A Genetic Screen for High Copy Number Suppressors of the Synthetic Lethality Between elg1Δ and srs2Δ in Yeast

Elg1 and Srs2 are two proteins involved in maintaining genome stability in yeast. After DNA damage, the homotrimeric clamp PCNA, which provides stability and processivity to DNA polymerases and serves as a docking platform for DNA repair enzymes, undergoes modification by the ubiquitin-like molecule SUMO. PCNA SUMOylation helps recruit Srs2 and Elg1 to the replication fork. In the absence of Elg1, both SUMOylated PCNA and Srs2 accumulate at the chromatin fraction, indicating that Elg1 is required for removing SUMOylated PCNA and Srs2 from DNA. Despite this interaction, which suggests that the two proteins work together, double mutants elg1Δ srs2Δ have severely impaired growth as haploids and exhibit synergistic sensitivity to DNA damage and a synergistic increase in gene conversion. In addition, diploid elg1Δ srs2Δ double mutants are dead, which implies that an essential function in the cell requires at least one of the two gene products for survival. To gain information about this essential function, we have carried out a high copy number suppressor screen to search for genes that, when overexpressed, suppress the synthetic lethality between elg1Δ and srs2Δ. We report the identification of 36 such genes, which are enriched for functions related to DNA- and chromatin-binding, chromatin packaging and modification, and mRNA export from the nucleus.

to mutations in lysine 164, those in lysine 127 do not lead to DNA damage sensitive phenotypes (Hoege et al. 2002).
The Elg1 protein resembles the large subunit of Replication Factor C, a protein complex in charge of loading/unloading PCNA from DNA during replication. Mutations in ELG1 lead to a variety of genomic instability phenotypes, including, among others, hyper-recombination, chromosome loss, elongated telomeres, and increased telomeric silencing (Banerjee and Myung 2004;Banerjee et al. 2007;Bellaoui et al. 2003;Ben-Aroya et al. 2003;Kanellis et al. 2003). Similarly to Srs2, mutations in ELG1 suppress the sensitivity to DNA damaging agents of mutants of the post-replication repair pathway (Parnas et al. 2010). Both proteins are recruited to SUMOylated PCNA by a similar mechanism involving PCNA-(PIP) and SUMO-interacting motifs (Armstrong et al. 2012;Kolesar et al. 2012;Parnas et al. 2010;Pfander et al. 2005). Moreover, deletion of ELG1 leads to accumulation of Srs2 at the chromatin fraction, suggesting that Elg1 may play a role in Srs2 unloading, perhaps together with SUMOylated PCNA (Parnas et al. 2010). Remarkably, however, double deletion of the ELG1 and SRS2 genes results in a synthetic fitness reduction in haploid cells (Parnas et al. 2010) and in complete lethality in diploids (this study). These results imply that at least one of them must be active for viability. Because both proteins are active during DNA replication, it is likely that they provide alternative mechanisms to deal with specific DNA lesions or intermediates. However, alternative possibilities exist. Here we try to gain information about the function of these proteins by carrying out a genetic screen for genes that, when overexpressed, are able to rescue the synthetic lethality (SL) between elg1 and srs2 mutations.

Genetic screen
A high copy number library in YEp24 (a 2-mm URA3 plasmid) was used in the screen, carried out as described (Parnas et al. 2009). Each positive plasmid was extracted and retransformed into OP738. Only those that gave sectors were analyzed. Individual genes were subcloned into high copy number plasmids and retested.
GO (Gene Ontology) enrichment was calculated using an in-house score algorithm. The algorithm is a simple hypergeometric calculation; categories annotated with two few (#3) or too many ($500) genes were excluded from the enrichment calculation. Scores were corrected for multiple hypotheses testing an FDR threshold of 0.001.

