INTRODUCTION

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Saccharomyces cerevisiae adapts to changing environmental conditions by initiating new programs of gene expression that alter the normal progression of mitosis. Depending on cell type and nutritional cues, budding cells switch to a form of invasive pseudohyphal growth, mate to form diploids, stably arrest in stationary phase, or undergo meiosis to form spores (see reference 48, 50, 61, and 91 for reviews). Sporulation typically occurs in MATa/MAT diploids starved for nitrogen and glucose in the absence of a fermentable carbon source and involves the coordinated expression of over 500 genes (13, 63). Analysis of this process in yeast is providing important new insights into common strategies and components that regulate not only meiosis and gametogenesis but also cell proliferation and differentiation in multicellular organisms.

Meiosis-specific genes in yeast have been divided into several classes depending on their time of expression (13, 48, 84). UME6 is one of nine UME genes (UME1 to UME9) whose loss causes unscheduled meiotic expression of early meiotic genes during vegetative growth (76, 77; B. Washburn, unpublished data). Although it was originally identified as a transcriptional repressor of early genes, UME6 has also been shown to function in their meiosis-specific activation (9, 65, 74). UME6 encodes a C₆ zinc cluster protein that binds to the URS1 cis-elements found upstream of most early meiotic genes (2, 74, 77) and some middle and late meiotic genes (13, 63, 94). Work from several labs, as well as recent whole-genome analysis, has indicated that many nonmeiotic genes containing URS1 elements are also regulated by UME6 (19, 20, 47, 71, 77, 80; R. Williams, M. Primig, E. A. Winzeler, B. K. Washburn, R. W. Davis, and R. E. Esposito, unpublished data). These genes participate in a wide variety of metabolic pathways, including phospholipid biosynthesis, peroxisomal function, acetyl coenzyme A synthesis, nitrogen metabolism, and heat shock response. UME6 also participates in regulating genes that contain noncanonical URS1 elements, such as PHR1 and other DNA repair genes (79). Although Ume6 is required for normal repression and/or activation of genes in these various pathways, their regulation also usually involves a complex interplay of additional trans-acting and cis-acting factors which integrate the various signals influencing the expression of each particular set of genes.

Repression of meiotic gene expression by UME6 during vegetative growth involves the additional participation of SIN3 (UME4) and RPD3 (UME7) (8, 85, 86, 88; Washburn, unpublished). Aside from UME6, these are the only other UME genes whose loss leads to a nearly complete failure to sporulate (32, 76, 85). Recent studies have demonstrated that Sin3 and Rpd3 are components of a corepressor complex that represses transcription of many genes in yeast as well as higher eukaryotes. Sin3, which can act as a transcriptional repressor when fused to a DNA binding domain (42), contains four paired amphipathic helices thought to be involved in protein-protein interactions (43). It has been shown to interact with Ume6 in vivo and in vitro, indicating that Ume6 acts to recruit the Sin3 corepressor to early meiotic gene promoters (40). Sin3 appears to exert its effect on gene expression, at least in part, by altering chromatin structure through its association with Rpd3 (39, 66). Rpd3 is a histone deacetylase that genetically and physically interacts with Sin3 in yeast (40, 43), and this interaction has been shown to result in the deacetylation of one to two nucleosomes at the Ume6-binding site (41, 66).

Sin3 and Rpd3 homologs also provide a similar repression function in multicellular organisms. In mammalian cells, corepressor complexes containing homologs of Sin3 (mSin3a or mSin3b) and Rpd3 (HDAC1p or HDAC2p) are involved in regulation of transcription by a number of important systems, including the nuclear hormone receptors (reviewed in reference 26) and the Max-interacting members of the Myc/Mad/Max family of basic helix-loop-helix-leucine zipper (bHLHZip) transcription factors (Mad1, Mad3, Mad4, Mxi, and Mnt[Rox] [reviewed in reference 57]). Like Ume6, the nuclear hormone receptors and Myc/Mad/Max families participate in both activation and repression of genes involved in differentiation and development (reviewed in references 14, 31, and 82; see also Discussion).

In yeast meiosis, the conversion of Ume6 from a repressor to an activator of early meiotic gene expression is critical for induction of the early genes and for the progression of meiosis. The switch in Ume6 activity requires the presence of Ime1 (inducer of meiosis), which accumulates to high levels very early in sporulation (9, 65, 74). Ime1 is known to function as an activator of transcription when fused to a DNA binding domain (56, 72) and, like Sin3, has been shown to interact with Ume6 in two-hybrid assays (65). Thus, one function of Ime1 is apparently to provide an activation domain to Ume6, allowing it to be converted to an activator. This interaction is facilitated by phosphorylation of the Ume6 amino terminus by either Rim11 or Mck1 (65, 93).

