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Journal of Bacteriology, May 1999, p. 3136-3143, Vol. 181, No. 10
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
SSB, Encoding a Ribosome-Associated Chaperone, Is
Coordinately Regulated with Ribosomal Protein Genes
Nelson
Lopez,1
John
Halladay,2
William
Walter,2 and
Elizabeth
A.
Craig2,*
Department of Biomolecular
Chemistry2 and Department of
Bacteriology,1 University of Wisconsin, Madison,
Wisconsin 53706
Received 4 February 1999/Accepted 16 March 1999
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ABSTRACT |
Genes encoding ribosomal proteins and other components of the
translational apparatus are coregulated to efficiently adjust the
protein synthetic capacity of the cell. Ssb, a Saccharomyces cerevisiae Hsp70 cytosolic molecular chaperone, is associated with the ribosome-nascent chain complex. To determine whether this
chaperone is coregulated with ribosomal proteins, we studied the mRNA
regulation of SSB under several environmental conditions. Ssb and the ribosomal protein rpL5 mRNAs were up-regulated upon carbon
upshift and down-regulated upon amino acid limitation, unlike the mRNA
of another cytosolic Hsp70, Ssa. Ribosomal protein and Ssb mRNAs, like
many mRNAs, are down-regulated upon a rapid temperature upshift. The
mRNA reduction of several ribosomal protein genes and Ssb was delayed
by the presence of an allele, EXA3-1, of the gene encoding
the heat shock factor (HSF). However, upon a heat shock the
EXA3-1 mutation did not significantly alter the reduction
in the mRNA levels of two genes encoding proteins unrelated to the
translational apparatus. Analysis of gene fusions indicated that the
transcribed region, but not the promoter of SSB, is
sufficient for this HSF-dependent regulation. Our studies suggest that
Ssb is regulated like a core component of the ribosome and that HSF is
required for proper regulation of SSB and ribosomal mRNA
after a temperature upshift.
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INTRODUCTION |
Molecular chaperones of the heat
shock protein 70-kDa (Hsp70) class are highly conserved proteins that
bind unfolded polypeptides, preventing nonproductive interactions that
can lead to misfolding or protein aggregation. Hsp70s are composed of
three domains: a conserved 44-kDa ATPase segment, an 18-kDa domain
which is the binding site for unfolded polypeptides, and a 10-kDa
variable region at the C terminus. A variety of cellular processes such as protein synthesis, protein folding, and polypeptide translocation across organellar membranes are assisted by these molecular chaperones (5).
The budding yeast Saccharomyces cerevisiae contains two
major classes of cytosolic Hsp70 chaperones, Ssa and Ssb
(3). This report focuses on the ribosome-associated
chaperone, Ssb. The SSB Hsp70 family is composed of two
genes, SSB1 and SSB2. In contrast to
SSA genes, SSB genes are not heat inducible; in
fact, their expression is reduced after a heat shock. The
SSB-encoded proteins have greater than 99% identity. In
this paper, both SSB genes will be collectively referred to
as SSB unless specified otherwise. Strains containing gene
disruptions for both SSB genes are hypersensitive to certain
translation inhibitors and are cold sensitive (24). These
two phenotypes are completely suppressed by one copy of either of the
SSB genes but not by a constitutive overexpression of the
heat-inducible SSA genes (4). Ssb associates with
translating ribosomes and can be cross-linked to the nascent
polypeptide chain (24, 28). Its association with translating
ribosomes is resistant to treatment with high concentrations of salt,
implying that Ssb associates with the ribosome like a core component of
this apparatus.
Genes encoding many components of the translational machinery have a
coordinated regulation in response to environmental changes even though
they are dispersed throughout the genome (9). Cells increase
or decrease their ribosomal protein (RP) mRNA pools based on growth
conditions to accommodate their needs for protein synthetic capacity.
For example, upon a carbon upshift (i.e., when glucose is added to a
culture growing on a poor carbon source such as ethanol or glycerol)
the mRNA levels for RP genes increase. Upon amino acid limitation,
cells elicit a response known as stringent control which induces
transcription of amino acid biosynthetic genes and reduces the mRNA
levels of RP genes (37). A promoter sequence found in some
RP genes, known as the RPG box, is required to regulate transcription
of RP genes upon a carbon upshift and amino acid limitation. This
promoter sequence is the binding site for the transcriptional regulator
Rap1 (6, 13, 22, 25).
