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Molecular and Cellular Biology, January 2000, p. 233-241, Vol. 20, No. 1
0270-7306/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
ei24, a p53 Response Gene Involved in Growth
Suppression and Apoptosis
Zhengming
Gu,1
Cathy
Flemington,2
Thomas
Chittenden,2 and
Gerard P.
Zambetti1,3,*
Department of Biochemistry, St. Jude
Children's Research Hospital, Memphis, Tennessee
381051; Department of Biochemistry,
University of Tennessee, Memphis Tennessee
381633; and Apoptosis Technology,
Inc., Cambridge, Massachusetts 021392
Received 26 August 1999/Returned for modification 24 September
1999/Accepted 7 October 1999
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ABSTRACT |
DNA damage and/or hyperproliferative signals activate the wild-type
p53 tumor suppressor protein, which induces a G1 cell cycle
arrest or apoptosis. Although the mechanism of p53-mediated cell cycle
arrest is fairly well defined, the p53-dependent pathway regulating
apoptosis is poorly understood. Here we report the functional
characterization of murine ei24 (also known as
PIG8), a gene directly regulated by p53, whose
overexpression negatively controls cell growth and induces apoptotic
cell death. Ectopic ei24 expression markedly inhibits cell
colony formation, induces the morphological features of apoptosis, and
reduces the number of 
-galactosidase-marked cells, which is
efficiently blocked by coexpression of Bcl-XL. The
ei24/PIG8 gene is localized on human chromosome
11q23, a region frequently altered in human cancers. These results
suggest that ei24 may play an important role in negative
cell growth control by functioning as an apoptotic effector of p53
tumor suppressor activities.
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INTRODUCTION |
Inactivation of the p53 tumor
suppressor is the most common genetic alteration detected in human
malignancies, occurring in more than 50% of all tumors. Genetically
engineered mice that lack p53 expression invariably develop lethal
tumors within 3 to 6 months of age, underscoring the importance of p53
in the prevention of cancer (9, 21). Wild-type p53 (wtp53)
plays a key role in tumor suppression by monitoring DNA damage and
executing pathways that negatively control cell growth, either by
blocking cells in the G1 phase of the cell cycle or
inducing apoptosis (for review, see reference 26).
wtp53 regulates these processes, at least in part, by functioning as a
transactivator of gene expression, and its activity as a tumor
suppressor correlates with this function (32). wtp53 induces
the expression of its target genes by binding to DNA in a
sequence-specific fashion and by interacting with various components of
the transcription complex. Some of the better-characterized target
genes transcriptionally activated by p53 include p21cipl, gadd45, cyclin G, mdm2,
bax, fas/APO1, and IGF-BP3
(24, 26).
A critical target that mediates wtp53-induced cell cycle arrest is
p21Cip1, which is a cyclin-dependent kinase inhibitor (11, 14,
37). Overexpression of p21Cip1 in murine fibroblasts, like that
of wtp53, inhibits cell growth in the G1 phase of the cell
cycle (11). Consistent with this observation, fibroblasts that lack p21Cip1 fail to efficiently arrest in G1 phase in
response to wtp53 during DNA damage (8). By contrast, the
mechanism by which p53 induces apoptosis is poorly understood. Several
p53-regulated target genes are bona fide proapoptotic factors, such as
bax and fas/APO1 (29, 30).
However, elimination of bax or
fas/APO1 gene expression has no consequence for
p53-induced cell death in gamma-irradiated murine thymocytes,
suggesting that there are alternative mediators of p53-dependent
apoptosis (23, 35).
ei24 is a DNA damage response gene originally isolated from
NIH 3T3 fibroblasts that were undergoing etoposide-induced cell death
(25). Since etoposide-induced apoptosis in these cells is
p53 dependent and requires new RNA and protein synthesis, it was
speculated that ei24 could be a p53-regulated gene. Indeed, subsequent studies with cells that conditionally express wtp53 or gamma
irradiation of normal and p53
/ thymocytes
established a clear correlation between p53 function and
ei24 gene expression. Subsequently, the human
ei24 gene, PIG8 (designated
ei24/PIG8) was isolated by Polyak and coworkers
from colon carcinoma cells undergoing apoptosis in response to the ectopic expression of wtp53 (33). In this study, serial
analysis of gene expression of more than 7,200 mRNA transcripts
revealed that PIG8 was one of only 14 identified genes that
were induced in a p53-dependent manner (33).
Murine ei24 mRNA is 2.4 kb in length, polyadenylated, and
widely expressed in many tissues to varying degrees (25).
The Ei24/PIG8 protein is highly conserved between mouse and human and
shares more than 50% similarity to an open reading frame in Caenorhabditis elegans. The deduced amino acid sequence
yields little or no information about the possible function of this
gene. Nonetheless, the fact that ei24 gene expression is
rapidly induced as part of a p53-dependent pathway in DNA-damaged cells
and that this response precedes or parallels the onset of apoptosis
suggest that ei24 may play an important role in negatively
controlling cell growth and/or tumor suppression (25, 33).
In the present study, we demonstrate that ei24 is an
immediate-early p53 response gene and that overexpression of
ei24 suppresses cell growth by inducing apoptotic cell
death. The ei24/PIG8 gene is located on human
chromosome 11q23 in a region that is frequently altered in several
human malignancies. These findings indicate that ei24 may be
a newly recognized tumor suppressor that plays an important role in the
prevention of certain cancers.