Taken together, these findings have led to the current view of Ume6 as a multifunctional DNA-binding protein component of transcriptional regulatory complexes, capable of alternately repressing or activating early meiotic transcription through its association with Sin3 or Ime1, respectively. The function and regulation of these interactions are further addressed below. In this study, we observed that fusion of a heterologous activation domain to Ume6 fails to convert it to an activator of early gene expression during vegetative growth. We took advantage of this behavior to isolate mutations in UME6 that allow the fusion to function as an activator. These mutations disrupt interaction with Sin3 in vivo and in vitro and identify the Sin3 binding domain of Ume6, the first target binding sequence for Sin3 defined in yeast. These mutations were used to further investigate the function and regulation of the Sin3-Ume6 interaction during vegetative growth and meiosis.

	MATERIALS AND METHODS

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Strains. All yeast strains used in genetic studies are closely related to W303 (81). SFY59 (MATa ade2 ade6 can1-100r his3-11,15 leu2-3,112 trp1-1 ura3-1) and YC105 (MATa ade2 ade6 can1-100r his3-11,15 leu2-3,112 trp1-1 ume6-1 ura3-1) were derived from W303 as previously described (74). YC121 (MAT ade2 can1-100:ADE2:CAN1 his3-11,15 leu2-3,112 trp1-1 ume6-1 ura3-1) was derived from W303 by insertion of the ume6 and can1-100:ADE2:CAN1 cassettes as previously described for YC122 (74). REE3574 (MATa ade2 ade6 can1-100r his3-11,15 leu2-3,112 trp1-1 ume6::KanMX ura3-1) was constructed by replacement of the UME6 open reading frame (ORF) in SFY59 with a KanMX6 cassette, using the short flanking PCR-generated homology (87). Isogenic derivatives of this strain containing UME6 (REE4175), ume6-6 (REE4178), ume6-7 (REE4181), ume6-9 (REE4184), ume6-6,9 (REE4187), and ume6-7,9 (REE4190) were produced by transformation with the integrating plasmids pBK100, pBK102, pBK103, pBK104, pBK105, and pBK106, respectively (see below), cut with PacI to select for integration adjacent to ume6::KanMX (64). An isogenic sin3 strain (REE4123) was similarly derived by integration of UME6 into REE3575 (MATa ade6 can1-100r his3-11,15 leu2-3,112 trp1-1 sin3::HIS3 ura3-1 ume6::KanMX). REE2276 (MATa ade2 ade6 can1-100r his3-11,15 ime1::URA3 leu2-3,112 trp1-1 ura3-1) was constructed by insertion of an ime1::URA3 disruption into SFY59, and REE3086 (MAT ade2 ade6 can1 his3 his4 leu2 trp1 ura3 ime1::URA3) was derived from outcrosses with W303.

trp1-901 leu2-3,112 ura3-52 his3-200 gal4 GAL80 GAL-ADE2 LYS2

GAL7-lacZ rpd3

Plasmids. pBK8 carries two SPO13 fusions, SPO13-URA3 and SPO13-lacZ, on a single 2µm TRP1 plasmid. Each fusion contains 847 to +45 of the SPO13 gene and exhibits meiosis-specific regulation similar to that of SPO13. pBK8 was constructed by inserting a BamHI fragment containing SPO13-lacZ (10) into the unique BglII site of pPL128 (provided by R. Surosky, this lab), which contains the SPO13-URA3 fusion from pMS49 (77) inserted into YEp13. The wild-type UME6 plasmid pPL5905 carries UME6 on a centromeric (CEN) LEU2 vector (77). pBK54, a ume6-6 derivative of this plasmid, was produced by swapping the BamHI-StuI and BssHII-SalI UME6 fragments, respectively, from pGAD-ume6-6 into pPL5905. Integrating UME6 and ume6-6 plasmids (pBK100 and pBK102, respectively) were constructed by cloning the SpeI-SalI UME6 fragments from pPL5905 and pBK54, respectively, into pRS305 (69). Integrating ume6-7, ume6-9, ume6-6,9, and ume6-7,9 plasmids (pBK103-106) were derived from pBK100 and pBK102 by swapping appropriate restriction fragments from the GAD-ume6 mutants.

Yeast and E. coli methods. Growth and sporulation media have been previously described (45). Yeast strains were transformed by the lithium acetate method (25), and E. coli strains were transformed by electroporation (Bio-Rad).