While expression of RP genes, SSB, and many other genes is
decreased, a set of genes called heat shock genes is induced upon temperature upshift (21). It has been reported that both
transcription and mRNA stability of RP genes are reduced after a heat
shock (12, 16), but sequences required for this regulation
have not been identified. In contrast, the induction of heat shock genes has been well characterized. The transcriptional activator of
many heat-inducible genes, the heat shock factor (HSF), is a homotrimer
that binds sequences known as heat shock elements (HSEs) in the
promoters of heat-inducible genes (23). Upon an increase in
temperature, HSF is activated, resulting in augmentation of
transcription from HSE-containing promoters. The yeast HSF monomer is
composed of four domains: an N-terminal activation domain, a DNA
binding domain, an oligomerization domain, and a C-terminal activation
domain. One HSF allele, EXA3-1, has a single base
substitution in the DNA binding domain that changes the proline at
position 214 to glutamine (10). This mutation reduces the ability of HSF to bind to the HSE, resulting in a delay in the induction of heat shock genes upon a temperature upshift.
Unlike heat-inducible proteins, RPs are coordinately expressed to allow
the cell to vary ribosome abundance depending on its needs for protein
synthesis. Ssb, while a member of a heat shock family of proteins, is a
component of translating ribosomes. To better understand Ssb's
regulation, we analyzed SSB mRNA levels under three
different growth conditions (carbon upshift, amino acid starvation, and
heat shock) known to affect RP gene expression. We report that
SSB and RP genes are regulated in a coordinated manner. In
addition, to elucidate components of the heat shock regulation of
SSB and RP mRNA, we analyzed mRNA levels in cells containing
a defective heat shock response due to the presence of the
EXA3-1 mutation. Our results indicate that the negative regulation of RP and SSB mRNAs after a heat shock is HSF dependent.
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MATERIALS AND METHODS |
S. cerevisiae strains.
With the exception of
F113 (21), yeast strains used in this study have the
following genotype: ura3-52 lys1 lys2 trp1-
1 his3-11,15
leu2-3,112. The F113 genotype is MATa can1
ino1-13 ura3-52 (22). The wild-type strains were DS10
(MATa) and JH27A (MAT
). The following
strains carry the additional alleles in parentheses: NL113
(ssb1:LEU2 and ssb2:HIS3), MH297
(EXA3-1) (10), and NL95 (ssb1:LEU2
ssb2:HIS3 EXA3-1 URA3). The EXA3-1 allele was
introduced into cells containing ssb1 ssb2 disrupted by
mating an ssb1:LEU2 ssb2:HIS3 strain (JN208) (24)
with an EXA3-1 strain (MH297) in which the EXA3-1
allele was genetically marked by the URA3 gene. The
resulting haploids (NL95 and NL113) were confirmed by marker
segregation and by using Northern blot analysis to measure the
transcript levels of an internal control RPL11 (previously
RPL16A) in a wild-type strain and the EXA3-1 strain after a heat shock.
Bacterial strains, transformations, plasmids, and gene fusion
constructions.
DH5 was the preferred Escherichia
coli strain for general cloning procedures [genotype:
80dlacZM15 endA1 recA1 hsdR17
(rK
mK+) supE44
thi-1 
gyrA relA1 F
lacZYA-argF]. E. coli cells were transformed
by CaCl2 procedures (20), and yeast strains were
transformed by the lithium acetate procedure described elsewhere
(8). Plasmids used in this study include pRS313-U2
(generously provided by Warren Heideman [27]), YEpCUP1-HSE-M-lacZ (a gift from Dennis Thiele [35]),
pSSB-URA3, pEC302, pJHSSB1P, and pCUP-SSB1. To construct pSSB-URA3, the
5' untranslated region and promoter of the SSB1 gene were
isolated from the plasmid pEC302 as a 617-bp
EcoRI-XbaI fragment. This fragment includes DNA
sequences from the polylinker which encode the restriction sites for
XbaI and SalI. The fragment was cloned directionally into pUC18 digested with EcoRI and
XbaI to create pJHSSB1P. The 962-bp
PstI-HindIII fragment from YEp24 containing the URA3 coding region and 19 nucleotides from the 5'-end
untranslated region was inserted into pJHSSB1P digested with
PstI and HindIII to create pJHSSB1P-URA3.
This construct contained the SSB1 promoter fused to the
coding region of the URA3 gene. The SSB-URA
fusion gene was cloned into the yeast centromeric pRS314 by removing the insert from pJHSSB1P-URA3 by HindIII and
EcoRI digestion. This fragment was inserted directionally
into pRS314 digested with EcoRI and BamHI (filled
in) to create pSSB-URA3.
