(Received for publication, October 21, 1996, and in revised form, February 11, 1997)
From the Department of Biochemistry and Biophysics
and the § Department of Microbiology and Immunology,
University of California, San Francisco, California 94143-0414
The Saccharomyces cerevisiae Tup1 protein is a member of a family of WD repeat containing proteins that are involved in repression of transcription. Tup1, along with the Ssn6 protein, represses a wide variety of genes in yeast including cell type-specific and glucose-repressed genes. Tup1 and Ssn6 are recruited to these specific gene sets by interaction with sequence-specific DNA binding proteins. In this work, a protein complex containing Ssn6 and Tup1 was purified to determine its composition. The size of the complex is estimated to be 440 kDa. Tup1 and Ssn6, which are both phosphoproteins, are the only proteins present in stoichiometric amounts in the complex. We also demonstrate that this purified complex represses transcription in an in vitro assay.
The Tup1 protein of Saccharomyces cerevisiae is one of
a family of repressor proteins that contain -transducin or WD
repeats. The majority of the WD repeat containing proteins are homologs of
-transducin and are known to function in signal transduction pathways within the cytoplasm. However, an increasing number of WD
repeat proteins have been identified that are nuclear localized and
function in the repression of transcription. These include Tup1, Hir1,
and Met30 in S. cerevisiae; SCON2 in Neurospora
crassa; extra sex combs and groucho in Drosophila; COP1
in Arabidopsis thaliana; and HIRA and the family of TLE
proteins in humans (1-10). These WD repeat repressor proteins turn off
a wide variety of genes, including those involved in segmentation, sex
determination, and neurogenesis (controlled by groucho) and those
involved in photomorphogenesis (controlled by COP1) (7, 11). The HIRA protein has been implicated in the human developmental disease DiGeorge
syndrome (8, 9).
Of these WD repeat repressor proteins, Tup1 is the best characterized.
Tup1 along with another protein, Ssn6, is required for the repression
of at least five sets of genes in yeast, including the
glucose-repressed genes, genes regulated by the presence of oxygen
(hypoxic genes), the a-specific and haploid-specific genes,
and a set of genes induced by DNA damage (12-16). A deletion of
SSN6 or TUP1 results in the constitutive
expression of all of these genes sets. Tup1 and Ssn6 are recruited to
these specific gene sets by interaction with sequence-specific DNA
binding proteins. In the case of the a-specific and
haploid-specific genes in yeast, the homeodomain protein 2 binds to
sequences (operators) located upstream of each gene in the set and
recruits Ssn6 and Tup1 by direct interaction with each of these
proteins (for review, see Ref. 17).
Tup1 and Ssn6 interact directly in vitro and are found associated in a large complex in yeast extracts estimated at 1.2 MDa (18). The size of this complex suggests that it consists of many protein subunits. Genetic experiments have implicated a number of additional proteins in the Ssn6-Tup1 repression pathway including Rox3, Sin4, Srb8, Srb9, Srb10, and Srb11 (19-23). Each of these proteins is required for full repression of transcription by Tup1 and Ssn6 in vivo. To determine the subunit composition of the Ssn6-Tup1 complex, we purified the complex, determined its size, characterized its components, and demonstrated its activity in an in vitro repression assay.
The Ssn6HIS construct is comprised of
the 3 1000 base pairs of the SSN6 coding sequence fused to
6 histidine codons followed by a stop codon in the vector pRS304 (24).
The final construct was sequenced (U. S. Biochemical Corp.) and
integrated into the yeast genome at the native SSN6 locus
resulting in the SSN6HIS fusion gene and a duplication of
the last 1000 nucleotides of the SSN6 gene. Proper
integration was confirmed by PCR. The glutathione S-transferase (GST)-Ssn61
includes the entire Ssn6 coding sequence fused with the GST coding sequence in pRS316-GAL1-GST.2 Ssn6HIS
function was checked by introducing the construct into a and
strains bearing the mfa2::lacZ reporter.
Repression was measured by 5-bromo-4-chloro-3-indolyl
-D-galactopyranoside filter
-galactosidase assay
(25). Standard mating assays were also performed to assay
complementation of the ssn6
9
-mating defect (26).