-Galactosidase assays. For plate assays, yeast cells were grown on paper filters (3MW; Midwest Scientific) overlaid on agar medium selective for the plasmids. Filters were then frozen in liquid nitrogen and placed on agar containing 5-bromo-4-chloro-3-indolyl--D-galactopyranoside (X-Gal) (76). After 2 to 36 h, color development was stopped by air drying. For determination of -galactosidase activity due to activation of SPO13-lacZ expression by GAD-Ume6 derivatives in liquid cultures, at least three independent transformants were grown to an optical density at 600 nm of 0.7 to 0.75 in synthetic dextrose medium and collected by centrifugation. Colorimetric assays of lysates obtained by bead beating were then performed with o-nitrophenyl--D-galactopyranoside (ONPG) as previously described (10). For determination of -galactosidase activity due to derepression of SPO13-lacZ by ume6 mutations, at least two independent transformants were grown on selective agar medium and lysed in Y-PER buffer (Pierce), and activity was determined using the reagents and protocols in the Pierce yeast -galactosidase activity kit.

Two-hybrid screen and assays. The two-hybrid strain and plasmids used to identify Ume6 interactors have previously been described (38). The PJ69-4A reporter strain was modified by replacement of the RPD3 ORF with KanMX6 (above), in order to alleviate repression of the reporters by the GAD-UME6 bait. Approximately 2 million transformants for each of the three reading frame Gal4 activation domain fusion libraries were plated to His medium. His⁺ transformants (~1,000) were replica plated to Ade medium, and His⁺ Ade⁺ isolates were then tested for bait dependence. Six bait-dependent clones were obtained. DNA sequencing (Applied Biosystems Inc.) indicated that four isolates encoded Tea1 fusions, and two encoded identical Sin3 fusions. A Sin3 paired amphipathic helix 1 (PAH1) deletion (amino acid residues 238 to 295) was derived from the Sin3 library clone by removal of the internal BspEI fragment. A deletion of the entire Sin3 PAH2 region (residues 290 to 670) was constructed by removal of the internal BsmI-PstI fragment, followed by treatment with T4 polymerase and ligase. The more precise PAH2 deletion (residues 424 to 450) was from plasmid M1285 (90), inserted on a BsmI-CelII fragment. All Sin3 deletion constructs were sequenced to verify intact reading frames.

Ume6 mutagenesis and mapping. Plasmid DNA was mutagenized by growth in the bacterial mutator strain XL1-Red (Stratagene) and used to transform wild-type yeast (SFY59) containing pBK8 (SPO13-lacZ SPO13-URA3). Ura⁺ Lac⁺ transformants were selected as described in Results. Restriction fragment swaps between mutant and wild-type parent plasmids were used to localize the mutations in UME6 responsible for causing activation of SPO13. Of the 10 mutations mapped, 9 localized to a 157-bp EcoRI-StuI fragment encoding amino acids 508 to 560 of Ume6, and one mutation localized to a PvuII-AlwNI fragment encoding amino acids 593 to 659. Sequencing of the indicated fragments indicated that none contained multiple mutations.

GST pulldowns. GST-Ume6 fusion plasmids were constructed by in-frame fusion of the PvuII-EcoRI fragment encoding amino acids 508 to 584 of Ume6 to GST in pGEX-KG (29). Plasmid M1155, containing ADH1-HA (hemagglutinin)-SIN3, was obtained from David Stillman (43). For production of GST-Ume6 fusion proteins in bacteria, E. coli BL21 containing GST-Ume6 fusions (Ume6 amino acid residues 508 to 584) was grown to an optical density at 600 nm of 0.5 at 37°C, and expression of the fusions was induced with 0.1 mM isopropyl--D-thiogalactopyranoside for 3 h. Cells were collected by centrifugation, and the pellet from 40 ml of cells was resuspended in 500 µl of bacterial lysis buffer (phosphate-buffered saline [PBS] containing 1 mM phenylmethylsulfonyl fluoride, 1 mM EDTA, and 1.5 µg of leupeptin/ml). Lysates were prepared by sonication. For production of yeast lysates containing HA-tagged Sin3, BJ2168 containing the Adh1-HA-Sin3 plasmid M1155 (43) was harvested at a density of 10⁷ cells/ml. Lysates were prepared by bead beating in 300 µl of yeast lysis buffer (20 mM Tris, 150 mM NaCl, 10 mM MgCl₂, 5% glycerol, 1 mM phenylmethylsulfonyl fluoride, 1 µM aprotinin, leupeptin [1.5 µg/ml], pepstatin A [3 µg/ml], chymostatin [1 µg/ml]).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Addition of an activation domain to Ume6 is not sufficient to convert it to an activator. Two-hybrid studies have indicated that Ime1 physically interacts with Ume6, providing a transcriptional activation domain for the induction of early meiotic gene expression (55, 65). If the only requirement for conversion of Ume6 from a repressor to an activator is the addition of an activation domain, one might predict that fusion of a heterologous activation domain to Ume6 would cause it to function as a constitutive activator of SPO13 and other early meiotic genes during vegetative growth (i.e., in the absence of Ime1 induction). The ability of such heterologous activation domains to activate transcription of reporter genes when linked to appropriate DNA-binding proteins is fundamental to the widespread success of yeast two-hybrid systems (6).

