From the Department of Biochemistry and Biophysics and the Center for Gene Research and Biotechnology, Oregon State University, Corvallis, Oregon 97331
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ABSTRACT |
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The prevalence of p53 gene mutations
in many human tumors implies that p53 protein plays an important role
in preventing cancers. Central among the activities ascribed to p53 is
its ability to stimulate transcription of other genes that inhibit
cells from entering S phase with damaged DNA. Human p53 can be studied
in yeast where genetic tools can be used to identify proteins that affect its ability to stimulate transcription. Although p53 strongly stimulated reporter gene expression in wild type yeast, it only weakly
stimulated reporter gene expression in trr1 yeast that lacked the gene encoding thioredoxin reductase. Furthermore, ectoptic expression of TRR1 in
trr1 yeast restored
p53-dependent reporter gene activity to high levels.
Immunoblot assays established that the
trr1 mutation
affected the activity and not the level of p53 protein. The results
suggest that p53 can form disulfides and that these disulfides must be
reduced in order for the protein to function as a transcription
factor.
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INTRODUCTION |
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Mutations in the p53 tumor suppressor gene have been found in more than half of human cancers. Of 5000 mutations documented, about 85% are missense mutations and greater than 95% are found in the DNA-binding core domain. Ectopic expression of wild type p53 in cells with p53 null mutations suppresses cell growth; expression of oncogenic forms does not (1). Moreover, oncogenic forms of p53 inhibit the ability of wild type p53 to stimulate reporter genes (2). Human tumors frequently express large amounts of p53 antigen. Mice homozygous for p53 null mutations develop normally but show a high tumor incidence (3). These and other results suggest that although p53 null mutations are oncogenic, oncogenicity is most frequently due to dominant negative mutations that result in production of a defective p53 that interferes with the function of wild type p53.
It is becoming increasingly clear that cancer results from defects in cell cycle control. Our understanding of cell cycle control derives largely from work first initiated in yeast. All eucaryotic cells have cyclins and cyclin-dependent protein kinases (CDKs)1 that initiate and orchestrate the transition from one cell cycle compartment to the next. In addition to CDKs, all cells have checkpoint systems that prevent CDKs from initiating the next cell cycle phase until critical processes in the current phase are complete (4). One major checkpoint mechanism is mediated by a set of proteins called cyclin-dependent kinase inhibitors, which bind and inactivate CDKs.
In both yeast and mammalian systems, initiation of S phase is delayed when G1 cells are UV-irradiated. In mammalian cells lacking p53 (or in cells with dominant negative p53), the delay in S phase does not occur, and cells enter S phase with damaged DNA. If wild type p53 is present, the cells enter S phase only when the damage is repaired, or, if the damage is too severe, the cells undergo apoptosis. The discovery that p53 stimulates transcription of the cyclin-dependent kinase inhibitor gene CIP1, which encodes a G1 cyclin/CDK inhibitor, in response to DNA damage provides a molecular understanding of the basis for S phase delay. The CIP1 upstream region contains a p53-binding site, and accumulation of Cip1 activity and cell cycle arrest in irradiated cells requires wild type p53 (5).
Although yeast does not contain a p53 gene, the similarity of cell cycle control mechanisms and transcriptional mechanisms in all eucaryotic organisms prompted investigators to ask whether human p53 was active in yeast. p53 binds the consensus RRRC(A/T)(T/A)GYYY (6). Reporter genes equipped with multiple copies of the consensus site are stimulated by ectopic expression of p53 not only in mammalian cells (2, 6) but in yeast (7, 8) as well. p53 activity is also affected by yeast mutations. Koerte et al. (9) screened for yeast mutations that created a requirement for human p53. They identified a gene, termed RFP1 (requires fifty-three protein), that results in cell cycle arrest at G2/M when inactivated. Thiagalingam et al. (8) screened for yeast mutations that prevented p53 transactivation of a p53-responsive LacZ reporter gene. Using one of the obtained mutants, they identified a high copy suppressor, termed PAK1 (p53 activating kinase), that encoded a protein with protein kinase motifs. They did not establish that Pak1 actually phosphorylated p53. Nigro et al. (10) investigated whether overexpression of p53 blocked cell cycle progression in Saccharomyces cerevisiae. Using a high copy plasmid and a galactose-inducible promoter they did not observe significant inhibition of growth by p53. However, by using a protease-deficient strain and by cotransforming with a plasmid encoding the human CDK p34cdc2, they showed that human p53 strongly inhibited yeast growth. Although human p34cdc2 was required to see strong growth inhibition by p53, it did not affect the phosphorylation state of p53 protein, suggesting that p34cdc2 acted indirectly, presumably by phosphorylating other yeast proteins.
