASg) and YSB35 (Aeb::3×UASg). sir derivativesof YSB2 and YSB35 include RS1072 and RS112 (sir1::URA3), RS1042and RS1132 (sir2::URA3), RS1061 and RS1133 (sir3::URA3), and RS1067(sir4::URA3) (1). The strain used to assess telomeric silencingwas UCC3505 (kind gift of D. Gottschling) (16). Complementationof GBD-TD-induced loss of telomeric silencing was tested by introducingSIR genes (kind gift of J. Rine) on a 2µm plasmid (pRS424 [11]).The SIR2 plasmid (pSZ270) carries a NotI-XhoI fragment from pRS315-SIR2,the SIR3 plasmid (pSZ282) carries a BamHI-SalI fragment from pJR104,and the SIR4 plasmid (pSZ269) carries a SacII-ClaI fragment frompRS316-SIR4. To measure silencing, an overnight culture was grownto saturation for each strain and adjusted to an optical densityat 600 nm of 1. Tenfold serial dilutions were made; 10 µl of eachdilution was spotted onto both the test plate and the controlplate. The plates were incubated at 30°C for 2days.

Two-hybrid assays. Two-hybrid assays were performed using yeast strain L40 (20), which has HIS3 and lacZ reporter genes under the control ofupstream LexA operators. The LexA-SIR4C construct was previouslydescribed (2) and includes the C-terminal region of Sir4p (aa951 to 1358). Control strains expressed LexA from plasmid pBTM116(4). GAD-INC fusions were constructed by inserting an XmaI-PstIfragment from pXW140 into pGAD (24); the GAD-inc construct isidentical, except that it carries the S1094L mutation. The controlexpressed GAD from pGAD. Strains with the relevant plasmids wereinoculated into 2 ml of selective medium and shaken at 30°C for24 h. Tenfold serial dilutions of the cultures were made, and5 µl of each dilution was plated onto synthetic complete medium(SC)-Trp-Leu or SC-Trp-Leu plus 5 mM 3-amino-1,2,4-triazole medium;plates were incubated at 30°C for 3days.

Protein analyses. Immunoblot analyses of Ty5 and GBD proteins were conducted as previously described using antibodies specific to the RGS-H₆tag (Qiagen) or GBD (Santa Cruz Biotechnology) (22). Two ofthe epitope-tagged Ty5 elements were described in that previousreport (pWW32 and pIP19). The element with the TD replaced bythe RGS-H₆ epitope (pWW59) was constructed by PCR mutagenesis(3). The Ty5 fragment within pWW37 (see above) was amplifiedusing the universal primer and the reverse primers DVO1180 (5'-TGA-TGG-TGA-TGC-GAT-CCT-CTC-GAT-GGA-GGA-GAT-TCG-ATT-G) and DVO1181(5'-CGC-ATC-ACC-ATC-ACC-ATC-ACA-ATA-CCT-CAT-TTA-ACG-CGG-C). TheBspEI-PflMI fragment contained within the amplification productwas used to replace the corresponding fragment in the wild-typeTy5 element carried on pSZ152 (54).