Gal1-GST-Ssn6 function was checked by introducing the plasmid into
ssn6
9 cells and assaying mating in media containing 2% galactose.
The protease-deficient
strains BJ5459, MATa ura3-52 trp1 lys2-801 leu2-1
his3-
200 pep4::HIS3 prb1-
1.6R can1 (27), and FM135, MATa leu2-3, 112 ura3-52 prb1-112 pep4-3 reg1-501
gal1 (provided by R. Deshaies, Cal-Tech), were used for the
purification of Ssn6HIS and GST-Ssn6 proteins, respectively. FM135
cells harboring the GST-SSN6 plasmid were grown in 3 liters of SD minus
uracil, minus leucine, plus 2% galactose to an
A600 of 0.5. The reg1-501 and
gal 1 mutations allow growth and induction in glucose and galactose (28). This culture was then used to inoculate 60 liters of
YEPD plus 2% galactose in a 60-liter fermentor. Cells were grown until
they reached an A600 of 2.4 and then harvested
by filtration. Cells containing the Ssn6HIS expression vector were grown in 40 liters of YEPD in the fermentor until they reached an
A600 of 2.
Yeast strains SM1196 and SM1179 containing
mfa2::lacZ were used to monitor the
function of the Ssn6HIS construct and have been described (29). Strains
EG123 MATa trp1 leu2 ura3 gal2 and 246-1-1
MAT trp1 leu2 ura3 gal2 transformed with the Ssn6HIS
construct were used for mating assays. The strain yCK12 MAT
ssn6
9 trp1 leu2 ura3 gal2 containing the GST-SSN6 plasmid was
used for mating assays (15).
Ssn6 and Tup1 antibodies were made against GST fusion proteins. The GST-Ssn6 fusion contains most of the tetratricopeptide repeat (TPR) coding region of SSN6 ligated into the pGEX1 vector (Pharmacia Biotech Inc.). The GST-CTERMTup1 fusion protein has been described previously (30). Purified fusion proteins were sent to Berkeley Antibody Company. Crude rabbit antibodies were then affinity purified against maltose binding protein fused to either Tup1 or Ssn6 (31). Ssn6 and Tup1 maltose binding fusion proteins contain the tetratricopeptide coding portion of SSN6, and the WD repeat coding sequence of TUP1 into pMAL2 (New England Biolabs Inc.).
Phosphatase AssaysApproximately 100 ng of the
GST-Ssn6-Tup1 preparation and about 10 ng of the Ssn6HIS-Tup1 were
added to a reaction mixture with the addition of 1 µg/ml of
leupeptin, pepstatin, and bestatin. The inhibitor sodium vanadate was
added to 4 mM. 200 units of phosphatase was added per
reaction (New England Biolabs Inc.). Reaction mixtures were incubated
at 30 °C for 30 min. The reactions were stopped by addition of
Laemmli sample buffer and heated to 65 °C for 10 min. A sample of
each reaction was then subjected to SDS-PAGE followed by Western
immunoblotting.
