Abstract
Background
Methylation of lysine 79 on histone H3 by Dot1 is required for maintenance of heterochromatin structure in yeast and humans. However, this histone modification occurs predominantly in euchromatin. Thus, Dot1 affects silencing by indirect mechanisms and does not act by the recruitment model commonly proposed for histone modifications. To better understand the role of H3K79 methylation gene silencing, we investigated the silencing function of Dot1 by genetic suppressor and enhancer analysis and examined the relationship between Dot1 and other global euchromatic histone modifiers.
Result
We determined that loss of H3K79 methylation results in a partial silencing defect that could be bypassed by conditions that promote targeting of Sir proteins to heterochromatin. Furthermore, the silencing defect in strains lacking Dot1 was dependent on methylation of H3K4 by Set1 and histone acetylation by Gcn5, Elp3, and Sas2 in euchromatin. Our study shows that multiple histone modifications associated with euchromatin positively modulate the function of heterochromatin by distinct mechanisms. Genetic interactions between Set1 and Set2 suggested that the H3K36 methyltransferase Set2, unlike most other euchromatic modifiers, negatively affects gene silencing.
Conclusion
Our genetic dissection of Dot1's role in silencing in budding yeast showed that heterochromatin formation is modulated by multiple euchromatic histone modifiers that act by non-overlapping mechanisms. We discuss how euchromatic histone modifiers can make negative as well as positive contributions to gene silencing by competing with heterochromatin proteins within heterochromatin, within euchromatin, and at the boundary between euchromatin and heterochromatin.
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Background
Post-translational modifications of histone proteins influence DNA transactions such as transcription, repair, recombination, and chromosome segregation. Many histone modifications affect local chromatin structure and function by recruitment of effector proteins that specifically recognize a modified state of a given residue [reviewed in [1–4]]. However, several histone modifications seem to act by alternative mechanisms. One such example is methylation of lysine 79 of histone H3 (H3K79) by Dot1. H3K79 methylation is required for heterochromatin formation in yeast and humans [5–10]. Paradoxically, methylation of H3K79 is low or absent from heterochromatic regions and is abundant in euchromatic regions of the genome [5, 7, 11–14]. Furthermore, methylation of H3K79, which causes small local changes of the nucleosome surface [15], negatively affects binding of the heterochromatin protein Sir3 in yeast [16–18]. Therefore, this histone modification most likely affects heterochromatin structure by mechanisms other than direct recruitment of repressive factors. We previously proposed that H3K79 methylation in yeast might act as an anti-binding signal to prevent non-specific binding of silencing proteins in euchromatin, thereby leading to efficient targeting of the limiting silencing proteins to the unmethylated heterochromatic regions of the genome [5, 19].
Heterochromatin in yeast, often referred to as silent chromatin, is found at telomeres, the silent mating type loci (HMLα and HMR a) and the ribosomal DNA repeats. At telomeres and HM loci, DNA elements called silencers recruit the Sir2/3/4 complex, which subsequently spreads along the chromosome to form a silent or heterochromatic domain [reviewed in [20]]. Besides H3K79 methylation, methylation of H3K4 and H3K36, histone acetylation, and deposition of the histone variant Htz1 (H2A.Z) in euchromatin have been shown to affect heterochromatin formation in yeast [reviewed in [20]]. Some euchromatic modifications have been suggested to act by (indirect) global effects, whereas others have been suggested to primarily act (directly) at the boundary between euchromatin and heterochromatin to prevent excessive spreading of the Sir2/3/4 complex. For example, loss of the histone variant Htz1, the H3K36 methyltransferase Set2, or the histone acetyltransferase Sas2 leads to loss of heterochromatin boundaries and excessive spreading at yeast telomeres [21–24], whereas in cells lacking Dot1 or the histone H3K4 methyltransferase Set1, Sir proteins become redistributed throughout the genome [5, 25, 26]. Methylation of H3K4 in euchromatin negatively affects binding of the C-terminus of Sir3, which led to the suggestion that Set1 enhances silencing by a mechanism similar to that of Dot1 [27].
The molecular mechanisms responsible for the different silencing functions of many of the euchromatic histone marks are still largely unknown. Here we used genetic suppressor and enhancer analysis to investigate the role of Dot1 in heterochromatin formation and its connection with several other global histone modifiers (see Table 1). We found that the silencing defect in strains lacking Dot1 was partial and could be suppressed by conditions that promote targeting of the Sir complex to telomeres. These results are in agreement with the proposed function of Dot1 in preventing non-specific binding to euchromatin. We show that Dot1 functions in parallel with the histone methyltransferase Set1 and histone acetyltransferases, suggesting that multiple euchromatic histone modifications promote silencing by non-overlapping mechanisms.
Results
Suppressor analysis of the silencing defect in strains lacking Dot1
Previous studies suggest that H3K79 methylation by Dot1 improves targeting of silencing proteins to heterochromatin by preventing promiscuous interactions of Sir3 within euchromatin [5, 16, 17, 28]. To test this hypothesis we investigated three predictions of this model: 1) loss of telomeric silencing in dot1Δ cells due to redistribution of the Sir proteins can be overcome by increased expression of Sir3, which is present in limiting amounts, 2) loss of telomeric silencing in dot1Δ cells can be suppressed by improving the recruitment of Sir proteins by increasing the strength of the Sir2/3/4-recruiting silencer element, 3) the telomeric silencing defect in dot1Δ cells can be suppressed by increased levels of other active marks that affect Sir protein binding or enhanced by decreased levels of these same marks. Our analyses were carried out in a strain carrying two reporter genes: ADE2 at the right arm of telomere V (VR) produces a color phenotype and URA3 at telomere VIIL provides a sensitive growth phenotype (Figure 1A).
Suppression of the silencing defects of dot1Δ strains. (A) Reporter genes used for telomeric silencing. Cells in which the ADE2 gene is silenced accumulate a red pigment whereas cells that express ADE2 are white. Cells in which URA3 is silenced are resistant to 5-FOA, whereas cells in which URA3 is expressed convert 5-FOA into a toxic product and are sensitive to 5-FOA. (B) Wild-type (WT) and dot1Δ strains were transformed with empty vector (p) or a Sir3 overexpression plasmid (pSir3) and were spotted in 10-fold dilution series on media (YC) with and without 5-FOA. (C) Immunoblot analysis of Sir3 expression in sir3Δ and WT cells, and cells containing the Sir3 overexpression plasmid. Ctrl indicates a non-specific band recognized by the Sir3 antibody that was used as a loading control. (D) Telomeric silencing in WT and dot1Δ strains lacking RIF1 or RPD3; sir2Δ and sir3Δ strains are shown as no-silencing controls (E) mRNA expression levels of ADE2 and URA3 relative to ACT1 were determined by RT-qPCR. mRNA was isolated and quantified in duplicate with the difference as the standard error. (F) Sir3 binding at ADE2-TEL-VR, URA3-TEL-VIIL and 3500 bp from telomere VIR (VIR3500) relative to binding at control locus ACT1 was determined by ChIP combined with real-time qPCR. Each clone was analyzed in duplicate with the difference as the standard error. (G) Silencing in strains lacking DEP1 (Rpd3L complex) or RCO1 (RPD3S complex).
First, Sir3 levels were increased by expression of SIR3 from a multi-copy plasmid. Overexpression of Sir3 partially suppressed the silencing defect of the dot1Δ strain (Figure 1B–C). Thus, Dot1 is not a critical component of heterochromatin. We note that Sir3 overexpression was not toxic for dot1Δ cells (Figure 1B and data not shown) indicating that an increase in Sir3 did not lead to ectopic silencing of essential genes.
