Chromatin assembly factor Asf1p-dependent occupancy of the SAS histone
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《核酸研究医学期刊》
Laboratory of Environmental Biochemistry, Graduate School of Pharmaceutical Sciences, Osaka University 1-6 Yamada-Oka, Suita, Osaka 565-0871, Japan
*To whom correspondence should be addressed. Tel: +81 6 6879 8242; Fax: +81 6 6879 8244; Email: osada@phs.osaka-u.ac.jp
ABSTRACT
Transcriptional repression of the silent mating-type loci HML and HMRa in Saccharomyces cerevisiae is regulated by chromatin structure. Sas2p is a catalytic subunit of the SAS histone acetyltransferase (HAT) complex. Although many HATs seem to relieve chromosomal repression to facilitate transcriptional activation, sas mutant phenotypes include loss of SIR1-dependent silencing of HML. To gain insight into the mechanism of the SAS complex mediated silencing at HML, we investigated the expression and chromatin structure of the 2 gene in the HML locus. We found that deletion of SAS2 in combination with a null allele of SIR1 changed the chromatin structure of the precisely positioned nucleosome, which includes the mRNA start site of the 2 gene and derepressed 2 transcription. The Sas2p HAT domain was required for this silencing. Furthermore, chromatin immunoprecipitation analysis revealed that the SAS complex was associated with the HML locus, and ASF1 (which encodes chromatin assembly factor Asf1p), but not SIR1 and SIR2, was necessary for this localization. These data suggest that the HAT activity and ASF1-dependent localization of the SAS complex are required for SIR1-dependent HML silencing.
INTRODUCTION
Silencing affects gene repression in a regional rather than promoter- or sequence-specific manner (1). The structure of the chromatin itself can affect gene expression, and changes in chromatin structure can result from the modification of histone tails as well as from the action of chromatin-remodeling complexes (2). A number of factors have been identified that contribute to transcriptional regulation by covalent modification of histones. In many cases, a relationship between histone acetylation and gene activation has been revealed by the identification of transcriptional co-activators, such as dedicated histone acetyltransferases (HATs) (3,4). Histone acetylation is reversed by histone deacetylases (HDACs), and many repression phenomena are regulated by HDACs (5). Moreover, HATs have been shown to contribute to repression and activation (4).
In Saccharomyces cerevisiae, silenced loci include the HML and HMRa mating-type loci, the telomere regions and the ribosomal DNA repeats (2). A variety of proteins, including the silent information regulator (Sir) proteins, are required to silence the mating information genes at silent loci (6). One of the Sir proteins, Sir2p, possesses HDAC activity important for silencing (7,8). Disruption of the SIR2, SIR3 or SIR4 gene results in loss of silencing at HM loci, and a SIR1-disrupted strain is composed of mixed populations of silenced and unsilenced cells (9).
Something About Silencing (SAS) 2 was identified as an enhancer of sir1 epigenetic HML silencing defects (10). Sas2p is a member of the MYST (MOZ, Ybf2/Sas3, Sas2 and TIP60) family of HATs and forms a complex, termed the SAS complex, with Sas4p and Sas5p (11–14). The SAS complex mainly acetylates histone H4 at lysine 16 (12–16). The role of SAS2 in silencing is different for each silenced locus. At HML, deletion of SAS2 has very little effect on silencing. However, deletion of SAS2 combined with deletion of SIR1 causes a severe silencing defect (10,17). Normal HMRa silencing is unaffected by SAS2 deletion, but sas2 mutation suppresses the silencing defect caused by mutations in silencer elements of HMRa (10,17). To determine the role of SAS2 in rDNA silencing, a strain in which the URA3 gene is integrated at the rDNA locus was used. The sas2 deletion strain showed more effective URA3 repression, indicating that the deletion of SAS2 increased rDNA repression (12). In the case of telomeres, loss of SAS2 causes hypoacetylation in adjacent sub-telomeric regions, leading to the recruitment of Sir3p to these regions and inactivation of gene expression (15,16). Therefore, sas2 mutations reduce silencing of HML (when combined with deletion of SIR1) but improve silencing at HMRa when accompanied by a weakened silencer element, hypoacetylated sub-telomeric regions, or the rDNA locus. To understand the differing roles of Sas2p, it is important to investigate the biochemical mechanisms by which these factors regulate gene silencing in each silent locus.
We previously showed that the chromatin assembly factor Asf1p interacts with the SAS complex, and ASF1 and SAS2 genetically function in the same pathway to repress the HML locus (11). In the present study, we show that SAS2 is essential for the organization of the chromatin structure at HML in a sir1 mutant and that ASF1 is required for the recruitment of the SAS complex to the HML locus.
MATERIALS AND METHODS
Yeast strains, plasmids and manipulations
The strains used in this study are listed in Table 1 and were either published previously or were created for this study by using standard yeast manipulations (18,19). Expression plasmids of wild-type and mutant alleles of SAS2 and ASF1 were described previously (11). Mating assays were performed as described previously (11,20).
Table 1 Yeast strains used in this study
RNA blots
A 40 μg aliquot of total RNA prepared from logarithmically growing cells was separated on 1.0% agarose–formaldehyde gels and transferred to Hybond-N+ membranes (Amersham Biosciences, Piscataway, NJ). Specific messages were detected using randomly labeled 2 and SCR1 probes.
High-resolution micrococcal nuclease mapping
Preparation of nuclei was carried out as described previously (21,22). Briefly, nuclei were isolated from yeast cells, which were grown to mid-log phase (OD600 = 1). The nuclear pellet from a 1 liter culture was resuspended in 2.4 ml digestion buffer (10 mM HEPES, pH 7.5, 0.5 mM MgCl2 and 0.05 mM CaCl2). The suspension was divided into 400 μl portions, each of which was digested at 37°C for 10 min by using increasing concentrations (0–16 U/ml) of micrococcal nuclease (MNase; Amersham Biosciences). The reaction was terminated by adding EDTA, and the DNA was purified after treatment with RNase, proteinase K digestion and phenol–chloroform extraction. The purified DNA was resuspended in 0.1x TE (1 mM Tris–HCl, pH 8.0, 0.1 mM EDTA). MNase cleavage sites were detected by multiple rounds of Taq DNA polymerase-based primer extension. The primer (5'-TATGTCTAGTATGCTGGATTTAAACTCAT-3') was end-labeled by T4 polynucleotide kinase. The cycling program was 94°C for 1 min, 53°C for 2 min and 72°C for 2 min for 35 cycles, and was followed by a 10 min chase at 72°C. The products were electrophoresed on a 6% polyacrylamide–8 M urea gel. The gel was dried and used to expose X-ray film. Relative MNase sensitivity was expressed graphically after scanning the autoradiogram and analyzing the scan by the NIH Image program (version 1.62).
