Ubp10/Dot4p Regulates the Persistence of Ubiquitinated Histone H2B: Distinct Roles in Telomeric Silencing and General Chromatin

doi:10.1128/MCB.25.14.6123-6139.2005

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Molecular and Cellular Biology, July 2005, p. 6123-6139, Vol. 25, No. 14
0270-7306/05/$08.00+0 doi:10.1128/MCB.25.14.6123-6139.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

Ubp10/Dot4p Regulates the Persistence of Ubiquitinated Histone H2B: Distinct Roles in Telomeric Silencing and General Chromatin

Richard G. Gardner, Zara W. Nelson, and Daniel E. Gottschling^*

Fred Hutchinson Cancer Research Center, Seattle, Washington 98109

Received 16 February 2005/ Returned for modification 23 March 2005/ Accepted 8 April 2005

ABSTRACT

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

We previously discovered that the ubiquitin protease Ubp10/Dot4pis important for telomeric silencing through its interactionwith Sir4p. However, the mechanism of Ubp10p action was unknown.We now provide evidence that Ubp10p removes ubiquitin from histoneH2B; cells with UBP10 deleted have increased steady-state levelsof H2B ubiquitination. As a consequence, ubp10 ${Delta}$ cells also haveincreased steady-state levels of histone H3 Lys4 and Lys79 methylation.Consistent with its role in silencing, Ubp10p is preferentiallylocalized to silent chromatin where its ubiquitin protease activitymaintains low levels of H3 Lys4 and Lys79 methylation to allowoptimal Sir protein binding to telomeres and global telomericsilencing. The ubiquitin protease Ubp8p has also been shownto remove ubiquitin from H2B, and ubp8 ${Delta}$ cells have increasedsteady-state levels of H2B ubiquitination similar to those inubp10 ${Delta}$ cells. Unlike ubp10 ${Delta}$ cells, however, ubp8 ${Delta}$ cells do nothave increased steady-state levels of H3 Lys4 and Lys79 methylation,nor is telomeric silencing affected. Despite their separatefunctions in silencing and SAGA-mediated transcription, respectively,deletion of both UBP10 and UBP8 results in a synergistic increasein the steady-state levels of H2B ubiquitination and in thenumber of genes with altered expression, indicating that Ubp10pand Ubp8p likely overlap in some of their target chromatin regions.We propose that Ubp10p and Ubp8p are the only ubiquitin proteasesthat normally remove monoubiquitin from histone H2B and, whilethere are regions of the genome to which each is specificallytargeted, both combine to regulate the global balance of H2Bubiquitination.

INTRODUCTION

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Posttranslational modifications of nucleosomal histones playpivotal regulatory roles in all aspects of eukaryotic chromosomedynamics: replication, recombination, repair, segregation, andgene expression. These modifications include acetylation, methylation,phosphorylation, ubiquitination, sumoylation, and ADP-ribosylation(71). Many of these modifications often occur together withinthe same histone or nucleosome or within neighboring nucleosomes,creating distinct chromatin domains (71). Particular combinationsof residue-specific modifications typically correlate with specificfunctional consequences for the modified chromatin domains (71).

In Saccharomyces cerevisiae, chromatin-mediated silencing attelomeres and the HM loci is particularly sensitive to histoneacetylation and methylation, which appear to disrupt the abilityof the silencing proteins Sir3p and Sir4p to bind to, or assemblealong, the nucleosome fiber. For example, tethering of histoneacetylases to silent domains increases histone acetylation withinthese domains and blocks the propagation of silencing (16).Similarly, overexpression of a histone methylase greatly increasesglobal histone methylation and disrupts silencing (85, 92).In vitro, fragments of Sir3p bind unacetylated and unmethylatedhistone peptides better than those that are acetylated or methylated(13, 81), demonstrating the preference of Sir3p for unmodifiedhistones. Because of this preference, histone acetylation andmethylation appear to be excluded from silent chromatin (5-7,63, 79, 88, 90).

In genetic screens looking for factors that compromise telomericsilencing, we previously identified a number of genes that encodeprotein modification enzymes, such as DOT1, DOT4, and RAD6 (37,85). Dot1p is a histone methyltransferase that methylates Lys79of histone H3 in the context of the nucleosome (24, 49, 65,92). H3 Lys79 methylation is primarily associated with activechromatin—approximately 90% of histone H3 in yeast ismethylated at this site (92)—and the modification is absentfrom silent chromatin loci (63). Loss of DOT1 completely abrogatesLys79 methylation, which results in a reduction of Sir proteinbinding to the telomeres and a concomitant loss of telomericsilencing (92). However, loss of DOT1 also results in increasedSir protein binding to subtelomeric regions (92). We have hypothesizedthat this reflects a promiscuous binding of Sir3p to nucleosomesoutside of silent regions due to the absence of H3 Lys79 methylation(92). Because Sir3p is limiting in the cell (11, 87, 89), suchpromiscuous binding reduces the effective amount of Sir3p availablefor the normally silenced loci (93).

Methylation also occurs on Lys4 of histone H3 by action of theSet1 protein (8, 45, 62, 69, 77). Lys4 methylation is similarto Lys79 methylation: it is normally associated with activechromatin (5, 82), and Sir protein binding is reduced in silentregions when Lys4 methylation is abolished (81). Simultaneousloss of H3 Lys79 and Lys4 methylation by deletion of DOT1 andSET1 synergistically reduces Sir protein binding to the telomeres(64), indicating that these two modifications function togetherto prevent the promiscuous binding of Sir proteins to activechromatin.

The ubiquitin-conjugating enzyme Rad6p is also required fortelomeric silencing (37). Rad6p functions with Bre1p, its cognateubiquitin-protein ligase (39, 95), to attach ubiquitin to Lys123of histone H2B (76). Over 25 years ago it was found that ubiquitinatedH2B and H2A are associated with transcriptionally active chromatinin higher eukaryotes (54, 68). Consistent with this, componentsof the Paf1 transcriptional elongation complex are requiredfor H2B ubiquitination in S. cerevisiae (46, 64, 96). Althoughits precise role in transcription is unclear, H2B ubiquitinationis required in vivo for H3 Lys4 and Lys79 methylation (9, 20,67, 91). It is proposed that the ubiquitin moiety on H2B mayrecruit proteasomal ATPases to prepare the chromatin for Set1pand Dot1p activity (22). Because loss of H3 Lys4 and Lys79 methylationdisrupts silencing (81, 92), the requirement of Rad6p functionfor telomeric silencing is likely to be indirect and due toits role in ubiquitinating H2B as a precursor to establishingboth H3 Lys4 and Lys79 methylation in active chromatin.

Taking all of this together, it is clear that silencing requiresboth the addition of histone acetylation and methylation inactive chromatin and the removal or prevention of these histonemodifications in silent regions. Removal of histone acetylationin silent regions is carried out by the silencing protein andhistone deacetylase Sir2p (40, 50, 86). Although a demethylasethat targets H3 Lys4 mono- and dimethylation has been identifiedin mammals (83), no homologous lysine demethylases are knownin S. cerevisiae. Thus, it is not known if H3 Lys4 and Lys79methylation can be directly removed from silent regions if established.Instead, removal of ubiquitin from H2B by ubiquitin proteasesprior to the establishment of H3 Lys4 and Lys79 methylationmay be one mechanism for limiting these H3 modifications insilent regions. Of the 17 known and putative ubiquitin proteasesin S. cerevisiae (2), Ubp8p has been shown to regulate the levelsof ubiquitinated H2B as part of the transcriptional activatorcomplex SAGA (18, 33, 80), indicating that removal of ubiquitinfrom H2B does occur. However, Ubp8p is not known to functionin silencing.

