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J. Biol. Chem., Vol. 277, Issue 16, 14060-14067, April 19, 2002
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From the Department of Pharmaceutical Sciences, School of Pharmacy
and Cancer Center, University of Colorado Health Sciences Center,
Denver, Colorado 80262
Received for publication, December 5, 2001, and in revised form, January 25, 2002
NAD(P)H:quinone oxidoreductase 1 (EC
1.6.99.2; DT-Diaphorase, NQO1) is predominantly a cytosolic flavoenzyme
that catalyzes a two-electron reduction. Using human tumor cell lines
devoid of NQO1 enzymatic activity, we have previously identified a
single nucleotide polymorphism (NQO1*2 allele) in the human NQO1 gene. This mutation has been characterized as a genetic polymorphism (NQO1*2), which leads to greatly diminished levels of protein due to
rapid degradation of the NQO1*2 protein by the ubiquitin proteasomal
pathway (UPP). In an attempt to decipher the mechanism responsible for
the differential stability of wild-type NQO1*1 and mutant NQO1*2
proteins, we have investigated the interactions of these proteins with
molecular chaperones of the Hsp family. Using co-immunoprecipitation
studies (co-IPs), no association was observed between Hsp90 and either
wild-type NQO1*1 or mutant NQO1*2 proteins. Hsp70, however, was found
to associate with NQO1*1 protein in cells when co-IPs were performed
with an anti-NQO1 antibody followed by immunoblotting with an
anti-Hsp70 antibody or vice versa. Hsp40 could also be
detected in the immunoprecipitated protein complex. Experiments were
also performed using either the NQO1*1 or NQO1*2 coding regions in an
in vitro transcription/translation system employing rabbit
reticulocyte lysates (RRLs). Consistent with the cellular data, co-IP
experiments in RRLs demonstrated an association of Hsp70 with wild-type
NQO1*1 protein but not with NQO1*2 protein. To further elucidate the
role of the association of Hsp70 with the NQO1*1 protein, site-directed
mutagenesis was used to modify a proposed Hsp70 binding site near the N
terminus of the NQO1 protein. We generated a plasmid containing an
NQO1*1 coding region with a mutated Hsp70 binding site (isoleucine to aspartic acid at position 8, NQO1*1/I8D). In contrast to the
NQO1*1 protein translated in RRLs, the NQO1*1/I8D protein did not
associate with Hsp70, as demonstrated by co-IP, was catalytically
inactive, and was degraded by the UPP. These data suggest that the
association of Hsp70 with NQO1*1 may play an important role in the
stability and functionality of the NQO1 protein.
NAD(P)H:quinone oxidoreductase 1 (EC 1.6.99.2; DT-Diaphorase,
NQO1)1 is a cytosolic
flavoenzyme that catalyzes the two-electron reduction of quinones and a
wide variety of substrates. NQO1 has relevance for both chemoprotection
and chemotherapy, since it can deactivate potentially toxic quinones
found in the environment but can also bioactivate anti-tumor quinones
such as mitomycin C (1-3). NQO1 gene expression has also shown to be
induced in response to xenobiotics, antioxidants, oxidants, heavy
metals, UV light, and ionizing radiation, and recently NQO1 has been
reported to stabilize p53 (4-6). In addition to the expression of NQO1
in normal tissues, a high level of NQO1 activity has been documented in
a wide ranging spectrum of human tumors and cell lines (7-10).
Using human tumor cell lines devoid of NQO1 activity our laboratory has
previously characterized a point mutation in exon six of the human NQO1
gene (11). The mutation is a C to T base pair substitution at position
609 of the NQO1 cDNA that codes for a proline to serine change at
position 187 of the amino acid sequence of the NQO1 protein. This
mutation in humans has been characterized as a genetic polymorphism
(NQO1*2), and the frequency of the NQO1*2/*2 (homozygous mutant)
genotype ranges from 4% in Caucasians to greater than 20% in Asian
populations (12). Low levels of NQO1 activity associated with the
NQO1*2 polymorphism has been shown to be associated with an increased
risk of benzene-induced hematotoxicity (13), an increased risk of acute
leukemia in adults (14) and children (15), and an increased risk of
secondary leukemia after treatment with chemotherapeutic agents
(16).