Second, silencer function of the telomeric repeats was altered. Recruitment of the Sir2/3/4 complex to telomeres is mediated by the telomere-binding protein Rap1 [reviewed in [20]]. Strains lacking the Rap1-interacting factor Rif1 have longer telomeres, which has been suggested to improve recruitment of Sir proteins to the chromosome ends and thereby enhance silencing [29–32]. When RIF1 was deleted, silencing of the URA3 gene in the dot1Δ strain was partially restored (Figure 1D). Using a different approach, we recently showed that Dot1 becomes critical for silencing of the HMLα locus when the silencer strength at that locus is compromised due to inactivation of Sir1, a silencer-binding protein that facilitates recruitment of the Sir complex to HMLα [33]. We conclude that the contribution of Dot1 to gene silencing depends on strength of the cis silencer element. Unexpectedly, deletion of RIF1 resulted in decreased silencing of the telomeric ADE2 gene in wild-type and dot1Δ cells in multiple independent clones (Figure 1D and data not shown), whereas a previous study using an ADE2 gene at a different telomere showed that deletion of Rif1 made cells more red [32]. Silencing of the ADE2 gene and/or color development in strains with no or low expression of ADE2 is somewhat variable and can depend on media and growth conditions (e.g. see Figure 2A below and compare WT and dot1Δ in Figure 1B with 1D) [34]. This may in part be due to the stochastic nature of ADE2 silencing that is observed in yeast colonies [34]. In general, strains lacking Dot1 showed a modest change in color development on complete synthetic media (Figure 1D and see below). To verify whether the changes in colony color and growth on FOA plates were caused by changes in ADE2 and URA3 expression, respectively, mRNA expression of these genes was determined by reverse-transcriptase combined with quantitative real-time PCR (RT-qPCR). Whereas deletion of Dot1 did not substantially affect ADE2 expression under these conditions, deletion of Rif1 caused derepression of the telomeric ADE2 gene (Figure 1E). The telomeric URA3 gene was derepressed in strains lacking Dot1, and additional deletion of Rif1 partially suppressed the silencing defect. These expression data are in agreement with the color and growth phenotypes of the rif1Δ strains (Figure 1D). To verify whether the changes in silencing were caused by changes in Sir protein targeting, binding of Sir3 to the telomeric reporter genes and to a third telomere was determined by chromatin immunoprecipitation (ChIP) combined with qPCR. As expected, Sir3 binding at all three telomeres was reduced in the dot1Δ strain (Figure 1F). In the rif1Δ and rif1Δdot1Δ strains, Sir3 binding was decreased at ADE2-TEL-VR, unaffected or slightly increased at URA3-TEL-VIIL and increased at TEL-VIR (Figure 1F). These results suggest that although deletion of Rif1 can partially suppress the URA3 silencing defect of dot1Δ cells, the role of Rif1 in silencing is context dependent.
Multiple euchromatic histone modifiers promote gene silencing by redundant mechanisms. (A) Analysis of telomeric silencing at 23, 30, and 37°C. (B-G) Single, double and triple mutants of the indicated genes involved in chromatin modification were analyzed as in Figure 1. dot1Δ strains have a partial silencing defect and are 5-FOA sensitive at 30°C. Cells were spotted at 37°C to partially restore silencing and identify mutants that enhance the partial silencing defect of dot1Δ. Each section represents a different experimental panel.
Third, to test whether additional histone modifications are involved in Sir protein targeting, we investigated the consequences of inactivation of the histone deacetylase (HDAC) Rpd3. Acetylation of lysines in the histone tails negatively affects interactions between Sir3 and Sir4 with histones in vitro [35, 36]. We deleted RPD3 because cells lacking Rpd3 activity show increased global levels of histone acetylation in euchromatin [37–43]. Deletion of RPD3 enhanced silencing of ADE2 in wild-type cells, which is consistent with previous observations [40, 44–47], and suppressed the URA3 silencing defect of the dot1Δ strain (Figure 1D), suggesting that increased acetylation in euchromatin can compensate for the loss of H3K79 methylation. Analysis of URA3 mRNA levels confirmed that deletion of Rpd3 improved transcriptional silencing of telomeric URA3 in wild-type cells and suppressed the silencing defect of dot1Δ cells (Figure 1E). Deletion of Rpd3 also improved silencing of the ADE2 gene but did not improve transcriptional silencing of ADE2 in cells lacking Dot1 (Figure 1E), despite the similar dark red colony color of rpd3Δ and dot1Δrpd3Δ cells. We expect that red color development was near saturation in rpd3Δ and dot1Δrpd3Δ cells due to a combination of partial ADE2 silencing and slow growth of cells lacking Rpd3 and that a small reduction in silencing did not result in a color change in these slow growing cells. To investigate how Rpd3 enhanced silencing, binding of Sir3 was examined by ChIP. In wild-type cells, deletion of Rpd3 led to an increase in Sir3 binding at all three telomeres examined (Figure 1F), which supports the idea that global histone acetylation can promote targeting of Sir proteins to heterochromatin. However, in cells lacking Dot1, loss of Rpd3 did not lead to a detectable increase in Sir3 binding (Figure 1F), suggesting that the suppression of the dot1Δ silencing defect of telomeric URA3 was not caused by restoration of Sir3 binding.
Rpd3 is active in two multi-subunit complexes (see Table 1). The larger Rpd3L complex localizes to promoter regions. The smaller Rpd3S complex is active at transcribed coding regions and is recruited to these regions via the subunits Eaf3 and Rco1, which together bind methylated H3K36, a histone modification co-transcriptionally introduced by Set2 [48–51]. DEP1 deletion, which specifically eliminates the Rpd3L complex, phenocopied deletion of RPD3 (Figure 1G). In contrast, deletion of RCO1, which eliminates the Rpd3S complex, did not affect silencing, showing that the Rpd3L complex and not the Rpd3S promoted gene silencing (Figure 1G). A very recent study identified a third Rpd3 complex, containing Rpd3, Snt2 and Ecm5 [52]. We expect that this complex is not involved in the silencing functions of Rpd3 that we identified here because deletion of ECM5 did not affect silencing (data not shown).
Together, the results shown in Figure 1A–G show that Dot1 modulates the strength of gene silencing and that the loss of this modifier can be compensated for by increased Sir3 dosage, strong silencers, and inactivation of Rpd3, a global HDAC.
Dot1 collaborates with histone acetyltransferases to promote gene silencing
To analyze the genetic relationship between DOT1 and other genes involved in euchromatic histone modification, we analyzed silencing of the reporter genes at different temperatures. Growth at high temperature enhances gene silencing in yeast by unknown mechanisms [33, 53] and was sufficient to suppress the dot1Δ silencing defect (Figure 2A). Perhaps non-specific association of Sir proteins with nucleosomes is decreased at higher temperatures, which improves binding at telomeres. This conditional silencing phenotype provided us with a genetic tool to identify enhancers of the silencing defect in dot1Δ strains. Having found that increased acetylation suppressed the dot1Δ silencing defect (Figure 1D–E), we examined which HAT might be responsible for the acetylation marks that promote gene silencing. We examined the non-essential HATs Elp3 [54], Gcn5 [55–60], Sas3 [61], and Sas2 [62–64], as well as Eaf1 [65], which encodes the only non-essential subunit of the NuA4 HAT complex (Table 1). Analysis of dot1Δ double and triple mutants showed that Elp3, Gcn5, and Sas2 were all required for efficient silencing in dot1Δ cells at high temperature (Figure 2B–F). These findings suggest that Gcn5 and Elp3, which have been shown to affect global levels of histone H3 acetylation [41, 66–68, 68–70], and Sas2, which has been shown to be the major H4K16 acetyltransferase [21, 62] all promote silencing in parallel to histone H3K79 methylation by Dot1. Analysis of sas2Δ in combination with elp3Δ or gcn5Δ showed that each double mutant had more severe silencing defects than either single mutant, suggesting that the three HATs affect silencing by redundant mechanisms (Figure 2E). Loss of Sas3, which affects bulk histone H3 acetylation when combined with loss of Gcn5 [70, 71], did not alter silencing in wild-type or dot1Δ cells (Figure 2C), whereas a single deletion of EAF1 was sufficient to disrupt telomeric silencing (Figure 2F), even at high temperature (Figure 2F). The histone variant Htz1 (H2A.Z), which is acetylated by NuA4 [72, 73] and of which the deposition into chromatin is dependent on Sas2 [74], was not critical for silencing in wild-type or dot1Δ strains (Figure 2G).