RESULTS AND DISCUSSION
SL between elg1D and srs2D Elg1 and Srs2 physically interact with SUMOylated PCNA in a similar manner through their PIP and SUMO-interacting domains (Armstrong et al. 2012;Kolesar et al. 2012;Parnas et al. 2010;Pfander et al. 2005). In addition, Elg1 seems to be required for the unloading of Srs2 from chromatin (Parnas et al. 2010). We would thus expect mutations in ELG1 and SRS2 to show epistasis, such that the double mutant would not show a phenotype more severe than the single mutants. However, elg1D srs2D double mutants show, in comparison with each of the single mutants, increased sensitivity to DNA-damaging agents, such as the alkylating agent methylmethane sulfonate, the inhibitor of deoxynucleotides synthesis hydroxyurea, and the topoisiomerase inhibitor camptothecin (Figure 1).
Mutations in each of the two genes cause an increase in homologous recombination Liefshitz et al. 1998). To characterize the type of recombination events that occur in the single and double mutants, we used strain MK166 (Liefshitz et al. 1995). This strain allows the detection of both gene conversion events between repeated sequences (Ty elements) or ectopic single sequences (lys2 alleles) and direct-repeat recombination (DRR) at Ty elements and at the HIS4 locus (Liefshitz et al. 1995). Whereas gene conversion transfers information between alleles, DRR results in the deletion of information located between the two repeats (Agmon et al. 2009). Table 1 shows that despite the fact that each mutant is hyperrecombinant, compared with the wt, they show a very different pattern of homologous recombination. Whereas srs2D shows increased levels of gene conversion events, the elg1D mutant shows both high gene conversion and high DRR levels. The elg1D srs2D double mutant shows the same level of DRR as elg1D; however, it exhibits a synergistic effect for gene conversion: lys2 gene conversion is elevated eightfold, and the level of Ty ectopic conversion is increased 80-fold above that of the wt strain (Table 1). We interpret these results as follows: The activity of Srs2 prevents gene conversion events, probably by evicting the Rad51 recombination protein from the DNA (Krejci et al. 2003;Veaute et al. 2003). In the absence of Srs2, we see an increase in gene Figure 1 The elg1D and srs2D mutants display synergistic sensitivity to DNA-damaging agents. Ten-fold serial dilutions of logarithmic cultures were plated on SD-complete plates containing either methylmethane sulfonate (MMS), hydroxyurea (HU), or camptothecin (CPT) at the concentrations shown.
conversion events but not in DRR events, which are probably carried out by single strand annealing and do not require Rad51 (Krejci et al. 2003). In contrast, the absence of Elg1 promotes all types of recombination events, either because Elg1 does not allow the first steps of recombination to take place, or, as has been suggested (Davidson et al. 2012), because in its absence spontaneous DNA damage accumulates. The results of the double mutant, however, suggest that Elg1 activity restricts the level of gene conversion events of srs2 mutants, and thus both proteins must play some role during the actual recombination process.
elg1D srs2D double mutants are extremely sick as haploids (Parnas et al. 2010), indicating that cells need at least one of the proteins to carry out a function important for fitness, probably some type of repair that is so common that it occurs often during DNA replication, such as fork stalling response. Previous work showed that many of the phenotypes of srs2D are stronger in diploids, and that several mutations affecting DNA repair produce a synthetic sick phenotype when combined with srs2D as haploids, but are completely lethal as diploids (Klein 2001). We thus crossed an elg1D srs2D haploid with either an elg1D haploid, an srs2D haploid or a double mutant elg1D srs2D of the opposite sex. Mating took place at normal frequencies.
Zygotes were micromanipulated under the microscope to fixed positions in the plate and were then incubated for 48 hr. Thirty-two of 32 zygotes and 31 of 32 zygotes were able to form colonies in the first two crosses (with single elg1D and srs2D mutants, respectively), whereas only 2 of the 80 elg1/elg1 srs2/srs2 zygotes formed viable colonies after micromanipulation. Microscopic observation of the zygotes showed that the majority produced between 0 and 2 cell divisions before dying. Thus, diploid elg1/elg1 srs2/srs2 strains are inviable.