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MATERIALS AND METHODS |
Cell lines and culture methods.
All cell lines were cultured
in Dulbecco's modified Eagle's medium supplemented with 10% fetal
bovine serum, glutamine (2 mM), and penicillin (100 IU/ml)-streptomycin
(100 µg/ml) at 37°C in 5% CO2 unless otherwise
indicated. 2a39pBabePuro and 2a39p53ER cells are derived from
p53-deficient mouse embryo fibroblasts and express E1A and
T24 H-ras oncogenes (25, 36). The 2a39pBabePuro cells serve as a vector-only negative control, whereas 2a39p53ER fibroblasts express a conditionally active human wtp53 gene fused to a
modified hormone-binding domain of the murine estrogen receptor (25, 36). Functional activation of the p53ER fusion protein was achieved by treating 2a39p53 ER cells with 3.3 µM tamoxifen (Sigma, St. Louis, Mo.), resulting in the induction of apoptosis in
these cells (36). COS-7 is an African green monkey kidney cell line that expresses functionally inactive wtp53 due to the simian
virus 40 large-T antigen oncogene (American Type Culture Collection,
Manassas, Va.). (10)1 cells are immortal murine fibroblasts containing
deletions in the endogenous p53 gene and are null for p53 expression
(15). Rat1 fibroblasts express endogenous wtp53 and were
used for the -galactosidase (-Gal) marker apoptosis assays, as
previously described (6). The parental murine myeloid leukemia M1 cell line, which is null for endogenous p53, and the derivative M1tsp53 cell line that expresses the temperature-sensitive mutant p53 protein (A135V) were kindly provided by Dan Liebermann (Temple University, Philadelphia, Pa.) and were cultured in RPMI 1640 supplemented with 10% horse serum at 37°C in 5% CO2.
M1tsp53 cells were cultured at 32.5°C to convert the
temperature-sensitive mutant p53A135V into the wild-type conformation.
Where indicated, cells were treated with 12.5 ng of recombinant IL-6
per ml (R & D Systems, Minneapolis, Minn.) to inhibit p53-mediated
apoptosis. Cells were transfected with plasmid DNA by the
lipofectin-mediated method as suggested by the manufacturer (Gibco BRL,
Gaithersburg, Md.) or by the calcium-phosphate precipitation method
(22).
Plasmid DNA.
The prkMei24 plasmid, which expresses a FLAG
epitope-tagged version of murine ei24, was constructed by
subcloning the 0.8-kb XbaI/NdeI and 0.47-kb
NdeI/NotI ei24 cDNA fragments from
pKSf1-clone 11 (25) into the prk5 vector. The FLAG
epitope-tagged coding sequence was fused at the 3' end of the murine
ei24 cDNA by PCR with the following pair of primers:
5'-GCTTAGCAAAGTTGTGAATGCC-3' (forward primer) and
5'-CGGCGGCCGCCTACTTGTCATCGTCGTCCTTGTAGTCATGGCCTGCAGCAGCTTTCAGTTTGGCAGGAGA-3' (reverse primer). The prkHei24 plasmid expressing human
ei24/Pig8 was constructed by subcloning the
1.3-kb NdeI/NotI cDNA fragment from
PIG8 (33) and a 0.7-kb
BamHI/NdeI fragment into prk5. The 0.7-kb
BamHI/NdeI DNA fragment was created by reverse
transcription-PCR with the following pair of primers:
5'-AAGAATTCATGGGGCAGGGCCGGAGCCG-3' (forward primer) and
5'-GGACATATGCAGGAGGCTAACCAGCT-3' (reverse primer). The
template for this reaction was total RNA prepared from human myeloid
leukemia ML-1 cells. The ei24 promoter-reporter plasmid
(pGLKH) was constructed by inserting the proximal 3.5-kb KpnI/HindIII DNA fragment from the murine
genomic BACM-83-M10 clone (Genome Systems, Inc., St. Louis, Mo.), which
contains the promoter region and exon 1 of the murine ei24
gene, upstream of the luciferase reporter in the pGL2 vector (Promega
Corp., Madison, Wis.).
Immunoblotting and immunoprecipitation.
Transiently
transfected COS-7 cells that remained attached or were nonadherent were
collected either separately or pooled and lysed in
radioimmunoprecipitation assay (RIPA) buffer (50 mM Tris-HCl [pH
7.6], 150 mM NaCl, 1% Triton X-100, 0.1% sodium deoxycholate, and
Protease Inhibitor Cocktail [Boehringer Mannheim, Indianapolis,
Ind.]). The samples were analyzed for protein content by the Bradford
method (Bio-Rad Laboratories, Hercules, Calif.), separated through a
sodium dodecyl sulfate (SDS)-12% polyacrylamide gel and transferred
to a PVDF-PLUS transfer membrane (Micron Separations, Inc., Westboro,
Mass.). The membranes were probed with rabbit antiserum (Ab22), which
is specific for the N-terminal murine Ei24 peptide (PQSVERKQESEPRIVS),
and subsequently incubated with a horseradish peroxidase-monkey
anti-rabbit IgG secondary antibody (Amersham, Arlington Heights, Il.).