Chromatin immunoprecipitation assay
The chromatin immunoprecipitation (ChIP) assay was performed essentially as described previously (23,24). A 50 ml culture of yeast (OD600 = 1) was treated with formaldehyde (final concentration of 1%) for 30 min at 20°C, and 2.5 ml of 2 M glycine was added to stop the cross-linking reaction. Cells were harvested and disrupted by vortexing in the presence of glass beads, and the lysate was sonicated to generate DNA fragments that ranged in size from 200 to 800 bp. To immunoprecipitate Myc-tagged proteins and Sir2p, we incubated anti-Myc antibody (9E10, Roche, Indianapolis, IN) and anti-Sir2p antibody (Santa Cruz Biotech., Santa Cruz, CA), respectively, with the extract overnight at 4°C, and the extract–antibody mixture then was incubated for an additional 3–4 h with protein G Sepharose beads (Amersham Biosciences). In some experiments, Myc-blocking peptide (Roche, final concentration 313 μg/ml) was added. Immunoprecipitates were washed with 1 ml each of lysis buffer (50 mM HEPES, pH 7.5, 140 mM NaCl, 1 mM EDTA, 1% Triton X-100, 0.1% sodium deoxycholate, 1 mM phenylmethylsulfonyl fluoride, 1 μg/ml leupeptin and 1 μg/ml pepstatin A), lysis buffer supplemented with 250 mM NaCl (for Myc-tagged Sas proteins) or 500 mM NaCl (for Sir2p), LiCl–detergent wash buffer (250 mM LiCl, 10 mM Tris–HCl, pH 8.0, 1 mM EDTA, 0.5% NP-40 and 0.5% sodium deoxycholate) and TE. DNA was eluted with elution buffer (50 mM Tris–HCl, pH 8.0, 10 mM EDTA and 1% SDS). After reversal of the formaldehyde-induced cross-links, 1/5000 of input DNA and 1/45 of each immunoprecipitated DNA were used as templates for amplification by PCR. The sequences of primers for PCR were as follows: for the HML region, 5 '-ATGCTCAGCTAGACGTTTTTCTTTC-3' and 5'-TATGTCTAGTATGCTGGATTTAAACTCAT-3'; for the ACT1 promoter region, 5'-CTTTTTCTTCCACGTCCTCTTGC-3' and 5'-TGGGATGGTGCAAGCGC-3'; and for the sub-telomeric chromatin at 7.5 kb from the end of chromosome VI, 5'-TCATGGTCTTGACAACTTTATGCG-3' and 5'-TATCTGACGTGAAAGTTCAGCGC-3'. Amplification was performed in a 20 μl reaction volume. The number of PCR cycles yielding product within the linear range was determined by analysis of 2-fold serial dilutions of the starting materials, and PCR products were separated on a 6% polyacrylamide gel and were detected by autoradiography. For quantitative analysis, 0.025 μl of dCTP (110 TBq/mmol; Amersham Biosciences) was added to the PCR. After electrophoresis, the gel was dried, and the radioactivity corresponding to a specific band was measured by a bioimage analyzer (model BAS 1800II, Fuji Film, Tokyo, Japan).
Determination of the molecular size of the SAS-containing complex
Whole-cell extracts were prepared as described previously (11,25). Approximately 0.4 mg of each whole-cell extract was loaded onto a 2.4 ml Superdex 200 PC 3.2/30 column (Amersham Biosciences) that had been equilibrated in buffer containing 50 mM Tris–HCl, pH 8.0, 500 mM NaCl, 10% glycerol, 0.1% Tween-20, 1 mM phenylmethylsulfonyl fluoride, 0.5 μg/ml leupeptin and 0.5 μg/ml pepstatin A. A 10 μl aliquot of each fraction was electrophoresed in an SDS–polyacrylamide gel, transferred to nitrocellulose membrane and detected with the ECL western blotting analysis detection system (Amersham Biosciences). Anti-Myc antibody (9E10, Roche) was used.
RESULTS
HML2 was derepressed in a sas2 sir1-deleted strain
The 2 protein, which is a repressor of transcription of a-specific genes, is encoded by MAT and an essential factor for the regulation of mating-type-specific genes in cells (26). The silent information is also stored at the HML locus in both a and cells. Previous work showed that the deletion of either SIR1 or SAS2 results in a very slight reduction of mating activity in a MATa strain, as indicated by quantitative mating analysis. The combined deletion of SIR1 and SAS2 strain causes a much more severe mating defect than that of the wild-type strain or the single-deletion strains (10,11). To show that the double deletion of SAS2 and SIR1 directly affects silencing at HML, we performed northern blotting analysis to detect the level of 2 mRNA in wild-type and deletion strains. 2 was transcribed not only in MAT cells but also in sir4 and sas2sir1 MATa cells (Figure 1A).
Figure 1 Deletion of SAS2 and SIR1 in a MATa strain leads to derepression of HML2 expression and a non-mating. (A) RNA from either wild-type (WT, W303-1b and W303-1a), sir4 (YJW257), sir1 (YJW252), sas2 (YJW253) or sas2sir1 (YJW258) strains was hybridized by northern blotting to a probe specific for either the 2 or SCR1 gene. RNA loading was standardized to SCR1. A qualitative mating assay was performed by patches, which were replica-plated to a lawn of MAT cells. WT and mutant strains are presented at the top of the panel. (B) A sas2sir1 double-deletion strain was transformed with a plasmid carrying the WT or a mutant form of the SAS2 gene (M1) under the control of its own promoter. Strains analyzed (ordered from left to right) were YSM119, YSM118, YSM120, YSM121, YSM122 and YSM123.
We previously showed that wild-type SAS2, but not SAS2 with a mutation in the conserved HAT domain, could restore the mating activity of the sas2sir1 strain. Furthermore, this mutation of amino acids 219–221 (GLG) to alanine residues (termed SAS2-M1) abolished the HAT activity of Sas2p but did not affect the formation of the SAS complex (11,13). To determine whether Sas2p HAT activity is required for the repression of 2 expression, wild-type and mutant SAS2 alleles were transformed into the sas2sir1 strain (Figure 1B). The mating activity and RNA level of 2 in the sir1 mutant were the same as those of the sas2 sir1 double-deletion strain carrying the wild-type SAS2 expression plasmid (Figure 1B, compare lanes 3 and 5). SAS2-M1 failed to restore mating activity and 2 repression to the sas2 sir1 double-mutant strain (Figure 1B, compare lanes 4 and 6). These results suggest that the Sas2p HAT activity is required for the repression of 2 expression from HML in a sir1 mutant.
A strain with deletions of SIR1 and SAS2 shows loss of nucleosome organization at HML
The unique and highly organized chromatin structure of HML has been determined by high-resolution chromatin mapping analysis using MNase, which preferentially cuts the linker DNA between nucleosomes (27). Although a precisely positioned nucleosome (NUC2) covers the transcription start site of the 2 gene at the HML locus, the promoter region of the 2 gene is nucleosome-free . We used MNase mapping to examine the effect of sas2 mutations on the chromatin structure of HML. Deletion of SIR4, which is essential for HML silencing, resulted in increased nuclease sensitivity of one site, indicated by the arrow, compared with that of the wild type (Figure 2A, compare lanes 6–8 with lanes 10–12). Although we used downstream and reverse-strand primers in the attempt to visualize the positioning of NUC2 clearly, we failed to obtain sufficient quantities of primer-extension products. For easy comparison of the MNase sensitivity, the lane treated with the highest concentration of MNase was selected for scanning (Figure 2A, lanes 8, 12, 16, 20 and 24). Relative MNase sensitivity is shown in Figure 2B after scanning and analyzing with the NIH Image software. The intensity of the induced sensitivity of the site highlighted in Figure 2A is the same in sas2 sir1 double-deleted cells as in SIR4-deleted cells (compare lanes 10–12 with lanes 22–24) and stronger than that of wild-type or singly deleted strains (compare lanes 6–8, 14–16 and 18–20 with lanes 22–24). The MNase sensitivity of this site in different mutants correlates inversely with their mating activity and directly with the level of 2 mRNA (Figure 1A). These results suggest that SAS2 is essential for the organization of the nucleosome precisely positioned over the transcriptional initiation site of the 2 in a sir1-mutant strain.
Figure 2 High-resolution MNase mapping of the promoter region of the 2 gene at the HML locus. (A) The chromatin structure of the Crick strand was mapped by primer-extension analysis of MNase-digested sites with the primer located at the coding region of the 2 gene. Strains used were as in Figure 1A. Extensions of undigested (0) and dose-dependent-digested chromatin are indicated. The ‘n’ lane shows the naked DNA digested with MNase (lane 25). The G, A, T and C columns indicate dideoxynucleotide-terminated sequencing reactions (lanes 1–4). The ellipse corresponds to the inferred position of the nucleosome, and boxes show the positions of the TATA-box and UAS regions. Arrow indicates sites in the 2 gene whose nuclease-sensitivity was increased in mutants relative to WT. The vertical bar indicates the region used for scanning to express the relative intensity in Figure 2B. (B) The relative MNase sensitivity expressed graphically after scanning and analyzing the autoradiogram in (A) by using NIH Image 1.62 software. Increased levels of nuclease-sensitive sites of the 2 gene in mutants (sir4 and sas2sir1) relative to WT are indicated by arrows. The position from the transcription start site is shown at the bottom of each panel.