Dot1 and Set1 have distinct functions in silencing and cell division
Having found that histone H3K79 methylation and various histone H3 and H4 acetylation events influence heterochromatin by distinct mechanisms, we next investigated the relationship between Dot1 and the H3K4 methyltransferase Set1 and the H3K36 methyltransferase Set2. These enzymes are the only known histone lysine methyltransferases in yeast. Strains lacking Dot1, Set1, or Set2 have no detectable methylation of H3K79, H3K4, and H3K36, respectively. Previous studies showed that histone H3K4 methylation by Set1 and H3K79 methylation by Dot1 may affect silencing by a similar mechanism [7, 27]. Indeed, overexpression of Sir3 has been shown to rescue telomeric silencing defects of a set1Δ strain [27]. Using our silencing reporters, we found that a dot1Δ set1Δ double knock-out strain has more severe silencing defects than either single knock-out strain (Figure 3), showing that they work through different mechanisms. SET2 deletion did not affect silencing of the two reporter genes in wild-type or dot1Δ cells (Figure 3). However, deletion of SET2 partially suppressed the silencing defect caused by deletion of SET1 (Figure 3), suggesting that some aspect of gene silencing is negatively regulated by the presence of Set2. Methylation of H3K36 by Set2 has been shown to lead to recruitment of the Rpd3S complex to coding regions [48–51]. The negative role of Set2 in gene silencing in set1Δ cells (Figure 3) was not mediated by Rpd3S since inactivation of the Rpd3S complex by deletion of RCO1 did not improve silencing in a set1Δ strain (Figure 4A). Deletion of RPD3 or deletion of DEP1, which specifically inactivates the Rpd3L complex, did suppress the silencing defects (Figure 4A), indicating that Set1 modulates gene silencing by a mechanism that acts in parallel with Dot1 as well as histone acetylation. To verify this idea, we deleted GCN5 and ELP3 in the set1Δ strain to determine whether reduced acetylation would enhance the silencing defect caused by loss of Set1 function, as we found for Dot1. We noticed that strains lacking Set1 and either one of the two HATs had severe growth defects, especially at 37°C (data not shown). In certain yeast mutants, growth defects are mediated by the Sir complex, presumably because of ectopic Sir-mediated silencing of genes required for cell growth [23, 75, 76]. These growth defects can be alleviated by deletion of one of the SIR2/3/4 genes. To determine whether the growth defects in set1Δ gcn5 and set1Δ elp3Δ strains were mediated by the Sir complex a diploid strain heterozygous for SET1, GCN5, ELP3, and SIR3 was sporulated to generate isogenic single, double, and triple histone modifier knock-out cells that were either silencing proficient (SIR3) or deficient (sir3Δ) (Figure 4B–C). Tetrad analysis confirmed that haploid spores lacking SET1 require GCN5 and ELP3 for normal growth. Cells lacking all three genes were extremely sick or did not grow at all, indicating that Set1, Gcn5, and Elp3 promote cell division by different mechanisms (Figure 4B–C). Deletion of SIR3 did not alleviate any of the growth defects of set1Δ, elp3Δ and gcn5Δ double and triple knockout strains (Figure 4B–C), which shows that the reduced fitness was not caused by ectopic silencing by the Sir complex.
Histone lysine methyltransferases Dot1, Set1 and Set2 affect silencing by different mechanisms. Telomeric silencing in strains lacking DOT1, SET1, and/or SET2 was analyzed by growth on media with or without 5-FOA, at 30 and 37°C as described in Figure 1.
Silencing and viability of strains lacking Set1 is modulated by histone acetylation. (A) Deletion of RPD3 or DEP1 (Rpd3L complex) suppressed the silencing defects of strains lacking SET1, whereas deletion of RCO1 (Rpd3S complex) had no effect. (B) A diploid strain homozygous for the ADE2 and URA3 silencing reporters and heterozygous for SET1/set1::NatMX, GCN5/gcn5::HphMX, ELP3/elp3::KanMX, and SIR3/sir3::HIS3 was sporulated and spore viability was analyzed by tetrad analysis. Each row indicates the four-spore progeny of one diploid cell. Genotypes and mating type of the individual colonies were determined by replica-plating. Only those tetrads are shown of which the genotype of all four spores could be determined or deduced. The genotype of each colony is indicated by the position of the squares, where white indicates the WT allele and black indicates the mutant allele. (C) Combined deletion of SET1, GCN5, and ELP3 affected cell viability. Colony sizes of panel B (large, small, very small/no colony) were scored for each genotype indicated in SIR3 and sir3Δ backgrounds. (D) Wild type and set1Δ strains were transformed with an empty multi-copy plasmid (p) or a multi-copy plasmid carrying a genomic copy of Dot1 (pDot1) to examine the effect of intermediate levels of Dot1 overexpression on telomeric silencing. (E) Protein levels of Dot1 expressed from its endogenous locus and from the multi-copy plasmid were examined by immunoblot analysis. Pgk1 was used as a loading control and a dot1Δ strain was used as a negative control.
Since the set1Δ silencing defect could be suppressed by increased histone acetylation by inactivation of Rpd3, we asked whether increased activity of Dot1 could also improve silencing and suppress the set1Δ silencing defect. To test this, wild type and set1Δ strains were transformed with a DOT1 multi-copy plasmid (Figure 4D). Under these conditions of Dot1 overexpression (Figure 4E) silencing of the telomeric URA3 gene was unaffected in wild-type strains and not or only slightly improved in set1Δ strains (Figure 4D). We conclude that the endogenous levels of H3K79 methylation are not limiting for silencing.
Sir2 and Sir3 expression in strains with silencing phenotypes
Our results show that heterochromatin function in budding yeast is positively affected by several euchromatic histone modifications and strong silencers. To exclude that phenotypes in the chromatin mutants studied here were caused by altered Sir protein levels we examined the expression of Sir2 and Sir3 by immunoblot analysis. We found that deletion of most of the chromatin modifiers investigated in this study did not affect expression of Sir2 or Sir3 (Figure 5). The immunoblots indicate that expression of Sir2 and Sir3 was reduced in the eaf1Δ strain, which might explain why the silencing defect in this strain could not be suppressed by growth at high temperature (Figure 2F) and why Eaf1 affects gene silencing while no changes have been observed in global levels of histone H4 acetylation [65].
Expression of Sir2 and Sir3 in strains with altered silencing properties. Immunoblot analysis of whole-cell protein extracts using antibodies against Sir2 and Sir3. A Pgk1 antibody was used as a loading control. The specificity of the Sir2 antibody is shown in the left panel. The specificity of the Sir3 antibody was shown previously [33] and is shown in Figure 1.