The samples were washed three times in TBST (10 mM Tris [pH 8], 44 mM
NaCl, 0.05% Tween 20) (17) and analyzed with the
SuperSignal Chemiluminescent Western blotting kit according to the
manufacturer's protocol (Pierce, Rockland, Ill.). Immunoprecipitations
(IP) were performed as previously described (17). Briefly,
cells were lysed in RIPA buffer without SDS and the nonspecific
adsorbents were removed by preincubating the cell extract with 40 µl
of 50% protein A-Sepharose. The specific antibodies were added to the
cell extract with 30 µl of 50% protein A-Sepharose in a final
volume of 500 µl and incubated at 4°C for 2 h. The
immunocomplexes were washed three times with RIPA buffer without SDS
and resuspended in sample buffer for SDS-polyacrylamide gel
electrophoresis analysis.
Gel mobility shift assays.
Electromobility shift assays
(EMSA) were carried out as previously described (12). The
synthetic double-stranded oligonucleotides used in this study included
the following sequences: p53CON, 5'-AGGCATGCCTAGGCATGCCT-3'; p53RE, 5'-GGGCTGGCAGGCCGGAGCTAGTTCCTAA-3'; and p53MRE,
5'-GGGCTGGTAGTCCGGAGTTATTTCCTAA-3'. The probes were
radiolabeled with [
-32P]ATP and T4 polynucleotide
kinase and incubated with 100 ng of baculovirus-expressed human p53
protein (>95% pure) alone or together with 2 µg of PAb421 (Oncogene
Research Products, Cambridge, Mass.) in binding buffer containing 20 mM
HEPES (pH 7.9), 25 mM KCl, 0.1 mM EDTA, 2 mM MgCl2, 0.5 mM
dithiothreitol, 0.25% Nonidet P-40, 2 mM spermidine, 10% glycerol,
0.1 ng of bovine serum albumin and 0.04 µg of poly(dG-dC) in a final
reaction volume of 20 µl at 22°C for 15 min. As previously
described, the monoclonal PAb421 antibody is required to activate wtp53
DNA binding (19). The protein-DNA complexes were resolved in
a native 4% polyacrylamide gel and analyzed by autoradiography.
Northern blot analyses.
Total RNA was harvested with the
RNeasy Mini Kit as recommended by the manufacturer (Qiagen, Valencia,
Calif.). The RNA samples (10 µg) were denatured in 1 M glyoxal-10 mM
NaH2PO4 (pH 7.0) for 1 h at 50°C and
resolved through a 1.2% agarose gel. The RNA samples were transferred
to a Zeta-Probe blotting membrane (Bio-Rad) in transfer buffer
containing 10 mM NaOH. The membrane was blocked in hybridization
solution (1 mM EDTA, 0.25 M Na2HPO4 [pH 7.2], and 7% SDS) for 5 min and hybridized with
-32P-radiolabeled DNA probes for 16 h in fresh
hybridization solution at 65°C. The membrane was washed twice at
65°C for 30 min per wash in buffer I (1 mM EDTA, 40 mM
Na2HPO4 [pH 7.2], and 5% SDS) followed by
two washes in buffer II (1 mM EDTA, 40 mM
Na2HPO4 [pH 7.2], and 1% SDS). The samples
were quantitated by PhosphorImager analysis with Imagequant software.
Microinjection.
Cells were microinjected with a Nikon
Diaphot 300 inverted microscope with an Eppendorf pressure injector
(model 5246) and micromanipulator (model 5171). Cells were plated on
glass coverslips 16 h prior to injection in Dulbecco's modified
Eagle's medium supplemented with 10% fetal bovine serum. The cells
were injected with a green fluorescent protein (GFP) expression plasmid
alone or with 10 pg of either prk5 vector only or
ei24/PIG8 expression plasmid DNA. On average, 100 to 150 cells were injected per sample. Twenty-four hours after
injection, cells expressing GFP were scored for morphological features
of apoptosis and photographed to document phenotypic changes.
-Gal marker apoptosis assay.
The effect of
ei24 expression on cell viability was examined in transient
transfection assays as previously described (6). Rat1
fibroblasts were plated in 24-well tissue culture dishes at 3.5 × 104 cells/well and transiently transfected by the
Lipofectamine procedure (Gibco BRL) with a -Gal plasmid to
biochemically mark productively transfected cells. Cells were
cotransfected in triplicate with the -Gal marker and either prk5
vector only (Vector), prk5Mei24 (Mei24), pBabeBcl-XL
(Bcl-XL), or Mei24 plus Bcl-XL (Mei24 + Bcl-XL) DNA. Transfections were balanced for equal amounts
of total DNA. Twenty-four hours posttransfection, the cells were fixed
and stained with X-Gal
(5-bromo-4-chloro-3-indolyl--D-galactopyranoside) to
detect -Gal-expressing cells. Transfected cells were quantitated by
counting the number of blue-stained cells within a defined area (five
randomly selected microscopic fields). The experiment was repeated
three times, once with independently prepared plasmid DNAs.
Fluorescence in situ hybridization.
A human
ei24/PIG8 bacterial artificial chromosome (BAC)
clone was labeled with digoxigenin-11-dUTP (Boehringer Mannheim) by nick translation and hybridized to normal metaphase chromosomes in a
solution containing 50% formamide, 10% dextran sulfate, and 2× SSC
(1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate). Specific hybridization signals were detected with fluorescein-labeled
digoxigenin antibody (green) (Oncor, Inc., Gaithersburg, Md.).