View larger version (19K): [in this window] [in a new window]   FIG. 1.   Activation of SPO13 expression by wild-type and mutant GAD-Ume6 fusions. A wild-type haploid (SFY59) containing pBK8 (SPO13-URA3 SPO13-lacZ) and UME6 plasmids was replica plated to either Ura medium or filters on X-Gal medium to detect expression of SPO13. (A) Comparison of SPO13 activation by wild-type (GAD-UME6; lane 1) and mutant (GAD-ume6-6; lane 4) fusions, and wild-type (pPL5905; lane 2) and mutant (pBK54; lane 3) UME6, in the absence of GAD. (B) Activation by GAD-UME6 derivatives lacking the Ime1 binding domain. Fusions contain either full-length UME6 (lane 1) or ume6-6 (lane 3), or derivatives of each (lanes 2 and 4, respectively) lacking the first 158 amino acids of Ume6. Deletions derivatives were created by cutting the parent plasmids with BamHI and religating, thus removing the coding region between the polylinker at the GAD-UME6 junction and UME6 nucleotide +474.

Isolation of mutations that allow activation by GAD-Ume6. To identify amino acid residues in Ume6 involved in regulating its conversion to an activator, mutations in GAD-UME6 that led to expression of SPO13 during vegetative growth were sought. These mutants were selected by transforming a wild-type haploid, containing SPO13-URA3 and SPO13-lacZ fusions, with a pool of mutagenized GAD-UME6 plasmid. Ura⁺ transformants were selected and then screened for -galactosidase activity to identify mutants exhibiting high-level expression of SPO13; 115 Ura⁺ Lac⁺ transformants were obtained from a population of ~10⁶ transformants. Since the Gal4 activation domain and Ume6 DNA binding domain are located at opposite ends of the GAD-Ume6 protein and are both required for activation of the reporters, this collection of mutants should not include simple loss-of-repression alleles resulting from frameshifts leading to a truncated protein or from mutations that cause a loss of transcription of UME6 or translation of the UME6 message or decreased Ume6 stability.

View larger version (25K): [in this window] [in a new window]   FIG. 2.   Activation of SPO13-lacZ expression by mutant GAD-Ume6. ONPG liquid assays of -galactosidase (gal) activity in a wild-type haploid (SFY59) containing pBK8 (SPO13-URA3 SPO13-lacZ) and plasmids carrying GAD, GAD-UME6, and various GAD-ume6 mutant fusions (denoted by the amino acid alteration [Fig. 3]) were performed as described in Materials and Methods. The M530T, L527P, S528P, and K635E alleles have been designated ume6-6, ume6-7 ume6-8, and ume6-9, respectively.

The mutations allowing activation cluster in a region of UME6 predicted to encode an amphipathic  helix. The locations of ume6-6 and the nine other mutations were determined to identify possible functional domains. As shown in Fig. 3A, ume6-6 (M530T) and all but one of the other nine mutations localized to an eight-amino-acid sequence (residues 523 to 530) in the central part of the protein. This sequence is within the only region of Ume6 (residues 508 to 584) previously identified as being sufficient for Sin3 binding and for conferring repression when fused to LexA (40). Sequence analysis indicates that this cluster of mutations lies within a region, residues 516 to 530, that is predicted to adopt an -helical configuration. This is also one of the few hydrophobic regions of an unusually hydrophilic protein (2). When displayed as a helical wheel plot (Fig. 3B), the hydrophobic residues appear to be distributed in an amphipathic pattern (i.e., one face of the helix is predominantly hydrophobic and the opposite face is predominantly hydrophilic). The nature of the ume6 mutations recovered in this study supports the conclusion that the ability of this region to adopt an amphipathic -helix configuration is important for repression by Ume6. Except for the M530V substitution, all of the mutations in the predicted  helix either change an amino acid residue on the hydrophobic face to hydrophilic (A523S, A524T, A525, V526Q, and M530T) or introduce a proline (L527P and S528P), which is expected to disrupt the  helix. The unusual deletion of an alanine at position 525, resulting from the loss of a single CAG triplet in a (CAG)₄ repeat, is predicted to cause a hydrophilic amino acid (S528) to shift into a position on the hydrophobic face previously occupied by a hydrophobic amino acid (L527).

View larger version (20K): [in this window] [in a new window]   FIG. 3.   Mutations in UME6 allowing activation by GAD-UME6. (A) Map of UME6 showing locations of mutations and predicted structure. Overall sequence predictions were by the Chou-Fasman method, performed by the Protean sequence analysis program (DNASTAR). The more detailed presentation of the  helix predicted from 516 to 530 (top) is the consensus of four prediction methods (16, 22-24, 52). Mutations are denoted as arrows. Regions known to contain the Ime1 binding domain (BD) (65), Sin3 binding domain (40), and C6Zn DNA binding domain (77) are indicated as boxes. (B) Helical wheel diagram of the predicted  helix (residues 516 to 530 are shown) showing locations of mutations. The curved arrow indicates the shift in position of amino acid 528 resulting from the deletion of amino acid 525.