Discussion
We investigated the role of Dot1 in gene silencing by looking for suppressors and enhancers of silencing defects of a dot1Δ strain. Our results show that Dot1 is not essential for gene silencing but modulates the efficiency of heterochromatin formation. Silencing in dot1Δ strains could be restored by conditions that improve recruitment of the Sir complex: increased Sir3 dosage and stronger silencers. These properties of the dot1Δ strains are compatible with a role for Dot1 in enhancing targeting of Sir proteins to regions of heterochromatin. Silencing in wild-type and dot1Δ strains was dependent on the activity of other histone modifiers; mutations that increase genome-wide histone acetylation enhanced silencing whereas several mutations that reduce histone acetylation or H3K4 methylation reduced silencing. Therefore, H3K79 methylation and other marks of euchromatin positively influence heterochromatin function by different mechanisms (Figure 6). The redundancy of these pro-silencing functions may reflect differences in genomic locations of the various histone marks. For example, Set2 mono-, di-, and tri-methylates H3K36 mainly in coding regions, Set1 generates mono-, di-, and trimethylated H3K4 preferentially in coding sequence, 5' coding sequence, and promoter regions, respectively, and Dot1 mono-, di-, and tri-methylates H3K79 at similar levels throughout the genome. The redundancy may also reflect the fact that the different marks are located on different areas of the nucleosome and thereby affect multiple contacts between the Sir complex and nucleosome arrays. H3K4, H3K36 and most of the acetylated lysines are located on the tails of histone H3 and H4, while H3K79 is located on the nucleosome core surface and might interact with the tail of histone H4. In vitro studies have shown that Sir3 can interact with the histone tails as well as with the nucleosome core and that methylation of H3K4 and H3K79 as well as acetylation of the tail of H3 or H4 can affect Sir-nucleosome interactions. Our genetic studies suggest that binding of the Sir complex to nucleosomes is not affected by post-translational modifications in a combinatorial manner by a specific histone code. Rather, many modifications all seem to make independent contributions to promoting gene silencing. We note that it cannot be excluded at this point that the histone modifying enzymes investigated in this study affect gene silencing by post-translational modification of non-histone proteins or by indirect effects on other histone modifications. For example, Gcn5 acetylates not only histone tails but also other chromatin-associated factors such as Rsc4, a subunit of the RSC nucleosome remodeling complex [68, 77]. In addition, Set1 has been shown to influence histone acetylation [78] and to methylate the kinetochore protein Dam1 [79]. Since Gcn5 is also involved in kinetochore function [80], it is perhaps loss of these functions that caused fitness problems in set1Δgcn5Δ (and set1Δelp3Δ) strains (Figure 4).
Summary of genetic relationships identified in this study. Genetic interactions between Dot1 and other histone modifiers. Grey nodes indicate positive regulators of silencing and black nodes indicate negative regulators of silencing. Grey lines indicate phenotypic enhancement; black lines indicate phenotypic suppression; arrows indicate the directions of the interactions. No silencing phenotypes were observed for SAS3, HTZ1, and RCO1.
Heterochromatin in yeast is characterized by the absence of post-translational modifications of histone proteins and biochemical and genetic studies indicate that binding of Sir proteins to nucleosomes is negatively affected by histone methylation and acetylation. Therefore, heterochromatin formation and spreading seems to be determined by a competition between binding of the Sir complex and action of euchromatic histone modifying enzymes. Competition between histone modifiers and the Sir proteins can in principle affect heterochromatin at three distinct genomic or chromatin locations (Figure 7). First, histone modifiers can compete with Sir proteins within heterochromatin domains. By doing so they are expected to destabilize heterochromatin domains. Indeed, when Sas2 or Dot1 are overexpressed and lead to increased global histone acetylation and methylation, respectively, Sir protein binding and silencing at telomeres is reduced [5, 17, 28, 81]. Furthermore, the presence of Sas2 and Dot1 in yeast cells delays the onset of silencing at a previously active locus [82]. Second, modifying enzymes can deposit an anti-silencing mark at the interface between euchromatin and heterochromatin and thereby form a boundary. By this mechanism, loss of a histone modifying enzyme is expected to lead to increased spreading of heterochromatin into adjacent regions. When excessive spreading occurs of the limiting Sir proteins this may be accompanied by reduced Sir protein binding and impaired silencing of the distal wild-type silenced loci, as has been observed for strains lacking SAS2, BDF1 or GCN5+ELP3 [21, 22, 75, 83]. Third, histone modifications throughout euchromatin can prevent non-specific binding of Sir proteins, which increases the availability of the limiting Sir proteins for heterochromatic regions [19]. By this model, loss of a modifying enzyme is expected to reduce targeting of Sir proteins to heterochromatic areas as well as their flanking regions, as has been described for DOT1 and SET1. In cells lacking Dot1 or Set1, Sir proteins do not spread excessively but become redistributed throughout the genome [5, 25, 26]. Also by this model, higher levels of a global and limiting histone modification are expected to improve targeting, silencing, and ectopic spreading of Sir proteins, in which case the degree of spreading will depend on how the increased mark affects competition within heterochromatin and at the boundary.
A competition model for positive and negative roles of euchromatic histone modifications in heterochromatin formation. Euchromatic histone modifications can have positive roles (arrows) and negative roles (blunt arrows) in heterochromatin formation. Competition between euchromatic histone modifiers and heterochromatin proteins for interactions with nucleosomes can occur at three locations and can have different outcomes (see text). 1) Competition within heterochromatin regions creates a semi-stable epigenetic state. 2) Competition at the interface between euchromatin and heterochromatin prevents local spreading of the Sir complex, thereby on the one hand avoiding ectopic silencing of regions adjacent to heterochromatin and on the other hand ensuring availability of limiting silencing proteins for the endogenous heterochromatic regions. 3) Competition throughout euchromatin prevents non-specific binding of the Sir2/3/4 complex to bulk chromatin, thereby enhancing targeting of Sir proteins to endogenous heterochromatic regions to ensure sufficient spreading of the Sir complex. By these mechanisms, the function of a euchromatic histone modification in gene silencing depends on the relative contribution that it makes to each of these mechanisms and to what extend the negative and positive functions counteract each other.
Our results and previous studies show that multiple euchromatic histone modifiers influence telomeric silencing and here we show that many of them seem to act by non-overlapping mechanisms. How might they affect gene silencing? Deletion of a histone modifier generally does not enhance silencing (e.g. Figures 2, 3 and 4). Therefore, they do not seem to weaken silencing by local competition with heterochromatin formation. Several factors might determine the importance of local competition. For example, euchromatic modifiers might not have access to the nucleosomal substrates in heterochromatin [17, 84], local disruption of silencing by histone modifiers might be counteracted by (indirect) positive silencing effects, or post-translational modification in heterochromatin might be counteracted by histone-demodifying activities such as the HDAC activity of Sir2 and the H2B deubiquitinating activity of UBP10, which is recruited to heterochromatin by Sir4 and negatively affects methylation by Dot1 and Set1 [85, 86]. We expect that Dot1, Set1, Gcn5, Elp3, and Sas2, which we investigated here, act at least in part by long-distance targeting effects because they deposit abundant histone modifications throughout the euchromatic genome and loss of the modifying enzymes leads to reduced silencing. Similarly, based on the phenotypes of rpd3Δ cells i.e. more spreading into flanking regions (Figure 1 and [31]) as well as increased silencing within wild-type heterochromatin regions (Figures 1 and 4), we propose that deletion of RPD3 leads to improved targeting of silencing proteins to heterochromatin domains, which can overrule the local boundary and lead to ectopic spreading. Set2 and Htz1 might act by a similar mechanism. Strains lacking Set2 show increased spreading [87] as well as increased silencing within existing heterochromatin regions in a set1Δ strain (Figure 4) and strains lacking Htz1 show increased spreading [24] without loss of silencing at wild-type heterochromatin loci (Figure 2). These silencing phenotypes suggest that Set2, Htz1, and Rpd3 might not act as local boundary factors, as has been proposed previously [23, 24, 31, 87], but instead affect the degree of spreading from a distance by reducing the targeting efficiency of Sir proteins to heterochromatin. Thus, these factors might set heterochromatin boundaries by weakening Sir-protein targeting to heterochromatin domains.