Interestingly, the nuclease sensitivity of the region between the UAS and TATA-box regions was decreased in sas2sir1 and sir4 strains. This region is generally less nuclease sensitive at MAT than at HML (27), and it is thought that in 2-positive cells, the protection of this region in chromatin from the nuclease might result from an association of transcription factors, including Rap1p, which bind to UAS (27). Overall, chromatin in this region is less accessible to nuclease in sas2sir1 strain than in wild-type strains.
The SAS complex associates with the HML locus
Genetic experiments revealed that combining the null allele of SIR1 with that of SAS2, SAS4, SAS5 or ASF1 results in the reduction of silencing at HML (11,17). Meijsing and Ehrenhofer-Murray (12) reported that Sas2p is physically present at the rDNA locus, but not ACT1. To determine whether Sas2p or the SAS complex is located at the HML locus, we performed ChIP analysis using strains expressing Sas2p–Myc. Immunoprecipitated DNA was amplified by PCR with a primer pair spanning the 1 and 2 promoter regions in the HML locus (Figure 3A). We used ACT1, a gene whose transcription is not regulated by SAS2, as a negative control, because the ACT1 mRNA level in the sas2 mutant was same as that in the wild-type strain (15). Two-fold serial dilutions of the input and the immunoprecipitated DNA were performed to verify that the amount of PCR product was dependent on the starting material. Input DNA also was used as a template to confirm that these regions were amplified equally by PCR. In a SAS2–Myc strain, Sas2p–Myc associated with the promoter regions of the 1 and 2 in the HML region relative to ACT1 (Figure 3A). This association was completely competed by adding a Myc-blocking peptide (compare lanes 11 and 12 with lanes 13 and 14).
Figure 3 The SAS complex occupancy at the promoter in the HML locus. (A) Association of Sas2p with the HML region is detected by the ChIP assay. Sonicated chromatin was prepared from wild-type (WT) and Sas2p–Myc-expressing (YJW265) strains. Immunoprecipitation was carried out using monoclonal antibodies to the Myc tag (lanes 3–6 and 11–14), and normal IgG was used as a negative control (lanes 7, 8, 15 and 16). Myc-blocking peptide was added in some immunoprecipitation experiments (lanes 5, 6, 13 and 14). Input and immunoprecipitated DNA were amplified by PCR using primer pairs spanning the promoter region of 1 and 2 genes or ACT1. PCR products were resolved on a 6% polyacrylamide gel and visualized by autoradiography. (B) Localization of subunits of the SAS complex to the promoter of the 1 and 2 genes. Soluble chromatin was prepared from the strains that expressed the C-terminal Myc epitope-tagged Sas2p (YJW265), Sas4p (YJW228) or Sas5p (YJW229), and immunoprecipitated with or without anti-Myc antibody. Final DNA extractions were amplified with dCTP. The PCR product was separated on the polyacrylamide gel and quantitated with a bioimage analyzer after drying the gel. ChIP efficiency is reported as a percentage of immunoprecipitated material (top panel). Data are presented as the mean ± SD from three independent experiments. Input DNA (input) was equally amplified by PCR in WT and Sas2p–Myc-expressing strains. Myc-tagged proteins were detected by western blotting (bottom panel). (C) SAS4 or SAS5 or both are required for the recruitment Sas2p to the HML locus. ChIP assay was performed with chromatin prepared from sas4 (YJW269), sas5 (YJW270) and sas4sas5 (YJW271) strains that expressed the C-terminal Myc epitope-tagged Sas2p. Results are shown as in Figure 3B.
We previously purified a complex containing Sas2p and showed that Sas4p and Sas5p were components of this complex, termed the SAS complex (11,13,14). We next asked whether Sas4p and Sas5p associate with the HML locus. ChIP analyses using SAS4–Myc and SAS5–Myc revealed that Sas4p–Myc and Sas5p–Myc were recruited together with Sas2p–Myc to the promoter regions of the 1 and 2 in the HML region (Figure 3B). This finding supports the possibility that these Sas proteins associate with chromatin as a complex. Accordingly, deletion of either SAS4 or SAS5 might disrupt the association of Sas2p with the HML locus.
To evaluate whether this disruption occurs, we performed ChIP using cells expressing Sas2p–Myc and deleted for SAS4, SAS5 or both genes (Figure 3C). The amount of amplified PCR products from the three deletion strains was markedly lower than from the wild-type strain, although Sas2p–Myc was expressed efficiently in all of the SAS2–Myc strains. These results show that mutations in SAS5 and especially SAS4 inhibit the association of Sas2p–Myc with the promoter regions of the 1 and 2 in the HML region and that Sas2p–Myc was recruited to this region as a component of the SAS complex.
SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoters in the HML locus
Four Sir proteins localize to HML and HMRa and are important for silencing. Sir1p binds to Orc1p, one of the silencer binding proteins, and helps to recruit Sir4p. Sir2p, Sir3p and Sir4p form a complex and spread in both directions from the silencers (1,28). A physical interaction between Sas and Sir proteins has not been reported, although all of them localize to the HML locus. To understand the role of the Sir proteins in the association of Sas2p with the HML locus, we first asked whether loss of Sir1p or Sir2p results in disruption of this association. To do this, Sas2p was tagged with Myc in SIR1 or SIR2 deletion strains. Western blot analysis revealed that Sas2p–Myc was expressed efficiently in both SIR1 and SIR2 deletion strains (Figure 4A). We prepared chromatin fractions from these strains and subjected them to ChIP analysis for the Myc epitope. As shown previously, Sas2p–Myc associated with the HML region in wild-type cells. Loss of SIR1 or SIR2 did not affect this association (Figure 4A). This finding indicates that SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoters in the HML locus.
Figure 4 (A) SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoter in the HML locus. ChIP assay was performed with chromatin prepared from sir1 (YSM85) and sir2 (YSM90) strains that expressed the C-terminal Myc epitope-tagged Sas2p. (B) Effect of deletion of SAS2 and SIR genes on the Sir2p occupancy. Soluble chromatin was prepared from wild-type and deletion strains, and immunoprecipitated with or without anti-Sir2p antibody. Strains analyzed (ordered from left to right) were W303-1a, sas2 (YJW253), sas2sir1 (YJW258), sir1 (YJW252), sir2 (YSM64) and sir3 (YS480). Results are shown as in Figure 3B.
Disruption of SAS2 in a wild-type strain increased the spreading of Sir proteins to the sub-telomeric region (15,16). Deletion of SAS2 in a sir1 mutant also may lead to spreading of the finite number of Sir2p molecules into sub-telomeric regions, resulting in a decrease in Sir2p occupancy at the HML locus. To test this hypothesis, we asked whether loss of SAS2 results in increased or decreased Sir2p association. We observed localization of Sir2p in the regions of the HML locus and sub-telomeric chromatin 7.5 kb from the end of chromosome VI in the wild-type and deletion strains (Figure 4B). Consistent with previous observations, the Sir2p association detected within the HML locus and sub-telomeric regions in the wild-type strain was greater than that in a sir2 deletion strain (Figure 4B, compare lanes 1 and 5) and was slightly increased in the sub-telomeric region by SAS2 deletion (16,29). Interestingly, although Sir2p was expressed efficiently in all of the strains except a sir2 deletion strain, the disruption of SAS2 or SIR1 decreased the amount of Sir2p localization at the HML locus (Figure 4B). In the combination of SAS2 deletion with the null allele of SIR1, the Sir2p association at the HML locus was completely lost, similar to that in the SIR2 and SIR3 deletion strains. This indicates that although Sas2p association at the HML locus does not require SIR1 or SIR2, Sir2p localization is partially dependent on SAS2.