A frozen 150-g pellet of cells expressing the Ssn6HIS fusion was lysed with glass beads (Biospec Products Inc.) in an equal volume of 2 × lysis buffer (1 M NaCl, 100 mM HEPES, pH7.9, 20% glycerol, 2% Triton X-100, plus the protease inhibitors 10 mM benzamidine, 2 mM phenylmethylsulfonyl fluoride, and 2 µg/ml each of bestatin, pepstatin, and leupeptin). Lysed cells were then centrifuged at 33,000 rpm in a type 35 rotor for 1 h at 4 °C. The supernatant was collected and 20 ml of nickel-agarose (Pharmacia) was added. This mixture was rocked for 2.5 h at 4 °C, after which it was poured into a column. The column was sequentially washed with 60 ml of 1 × lysis buffer, 80 ml of 1 × lysis buffer containing 5 mM imidazole, 60 ml of 1 × lysis buffer plus 10 mM imidazole, and 40 ml of 20 mM imidazole plus 1 × buffer. Finally, the column was washed with 40 ml of low salt buffer (100 mM NaCl, 20 mM Tris, pH 8.0, 10% glycerol, 0.1% Tween 20) and eluted with the same buffer plus 150 mM imidazole. The Ssn6HIS and Tup1 elution profiles were followed by a dot blot antibody assay. The peak fractions were pooled and loaded over a 5-ml HiTrap-Q column (Pharmacia). Protein was eluted with a gradient of NaCl from 100 mM to 500 mM. The peak fractions were pooled, concentrated, and loaded over a Superose-6 column (Pharmacia) in 500 mM NaCl, 50 mM HEPES, pH 8.0, 10% glycerol, and 0.1% Tween 20. Fractions were collected, and samples from each were subjected to SDS-PAGE. The fractions bearing Ssn6HIS-Tup1 were identified by Western immunoblotting. The total yield was approximately 50 µg of Ssn6HIS-Tup1. The Stokes radius was determined by comparing the migration of Ssn6HIS-Tup1 through the Superose-6 column with that of molecular size standards (see below for the glycerol gradient) as in Siegal and Monty (32).
150 g of cells harboring the GST-Ssn6 and Tup1 expression vectors were lysed with glass beads following the addition of an equal volume of 2 × lysis buffer (1 M (NH4)2SO4, 100 mM HEPES, pH 7.9, 10 mM EDTA, 10 mM DTT, 20% glycerol, with protease inhibitors as above). The lysate was then spun at 7000 rpm in a Sorvall GSA rotor for 10 min to remove cellular debris. The supernatant was collected. (NH4)2SO4 was then added to 70%. The mixture was stirred on ice for 30 min. Protein was then pelleted by centrifugation in a SS34 rotor at 15,000 rpm for 20 min. The protein pellet was then resuspended in an equal volume of 50 mM HEPES, 5 mM DTT, 5 mM EDTA, 10% glycerol, plus protease inhibitors. The resuspension was then dialyzed against the same buffer for 2 h at 4 °C (14,000 molecular weight cutoff). The lysate was spun at 30,000 rpm in a type 35 rotor for 45 min. The supernatant was loaded over a 5-ml glutathione-agarose (Sigma) column. The column was washed with 100 ml of 1 × lysis buffer plus 0.5% Triton X-100, followed by a wash with 15 ml of 200 mM KOAc, 50 mM K-HEPES, pH 7.6, 1 mM DTT, 10% glycerol. The column was eluted in the same plus 10 mM glutathione. The proteins were concentrated approximately 10-fold by Centricon (Amicon). The total yield of GST-Ssn6-Tup1 was approximately 200 µg.
Glycerol Gradient SedimentationA 5-ml gradient was made by stepwise addition of 1 ml of 35, 30, 25, 20, and 15% glycerol plus 20 mM HEPES, pH 7.6, 10 mM MgOAc, 1 mM EDTA, and 1 mM DTT. The gradient was allowed to diffuse for 3 h at 4 °C. Protein samples in the same buffer, with 10% glycerol, were then layered on the top of the gradient along with protein size standards thyroglobulin, ferritin, catalase, lactate dehydrogenase, and bovine serum albumin (Pharmacia). The gradient was then spun at 45,000 rpm in a SW.1 rotor for 12 h at 4 °C. 250-µl fractions were taken from the top of the gradient. Samples of each fraction were subjected to SDS-PAGE and visualized by silver staining. The S value of the protein complexes was determined by comparison of the position in the gradient with that of the size standards of known S value.
StoichiometryPurified Ssn6HIS-Tup1 was separated by SDS-PAGE and stained with 0.25% Coomassie Brilliant Blue R-250 in 45% methanol, 10% acetic acid. The gel was destained in 25% methanol, 7% acetic acid followed by drying within cellophane membrane. The dry gel was scanned with a La Cie Silver Scan III Scanner and Adobe Photoshop (Adobe Systems Inc., Mountain View, CA). The amount of Ssn6 relative to Tup1 was determined by densitometry of the stained bands. Since dye binding per microgram of protein varies with each protein, the accuracy of this method is ± 30%.