Genotype-phenotype studies of the NQO1*2 allele have been performed,
and no measurable NQO1 activity or protein could be detected in cell
lines or saliva samples from individuals with the NQO1*2/*2 genotype.
In agreement, no NQO1*2 mutant protein could be detected in NQO1*2/*2
tissue samples using immunohistochemistry (17). A small amount of
NQO1*2 protein could be detected in NQO1*2/*2 cell lines by immunoblot
analysis with enhanced chemiluminesence detection and prolonged
exposure times (17). These cell lines, however, had no measurable NQO1
activity, since the mutant NQO1*2 protein has very low catalytic
activity as compared with the wild-type NQO1*1 protein (11).
We have recently demonstrated that the lack of NQO1*2 protein in
tissues and cells from individuals carrying the homozygous NQO1*2/*2
polymorphism is due to rapid degradation of the mutant protein by the
ubiquitin proteasomal pathway (UPP) (18). Degradation of the mutant
NQO1*2 protein by the UPP could be observed in both cells and cell-free
systems, while the wild-type NQO1*1 protein demonstrated prolonged
stability in both systems. The mechanisms underlying the differential
stability of NQO1*1 and NQO1*2 proteins, however, remain to be
characterized. Heat shock proteins (Hsp) and particularly the Hsp70
protein chaperone family play a key role in catalyzing protein folding.
Hsp70, in association with Hsp40, binds hydrophobic regions of unfolded
proteins, and through cycles of ATP-dependent binding and
release by the Hsp70/40 complex, the nascent protein is manipulated
into an active conformation (19). The present investigation was
initiated to examine the potential association of Hsp protein
chaperones in the modulation of activity and stability of wild-type
NQO1*1 and mutant NQO1*2 proteins.
Chemicals and Reagents--
TNT-RRLs (SP6, Quick Coupled
Transcription/Translation System) and untreated RRLs were
purchased from Promega (Madison, WI). Apyrase (EC 3.6.1.5), E-64, PMSF,
cycloheximide, bovine serum albumin, and
2,6-dicholorphenol-indophenol were purchased from Sigma. Protein
A/G-agarose and clasto-lactacystin- Antibodies--
Anti-ubiquitin (rabbit polyclonal) was purchased
from Sigma. Hsp-40 (SC-1800, goat polyclonal) was obtained from Santa
Cruz Biotechnology (Santa Cruz, CA). Hsp70 (SPA-810, mouse monoclonal) was a product of Stressgen Biotechnologies Corp. (Victoria, British Columbia, Canada), and Hsp90 (Ab-1, rabbit polyclonal) was obtained from Neo Markers (Union City, CA). Horseradish peroxidase-conjugated secondary antibodies were purchased from Jackson ImmunoResearch Laboratories, Inc. (West Grove, PA). Hybridoma tissue culture supernatant (RPMI 1640 with 10% (v/v) fetal bovine serum) containing anti-NQO1 mouse monoclonal antibody clones A180 and B771 (IgG) mixed
1:1 were used in the study. Both A180 and B771 anti-NQO1 monoclonal
antibodies have demonstrated immunoreactivity toward NQO1*1 and NQO1*2
proteins (11).
Cell Lines--
HT-29 (human colon carcinoma) and MDA-MB 231 (human breast carcinoma) cell lines were obtained from the American
Type Culture Collection (Manassas, VA). Cells were grown as monolayers
at 37 °C in 5% CO2 with minimal essential medium
supplemented with 10% (v/v) fetal bovine serum, 10 units/ml
penicillin/streptomycin and 2 mM
L-glutamine.
Plasmids--
Human wild-type and mutant NQO1 coding regions
were subcloned into the pSP64poly(A) expression vector (Promega) by
polymerase chain reaction (PCR) amplification of the full coding region
using oligomers 5'-cccaagcttATGGTCGGCAGAAGAGCA-3' and
5'-tgctctagaTCATTTTCTAGCTTTGATCTG-3' containing HindIII and
XbaI restriction sites, respectively.
Site-directed Mutagenesis--
Plasmid pwtSP64poly(A) containing
the wild-type NQO1*1 coding region of human NQO1 served as a template.