To construct pCUP1-SSB, a modified version of the CUP1
promoter designated CUP1 hse-m and the first half of the
SSB1 gene were amplified by two separate PCRs. The
CUP1 hse-m promoter was amplified from plasmid
YEpCUP1-HSE-M-lacZ with two oligonucleotides: CupSSBa (TTT TCT CGA GCG
AGA TGA AAT GAA TAG C) and CupSSBb (CTG TAA TGA TCC TAT ATG ATA TTG CAC
TAA C). The amplified first half of the SSB1 gene started
from the first guanine nucleotide in the transcript and ended at the
BglII site in the middle of the gene. This SSB1
fragment was amplified with the following oligonucleotides: CupSSBc
(GCA ATA TCA TAT AGG ATC ATT ACA GTA TTT TAA TTG) and CupSSBd (CTT CGT
CGA TTT GAG AC). The two PCR products were fused to each other by
PCR-mediated overlapping extension (14), and the resulting
2.6-kb PCR fragment placed the first guanine nucleotide of the
SSB1 transcript immediately after the first start of
transcription found in the CUP1 hse-m promoter. The 2.6-kb
PCR fragment has two restriction sites at the ends (XhoI and
BglII) that were used to digest and subclone it into a
6.5-kb XhoI-BglII-opened pRS314-SSB1 vector. This
6.5-kb XhoI-BglII pRS314-SSB1 fragment provided
the other half of the SSB1 gene to the Cup1-SSB1 fusion
after the BglII site. This plasmid was used to transform
NL113 (ssb1 ssb2) and NL95 (ssb1 ssb2 EXA3-1)
strains. This gene fusion was functional, as it completely suppressed
the ssb1 ssb2 mutant phenotypes of cold sensitivity and
hypersensitivity to translation inhibitors. In addition, transcript
levels from this gene fusion increased upon addition of copper (data
not shown). The analysis of this gene fusion did not require addition
of copper to the medium due to appropriate basal expression under our
growth conditions.
Chemicals.
Yeast extract, peptone, and yeast nitrogen base
without amino acids were from Difco Laboratories (Detroit, Mich.);
dextrose and 3-amino-1,2,4-triazole (3AT) were from Sigma Chemical Co. (St. Louis, Mo.); SeaKem agarose was from FMC Corp. (Rockland, Maine).
Growth conditions.
The carbon upshift was performed by
growing cells in glycerol-based medium (YPG [1% yeast extract, 2%
peptone, 5% glycerol]) to exponential growth
(A600 between 0.4 and 0.8) and then adding glucose to the culture to a final concentration of 2%. For amino acid
starvation, 10 mM 3AT was added to exponentially growing cells cultured
in SD minimal medium (29). The heat shock response was
elicited by growing cells on YPD (1% yeast extract, 2% peptone, 2%
dextrose) rich medium at 23°C and then shifting the medium to 39°C.
The temperature upshift for stable messages (i.e., 50% reduction of
basal levels takes longer than 5 min) was done by moving a 25-ml
aliquot of the cell suspension to a 39°C prewarmed 250-ml flask. For
short-half-life mRNAs such as that for URA3, the temperature
upshift was done by mixing approximately 10 ml of prewarmed YPD medium
at 68°C into a 15-ml culture growing at 23°C and placing it in a
39°C water bath. In each condition, aliquots of the cell suspension
were taken at times indicated and total RNA was prepared from pelleted
cells by the heat-freeze method (31).
Northern (RNA) blot analysis and primer extension analysis.
Northern blot analysis was done by separating 4 to 10 µg of total RNA
in a 1% agarose-formaldehyde gel, transferring the gel to a nylon
membrane, and hybridizing it with radiolabeled probes (specific
activity 
107 cpm/µg) made by random priming
(2). Probes were generated with [-32P]dCTP
(3,000 Ci/mmol) (DuPont NEN). After stringent washes, filters were
exposed to a detection screen with a PhosphorImager, and the signal was
quantified with the ImageQuant software package (Molecular Dynamics).
Differences in RNA loading on Northern blots were normalized with
indicated loading controls on each experiment. rRNA was used to
normalize loaded amounts of RNA in heat shock experiments since even
the levels of relatively stable transcripts decrease significantly
during the time course of the experiment, making quantitative analysis
difficult. The validity of this method has been confirmed elsewhere
(10).
For primer extension analysis, a 20-mer oligonucleotide (5'-GAT AGC ACC
TTG GAA AAC AC-3') complementary to the 5' ends of
the
SSB1
and
SSB2 coding regions was used to prime cDNA synthesis.
To
normalize amounts of RNA used per reaction, a primer with sequence
complementary to the small nuclear RNA (snRNA) U4 (CGG ACG AAT
CCT CAC
TGA TAT GC) was included on each reaction. Gel-purified
oligonucleotides were radiolabeled at the 5' end with T4 polynucleotide
kinase and [
-
32P]ATP (3,000 Ci/mmol) (DuPont NEN)
(
2). Radiolabeled primers
were hybridized to 20 to 30 µg
of total RNA at 90°C for 3 min
and then quickly chilled on ice.