ImmunoblottingProtein samples were run on 8.5% SDS-polyacrylamide gels followed by electrotransfer to polyvinylidene difluoride membrane. The membrane was blocked in Tris-buffered saline plus 5% milk and 0.2% Tween (TBST) for 1 h, then incubated with Ssn6 or Tup1 antibodies at 1:1000 dilution for 1 h. Membranes were washed 3 × in TBST for 5 min. Anti-rabbit antibodies conjugated to horseradish peroxidase (Amersham Life Sciences, Inc.) were then incubated with the filters in TBST at a dilution of 1:10,000 for 1 h. Blots were washed 3 × in TBST for 10 min. The blots were developed with ECL development reagents (Amersham Corp.) and exposed to Kodak XAR film. Dot blot assays were performed by dotting 1 µl of a column fraction on nitrocellulose followed by the above immunoblotting protocol.
In Vitro Transcription In vitro transcription
experiments were conducted as in Herschbach et al. (33),
with some exceptions. The yeast strain from which the transcription
extracts were made does not overexpress Tup1 or Ssn6. The transcription
reaction contains 3.7 mM EGTA, 180 mM potassium
glutamate, 27 mM potassium acetate, and 6.7 µg/ml acetylated bovine serum albumin. 86 nM 2 was added to
reactions where noted. The extent of repression is calculated as the
relative amount of 32P-labeled transcript from the reporter
in the absence and presence of the
2 protein, normalized to the
amount of transcript from the control reporter in the presence and
absence of
2. Band intensities were quantitated using a Molecular
Dynamics PhosphorImager.
The large size of the complex in which Ssn6 and Tup1 are found suggests that it has many subunits. To determine whether it contains components other than Ssn6 and Tup1, we purified the complex to near homogeneity. To facilitate purification, the SSN6 gene was affinity tagged at its C terminus with a nickel binding six histidine sequence. The resulting Ssn6HIS fusion gene was integrated at the SSN6 locus, under the control of its own promoter. A GST Ssn6 fusion was also constructed with the GST protein fused to the N terminus of Ssn6. The GST-SSN6 fusion gene was carried on a plasmid, and its transcription was under the control of the GAL 1 promoter. Both tagged versions of Ssn6 were expressed in yeast and complemented a deletion of the endogenous SSN6 gene (data not shown).
The Ssn6HIS fusion is expressed at approximately the same level as is
the endogenous Ssn6 protein and, therefore, should be present at normal
levels in the Ssn6-Tup1 complex. Cells containing Ssn6HIS as the only
source of Ssn6 were lysed and fractionated over a nickel-agarose
column, and peak fractions were assayed by Western immunoblotting with
antibodies prepared separately against Ssn6 and Tup1. Ssn6HIS and Tup1
co-fractionated, as expected for proteins that are tightly associated.
The peak fractions were pooled and loaded over a HiTrap-Q anion
exchange column and eluted with a salt gradient (100-500
mM NaCl). Ssn6HIS and Tup1 bound to the resin and co-eluted
at approximately 170 mM NaCl. The peak fractions were
pooled and further fractionated by gel filtration. As determined by
Western immunoblotting, Ssn6HIS and Tup1 were among the first proteins
to flow through the filtration column, consistent with the results of
Williams et al. (18) that these proteins are present
together in a large complex (Fig. 1A,
fraction 9 and 10). The protein elution profile
was visualized by silver staining an SDS-PAGE gel containing samples of
the column fractions. Purified Ssn6HIS and Tup1 migrated as doublets on
polyacrylamide gels as was previously noted for Ssn6 and Tup1 in crude
yeast extracts (18) (Fig. 1A, lanes 9 and
10). No other protein fractionated stoichiometrically with
Ssn6HIS and Tup1 in this or in any other preparation, suggesting that
this large complex is primarily if not exclusively composed of Ssn6 and
Tup1. We estimate that the Ssn6HIS-Tup1 preparation is purified
approximately 1800-fold and that approximately 6% of the Ssn6HIS was
recovered from the original lysate. The total yield of the Ssn6HIS-Tup1
complex was approximately 50 µg from 150 g of cells.