To measure in vitro interactions between the TD and Sir4p, we first constructed a plasmid expressing the C terminus of SIR4(aa 950 to 1358) by PCR amplifying pSZ269 (see above) with primersDVO1137 (5'-GAA-GGA-TCC-AGA - GGA - TCG - CAT - CAC - CAT - CAC- CAT - CAC - AGA - AGA - GTG - TCG - CAT-AGT-G) and DVO1085 (5'-TGA-TCT-CGA-GTC-AAT-ACG-GTT-TTA-TCT-CC).The amplification product was digested with BamHI and XhoI andinserted into pCITE-2a(+) (Novagen) to generate pWW56. pWW56 DNA(0.5 µg) was used in a 50-µl coupled transcription-translationreaction mixture (Promega) containing 20 µCi of [³⁵S]methionine. GBD fusion proteins were immunoaffinity purifiedas previously described (41) from 250-ml yeast cultures (opticaldensity at 600 nm, 0.8 to 1.2) with either pXW205, pXW213, orpGBDU. Cells were harvested, washed with ice-cold water, and resuspendedin 1.8 ml of lysis buffer B (50 mM HEPES [pH 7.5], 0.5 M NaCl,10% glycerol, 0.1% IGPEL CA-630 [Sigma], 2 mM dithiothreitol,2.5 mM benzamidine, 0.5 mM phenylmethylsulfonyl fluoride, 2 µgof leupeptin per ml, 2 µg of bestatin per ml, and 2 µg of pepstatinper ml). Cells were disrupted by the glass bead method (3),and the lysate was centrifuged at 12,000 rpm (JA-20 rotor; Beckman)at 4°C for 30 min. Levels of fusion protein in the supernatantwere assessed by immunoblot analysis using anti-GBD antibodies(Santa Cruz Biotechnology). The GBD fusion proteins were immunoaffinitypurified from 300 µl of supernatant using 10 µl of an anti-GBDagarose bead slurry (Santa Cruz Biotechnology). After a 2-h incubation,the beads were collected by centrifugation (500 × g, 2 min), washedtwice with 300 µl of wash buffer (50 mM HEPES [pH 7.5], 150 mMNaCl, 5 mM Mg diacetate, protease inhibitors) and once with 1×PBS (137 mM NaCl, 2.7 mM KCl, 4.3 mM Na₂HPO₄, 1.4 mM KH₂PO₄).The 50-µl in vitro transcription-translation reaction mixturecontaining the labeled Sir4p was then added to the washed anti-GBDagarose beads, and the mixture was incubated at room temperaturefor 30 min. The beads were collected by centrifugation (500 ×g, 2 min) and washed three times with PBS. Ten microliters of2× sodium dodecyl sulfate (SDS) sample buffer (3) was addedto each tube; samples were heated (95°C for 10 min) and separatedby SDS-polyacrylamide gel electrophoresis (PAGE). The gel wasdried and exposed to X-ray filmovernight.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Defining the Ty5 targeting domain. We previously found that a single amino acid substitution at position 1094 in the Ty5 polyprotein (S1094L) dramatically decreasedtargeting to the telomeres and silent mating loci (14). Thisindicated that Ty5 plays an active role in selecting targets andpointed to a possible targeting domain around S1094. To furtherdefine Ty5-encoded targeting determinants, a 758-bp BspEI-PflMIrestriction fragment encompassing S1094 was mutagenized by PCR(Fig. 1A). The PCR products were used to replace the correspondingwild-type fragment, and sequencing of several recombinants revealedthat each carried two to eight base pair changes. Over 2,100 mutagenizedelements were screened for targeting defects using our plasmid-basedtargeting assay, which we have previously shown is an effectivemeasure of chromosomal integration patterns (14). In this assay,targeting is quantified as the percentage of integration eventsthat occur at a plasmid-borne HMR locus. We identified 11 elementsthat were impaired in targeting to various degrees (Table 1).DNA sequencing revealed multiple nucleotide changes in the BspEI-PflMIfragments of these elements. Whereas some mutations were silent,the number of amino acid substitutions ranged from two (mutantsut41 and ut38) to eight (mutant ut46) (Table 1).

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TABLE 1. PCR mutagenesis defines the Ty5 TD

We made three observations regarding the targeting mutants: (i) one mutant (ut5) had an S1094L substitution identical to themutation described in our previous study; (ii) all of the remainingmutants had an amino acid substitution in the vicinity of S1094(encompassing a span of 6 aa residues); and (iii) independentmutations in the same residue near S1094 had similar targetingdefects (e.g., mutants ut23, ut31, and ut33). These observationssuggested that the mutations near S1094 were primarily responsiblefor the loss of target specificity. To test this hypothesis, weconstructed seven new mutants that carried only one amino acidsubstitution near S1094 (Table 1). The S1094L mutation was notincluded because it was previously characterized (14). Targetingassays indicated that in all seven cases, the single mutationsconferred a targeting defect nearly identical to that of the originalmutants. This was the case even for conservative substitutions;for example, the L1092V mutation dramatically decreased targeting.Based on these data, we concluded that Ty5 encodes a TD and thatit may be limited to a short stretch of 6 aa(LDSSPP).