The mechanism by which Rpd3 weakens silencing is still unclear, however. Whereas increased gene silencing in rpd3Δ cells (Figure 1D+E) was accompanied by increased Sir3 binding (Figure 1F), deletion of Rpd3 in dot1Δ cells restored URA3 silencing without any detectable changes in Sir3 binding (Figure 1D–F). Although Sir3 is the major Sir protein that can spread along the chromosome over long distances, these results suggest that factors other than Sir3 restored silencing in rpd3Δdot1Δ cells. Whether Rpd3 affects binding of one of the other Sir proteins remains to be determined. Changes in silencing without detectable changes in Sir protein binding have been described previously, however [88]. Therefore, it is also possible that Rpd3 might affect the activity of the Sir proteins, such as the deacetylase activity of Sir2, or targeting of repressor proteins that can act as heterochromatin factors but are normally not found in Sir-occupied heterochromatin domains, such as Sum1, Hst1, or Hda1 [89–94]. Interestingly, our results also indicate that the effect of Rpd3 on Sir3 targeting to telomeric heterochromatin requires the presence of Dot1. This suggests that targeting of Sir proteins to heterochromatin by increased histone acetylation might involve simultaneous recognition of methylated H3K79. The redundant roles of Dot1 and the histone H3 HATs Gcn5 and Elp3 in promoting gene silencing indicates that histone H3 acetylation and H3K79 methylation involve non-linked mechanisms. To fully understand the connection between Dot1 and Rpd3, it will be important to determine which of the many target lysines of Rpd3 affect Sir3 targeting in a Dot1-dependent manner and whether Rpd3 and Dot1 affect each others activity.
Conclusion
Targeting of the Sir complex to regions of heterochromatin in yeast is positively modulated by a range of euchromatic factors indicating that euchromatin and heterochromatin are interdependent. Our results and previous studies suggest that histone modifiers can compete with heterochromatin proteins at different locations and thereby make positive as well as negative contributions to heterochromatin formation. We expect that similar rules apply to histone modifications in higher eukaryotes, which might help to explain the paradoxical role of Dot1 in gene activation and repression in flies and mammals [8, 9, 11, 95–98].
Methods
Yeast strains are described in Table 2. Gene knock-outs were made by replacing the coding sequences of the respective genes by homologous recombination with PCR products of plasmids pRS400 (KanMX), pRS40NatMX, pRS40HygMX, or pRS303 (HIS3) [33, 99]. Most gene deletions were generated as heterozygous diploids. Haploids were subsequently obtained by sporulation. For spore analysis of the elp3Δgcn5Δset1Δsir3Δ heterozygous diploid (NKI1121) genotypes of the four spores of each tetrad were determined by drug resistance, histidine prototrophy, and mating to tester strains PT1a and PT2α [34]. Genotypes that could not be determined directly (due to synthetic lethality or due to loss of mating type caused by the absence of Sir3) were deduced from the segregation of the markers in the remaining spores. Only tetrads of which the genotypes of all four spores could be unambiguously assigned were included for further analysis. Yeast media were prepared and silencing assays were performed as previously described [28, 34] and repeated at least two times. Silencing assays were performed with cells that had been pre-grown at the appropriate temperature for at least one day. Plasmids pRS424 (2 μ-TRP1) and pHR67-23 containing a SIR3 genomic region in pRS424 were described previously [33, 99].
Immunoblots
Whole-cell extracts were obtained from approximately 5 × 107 cells by the classical glass beads breakage method using 200 μl of glass beads and SUMEB (1% SDS, 8 M Urea, 10 mM MOPS pH 6.8, 10 mM EDTA, 0.01% bromophenol blue, 1 mM DTT) [100] complemented with PMSF (1 mM), benzamidine (5 mM), pepstatin (1 μg/ml), leupeptin (1 μg/ml) and DTT (1 μM). Primary antibody incubations were performed in Tris-buffered saline-Tween with 2% dry milk. Antibodies used were Sir3 [33], Dot1 [28], Sir2 (Santa Cruz, Sc-6666), and Pgk1 (Invitrogen, A-6457).
Reverse-transcription
Total yeast RNA was prepared from 5 × 107 cells of each of the indicated growth condition using the RNeasy kit (Qiagen) according to the manufacturer's protocol. RNA samples were treated with RNase free DNAse (Qiagen), and cDNA was made by using Super-Script II reverse transcriptase (Invitrogen).
Chromatin immunoprecipitation
ChIP was performed as described previously [101]. Briefly, the chromatin was sheared using a bioruptor (Diagenode) for 6 minutes with 30 seconds intervals at high. The obtained fragments have an average size of 500 bp, as determined on a 2% TAE gel stained with ethidium bromide and quantified using TINA software. The isolated chromatin of the equivalent of 5 × 107 cells was immunoprecipitated overnight at 4°C using magnetic Dynabeads (Invitrogen) which were previously incubated with antibody o/n at 4°C.
Real-time PCR
ChIP DNA and cDNA was quantified by real-time PCR using the SYBR® Green PCR Master Mix (Applied Biosystems) and the ABI PRISM 7500. A ChIP input sample was used to make a standard curve, which was then used to calculate relative IP efficiencies and mRNA expression levels, using the 7500 fast system software. Primers used for qPCR are listed in Table 3.
References
Bhaumik SR, Smith E, Shilatifard A: Covalent modifications of histones during development and disease pathogenesis. Nat Struct Mol Biol. 2007, 14: 1008-1016.
Kouzarides T: Chromatin modifications and their function. Cell. 2007, 128: 693-705.
Taverna SD, Li H, Ruthenburg AJ, Allis CD, Patel DJ: How chromatin-binding modules interpret histone modifications: lessons from professional pocket pickers. Nat Struct Mol Biol. 2007, 14: 1025-1040.
Sims RJ, Reinberg D: Is there a code embedded in proteins that is based on post-translational modifications?. Nat Rev Mol Cell Biol. 2008, 9: 815-820.
van Leeuwen F, Gafken PR, Gottschling DE: Dot1p modulates silencing in yeast by methylation of the nucleosome core. Cell. 2002, 109: 745-756.
Ng HH, Feng Q, Wang H, Erdjument-Bromage H, Tempst P, Zhang Y, Struhl K: Lysine methylation within the globular domain of histone H3 by Dot1 is important for telomeric silencing and Sir protein association. Genes Dev. 2002, 16: 1518-1527.
Ng HH, Ciccone DN, Morshead KB, Oettinger MA, Struhl K: Lysine-79 of histone H3 is hypomethylated at silenced loci in yeast and mammalian cells: a potential mechanism for position-effect variegation. Proc Natl Acad Sci USA. 2003, 100: 1820-1825.
Gazin C, Wajapeyee N, Gobeil S, Virbasius CM, Green MR: An elaborate pathway required for Ras-mediated epigenetic silencing. Nature. 2007, 449: 1073-1077.
Jones B, Su H, Bhat A, Lei H, Bajko J, Hevi S, Baltus GA, Kadam S, Zhai H, Valdez R, et al: The histone H3K79 methyltransferase Dot1L is essential for mammalian development and heterochromatin structure. PLoS Genet. 2008, 4: e1000190-
Lacoste N, Utley RT, Hunter J, Poirier GG, Cote J: Disruptor of telomeric silencing-1 is a chromatin-specific histone H3 methyltransferase. J Biol Chem. 2002, 30: 3-
Krivtsov AV, Feng Z, Lemieux ME, Faber J, Vempati S, Sinha AU, Xia X, Jesneck J, Bracken AP, Silverman LB, et al: H3K79 methylation profiles define murine and human MLL-AF4 leukemias. Cancer Cell. 2008, 14: 355-368.