We previously discovered that the ubiquitin protease Dot4p (nowknown as Ubp10p) is important for silencing in vivo (43). Theabsence of Dot4p ubiquitin protease activity, either by deletionof DOT4 or mutation of the catalytic residue, results in reducedsilencing, especially at telomeres (43, 85). By two-hybrid analysis,we found that Dot4p interacts with the silencing protein Sir4p(43), and we proposed that Dot4p acts at, or is part of, silentchromatin. However, we had not identified any in vivo substratesof Dot4p. Given the association of Dot4p with silent chromatinand the role of H2B ubiquitination in H3 Lys4 and Lys79 methylation,we investigated whether Dot4p's ubiquitin protease activityregulates the levels of H2B ubiquitination to limit H3 Lys4and Lys79 methylation in silent regions, as has been previouslyproposed (78).

MATERIALS AND METHODS

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Reagents. General chemical and enzymatic reagents were obtained from NewEngland Biolabs (Beverley, MA), Sigma (St. Louis, MO), Fisher(Pittsburgh, PA) and Pierce (Rockford, IL). Nitrocellulose (Protran;pore size of 0.2 µM) was obtained from Schleicher andSchuell (Keene, NH). The anti-Myc and anti-FLAG antibodies wereobtained from Sigma and used at 1:10,000 dilutions for Westernblotting or 1:500 dilutions for chromatin immunoprecipitations(ChIP). Anti-monomethyl, -dimethyl, and -trimethyl Lys4 histoneH3 antibodies were obtained from Upstate (Waltham, MA) and usedat 1:5,000 dilutions for Western blotting and 1:500 dilutionsfor ChIP. Anti-dimethyl Lys79 histone H3 antibody was made aspreviously described (92) and used at 1:2,000 dilutions forWestern blotting and at 1:100 dilutions for ChIP. Purified anti-Sir2ppolyclonal antibodies against the N-terminal 19 residues ofSir2p were obtained from Santa Cruz Biotechnology (Santa Cruz,CA), and used at a 1:500 dilution for ChIP. Mouse anti-Sir3pmonoclonal antibodies were made as previously described (92),and used at 1:3 dilutions for ChIP. Vistra Green, ECL chemiluminescenceimmunodetection reagents, sheep anti-mouse horseradish peroxidase-conjugatedantiserum, and donkey anti-rabbit horseradish peroxidase-conjugatedantiserum were obtained from Amersham Biosciences (Piscataway,NJ); the antisera were used at 1:2,000 dilutions. IRDye800-conjugatedgoat anti-mouse and anti-rabbit antibodies were obtained fromRockland Immunochemicals (Gilbertsville, PA). Protein G Dynabeadswere obtained from Dynal (Brown Deer, WI).

Recombinant DNA, molecular cloning, and yeast strains. Standard molecular biology techniques were used. Plasmids andyeast strains used in this study are described in Table 1. Yeastdeletion alleles were made by PCR amplification of the appropriateknockout construct, followed by transformation into yeast cellsusing standard yeast transformation techniques (http://www.fhcrc.org/labs/gottschling).

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TABLE 1. Plasmids, yeast strains, and oligonucleotides used in this study

ChIP assays. ChIP assays were performed similar to those previously described(92), with some changes. Yeast extract-peptone-dextrose (YEPD;200 ml) cultures were grown to a cell density of 2 x 10⁷ cells/mland subjected to cross-linking with 1% formaldehyde. Cell lysateswere prepared, and lysates were sonicated eight times for 30s using a Fisher Scientific sonic dismembrator model 60. Sonicationresulted in an average fragment size of 500 to 800 bp (datanot shown). Clarified lysates were stored at –80°Cuntil required.

For the Ubp10p-Myc ChIPs, cross-linking was performed differently.Cells were first harvested by centrifugation, washed twice inphosphate-buffered saline, and resuspended in 50 ml of phosphate-bufferedsaline. Dimethyl adipimidate was added to a final concentrationof 10 mM to improve cross-linking (48), and the cells were incubatedat room temperature for 45 min. Formaldehyde was added to afinal concentration of 1%, and the cultures were incubated atroom temperature for an additional 15 min. Samples were preparedas described above.

Initial multiplex PCR amplifications were performed on variousconcentrations of immunoprecipitates and total lysates to determinethe concentration required for amplification in the linear range.Final multiplex PCR amplifications were performed using a singleconcentration previously determined to be in the linear amplificationrange. PCR products were resolved on 2% agarose (1x Tris-acetate-EDTA)gels. Gels were stained with Vistra Green and analyzed usinga PhosphorImager (Molecular Dynamics) and ImageJ software. Oligonucleotidesequences for PCR amplifications are listed in Table 1.

Western analyses. Whole-cell lysates were prepared as previously described (26),with some changes. Cultures were grown in YEPD or yeast complete(YC) medium at 30°C to the desired optical density (2 x10⁷ cells/ml for logarithmically growing cells, overnight saturationfor diauxic cells, and 7-day saturation for stationary cells),and equal numbers of cells (1.6 x 10⁸) were harvested by centrifugation.Cells were lysed in 300 µl of SUME (8 M urea, 1% sodiumdodecyl sulfate, 10 mM morpholinepropanesulfonic acid, pH 6.8,10 mM EDTA) containing 0.01% bromophenol blue and 10 mM phenylmethylsulfonylfluoride by mechanical shearing using acid-washed glass beads.For immunoblotting, 5- to 20-µl samples of the cellularlysates were resolved on 16% sodium dodecyl sulfate-polyacrylamidegel electrophoresis gels, and the proteins were transferredto nitrocellulose and immunoblotted with the appropriate antibody.

Transcript DNA microarrays. Transcript DNA microarrays similar to those previously described(23) were performed in triplicate. Dye-reversal experimentswere performed to identify sequence-specific dye biases. Statisticalanalysis of microarray data was performed as previously described(17), using a Bayesian t statistic derived for microarray analyses(3) and a false discovery rate methodology (4) to account formultiple testing. The entire normalized data set is in TableS1 in the supplemental material; the National Center for BiotechnologyInformation Gene Expression Omnibus accession numbers for theseries of individual data sets are GSE2329 (ubp10 ${Delta}$ and ubp8 ${Delta}$ series)and GSE2330 (ubp10^C371S and ubp10^94-250 series).

RESULTS

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

In our earlier work, we found that loss of DOT4 results in reducedsteady-state levels of HA epitope-tagged Sir4p, and we speculatedthat Dot4p might control Sir4p stability, perhaps by regulatingits ubiquitin-dependent degradation (43). However, in subsequenttesting we found that the HA epitope tag (or the T7- or Myc-epitopetag) added to the N terminus of Sir4p results in aberrant degradationof Sir4p (data not shown). Using new antibodies, we found thatuntagged Sir4p is normally stable and not subject to ubiquitination(27). We also found that the steady-state levels of untaggedwild-type Sir4p are unchanged in dot4 ${Delta}$ cells (data not shown).Thus, the alteration of Sir4p stability by loss of DOT4 is anartifact of epitope tagging the protein and not a normal modeof regulation. As a result, we turned our attention to otherpotential substrates of Dot4p.

(Concurrent with our initial discovery (85), DOT4 was also foundby homology searches for ubiquitin proteases and named UBP10(36). Because UBP10 is now the standard name for the gene inthe Saccharomyces Genome Database (http://db.yeastgenome.org/cgi-bin/locus.pl?locus= ubp10), we will henceforth use UBP10 rather than DOT4. Bydoing so, we have renamed the previously constructed dot4 alleles,dot4-1 and dot4-5 (43), with the more descriptive ubp10 nomenclature,ubp10^C371S and ubp10^94-250, respectively.)