Because our mutagenesis recovered multiple substitutions in the same amino acid, this suggested that the mutagenesis of thePCR fragment was saturated. To confirm the boundaries of the TDand to ensure that all critical amino acid residues near the LDSSPPmotif had been identified, directed PCR mutagenesis was used tochange residues near S1094 to alanine that were not identifiedas important for targeting. This included two residues (Asp1093and Pro1096) that are located between other amino acids criticalfor targeting as well as residues upstream and downstream of theLDSSPP motif (Table 2). These substitutions had at most a modesteffect on targeting (e.g., P1096, pWW41) or no effect at all (e.g.,N1098, pWW42). It is interesting that each of the targeting mutantsidentified in this study had transposition frequencies from two-to sixfold lower than that of the wild type (Table 1). In contrast,the mutants without altered target specificity transposed at nearwild-type levels (data not shown). This observation was also madein our original study, wherein the S1094L mutation caused a fourfolddecrease in transposition (14). This indicates that TD mutationsalso affect transposition efficiency.

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TABLE 2. Site-directed mutagenesis indicates that only 4 of the 6 aa in the Ty5 TD are required for integration specificity

The TD is located in the integrase C terminus. Ty5 encodes a single open reading frame that is processed by a Ty5 gene-encoded protease into several proteins, includingIN (80 kDa) and reverse transcriptase (RT; 59 kDa) (22). Extrapolatingmolecular weights from the Ty5 amino acid sequence, we predictthat the protease cleavage site separating IN from RT is withinthe vicinity of the TD and therefore that the TD may reside eitherwithin the C terminus of IN or within the N terminus of RT. Todistinguish between these possibilities, the TD was replaced withan epitope tag (RGS-H₆). Like the other TD mutants, the epitope-taggedelement transposed at a level more than fivefold lower than thatof the wild type (data not shown). Proteins were prepared fromstrains expressing the TD-tagged element (pWW59) as well as fromcontrol strains expressing elements with the same epitope at eitherthe C terminus of RT (pIP19) or within the middle of the IN codingregion (pWW32) (Fig. 1A). Immunoblot analysis indicated that theelement with the tag located at the TD expressed a protein withthe same mobility on SDS-PAGE gels as that of IN (Fig. 1B). Othertagged proteins revealed by immunoblotting represent various processingproducts or intermediates (22). All lanes contained equivalentamounts of total protein, yet levels of the TD-tagged IN wereseveralfold lower than those of the other tagged IN, suggestingthat mutations in the TD may affect protein stability. Nonetheless,we could conclude from this experiment that the TD resides withinIN, consistent with its role in target siteselection.

Tethering the TD to DNA nucleates silent chromatin. Our model for target specificity predicts that the TD interacts with silent chromatin to tether the integration apparatusto its target sites. If this is the case, then the converse mayalso be true: a TD tethered to DNA may recruit silencing factorsand establish silent chromatin. To test this idea, we used anassay that evaluates a protein's ability to establish transcriptionalsilencing (10). The test protein was first fused to the GBD,and the fusion protein was expressed in a yeast strain with aweakened HMR-E silencer that contains Gal4p binding sites (UASg).The effectiveness of the tethered proteins in nucleating silentchromatin was measured by the transcriptional status of a reportergene at HMR (e.g., TRP1). We constructed four Ty5-GBD fusion proteins(Fig. 1C), one of which has 258 aa of the Ty5 INC (GBD-INC) andanother of which has only 9 Ty5 aa (GBD-TD), 6 of which constitutethe TD. The remaining two fusion constructs differed only by theS1094L mutation (GBD-inc, GBD-td). Immunoblot analysis indicatedthat the wild-type and mutant forms of the fusion proteins wereexpressed equivalently in yeast (Fig. 1D).