Barski A, Cuddapah S, Cui K, Roh TY, Schones DE, Wang Z, Wei G, Chepelev I, Zhao K: High-resolution profiling of histone methylations in the human genome. Cell. 2007, 129: 823-837.
Roh TY, Ngau WC, Cui K, Landsman D, Zhao K: High-resolution genome-wide mapping of histone modifications. Nat Biotechnol. 2004, 22: 1013-1016.
Schubeler D, MacAlpine DM, Scalzo D, Wirbelauer C, Kooperberg C, van Leeuwen F, Gottschling DE, O'Neill LP, Turner BM, Delrow J, et al: The histone modification pattern of active genes revealed through genome-wide chromatin analysis of a higher eukaryote. Genes Dev. 2004, 18: 1263-1271.
Lu X, Simon MD, Chodaparambil JV, Hansen JC, Shokat KM, Luger K: The effect of H3K79 dimethylation and H4K20 trimethylation on nucleosome and chromatin structure. Nat Struct Mol Biol. 2008, 15: 1122-1124.
Onishi M, Liou GG, Buchberger JR, Walz T, Moazed D: Role of the conserved Sir3-BAH domain in nucleosome binding and silent chromatin assembly. Mol Cell. 2007, 28: 1015-1028.
Altaf M, Utley RT, Lacoste N, Tan S, Briggs SD, Cote J: Interplay of chromatin modifiers on a short basic patch of histone H4 tail defines the boundary of telomeric heterochromatin. Mol Cell. 2007, 28: 1002-1014.
Martino F, Kueng S, Robinson P, Tsai-Pflugfelder M, van Leeuwen F, Ziegler M, Cubizolles F, Cockell MM, Rhodes D, Gasser SM: Reconstitution of Yeast Silent Chromatin: Multiple Contact Sites and O-AADPR Binding Load SIR Complexes onto Nucleosomes In Vitro. Mol Cell. 2009, 33: 323-334.
van Leeuwen F, Gottschling DE: Genome-wide histone modifications: gaining specificity by preventing promiscuity. Curr Opin Cell Biol. 2002, 14: 756-762.
Rusche LN, Kirchmaier AL, Rine J: The establishment, inheritance, and function of silenced chromatin in Saccharomyces cerevisiae. Annu Rev Biochem. 2003, 72: 481-516.
Kimura A, Umehara T, Horikoshi M: Chromosomal gradient of histone acetylation established by Sas2p and Sir2p functions as a shield against gene silencing. Nat Genet. 2002, 32: 370-377.
Suka N, Luo K, Grunstein M: Sir2p and Sas2p opposingly regulate acetylation of yeast histone H4 lysine16 and spreading of heterochromatin. Nat Genet. 2002, 32: 378-383.
Venkatasubrahmanyam S, Hwang WW, Meneghini MD, Tong AH, Madhani HD: Genome-wide, as opposed to local, antisilencing is mediated redundantly by the euchromatic factors Set1 and H2A.Z. Proc Natl Acad Sci USA. 2007, 104: 16609-16614.
Meneghini MD, Wu M, Madhani HD: Conserved histone variant H2A.Z protects euchromatin from the ectopic spread of silent heterochromatin. Cell. 2003, 112: 725-736.
San Segundo PA, Roeder GS: Role for the silencing protein Dot1 in meiotic checkpoint control. Molecular Biology of the Cell. 2000, 11: 3601-3615.
Santos-Rosa H, Schneider R, Bernstein BE, Karabetsou N, Morillon A, Weise C, Schreiber SL, Mellor J, Kouzarides T: Methylation of histone H3 K4 mediates association of the Isw1p ATPase with chromatin. Mol Cell. 2003, 12: 1325-1332.
Santos-Rosa H, Bannister AJ, Dehe PM, Geli V, Kouzarides T: Methylation of H3 lysine 4 at euchromatin promotes Sir3p association with heterochromatin. J Biol Chem. 2004, 279: 47506-47512.
Frederiks F, Tzouros M, Oudgenoeg G, van Welsem T, Fornerod M, Krijgsveld J, van Leeuwen F: Nonprocessive methylation by Dot1 leads to functional redundancy of histone H3K79 methylation states. Nat Struct Mol Biol. 2008, 15: 550-557.
Wotton D, Shore D: A novel Rap1p-interacting factor, Rif2p, cooperates with Rif1p to regulate telomere length in Saccharomyces cerevisae. Genes Dev. 1997, 11329: 748-760.
Marsellach FX, Huertas D, Azorin F: The multi-KH domain protein of Saccharomyces cerevisiae Scp160p contributes to the regulation of telomeric silencing. J Biol Chem. 2006, 281: 18227-18235.
Raisner RM, Madhani HD: Genomewide screen for negative regulators of sirtuin activity in Saccharomyces cerevisiae reveals 40 loci and links to metabolism. Genetics. 2008, 179: 1933-1944.
Kyrion G, Liu K, Liu C, Lustig AJ: RAP1 and telomere structure regulate telomere position effects in Saccharomyces cerevisae. Genes Dev. 1993, 7350: 1146-1159.
van Welsem T, Frederiks F, Verzijlbergen KF, Faber AW, Nelson ZW, Egan DA, Gottschling DE, van Leeuwen F: Synthetic lethal screens identify gene silencing processes in yeast and implicate the acetylated amino terminus of Sir3 in recognition of the nucleosome core. Mol Cell Biol. 2008, 28: 3861-3872.
van Leeuwen F, Gottschling DE: Assays for gene silencing in yeast. Methods Enzymol. 2002, 350: 165-186.
Hecht A, Laroche T, Strahl-Bolsinger S, Gasser SM, Grunstein M: Histone H3 and H4 N-termini interact with SIR3 and SIR4 proteins: a molecular model for the formation of heterochromatin in yeast. Cell. 1995, 80: 583-592.
Carmen AA, Milne L, Grunstein M: Acetylation of the yeast histone H4 N-terminus regulates its binding to heterochromatin protein SIR3. J Biol Chem. 2001, 190: 19-
Vogelauer M, Wu JS, Suka N, Grunstein M: Global histone acetylation and deacetylation in yeast. Nature. 2000, 408: 495-498.
Robyr D, Kurdistani SK, Grunstein M: Analysis of genome-wide histone acetylation state and enzyme binding using DNA microarrays. Methods Enzymol. 2004, 376: 289-304.
Reid JL, Moqtaderi Z, Struhl K: Eaf3 regulates the global pattern of histone acetylation in Saccharomyces cerevisiae. Mol Cell Biol. 2004, 24: 757-764.
Rundlett SE, Carmen AA, Kobayashi R, Bavykin S, Turner BM, Grunstein M: HDA1 and RPD3 are members of distinct yeast histone deacetylase complexes that regulate silencing and transcription. Proc Natl Acad Sci USA. 1996, 93: 14503-14508.
Lin YY, Qi Y, Lu JY, Pan X, Yuan DS, Zhao Y, Bader JS, Boeke JD: A comprehensive synthetic genetic interaction network governing yeast histone acetylation and deacetylation. Genes Dev. 2008, 22: 2062-2074.
Bernstein BE, Humphrey EL, Erlich RL, Schneider R, Bouman P, Liu JS, Kouzarides T, Schreiber SL: Methylation of histone H3 Lys 4 in coding regions of active genes. Proc Natl Acad Sci USA. 2002, 990: 8659-8700.
Deckert J, Struhl K: Histone acetylation at promoters is differentially affected by specific activators and repressors. Mol Cell Biol. 2001, 21: 2726-2735.