Definitive chromosomal assignment was confirmed by cohybridization of
human ei24/PIG8 BAC clone with a biotinylated
chromosome 11 centromere-specific probe, D11Z1 (red) (Oncor, Inc.). The
labeled probes were hybridized to metaphase cells in a solution
containing 60% formamide, 10% dextran sulfate, and 2× SSC. Specific
probe signals were detected by incubating the slides in
fluorescein-labeled anti-digoxigenin and Texas red avidin (Oncor,
Inc.). The chromosomes were then stained with
4',6-diamidino-2-phenylindole (DAPI) and photographed.
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RESULTS |
ei24 gene expression is specifically induced by
p53.
Previous studies demonstrated that ei24 gene
expression is induced in response to elevated levels of wtp53 in a
variety of different cell-based assays, suggesting that ei24
is a p53-regulated target gene. However, it should be noted that in
each case studied, the cells responded to the elevated levels of p53 by
undergoing apoptosis (25, 33). This fact raised the
possibility that ei24 is not a p53-regulated gene per se;
rather, ei24 may be a sensor of cell death which is
indirectly induced during apoptosis.
To directly address this issue, we employed the murine myeloid leukemia
M1 cell line, which expresses the temperature-sensitive mutant
p53-val135 (tsp53) gene (40). The
M1tsp53 cells express high levels of p53 in the mutant conformation and
actively proliferate when grown at 37°C. However, when the cells are
shifted to 32.5°C, the tsp53 protein assumes a wild-type
conformation, which rapidly induces cell death. Interestingly, the
M1tsp53 cells are efficiently rescued from p53-mediated cell death at
32.5°C by the addition of interleukin-6 (IL-6) (40). We
and others have recently demonstrated that certain cytokines, such as
IL-6, inhibit p53-mediated cell death by blocking the p53 pathway at a
point that is downstream from the regulation of its target genes
(4, 34). This system therefore affords the opportunity to
study the regulation of gene expression in response to wtp53 without
inducing apoptosis. When M1tsp53 cells were cultured at 32.5°C,
ei24 mRNA levels were markedly induced and this response was
concomitant with a loss in cell viability (Fig.
1). Pretreatment of the M1tsp53 cells
with IL-6 before shifting the temperature to 32.5°C completely
blocked cell death but had no effect on the induction of
ei24 gene expression (Fig. 1). Identical results were
obtained when bax expression was examined under these
conditions (data not shown). Therefore, ei24 gene expression
directly responds to p53 and is not induced as a secondary response to
p53-mediated cell death.
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FIG. 1.
ei24 expression is selectively induced in
response to wtp53. (Left) Murine M1 myeloid cells expressing a
temperature-sensitive mutant p53 were grown at 37°C (mutant
conformation) or shifted to 32.5°C (wtp53 conformation and function).
In parallel and prior to the temperature shift, cells were pretreated
with 12.5 ng of IL-6 per ml (treatment is indicated by a +), which
blocks p53-mediated cell death and induces differentiation
(40). At the indicated intervals, cells were harvested and
analyzed for ei24 gene expression by Northern blotting.
Ethidium bromide-stained RNA was photographed prior to transfer to
confirm equal loading of samples (bottom). PhosphorImager analysis
demonstrates the induction of steady-state levels of ei24
mRNA during activation of p53 at the permissive temperature (top). Cell
viability was monitored by propidium iodide staining and
fluorescence-activated cell sorter analysis (right). Cells grown at the
permissive temperature undergo apoptosis in the absence of IL-6 and
maintain viability while arresting in the G1 phase of the
cell cycle in the presence of IL-6.
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ei24 is a direct target for wild-type p53.
Although ei24 gene expression correlated with p53 levels and
was not a by-product of cell death, it was not clear whether ei24 was an immediate- or delayed-early p53 response gene.
For example, p53 could activate ei24 gene
expression by inducing an intermediate factor that regulates
ei24 expression. To address this mechanism, we utilized a
p53/ mouse embryo fibroblast cell line that
constitutively expresses a p53 estrogen receptor (p53ER) fusion protein
that is not active under normal growth conditions (25, 27).
The p53ER fusion protein is functionally activated by the addition of
tamoxifen (Tam), and this subsequently induces the expression of p53
target genes and apoptotic cell death (Fig.
2) (25, 36). To test the
possibility that an intermediate factor may regulate ei24 expression, we pretreated cells with cycloheximide (10 µg/ml) for 45 min to inhibit de novo protein synthesis and then added 3.3 µM Tam
for an additional 3 or 6 h to functionally activate p53ER.
Preliminary characterization of the assay determined that protein
synthesis was inhibited approximately 93% by cycloheximide within 45 min, as determined by 35S-methionine-cysteine
incorporation (data not shown). We also considered the nature of the
very short half-life of wtp53 (~15 to 20 min), since protein
synthesis was inhibited during the cycloheximide treatments. Stability
measurements determined that the half-life of p53ER was greater than
5 h when activated by Tam (data not shown), thus ensuring the
availability of p53ER at the later time points (3 and 6 h).