Ubp10/Dot4p negatively regulates histone H2B ubiquitination in vivo. With Sir4p eliminated as a substrate of Ubp10p, we turned ourattention to histone H2B due to the fact that H2B ubiquitinationis required for histone H3 Lys4 and Lys79 methylation (9, 20,67, 91), both of which antagonize Sir protein binding to chromatin(64, 81, 92). To determine if Ubp10p targets ubiquitinated H2B,we examined the steady-state levels of H2B ubiquitination inubp10 ${Delta}$ cells. Compared to wild-type cells, ubp10 ${Delta}$ cells have approximatelythreefold higher steady-state levels of H2B ubiquitination (Fig.1), supporting the idea that ubiquitinated H2B is a bona fidesubstrate of Ubp10p. In fact, the increased steady-state levelsof H2B ubiquitination in ubp10 ${Delta}$ cells are similar to the approximatelyfivefold higher levels observed in ubp8 ${Delta}$ cells (Fig. 1); Ubp8pis a ubiquitin protease recently shown to regulate H2B ubiquitination(18, 33). Deletion of both UBP10 and UBP8 results in a furtherincrease in the steady-state levels of H2B ubiquitination thatis greater than that seen in either ubp10 ${Delta}$ or ubp8 ${Delta}$ cells (Fig.1). These results indicate that Ubp10p and Ubp8p act upon separatepopulations of ubiquitinated H2B in part, which is consistentwith their distinct roles in silencing and SAGA-mediated transcription,respectively (33, 43).

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FIG. 1. Ubp10p negatively regulates histone H2B ubiquitination and H3 Lys4 and Lys79 methylation levels. Global steady-state H2B ubiquitination levels from whole-cell lysates were assayed using anti-FLAG antibodies that recognize the FLAG epitope placed on the N terminus of H2B (76). Global steady-state H3 Lys4 and Lys79 methylation levels were also assayed using antibodies specific for mono-, di-, and trimethylated Lys4 forms of H3 as well as an antibody generated against the dimethylated Lys79 form of H3 (92). Whole-cell lysates were derived from strains UCC6369 (wild type), UCC6390 (ubp10 ${Delta}$ ), UCC6392 (ubp8 ${Delta}$ ), UCC6393 (ubp10 ${Delta}$ ubp8 ${Delta}$ ), and UCC6163 (rad6 ${Delta}$ ) that were harvested during log-phase growth. rad6 ${Delta}$ cells served as a negative control for H2B lacking ubiquitin. Changes in levels (n-fold) of H2B ubiquitination and H3 Lys4 and Lys79 methylation for each mutant strain relative to the wild-type strain are shown below each corresponding lane and are the average of three independent experiments. Quantitation was performed using National Institutes of Health ImageJ software.

Ubp10/Dot4p negatively regulates global histone H3 Lys4 and Lys79 methylation. The previously documented dependence of histone H3 Lys4 andLys79 methylation on H2B ubiquitination led us to examine ifloss of UBP10 or UBP8 altered H3 methylation. Using specificantibodies, we examined steady-state levels of H3 Lys4 mono-,di- or trimethylation or H3 Lys79 dimethylation. Although thechanges were often modest, ubp10 ${Delta}$ cells did have reproduciblyhigher steady-state levels of all forms of H3 Lys4 methylationand of H3 Lys79 methylation compared to wild-type cells (Fig.1, and see Fig. 6 and 7). In contrast, we observed no detectableincrease in H3 Lys4 or Lys79 methylation in ubp8 ${Delta}$ cells (Fig.1), indicating that increased H2B ubiquitination alone is notsufficient for increased H3 methylation. In ubp10 ${Delta}$ ubp8 ${Delta}$ cells,H3 Lys4 and Lys79 methylation are also increased similar toubp10 ${Delta}$ cells (Fig. 1B). Altogether, the higher steady-state levelsof H2B ubiquitination in ubp10 ${Delta}$ cells likely present an increasedopportunity for H3 Lys4 and Lys79 methylation.

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FIG. 6. Loss of silencing does not affect global H2B ubiquitination levels. (A) Loss of Ubp10p catalytic activity but not loss of Sir4p binding affects H2B ubiquitination and H3 Lys4 methylation. Global steady-state H2B ubiquitination and H3 Lys4 dimethylation levels from whole-cell lysates derived from strains UCC6195 (wild-type UBP10), UCC6199 (ubp10 ${Delta}$ ), UCC6184 (ubp10^C371S-6Myc), UCC6185 (ubp10^94-250-6Myc), and UCC6186 (UBP10-6Myc) were assayed using anti-FLAG antibodies (FLAG-tagged H2B) or antibodies that specifically recognized H3 Lys4 dimethylation. (B) Loss of silencing does not affect H2B ubiquitination or H3 Lys4 methylation. Global steady-state H2B ubiquitination and H3 Lys4 dimethylation levels were assayed as described in panel A using strains UCC6195 (UBP10), UCC6196 (sir2 ${Delta}$ ), UCC6197 (sir3 ${Delta}$ ), UCC6198 (sir4 ${Delta}$ ), and UCC6199 (ubp10 ${Delta}$ ).

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FIG. 7. Ubp10p and Ubp8p overlap in their target chromatin regions. (A) Global steady-state levels of H2B ubiquitination and H3 Lys4 and Lys79 methylation from whole-cell lysates were assayed as described in the legend of Fig. 1. Whole-cell lysates were derived from strains UCC6369 (wild type), UCC6390 (ubp10 ${Delta}$ ), UCC6392 (ubp8 ${Delta}$ ), UCC6393 (ubp10 ${Delta}$ ubp8 ${Delta}$ ), and UCC6163 (rad6 ${Delta}$ ) that were harvested during log-phase growth, diauxie (overnight growth to saturation), and stationary phase (7-day saturation). (B) Some H2B ubiquitination persists in ubp10 ${Delta}$ and ubp8 ${Delta}$ cells in diauxie. H2B ubiquitination was assayed as described in the legend of Fig. 1. Arrow indicates where diubiquitinated form of H2B would run as expected in ubp10 ${Delta}$ ubp8 ${Delta}$ cells.

A recent study found modest decreases in the steady-state levelsof H3 Lys4 di- and trimethylation but a 10-fold increase inthe steady-state levels H3 Lys4 monomethylation in ubp8 ${Delta}$ cells(18). However, we do not see much change in the levels of anyform of H3 Lys4 methylation in ubp8 ${Delta}$ cells (Fig. 1). One possibilityfor the difference is that H3 Lys4 methylation was analyzedin acid-extracted histones in the previous study (18), whereaswe examined H3 Lys4 methylation in whole yeast cell extracts(see Materials and Methods). Perhaps there exists a soluble,nonnucleosomal pool of Lys4-methylated histone H3 that is detectedby the whole-cell extract but not by the differential extractionmethod. If so, the extraction method would reveal informationabout the state of H3 Lys4 methylation exclusively in the nucleosome.Alternatively, the various forms of Lys4-methylated histoneH3 could have different solubilities that affect recovery duringthe extraction procedure. Whatever the reason, our results inwhole-cell extracts are reproducible and show little changein global H3 Lys4 methylation in the absence of UBP8 (Fig. 1;see Fig. 7), which is consistent with very little role for Ubp8pin global transcription (see Fig. 8).

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FIG. 8. Loss of UBP10 and UBP8 has synergistic transcriptional effects primarily in active chromatin. Transcript array analysis using strains UCC6389 (wild type), UCC6390 (ubp10 ${Delta}$ ), UCC6392 (ubp8 ${Delta}$ ), and UCC6393 (ubp10 ${Delta}$ ubp8 ${Delta}$ ) was performed as described in the legend of Fig. 2. (A) Venn diagrams show the degree of overlap in expression changes between ubp10 ${Delta}$ , ubp8 ${Delta}$ , and ubp10 ${Delta}$ ubp8 ${Delta}$ cells. (B) Expression changes in ubp10 ${Delta}$ ubp8 ${Delta}$ cells are primarily in nontelomeric regions. Positional cluster analysis shows expression changes of genes based on distance from telomeres. Only genes that were expressed greater than or less than 1.5-fold in at least one of the strains are shown (total genes shown is 368). Genes located in telomeric regions are marked on the left. See Table S1 in the supplemental material for the entire normalized data set.