The 822-bp fragment was amplified by PCR. The sequence of
oligonucleotides that served as primers to introduce the isoleucine
The altered bases are underlined and encode the mutated amino acid. The
temperature cycles used for this PCR amplification were as follows:
95 °C for 5 min, 25 cycles of 95 °C for 1 min, 50 °C for 1 min, followed by 72 °C for 1 min. After the final cycle the reaction
was kept at 4 °C. The resulting mutated product was then cut with
HindIII and XbaI followed by subcloning into pSP64poly(A). The construct was verified by digestion and sequencing. This construct is referred henceforth as NQO1*1/I8D.
In Vitro Transcription/Translation--
NQO1 in vitro
transcription/translation was carried out using SP6 Quick Coupled
Transcription/Translation System (TNT-RRL; Promega) according to
the manufacturer's instructions using 1 µg of plasmid DNA. Reactions
(50 µl) were carried out for 1 h at 32 °C, after which a
small aliquot of reaction mixture was removed, and NQO1 protein
translation was monitored by SDS-PAGE (21) followed by immunoblot
analysis (see below). Prior to immunoprecipitation, apyrase (EC
3.6.1.5, 5 units) was added and the TNT-RRLs placed on ice for 10 min.
The reaction was terminated by the addition of 200 µl of RIPA buffer,
and immunoprecipitation was carried out using the appropriate
antibodies. Proteasome-mediated degradation of NQO1*1/I8D was assayed
as described previously in untreated RRL (18). NQO1*1/I8D was generated
by in vitro transcription/translation (as described above),
and 5 µl of reaction mixture was added to untreated RRLs to measure
degradation (18).
SDS-PAGE, Immunoprecipitation, and Immunoblot
Analysis--
Exponentially growing cells were seeded at ~2 × 106 in 60-mm plates, and 12 h later the cells were
harvested. For immunoprecipitation studies, medium was removed, and
cells were washed with phosphate-buffered saline (PBS, pH 7.4), lysed
on ice in RIPA buffer (250 µl), then centrifuged at 13 K for 10 min.
To this supernatant 200 µl of anti-NQO1 monoclonal antibody or 10 µg of anti-HSP antibody were added, and the mixture was gently
rotated at 4 °C for 16 h. Protein A/G-agarose (40 µl) was
then added, and the incubations were continued for an additional 90 min. The protein A/G-agarose was collected by centrifugation and the
beads washed three times with 50 mM Tris-HCl, pH 8.0, containing 150 mM NaCl, 1% (v/v) Nonidet P-40. The protein
A/G-agarose beads were then suspended in 2× Laemmli SDS sample buffer
and heated to 90 °C for 5 min. Immunoprecipitated proteins were
analyzed by SDS-PAGE (12%, minigel) followed by transfer to a
polyvinylidene difluoride membrane (0.4 µm) in 25 mM
Tris, 192 mM glycine, and 20% (v/v) methanol at 110 V for
1 h. Membranes were blocked overnight in 10 mM
Tris-HCl, pH 8.0, 125 mM NaCl, 0.2% (v/v) Tween 20 containing 5% (w/v) nonfat dry milk (TBST-M5). Immunoblot analysis of
polyubiquitinated NQO1 was performed using anti-ubiquitin antibodies
diluted at 1:100. Immunoblot analysis of Hsp proteins (Hsp40, Hsp70,
and Hsp90) was performed using the following antibody dilutions; Hsp40
and Hsp90, 1:250; Hsp70, 1:1,500. Antibodies were diluted in 10 ml of
TBST-M5 and incubated with membranes for 1 h at 27 °C.
Horseradish peroxidase-labeled secondary antibodies were diluted at
1:5,000 in 20 ml of TBST-M5 and incubated for 30 min. For
determinations of cellular levels of NQO1 and Hsp proteins, cells were
scrapped, washed with PBS, collected in 200 µl of ice-cold RIPA
buffer, and then lysed by sonication on ice. The supernatant was
cleared by centrifugation at 13 K for 5 min, and the protein
concentration was determined by the method of Lowry (22). Protein bands
were visualized using enhanced chemiluminescence as described by the manufacturer (PerkinElmer Life Sciences). Densitometric analysis of the membranes was performed using GelDoc 2000 (Bio-Rad).
Cell Lines and Inhibitor Studies--
Cells were grown to 85%
confluence in 60-mm dishes in complete minimal essential medium. Fresh
medium (5 ml) containing various inhibitors MG132,
clasto-lactacystin- NQO1 Protein Turnover Studies--
NQO1 protein stability was
determined in the presence and absence of proteasomal inhibitor MG132.