Northern blot analysis of the vector-only control cells (pBabe)
demonstrated that cycloheximide or cotreatment with cycloheximide and
Tam had no significant effect on the expression of endogenous
ei24 mRNA steady-state levels. By contrast, functional activation of wtp53 by Tam treatment of p53ER fibroblasts dramatically induced ei24 mRNA levels in either the presence or the
absence of cycloheximide (Fig. 2). These data indicate that
ei24 is an immediate-early-response gene that is directly
regulated by wtp53.
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FIG. 2.
ei24 is an immediate-early wtp53 response
gene. Murine 2a39 fibroblast cell lines harboring either the
pBabepuro-only vector (pBabe) or expressing the conditional wild-type
p53ER fusion protein (p53ER) were cultured under normal growth
conditions (Cont) or treated with either 10 µg of cycloheximide
(Cyclo) per ml, 100 µM Tam, or cycloheximide plus Tam (Cyclo/Tam) for
the indicated times. Cells that were treated with both cycloheximide
and Tam were preincubated with cycloheximide for 45 min to efficiently
inhibit protein synthesis prior to activation of p53ER with Tam. Total
RNA was isolated and analyzed by Northern blotting for ei24,
p21cip1, and bax expression (top). RNA was
stained with ethidium bromide prior to transfer and photographed to
document equal loading of RNA (bottom).
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To confirm these findings, we isolated an ~150-kb murine
ei24 genomic BAC clone that contains the entire cDNA coding
region.
From this BAC clone, we isolated a 3.5-kb DNA fragment
containing
the promoter region and exon 1 and subcloned these sequences
into
a luciferase reporter plasmid (see Materials and Methods).
Reporter
activity was examined in transiently transfected (10)1
fibroblasts,
which are devoid of endogenous p53 protein, thereby
eliminating
potential complications of
trans-dominant
effects (
15,
41).
Transient transfection of the
ei24 luciferase reporter into
p53-null
cells
resulted in a low but significant level of activity (~30-fold
higher
than that of the promoterless reporter), demonstrating
that the
subcloned
ei24 DNA sequence functions as a promoter to
drive
luciferase expression (Fig.
3).
Cotransfection of the reporter
with wtp53 resulted in a 15- to 25-fold
higher induction of luciferase
activity, demonstrating that the
ei24 promoter fragment is inducible
by p53 (Fig.
3). The
promoter region was sequenced and found to
contain putative p53 DNA
binding consensus sites (Fig.
3 and
4).
To verify this potential site as a specific p53 binding element,
we
synthesized complementary oligonucleotides corresponding to
this
element (p53RE) and mutated oligonucleotides as a negative
control
(p53MRE). The mutations were introduced into the fourth
and seventh
positions of sites I and II of the
ei24 probe (p53MRE),
and
these nucleotides were selected and targeted on the basis
of earlier
studies demonstrating the strict requirement of these
residues for p53
DNA binding (
10). Human wtp53 protein, purified
from
recombinant baculovirus-infected insect cells, was used in
these
binding assays. Consistent with previous reports, it was
also necessary
to include the murine monoclonal antibody PAb421,
which activates DNA
binding by binding to its epitope in the C
terminus of p53
(
19). Electrophoretic mobility shift analysis
demonstrated
that purified wtp53 protein can specifically bind
to the
ei24 wild-type site (p53RE) but not to the mutated probe
(p53MRE) (Fig.
4). These results demonstrate that the
ei24
promoter
contains functional p53 DNA binding sites and is efficiently
transactivated
by wtp53. Together with the p53ER-cycloheximide studies,
these
data establish
ei24 as an immediate-early
wtp53-inducible gene.
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FIG. 3.
The ei24 promoter is transactivated by wtp53.
The 3.5-kb DNA fragment containing the ei24 promoter region
was inserted upstream of a luciferase reporter (pGLKH) as schematically
diagrammed (top). The location of the p53 DNA binding consensus sites
are identified. To test the transcriptional activity and p53
responsiveness of the ei24 promoter, murine 10(1)
fibroblasts (p53-null cells) were cotransfected with pGLKH
and either a vector-only (CMV) or wtp53 expression plasmid (p53). In
parallel, 10(1) cells were cotransfected with p50-2, a previously
characterized p53 responsive reporter (41), and either CMV
or p53 to serve as a positive control for p53 function. Levels of
promoter activity, which are measured in relative light units (RLU), in
the absence of p53 (CMV) have been normalized. Fold activation
represents the increased reporter activity during wtp53 expression
(p53) as compared to that of the CMV samples (bottom). Open and filled
bars represent the results obtained from two independent experiments.
The average basal activity of the promoterless luciferase reporter
(pGL) and ei24 promoter-containing reporter (pGLKH) is
~7,000 RLU and 190,000 RLU, respectively.
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FIG. 4.
The ei24 promoter contains wtp53 DNA binding
sites. The p53 DNA binding consensus site (p53CON) (10)
consists of two 10-bp repeats (top). The potential p53 consensus site
located at positions  67 to 48 in the ei24 promoter
(p53RE) and a corresponding mutated sequence (p53MRE) are listed below
for comparison. Radiolabeled probes corresponding to these
double-stranded DNA sites were incubated with 100 ng of purified human
p53 protein with and without 2 µg of PAb421 as described in Materials
and Methods. As previously reported, the monoclonal antibody PAb421 is
required to activate purified p53 protein for DNA binding
(19). The protein-DNA complexes were resolved in native 4%
polyacrylamide gels and visualized by PhosphorImager analysis
(bottom).