Ubp10/Dot4p is enriched at silenced loci. Negative regulation of H2B ubiquitination would explain therole of Ubp10p in silencing, given that H2B ubiquitination isrequired for histone H3 Lys4 and Lys79 methylation (9, 20, 67,91), both of which antagonize Sir protein binding to chromatin(64, 81, 92). Because Ubp10p is involved in silencing telomericgene expression through a direct interaction with Sir4p (43,85), it seemed likely that Ubp10p is localized specificallyto silent chromatin to reverse H2B ubiquitination. By chromatinimmunoprecipitation, we found that Ubp10p is preferentiallylocalized to the silent telomere VIR and the silent mating locusHMRa compared to active chromatin regions such as GAL1 and SAN1(Fig. 2).

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FIG. 2. Ubp10p is preferentially localized to silent chromatin. In vivo cross-linking analysis was performed using strains UCC6389 (untagged UBP10), UCC6390 (ubp10 ${Delta}$ ), UCC6408 (UBP10-6Myc), UCC6406 (ubp10^C371S-6Myc), UCC6407 (ubp10^94-250-6Myc), UCC6475 (UBP10-6Myc, sir2 ${Delta}$ ), UCC6477 (UBP10-6Myc, sir3 ${Delta}$ ), and UCC6479 (UBP10-6Myc, sir4 ${Delta}$ ). A ChIP assay of Ubp10 proteins was performed using anti-Myc antibodies specific for the six-Myc tag fused to the C termini of the wild-type Ubp10, mutant Ubp10^C371S, and mutant Ubp10^94-255 proteins. ChIP was also performed using untagged wild-type Ubp10p as a control. Multiplex PCR amplifications were performed to assess Ubp10p binding at the silent domains of telomere VIR and HMRa, the active SAN1 gene, and the repressed GAL1 gene. DNA of the total lysate was amplified as a control. (A) Representative example of Vistra Green-stained PCR amplifications. (B) Quantitative analysis of data in shown in panel A. Values represent the ratio of immunoprecipitate to total lysate for the query gene normalized to the ratio of immunoprecipitate to total lysate for SAN1. All values are the averages of at least two independent experiments. Error bars represent the standard deviation.

Previously, we made a number of ubp10/dot4 mutant alleles thatare compromised for telomeric silencing (43). In particular,we constructed two alleles: ubp10^C371S (originally named dot4-1),which renders Ubp10p nonfunctional by substitution of the activesite Cys371 with Ser, and ubp10^94-250 (originally named dot4-5),which is catalytically active but can no longer bind Sir4p dueto deletion of the Sir4p-binding region spanned by residues94 to 250. We found that the Ubp10^C371S protein is preferentiallylocalized to the silent regions at telomere VIR and HMRa, similarto wild-type Ubp10p (Fig. 2), whereas the Ubp10^94-250 proteinhas no preference for silent loci (Fig. 2). Loss of Ubp10p preferentiallocalization to silent regions was also observed when the silencinggenes SIR2, SIR3, or SIR4 were deleted. Thus, Ubp10p is enrichedat silent chromatin via its interaction with Sir4p, and Ubp10plocalization is independent of its ubiquitin protease activity.

Loss of Ubp10/Dot4p function and targeting disrupts global silencing of telomeric genes. We next determined if Ubp10p's function in gene repression issimilarly biased toward silent regions by examining global geneexpression in ubp10 mutant cells using DNA microarrays. To avoidsecondary effects due to the slow-growth phenotype of ubp10 ${Delta}$ and ubp10^C371S cells in synthetic (YC) medium (43), we grewcells used for the expression analysis in rich (YEPD) medium.After applying rigorous statistical criteria (see Materialsand Methods), we found that 90 genes have increased expressionby 1.5-fold or greater in ubp10 ${Delta}$ cells, and 50 of these genesare located within 20 kbp of the telomeres (Fig. 3A and seeTable S1 in the supplemental material). Because less than 5%of all genes are located within 20 kbp of the telomere, theenrichment of telomeric genes in the ubp10 ${Delta}$ expression profileindicates that the role of Ubp10p in gene expression is biasedtoward regulation of telomeric silencing. We also found that40 genes have decreased expression by at least 1.5-fold in ubp10 ${Delta}$ cells; 7 of these genes are located within 20 kbp of the telomeres(Fig. 3A; see Table S1 in the supplemental material). As expected,the gene expression profile of ubp10^C371S cells significantlyoverlaps that of ubp10 ${Delta}$ cells (Fig. 3B and see Table S1 in thesupplemental material), indicating that Ubp10p's ubiquitin proteaseactivity is largely responsible for its role in gene regulationnear telomeres and elsewhere in the genome.

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FIG. 3. Loss of UBP10 primarily affects the expression of telomeric regions. Transcript array analysis was performed using strains UCC6389 (wild type) and UCC6390 (ubp10 ${Delta}$ ) for panel A and strains UCC6432 (wild type), UCC6435 (ubp10 ${Delta}$ ), UCC6406 (ubp10^C371S), and UCC6407 (ubp10^94-250) for panel B. Cells were grown to log phase in rich medium (YEPD), and transcripts were isolated and analyzed. (A) Increased expression in ubp10 ${Delta}$ cells shows a telomeric bias. Number of genes increased in ubp10 ${Delta}$ cells plotted by position from the telomere. Histograms represent 20-kb increments from the telomeres. Red histograms represent genes with increased expression; green histograms represent genes with decreased expression. (B) ubp10^94-250 cells are specifically defective in telomeric silencing. Positional cluster analysis shows expression changes of genes based on distance from telomeres. Only genes expressed greater than or less than 1.5-fold in at least one of the strains are shown (total number of genes shown is 222). Genes located within 20 kbp of their respective telomeres are marked on the left as "telomeric regions." See Table S1 in the supplemental material for the entire normalized data set.

The gene-expression profile of ubp10^94-250 cells contrasts withthat from ubp10 ${Delta}$ and ubp10^C371S cells in one notable way. Onlytelomeric genes have increased expression in ubp10^94-250 cells;none of the other nontelomeric genes with altered expressionin ubp10 ${Delta}$ or ubp10^C371S cells is affected in ubp10^94-250 cells(Fig. 3B and see Table S1 in the supplemental material), indicatingthat the Ubp10^94-250 protein, which has the Sir4p-binding regiondeleted, is specifically defective in telomeric silencing. Theseresults also indicate that the nontelomeric gene expressionchanges in ubp10 ${Delta}$ and ubp10^C371S cells are not an indirect resultof losing telomeric gene silencing.

Ubp10/Dot4p reduces histone H3 Lys4 and Lys79 methylation at telomeric loci. Ubp10p is preferentially localized to silent chromatin, importantfor repression of telomere-proximal genes, and negatively regulatesH2B ubiquitination levels. It is therefore likely that the increasedexpression of telomere-proximal genes in the absence of Ubp10pfunction is the result of increased H2B ubiquitination withinsilent loci. To determine directly if this is the case, we requiredreagents (i.e., antibodies) that specifically recognize ubiquitinatedH2B and can be used in chromatin immunoprecipitation experiments.Despite multiple efforts, we were unable to generate such reagents,and none are available elsewhere. Instead, we chose to use H3Lys4 and Lys79 methylation as indirect markers of H2B ubiquitinationbecause these modifications both require H2B ubiquitinationand because antibodies specific for these modifications arereadily available (9, 20, 67, 91).

For the ChIP assay, we used several loci indicative of differentchromatin states including the repressed GAL1 locus, the activelytranscribed SAN1 locus, the silent HMRa locus, and a silentregion adjacent to telomere VIR. Under the growth conditionsthat we used for the assay, neither the repression of GAL1 northe expression of SAN1 is altered by deletion or mutation ofUBP10 (see Table S1 in the supplemental material). Thus, theGAL1 and SAN1 loci served as independent internal controls tojudge the relative changes in H3 Lys4 and Lys79 methylationat the silent regions in HMRa and near telomere VIR.