A high copy number screen for suppressors of the SL between elg1D and srs2D Our high copy number screen was based on a red/white colony phenotype Koshland et al. 1985;Parnas et al. 2009). ade2 mutants form red colonies due to the accumulation of a red pigment. Mutations in the upstream-acting gene ADE3 prevent the accumulation of the red pigment and render the cells white. An ade2 ade3 elg1D srs2D diploid strain (OP738) kept alive by the presence of a LEU2-marked plasmid carrying the ELG1 gene as well as the ADE3 gene forms uniformly red colonies (as the ade3 mutation is complemented, and any cell that loses the plasmid dies; Figure 2). These cells were then transformed with a yeast genomic library cloned in a high copy number plasmid (containing the URA3 marker). Cells that received a plasmid with a gene that, when overexpressed, can suppress the SL phenotype of elg1D srs2D, are now able to lose the ELG1-ADE3-LEU2 plasmid, and therefore show white/red sectored colonies ( Figures  2 and 3). The sectoring pattern (number and size of sectors) reflects the rate of viable plasmid loss, and thus provides a measure of the efficiency of suppression. Examples of such patterns are seen in Figure 3.
After screening~50,000 yeast transformants, 92 candidates showed some level of colony sectoring. Plasmids (each containing a~8 kb insert on average) were obtained from these colonies and retransformed into OP738. Only 54 of these candidates clearly exhibited sectors upon retransformation. These plasmids were sequenced to determine the genomic region responsible for the suppression. Many plasmids carried overlapping genomic fragments, and in total were found to represent 34 genomic regions. Subcloning experiments were then carried out to identify the genes responsible for the suppressive phenotype. With a few exceptions (RTT103 and NSE3; CHD1 and PAB1), only one gene per plasmid caused increased white sectoring. Table 2 shows the names and functions of the 36 genes identified.
The genes identified span a large number of functions, pathways and cellular location. Analysis of GO (gene onthology) term enrichment (Table 3) shows that this gene set is enriched for genes of chromosomal location, with functions related to DNA-and chromatinbinding and involved in biological processes related to DNA packaging and modification. Additionally, there is an enrichment for genes involved in regulatory mechanisms as well as genes that participate in the response to DNA damage. Below, we present the genes, divided into functional categories obtained by reading the literature regarding each of the genes. Naturally, this division is artificial, as many of the categories overlap, and the precise mechanism of suppression is still unknown.
Genes affecting genome stability: This category includes the following genes: ECO1/CTF7: Eco1 is a protein essential for sister chromatid cohesion (Skibbens et al. 1999;Toth et al. 1999). It has an acetyltransferase activity that acetylates the cohesin subunit Smc3. This acetylation has been shown to be critical for the establishment of cohesion during S phase (Unal et al. 2008). Eco1 interacts with PCNA through a PIP motif (Moldovan et al. 2006), thus effectively coordinating between cohesion establishment and DNA replication. It was found that loss of PCNA SUMOylation by deletion of the SUMO ligase SIZ1 rescued the temperature sensitivity of eco1 mutants, indicating a role for SUMO in this process (Moldovan et al. 2006). Elg1 has been shown to affect sister chromatid cohesion (Parnas et al. 2009) and genetic antagonistic interactions have been observed between Elg1 and Eco1: deletion of ELG1 partially rescues the phenotypes of a temperature sensitive eco1 mutant, whereas its overexpression enhances its phenotypes (Maradeo and Skibbens 2009;Maradeo and Skibbens 2010). Despite their common interaction with PCNA, no physical or genetic interactions have been detected between Eco1 and Srs2.