The fusion constructs were introduced into yeast strains with two different HMR-E mutations: one lacking binding sites forORC and Rap1p (aeB) and the other lacking binding sites for Rap1pand Abf1p (Aeb) (10). The ability of the fusion proteins toestablish silencing was measured by spotting 10-fold serial dilutionsof the various strains onto media lacking tryptophan. The GBD-INCfusion was found to repress transcription over 100-fold (Fig.2). Surprisingly, even the 9-aa GBD-TD fusion protein silencedTRP1 more than 10-fold. In both cases, the transcriptional silencingrequired the presence of the UASg, and in agreement with previouswork (1, 10), the fusion proteins were more effective atsilencers with a wild-type ORC binding site (Aeb). If the TD interactswith silent chromatin as predicted, then mutations that disrupttargeting should decrease its effectiveness in recruiting silencingfactors. Consistent with this hypothesis, both GBD-inc and GBD-tdwere unable to establish transcriptional silencing (Fig. 2C).All of the above observations were confirmed in a strain witha URA3 reporter gene at HMR, indicating that the silencing wasnot reporter gene dependent (data not shown).

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FIG. 2. The Ty5 TD nucleates silent chromatin. (A) A cartoon depicting the tethered silencing assay. Yeast strains were used with deletions in two of the protein binding sites in HMR-E (A, E, and B) and three copies of UAS_G, binding sites for Gal4p (10). In the example depicted, the E and B binding sites are deleted (e, b), resulting in derepression of transcription at HMR. Expression of a fusion protein between GBD and the Ty5 TD (GBD-TD) was tested for its ability to recruit components of silent chromatin and restore silencing. Silencing is measured by expression of the adjacent TRP1 marker gene. (B) Silencing was established when GBD-INC and GBD-TD were tethered to the weakened HMR locus by the triple UAS_G. Serial, 10-fold dilutions of cells were plated onto control (SC-Ura) or test (SC-Ura-Trp) medium to measure silencing of the TRP1 reporter gene at HMR. (C) A point mutation that abolishes targeting fails to restore silencing for both fusion proteins (GBD-inc and GBD-td) in both test strains.

Silent chromatin, by definition, requires the actions of Sir2p, Sir3p, and Sir4p. To determine whether the TD fusions establishsilent chromatin or rather act in some other way to occlude thetranscriptional machinery from the TRP1 promoter, the TD fusionswere introduced into various sir $Delta$ strains (10) (Fig. 3). Sir1pwas not required for TD-mediated silencing, consistent with itsprimary role in recruiting components of silent chromatin to theHM loci (48). However, the structural components of silent chromatin,Sir2p, Sir3p, and Sir4p, were all required, indicating that theTy5 TD represses the reporter gene at HMR by establishing silentchromatin.

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FIG. 3. Silencing conferred by the TD is Sir dependent. The assay system is described in the legend to Fig. 2. In strains with deletions of SIR2, SIR3, or SIR4, GBD-TD fails to establish silencing at a weakened HMR locus. Silencing, however, does not require the SIR1 gene. The Ade phenotype of the sir2 $Delta$ , sir3 $Delta$ , and sir4 $Delta$ strains confers their dark color; the sir1 $Delta$ stain is Ade⁺.