Mutations in the  helix interfere with the ability of Ume6 to interact with Sin3. Two-hybrid assays were used to test the ability of Ume6-6 to form stable complexes in vivo. For these experiments, full-length Ume6 was fused to the Gal4 DNA binding domain as bait. The interactions were tested using two Gal4 activation domain fusions that we isolated from a two-hybrid screen designed to identify Ume6 interactors (see Materials and Methods). The first of these interactors is Sin3. The interaction of Sin3 with Ume6 had previously been demonstrated in a pairwise two-hybrid test and with GST pulldown assays (40). Our recovery of Sin3 in this screen provides additional evidence for the interaction of Sin3 and Ume6 in vegetatively growing yeast cells. The second gene isolated from this screen was TEA1. Like UME6, TEA1 encodes a C₆ zinc cluster DNA-binding protein. Tea1 has been shown to bind a cis-element in the Ty enhancer and is required to achieve full levels of Ty enhancer-mediated transcription (28). The nature of the relationship between Ume6 and Tea1 is the subject of a separate study (Washburn, unpublished).

View larger version (56K): [in this window] [in a new window]   FIG. 4.   Two-hybrid analysis of Ume6 interactions, using an rpd3 derivative of PJ69-4A containing GBD-Ume6 baits and either GAD-Sin3 or GAD-Tea1 library clones. (A) Interaction between Ume6 and library clones is shown by growth on Ade medium resulting from expression of the GAL2-ADE2 reporter. (B) Interaction between GBD-Ume6 with deletion derivatives of GAD-Sin3, shown by growth on His medium resulting from expression of the GAL1-HIS3 reporter.

View larger version (44K): [in this window] [in a new window]   FIG. 5.   GST pulldown assay. HA-Sin3 from yeast extracts was bound to GST (lane 1) or GST fused to amino acids 508 to 584 of wild-type (wt; lane 2) or mutant (lanes 3 to 8) Ume6 as described in Materials and Methods. A single HA-Sin3 lysate was evenly divided among the tubes (500 µg each). Complexes were eluted with boiling loading buffer, separated by SDS-polyacrylamide gel electrophoresis and visualized with anti-HA antibodies (top) to assay Sin3 interaction or Coomassie (bottom) to verify equivalent amounts of GST-Ume6 fusion in each sample. Several presumed GST-Ume6 degradation products uniformly appear (as previously observed [55]) in all of the GST-Ume6 lanes.

Ume6 interacts with the PAH2 region of Sin3. Having identified the region of Ume6 that interacts with Sin3, it was of interest to identify the corresponding region in Sin3 that interacts with Ume6. Sin3 contains four paired amphipathic helices (PAH1 to PAH4) which have been proposed to be involved in protein-protein interactions (43). Sin3 is now known to interact with several corepressors in higher eukaryotes, through a variety of contact points (1, 3). We found that both of the Ume6-interacting Sin3 clones isolated from the two-hybrid screen encoded fusions to Sin3 amino acid residues 228 to 671 and therefore contain only PAH1 (residues 238 to 285) and PAH2 (residues 426 to 472); PAH3 and PAH4 are predicted to start at residues 680 and 1153, respectively (88). The region of Sin3 required for interaction with Ume6 was further determined by deletion analysis of the GAD-Sin3 clones. These studies showed that removal of residues 238 to 295, encompassing PAH1 in Sin3, has no effect on its ability to interact with Ume6 (Fig. 4B, lane 4). Thus, neither PAH1, PAH3, nor PAH4 in Sin3 is required for interaction with Ume6. That PAH2 is necessary for the interaction was initially suggested by the finding that deletion of residues 290 to 670 abolishes the interaction (Fig. 4B, lane 2). A more precise deletion specifically localized within PAH2 (residues 424 to 450; lane 3) confirmed this conclusion. Among known Sin3-binding proteins, the Max-interacting proteins, which as described above also contain a Sin3 binding domain with some similarity to that of Ume6, have also been shown to interact with PAH2 of yeast Sin3 (42) and mammalian Sin3 homologs (5, 18, 35, 59, 68).