Annealed primers were extended
with avian myeloblastosis virus reverse
transcriptase (Promega,
Madison, Wis.), and primer extension products
were separated with
6% polyacrylamide gels. Signals were visualized
with a PhosphorImager
and quantified with the ImageQuant software
package.
RP nomenclature.
RPs of S. cerevisiae have been
named in this work according to the new nomenclature described in the
work of Mager et al. (18).
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RESULTS |
SSB mRNA levels increase upon a carbon upshift.
Most RP genes possess a transcriptional regulatory sequence designated
an RPG box (CCC ATA CAT CT) (39, 40) and a T-rich region
important for constitutive expression (30). Analysis of the
SSB promoter sequence indicates that both genes possess a
T-rich region; the SSB1 promoter also has a putative RPG box centered at 261 bases upstream of the adenine of the start codon with
the sequence CCC ATA CAC CG. These common structural features and the
fact that both are components of ribosomes suggested to us that
SSB and RP gene regulation may be coordinated.
It has been observed that mRNA levels of RPs rapidly increase by more
than twofold upon a carbon upshift (
13,
15). We
analyzed
SSB mRNA levels by Northern blot analysis after supplying
glucose to wild-type cells growing in glycerol-based medium. As
shown
in Fig.
1,
SSB mRNA levels
increased by more than twofold
within 30 min of carbon upshift, similar
to the mRNA increase
of the RP gene
RPL5 (previously called
L1a). In contrast, the
mRNA levels of genes encoding another cytosolic
chaperone, Ssa,
did not increase but rather transiently decreased upon
glucose
addition.
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FIG. 1.
mRNA levels of SSB genes upon a carbon
upshift. At time zero, glucose was added to wild-type cells growing in
glycerol-based medium. At left, signals from Northern blotting of
several transcripts upon a carbon upshift are shown. The graph at right
shows quantification of the signals after normalization to snRNA U2
levels.
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The
SSB chaperone family is composed of two genes,
SSB1 and
SSB2, which are more than 90%
identical. To determine whether
both
SSB transcripts
increase upon a carbon upshift, we analyzed
the mRNA levels of both
genes in wild-type cells. Primer extension
analysis was used to
distinguish between the two transcripts.
We designed an oligonucleotide
complementary to the 5' end of
the
SSB coding sequence. Due
to the complete sequence identity
of
SSB1 and
SSB2 in this region, both
SSB transcripts are
able
to efficiently serve as templates during a primer extension
reaction.
As shown in Fig.
2A, the
analysis of the
SSB mRNA species in a
wild-type strain
resulted in two predominant bands (lane 2) representing
products
extending 29 and 22 bases beyond the initiation codon
ATG. It seemed
likely that each band represented the transcript
from a single
SSB gene, but it was unclear which band was the
extension
product of which mRNA. We reasoned that increasing the
gene dosage of
either
SSB1 or
SSB2 would result in higher
amounts
of the respective mRNA than that expressed from a single
chromosomal
copy. Consequently, we overexpressed
SSB1 or
SSB2 by supplying
wild-type cells with a high-copy-number
plasmid containing either
SSB1 or
SSB2.
Overexpression of
SSB1 resulted in enhanced levels
of the
upper band, while overexpression of
SSB2 caused an increase
in the signal of the lower band (Fig.
2A, lanes 1 and 3, respectively).
Interestingly, overexpression of the
SSB1 gene appears to
decrease
SSB2 mRNA levels, although the reverse does not
appear to be true.
We conclude that the upper band is an extension of
the
SSB1 gene
and that the lower band is an extension of the
SSB2 gene. This
experiment localized the 5' end of the
SSB1 and
SSB2 genes to
29 and 22 nucleotides,
respectively, upstream from the A of the
initiating ATG codon (Fig.
2B).
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FIG. 2.
Localization of the 5' ends of the SSB1 and
SSB2 genes and analysis of their mRNA levels upon a carbon
upshift. (A) Primer extension reactions are shown in the center: lane
1, strain overexpressing the SSB1 gene; lane 2, wild-type
cells; lane 3, strain overexpressing the SSB2 gene.
Sequencing reactions are shown on the left for the SSB1 gene
and on the right for the SSB2 gene. (B) Sequences from the
SSB1 and SSB2 genes showing the start site of
transcription relative to the initiation ATG codon. Sequences
complementary to the primer are located above the arrow labeled as
primer. (C) mRNA levels of SSB1 and SSB2 genes
after a carbon upshift. Samples of the culture were collected at the
indicated times after glucose addition. At left is shown a sequencing
gel which separates the primer extension products. Lane G shows results
from cells grown on glucose-based medium. The graph shows the
quantification of the signal obtained after normalization to snRNA
U4.