2 expression in the asf1 sir1 deletion strain
We and others (11,12) previously showed that the SAS complex physically interacts with Asf1p and these factors function in a pathway that enhances the epigenetic silencing defects of sir1 mutants. To learn more about the function of ASF1 in the HML silencing, we measured the expression of 2 in an ASF1 deletion strain (Figure 5). Deletion of ASF1 results in a very slight reduction in silencing at HML as indicated by quantitative mating analysis (11), and the 2 mRNA level in the asf1 mutant was indistinguishable from that of the wild-type strain. We previously showed that the combined deletion of ASF1 and SIR1 caused much more severe silencing defects at HML than does the deletion of ASF1 alone (11). Derepression of 2 repression occurred in the asf1 sir1 double-deletion strain but not in the asf1sas2 strain. Loss of mating activity correlated with the increased 2 expression in the asf1 sir1 deletion strain (Figure 5).
Figure 5 ASF1 and SAS2 function in the same pathway in HML silencing. Disruption of ASF1 in combination with a null allele of SIR1, but not of SAS2, derepressed 2 expression. RNA from either wild-type (WT: W303-1b and W303-1a), asf1 (YJW433), asf1sir1 (YJW435) or asf1sas2 (YJW436) was hybridized by northern blotting to a probe specific for either the 2 or SCR1 gene. A qualitative mating assay was performed by patches, which were replica-plated to a lawn of cells.
Loss of ASF1 disrupts the recruitment of the SAS complex to the HML locus
We showed that SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoters in the HML locus (Figure 4). Next, we investigated whether ASF1 is required for Sas2p–Myc recruitment. Loss of ASF1 markedly decreased Sas2p association with the HML locus (Figure 6A). This decrease was restored by a plasmid carrying ASF1 (compare lanes 3 and 4). In a sir1 mutant, the effect of ASF1 on the Sas2p recruitment was the same as for the SIR1 wild-type strain. These results indicate that ASF1, but not SIR1, is required for the recruitment of Sas2p to the HML locus. Sas2p expression levels in whole-cell extracts from wild-type, asf1, and asf1sir1 strains were indistinguishable, and disruption of ASF1 did not affect the size of the SAS complex (Figure 6A and B). These data indicate that loss of the association of Sas2p with the HML locus in the asf1 mutants is not due to a decrease in Sas2p expression or disruption of the SAS complex.
Figure 6 Sas2 occupancy at the HML region is dependent on ASF1. (A) Chromatin was prepared from the Sas2p–Myc-expressing strains containing either an empty vector or a CEN-based ASF1 plasmid expressed from its own promoter. Strains for the ChIP assay (ordered from left to right) were YSM112, YSM113, YSM114, YSM115, YSM116 and YSM117. Results are shown as in Figure 3B. (B) Comparison of the Sas2p–Myc elution profiles from Superdex 200 size exclusion chromatography after fractionation of whole-cell extracts prepared from wild-type (YJW265) and asf1 (YSM87) mutant strains. Shown are western blots of column fractions probed with the anti-Myc antibody.
DISCUSSION
Deletion of SIR1 in combination with a null allele of either SAS2 or ASF1 causes a much more severe silencing defect at HML than does deletion of either gene alone (11), but the role of these factors in silencing was unclear. We showed that the combination of mutation of SAS2 with SIR1 induced derepression of 2 expression and changed the precisely positioned nucleosome that includes the transcriptional initiation site of the 2, and that the HAT activity of Sas2p is critical for this effect. Furthermore, ChIP assays revealed specific association of the SAS complex with the HML locus, and the SAS complex recruitment required ASF1 but not SIR1 and SIR2.
The effect of the disruption of SAS2 on silencing is different among loci. For example, normal HMRa silencing is unaffected by SAS2 deletion, but sas2 mutations suppress the silencing defect caused by mutation in the silencer elements of HMRa (10,17). Deletion of SAS2 leads to loss of hyperacetylation of histone H4 at lysine 16 in regions adjacent to telomeres. This results in the spreading of Sir3p away from the telomeres into these sub-telomeric regions, leading to repression of gene expression in the sub-telomeric region (15,16). However, deletion of SAS2 causes the loss of silencing at the telomeres themselves, presumably because of titration of Sir proteins away from this locus.
In present study, Sas2p was found to be associated with the HML locus, and Sir2p was not required for this Sas2p association. Disruption of SAS2 increased the spreading of Sir proteins to the sub-telomeric region (15,16). Deletion of SAS2 in sir1 mutants also led to the spreading of the finite number of Sir2p molecules into sub-telomeric regions and resulted in a decrease in Sir2p occupancy at the HML locus. We also showed that the Sas2p HAT activity is essential for 2 repression. Acetylation of lysine 16 of histone H4 might be a landmark for Sir2p assembly: once lysine 16 of histone H4 is acetylated by Sas2p, Sir2p recognizes and deacetylates that residue in the silenced domain and is held in this region. Sas2p might contribute to regulating the histone H4 lysine 16 acetylation state at the chromosome level as well as at the locus level. Deletion of ASF1 likely would bring about the same phenomenon, because we found that Sas2p occupancy at the HML locus was dependent on ASF1. Other investigators have shown that the association of Sir proteins at the HML silencer is somewhat reduced in sir1-mutant cells (29). The deletion of SIR1 in combination with null alleles of either SAS2 or ASF1 may decrease the association of Sir proteins to a much greater extent than that seen after deletion of SIR1 only, thereby causing a much more severe silencing defect at HML than that seen after deletion of either gene alone.
We previously showed that Sas4p, one of the subunits of the SAS complex, directly interacts with Asf1p (11). Therefore, recruitment of the SAS complex to the HML region might require physical interaction with Asf1p. In the present study, we found that the SAS complex is associated with the HML region, but not the ACT1 promoter. However, Moshkin et al. (30) showed that Drosophila Asf1 associated with multiple sites, including heterochromatic and transcriptionally active regions. Furthermore, asf1 mutants are defective in the repression of histone gene transcription during the cell cycle and in cells arrested in the early S phase (31). Finally, Asf1 interacts with bromodomain-containing subunits of TFIID and the Brahma complex, a member of the SWI/SNF ATP-utilizing chromatin-remodeling factors (30,32). These results indicate that ASF1 affects transcriptional control through a variety of mechanisms. The estimated numbers of Asf1p and Sas4p molecules per yeast cell are 6230 and 768, respectively (33). This distribution suggests that the SAS complex interacts with a subset of Asf1 proteins. The mechanism of the recruitment specificity of the SAS complex is still unknown. HML binding factors other than Sir proteins may enhance the SAS complex association with the HML locus. Alternatively, Asf1p-associated factors that selectively bind to Asf1p within transcriptionally active regions may inhibit the interaction between the SAS complex and Asf1p. To address this possibility, we are purifying the factors that interact with the SAS complex and Asf1p.
ACKNOWLEDGEMENTS
The authors gratefully acknowledge Drs Xi Wang and Robert Simpson (Pennsylvania State University) for assistance in establishing the chromatin mapping methods in our laboratory. The authors thank Drs Jerry Workman, Ann Sutton, Rolf Sternglanz, David Rivier and Peter Philippsen for kindly providing yeast strains and plasmids. The authors also thank Drs Ann Sutton, LeAnn Howe and Jerry Workman for critical reading of the manuscript and for advice in designing experiments. The authors thank the staff of the Radioisotope Research Center, Osaka University, and the Central Laboratory for Research and Education, Osaka University Medical School. This research was supported in part by grants from the Japanese Ministry of Education, Culture, Sports, Science and Technology (MEXT), the NISSAN Science Foundation, the Inamori Foundation and the Sasakawa Scientific Research Grant from the Japan Science Society. Funding to pay the Open Access publication charges for this article was provided by MEXT.