Migration through gel filtration is a function the Stokes radius of a protein complex. To determine the Stokes radius of the Ssn6HIS-Tup1 complex, size standards of known Stokes radii were also fractionated over the same gel filtration column. Using the methods of Siegal and Monty (32), the Stokes radius of the Ssn6HIS-Tup1 complex was determined to be approximately 14.7 nm.
To obtain a greater yield of the Ssn6-Tup1 complex, the GST-Ssn6 fusion protein was purified from a strain that overexpressed both GST-Ssn6 and Tup1. Purification of the overexpressed complex was carried out in a single step using a glutathione-agarose column. Again, Tup1 co-purified with GST-Ssn6. Fig. 1C shows the purified proteins on a silver-stained SDS-polyacrylamide gel. The higher mobility doublet at approximately 75 kDa associates with GST alone (data not shown). The overall yield of the GST-Ssn6-Tup1 complex was approximately 200 µg from 150 g of yeast. Only a small percentage (approximately 1%) of the GST-Ssn6 within the extract bound to the glutathione-agarose column.
Determination of the Size of the Ssn6-Tup1 ComplexIt has been suggested that the previous estimate of the molecular mass of the Ssn6-Tup1 complex of 1.2 MDa may be an overestimate if the complex is elongated or extended (18). Glycerol gradient sedimentation in conjunction with gel filtration can be used to estimate the molecular mass of a molecule with greater accuracy than can either method alone (32). To this end, the purified Ssn6HIS-Tup1 complex was subjected to glycerol gradient sedimentation in the presence of molecular standards of known S value (Fig. 1B). The peak of the Ssn6HIS-Tup1 complex (fraction 7) was in close proximity to that of the lactate dehydrogenase standard and corresponded to an S value of 7.3 (Fig. 1B, fraction 7). Taking into account both the Stokes radius and the S value, the molecular mass of the Ssn6-Tup1 complex was estimated at 440,000 Da. The behavior of Ssn6HIS-Tup1 on gel filtration and gradient sedimentation suggests that this complex is indeed asymmetrically shaped. Since the molecular mass of Ssn6 is approximately 107,000 Da and Tup1 is 78,000 Da, the complex must be composed of multiple Ssn6 and Tup1 molecules.
Densitometry of a Coomassie Blue-stained gel can be used to estimate stoichiometry of subunits in a complex. Coomassie Blue binding is approximately proportional to the number of positively charged groups in a protein (34). Since the Ssn6HIS and Tup1 proteins contain similar densities (9.2% and 10.6%, respectively) of arginine, lysine, and histidine, densitometry of a Coomassie-stained SDS gel was performed to obtain a crude estimate of the stoichiometry of these protein subunits in the complex. This analysis yielded a stoichiometry of one Ssn6 to three Tup1 molecules.
Tup1 Is a PhosphoproteinWhile Ssn6 is a known phosphoprotein
(35), it has not been established whether Tup1 is also modified in this
way. The appearance of both Ssn6 and Tup1 as multiple bands after
SDS-PAGE (see above) is consistent with both proteins being
phosphorylated. If phosphorylation is responsible for the observed
multiple-banding pattern, then removal of the phosphates should result
in each protein migrating as a single band on an SDS-polyacrylamide
gel. This is indeed the case as is shown in Fig. 2.
Purified GST-Ssn6-Tup1 complex was subjected to phosphatase
treatment followed by SDS-PAGE and Western blotting with antibodies
against both Tup1 and Ssn6. As seen in Fig. 2, phosphatase treatment of
GST-Ssn6-Tup1 results in the loss of the lower mobility forms of Tup1.
Since Ssn6 is known to be phosphorylated, the
phosphatase-dependent disappearance of the lower mobility Ssn6
species can be viewed as a control for
phosphatase activity.
Purified GST-Ssn6-Tup1 Complex Has Repression Activity in Vitro
As discussed in the Introduction, the DNA binding protein
2 recruits Tup1 and Ssn6 to DNA and thereby directs repression of
many target genes. Transcriptional repression directed by the
2
protein in vivo is thus completely dependent on both Ssn6
and Tup1.