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The individual increase in mRNA levels of
SSB1 and
SSB2 after a carbon upshift was studied by primer extension
analysis with
the same oligonucleotide that was used to localize the
start site
of transcription of these RNAs. We also included in the
reactions
a primer that complements sequences of the U4 snRNA to
normalize
amounts of RNA used in reactions. Both
SSB1 and
SSB2 mRNA species
increased upon a carbon upshift, although
SSB1 mRNA increased
to a greater extent than did
SSB2 mRNA (Fig.
2C).
The stringent control response results in a coordinated reduction
in the mRNA levels of SSB and RP genes.
Amino acid
starvation elicits a cellular response known as stringent control
resulting in the transcriptional activation of amino acid biosynthetic
genes and reduction in the expression of RP genes (37). We
hypothesized that if Ssb is a component of the ribosome it would have a
pattern of regulation similar to that of RP genes not only under carbon
upshift but under other nutritional conditions as well. We expanded the
analysis of SSB mRNA regulation by studying its mRNA levels
after amino acid starvation. The stringent response was induced by
adding 3AT, a competitive inhibitor of an enzyme required for histidine
biosynthesis (22), to cells growing in minimal medium. Total
RNA was prepared from aliquots of the culture taken at various times
after 3AT addition. Northern blot analysis was used to quantify mRNA
levels of SSB and the RP gene RPL5. As negative
controls, we analyzed mRNAs of two genes whose products do not function
in translation: SSA, which encodes another cytosolic Hsp70
chaperone, and HHO1, the histone H1 gene. RPL5
and SSB mRNA levels gradually decreased, dropping below 50%
of the control levels by 90 min after addition of 3AT. We observed a
rapid and transient decrease of SSA and histone H1 mRNAs 30 min after 3AT addition with a return to basal levels by 90 min (Fig.
3). To examine the effectiveness of the 3AT treatment, we measured the mRNA levels of HIS3, a
histidine biosynthetic gene. As we expected, after amino acid
limitation the mRNA levels of HIS3 increased up to fourfold.
Thus, we conclude that SSB is regulated in coordination with
RP genes during amino acid starvation, while the gene encoding the
other cytosolic Hsp70, Ssa, is not.
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FIG. 3.
mRNA levels of various transcripts after amino acid
limitation. 3AT was added to cells (strain F113) growing in SD minimal
medium at time zero. RNA samples were analyzed by Northern blotting.
(A) (Left) Control from cells that had no 3AT ( 3AT) treatment.
(Right) Signals obtained from cells treated with 3AT. Genes analyzed
were SSB, RPL5 (RP), SSA (a yeast
cytosolic Hsp70), and HHO1 (histone H1). HIS3 was
used as a control to detect the efficiency of the treatment. (B and C)
Quantification of the mRNA levels in the presence of 3AT (+3AT) and of
HIS3 mRNA with (+3AT) and without (3AT) 3AT, as shown in
panel A, after normalization to actin transcript levels.
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EXA3-1, an allele of HSF1 which encodes the yeast HSF,
causes a delay in mRNA reduction of SSB and RP genes upon a
heat shock.
As shown previously, the mRNA levels of RP genes and
SSB decrease drastically upon a heat shock in a wild-type
strain (16, 38). However, the cause of the negative
regulation is not known. Since induction of many heat shock genes is
dependent on the transcriptional activator HSF, we asked whether HSF
activity has an effect on the negative regulation of SSB and
RP genes. Therefore, we analyzed the heat shock regulation of several
mRNAs in a mutant strain (MH297) containing the EXA3-1 HSF
allele. Cells were grown in rich medium to mid-log phase at 23°C and
then shifted to 39°C. Aliquots of the culture were taken at the
indicated times, and mRNA levels were quantified by Northern blot
analysis. The SSB mRNA reduction was much less rapid in
MH297 than in a wild-type strain (Fig.
4). For example, after 20 min of a heat
shock the SSB mRNA levels in wild type were reduced by
greater than 75% while the levels in the MH297 strain were reduced by
less than 20%. A similar delay in the reduction of mRNA levels was
seen for the RP mRNAs of RPL5, RPL11,
RPS14 (previously known as CRY1 and
CRY2), and RPS17 (formerly known as
RP51) (Fig. 4 and data not shown).