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*To whom correspondence should be addressed. Tel: +81 6 6879 8242; Fax: +81 6 6879 8244; Email: osada@phs.osaka-u.ac.jp
ABSTRACT
Transcriptional repression of the silent mating-type loci HML and HMRa in Saccharomyces cerevisiae is regulated by chromatin structure. Sas2p is a catalytic subunit of the SAS histone acetyltransferase (HAT) complex. Although many HATs seem to relieve chromosomal repression to facilitate transcriptional activation, sas mutant phenotypes include loss of SIR1-dependent silencing of HML. To gain insight into the mechanism of the SAS complex mediated silencing at HML, we investigated the expression and chromatin structure of the 2 gene in the HML locus. We found that deletion of SAS2 in combination with a null allele of SIR1 changed the chromatin structure of the precisely positioned nucleosome, which includes the mRNA start site of the 2 gene and derepressed 2 transcription. The Sas2p HAT domain was required for this silencing. Furthermore, chromatin immunoprecipitation analysis revealed that the SAS complex was associated with the HML locus, and ASF1 (which encodes chromatin assembly factor Asf1p), but not SIR1 and SIR2, was necessary for this localization. These data suggest that the HAT activity and ASF1-dependent localization of the SAS complex are required for SIR1-dependent HML silencing.
INTRODUCTION
Silencing affects gene repression in a regional rather than promoter- or sequence-specific manner (1). The structure of the chromatin itself can affect gene expression, and changes in chromatin structure can result from the modification of histone tails as well as from the action of chromatin-remodeling complexes (2). A number of factors have been identified that contribute to transcriptional regulation by covalent modification of histones. In many cases, a relationship between histone acetylation and gene activation has been revealed by the identification of transcriptional co-activators, such as dedicated histone acetyltransferases (HATs) (3,4). Histone acetylation is reversed by histone deacetylases (HDACs), and many repression phenomena are regulated by HDACs (5). Moreover, HATs have been shown to contribute to repression and activation (4).
In Saccharomyces cerevisiae, silenced loci include the HML and HMRa mating-type loci, the telomere regions and the ribosomal DNA repeats (2). A variety of proteins, including the silent information regulator (Sir) proteins, are required to silence the mating information genes at silent loci (6). One of the Sir proteins, Sir2p, possesses HDAC activity important for silencing (7,8). Disruption of the SIR2, SIR3 or SIR4 gene results in loss of silencing at HM loci, and a SIR1-disrupted strain is composed of mixed populations of silenced and unsilenced cells (9).
Something About Silencing (SAS) 2 was identified as an enhancer of sir1 epigenetic HML silencing defects (10). Sas2p is a member of the MYST (MOZ, Ybf2/Sas3, Sas2 and TIP60) family of HATs and forms a complex, termed the SAS complex, with Sas4p and Sas5p (11–14). The SAS complex mainly acetylates histone H4 at lysine 16 (12–16). The role of SAS2 in silencing is different for each silenced locus. At HML, deletion of SAS2 has very little effect on silencing. However, deletion of SAS2 combined with deletion of SIR1 causes a severe silencing defect (10,17). Normal HMRa silencing is unaffected by SAS2 deletion, but sas2 mutation suppresses the silencing defect caused by mutations in silencer elements of HMRa (10,17). To determine the role of SAS2 in rDNA silencing, a strain in which the URA3 gene is integrated at the rDNA locus was used. The sas2 deletion strain showed more effective URA3 repression, indicating that the deletion of SAS2 increased rDNA repression (12). In the case of telomeres, loss of SAS2 causes hypoacetylation in adjacent sub-telomeric regions, leading to the recruitment of Sir3p to these regions and inactivation of gene expression (15,16). Therefore, sas2 mutations reduce silencing of HML (when combined with deletion of SIR1) but improve silencing at HMRa when accompanied by a weakened silencer element, hypoacetylated sub-telomeric regions, or the rDNA locus. To understand the differing roles of Sas2p, it is important to investigate the biochemical mechanisms by which these factors regulate gene silencing in each silent locus.
We previously showed that the chromatin assembly factor Asf1p interacts with the SAS complex, and ASF1 and SAS2 genetically function in the same pathway to repress the HML locus (11). In the present study, we show that SAS2 is essential for the organization of the chromatin structure at HML in a sir1 mutant and that ASF1 is required for the recruitment of the SAS complex to the HML locus.
MATERIALS AND METHODS
Yeast strains, plasmids and manipulations
The strains used in this study are listed in Table 1 and were either published previously or were created for this study by using standard yeast manipulations (18,19). Expression plasmids of wild-type and mutant alleles of SAS2 and ASF1 were described previously (11). Mating assays were performed as described previously (11,20).
Table 1 Yeast strains used in this study
RNA blots
A 40 μg aliquot of total RNA prepared from logarithmically growing cells was separated on 1.0% agarose–formaldehyde gels and transferred to Hybond-N+ membranes (Amersham Biosciences, Piscataway, NJ). Specific messages were detected using randomly labeled 2 and SCR1 probes.
High-resolution micrococcal nuclease mapping
Preparation of nuclei was carried out as described previously (21,22). Briefly, nuclei were isolated from yeast cells, which were grown to mid-log phase (OD600 = 1). The nuclear pellet from a 1 liter culture was resuspended in 2.4 ml digestion buffer (10 mM HEPES, pH 7.5, 0.5 mM MgCl2 and 0.05 mM CaCl2). The suspension was divided into 400 μl portions, each of which was digested at 37°C for 10 min by using increasing concentrations (0–16 U/ml) of micrococcal nuclease (MNase; Amersham Biosciences). The reaction was terminated by adding EDTA, and the DNA was purified after treatment with RNase, proteinase K digestion and phenol–chloroform extraction. The purified DNA was resuspended in 0.1x TE (1 mM Tris–HCl, pH 8.0, 0.1 mM EDTA). MNase cleavage sites were detected by multiple rounds of Taq DNA polymerase-based primer extension. The primer (5'-TATGTCTAGTATGCTGGATTTAAACTCAT-3') was end-labeled by T4 polynucleotide kinase. The cycling program was 94°C for 1 min, 53°C for 2 min and 72°C for 2 min for 35 cycles, and was followed by a 10 min chase at 72°C. The products were electrophoresed on a 6% polyacrylamide–8 M urea gel. The gel was dried and used to expose X-ray film. Relative MNase sensitivity was expressed graphically after scanning the autoradiogram and analyzing the scan by the NIH Image program (version 1.62).