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ei24/PIG8 is highly conserved throughout
evolution.
It was previously reported that murine and human
ei24/PIG8 cDNAs encode 317- and 318-amino-acid
proteins, respectively (25, 33). A search of the GenBank
database for related sequences revealed a series of human expressed
sequence tag (EST) clones that matched the murine C-terminal coding
region, with the exception of a single cytidine insertion that shifts
the reading frame of the published sequence at codon 266. Sequencing of
both the human (33) and murine (25) cDNA clones
obtained from these groups, with high-temperature Taq1
polymerase, confirmed the accuracy of the EST sequence and demonstrated
that the published ei24/PIG8 sequences were
incorrect. Furthermore, sequence analysis of the murine genomic
ei24 BAC clone within the corresponding coding region also
confirmed the existence of the extra nucleotide which we had previously
detected in the EST and cDNA clones. Therefore the C-terminal 50 amino
acids (residues 267 to 317) of the published murine Ei24 protein
sequence do not exist and are replaced by an additional 92 amino acids
(Fig. 5). Similarly, the published C-terminal 50 amino acids of human PIG8 are incorrect and are replaced
by an additional 92 amino acids (data not shown). The corrections in
the murine and human ei24/PIG8 sequences have
been deposited in GenBank. Comparison of the corrected mouse and human ei24/PIG8 sequences demonstrates 98% identity
between these species and murine Ei24 is 27% identical (52% similar)
to an open reading frame in C. elegans (CELF37C12.2; GenBank
accession no. U00033). These results indicate that ei24 is
remarkably conserved during evolution, possibly to maintain an
important biological function.
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FIG. 5.
Predicted amino acid sequence of murine Ei24 protein.
The previously published sequences of murine and human Ei24/PIG8
proteins contained a frameshift mutation corresponding to codon 266 (25, 33). The corrected murine Ei24 primary amino acid
sequence is presented and the site of divergence from the published
sequence is indicated by the arrowhead. The open reading frame of
murine Ei24 is 358 amino acids, which is 98% identical to human
Ei24/PIG8 and more than 50% similar to sequences found in C. elegans. The predicted sequence lacks obvious functional motifs
but does contain six putative membrane-spanning domains, which are
underlined.
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ei24 suppresses cell growth and induces cell
death.
To study the function of ei24, sequences
encoding murine ei24, which is FLAG tagged at the C
terminus, and the full-length human ei24/PIG8
cDNA (unmodified) were cloned into the prk5 vector under the
transcriptional control of a cytomegalovirus (CMV) promoter. These
plasmids were transiently transfected into COS-7 cells with Lipofectamine or by calcium phosphate precipitation. Ei24 protein expression was analyzed by Western blot with a rabbit polyclonal serum
that was prepared from animals immunized with an N-terminal Ei24-conjugated peptide. This antiserum cross-reacts with both mouse
and human Ei24/PIG8 protein (Fig. 6 and
data not shown). Murine ei24 expression was detected with Ab22 only in
samples transiently transfected with full-length ei24 expression
vectors (Fig. 6A). Although Ab22 is specific and can readily recognize ectopically expressed Ei24 protein, it is not yet of sufficient titer
or affinity to detect endogenous Ei24. Expression of murine Ei24 was
also confirmed by IP-Western blot analysis with a FLAG-specific antibody for the IP step and Ab22 for probing the nylon membrane (Fig.
6B). Interestingly, murine ei24/PIG8 gene
expression in the floating cells was approximately 500-fold higher per
microgram of protein than in the healthy cells that remained attached
to the tissue culture dish (Fig. 6B). These results suggested that ei24/PIG8 may be antithetical to cell growth.
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|
FIG. 6.
Expression of ei24 in transiently transfected
COS-7 cells. COS-7 cells were transfected with 1 or 10 µg of prk5
vector-only or mouse ei24-FLAG expression plasmids
(prkMei24-1 and -3 are identical but independently prepared DNA). At
48 h posttransfection, detached and adherent cells were harvested
either separately or pooled. (A) Lysates were prepared from pooled
cells and 50 µg of total protein was analyzed by direct Western
blotting with Ei24-specific rabbit polyclonal Ab-22 antiserum, as
described in Materials and Methods. (B) Lysates were prepared from
detached (D) and adherent (A) cells and either 50 µg or 500 µg of
total cell protein was immunoprecipitated with anti-FLAG antibody and
analyzed by Western blotting with Ab-22 as the primary antibody. A
10-fold-smaller amount of protein from the detached cells yielded
severalfold-higher levels of Ei24 than the adherent cells. The position
of the 32-kDa molecular weight marker is indicated.
Hemagglutinin-tagged murine Ei24 protein (HA-Mei24) isolated from
recombinant baculovirus-infected Sf9 cells was used as a positive
control.
|
|
The effects of
ei24 on cell growth were initially addressed
in colony reduction assays by cotransfecting COS-7 cells with
pcDNA3-neo and either prk5 vector-only or prkHEI24 plasmid DNA.
The
cells were selected in 0.7 mg of G418 per ml for 10 days and
colonies
that formed during this time were then stained with Wright-Giemsa
dye.
As shown in Fig.