Using antibodies that recognize H3 Lys4 trimethylation or Lys79dimethylation, we found that both modifications are increasedat the telomere-proximal position on telomere VIR in ubp10 ${Delta}$ cells(Fig. 4). We also found similar increases at a telomere-proximalposition on telomere VIIL (data not shown). We could not detectan increase in Lys4 methylation at the silent mating-type lociHMRa in ubp10 ${Delta}$ cells but did detect a small increase in Lys79methylation (Fig. 4). The lack of a significant increase inH3 Lys4 or Lys79 methylation at HMRa is consistent with theabsence of transcription at the silent mating loci in ubp10 ${Delta}$ cells (see Table S1 in the supplemental material).

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FIG. 4. Loss of Ubp10p activity results in increased histone H3 Lys4 and Lys79 methylation and decreased Sir3p binding at telomeres. In vivo cross-linking analysis was performed using strains UCC4825 (wild type), UCC4857 (ubp10 ${Delta}$ ), UCC4870 (ubp10^C371S), UCC4836 (ubp10^94-250), and UCC4836 (sir4 ${Delta}$ ). ChIP assays of H3 Lys4 and Lys79 methylation and Sir3p binding were performed using antibodies specific for H3 Lys4 trimethylation, H3 Lys79 dimethylation, or Sir3p. Multiplex PCR amplifications were performed to assess the degree of H3 Lys4 methylation, H3 Lys79 methylation, and Sir3p binding at the silent domains of telomeres VIR and HMRa, the active SAN1 gene, and the repressed GAL1 gene. DNA of the total lysate was amplified as a control. (A) Representative example of Vistra Green-stained PCR amplifications. (B to D) Quantitative analysis of data in panel A. Values for H3 Lys4 and Lys79 methylation represent the ratio of immunoprecipitate to total lysate for the query gene normalized to the ratio of immunoprecipitate to total lysate for SAN1. Values for Sir3p binding represent the ratio of immunoprecipitate to total lysate for telomere VIR normalized to the ratio of immunoprecipitate to total lysate for HMRa. All values are the averages of at least two independent experiments. Error bars represent the standard deviation. (B) Relative fold change of H3 Lys4 tri-methylation at telomere VIR and GAL1. (C) Relative increase in H3 Lys79 methylation at telomere VIR and GAL1. (D) Relative decrease in Sir3p binding at telomere VIR.

We also performed the ChIP analysis with either ubp10^C371S orubp10^94-250 cells. Interestingly, in ubp10^C371S cells we sawa greater increase in H3 Lys4 and Lys79 methylation in the silentregions at telomeres VIR and HMRa, even though both ubp10 ${Delta}$ andubp10^C371S cells are equivalently deficient in Ubp10p catalyticactivity (Fig. 4). Although ubp10^94-250 cells also have increasedH3 Lys4 methylation at telomere VIR, the increases are lessthan in ubp10 ${Delta}$ cells (Fig. 4), which is consistent with a weakersilencing defect in ubp10^94-250 cells (see Table S1 in the supplementalmaterial). We did not observe statistically significant increasesin H3 Lys79 methylation at telomere VIR in ubp10^94-250 cells.However, is possible that the normally high levels of H3 Lys79methylation in the genome (>90% of all nucleosomes) resultin a higher background that masks small increases. Accordingly,increases in H3 K79 methylation at silent regions were consistentlytwo- to threefold lower than increases in H3 Lys4 methylation(Fig. 4 and 5).

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FIG. 5. Loss of UBP8 does not result in increased histone H3 Lys4 and Lys79 methylation and decreased Sir3p binding at telomeres. In vivo cross-linking analysis was performed as described in the legend of Fig. 4 using stains UCC6389 (wild type), UCC6392 (ubp8 ${Delta}$ ), UCC6390 (ubp10 ${Delta}$ ), UCC6393 (ubp10 ${Delta}$ ubp8 ${Delta}$ ), and UCC6391 (sir4 ${Delta}$ ). (A) Representative example of Vistra Green-stained PCR amplifications. (B to D) Quantitative analysis of data in shown in panel A was performed identically as described in the legend of Fig. 4B to D. (B) Relative increase in H3 Lys4 trimethylation at telomere VIR and GAL1. (C) Relative increase in H3 Lys79 methylation at telomere VIR and GAL1. (D) Relative decrease in Sir3p binding at telomere VIR. (E) Ubp8p does not function in telomeric silencing. Overnight, saturated cultures of yeast strains UCC6422 (wild type), UCC6423 (ubp10 ${Delta}$ ), UCC6424 (sir4 ${Delta}$ ), UCC6425 (ubp8 ${Delta}$ ), and UCC6426 (ubp10 ${Delta}$ ubp8 ${Delta}$ ), which all carry the URA3 gene located near telomere VIIL (85), were serially diluted and spotted onto YC plates, with or without uracil. Cells were grown at 30°C for 3 days.

As expected, the greatest increases in H3 Lys4 and Lys79 methylationat telomeres VIR and HMRa occur in sir4 ${Delta}$ cells (Fig. 4), in whichsilencing is completely disrupted (Fig. 5E). Although loss ofUbp10p function at telomeres does not have as great an effectas loss of Sir4p function, all ubp10 mutations result in increasedhistone H3 modifications at silenced loci.

Increased H3 Lys4 and Lys79 methylation at telomere VIR in ubp10mutant cells would be expected to result in reduced Sir proteinbinding. In ubp10 ${Delta}$ cells, we observed modest decreases in Sir3pbinding to telomere VIR (Fig. 4) and telomere VIIL (data notshown), but there is no effect on Sir3p localization to HMRa(Fig. 4), which is consistent with the fact that ubp10 ${Delta}$ cellsshow little change in silencing at HMR (or HML) and are stillable to mate with high efficiency (43, 85). As with the aboveH3 Lys4 and Lys79 methylation increases, the decreases in Sir3plocalization at telomere VIR are far greater in ubp10^C371S cellsthan in ubp10 ${Delta}$ cells (Fig. 4). One possible explanation for thisdifference is that the full-length, but catalytically inactive,Ubp10^C371S protein has a longer association with Sir4p thanwild-type Ubp10p, and this interferes with the binding of theother Sir proteins. Like ubp10 ${Delta}$ cells, ubp10^94-250 cells havemodest reductions in Sir3p binding to telomeres. In all mutantubp10 cells, changes in Sir2p binding to telomeres were similarto those observed for Sir3p, with no detectable change at thesilent mating loci (data not shown).

While Sir2p and Sir3p binding in all ubp10 mutant cells canstill be detected, Sir2p and Sir3p binding is eliminated insir4 ${Delta}$ cells (Fig. 4 and data not shown), which is consistentwith loss of SIR4 having a far greater effect on silencing thanloss of UBP10 (85). Thus, it appears that Ubp10p activity isnot required for Sir protein binding at silent loci but optimizesSir protein association instead.

Ubp8p does not regulate Lys4 and Lys79 methylation within silent regions. Loss of UBP10 results in increased H2B ubiquitination (Fig.1), which is the likely cause for the increases in H3 Lys4 andLys79 methylation in silent regions. Loss of UBP8 also resultsin increased H2B ubiquitination (Fig. 1), so we tested if similarincreases in H3 Lys4 and Lys79 methylation occur at silent regionsin ubp8 ${Delta}$ cells as they do in ubp10 ${Delta}$ cells. By ChIP analysis, wefound no effect of losing UBP8 on H3 Lys4 or Lys79 methylationin silent regions, nor did we find a detectable change in Sir2por Sir3p binding to the telomeres (Fig. 5A to D). Loss of UBP8also has no effect on telomeric silencing (Fig. 5E; see Fig.8). Ubp8p's lack of involvement in any aspect of silencing indicatesthat it is specifically Ubp10p's regulation of H2B ubiquitinationthat is required for silencing.