NSE3: Nse3 is part of the Smc5-6 complex, which is structurally similar to cohesin, but whose precise function still remains enigmatic (Bustard et al. 2012). This complex was found to be required for a variety of DNA repair activities, including sister chromatid recombination, and mutants defective for its components exhibit an unusual amount of recombination intermediates (Bustard et al. 2012), a phenotype shared with both elg1D and srs2D mutants. Interestingly, the complex contains a SUMO-ligase and potentially a ubiquitin-ligase. A recent publication links cohesin SUMOylation by the Smc5-6 complex n DDC1: Ddc1 forms part of a PCNA-like molecule (called the 9-1-1 clamp). Loading of this heterotrimeric ring onto DNA is essential for the activation of the DNA damage response (Melo et al. 2001). This clamp has been recently been proposed to play a pivotal role in an error-free lesion bypassing mechanism that operates in parallel to Srs2 (Karras et al. 2013). These four genes seem to be exerting their suppressive effect by affecting processes that take place during DNA replication, at the fork. Their overexpression may prevent stalling or may be able to act in DNA repair, either replacing a common function of Elg1 and Srs2, or providing alternative repair mechanisms. Ddc1 overexpression may lead to a stronger or extended DNA checkpoint response, which may help cope with fork stalling. Alternatively, the lethality between elg1 and srs2 may be due to lesions left behind the fork in the absence of the two repair activities, and overexpression of proteins that participate in alternative repair mechanisms may be able to repair this lethal damage, rescuing the cells.
Genes affecting histones and chromatin: This category includes the following genes: HTB1: DNA is packaged in eukaryotic cells around nucleosomes composed of two units each of the H2A-H2B and H3-H4 heterodimers. HTB1 encodes a copy of histone H2B. Ubiquitination of this histone on residue K123 is a prerequisite for histone H3 modification and is essential for a variety of cellular processes, including gene expression and DNA repair (Dover et al. 2002;Robzyk et al. 2000).

RTT106
: During DNA replication, nucleosomes ahead of the replication fork are disassembled, and the recently replicated DNA is reassembled into nucleosomes using both the old, parental histones, as well as newly synthesized histones. Deposition of newly synthesized H3-H4 requires histone chaperones, including Rtt106 ). The dimeric histones delivered by Rtt106 are marked by acetylation at lysine 56 of histone H3 (Su et al. 2012).
RTT109: Rtt109 is a histone acetyltransferase that is required for proper acetylation of histone H3 at lysine 56 (H3K56), which occurs during S phase and DNA damage repair. The formation of H3K56ac  Schematic representation of the screen. A diploid double mutant elg1D srs2D strain is kept alive by the presence of a plasmid carrying the ELG1 gene. The ADE3 marker on the plasmid confers a red pigment to the cells carrying it (as the strain is ade2 ade3). Since any cell that loses the plasmid during colony formation dies, all colonies are uniformly red. This strain was transformed with a high copy number library carrying random fragments of the yeast genome. Cells that received a plasmid that suppresses the SL phenotype (SUPP1) can now lose the ELG1-containing plasmid, becoming white. These cells create white or red/white sectored colonies.
by Rtt109 and its deposition by Rtt106 stabilize the advancing replication forks and allow the repair of lesions that occur during replication (Clemente- Ruiz et al. 2011). CHD1: Chd1 is a chromatin remodeler that belongs to the chromodomain-containing subfamily of Snf2-like proteins; these proteins are believed to be recruited through methylated histone lysine residues and to promote nucleosome remodeling. Interestingly, it was recently shown that Chd1 is required for histone H2B ubiquitination, which is required for histone restoration after RNA polymerase passage .
NHP6A: Nhp6A is an abundant small protein that binds DNA nonspecifically and bends it sharply. By binding the minor groove of DNA with a single HMGB domain and wrapping around the DNA to contact the major groove, it helps remodeling the nucleosomes (Stillman 2010). A less-abundant, very similar protein, Nhp6B, exists. Both were found to be components, together with Spt16p and Pob3p, of the FACT complex, which plays important roles in transcription and DNA replication (Ruone et al. 2003).