Chromatin immunoprecipitation assay
The chromatin immunoprecipitation (ChIP) assay was performed essentially as described previously (23,24). A 50 ml culture of yeast (OD600 = 1) was treated with formaldehyde (final concentration of 1%) for 30 min at 20°C, and 2.5 ml of 2 M glycine was added to stop the cross-linking reaction. Cells were harvested and disrupted by vortexing in the presence of glass beads, and the lysate was sonicated to generate DNA fragments that ranged in size from 200 to 800 bp. To immunoprecipitate Myc-tagged proteins and Sir2p, we incubated anti-Myc antibody (9E10, Roche, Indianapolis, IN) and anti-Sir2p antibody (Santa Cruz Biotech., Santa Cruz, CA), respectively, with the extract overnight at 4°C, and the extract–antibody mixture then was incubated for an additional 3–4 h with protein G Sepharose beads (Amersham Biosciences). In some experiments, Myc-blocking peptide (Roche, final concentration 313 μg/ml) was added. Immunoprecipitates were washed with 1 ml each of lysis buffer (50 mM HEPES, pH 7.5, 140 mM NaCl, 1 mM EDTA, 1% Triton X-100, 0.1% sodium deoxycholate, 1 mM phenylmethylsulfonyl fluoride, 1 μg/ml leupeptin and 1 μg/ml pepstatin A), lysis buffer supplemented with 250 mM NaCl (for Myc-tagged Sas proteins) or 500 mM NaCl (for Sir2p), LiCl–detergent wash buffer (250 mM LiCl, 10 mM Tris–HCl, pH 8.0, 1 mM EDTA, 0.5% NP-40 and 0.5% sodium deoxycholate) and TE. DNA was eluted with elution buffer (50 mM Tris–HCl, pH 8.0, 10 mM EDTA and 1% SDS). After reversal of the formaldehyde-induced cross-links, 1/5000 of input DNA and 1/45 of each immunoprecipitated DNA were used as templates for amplification by PCR. The sequences of primers for PCR were as follows: for the HML region, 5 '-ATGCTCAGCTAGACGTTTTTCTTTC-3' and 5'-TATGTCTAGTATGCTGGATTTAAACTCAT-3'; for the ACT1 promoter region, 5'-CTTTTTCTTCCACGTCCTCTTGC-3' and 5'-TGGGATGGTGCAAGCGC-3'; and for the sub-telomeric chromatin at 7.5 kb from the end of chromosome VI, 5'-TCATGGTCTTGACAACTTTATGCG-3' and 5'-TATCTGACGTGAAAGTTCAGCGC-3'. Amplification was performed in a 20 μl reaction volume. The number of PCR cycles yielding product within the linear range was determined by analysis of 2-fold serial dilutions of the starting materials, and PCR products were separated on a 6% polyacrylamide gel and were detected by autoradiography. For quantitative analysis, 0.025 μl of dCTP (110 TBq/mmol; Amersham Biosciences) was added to the PCR. After electrophoresis, the gel was dried, and the radioactivity corresponding to a specific band was measured by a bioimage analyzer (model BAS 1800II, Fuji Film, Tokyo, Japan).
Determination of the molecular size of the SAS-containing complex
Whole-cell extracts were prepared as described previously (11,25). Approximately 0.4 mg of each whole-cell extract was loaded onto a 2.4 ml Superdex 200 PC 3.2/30 column (Amersham Biosciences) that had been equilibrated in buffer containing 50 mM Tris–HCl, pH 8.0, 500 mM NaCl, 10% glycerol, 0.1% Tween-20, 1 mM phenylmethylsulfonyl fluoride, 0.5 μg/ml leupeptin and 0.5 μg/ml pepstatin A. A 10 μl aliquot of each fraction was electrophoresed in an SDS–polyacrylamide gel, transferred to nitrocellulose membrane and detected with the ECL western blotting analysis detection system (Amersham Biosciences). Anti-Myc antibody (9E10, Roche) was used.
RESULTS
HML2 was derepressed in a sas2 sir1-deleted strain
The 2 protein, which is a repressor of transcription of a-specific genes, is encoded by MAT and an essential factor for the regulation of mating-type-specific genes in cells (26). The silent information is also stored at the HML locus in both a and cells. Previous work showed that the deletion of either SIR1 or SAS2 results in a very slight reduction of mating activity in a MATa strain, as indicated by quantitative mating analysis. The combined deletion of SIR1 and SAS2 strain causes a much more severe mating defect than that of the wild-type strain or the single-deletion strains (10,11). To show that the double deletion of SAS2 and SIR1 directly affects silencing at HML, we performed northern blotting analysis to detect the level of 2 mRNA in wild-type and deletion strains. 2 was transcribed not only in MAT cells but also in sir4 and sas2sir1 MATa cells (Figure 1A).
Figure 1 Deletion of SAS2 and SIR1 in a MATa strain leads to derepression of HML2 expression and a non-mating. (A) RNA from either wild-type (WT, W303-1b and W303-1a), sir4 (YJW257), sir1 (YJW252), sas2 (YJW253) or sas2sir1 (YJW258) strains was hybridized by northern blotting to a probe specific for either the 2 or SCR1 gene. RNA loading was standardized to SCR1. A qualitative mating assay was performed by patches, which were replica-plated to a lawn of MAT cells. WT and mutant strains are presented at the top of the panel. (B) A sas2sir1 double-deletion strain was transformed with a plasmid carrying the WT or a mutant form of the SAS2 gene (M1) under the control of its own promoter. Strains analyzed (ordered from left to right) were YSM119, YSM118, YSM120, YSM121, YSM122 and YSM123.
We previously showed that wild-type SAS2, but not SAS2 with a mutation in the conserved HAT domain, could restore the mating activity of the sas2sir1 strain. Furthermore, this mutation of amino acids 219–221 (GLG) to alanine residues (termed SAS2-M1) abolished the HAT activity of Sas2p but did not affect the formation of the SAS complex (11,13). To determine whether Sas2p HAT activity is required for the repression of 2 expression, wild-type and mutant SAS2 alleles were transformed into the sas2sir1 strain (Figure 1B). The mating activity and RNA level of 2 in the sir1 mutant were the same as those of the sas2 sir1 double-deletion strain carrying the wild-type SAS2 expression plasmid (Figure 1B, compare lanes 3 and 5). SAS2-M1 failed to restore mating activity and 2 repression to the sas2 sir1 double-mutant strain (Figure 1B, compare lanes 4 and 6). These results suggest that the Sas2p HAT activity is required for the repression of 2 expression from HML in a sir1 mutant.
A strain with deletions of SIR1 and SAS2 shows loss of nucleosome organization at HML
The unique and highly organized chromatin structure of HML has been determined by high-resolution chromatin mapping analysis using MNase, which preferentially cuts the linker DNA between nucleosomes (27). Although a precisely positioned nucleosome (NUC2) covers the transcription start site of the 2 gene at the HML locus, the promoter region of the 2 gene is nucleosome-free . We used MNase mapping to examine the effect of sas2 mutations on the chromatin structure of HML. Deletion of SIR4, which is essential for HML silencing, resulted in increased nuclease sensitivity of one site, indicated by the arrow, compared with that of the wild type (Figure 2A, compare lanes 6–8 with lanes 10–12). Although we used downstream and reverse-strand primers in the attempt to visualize the positioning of NUC2 clearly, we failed to obtain sufficient quantities of primer-extension products. For easy comparison of the MNase sensitivity, the lane treated with the highest concentration of MNase was selected for scanning (Figure 2A, lanes 8, 12, 16, 20 and 24). Relative MNase sensitivity is shown in Figure 2B after scanning and analyzing with the NIH Image software. The intensity of the induced sensitivity of the site highlighted in Figure 2A is the same in sas2 sir1 double-deleted cells as in SIR4-deleted cells (compare lanes 10–12 with lanes 22–24) and stronger than that of wild-type or singly deleted strains (compare lanes 6–8, 14–16 and 18–20 with lanes 22–24). The MNase sensitivity of this site in different mutants correlates inversely with their mating activity and directly with the level of 2 mRNA (Figure 1A). These results suggest that SAS2 is essential for the organization of the nucleosome precisely positioned over the transcriptional initiation site of the 2 in a sir1-mutant strain.
Figure 2 High-resolution MNase mapping of the promoter region of the 2 gene at the HML locus. (A) The chromatin structure of the Crick strand was mapped by primer-extension analysis of MNase-digested sites with the primer located at the coding region of the 2 gene. Strains used were as in Figure 1A. Extensions of undigested (0) and dose-dependent-digested chromatin are indicated. The ‘n’ lane shows the naked DNA digested with MNase (lane 25). The G, A, T and C columns indicate dideoxynucleotide-terminated sequencing reactions (lanes 1–4). The ellipse corresponds to the inferred position of the nucleosome, and boxes show the positions of the TATA-box and UAS regions. Arrow indicates sites in the 2 gene whose nuclease-sensitivity was increased in mutants relative to WT. The vertical bar indicates the region used for scanning to express the relative intensity in Figure 2B. (B) The relative MNase sensitivity expressed graphically after scanning and analyzing the autoradiogram in (A) by using NIH Image 1.62 software. Increased levels of nuclease-sensitive sites of the 2 gene in mutants (sir4 and sas2sir1) relative to WT are indicated by arrows. The position from the transcription start site is shown at the bottom of each panel.