Overexpression of the TD disrupts telomeric silencing. Transcriptional silencing is very sensitive to the expression level of some components of silent chromatin. Overexpressionof Sir4p, for example, disrupts telomeric silencing, presumablyby titrating away other components of silent chromatin or by disruptingcomplex formation (23, 39) (Fig. 4B). We tested whether overexpressionof GBD-TD could disrupt telomeric silencing by monitoring theexpression of telomeric (and therefore normally silenced) URA3and ADE2 genes (16). Overexpression of GBD-TD (Fig. 1D) resultedin the loss of telomeric silencing, as evidenced by the abilityof cells to grow on media lacking uracil (Fig. 4A). ADE2 expressionwas also evident by the white colony phenotype rather than thepinkish color characteristic of ADE2 repression and adenine precursoraccumulation. As observed in the tethering experiments, expressionof the fusion with the S1094L mutation did not affect telomericsilencing.

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FIG. 4. Overexpression of the Ty5 TD disrupts telomeric silencing and loss of silencing is complemented by overexpression of Sir3p. Two reporter genes, URA3 and ADE2, are located at telomeres VIIL and VR, respectively (16). URA3 expression was measured by growth of the yeast cells on selective media. ADE2 expression is indicated by colony color; when ADE2 is repressed, the colonies are red or pink. (A) Overexpression of GBD-TD disrupts telomeric silencing (i.e., causes URA3 expression), in contrast to what occurs in its mutant form (GBD-td) and with GBD alone. (B) Overexpression of Sir2p and Sir3p strengthen silencing, and Sir4p breaks silencing, as previously reported (23, 39). This is demonstrated in the GBD control strains and GBD-td strains. When the TD and SIR genes are overexpressed in the same strains, Sir3p, but not Sir2p or Sir4p, restores silencing.

To test whether GBD-TD disrupts telomeric silencing by titrating away components of silent chromatin, the SIR genes were ectopicallyexpressed by introducing them on high-copy-number 2µm plasmids(Fig. 4B). Overexpression of Sir4p by this means has previouslybeen shown to disrupt telomeric silencing (39), and we madethe same observation regardless of whether GBD-TD was coexpressed.Overexpression of Sir2p did not restore telomeric silencing toGBD-TD-expressing strains; however, it did increase telomericsilencing in GBD or GBD-td strains. In contrast, overexpressionof Sir3p overcame the GBD-TD-dependent loss of telomeric silencing.This suggests that Sir3p is titrated away (either directly orindirectly) by interacting with the TD. Alternatively, excessSir3p could dominantly restore silencing by bypassing a factorbeing titrated away by TD. In addition, a growth defect was observedon nonselective media when Sir3p and GBD-TD were both overexpressed(Fig. 4B).

Sir4p interacts with Ty5 IN. Several lines of evidence suggest that Sir3p and Sir4p are likely candidates for interacting with the Ty5 IN to mediate targetspecificity: (i) targeting is largely abolished in sir3 $Delta$ and sir4 $Delta$ strains (53); (ii) in sir4-42 strains, Ty5 integration specificitychanges with the chromosomal localization of Sir3p and Sir4p;and (iii) as described above, loss of telomeric silencing dueto overexpression of the TD can be complemented by overexpressionof Sir3p. To test whether Ty5 IN interacts with Sir3p or Sir4p,two-hybrid assays were conducted. An interaction was detectedbetween the C terminus of Sir4p (SIR4C, aa 951 to 1358 expressedas a LexA fusion protein) and the Ty5 INC (expressed as a GADfusion protein). This interaction strongly activated the HIS3reporter gene and enabled growth of yeast cells on selective media(Fig. 5A). Consistent with the role of the TD in silencing, thisinteraction required a wild-type TD: the S1094L mutation greatlyweakened the two-hybrid interaction. These data indicate thatINC binds to Sir4p (either directly or indirectly) and that theTD is required for this interaction.