Premature expression of Ume6-Sin3-regulated meiotic genes is not detrimental to subsequent sporulation. As shown above, the mutant GAD-ume6 fusions cause early meiotic genes to be expressed during vegetative growth, whereas normally the early genes are not induced until several hours after the initiation of meiosis. The three regulators whose loss leads to the highest level of derepressed early meiotic gene expression (ume6, sin3, and rpd3) also confer a severe sporulation defect (32, 76, 85). Until now it has been difficult to determine whether premature expression interfering with meiotic progression is a cause of the Spo defect of these strains and/or whether it due to other meiotic roles of these genes, such as Ume6 function in activation. The properties of the GAD-ume6-6 fusion provided a convenient tool to address this question. As described above, the introduction of a GAD-ume6-6 plasmid into an otherwise wild-type strain (i.e., UME6⁺ SIN3⁺ RPD3⁺) results in vegetative expression of the early genes, similar to the levels observed in sin3 and rpd3 mutants. If premature expression of early meiotic genes is responsible for the sin3 and rpd3 sporulation defects, then dominant overexpression of the early genes conferred by GAD-ume6-6 is expected to inhibit sporulation. As shown in Fig. 6, wild-type diploids containing GAD-ume6-6 (column 3) sporulate as efficiently as strains containing the wild-type GAD-UME6 fusion (column 2) or no fusion at all (column 1). We thus conclude that premature expression of the early genes alone does not interfere with subsequent sporulation and is therefore an unlikely explanation for the inability of sin3 and rpd3 mutants to sporulate.

View larger version (21K): [in this window] [in a new window]   FIG. 6.   Sporulation of strains containing fusions of the Gal4 activation domain to UME6 or ume6-6. A wild-type diploid (W303a/; lanes 1 to 3) or ime1 diploid (REE2276/REE3086; lanes 4 to 6) was transformed with GAD, GAD-UME6, or GAD-ume6-6 plasmids. Transformants were replica plated to sporulation medium, and asci were counted after 5 days at 37°C.

Activation of early meiotic gene expression by GAD-ume6-6 can partially substitute for Ime1. Since the GAD-ume6-6 mutant exhibits a dominant gain of vegetative activation function, it seemed plausible that in the absence of Sin3 binding, high-level activation of early gene transcription by the Gal4 activation domain might be able to substitute for Ime1 in sporulation. To test this, an ime1 diploid was transformed with GAD fusion plasmids and transformants were tested for the ability to sporulate. As shown in Fig. 6, the GAD-ume6-6 plasmid (column 6) conferred a significant level of sporulation in the absence of Ime1 (~25% of the wild-type level), in contrast to plasmids containing GAD (column 4) or the wild-type GAD-UME6 fusions (column 5). Thus, the addition of a functional heterologous activation domain to Ume6-6 can partially substitute for the presence of Ime1 in meiosis. Although the sporulation level afforded by GAD-ume6-6 is less than in the wild-type level (columns 1 to 3), this difference may be explained by the poor expression of the ADH1-GAD-ume6-6 fusion in meiosis (65). The failure of a wild-type GAD-UME6 fusion to promote sporulation in an ime1 strain implies that the Sin3-Ume6 interaction resulting in repression persists in the absence of Ime1 even after the shift to sporulation medium. Taken together, these data suggest that in wild-type strains, Ime1 may play a dual role in relieving Sin3-mediated repression as well as providing an activation domain (see Discussion).

Mutations in the  helix cause a loss of repression by Ume6. The experiments above indicate that ume6-6 and the other mutations in the  helix allow a GAD-ume6 fusion to activate gene expression by interfering with the ability of Sin3 to bind Ume6. Therefore, these mutants should exhibit a repression defect in the absence of the Gal4 activation domain. This was tested by introducing the mutations into otherwise wild-type UME6 (lacking GAD) on CEN plasmids and transforming a diploid ume6/ume6 mutant. As shown in Fig. 7, all of the mutations tested cause a loss of repression by Ume6. Like the uncomplemented ume6 mutant containing only vector (lane 1), ume6 cells containing ume6-6 and the other mutant ume6 alleles (lanes 3 to 6) are Ura⁺, indicating that expression of SPO13-URA3 is derepressed.

View larger version (43K): [in this window] [in a new window]   FIG. 7.   Complementation of a ume6 diploid by UME6 plasmids. Vegetative derepression and sporulation in a ume6 diploid (YC105/YC121) containing pBK8 and either vector (pRS315; lane 1), wild-type (WT) UME6 plasmid (pPL5905; lane 2), or mutant derivatives of pPL5905 containing the indicated mutations in the  helix (lanes 3 to 6). Lanes 4 and 5 represent two independent isolates of the L527P mutation.

sin3

ume6

View larger version (37K): [in this window] [in a new window]   FIG. 8.   Derepression of SPO13 expression in chromosomal ume mutants. Strains containing UME6, ume6::KanMX, ume6-6, ume6-7, ume6-9, ume6-6,9 and ume6-7,9, or sin3 were constructed as described in Materials and Methods. (A) Plate assays of SPO13-URA3 and SPO13-lacZ expression. (B) Quantitative -galactosidase (-gal) assays of SPO13-lacZ expression of cells grown on plates, normalized to wild-type levels.