2-directed repression has also been observed in an
in vitro transcription system utilizing whole cell yeast
extracts (33). In vitro,
2 repression is dependent on the
overexpression of Ssn6 and Tup1 in the yeast from which the
transcription extracts are prepared, suggesting that the amount of Ssn6
and Tup1 is a limiting factor for repression in this in
vitro system. To test this idea and to determine whether the
purified Ssn6-Tup1 complex analyzed above can supply repressor
activity, the following experiments were carried out. Transcription
from a reporter containing two a-specific gene operators
(
2/Mcm1 sites) upstream of a UAS-less CYC1 promoter is
measured in parallel reactions, one lacking
2 and one containing 86 nM
2. Mcm1, which binds cooperatively with
2, is
present in the yeast extract. Each reaction also contains a control
reporter that lacks a-specific gene operators. Transcription
extracts were prepared from yeast that do not overexpress Ssn6 and Tup1
and thus show no significant repression upon addition of purified
2
(Fig. 3, lanes 1 and 2). The
addition of purified GST-Ssn6-Tup1 gives approximately 5-fold
repression, which is also dependent on added
2 (Fig. 3, lanes
3 and 4).
In this report, we describe the purification of the Ssn6-Tup1 complex from yeast. We determined that the complex contains only Ssn6 and Tup1 proteins in stoichiometric quantities, and its size (approximately 440,000 Da) is smaller than the original estimate by Willams et al. (18), probably due to the asymmetric shape of the complex. The molecular mass estimate of 440 kDa is consistent with the complex being composed of multiple Ssn6 (107 kDa) and Tup1 (78 kDa) proteins, estimated at one Ssn6HIS to three Tup1 molecules. The purified Ssn6-Tup1 complex is active in an in vitro repression assay. Finally, we show that, like Ssn6, Tup1 is a phosphoprotein.
Ssn6 contains a repeated motif termed the tetratricopeptide repeats,
TPRs (35). This 34 amino acid repeat is found in proteins involved in a
variety of cellular functions from cell cycle progression to
mitochondrial protein import (for review, see Ref. 36). The only known
function of TPRs is to mediate protein-protein interactions. The TPRs
of Ssn6 are essential for repression in vivo and mediate in vitro binding to both Tup1 and 2 (35, 37, 38). A
complex composed of several Tup1 proteins and Ssn6 would, therefore,
contain numerous protein-protein interaction domains. There are a
number of proteins that have been predicted to interact with the
Ssn6-Tup1 complex, i.e. Mig1 and Rox1, the DNA binding proteins
required for glucose repression and hypoxic gene regulation (15). After recruitment to a particular gene set by interaction with a DNA binding
protein, the Ssn6-Tup1 repression complex may interact with downstream
elements, possibly Rox3, histones, Sin4, or Srb8, Srb9, Srb10, and
Srb11 (19-23, 39).
The phosphorylation of Tup1 may have a regulatory significance.
Groucho, another member of the WD repeat repressor proteins, is also
phosphorylated, and phosphorylation has been implicated in increasing
the affinity of groucho for the nucleus (40). Ste4, a WD repeat protein
involved in signal transduction in yeast, is also known to be
phosphorylated. Ste4 is the -subunit of a heterotrimeric G protein
complex and is multiply phosphorylated in response to mating
pheromones. This phosphorylation is required for the adaptation or
down-regulation of Ste4 activity in the continued presence of mating
factors (41). Phosphorylation of WD proteins may be a general way of
regulating protein-protein interactions. In the case of Tup1,
phosphorylation could regulate interaction with one or more of the DNA
binding proteins with which it interacts, Ssn6, Tup1 itself, or with
its downstream targets.
We are especially grateful to Danesh Moazed for technical advice and assistance as well as for reading of this manuscript. We thank the members of the Johnson lab for valuable discussions and advice.
After the submission of this manuscript, Varnassi et al. (1996) reported that the Ssn6-Tup1 complex is composed of one Ssn6 to four Tup1 subunits (42).