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FIG. 5. The Ty5 INC interacts with the C terminus of Sir4p. (A) Yeast two-hybrid assays reveal an interaction between GAD-INC and LexA-SIR4C. Liquid cultures expressing the various LexA and GAD proteins were serially diluted 10-fold and spotted onto plates. A positive two-hybrid interaction was measured by transcriptional activation of the HIS3 reporter, which allowed for growth on selective media (SC-Trp-Leu-His with 5 mM 3-amino-1,2,4-triazole [3AT]). Activation of the HIS3 marker requires both SIR4C and the wild-type TD. (B) SIR4C interacts with GBD-TD in vitro. SIR4C was expressed and labeled with [³⁵S]methionine by coupled transcription and translation. GBD-TD and GBD-td were expressed in yeast and immunoaffinity purified with anti-GBD agarose beads. The top lanes indicate the amount of labeled SIR4C bound by the various GBD proteins. The bottom lanes are from an immunoblot performed with anti-GBD antibodies, and they indicate the levels of GBD proteins in the extract used for immunoaffinity purification.

To confirm the two-hybrid data, we tested whether the Sir4p C terminus and the Ty5 TD could interact in vitro. GBD, GBD-TD,and GBD-td were expressed in yeast and immunoaffinity purifiedusing anti-GBD agarose beads. Beads with the bound GBD proteinswere incubated with SIR4C that had been labeled with [³⁵S]methionine. The beads were washed, and the proteins were elutedand separated by SDS-PAGE. Sir4p bound to GBD-TD. Lower, backgroundlevels of binding were observed for GBD and GBD-td (Fig. 5B).These in vitro data support the results obtained in the two-hybridassays and collectively suggest that the biological activity ofthe TD is mediated by interactions withSir4p.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In a simple model to explain LTR retroelement target specificity, the interaction between the preintegration complex and DNA-boundproteins tethers the integration machinery to target sites andresults in integration site biases (7). Support for this modelcomes from the study of the yeast Ty retrotransposons. These elementshave different target preferences: Ty1 and Ty3 prefer sites ofRNAP III transcription (9, 13), and Ty5 prefers silent chromatin(56). In both cases, DNA-bound protein complexes are requiredfor targeting. Human immunodeficiency virus (HIV) IN interactswith a human homolog of the transcription factor SNF5 in two-hybridassays (25); however, there is no evidence that this interactionmediates target site choice. In this study, we define a Ty5-encodedTD (LXSSXP) and show that it interacts with Sir4p, a componentof silent chromatin. To our knowledge, this interaction betweena retroelement-encoded protein and a chromatin factor providesthe first direct evidence for the targetingmodel.

Integrase C terminus and the TD. Retrotransposon and retroviral INs consist of three distinct domains (26): (i) an N-terminal region with a zinc-bindingmotif that is required for IN activity and likely binds cDNA,(ii) a catalytic domain that executes the integration reaction,and (iii) a C-terminal region which, for the retroviruses andsome retrotransposons, is required for cDNA 3'-end processing.The retrotransposon integrase C termini are considerably largerthan their retroviral counterparts; the Ty1 and Ty5 C terminiconstitute more than half of IN (e.g., HIV IN is 288 aa; Ty1 INis 635 aa). Little is known about the function of the retrotransposonC-terminal extensions, with the exception that the very C terminusof Ty1 IN encodes a nuclear localization signal that is requiredfor the preintegration complex to gain nuclear access (28, 42).For Ty1 and Ty5, the coding region of IN lies upstream of RT,and both are released from the polyprotein by proteolytic cleavage.In our earlier study of a Ty5 targeting mutant, we could not determinewhether the targeting mutation was located in the C terminus ofIN or the N terminus of RT (14). By replacing the TD with anepitope tag and comparing its electrophoretic mobility to thoseof other tagged forms of RT and IN, we demonstrate here that theTD resides within IN. This indicates that IN is responsible fortarget specificity and demonstrates a new function for the INC.For some members of the more distantly related Ty3/gypsy groupretrotransposons (Metaviridae), the INC encodes a chromodomain,a motif implicated in targeting proteins to chromatin (37).The INC, therefore, may generally be used by retroelements forintegration siteselection.