Sun ZW, Hampsey M: A general requirement for the Sin3-Rpd3 histone deacetylase complex in regulating silencing in Saccharomyces cerevisiae. Genetics. 1999, 152: 921-932.
Bernstein BE, Tong JK, Schreiber SL: Genomewide studies of histone deacetylase function in yeast. Proc Natl Acad Sci USA. 2000, 97: 13708-13713.
De Rubertis F, Kadosh D, Henchoz S, Pauli D, Reuter G, Struhl K, Spierer P: The histone deacetylase RPD3 counteracts genomic silencing in Drosophila and yeast. Nature. 1996, 384: 589-591.
Zhou J, Zhou BO, Lenzmeier BA, Zhou JQ: Histone deacetylase Rpd3 antagonizes Sir2-dependent silent chromatin propagation. Nucleic Acids Res. 2009, 37: 3699-3713.
Li B, Gogol M, Carey M, Lee D, Seidel C, Workman JL: Combined action of PHD and chromo domains directs the Rpd3S HDAC to transcribed chromatin. Science. 2007, 316: 1050-1054.
Keogh MC, Kurdistani SK, Morris SA, Ahn SH, Podolny V, Collins SR, Schuldiner M, Chin K, Punna T, Thompson NJ, et al: Cotranscriptional set2 methylation of histone H3 lysine 36 recruits a repressive Rpd3 complex. Cell. 2005, 123: 593-605.
Carrozza MJ, Li B, Florens L, Suganuma T, Swanson SK, Lee KK, Shia WJ, Anderson S, Yates J, Washburn MP, et al: Histone H3 methylation by Set2 directs deacetylation of coding regions by Rpd3S to suppress spurious intragenic transcription. Cell. 2005, 123: 581-592.
Joshi AA, Struhl K: Eaf3 chromodomain interaction with methylated H3-K36 links histone deacetylation to Pol II elongation. Mol Cell. 2005, 20: 971-978.
Shevchenko A, Roguev A, Schaft D, Buchanan L, Habermann B, Sakalar C, Thomas H, Krogan NJ, Shevchenko A, Stewart AF: Chromatin Central: towards the comparative proteome by accurate mapping of the yeast proteomic environment. Genome Biol. 2008, 9: R167-
Bi X, Yu Q, Sandmeier JJ, Elizondo S: Regulation of transcriptional silencing in yeast by growth temperature. J Mol Biol. 2004, 344: 893-905.
Wittschieben BO, Otero G, de Bizemont T, Fellows J, Erdjument-Bromage H, Ohba R, Li Y, Allis CD, Tempst P, Svejstrup JQ: A novel histone acetyltransferase is an integral subunit of elongating RNA polymerase II holoenzyme. Mol Cell. 1999, 4: 123-128.
Sendra R, Tse C, Hansen JC: The yeast histone acetyltransferase A2 complex, but not free Gcn5p, binds stably to nucleosomal arrays. J Biol Chem. 2000, 275: 24928-24934.
Grant PA, Duggan L, Cote J, Roberts SM, Brownell JE, Candau R, Ohba R, Owen-Hughes T, Allis CD, Winston F, et al: Yeast Gcn5 functions in two multisubunit complexes to acetylate nucleosomal histones: characterization of an Ada complex and the SAGA (Spt/Ada) complex. Genes Dev. 1997, 11: 1640-1650.
Sterner DE, Belotserkovskaya R, Berger SL: SALSA, a variant of yeast SAGA, contains truncated Spt7, which correlates with activated transcription. Proc Natl Acad Sci USA. 2002, 99: 11622-11627.
Eberharter A, Sterner DE, Schieltz D, Hassan A, Yates JR, Berger SL, Workman JL: The ADA complex is a distinct histone acetyltransferase complex in Saccharomyces cerevisiae. Mol Cell Biol. 1999, 19: 6621-6631.
Pray-Grant MG, Schieltz D, McMahon SJ, Wood JM, Kennedy EL, Cook RG, Workman JL, Yates JR, Grant PA: The novel SLIK histone acetyltransferase complex functions in the yeast retrograde response pathway. Mol Cell Biol. 2002, 22: 8774-8786.
Sklenar AR, Parthun MR: Characterization of yeast histone H3-specific type B histone acetyltransferases identifies an ADA2-independent Gcn5p activity. BMC Biochem. 2004, 5: 11-
John S, Howe L, Tafrov ST, Grant PA, Sternglanz R, Workman JL: The something about silencing protein, Sas3, is the catalytic subunit of NuA3, a yTAF(II)30-containing HAT complex that interacts with the Spt16 subunit of the yeast CP (Cdc68/Pob3)-FACT complex. Genes Dev. 2000, 14: 1196-1208.
Shia WJ, Osada S, Florens L, Swanson SK, Washburn MP, Workman JL: Characterization of the yeast trimeric-SAS acetyltransferase complex. J Biol Chem. 2005, 280: 11987-11994.
Meijsing SH, Ehrenhofer-Murray AE: The silencing complex SAS-I links histone acetylation to the assembly of repressed chromatin by CAF-I and Asf1 in Saccharomyces cerevisiae. Genes Dev. 2001, 15: 3169-3182.
Osada S, Sutton A, Muster N, Brown CE, Yates JR, Sternglanz R, Workman JL: The yeast SAS (something about silencing) protein complex contains a MYST-type putative acetyltransferase and functions with chromatin assembly factor ASF1. Genes Dev. 2001, 15: 3155-3168.
Auger A, Galarneau L, Altaf M, Nourani A, Doyon Y, Utley RT, Cronier D, Allard S, Cote J: Eaf1 is the platform for NuA4 molecular assembly that evolutionarily links chromatin acetylation to ATP-dependent exchange of histone H2A variants. Mol Cell Biol. 2008, 28: 2257-2270.
Winkler GS, Kristjuhan A, Erdjument-Bromage H, Tempst P, Svejstrup JQ: Elongator is a histone H3 and H4 acetyltransferase important for normal histone acetylation levels in vivo. Proc Natl Acad Sci USA. 2002, 99: 3517-3522.
Kristjuhan A, Walker J, Suka N, Grunstein M, Roberts D, Cairns BR, Svejstrup JQ: Transcriptional inhibition of genes with severe histone h3 hypoacetylation in the coding region. Mol Cell. 2002, 10: 925-933.
Choi JK, Grimes DE, Rowe KM, Howe LJ: Acetylation of Rsc4p by Gcn5p is essential in the absence of histone H3 acetylation. Mol Cell Biol. 2008, 28: 6967-6972.
Shahbazian MD, Grunstein M: Functions of site-specific histone acetylation and deacetylation. Annu Rev Biochem. 2007, 76: 75-100.
Howe L, Auston D, Grant P, John S, Cook RG, Workman JL, Pillus L: Histone H3 specific acetyltransferases are essential for cell cycle progression. Genes Dev. 2001, 15: 3144-3154.
Durant M, Pugh BF: Genome-wide relationships between TAF1 and histone acetyltransferases in Saccharomyces cerevisiae. Mol Cell Biol. 2006, 26: 2791-2802.
Keogh MC, Mennella TA, Sawa C, Berthelet S, Krogan NJ, Wolek A, Podolny V, Carpenter LR, Greenblatt JF, Baetz K, et al: The Saccharomyces cerevisiae histone H2A variant Htz1 is acetylated by NuA4. Genes Dev. 2006, 20: 660-665.
Babiarz JE, Halley JE, Rine J: Telomeric heterochromatin boundaries require NuA4-dependent acetylation of histone variant H2A.Z in Saccharomyces cerevisiae. Genes Dev. 2006, 20: 700-710.
Shia WJ, Li B, Workman JL: SAS-mediated acetylation of histone H4 Lys 16 is required for H2A.Z incorporation at subtelomeric regions in Saccharomyces cerevisiae. Genes Dev. 2006, 20: 2507-2512.