Approximately 2 × 107 cells were plated into 100-mm
plates, and 12 h later fresh medium was added containing
cycloheximide (50 µg/ml). At the indicated intervals, cells were
scraped and pelleted by centrifugation. The cell pellet was washed with
ice-cold PBS, pH 7.4, and then lysed in 500 µl of ice-cold RIPA
buffer. Supernatant was collected by centrifugation at 13 K for 10 min. To this supernatant, 200 µl of anti-NQO1 monoclonal antibody was
added, and the incubation was carried out for 1 h on a shaker at
4 °C, followed by the addition of 30 µl of protein A/G-conjugated
agarose for an additional hour. Agarose beads were washed and processed
for immunoblot analysis as described above. To assess NQO1 turnover in
the presence of proteasomal inhibitor MG132, cells were treated with
MG132 (10 µM) and cycloheximide (50 µg/ml)
simultaneously. Proteasomal inhibitor and cycloheximide were present
during the entire duration of the experiment.
Determination of NQO1 Activity--
Aliquots (5 µl) of TNT-RRL
reactions were diluted with 10 µl of ice-cold 25 mM
Tris-HCl, pH 7.4, containing 250 mM sucrose and 5 µM FAD. NQO1 activity was measured spectrophotometrically using 2,6-dichlorophenol-indophenol as the terminal electron acceptor as described previously (23).
NQO1*2 Protein Is Degraded via the UPP--
The effect of UPP
inhibitors MG132 and clasto-lactacystin- NQO1*2 Protein Is Short-lived in Cells--
The half-life of
mutant NQO1 was investigated in MDA-MB 231 cells. Cells were pretreated
with cycloheximide to inhibit de novo protein synthesis
followed by treatment with LC to inhibit the UPP, and cell lysates were
monitored for the disappearance of the NQO1*2 protein. Because of the
low levels of NQO1*2 protein in MDA-MB 231 cells, we utilized NQO1
immunoprecipitation followed by NQO1 immunoblot analysis to increase
the sensitivity of this assay. The half-life of the NQO1*2 protein was
determined to be ~1.5 h in MDA-MB 231 cells (Fig.
2A). This observation is in
agreement with the short half-life of NQO1*2 protein in BE colon
carcinoma cells, which are also homozygous for the NQO1*2 allele (18). In contrast to the rapid degradation of the NQO1*2 protein, the wild-type NQO1*1 protein exhibits considerable stability and has a
half-life of greater than 18 h in HT-29 cells (18).
NQO1*2 Protein Half-life Increases in Response to UPP
Inhibitors--
Since the NQO1*2 protein is efficiently degraded by
the UPP, inhibitors of the UPP such as MG132 would be predicted to
increase the half-life of mutant NQO1. MDA-MB 231 cells were treated
with both cycloheximide and MG132, and the rate of NQO1 degradation was
followed by immunoprecipitation and immunoblot analysis (Fig. 2B). Treatment with MG132 led to increased stability of the
NQO1*2 protein in MDA-MB 231 cells, and there was an approximately
4-fold increase in the half-life of the NQO1*2 protein as determined by
the densitometric analysis of the blots (Fig. 2, A and
B).
Wild-type NQO1*1, but Not Mutant NQO1*2, Protein Associates with
the Molecular Chaperone Hsp70 in Cells--
To examine the potential
role of the molecular chaperone Hsp70 in the differential stability of
NQO1*1 and NQO1*2 proteins, we investigated whether an interaction
between the different forms of NQO1 and Hsp70 could be observed. For
this purpose, cell sonicates from HT-29 (NQO1*1/*1) and MDA-MB 231 (NQO1*2/*2) cells were analyzed by immunoprecipitation followed by
immunoblot analysis. Immunoprecipitation was carried out using
anti-NQO1 monoclonal antibodies, and the blots were probed with
anti-Hsp70 monoclonal antibodies. In HT-29 cells an
Hsp70·NQO1*1 protein complex could be co-immunoprecipitated using anti-NQO1 antibodies (Fig.