Loss of UBP8 has been previously reported to result in an increasein H3 Lys4 trimethylation at GAL1 under repressing conditionsof growth in glucose (33). This is curious because H3 Lys4 trimethylationhas been shown to occur specifically in the 5' coding portionof active genes and is absent from inactive and repressed genes(66, 82). Consistent with GAL1 repression in glucose-grown cells,we find no noticeable change in H3 Lys4 trimethylation at GAL1in the absence of UBP8 (Fig. 5A to C). The difference betweenour results and those from the earlier study might be explainedby differences in the strains used in each study: Henry andcolleagues used yeast strains derived from W303 (33), whereaswe used yeast strains derived from S288c. In general, glucoserepression appears to be less stringent in W303-derived strainsthan in S288c-derived strains (10). For GAL1 gene repressionin particular, it has been shown that short-term GAL1 repressionin W303-derived strains occurs more slowly and is less stringentthan in S288c-derived strains (25). A low level of GAL1 expressionin glucose-grown W303-derived strains, but not in S288c-derivedstrains, might explain the difference in the results.

Function of Ubp10/Dot4p is not restricted to silent loci. The gene expression profiles of dot4 mutant cells (Fig. 3) indicatedthat Ubp10p activity is not restricted to the regulation oftelomeric loci since the majority of total genes with alteredexpression in ubp10 ${Delta}$ cells (73 out of 130) are nontelomeric.The transcriptional effects at these loci are not the indirectresult of derepression at telomeres because none of these genesshows altered expression in ubp10^94-250 cells, which are specificallydefective in telomeric silencing (Fig. 3). Thus, Ubp10p likelyhas a direct effect on gene expression at these nontelomericloci. However, it was not clear whether the expression of thesenontelomeric loci is also regulated via modulation of H2B ubiquitinationlevels by Ubp10p. To address this issue, we examined total H2Bubiquitination and H3 Lys4 dimethylation levels in the variousubp10 alleles described above. Steady-state levels of both H2Bubiquitination and H3 Lys4 dimethylation are increased to thesame level in ubp10 ${Delta}$ and ubp10^C371S cells (Fig. 6A). Surprisingly,H2B ubiquitination and H3 Lys4 dimethylation levels in ubp10^94-250cells are identical to wild-type UBP10 cells (Fig. 6A), eventhough silencing at telomeric loci is compromised in ubp10^94-250cells. Because silent regions comprise approximately 10% oftotal chromatin (52, 55, 92), any increases in the steady-statelevels of H2B ubiquitination that occur solely as a result ofloss of silencing might not be detected by Western analysis.Supporting this idea, deletion of any individual SIR gene hasno effect on the steady-state levels of H2B ubiquitination orH3 Lys4 dimethylation (Fig. 6B). Thus, the ubp10^94-250 allelereveals that Ubp10p activity is not restricted to silent regionsand that Ubp10p also acts on nontelomeric regions to regulateH2B ubiquitination levels.

Ubp10/Dot4p and Ubp8p act on the same chromatin regions. As shown above, ubp10 ${Delta}$ cells have higher steady-state levelsof H2B ubiquitination than wild-type cells, and the levels arecomparable to those in ubp8 ${Delta}$ cells (Fig. 1 and 7). Interestingly,deletion of both UBP10 and UBP8 results in a synergistic increasein H2B ubiquitination (Fig. 1 and 7). We estimate from dilutionblotting and densitometric analyses of blots that 2 to 3% oftotal H2B is ubiquitinated in wild-type cells, 7 to 10% in ubp10 ${Delta}$ cells, 12 to 16% in ubp8 ${Delta}$ , and 35 to 40% in ubp10 ${Delta}$ ubp8 ${Delta}$ cells.An additive increase in the steady-state levels of H2B ubiquitinationin ubp10 ${Delta}$ ubp8 ${Delta}$ cells would indicate that Ubp10p and Ubp8p exclusivelyact on separate regions of chromatin. However, the synergisticincrease in H2B ubiquitination levels in ubp10 ${Delta}$ ubp8 ${Delta}$ cells indicatesthat Ubp10p and Ubp8p also act on overlapping regions of chromatin.

It was recently shown that as yeast cells enter diauxie or whenglucose is depleted, H2B ubiquitination is no longer detectable(19). We examined wild-type cells in diauxie and similarly foundthat H2B ubiquitination completely disappears (Fig. 7A). H2Bubiquitination also disappears in either ubp10 ${Delta}$ or ubp8 ${Delta}$ cellsduring diauxie, though not completely as trace amounts of H2Bubiquitination could often be detected in both ubp10 ${Delta}$ and ubp8 ${Delta}$ cells with longer exposures (Fig. 7A and B). In ubp10 ${Delta}$ ubp8 ${Delta}$ cells,however, the majority of H2B ubiquitination originally detectedin log phase is retained in diauxie (Fig. 7A). Although it isnot known whether Rad6p-Bre1p ubiquitination activity is reducedas cells enter diauxie, maintenance of the high steady-statelevels of H2B ubiquitination in ubp10 ${Delta}$ ubp8 ${Delta}$ cells indicates thatUbp10p and Ubp8p are the primary enzymes required for reductionof H2B ubiquitination during this time. The persistence of globalH2B ubiquitination in ubp10 ${Delta}$ ubp8 ${Delta}$ cells during diauxie, but notin ubp10 ${Delta}$ or ubp8 ${Delta}$ cells, further supports the idea that Ubp10pand Ubp8p overlap in many of the chromatin regions that theymodify.

The H2B ubiquitination that is still present in ubp10 ${Delta}$ ubp8 ${Delta}$ cellsduring diauxie is eliminated as cells enter stationary phase(Fig. 7A). The loss of H2B ubiquitination in stationary phaseis the likely the result of two things: Rad6p-Bre1p no longerubiquitinates H2B and another mechanism eliminates ubiquitinatedH2B. In ubp10 ${Delta}$ ubp8 ${Delta}$ cells we frequently observed an additionalmodified form of H2B with an increased molecular weight indicativeof diubiquitination (Fig. 7B). This correlated with the slowloss of H2B ubiquitination in ubp10 ${Delta}$ ubp8 ${Delta}$ cells as they transitedinto stationary phase (Fig. 7A). We speculate that the persistenceof monoubiquitin on H2B in ubp10 ${Delta}$ ubp8 ${Delta}$ cells increases the chancethat H2B will become polyubiquitinated and ultimately removedby the proteasome, perhaps by degradation. It is not clear ifthis mode of H2B ubiquitination removal is normally operativein wild-type cells or if it is only a condition of losing bothUbp10p and Ubp8p function.

We also examined the steady-state levels of H3 Lys4 and Lys79methylation in diauxic and stationary cells. In contrast tothe increased steady-state levels of H2B ubiquitination thatdisappear in ubp10 ${Delta}$ cells during diauxie and stationary phase,the increased steady-state levels of H3 Lys4 and Lys79 methylationremain throughout all phases (Fig. 7A). Thus, the transientincrease in H2B ubiquitination levels in ubp10 ${Delta}$ cells leads torelatively stable increases in H3 Lys4 and Lys79 methylation.

Ubp10/Dot4p has a role in gene expression beyond telomeric loci. From the synergistic increase in H2B ubiquitination in ubp10 ${Delta}$ ubp8 ${Delta}$ cells (Fig. 1 and 7), it seemed that Ubp10p and Ubp8p mightregulate H2B ubiquitination levels within some of the same chromatinregions. To examine this issue further, we examined gene expressionprofiles of ubp10 ${Delta}$ , ubp8 ${Delta}$ , and ubp10 ${Delta}$ ubp8 ${Delta}$ cells.