Kristjuhan A, Wittschieben BO, Walker J, Roberts D, Cairns BR, Svejstrup JQ: Spreading of Sir3 protein in cells with severe histone H3 hypoacetylation. Proc Natl Acad Sci USA. 2003, 100: 7551-7556.
Jin Y, Rodriguez AM, Stanton JD, Kitazono AA, Wyrick JJ: Simultaneous mutation of methylated lysine residues in histone H3 causes enhanced gene silencing, cell cycle defects, and cell lethality in Saccharomyces cerevisiae. Mol Cell Biol. 2007, 27: 6832-6841.
VanDemark AP, Kasten MM, Ferris E, Heroux A, Hill CP, Cairns BR: Autoregulation of the rsc4 tandem bromodomain by gcn5 acetylation. Mol Cell. 2007, 27: 817-828.
Martin DG, Grimes DE, Baetz K, Howe L: Methylation of histone H3 mediates the association of the NuA3 histone acetyltransferase with chromatin. Mol Cell Biol. 2006, 26: 3018-3028.
Zhang K, Lin W, Latham JA, Riefler GM, Schumacher JM, Chan C, Tatchell K, Hawke DH, Kobayashi R, Dent SY: The Set1 methyltransferase opposes Ipl1 aurora kinase functions in chromosome segregation. Cell. 2005, 122: 723-734.
Vernarecci S, Ornaghi P, Bagu A, Cundari E, Ballario P, Filetici P: Gcn5p plays an important role in centromere kinetochore function in budding yeast. Mol Cell Biol. 2008, 28: 988-996.
Singer MS, Kahana A, Wolf AJ, Meisinger LL, Peterson SE, Goggin C, Mahowald M, Gottschling DE: Identification of high-copy disruptors of telomeric silencing in Saccharomyces cerevisiae. Genetics. 1998, 150: 613-632.
Katan-Khaykovich Y, Struhl K: Heterochromatin formation involves changes in histone modifications over multiple cell generations. EMBO J. 2005, 24: 2138-2149.
Ladurner AG, Inouye C, Jain R, Tjian R: Bromodomains mediate an acetyl-histone encoded antisilencing function at heterochromatin boundaries. Mol Cell. 2003, 11: 365-376.
Fingerman IM, Li HC, Briggs SD: A charge-based interaction between histone H4 and Dot1 is required for H3K79 methylation and telomere silencing: identification of a new trans-histone pathway. Genes Dev. 2007, 21: 2018-2029.
Gardner RG, Nelson ZW, Gottschling DE: Ubp10/Dot4p regulates the persistence of ubiquitinated histone H2B: distinct roles in telomeric silencing and general chromatin. Mol Cell Biol. 2005, 25: 6123-6139.
Emre NC, Ingvarsdottir K, Wyce A, Wood A, Krogan NJ, Henry KW, Li K, Marmorstein R, Greenblatt JF, Shilatifard A, et al: Maintenance of low histone ubiquitylation by Ubp10 correlates with telomere-proximal Sir2 association and gene silencing. Mol Cell. 2005, 17: 585-594.
Tompa R, Madhani HD: Histone H3 lysine 36 methylation antagonizes silencing in Saccharomyces cerevisiae independently of the Rpd3S histone deacetylase complex. Genetics. 2007, 175: 585-593.
Yang B, Kirchmaier AL: Bypassing the catalytic activity of SIR2 for SIR protein spreading in Saccharomyces cerevisiae. Mol Biol Cell. 2006, 17: 5287-5297.
Lynch PJ, Rusche LN: A silencer promotes the assembly of silenced chromatin independently of recruitment. Mol Cell Biol. 2008, 29: 43-56.
Rusche LN, Rine J: Conversion of a gene-specific repressor to a regional silencer. Genes Dev. 2001, 15: 955-967.
Robyr D, Suka Y, Xenarios I, Kurdistani SK, Wang A, Suka N, Grunstein M: Microarray deacetylation maps determine genome-wide functions for yeast histone deacetylases. Cell. 2002, 109: 437-446.
Mead J, McCord R, Youngster L, Sharma M, Gartenberg MR, Vershon AK: Swapping the gene-specific and regional silencing specificities of the Hst1 and Sir2 histone deacetylases. Mol Cell Biol. 2007, 27: 2466-2475.
Sutton A, Heller RC, Landry J, Choy JS, Sirko A, Sternglanz R: A novel form of transcriptional silencing by Sum1-1 requires Hst1 and the origin recognition complex. Mol Cell Biol. 2001, 21: 3514-3522.
Halme A, Bumgarner S, Styles C, Fink GR: Genetic and epigenetic regulation of the FLO gene family generates cell-surface variation in yeast. Cell. 2004, 116: 405-415.
Shanower GA, Muller M, Blanton JL, Honti V, Gyurkovics H, Schedl P: Characterization of the grappa gene, the Drosophila histone H3 lysine 79 methyltransferase. Genetics. 2005, 169: 173-184.
Okada Y, Feng Q, Lin Y, Jiang Q, Li Y, Coffield VM, Su L, Xu G, Zhang Y: hDOT1L links histone methylation to leukemogenesis. Cell. 2005, 121: 167-178.
Zhang W, Xia X, Reisenauer MR, Hemenway CS, Kone BC: Dot1a-AF9 complex mediates histone H3 Lys-79 hypermethylation and repression of ENaCalpha in an aldosterone-sensitive manner. J Biol Chem. 2006, 281: 18059-18068.
Okada Y, Jiang Q, Lemieux M, Jeannotte L, Su L, Zhang Y: Leukaemic transformation by CALM-AF10 involves upregulation of Hoxa5 by hDOT1L. Nat Cell Biol. 2006, 8: 1017-1024.
Brachmann CB, Davies A, Cost GJ, Caputo E, Li J, Hieter P, Boeke JD: Designer deletion strains derived from Saccharomyces cerevisiae S288C: a useful set of strains and plasmids for PCR-mediated gene disruption and other applications. Yeast. 1998, 14: 115-132.
Gardner R, Cronin S, Leader B, Rine J, Hampton R: Sequence determinants for regulated degradation of yeast 3-hydroxy-3-methylglutaryl-CoA reductase, an integral endoplasmic reticulum membrane protein. Mol Biol Cell. 1998, 9: 2611-2626.
McConnell AD, Gelbart ME, Tsukiyama T: Histone fold protein Dls1p is required for Isw2-dependent chromatin remodeling in vivo. Mol Cell Biol. 2004, 24: 2605-2613.
Acknowledgements
We thank E. Battaglia for help with strain constructions, J.M.M. den Haan for Sir3 antibody purification, and D.E. Gottschling, F. Frederiks, and M. Fornerod, for discussions and/or critical reading of the manuscript. This work was supported by the EU 6th framework program (NOE 'The Epigenome' LSHG-CT-2004-503433) and by a VIDI fellowship from NWO-ALW.
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KFV, AWF, and FvL designed the experiments. AWF and FvL made the yeast strains and performed silencing assays. FvL and KFV performed tetrad analyses. KFV performed qRT-PCR and ChIP analyses. IJES and FvL performed immunoblots. FvL conceived the study. KFV, IJES, and FvL wrote the paper. All authors read and approved the final manuscript.
Kitty F Verzijlbergen, Alex W Faber contributed equally to this work.
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Verzijlbergen, K.F., Faber, A.W., Stulemeijer, I.J. et al. Multiple histone modifications in euchromatin promote heterochromatin formation by redundant mechanisms in Saccharomyces cerevisiae. BMC Molecular Biol 10, 76 (2009). https://doi.org/10.1186/1471-2199-10-76
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DOI: https://doi.org/10.1186/1471-2199-10-76