7, colonies readily
formed when transfected
with pcDNA3-neo and the vector-only plasmid
(101 ± 12 CFU). By
contrast, the number of colonies that formed
when cotransfected
with the neomycin resistance marker and
ei24/
PIG8 expression vectors
were dramatically
reduced (8 ± 2 CFU for murine
ei24 and 7 ± 2
CFU
for human
ei24/
PIG8), representing a >90%
reduction in colony
formation when
ei24/
PIG8 is
expressed. Efficient growth suppression
was also observed upon
transfection of human lung carcinoma H358
cells with
ei24/
PIG8 (data not shown). These results
demonstrate
that
ei24/
PIG8 is a negative growth
regulator but do not distinguish
between possible effects on cell cycle
arrest or cell death.
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|
FIG. 7.
ei24 suppresses colony growth of COS-7 cells.
Cells were cotransfected with pcDNA3-neo and either prk5 vector-only
DNA (Vector) or prkHei24 (EI24), which expresses human ei24/PIG8
protein. The transfected cells were selected in 0.7 mg of G418 per ml
for 10 days, stained with Wright-Giemsa dye, and quantitated for colony
formation.
|
|
To study these biological processes in more detail, NIH 3T3 fibroblasts
were coinjected with a GFP expression plasmid together
with the prk5
vector-only or
ei24 expression constructs. Twenty-four
hours
after injection, the cells were analyzed for morphological
changes by
phase-contrast and fluorescence microscopy and photographed.
As shown
in Fig.
8, the GFP-positive cells
injected with the vector-only
DNA appeared normal, whereas the cells
that were injected with
the
ei24 expression plasmid
displayed the typical morphological
features of apoptosis
(
39), including significant membrane blebbing,
vacuolization, and nuclear condensation. Induction of apoptosis
was
similarly observed in microinjection assays when using HeLa
cells (data
not shown). These results suggest that
ei24 suppresses
cell
growth through the activation of an apoptotic pathway.
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|
FIG. 8.
Ectopic expression of ei24 in immortal murine
fibroblasts induces morphological features of apoptosis. NIH 3T3 cells
were coinjected with a GFP expression plasmid and either prk5
vector-only (Vector), prkHei24 (Hei24), or prkMei24 (Mei24) DNA.
Twenty-four hours after injection, cells were examined by
phase-contrast (bottom) and fluorescence (top) microscopy to identify
productively injected cells and photographed. Morphological changes
consistent with an apoptotic response were only apparent in
ei24-expressing cells. These results are representative of
three independent experiments, including studies with HeLa cells.
|
|
Induction of apoptosis by
ei24 was demonstrated with a
transient transfection
-Gal reporter assay (
6). In these
experiments,
Rat1 cells were transfected with a
-Gal reporter, which
allows
productively transfected cells to be identified by staining them
blue with X-Gal (
6). Cotransfection of Rat1 fibroblasts with
the prk5 vector-only and
-Gal reporter plasmids resulted in the
formation of approximately 1,200 blue-stained cells per defined
area
(Fig.
9). By contrast, cotransfection of
Rat1 cells with
-Gal and
ei24 reduced this number by
approximately 90%. Inclusion
of a Bcl-X
L expression
plasmid, which encodes a suppressor of
apoptosis (
2), in the
-Gal- and
ei24-cotransfected samples
effectively restored
the number of blue cells to the level observed
in control-transfected
cells. These results demonstrate that
ei24 can function in
an apoptotic pathway that is efficiently repressed
by
Bcl-X
L.
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|
FIG. 9.
Ectopic expression of ei24 induces apoptosis
that is inhibited by Bcl-XL. Rat1 fibroblasts were
transiently transfected in triplicate with the -Gal reporter and
prk5 vector-only plasmid (Vector) or cotransfected with the -Gal
reporter and either prk5Mei24 (Mei24), pBabeBcl-XL
(Bcl-XL), or Mei24 plus Bcl-XL (Mei24 + Bcl-XL). Forty-eight hours after transfection, cells were
stained for -Gal activity and quantitated by scoring blue positive
cells within a defined area. These experiments were repeated three
times, once with independently prepared plasmid DNAs. Error bars,
standard error.
|
|
| |
DISCUSSION |
DNA damage inhibits normal cell growth by activating p53-regulated
pathways leading to either a G1 phase cell cycle arrest or
apoptosis. The mechanism for p53-mediated cell cycle arrest has been
well characterized, whereas its role in regulating cell death is poorly
understood. We report here the characterization of
ei24/PIG8, which is a highly conserved gene that
is directly regulated by wtp53 and negatively controls cell growth by
inducing apoptosis.
The ei24 promoter lacks a canonical TATA box but does
contain multiple copies of putative SP1, AP1, and AP2 sites (data not shown). These features are characteristic of many housekeeping genes,
and consistent with this observation, ei24 is expressed in
many tissues, including heart, skeletal muscle, lung, and liver (25). Our data also demonstrate that the ei24
promoter contains p53 DNA binding sites and is directly regulated by
wtp53. Although the human promoter has not yet been isolated,
ei24/PIG8 expression is inducible in human cells
by wtp53 (33), implying that the p53 response element has
been conserved. Therefore, ei24 is a DNA damage-inducible
gene that lies downstream in the p53 pathway. An interesting model
proposed by Chen and coworkers (5) suggests that the levels
of wtp53 are an important determinant in whether a cell undergoes cell
cycle arrest or apoptosis. Growth arrest has been correlated with low
levels of p53, whereas at higher levels of p53 cells are more prone to
apoptosis. It remains to be determined whether ei24
expression is selectively regulated by p53 in a dose-dependent and/or
cell context-specific manner. In addition, other signals (e.g.,
differentiation) that are p53 independent may also regulate
ei24 gene expression and will need to be addressed.