The Ume6-Sin3 interaction is not required for sporulation. sin3 mutants were previously shown to be Spo, and it was initially proposed that their failure to sporulate might be due to premature expression of the early genes (76). The results described above indicate that this explanation is unlikely to be correct. Since both sin3 and rpd3 mutants show a failure to rerepress the early genes later in meiosis (32), an alternative hypothesis is that the Spo defect is due to the absence of repression, which may be necessary for meiotic progression. The process of restoring the early meiotic genes to the repressed state is expected to require binding of Sin3 to Ume6, presumably using the same mechanisms as employed for vegetative repression. Another possibility is that Sin3, like Ume6, is involved in activation of meiotic gene expression as well as repression. If so, this activation pathway may also involve interaction with Ume6.

ume6

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

This study addresses the mechanism by which Ume6 switches from a repressor to an activator of meiosis-specific genes and the role of Sin3-mediated repression in the regulation of meiosis by Ume6. Prior studies have shown that Ume6 binds to URS1 elements in the promoters of early meiotic genes (2, 77) and that UME6 and URS1 are both required for repression as well as activation (8, 9, 74, 77). Ume6-mediated activation is known to be dependent on interaction with Ime1 (65), which does not bind to DNA on its own but exhibits activation function when fused to LexA (72) or the Gal4 DNA- binding domain (56). It has therefore been proposed that one role of Ime1 is to provide an activation domain to the Ume6 complex (9, 65, 74). This model gained support from the finding that a GAD-UME6 fusion was able to cause Ime1-independent vegetative activation of the early meiotic gene HOP1 (65). We constructed a similar GAD-UME6 fusion in the course of our two-hybrid studies, using a weaker ADH1 promoter variant to alleviate the poor viability resulting from high-level overexpression of GAD-Ume6 from the stronger ADH1 promoter construct (see Materials and Methods) and found that it did not activate transcription of HOP1 or SPO13. For this fusion the repression activity provided by the Sin3 binding domain appeared to be dominant and in that respect similar to Sin3 interaction domains in other proteins (4, 30, 35, 42) as well as to direct fusions of activation domains to yeast Sin3, which fail to activate transcription (44). The only critical difference between the constructs in the two studies appears to be the promoters used to express the GAD-Ume6 fusions. The possibility that variations in the GAD-Ume6 protein sequence are responsible was excluded by demonstrating that the coding region from the wild-type Ume6 fusion used in this study can activate expression of SPO13 and HOP1 when moved into the expression plasmid used by Rubin-Bejerano et al. (not shown). We further determined that neither the strains or lacZ reporters used in the two studies can account for the different results, since the GAD-Ume6 fusion used in the previous study (65) activates the same reporter fusions and strains that fail to be activated by the GAD-Ume6 fusion used in this study (not shown). The analysis of ume6 mutants in this study indicates that the higher level of GAD-UME6 expression from the stronger ADH1 promoter variant used by Rubin-Bejerano et al. may exceed the steady-state levels of Sin3 available to bind to Ume6, thereby allowing activation.

Our finding that fusion of the Gal4 activation domain to Ume6 fails to activate early meiotic genes (e.g., SPO13 and HOP1) indicated that an additional function that cannot be substituted for by Gal4 is required. Here we provide evidence indicating that two genetically separable stepsrelief of Sin3-mediated repression and addition of an activation domainare involved in conversion of Ume6 to an activator. When ume6 mutations that disrupt Sin3-Ume6 interaction are introduced, GAD-Ume6 can function as a transcriptional activator of meiosis-specific genes. Furthermore, GAD-Ume6 under these conditions can substitute for the presence of Ime1 in meiosis.