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FIG. 4.
mRNA levels of ribosomal components upon a heat shock in
the wild-type (WT) strain and in cells containing the EXA3-1
mutation. JH27A (wild-type) and MH297 (EXA3-1) cells growing
in YPD medium at 23°C were rapidly shifted to 39°C. Aliquots of the
culture were collected at the times indicated after the temperature
upshift, and extracted RNA was subjected to Northern blot analysis.
(Top) Northern blot images. (Bottom) Quantification after normalization
to rRNA (see Materials and Methods).
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It is known that most mRNA species are reduced in abundance upon a heat
shock. To determine whether
EXA3-1 has a global effect
on
the negative regulation of genes after a heat shock, we tested
the
effect of the mutation on the mRNA levels of two genes whose
products
are unrelated to the protein synthesis process.
URA3 encodes
a biosynthetic enzyme required for uracil synthesis;
MAT encodes the mating pheromone
-factor. Little or no difference
was
observed in the rate of decrease of either of these two mRNAs
upon a
heat shock (Fig.
5), indicating that
EXA3-1 does not have
a global effect on the regulation of
all mRNAs upon temperature
upshift.
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FIG. 5.
Levels of MAT1/2 and URA3
transcripts upon a heat shock in the wild-type (WT) (JH27A) strain and
in cells containing the EXA3-1 mutation (MH297). Experiments
were performed as described for Fig. 4. In the case of the
short-half-life message URA3, samples were taken at 0 to 18 min after a temperature upshift (see Materials and Methods). (Top)
Northern blot images. (bottom) Graphs showing the quantification of
signal after normalization to rRNA.
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The SSB promoter is not sufficient to decrease its mRNA
levels in an HSF-dependent manner.
To aid in understanding the
regulation of mRNA levels by HSF, we wanted to determine the sequences
in the SSB gene essential for this regulation. To test the
sufficiency of the SSB1 promoter, we utilized an
SSB1:URA3 engineered fusion to analyze the SSB1 promoter contribution to the URA3 mRNA regulation in the
wild type and the MH297 mutant strain. This gene fusion expressed a functional protein that allowed growth of cells lacking a functional genomic URA3 gene in medium lacking uracil (data not shown).
Since the ura3-52 genomic allele in this strain background
does not encode detectable transcript (data not shown), we were assured that URA3 mRNA detected in our experiments was expressed
from the SSB1 promoter. URA3 was appropriate for
this analysis because the decrease of its mRNA after heat shock is
unaffected by EXA3-1 mutation (Fig. 5B).
Wild-type and MH297 strains were transformed with pSSB-URA. As shown in
Fig.
6, the
EXA3-1 mutation in
MH297 did not have
an obvious effect on the reduction of
URA3 mRNA produced from
the
SSB1:URA3 gene fusion
after a temperature upshift. In contrast,
the internal control of the
RP transcript encoded by the chromosomal
copy of
RPL11
showed a significant delay in its rapid reduction
in the MH297 strain.
These results indicate that the
SSB promoter
is not
sufficient to regulate its mRNA after heat shock in an
HSF-dependent
manner.
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FIG. 6.
mRNA levels of an SSB1:URA3 fusion
in wild-type (WT) and mutant MH297 cells after a heat shock. The
experiment was performed as described for URA3 in Materials
and Methods. Northern blot images of each transcript are shown at left.
(A) SSB1:URA3 fusion; (B) RPL11.
Quantification of the signals detected in panels A and B is shown on
the right. Signals were normalized to rRNA levels.
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Sequences within the transcribed region of SSB are
sufficient to regulate SSB transcript levels after a heat
shock in an HSF-dependent manner.
Since the promoter of
SSB1 was not sufficient for the HSF-dependent SSB
mRNA regulation upon a heat shock, we tested whether the transcribed
region of the SSB1 gene possesses sequences sufficient for
such regulation. We designed a gene fusion that contained the entire
SSB1 transcribed region downstream of the CUP1
promoter (Fig. 7). Since the native
CUP1 promoter is induced by a heat shock through the action
of HSF, we used a CUP1 hse-m promoter which has no
functional interaction with HSF (Cup1 hse-m)
(35). Therefore, transcription from this promoter is not
heat induced (data not shown). The fusion was created in such a way
that the start of transcription of CUP1 hse-m is the first
nucleotide in the SSB1 transcript. This CUP1:SSB1
fusion suppressed both phenotypes (cold sensitivity and
hypersensitivity to translation inhibitors) of a mutant strain
containing deletions of both SSB genes. In addition, primer
extension analysis showed that the 5' end of the CUP1:SSB1
transcript is similar in size to that of the native SSB1
transcript (data not shown).
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FIG. 7.
Influence of the EXA3-1 mutation on the
transcript levels of a CUP1:SSB1 fusion. The
experiment was done as described in the legend to Fig. 5. At left,
Northern blot images for CUP1:SSB1 fusion (A) and
RPL11 (B) are shown. At right is shown quantification of the
signals after a heat shock with rRNA as a loading control.