The above studies were done with the budding yeast S. cerevisiae. A recent study, done with the fission yeast Schizosaccharomyces pombe, prompted our investigation of the involvement of thioredoxin reductase in p53 activity. Casso and Beach (11) found that high level expression of p53 in S. pombe arrested cell growth. A mutant circumventing growth arrest was identified, and the wild type gene, a homolog of thioredoxin reductase, was cloned by complementation. To determine whether the S. pombe results reflected a conserved mechanism whereby the ability of p53 to stimulate transcription requires thioredoxin reductase activity, the effect of deleting the thioredoxin reductase gene on p53-dependent reporter gene expression was investigated in the evolutionarily distant organism S. cerevisiae. The results showed that the transactivating activity of p53 in budding yeast also required thioredoxin reductase. The data suggest that p53 may be subject to redox regulation.
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EXPERIMENTAL PROCEDURES |
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Yeast Strains--
Yeast strain MY301 (mat-a ade2 ura3
leu2 trp1 his3 trr1:HIS3 bar1) was
derived by crossing MY199 (12) to W303-1 (13) and serially
backcrossing
trr1:HIS3 segregants to W303-1
or SY2626 (a bar1 derivative of W303-1). Inheritance of the
trr1:HIS3 allele was confirmed by Southern
blot analysis and hydrogen peroxide sensitivity. MY301 was
temperature-sensitive for growth and auxotrophic for methionine. Yeast
carrying effector and reporter plasmids were derived and grown at
25 °C in minimal medium consisting of yeast nitrogen broth, 2%
glucose, and required supplements.
Plasmids--
pRS314, pRS315, and pRS316 are ARS/CEN vectors
marked respectively with TRP1, LEU2, and
URA3 (14). The plasmid expressing thioredoxin reductase
(pRS316-TRR1) was derived by inserting a 2.3-kilobase pair
EcoRI fragment containing the TRR1 coding region and flanking regions into pRS316. The plasmid expressing human p53 from
the yeast PGK promoter (pRS314-p53, formerly called
pRS314-PGK-SN) and the plasmid carrying the p53-responsive reporter
gene (pRS315--gal, formerly called pRS315-PG-
-gal) were obtained
from S. Thiagalingam et al. (8).
-Galactosidase Assays--
-Galactosidase assays were
performed as described by Kippert (15) using the liquid nitrogen
freezing/sodium lauroyl sarcosinate method. Results are expressed as
nmol o-nitrophenol generated per 30-min incubation
normalized to 107 cells (1 A420 = 222 nmol o-nitrophenol/ml). Values are the means ± the
S.D. of the indicated number of transformants each assayed in
quadruplicate.
Western Blot Assays--
Cells (109) were washed
with TE buffer (10 mM Tris, 1 mM EDTA, pH 7.0),
and the cell pellets were frozen in liquid nitrogen. Cells were
disrupted by grinding frozen pellets, with frequent additions of liquid
nitrogen, in a mortar with a pestle until less than 5% intact cells
remained. Disrupted cells were diluted with an equal volume of 2×
sample buffer (125 mM Tris, 2% SDS, 25% glycerol, 140 mM -mercaptoethanol, 40 mM EDTA, pH 6.8),
heated to 100 °C for 3 min and centrifuged (12,000 × g) for 15 min to remove cell debris. Protein concentrations
in the supernatants were determined by the Bradford method (16) using
bovine serum albumin as standard.
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RESULTS |
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Thioredoxin Reductase Is Required for p53-dependent
Reporter Gene Expression in Budding Yeast--
Prompted by the work
implicating thioredoxin reductase in the growth-inhibitory and
transactivational action of p53 in S. pombe (11), we
investigated the effect of thioredoxin reductase gene mutations on p53
transcriptional activity in S. cerevisiae. A plasmid
encoding a p53-responsive LacZ reporter gene
(pRS315--gal) and an effector plasmid encoding human p53 under the
control of the constitutive PGK promoter (pRS314-p53) were
introduced into strains that carried either a wild type
(TRR1) or a null (
trr1) allele of the gene
encoding thioredoxin reductase. Table I
summarizes the results of the
-galactosidase assays. Reporter gene
expression was high in transformants of the TRR1 strain. In
contrast,
trr1 transformants had more than 10-fold lower
but nevertheless detectable levels of
-galactosidase activity.
Furthermore, reporter gene activity required p53 expression because
-galactosidase activity could not be detected in transformants of
either the wild type strain or the null mutant strain when the
p53-effector plasmid was replaced with the empty pRS314 vector.
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Characterization of p53 Requirement for Thioredoxin
Reductase--
The observation that p53 cannot transactivate a
p53-responsive reporter gene in yeast lacking thioredoxin reductase
could have two basic explanations. In the absence of thioredoxin
reductase, either the steady state levels of p53 protein could be
reduced or the activity of p53 itself could be inhibited. To invesigate the effect of the trr1 mutation on the amount of p53
protein in S. cerevisiae, p53 levels were determined by
immunoblot analysis as shown in Fig.