Thus, overexpression of histone H2B, or of proteins that promote nucleosome re-establishment after DNA or RNA polymerase transit, alleviate the SL phenotype of elg1D and srs2D. We can think of three possible models for this: (1) mutations in these genes cause replication fork instability, which can be suppressed by accelerating replication in the presence of excess histone dimers ready to be assembled into the newly replicated DNA. (2) Alternatively, Srs2 and Elg1 may play a direct role in the regulation of histone levels in the cell, and their SL is alleviated when histone levels are increased by other means. (3) A third model, involving an effect of these chromatin regulators in transcription regulation (which is also affected by histone levels and deposition), seems to us less likely, although recent evidence supports a role for histone levels in the regulation of promoter fidelity (Silva et al. 2012).
n Major karyopherin, involved in export of proteins, RNAs, and ribosomal subunits from the nucleus Strong

MOB1
Component of the mitotic exit network Strong DDC1 Member of the 9-1-1 clamp essential for the DNA damage response Strong CST6 Basic leucine zipper (bZIP) transcription factor Strong MPH1 Helicase that functions in an error-free DNA damage bypass pathway Strong YKL044w Gene of unknown function Strong SIS2 Negative regulatory subunit of the protein phosphatase 1 Ppz1 Strong UBC11 Ubiquitin-conjugating enzyme Strong NHP6A High-mobility group non-histone chromatin protein Strong TPT1 tRNA 2'-phosphotransferase, catalyzes the final step in yeast tRNA splicing Strong TAF3

TFIID subunit involved in transcription initiation Strong RTT103
Involved in transcription termination Medium SRL3 Cytoplasmic protein that, when overexpressed, suppresses the lethality of a rad53 null mutation

RTT109
Histone H3 acetylase Medium GID8 Member of a ubiquitin ligase that carries out poly-ubiquitination. Medium GIS2 Protein with seven cysteine-rich CCHC zinc-finger motifs Medium RTT106 Histone chaperone Medium YOL114c Gene of unknown function Medium IRC13 Null mutant displays increased levels of spontaneous Rad52 foci Medium NUP1 Nuclear pore complex (NPC) subunit, involved in protein import/export and in export of RNAs

PPS1
Protein phosphatase with specificity for serine, threonine, and tyrosine Weak UBP14 Ubiquitin-specific protease Weak NSE3 Essential subunit of the Mms21-Smc5-Smc6 complex Weak PAB1 Poly(A) binding protein, part of the 39-end RNA-processing complex Weak DAM1 Essential subunit of the Dam1 complex, involved in kinetochore movement

CPD1
Cyclic nucleotide phosphodiesterase Weak UBP7 Ubiquitin-specific protease that cleaves ubiquitin-protein fusions Weak RPB4 Subunit of RNA polymerase involved in 39-end RNA processing and export

RFX1
Major transcriptional repressor of DNA-damage-regulated genes Weak HAS1 ATP-dependent RNA helicase, localizes to nuclear pore Weak CNM67 Component of the spindle pole body outer plaque Weak It is interesting to note that elg1 mutants are synthetic sick with mutations in HTB1 (data not shown), RTT106 (Imbeault et al. 2008), RTT109 (Bellaoui et al. 2003), although not with chd1D, nhp6aD or the double nhp6aD nhp6bD (data not shown). In contrast, srs2D shows a synthetic fitness phenotype when combined with chd1D (Pan et al. 2006), rtt109D (Costanzo et al. 2010), but not with htb1D, rtt106D, nhp6aD or the double nhp6aD nhp6bD (data not shown). Thus, the spectrum of synthetic phenotypes between elg1D and srs2D only partially overlap, consistent with nonoverlapping functions for the two genes.