Despite the large size of the INC, the Ty5 TD identified through our mutant screen spans only 6 aa residues. This short domainis biologically active: when as few as 9 aa encompassing the TDare expressed as part of a fusion protein (e.g., GBD-TD), theynucleate silent chromatin or disrupt telomeric silencing. Fusionproteins expressing larger fragments of the INC are at least 10-foldmore effective in nucleating silent chromatin. This suggests thatother regions of the INC play a role in targeting. These regionsmay not have been identified by our mutant screen if they arerequired for transposition. Transposition defects were observedduring characterization of several targeting mutants. For example,the transposition efficiency of mutant ut15 was more than 30-foldlower than that of the wild type. This mutant had three missensemutations in the INC in addition to the mutation in the TD (Table1). When the ut15 TD was evaluated in isolation (see rut15, Table1), the level of transposition was only fivefold lower than thatof the wild type. Additionally, we observed that most of the mutagenizedelements (~60%) were unable to transpose or showed greatly reducedlevels of transposition (unpublished data). Some of these likelycarry stop codons or frameshift mutations that prevent synthesisof the downstream RT; however, the frequency of nontransposingelements was too high based on the extent of mutagenesis (~0.5%).This implies that regions of the C terminus outside of the TDare important fortransposition.

In addition to loss of target specificity, a second phenotype shared by all of the TD mutants is an overall decrease in transposition(two- to sixfold). For wild-type Ty5, more than 94% of Ty5 integrationevents occur within regions of silent chromatin whereas the remainderappear to be randomly distributed throughout the genome (55,57). If the TD is not required for integration, then TD mutationsshould not alter transposition frequencies. If the TD is requiredonly for targeted integration, then the transposition frequencieswould be predicted to drop ~15-fold (94% divided by 6%). The intermediateeffect of TD mutations on transposition suggests that the TD playsa role beyond tethering the integration apparatus to its preferredtarget sites. Possibilities include facilitating the integrationreaction, facilitating reverse transcription (which is supportedby recent data indicating that the INC is required to producefunctional Ty1 RT in vitro [49]), or facilitating nuclear localization(the Ty1 nuclear localization signal is located in approximatelythe same region of the protein as the Ty5 TD [28, 42]). Instrains expressing a modified Ty5 in which the TD was replacedby an epitope tag, we observed significantly lower levels of INprotein (Fig. 1). It is also possible that a wild-type TD is requiredfor proteinstability.

The TD and silent chromatin. A large number of proteins are involved in the assembly and maintenance of silent chromatin (reviewed in references 35 and36). These include proteins such as Sir3p and Sir4p that carryout structural or scaffolding roles and proteins like Sir1p andRap1p that recruit and nucleate the structural proteins at thesilencers. Tethering either class of these proteins to weakenedHMR-E silencers effectively establishes silencing (10, 38).Likewise, the INC is very effective in nucleating silencing andcauses a 100- to 1,000-fold decrease in the expression of reportergenes at HMR. The TD does not simply recruit a protein complexthat occludes the RNAP II machinery from the reporter gene. Rather,it establishes silent chromatin as defined by the requirementfor Sir2p, Sir3p, and Sir4p. TD-mediated silencing does not needSir1p, which primarily acts at HM loci and is not required forsilencing at the telomeres or rDNA. At the HM loci, Sir1p interactswith the ORC (48), and it is interesting that the TD is moreeffective when the ORC binding site is intact. This has also beenobserved with other nucleators of silent chromatin (1, 10).Although a number of S. cerevisiae proteins have motifs that matchthe TD consensus (LXSSXP), none are known components of silentchromatin.