1A. The wild type
TRR1 strain transformed with (lanes 1-3) or
without (lane 4) the p53-expressing effector plasmid served
respectively as positive and negative controls for the Western blot
assay. Quantitative densitometry established that two
trr1 transformants lacking thioredoxin reductase
(lanes 6 and 8) had just as high or higher p53
protein levels as two other
trr1 transformants
ectopically expressing thioredoxin reductase (lanes 5 and
7). Because p53 protein levels clearly remained unaffected in the absence of thioredoxin reductase, it is the ability of p53 to
act as a transcriptional activator, not the amount of p53 protein
per se, that is down-regulated in the
trr1
mutant.
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DISCUSSION |
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The results presented here show that transactivation of a
-galactosidase reporter gene by human p53 was markedly inhibited in
a S. cerevisiae
trr1 mutant lacking
thioredoxin reductase. Ectopic expression of thioredoxin reductase from
a single copy plasmid in the
trr1 mutant circumvented the
inhibition and restored strong p53-dependent
transactivation. Inhibition of reporter gene expression was not due to
diminished amounts of p53 protein. Because thioredoxin reductase was
also found necessary for p53 activity in S. pombe (11), an
organism estimated to be separated evolutionarily from S. cerevisiae by one billion years, the thioredoxin reductase requirement likely reflects a conserved mechanism also operating in
humans. Thioredoxin reductase is a protein disulfide reductase. Our
results thus suggest that p53 can form disulfides and that these
disulfides must be reduced in order for the protein to function as a
transcription factor. Recent biochemical experiments have shown that
the pharmacological application of oxidizing and reducing agents can
modulate the biological activities of murine (17) and human (18) p53.
In particular, treatment of p53 with reducing agents enhances
sequence-specific DNA binding (17).
Human p53 is a tetrameric phosphoprotein. The 393-residue polypeptide
contains five conserved regions (I-V) that are nearly identical in all
vertebrates analyzed. Biochemical and reverse genetic experiments have
defined three functional domains. The proline-rich, acidic N-terminal
domain (residues 1-43) contains conserved region I, has been shown to
interact with TATA-binding protein, and is involved in transcriptional
activation. The large, central core domain (residues 100-300) contains
conserved regions II-V, is involved in DNA binding, and is the
location of almost all oncogenic p53 mutations. The basic C-terminal
domain (residues 320-360) contains nuclear localization signals and is
involved in p53 tetramerization. X-ray diffraction and NMR structures
of the core domain and oligomerization domain, respectively, have been
determined (19, 20). The core domain is tightly folded and resembles
NF-B in having nine
structures arranged in two sheets. A
tetrahedrally coordinated zinc atom holds two loops, L2 and L3, such
that a critical Arg residue in L3 contacts bases in the minor groove. A
loop-sheet-helix structure contacts bases in the major groove.
As depicted in Fig. 2, the core domain of human p53 has five surface cysteines. If a particular Cys-to-Ser mutation were to result in a p53 protein that no longer required thioredoxin reductase for activity, it would constitute strong evidence that the cysteine normally resident at the site is prone to oxidation and that thioredoxin reductase keeps the cysteine reduced and the protein active. The role of cysteine residues in the regulation of murine p53 activity has been investigated by Rainwater et al. (17). Cys-to-Ser mutations at Cys173 or Cys239 (corresponding to human Cys176 and Cys242) abolish DNA binding, transactivation of reporter gene expression, and tumor suppression. These two cysteines are critical for coordinating zinc and stabilizing the structures of loops L2 and L3. In contrast, Cys-to-Ser mutations at Cys179 or Cys274 (corresponding to human Cys182 and Cys277) have little or no effect on the biological activities of p53, but these mutants were not further tested to see if treatment with reducing agents was still required for enhanced sequence-specific DNA binding of p53.
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Evidence for redox control of p53 activity has broad implications. At
present, it is not clear how the activity of p53 is regulated. Redox
regulation offers a new paradigm for control of transcription factor
activity that compliments other mechanisms involving phosphorylation
(21) and acetylation (22). Reduction of disulfides might be part of the
mechanism by which p53 is activated as a transcription factor by DNA
damage. Alternatively, oxidation of thiols may be part of the mechanism
by which p53 is inactivated once damaged DNA has been repaired and it
is appropriate for cells to enter S phase. Evidence suggestive of redox
control of transcription factor activity has been obtained for NF-B
(23), Myb (24), AP-1 (25), and PEBP2/CBF (26).
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ACKNOWLEDGEMENTS |
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We thank André Machado for suggesting
this study. Jay Evans and Margot Pearson provided advice about and help
with the Western blot assays. Sam Thiagalingam generously supplied
plasmids pRS314-PGK-SN and pRS315-PG--gal. Ahmet Koc, Chris Day, and
Jeff Hutchinson helped with some of the experiments.
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FOOTNOTES |
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* This work was supported by Grant MRF 598 from the Medical Research Foundation of Oregon and Grant ACS 898 from the Oregon Division of the American Cancer Society, Inc.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed. Tel.: 541-737-3119;
Fax: 541-737-0481; E-mail: merrillg{at}ucs.orst.edu.
1 The abbreviation used is: CDK, cyclin-dependent protein kinase.
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REFERENCES |
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