Genes affecting RNA end-processing and/or nuclear transport: This category includes the following genes: RTT103: Transcription by RNA polymerase II (PolII) and transcript processing are coordinated by the phosphorylation status of the PolII C-terminal domain (CTD). Transcription termination requires, surprisingly, the activity of RNA nucleases such as Rat1, which is recruited by Rtt103 (Kim et al. 2004). This requires an interaction between Rtt103 and the Ser2-phosphorylated form of PolII CTD. It was recently found that phosphorylation of the Tyr-1 residue in the CTD prevents Rtt103 binding, thus enhancing transcription processivity. At the 39 end of the transcript Tyr-1 levels drop, allowing Rtt103 binding and transcription termination followed by poly-adenylation (Mayer et al. 2012).
PAB1: Pab1 associates with RNA poly(A) tails, mediating the interactions between the 59 cap structure and the 39 mRNA poly(A) tail. It plays a role in mRNA stability and stimulates the initiation of translation (Amrani et al. 2008;Amrani et al. 1997). In addition, Pab1 is essential in the coupling of 39 RNA processing and nuclear export of the mRNA (Dunn et al. 2005).
RPB4: Rpb4 is an RNA polymerase II subunit that forms a complex with Rpb7. Contrary to other subunits of RNA polymerase II, Rpb4 is not essential under normal conditions; however, it becomes essential under stress. Lately it was found that this complex plays an important role in coordinating transcription in the nucleus with mRNA degradation and translation in the cytoplasm (Harel-Sharvit et al. 2010).
GIS2: Gis2 binds to a subset of mRNA molecules and promotes their translation by a still poorly understood mechanism (Sammons et al. 2011;Tsvetanova et al. 2010). Both Gis2 and its human ortholog, CNBP, mutations that cause muscular dystrophy, are part of stress granules (Rojas et al. 2012).

HAS1:
The HAS1 gene encodes an ATP-dependent RNA helicase that plays an important role in ribosomal RNA processing and nuclear export. Accordingly, it is highly enriched in nuclear pore complex fractions (Rout et al. 2000).

NUP1:
The Nup1 protein is a component of the central core of the nuclear pore complex. It plays a role in RNA and protein transport through the pore, by serving as a release factor for karyopherin (Aitchison and Rout 2012;Izaurralde and Adam 1998). CRM1: Crm1 is the main karyopherin protein, involved in export of proteins, RNAs, and ribosomal subunits from the nucleus. It plays a central role in cargo export (exportin function) (Aitchison and Rout 2012).
The common mechanism suggested by these genes is that the SL phenotype observed can be suppressed by increasing the levels of certain mRNA(s) as well as their transport from the nucleus (through the nuclear pore), perhaps causing an increase in the translation level of (a) target gene(s).
Spindle pole body and spindle checkpoints: CNM67: Cnm67 is a component of the spindle pole body outer plaque. It plays a central role in spindle orientation and in mitotic nuclear migration (Brachat et al. 1998). Cnm67 interacts physically and genetically with Gis2 (Scherrer et al. 2011;Wilmes et al. 2008). It also interacts with several kinetochore components, and mutations in CNM67 exhibit a synthetic fitness defect when combined with srs2 mutations (Pan et al. 2006). DAM1: Dam1 is a member of the DASH complex, which facilitates microtubule-kinetochore interactions, thereby playing an essential role in chromosome segregation. The DASH complex forms a ring around microtubules that stabilizes the microtubule and promotes its growth (Miranda et al. 2005). It also allows the kinetochore to preferentially bind to the microtubule plus end (Miranda et al. 2005). Dam1 is phosphorylated by the Ipl1 Aurora kinase; although this phosphorylartion does not seem to affect the binding activities of the complex, it is essential for the establishment of bipolar attachments. Notably, Dam1 is also methylated by the Set1 methyltransferase, the same enzyme in charge of methylating histone H3 at lysine4 (H3K4). Remarkably, both H3K4 and Dam1 methylation depend on prior ubiquitination of histone H2B (Latham et al. 2011). Mutations in DAM1 show synthetic fitness defects with mutations in RTT103. MOB1: Mob1 is a member of the mitotic exit network. It is located at the spindle pole body, where it binds and regulates the Dbf2 protein n kinase. Activation by Cdc15p-dependent phosphorylation leads to a change in its location, inducing cytokinesis and cell separation (Mah et al. 2001). Interestingly, Mob1 is important for the proper localization of the Ipl1 Aurora kinase (Stoepel et al. 2005), which phosphorylates Dam1. Thus, mitotic exit network activity is important for proper kinetochore activity, and controls the spindle checkpoint (Tan et al. 2005). The mechanism by which these genes may suppress the SL of elg1D srs2D cells could be related to the spindle checkpoint, which gets activated as a secondary response to DNA damage and prevents adaptation to DNA damage in srs2D mutants (Dotiwala et al. 2010).