Interestingly, the nuclease sensitivity of the region between the UAS and TATA-box regions was decreased in sas2sir1 and sir4 strains. This region is generally less nuclease sensitive at MAT than at HML (27), and it is thought that in 2-positive cells, the protection of this region in chromatin from the nuclease might result from an association of transcription factors, including Rap1p, which bind to UAS (27). Overall, chromatin in this region is less accessible to nuclease in sas2sir1 strain than in wild-type strains.
The SAS complex associates with the HML locus
Genetic experiments revealed that combining the null allele of SIR1 with that of SAS2, SAS4, SAS5 or ASF1 results in the reduction of silencing at HML (11,17). Meijsing and Ehrenhofer-Murray (12) reported that Sas2p is physically present at the rDNA locus, but not ACT1. To determine whether Sas2p or the SAS complex is located at the HML locus, we performed ChIP analysis using strains expressing Sas2p–Myc. Immunoprecipitated DNA was amplified by PCR with a primer pair spanning the 1 and 2 promoter regions in the HML locus (Figure 3A). We used ACT1, a gene whose transcription is not regulated by SAS2, as a negative control, because the ACT1 mRNA level in the sas2 mutant was same as that in the wild-type strain (15). Two-fold serial dilutions of the input and the immunoprecipitated DNA were performed to verify that the amount of PCR product was dependent on the starting material. Input DNA also was used as a template to confirm that these regions were amplified equally by PCR. In a SAS2–Myc strain, Sas2p–Myc associated with the promoter regions of the 1 and 2 in the HML region relative to ACT1 (Figure 3A). This association was completely competed by adding a Myc-blocking peptide (compare lanes 11 and 12 with lanes 13 and 14).
Figure 3 The SAS complex occupancy at the promoter in the HML locus. (A) Association of Sas2p with the HML region is detected by the ChIP assay. Sonicated chromatin was prepared from wild-type (WT) and Sas2p–Myc-expressing (YJW265) strains. Immunoprecipitation was carried out using monoclonal antibodies to the Myc tag (lanes 3–6 and 11–14), and normal IgG was used as a negative control (lanes 7, 8, 15 and 16). Myc-blocking peptide was added in some immunoprecipitation experiments (lanes 5, 6, 13 and 14). Input and immunoprecipitated DNA were amplified by PCR using primer pairs spanning the promoter region of 1 and 2 genes or ACT1. PCR products were resolved on a 6% polyacrylamide gel and visualized by autoradiography. (B) Localization of subunits of the SAS complex to the promoter of the 1 and 2 genes. Soluble chromatin was prepared from the strains that expressed the C-terminal Myc epitope-tagged Sas2p (YJW265), Sas4p (YJW228) or Sas5p (YJW229), and immunoprecipitated with or without anti-Myc antibody. Final DNA extractions were amplified with dCTP. The PCR product was separated on the polyacrylamide gel and quantitated with a bioimage analyzer after drying the gel. ChIP efficiency is reported as a percentage of immunoprecipitated material (top panel). Data are presented as the mean ± SD from three independent experiments. Input DNA (input) was equally amplified by PCR in WT and Sas2p–Myc-expressing strains. Myc-tagged proteins were detected by western blotting (bottom panel). (C) SAS4 or SAS5 or both are required for the recruitment Sas2p to the HML locus. ChIP assay was performed with chromatin prepared from sas4 (YJW269), sas5 (YJW270) and sas4sas5 (YJW271) strains that expressed the C-terminal Myc epitope-tagged Sas2p. Results are shown as in Figure 3B.
We previously purified a complex containing Sas2p and showed that Sas4p and Sas5p were components of this complex, termed the SAS complex (11,13,14). We next asked whether Sas4p and Sas5p associate with the HML locus. ChIP analyses using SAS4–Myc and SAS5–Myc revealed that Sas4p–Myc and Sas5p–Myc were recruited together with Sas2p–Myc to the promoter regions of the 1 and 2 in the HML region (Figure 3B). This finding supports the possibility that these Sas proteins associate with chromatin as a complex. Accordingly, deletion of either SAS4 or SAS5 might disrupt the association of Sas2p with the HML locus.
To evaluate whether this disruption occurs, we performed ChIP using cells expressing Sas2p–Myc and deleted for SAS4, SAS5 or both genes (Figure 3C). The amount of amplified PCR products from the three deletion strains was markedly lower than from the wild-type strain, although Sas2p–Myc was expressed efficiently in all of the SAS2–Myc strains. These results show that mutations in SAS5 and especially SAS4 inhibit the association of Sas2p–Myc with the promoter regions of the 1 and 2 in the HML region and that Sas2p–Myc was recruited to this region as a component of the SAS complex.
SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoters in the HML locus
Four Sir proteins localize to HML and HMRa and are important for silencing. Sir1p binds to Orc1p, one of the silencer binding proteins, and helps to recruit Sir4p. Sir2p, Sir3p and Sir4p form a complex and spread in both directions from the silencers (1,28). A physical interaction between Sas and Sir proteins has not been reported, although all of them localize to the HML locus. To understand the role of the Sir proteins in the association of Sas2p with the HML locus, we first asked whether loss of Sir1p or Sir2p results in disruption of this association. To do this, Sas2p was tagged with Myc in SIR1 or SIR2 deletion strains. Western blot analysis revealed that Sas2p–Myc was expressed efficiently in both SIR1 and SIR2 deletion strains (Figure 4A). We prepared chromatin fractions from these strains and subjected them to ChIP analysis for the Myc epitope. As shown previously, Sas2p–Myc associated with the HML region in wild-type cells. Loss of SIR1 or SIR2 did not affect this association (Figure 4A). This finding indicates that SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoters in the HML locus.
Figure 4 (A) SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoter in the HML locus. ChIP assay was performed with chromatin prepared from sir1 (YSM85) and sir2 (YSM90) strains that expressed the C-terminal Myc epitope-tagged Sas2p. (B) Effect of deletion of SAS2 and SIR genes on the Sir2p occupancy. Soluble chromatin was prepared from wild-type and deletion strains, and immunoprecipitated with or without anti-Sir2p antibody. Strains analyzed (ordered from left to right) were W303-1a, sas2 (YJW253), sas2sir1 (YJW258), sir1 (YJW252), sir2 (YSM64) and sir3 (YS480). Results are shown as in Figure 3B.
Disruption of SAS2 in a wild-type strain increased the spreading of Sir proteins to the sub-telomeric region (15,16). Deletion of SAS2 in a sir1 mutant also may lead to spreading of the finite number of Sir2p molecules into sub-telomeric regions, resulting in a decrease in Sir2p occupancy at the HML locus. To test this hypothesis, we asked whether loss of SAS2 results in increased or decreased Sir2p association. We observed localization of Sir2p in the regions of the HML locus and sub-telomeric chromatin 7.5 kb from the end of chromosome VI in the wild-type and deletion strains (Figure 4B). Consistent with previous observations, the Sir2p association detected within the HML locus and sub-telomeric regions in the wild-type strain was greater than that in a sir2 deletion strain (Figure 4B, compare lanes 1 and 5) and was slightly increased in the sub-telomeric region by SAS2 deletion (16,29). Interestingly, although Sir2p was expressed efficiently in all of the strains except a sir2 deletion strain, the disruption of SAS2 or SIR1 decreased the amount of Sir2p localization at the HML locus (Figure 4B). In the combination of SAS2 deletion with the null allele of SIR1, the Sir2p association at the HML locus was completely lost, similar to that in the SIR2 and SIR3 deletion strains. This indicates that although Sas2p association at the HML locus does not require SIR1 or SIR2, Sir2p localization is partially dependent on SAS2.