ei24/PIG8 was mapped by fluorescence in situ
hybridization analysis to human chromosome 11q23, a region frequently
altered in human cancers (data not shown). Within this region is the
ATM (mutated in ataxia telangiectasia) gene and the
MLL gene, the latter a primary target for rearrangement in
acute lymphoblastic and therapy-related myelogenous leukemias. However,
there are a number of human malignancies, such as invasive cervical
cancer, breast carcinoma, and malignant melanoma, that exhibit loss of heterozygosity within 11q23, and the putative tumor suppressor gene(s)
located in this region has not yet been identified (1, 13, 16,
18). Since ei24 is a downstream target of wild-type p53 and overexpression of ei24 inhibits cell growth and
induces apoptosis, we propose that ei24/PIG8 is a
reasonable tumor suppressor candidate that should be addressed in these cancers.
Our data indicate that enforced expression of ei24 induces
apoptosis independent of functional p53. Microinjection studies demonstrated that ei24 induces an apoptotic response in HeLa
cells (data not shown), which encode wtp53 but fail to express
functional p53 protein due to its rapid degradation directed by the
human papillomavirus E6 oncogene product (26). Similarly,
transfection of ei24 into COS-7 cells, which are
functionally null for p53 due to inactivation by simian virus T antigen
(26), inhibits cell growth and induces cell death. These
results suggest that once expressed, ei24 can initiate an
apoptotic response without further requirement for wtp53 activity.
These results also strengthen the argument that ei24 is
downstream within the p53 pathway and suggest that ei24 may
play an important role as an apoptotic effector of p53 tumor suppressor
activity. However, physiological levels of ei24 may not
always lead to cell death and other genetic factors or signals may
modify or override its function (e.g., cytokine inhibition of
p53-mediated cell death; see below).
The finding that IL-6 efficiently blocked apoptosis of M1-tsp53 cells
at the permissive temperature without down-regulating ei24
expression is not surprising (Fig. 1). Cytokines override p53-mediated
cell death by inhibiting a downstream step of the pathway and not by
directly blocking the induction of target genes (4, 34).
Cytokine-signaling pathways clearly activate the expression of
Bcl-XL and Bcl-2 and it is presumably through these potent
survival factors that cytokines block p53-induced apoptosis (31,
34). Consistent with these observations, Bcl-XL was
also found to block ei24-mediated apoptosis of Rat1 cells
(Fig. 9).
The mechanism by which ei24 activates apoptosis is not yet
understood. The data supporting a role of ei24 in negatively
controlling cell growth and mediating cell death are fourfold. (i)
ei24 is induced in cells undergoing p53-mediated apoptosis.
(ii) Microinjection of an ei24 expression vector into murine
NIH 3T3 fibroblasts (Fig. 8) or human HeLa cervical carcinoma cells
(data not shown) induces morphological features of apoptosis. (iii)
ei24 efficiently blocks cell growth in colony reduction
assays. (iv) Bcl-XL overrides the reduction of
-Gal-marked cells when transiently transfected with ei24.
It is important to note that ei24 is overexpressed in these
assays, and therefore, the significance of ei24 in apoptosis must be addressed in a more physiological setting. To do so, we are
generating an ei24-deficient mouse model to examine the
contribution of endogenous ei24 to p53-mediated apoptosis
and tumor suppressor pathways in more detail.
Previously identified downstream target genes of p53 that may play a
role in apoptosis include bax,
killer/DR5, IGF-BP3,
PAG608, and fas/APO1 (3, 20, 29,
30, 38). However, mice deficient in bax or
fas are completely competent for p53-mediated thymic cell
death in response to irradiation, suggesting that other targets or
multiple targets are required for apoptosis (7, 23, 28, 35).
In light of the data presented here, we propose that ei24 may be a component of this apoptotic cascade in response to p53 and so
contributes to tumor suppression.
| |
ACKNOWLEDGMENTS |
We especially thank JinLing Wang and John R. Jeffers for their
technical assistance and John L. Cleveland for critically reviewing the
manuscript. We also acknowledge the contributions of Sam Lucas and
Richard Ashmun to cell cycle analyses, of Linda Valentine and Thomas
Look to the cytogenetic analyses, and of Richard Bram to the
microinjection studies. We thank Richard Kriwacki for his advice on the
predicted structure of ei24/PIG8.
This work was supported in part by NIH/NCI grant CA63230 (to G.P.Z.),
NIH/NCI Cancer Center Support Grant 5 P30 CA21765, and the American
Lebanese Syrian Associated Charities of St. Jude Children's Research
Hospital (ALSAC).
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Biochemistry, St. Jude Children's Research Hospital, 332 North
Lauderdale, Memphis, TN 38105. Phone: (901) 495-3429. Fax: (901)
525-8025. E-mail: gerard.zambetti{at}stjude.org.
| |
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Molecular and Cellular Biology, January 2000, p. 233-241, Vol. 20, No. 1
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Copyright © 2000, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