Protein modification: A number of genes encoding protein modifiers were identified; these include ubiquitin-related proteins, as well as a protein phosphatase and a regulator of another phosphatase. The targets of these proteins that allow suppression of the SL phenotype is still unclear: CDC34: Cdc34 encodes a ubiquitin-conjugating enzyme (E2) that is the catalytic subunit of the SCF ubiquitin-protein ligase complex. This complex is in charge of targeting proteins for degradation, particularly those involved in cell cycle progression. Cdc34 levels are increased under conditions of DNA replication stress, suggesting that it plays an important role in coping with this type of genotoxic situation (Tkach et al. 2012).
GID8: Gid8 is part of another multiprotein complex that functions as an E3 ubiquitin ligase to ubiquitinate proteins to send them to degradation by the proteasome (Menssen et al. 2012).
UBP14: Ubp14 is a deubiquitinating protein that disassembles free poly-ubiquitin chains, thus controlling the rate of degradation by the proteasome (Amerik et al. 1997). Interestingly, Ubp14 collaborates with the Gid complex (Regelmann et al. 2003) and mutations in this gene are synthetic lethal with mutations in Cdc34 (Cocklin et al. 2011). UBP7: Ubp7 is another deubiquitination enzyme of unknown function.
PPS1: Pps1 is a phosphatase that plays a role during S-phase (Ernsting and Dixon 1997). Its targets remain unknown. SIS2: Sis2/Hal3 binds to the C-terminal catalytic domain of the serine/threonine phosphatase Ppz1 and strongly inhibits its activity (de Nadal et al. 1998). Decreased activity of Ppz1 leads to salt tolerance, compromised cell integrity and accelerated G1/S transition (Munoz et al. 2003;Posas et al. 1995). In addition, SIS2/HAL3 has a role in the biosynthetic pathway of coenzyme A, as part of a different complex, the PPCDC (phosphopantothenoylcysteine decarboxylase complex), which also includes the Cab3 and Vhs3 subunits (Ruiz et al. 2009). However, transformation of the elg1D srs2D strain with plasmids overexpressing these two subunits conferred no suppression. We thus conclude that it is likely that its interaction with Ppz1 phosphatase is the one responsible for the suppression (although we cannot rule out the possibility that Sis2, and only Sis2, is the limiting factor in the activity of the CoA synthesis complex). Overexpression of a phosphatase repressor may increase the level of a phosphorylated protein, which may be limiting in the elg1D srs2D strains.
tRNA splicing: Two genes were found, encoding successive steps in tRNA splicing. TPT1: TPT1 is an essential gene that encodes tRNA 29phosphotransferase, which catalyzes the final step of tRNA splicing (Culver et al. 1997). tRNA splicing is carried out by a multisubunit endonuclease, followed by ligation. Tpt1 catalyzes the transfer of the splice junction 2'-phosphate from the ligated tRNA to NAD to produce ADP-ribose 199-299 cyclic phosphate (Appr . p) (Culver et al. 1997). In a conditional lethal tpt1 mutant, 2'-phosphorylated tRNAs accumulate, and the tRNAs show altered posttranscriptional modification (Spinelli et al. 1997).