As stated above, 90 genes in ubp10 ${Delta}$ cells have increased expressionof 1.5-fold or greater, with 50 of these located within 20 kbpof the telomeres (Fig. 3 and 8). Forty genes have reduced expressionof at least 1.5-fold in ubp10 ${Delta}$ cells, with only 7 genes locatedwithin 20 kbp of the telomeres (Fig. 3 and 8).

By contrast, 17 genes have increased expression of 1.5-foldor greater in ubp8 ${Delta}$ cells, and none are located within 20 kbpof telomeres (Fig. 8), which is consistent with the fact thatUbp8p does not function in telomeric silencing (Fig. 5). Alsoin ubp8 ${Delta}$ cells, 17 genes have reduced expression of at least1.5-fold, and only 4 of these genes are located within 20 kbpof the telomeres. Of the genes with altered expression in theubp8 ${Delta}$ transcript profile, the majority (22 of a total of 34)have SAGA-dominated gene expression (38), as expected from Ubp8pfunction in SAGA-mediated transcription (18, 33, 80). It isworth noting that none of the 17 genes with increased expressionin ubp8 ${Delta}$ cells overlaps with those affected in ubp10 ${Delta}$ cells, whilejust 3 genes with decreased expression in ubp8 ${Delta}$ cells are sharedwith ubp10 ${Delta}$ cells (Fig. 8A).

As expected, the majority of genes affected in ubp10 ${Delta}$ and ubp8 ${Delta}$ cells are also affected in ubp10 ${Delta}$ ubp8 ${Delta}$ cells (Fig. 8A). However,over 160 additional genes have increased expression of 1.5-foldor greater in ubp10 ${Delta}$ ubp8 ${Delta}$ cells compared to cells carrying eitherubp10 ${Delta}$ or ubp8 ${Delta}$ alone. Of these additional genes, only 13 arelocated within 20 kbp of the telomeres (Fig. 8B; see also TableS1 in the supplemental material). The greater number of nontelomericgenes with increased expression in ubp10 ${Delta}$ ubp8 ${Delta}$ cells indicatesa possible redundancy for Ubp10p and Ubp8p at these additionalloci—either ubiquitin protease may be able to compensatein the absence of the other to maintain lower levels of transcriptionor repression at these loci. A similar situation was seen forgenes that have decreased expression in ubp10 ${Delta}$ ubp8 ${Delta}$ cells. Over40 additional genes have reduced expression of at least 1.5-foldin ubp10 ${Delta}$ ubp8 ${Delta}$ cells compared to cells carrying either ubp10 ${Delta}$ or ubp8 ${Delta}$ alone (Fig. 8A). Together, these data support the ideathat Ubp10p and Ubp8p regulate H2B ubiquitination and gene expressionat a shared set of loci in the genome.

DISCUSSION

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

We previously identified Ubp10/Dot4p as a ubiquitin proteasewhose enzymatic activity is required for optimal telomeric silencing(43, 85). However, we had not identified any ubiquitinated proteinsthat are Ubp10p substrates. Here we report that Ubp10p negativelyregulates histone H2B ubiquitination.

Ubp10/Dot4p's role in telomeric silencing may be the removal of H2B ubiquitination. Consistent with a role in silencing, we found that Ubp10p istargeted to silent regions by its Sir4p-interaction domain (Fig.2), and this interaction facilitates telomeric silencing bypreventing the accumulation of H3 Lys4 and Lys79 methylation(Fig. 4). Given Ubp10p's ubiquitin protease activity and therequirement of H2B ubiquitination for H3 Lys4 and Lys79 methylation(9, 20, 67, 91), we propose that Sir4p targets Ubp10p to silentchromatin to remove ubiquitin from H2B. This, in turn, woulddecrease the probability that H3 Lys4 and Lys79 become methylatedwithin silenced regions.

The role for Ubp10p in silencing is best considered in lightof the dynamic binding nature of chromatin proteins. Chromatinproteins continually associate and dissociate from chromatin,including the proteins considered to have relatively stableassociations in vitro (72, 73). Indeed, Sir protein bindingto silent chromatin is dynamic throughout the cell cycle, evenin G₁ and M when the genome is not being replicated (14, 51,56). Temporary dissociation of Sir proteins from silent chromatincould leave these regions briefly accessible to the Rad6p-Bre1pcomplex and thereby susceptible to H2B ubiquitination. If fortuitousH2B ubiquitination persists for too long, this reversible histonemark could be converted into the more permanent marks of H3Lys4 and Lys79 methylation, which would prevent the reassociationof Sir proteins and result in the loss of silencing. We postulatethat Sir4p-dependent enrichment of Ubp10p at silent chromatinconcentrates its ubiquitin protease activity to maintain silencingin the face of Sir protein dynamics.

While Ubp10p is localized to the silent mating region HMRa ina Sir4p-binding domain-dependent manner (Fig. 2), loss of UBP10does not appreciably alter HM silencing as measured by silencingreporters placed at either HM loci (85), global transcript analysis(see Table S1 in the supplemental material), ChIP assay of H3Lys4 methylation (Fig. 4), and quantitative mating assays ofubp10 ${Delta}$ cells (data not shown). HM silencing is inherently morestable than telomeric silencing (31), due to the significantstabilization of Sir protein association with chromatin by thebinding of Sir1p to HM loci silencer regions (15). If this greaterstability occurs by a reduction in Sir protein dissociation,it would readily explain the reduced reliance on Ubp10p actionat the silent mating loci and maximal Sir protein binding toHMRa in the absence of UBP10 (Fig. 4).

Ubp10/Dot4p negatively regulates global H2B ubiquitination and H3 Lys4 and Lys79 methylation. We found that loss of silencing, by deletion of any single SIRgene or the Sir4p-binding region in Ubp10p, does not resultin higher steady-state levels of H2B ubiquitination or H3 Lys4methylation (Fig. 6), despite the fact that these manipulationsresult in increases in H3 Lys4 methylation in silent regions(Fig. 4). Yet loss of Ubp10p catalytic activity, by deletionof UBP10 or mutation of the catalytic Cys residue, does resultin higher steady-state levels of H2B ubiquitination and H3 Lys4and Lys79 methylation (Fig. 6), indicating that Ubp10p activityis not limited to silent chromatin.

From these observations, it is likely that Ubp10p has a similarfunction elsewhere in the genome as it does in silent chromatin—tolimit or prevent H3 Lys4 and Lys79 methylation by reversingH2B ubiquitination. However, there may be a significant differencein how Ubp10p activity is used. In silent chromatin, it is proposedthat all forms of H3 Lys4 and Lys79 methylation will interferewith Sir protein binding (64, 81, 92), so Ubp10p may be recruitedto prevent any methylation of H3 Lys4 and Lys79. Elsewhere inthe genome, the degree of methylation coincides with differentfunctional states. For example, H3 Lys4 dimethylation and Lys79methylation are present throughout the genome (5, 63, 64, 66,82, 92) and help prevent the promiscuous binding of Sir proteins(82, 92). By contrast, H3 Lys4 trimethylation specifically occursin the 5' coding portion of active genes and is absent frominactive genes (66, 82). It has been suggested that H3 Lys4trimethylation facilitates gene transcription and possibly servesas a memory mark for recent transcriptional activity (66, 82).At inactive genes, H2B ubiquitination would have to persistlong enough for some methylation of H3 Lys4 and Lys79 to occurbut be eliminated before H3 Lys4 trimethylation occurs. Consideringhow loss of UBP10 affects the steady-state levels of H3 Lys4methylation (Fig. 1 and 7), we propose that Ubp10p acts at inactiveor repressed genes to facilitate this timely removal of ubiquitinfrom H2B. Consistent with this idea, the majority of nontelomericgenes with altered expression in ubp10 ${Delta}$ and ubp10 ${Delta}$ ubp8 ${Delta}$ cellshave increased transcription (Fig. 3 and 8), indicating thatUbp10p may be involved in maintaining their inactivity or repression.This is not an indirect effect of losing silencing because thealtered expression of these genes does not occur in ubp10^94-250cells, which are specifically defective in telomeric silencing.Perhaps Ubp10p is targeted to inactive genes by repressive complexes,similar to recruitment by Sir4p to silent regions. If so, Ubp10pbinding to repressors would have to be through a different domainthan that used for binding to Sir4p. Alternatively, the lossof Ubp10p activity might indirectly affect transcription byalterations in the ubiquitination levels of other proteins inaddition to H2B.