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This
CUP1:SSB1 fusion was used to transform two strains that
have the following genotypes:
ssb1 ssb2 EXA3-1 (NL95) and
ssb1 ssb2 (NL113). Analysis of the
CUP1:SSB1
fusion showed rapid reduction
of its mRNA levels in NL113. This
reduction was retarded in the
presence of the
EXA3-1 allele.
The delay in the heat shock regulation
of the
CUP1:SSB1
transcript in NL95 is comparable to what was
observed for the internal
control, the genomic RP gene
RPL11.
After 20 min of the
temperature upshift, the mRNA levels of both
RPL11 and
CUP1:SSB1 were about threefold higher in NL95 than in
NL113.
Therefore, the sequences included in the
SSB1 transcribed
region are sufficient to provide a heat shock mRNA regulation
dependent
on
HSF.
| |
DISCUSSION |
It has been established that cells regulate components of the
ribosome according to their growth rates and stress conditions that
compromise protein synthesis (19, 39). Here we have
demonstrated that mRNA levels of the Hsp70 molecular chaperone Ssb are
coregulated with RP mRNA levels under three different growth
conditions: carbon upshift, amino acid starvation, and heat shock.
Other data indicate a relationship of Ssb with ribosomes. Ssb, which is
present within the cell in a two- to three-times molar excess over
ribosomes (28), is associated with the ribosome-nascent
chain complex in a salt-resistant manner (28). In addition,
strains lacking Ssb are more sensitive to certain translation
inhibitors (24). Hence, the regulation reported here coupled
with previous results supports the hypothesis that Ssb should be
considered an important component of the translational apparatus.
The regulation of SSB and SSA, which encode two
major classes of cytosolic Hsp70s, is strikingly different. These two
Hsp70s have evolved with similar protein structures as evidenced by the fact that they are more than 60% identical in sequence, but their regulation is different, presumably because of their different functional niches within the cell. Ssa has been implicated in the
refolding of proteins partially denatured upon exposure to increased
temperatures and in regulation of the heat shock response. Therefore,
it is not surprising that SSA expression is induced by a
heat shock to cope with the protein damage generated at high temperatures. In contrast, expression of Ssb, as well as of RPs, is
repressed after a temperature upshift. Apparently, it is advantageous for cells not to expend energy in translation under conditions in which
proteins will be jeopardized by denaturation conditions and subjected
to aggregation. Also, both SSB and RP gene mRNA levels are
regulated according to the growth rates of the cell. For example, we
observed that mRNA levels of SSB and RP genes decline upon
starvation for amino acids when the level of protein synthesis is
dropping. Moreover, SSB mRNA levels increase rapidly upon
addition of a rich carbon source when the rates of protein synthesis in
a cell are rising. Therefore, the synthesis of Ssb and structural RPs
is carefully regulated by the cell, presumably to minimize the energy
used in forming the translational apparatus, which comprises about 16 to 18% of cellular protein.
The mechanism of down-regulation of RP mRNA levels upon a heat shock is
not well understood. Regulation at the level of transcription and mRNA
degradation have been suggested (12, 16). We found the
negative heat shock regulation of both SSB and four RP genes analyzed to be dependent on HSF. This conclusion is based on our observation that a strain containing the HSF allele EXA3-1
has a delay in the reduction of mRNA levels of SSB and RP
genes upon a heat shock. Moreover, the EXA3-1 mutation did
not affect the negative heat shock mRNA regulation of two proteins
whose function is not related to the translation machinery, the mating
-factor gene MAT1/2 and the URA3 gene
transcripts. The rate of reduction for these two mRNAs after a
temperature upshift was similar in wild type and in cells containing
the EXA3-1 mutation. These data suggest that two mechanisms
are responsible for reducing mRNA species upon a heat shock: a global
mechanism that is HSF independent and a specific mechanism for RP mRNAs
that requires HSF.
Considering the results reported here, it is somewhat surprising that
another HSF allele (hsf1-m3/mas3) was reported to have no
effect on the mRNA regulation of RP genes upon a heat shock (7). This HSF allele was thought to abolish its heat
activation, reducing drastically the induction of heat-inducible genes
(34). Recently, it was found that a mutant strain containing
the hsf1-m3 allele did not have an obvious decrease in the
induction of several heat shock proteins (17, 36), including
Hsp104. However, we have observed that the EXA3-1 mutation
appears to retard the heat induction of Hsp104 as well as that of other
Hsp proteins (10). Consistent with this result, the
EXA3-1 mutation also delays the reduction of SSB
and RP transcripts. It is possible that the hsf1-m3 mutation
does not significantly affect the activity important in the
up-regulation of Hsp104 as well as the down-regulation of genes
encoding ribosomal components.