2 expression in the asf1 sir1 deletion strain
We and others (11,12) previously showed that the SAS complex physically interacts with Asf1p and these factors function in a pathway that enhances the epigenetic silencing defects of sir1 mutants. To learn more about the function of ASF1 in the HML silencing, we measured the expression of 2 in an ASF1 deletion strain (Figure 5). Deletion of ASF1 results in a very slight reduction in silencing at HML as indicated by quantitative mating analysis (11), and the 2 mRNA level in the asf1 mutant was indistinguishable from that of the wild-type strain. We previously showed that the combined deletion of ASF1 and SIR1 caused much more severe silencing defects at HML than does the deletion of ASF1 alone (11). Derepression of 2 repression occurred in the asf1 sir1 double-deletion strain but not in the asf1sas2 strain. Loss of mating activity correlated with the increased 2 expression in the asf1 sir1 deletion strain (Figure 5).
Figure 5 ASF1 and SAS2 function in the same pathway in HML silencing. Disruption of ASF1 in combination with a null allele of SIR1, but not of SAS2, derepressed 2 expression. RNA from either wild-type (WT: W303-1b and W303-1a), asf1 (YJW433), asf1sir1 (YJW435) or asf1sas2 (YJW436) was hybridized by northern blotting to a probe specific for either the 2 or SCR1 gene. A qualitative mating assay was performed by patches, which were replica-plated to a lawn of cells.
Loss of ASF1 disrupts the recruitment of the SAS complex to the HML locus
We showed that SIR1 and SIR2 are not required for the recruitment of Sas2p to the promoters in the HML locus (Figure 4). Next, we investigated whether ASF1 is required for Sas2p–Myc recruitment. Loss of ASF1 markedly decreased Sas2p association with the HML locus (Figure 6A). This decrease was restored by a plasmid carrying ASF1 (compare lanes 3 and 4). In a sir1 mutant, the effect of ASF1 on the Sas2p recruitment was the same as for the SIR1 wild-type strain. These results indicate that ASF1, but not SIR1, is required for the recruitment of Sas2p to the HML locus. Sas2p expression levels in whole-cell extracts from wild-type, asf1, and asf1sir1 strains were indistinguishable, and disruption of ASF1 did not affect the size of the SAS complex (Figure 6A and B). These data indicate that loss of the association of Sas2p with the HML locus in the asf1 mutants is not due to a decrease in Sas2p expression or disruption of the SAS complex.
Figure 6 Sas2 occupancy at the HML region is dependent on ASF1. (A) Chromatin was prepared from the Sas2p–Myc-expressing strains containing either an empty vector or a CEN-based ASF1 plasmid expressed from its own promoter. Strains for the ChIP assay (ordered from left to right) were YSM112, YSM113, YSM114, YSM115, YSM116 and YSM117. Results are shown as in Figure 3B. (B) Comparison of the Sas2p–Myc elution profiles from Superdex 200 size exclusion chromatography after fractionation of whole-cell extracts prepared from wild-type (YJW265) and asf1 (YSM87) mutant strains. Shown are western blots of column fractions probed with the anti-Myc antibody.
DISCUSSION
Deletion of SIR1 in combination with a null allele of either SAS2 or ASF1 causes a much more severe silencing defect at HML than does deletion of either gene alone (11), but the role of these factors in silencing was unclear. We showed that the combination of mutation of SAS2 with SIR1 induced derepression of 2 expression and changed the precisely positioned nucleosome that includes the transcriptional initiation site of the 2, and that the HAT activity of Sas2p is critical for this effect. Furthermore, ChIP assays revealed specific association of the SAS complex with the HML locus, and the SAS complex recruitment required ASF1 but not SIR1 and SIR2.
The effect of the disruption of SAS2 on silencing is different among loci. For example, normal HMRa silencing is unaffected by SAS2 deletion, but sas2 mutations suppress the silencing defect caused by mutation in the silencer elements of HMRa (10,17). Deletion of SAS2 leads to loss of hyperacetylation of histone H4 at lysine 16 in regions adjacent to telomeres. This results in the spreading of Sir3p away from the telomeres into these sub-telomeric regions, leading to repression of gene expression in the sub-telomeric region (15,16). However, deletion of SAS2 causes the loss of silencing at the telomeres themselves, presumably because of titration of Sir proteins away from this locus.
In present study, Sas2p was found to be associated with the HML locus, and Sir2p was not required for this Sas2p association. Disruption of SAS2 increased the spreading of Sir proteins to the sub-telomeric region (15,16). Deletion of SAS2 in sir1 mutants also led to the spreading of the finite number of Sir2p molecules into sub-telomeric regions and resulted in a decrease in Sir2p occupancy at the HML locus. We also showed that the Sas2p HAT activity is essential for 2 repression. Acetylation of lysine 16 of histone H4 might be a landmark for Sir2p assembly: once lysine 16 of histone H4 is acetylated by Sas2p, Sir2p recognizes and deacetylates that residue in the silenced domain and is held in this region. Sas2p might contribute to regulating the histone H4 lysine 16 acetylation state at the chromosome level as well as at the locus level. Deletion of ASF1 likely would bring about the same phenomenon, because we found that Sas2p occupancy at the HML locus was dependent on ASF1. Other investigators have shown that the association of Sir proteins at the HML silencer is somewhat reduced in sir1-mutant cells (29). The deletion of SIR1 in combination with null alleles of either SAS2 or ASF1 may decrease the association of Sir proteins to a much greater extent than that seen after deletion of SIR1 only, thereby causing a much more severe silencing defect at HML than that seen after deletion of either gene alone.
We previously showed that Sas4p, one of the subunits of the SAS complex, directly interacts with Asf1p (11). Therefore, recruitment of the SAS complex to the HML region might require physical interaction with Asf1p. In the present study, we found that the SAS complex is associated with the HML region, but not the ACT1 promoter. However, Moshkin et al. (30) showed that Drosophila Asf1 associated with multiple sites, including heterochromatic and transcriptionally active regions. Furthermore, asf1 mutants are defective in the repression of histone gene transcription during the cell cycle and in cells arrested in the early S phase (31). Finally, Asf1 interacts with bromodomain-containing subunits of TFIID and the Brahma complex, a member of the SWI/SNF ATP-utilizing chromatin-remodeling factors (30,32). These results indicate that ASF1 affects transcriptional control through a variety of mechanisms. The estimated numbers of Asf1p and Sas4p molecules per yeast cell are 6230 and 768, respectively (33). This distribution suggests that the SAS complex interacts with a subset of Asf1 proteins. The mechanism of the recruitment specificity of the SAS complex is still unknown. HML binding factors other than Sir proteins may enhance the SAS complex association with the HML locus. Alternatively, Asf1p-associated factors that selectively bind to Asf1p within transcriptionally active regions may inhibit the interaction between the SAS complex and Asf1p. To address this possibility, we are purifying the factors that interact with the SAS complex and Asf1p.
ACKNOWLEDGEMENTS
The authors gratefully acknowledge Drs Xi Wang and Robert Simpson (Pennsylvania State University) for assistance in establishing the chromatin mapping methods in our laboratory. The authors thank Drs Jerry Workman, Ann Sutton, Rolf Sternglanz, David Rivier and Peter Philippsen for kindly providing yeast strains and plasmids. The authors also thank Drs Ann Sutton, LeAnn Howe and Jerry Workman for critical reading of the manuscript and for advice in designing experiments. The authors thank the staff of the Radioisotope Research Center, Osaka University, and the Central Laboratory for Research and Education, Osaka University Medical School. This research was supported in part by grants from the Japanese Ministry of Education, Culture, Sports, Science and Technology (MEXT), the NISSAN Science Foundation, the Inamori Foundation and the Sasakawa Scientific Research Grant from the Japan Science Society. Funding to pay the Open Access publication charges for this article was provided by MEXT.
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