The Sin3 binding domain in Ume6. Prior two-hybrid and GST pulldown assays localized the Sin3 binding domain in Ume6 to the region between amino acid residues 508 and 584 (40). The mutant analysis described in this study has now allowed the domain to be precisely mapped to sequences within a predicted amphipathic helix encoded by amino acid residues 515 to 530. Although Sin3 was first identified in yeast (75, 89) and has mammalian homologs and binding partners that are currently the subject of extensive investigation, this is the first time a Sin3 interaction site in a yeast protein has been defined. Here we show that the Ume6 amphipathic helix that binds Sin3 is similar in structure, but not sequence, to the amino-terminal Sin3 binding domains of Mad1 and other mammalian Max-interacting bHLHZip proteins (reviewed in reference 57). These proteins also resemble Ume6 in that their repression domains interact with Sin3 PAH2 and are dominant with respect to linked activators (42, 57). At present, Sin3 PAH2 is also thought to interact with as many as six other yeast proteins (STB1 to STB6) (44), but none of these proteins appear to contain strong homologies to the Sin3 binding domain in Ume6. Therefore, if any of them interact with Sin3 PAH2 by a direct physical contact, they may do so by a mechanism that differs from that used by Ume6. Intriguingly, one yeast protein that shows significant homology to the Ume6 Sin3 binding domain is the DNA-binding protein Sum1. Six of eight consecutive amino acids within a predicted  helix in Sum1 are identical to the critical eight-amino-acid Sin3 binding sequence (residues 523 to 530) in the Ume6  helix. Both Sum1 and Sin3 have been implicated in DNA silencing (12, 83), and both were identified as regulators of middle gene expression (32, 94). The possibility that Sum1, like Ume6, recruits Sin3 to repress transcription is currently being investigated. In higher eukaryotes, aside from the Max-interacting proteins, most of the proteins that appear to interact directly with Sin3 (including the Krüppel-like transcriptional repressors Laz3 [BCL6] and PLZF, the corepressors NCoR and SMRT, Sin3-associated polypeptides SAP18 and SAP30, and Rpd3 histone deacetylase homologs) do so through regions other than Sin3 PAH2 (15, 17, 49, 92, 95). Although the precise sequences through which most of these proteins make contacts with Sin3 are not yet known, current indications suggest that multiple mechanisms are involved.

What is the role of Ime1 in conversion of Ume6 to an activator? Our analysis of GAD-Ume6 fusions has indicated that the conversion of Ume6 to an activator requires two steps that are genetically separable: (i) relief of Sin3-mediated repression and (ii) introduction of an activation domain. We propose that for wild-type Ume6, Ime1 is essential for both processes. With regard to the derepression step, there are two lines of evidence that support the idea that Sin3 remains present and functional in the nucleus when Ume6 is actively promoting transcription, and that it must be inactivated or physically removed from Ume6 by an Ime1-dependent mechanism for activation to occur. First, wild-type GAD-UME6 is unable to promote sporulation if Ime1 is absent but can do so if the Sin3 binding site is disrupted (Fig. 6). This indicates that the Sin3 protein is normally still present during meiosis and that if an activation domain is added to Ume6, Ime1 is dispensable only if repression is also removed (i.e., ume6-6). Second, it is well established that vegetative expression of Ime1 under control of the GAL1 promoter can cause activation of early meiotic genes in vegetative cells, when Sin3 normally functions in repression of transcription (73).

ime1

View larger version (22K): [in this window] [in a new window]   FIG. 9.   Transcriptional regulation by Ume6, nuclear hormone receptors, and Myc/Mad/Max. DNA-binding proteins (Ume6, nuclear hormone receptors [NHR], or Max heterodimer) in conjunction with cis-acting DNA elements (e.g., URS1, hormone response element [HRE], or E box, as indicated), repress transcription through interaction with a corepressor complex containing Sin3, Rpd3, and additional proteins (not all are shown). In each system, the switch from repression to activation requires that the Sin3 corepressor complex be replaced by an activation complex. In meiosis, this involves the binding of Ime1. For NHR, this involves binding of hormone and a number of potential coactivators (not all are shown) including histone acetylases (HAT) (see references 26, 31, and 82 for reviews). For Max, it involves heterodimerization with Myc, which possesses a transactivation domain that may act through a variety of additional proteins (14, 31, 58).

UME6-dependent and UME6-independent roles of SIN3. In the absence of the Gal4 activation domain, mutations in the potential amphipathic  helix (e.g., ume6-6 [M530T], ume6-7 [L527P], and ume6-8 [S528P]) result in a partial loss of repression to a level similar to a deletion of SIN3, as expected for Ume6 mutants that have lost the ability to interact with Sin3. Since the level of derepression that occurs in sin3 and the ume6 Sin3-binding-domain mutants is less than occurs in ume6 or URS1 mutants, we have concluded that Ume6 must have a repression function at early meiotic promoters that is independent of Sin3. A similar Sin3-independent repression function is seen at the nonmeiotic INO1 promoter, which shows a much higher level of derepression when URS1 or Ume6 is mutated than when SIN3 is deleted (20, 70). The repression conferred by Ume6 in the absence of Sin3 may result from either a Sin3-independent repression site in Ume6 (e.g., perhaps defined by ume6-9/K635E, the derepressing mutation that lay outside the  helix) or simply to the binding of Ume6 to URS1, excluding binding of other activators to URS1 or nearby sequences (21, 80). Ume6-dependent Sin3-independent repression probably does not involve Sin3-independent recruitment of Rpd3, since activity of Rpd3 at URS1 has been shown to require the presence of Sin3 (40, 85). Recent studies suggest that a likely mechanism for Sin3-independent repression of SPO13 by Ume6 may involve the Isw-2 chromatin remodeling complex, which has now been shown to bind to Ume6 and repress transcription independently of Sin3 (27).