We can envision two general ways in which HSF may be acting in the
regulation of SSB and RP genes: (i) HSF may act as a
transcriptional repressor of SSB and RP genes or (ii) HSF is
a transcriptional activator of a heat-inducible regulatory factor
needed for the down-regulation of RP and SSB genes. We favor
the second idea, that the EXA3-1 mutation causes a delay in
the expression of a heat-inducible factor, for several reasons. If HSF
is a repressor, it must be binding to cryptic sequences since neither
SSB gene contains a canonical HSE. There is a precedent for
the binding of a transcriptional activator or repressor to variant
sequences in different modes of regulation (32). However,
alignment of SSB and the RP genes studied here did not
reveal a conserved sequence present in these genes which might act as a
novel binding site for HSF acting as a repressor. In addition, our
results show that the transcribed region of SSB is
sufficient to regulate its mRNA levels after a heat shock in an
HSF-dependent manner, while the promoter is not. This result does not
preclude HSF acting directly as a repressor since binding of repressors
to the coding region has been found previously (11, 33).
However, such cases appear to be rare, particularly in yeast. Finally,
previous experiments suggest that a factor needs to be synthesized de
novo for the appropriate mRNA regulation of RP genes upon a heat shock
(12, 26). Together, these observations suggest that HSF acts
as a transcriptional activator of a heat-inducible factor, not as a transcriptional repressor of SSB and RP genes.
What might the function of such a heat-inducible factor be? Such a
factor could be or could activate a heat-inducible transcriptional repressor or an RNase activity specific for these genes or mRNAs. Unfortunately, it is very difficult to determine directly whether the
differences in SSB regulation in wild-type and HSF mutant cells are at the transcriptional or the posttranscriptional level due
to unique problems in studying RNA regulation during the heat shock
response. The methods currently available to measure RNA stability are
inadequate under these conditions. The addition of drugs such as
1,10-phenanthroline and thiolutin, which inhibit the vast majority of
mRNA synthesis, induces the synthesis of heat shock mRNAs
(1). The temperature-sensitive mutation in the RNA
polymerase subunit RPB1 commonly used (26)
requires a "heat shock" to inhibit RNA synthesis, but the
temperature inactivation of the RPB1 subunit is too slow to
eliminate induction of a heat-inducible factor (data not shown). In the
absence of additional experimental data, we favor the simplest idea,
that HSF is required for induction of an RNase or of a factor required
for activation of an RNase. This RNase or factor may recognize an RNA
secondary structure common to both SSB and RP mRNAs which is
not recognizable at the primary sequence level.
The experiments reported here emphasize an HSF-dependent mode of
regulation of mRNA levels upon a temperature upshift. This mode of
regulation does not affect all genes, as the rates of decrease of
MAT1/2 and URA3 mRNAs were not significantly
affected by the EXA3-1 mutation. There is certainly a second
mechanism of regulation, as both these mRNAs, as well as many others,
decrease in levels upon a heat shock. The regulatory mechanism
unaffected by the EXA3-1 mutation which controls the
expression of many genes, including SSB and RP genes, may be
a general cessation of transcription of non-heat-inducible genes, as
pulse-labeling experiments indicate that transcription of RP genes in
S. cerevisiae is reduced after a heat shock (16).
However, this regulatory pathway is overlaid by an HSF-dependent
mechanism that down-regulates SSB and RP mRNAs, perhaps by
hastening the degradation of existing mRNA molecules. This
HSF-dependent mechanism is an extremely efficient way for the cell to
couple the activation of heat-inducible genes with the negative
regulation of the translational apparatus, by linking both modes of
regulation to the same regulatory molecules. This coupling implies that
the down-regulation of the translational apparatus is an important
component of the regulatory pathways that the cell has evolved to
cope with environmental stress.
| |
ACKNOWLEDGMENTS |
We thank Warren Heideman, Alan Hinnebusch, Dennis Thiele, and
John Woolford for providing plasmids and strains and Bonnie K. Baxter,
Philip James, and Christine Pfund for thoughtful comments on the manuscript.
This work was supported by NIH grant 5RO1 GM31107 (E.A.C.) and NIH
Predoctoral Fellowship GM18507-02 (N.L.).
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Biomolecular Chemistry, 587 Medical Science Center, 1300 University
Ave., Madison, WI 53706. Phone: (608) 263-7105. Fax: (608) 262-5253. E-mail: ecraig{at}facstaff.wisc.edu.
| |
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Top
Abstract
Introduction