The significance of having found these two related enzymes in our screen is not clear. One possibility is that Appr1p or its derivatives may serve as signaling molecules in the cell, and an increase in its level may somehow be beneficial. We note that Tpt1 was identified as a histone H3-interacting protein (Gilmore et al. 2012).
Transcription factors: The genes in this category are as follows: CST6: CST6 was identified in a search for genes that are important for chromosome stability (CST genes) (Ouspenski et al. 1999). Interestingly, this screen also identified, among others, PAB1, as well as ubiquitin and histone genes (Ouspenski et al. 1999). Cst6 is a transcription factor activator, a member of the S. cerevisiae ATF/CREB family (Garcia-Gimeno and Struhl 2000). Its targets are still unknown. RFX1: RFX1 encodes the major transcriptional repressor of some DNA-damage-regulated genes. It helps recruit the repressors Tup1 and Cyc8 to the promoters of the relevant genes, such as the subunits of the ribonucleotide reductase enzyme. Upon DNA damage Rfx1 becomes phosphorylated and is released from the genes, allowing the recruitment of SAGA or TFIID subunits required for their expression (Ghosh and Pugh 2011). TAF3: Taf3 is a subunit of the TFIID complex, required for gene expression. It has lately been found that TFIID is preferentially recruited to promoters that lack TATA boxes, whereas SAGA binds preferentially TATA-containing regulatory sequences (Rhee and Pugh 2012).
The detection of these genes, involved in transcriptional regulation, as suppressors of the SL phenotype of elg1D and srs2D, implies that the suppression is possible by transcriptional activation or repression of target genes. However, the identity of the regulated genes, albeit, is still to be found.
Additional genes: BAP2: Bap2 encodes a high-affinity leucine permease that can also function as a branched-chain amino acid permease involved in the uptake of isoleucine and valine (Grauslund et al. 1995).

SRL3:
The SRL3 gene was identified in a screen for high copy number suppressors of the essential function of the DNA damage response genes MEC1 (ATR in humans) and RAD53 (CHK2) (Desany et al. 1998). Its exact function remains enigmatic. IRC9, IRC13: These two genes were identified in a screen for mutants exhibiting increased levels of Rad52 foci. Both are considered "dubious ORFs" by the Saccharomyces Gene Database (http://www. yeastgenome.org).
YOL114c: YOL114c is an uncharacterized ORF. YKL044w: This small ORF is present within the UTR of the PHD1 gene. Evidence for its being translated comes from ribosomal profiling experiments (Brar et al. 2012).
In summary, we have carried out a screen for genes that, when overexpressed, can suppress the SL of an elg1D srs2D strain. We did not isolate plasmids carrying the ELG1 or SRS2 genes; however, this is an expected result: overexpression of these genes is slightly toxic to the cells, and these genes tend to be underrepresented when screening high copy number libraries (Leon Ortiz et al. 2011;Parnas et al. 2009). The coverage used (.x20) allowed us to identify a relatively large number of candidate genes, which were confirmed one by one by re-cloning and re-testing. Although most genes were identified only once, several of the genomic regions were independently isolated several times, and some (e.g., PAB1) were identified six times. Thus, we are confident that our results represent a significant fraction of the genes that affect the genetic interactions between SRS2 and ELG1. It appears that there is a large number of ways in which the SL phenotype can be bypassed. Our results suggest that chromatin modification and sister chromatid cohesion are processes related to the function defective in elg1D srs2D double mutants. In addition, increased transcription/translation and nuclear export seem to be able to bypass the synthetic phenotype, possibly by affecting an effector protein(s). We believe that the results obtained from this overexpression screen will provide valuable information for further research needed to better understand the functions carried out by these genes and their interactions.