We have previously shown that, in contrast to what occurs in sir3 $Delta$ and sir4 $Delta$ strains, targeting of Ty5 to the telomeres andHM loci is only partially impaired in sir2 $Delta$ strains and occursat levels approximately 50% of those of the wild type (53).Furthermore, the loss of telomeric silencing caused by overexpressingthe TD cannot be restored by overexpressing Sir2p. In light ofrecent findings that Sir2p is a histone deacetylase (21, 33,47), this suggests that the Ty5 integration apparatus does notsense Sir2p-mediated acetylation patterns. The targeting defectin sir2 $Delta$ strains is likely a secondary consequence of perturbationsin silent chromatin. In contrast, the loss of telomeric silencingcaused by overexpressing the TD can be restored by additionalSIR3 expression. The Sir4p C terminus interacts directly withSir3p, and it may be that overexpression of the TD disrupts thisinteraction, which, in turn, is stabilized by additional Sir3p.In that regard, it has been observed that loss of telomeric silencingcaused by overexpression of the Sir4p C terminus can be complementedby overexpressing Sir3p (15). Finally, it is important to notethat the combined expression of Sir3p and a wild-type TD causesa growth defect, indicating that, although the TD may not interactdirectly with Sir3p, Sir3p does modulate the biological activityof theTD.

The TD and Sir4p. Prior to the carrying out of our two-hybrid assays, no evidence distinguished the roles of Sir3p and Sir4p in Ty5 target specificity.The only notable difference was that Ty5 cDNA recombination increasedmore than 10-fold in sir4 $Delta$ strains and was only marginally affectedin sir3 $Delta$ strains (53). In strains with the sir4-42 allele, whichexpresses a C-terminally truncated form of Sir4p (aa 1 to 1237),Ty5 integrates preferentially into the rDNA (53). Here we demonstratethat the Ty5 TD interacts with the Sir4p C terminus (aa 951 to1358), suggesting that the relevant region of interaction is locatedbetween aa 951 and 1237. The Sir4p C terminus interacts with manyproteins, including Sir2p and Sir3p (41), Rap1p (6, 43),Sif2p (12), and Dis1p (52). Two-hybrid interactions may resultif one or more of these proteins serve as a bridge between theTD and Sir4p. However, we have not observed two-hybrid interactionsbetween IN and other components of silent chromatin (data notshown). Furthermore, the observed in vitro binding between Sir4pand the TD argues that these molecules interact directly. Nonetheless,because we used fusion proteins purified from yeast cells forthese experiments, we cannot exclude the possibility that otherfactors copurified or modified the TD to yield productiveinteractions.

Concluding remarks. Previous studies demonstrated that DNA bound in silent chromatin is inaccessible to proteins like HO endonuclease, restrictionenzymes, and transcription factors (34). However, the abilityof Ty5 to integrate into silent chromatin suggests that this DNAis accessible to Ty5 IN. Our model suggesting that target specificityresults from simply tethering the preintegration complex to chromatinmay therefore require additional refinements. For example, theintegration complex may induce changes in silent chromatin duringintegration, and the role of the TD in such processes is an importantarea of futureresearch.

An increased understanding of targeting mechanisms may make it possible to manipulate retroelement target site choice. Itmay be possible to change the integration preference of retrotransposonsby replacing TDs with peptide motifs that interact with specificchromosomal proteins. Such engineered retrotransposons may becomeuseful tools for studying chromatin organization and may providenovel methods for genome manipulation. Retroviral vectors arewidely used for DNA delivery in human gene therapy; however, uncontrolled,random integration into the host genome is one of their majordrawbacks. It may now be possible to better control retroviralintegration site choice to improve the efficacies of these vectorsin genedelivery.

	ACKNOWLEDGMENTS

W. Xie and X. Gai contributed equally to thiswork.

We thank Phil Irwin for his expert technical assistance. J. Rine and D. Gottschling graciously provided plasmids used in thisstudy.

This work was supported by a grant from the American Cancer Society (RPG9510106MBC) to D.F.V. and by Hatch Act and State ofIowafunds.

	FOOTNOTES

^* Corresponding author. Mailing address: 2208 Molecular Biology Bldg., Iowa State University, Ames, IA 50011. Phone: (515) 294-1963.Fax: (515) 294-7155. E-mail: voytas{at}iastate.edu.

This is Journal Paper J-19154 of the Iowa Agriculture and Home Economics Experiment Station, Ames, project3383.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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