Ubp10/Dot4p and Ubp8p have separate and overlapping functions. In addition to its role in silencing, we propose that Ubp10p'sregulation of global H2B ubiquitination levels overlaps, inpart, with that of Ubp8p. While loss of either UBP10 or UBP8results in higher steady-state levels of H2B ubiquitinationand functionally different phenotypic consequences for the cell(Fig. 1 and 5), the absence of both UBP10 and UBP8 togetherresults in a synergistic increase in H2B ubiquitination levelsand transcription (Fig. 7 and 8). Overlapping roles for Ubp10pand Ubp8p in gene regulation or other chromatin-related functionsis further underscored by the persistence of ubiquitinated H2Bin ubp10 ${Delta}$ ubp8 ${Delta}$ cells as they enter diauxie, which contrasts withthe virtual disappearance of ubiquitinated H2B in ubp10 ${Delta}$ andubp8 ${Delta}$ cells (Fig. 7). Of course, Ubp8p and Ubp10p are separablein some functions: Ubp8p functions in SAGA-mediated transcription(18, 33, 80), whereas Ubp10p functions in silencing (Fig. 5).Also, Ubp10p, but not Ubp8p, regulates steady-state H3 Lys4and Lys79 methylation levels, even though both regulate steady-stateH2B ubiquitination levels (Fig. 1). Despite these separablefunctions, the synergistic increases in steady-state H2B ubiquitinationlevels and transcription in ubp10 ${Delta}$ ubp8 ${Delta}$ cells underscore a potentialoverlapping role for these ubiquitin proteases.

The ubp10^94-250 allele demonstrates that Ubp10p regulates H2Bubiquitination outside of its defined role in silencing, butno such separation-of-function alleles that demonstrate a rolefor Ubp8p outside of the SAGA complex have been isolated. Itwas recently found that Sgf11p facilitates the interaction ofUbp8p with SAGA (41, 53, 74). Interestingly, while purificationof Sgf11p resulted primarily in the copurification of SAGA components,other transcriptional regulators also copurified with Sgf11p(74), indicating that Sgf11p may link Ubp8p to other chromatin-relatedprocesses in addition to SAGA-mediated transcription. Takingthis and our findings into consideration, we believe Ubp8p functionsin other aspects of H2B deubiquitination in addition to itsdefined role in SAGA-mediated transcription.

Although it is not clear at this point how Ubp10p and Ubp8pregulate H2B ubiquitination at common loci, such an effect couldbe the result of nonspecific chromatin binding that is independentof their targeted recruitment by Sir complexes and SAGA, respectively.As is the case for a number of histone acetylases and deacetylases(44, 47, 75, 94), Ubp10p and Ubp8p may be able to remove H2Bubiquitination from chromatin throughout the genome withouta high-affinity interaction. Some loci may be more susceptibleto such "hit-and-run" activities, and alterations in H2B ubiquitinationand gene expression are only revealed when both Ubp10p and Ubp8pare absent.

Multiple reasons for removal of ubiquitin from H2B. The cell may modulate H2B ubiquitination levels by these ubiquitinproteases for a variety of reasons. Removal of ubiquitin fromH2B may be used during gene repression to prevent H3 Lys4 andLys79 methylation, similar to Ubp10p's role in silencing (43,85). Deubiquitination of H2B may also facilitate transcription,as is the case for Ubp8p's role in SAGA-mediated transcription(18, 33, 80). There is evidence that deubiquitination of H2Bmay also occur during mitosis to allow chromatin compaction(12, 57, 61). Removal of ubiquitin from H2B may be importantin halting transcription of mitotic genes as cells exit thecell cycle and may be the reason for deubiquitination of H2Bas yeast cells transit into stationary phase (Fig. 7). Lastly,removal of the single ubiquitin moiety from ubiquitinated H2Bmay be required to prevent multiubiquitination and subsequentdegradation of modified H2B by chromatin-associated proteasomes(29, 30, 60). These and other yet to be discovered outcomesof removing H2B ubiquitination likely contribute to the dynamicand flexible nature of chromatin.

Ubp10/Dot4p may have other roles beyond regulating H2B ubiquitination. It is important to note that Ubp10p may target other ubiquitinatedproteins in addition to histone H2B. For instance, Ubp10p alsoappears to regulate the steady-state levels of the general aminoacid permease Gap1p (42). Because plasma membrane permeasesare subject to regulated ubiquitination and endocytosis (34),Ubp10p may indirectly affect transcription of some genes asa result of altered nutrient transport. In fact, ubp10 ${Delta}$ cellshave a slow-growth phenotype that is exacerbated in syntheticmedium and by the presence of multiple amino acid and nucleotideauxotrophies (43). Thus, in the absence of de novo biosyntheticcapabilities, ubp10 ${Delta}$ cells may be starved for essential nutrientsdue to impaired transport. Previous transcript analyses of ubp10 ${Delta}$ cells grown in minimal medium found a large number of stressresponse genes with increased expression, coincident with anincrease in cellular oxidative damage (70). Nutrient starvationoften results in a significant transcriptional stress response(28), which is similar to that observed in ubp10 ${Delta}$ cells grownin minimal medium (70). Furthermore, protracted amino acid starvationinduces production of reactive oxygen species and increasesapoptosis in wild-type cells (21), similar to what is observedin ubp10 ${Delta}$ cells (70). The increased expression of stress responsegenes is likely a secondary response to nutrient starvationin ubp10 ${Delta}$ cells. Deletion of any SIR gene can partially compensatefor the slow-growth phenotype and the transcriptional stressresponse in ubp10 ${Delta}$ cells (43, 70). Because a number of subtelomericgenes encoding cell wall stress proteins are regulated by modulationof silencing (1), sir ${Delta}$ suppression is also likely to be a secondaryeffect resulting from the increased expression of these proteinsthat allows sufficient cell wall structural changes to facilitatenutrient transport and partially alleviate the starvation ofubp10 ${Delta}$ cells.

Understanding the complete nature of Ubp10p action in the cellwill require efforts aimed at identifying all of its substratesand target chromatin regions. Construction and analysis of separation-of-functionalleles, as done here with ubp10^94-250, will help delineateUbp10p action in active chromatin from that in silent chromatin.Because histone deubiquitination may be operative in many differentspecies as a regulatory mode (12, 32, 58, 59, 61), we believefurther understanding of the role of Ubp10p in modulating histoneH2B ubiquitination will yield greater insight into this commonaxis of chromatin regulation.

ACKNOWLEDGMENTS

We thank M. A. Osley for the FLAG-tagged H2B plasmids and J.Delrow for statistical analysis of the transcript microarraydata. We thank H. Eisen and the members of the Gottschling labfor insightful discussions and critical reading of the manuscript.

R.G.G. is a Bristol Myers Squibb fellow of the Life SciencesResearch Foundation. This work was supported by National Institutesof Health grant GM43893 to D.E.G.

FOOTNOTES

* Corresponding author. Mailing address: Fred Hutchinson Cancer Research Center, Mail stop A3-025, P.O. Box 19024, Seattle, WA 98109-1024. Phone: (206) 667-4494. Fax: (206) 667-5894. E-mail: dgottsch{at}fhcrc.org.

Supplemental material for this article may be found at http://mcb.asm.org/.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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