3A). No Hsp70·NQO1 complex
was observed in MDA-MB 231 cells. To further confirm these
observations, we used anti-Hsp70 antibodies to first carry out the
immunoprecipitation, and the membrane was then probed with anti-NQO1
antibodies (Fig. 3B). Using this reverse
immunoprecipitation, an association of Hsp70 could be observed with the
NQO1*1 protein but not with the mutant NQO1*2 protein. Furthermore,
increasing the cellular levels of mutant NQO1*2 protein in MDA-MB 231 cells following treatment with UPP inhibitors did not result in
immunoprecipitation of an Hsp70·NQO1 complex (Fig.
4A). Treatment of HT-29 cells
with UPP inhibitors had no effect on the levels of NQO1·Hsp70 complex
(Fig. 4A). These experiments confirm that the molecular
chaperone Hsp70 associates with the NQO1*1 protein in HT-29 cells but
not with mutant NQO1*2 protein in MDA-MB 231 cells. Both HT-29 and
MDA-MB 231 cells used in this study have approximately equivalent
levels of Hsp70 (Fig. 4B). Since molecular chaperones such
as Hsp70 can function as catalysts and are released from interactions
with target proteins after the facilitation of correct folding, we investigated the time course of association of NQO1*1 and Hsp70. De novo protein synthesis was blocked by cycloheximide
treatment in HT-29 cells, and samples were analyzed for the
Hsp70·NQO1*1 complex. Samples were collected at the indicated times,
and immunoprecipitation was carried out using anti-NQO1 antibodies
followed by immunoblot analysis with anti-Hsp70 antibodies. Maximal
interaction of Hsp70 and NQO1*1 was observed at 1 h; however, at
later time points of 4 and 6 h the interaction between Hsp70 and
NQO1 was markedly decreased (Fig.
5A). This suggested that the
chaperone may interact with unfolded or a partially folded immature
form of NQO1*1. Treatment of HT-29 cells with cycloheximide did not
have a major effect on cellular levels of either Hsp70 or NQO1 for the
duration of the experiment (Fig. 5, B and C).
When the membranes were stripped and probed for Hsp40, we were able to
detect the presence of Hsp40 in the immunoprecipitated complexes of
NQO1*1 and Hsp70, suggesting the formation of a ternary complex of
Hsp40, Hsp70, and NQO1 (data not shown, see below).
The Association of Hsp70 with RRL Generated NQO1 Proteins--
The
level of the NQO1*2 protein in cells homozygous for the NQO1*2 allele
such as MDA-MB 231 cells is low relative to cell homozygous for the
wild-type NQO1*1 allele. The inability to observe an association of the
NQO1*2 protein with Hsp70 may, therefore, be explained by the low
cellular levels of NQO1*2 protein in MDA-MB 231 cells. This explanation
seemed unlikely, however, since an interaction between Hsp70 and the
NQO1*2 protein could not be detected even in the presence of UPP
inhibitors, which increased the cellular levels of the NQO1*2 protein
(Fig. 4A). To circumvent this potential problem we generated
recombinant NQO1*1 and NQO1*2 proteins using a coupled
transcription/translation approach in a cell-free rabbit reticulocyte
lysate (TNT-RRL) system. Association of Hsp70 with the wild-type NQO1*1
protein could be observed by immunoprecipitation using anti-NQO1
antibodies followed by immunoblotting with anti-Hsp70 antibodies (Fig.
6A, lane 4). In
contrast, very little association of Hsp70 was detected with mutant
NQO1*2 protein (Fig. 6A, lane 3). Immediately
prior to immunoprecipitation, a small aliquot of the RRL reaction was
removed for NQO1 immunoblot analysis, which demonstrated that plasmids
containing coding regions for NQO1*1 and NQO1*2 proteins were
transcribed and translated with approximately equal efficiency in the
RRL system (Fig. 6B). Importantly, no association of Hsp70
with NQO1 could be detected when mature purified recombinant NQO1*1
protein was substituted for newly synthesized NQO1, suggesting
association of Hsp70 with an early nascent form of NQO1 (Fig.
6A, lane 2).
Site-directed Mutagenesis of a Hsp70 Binding Site on NQO1--
To
further investigate the interaction of Hsp70 with NQO1, we examined the
NQO1 amino acid sequence for potential Hsp70 binding sites. Previous
work has identified a potential Hsp70 binding motif described by a
central hydrophobic core region enriched in leucine and isoleucine and
flanked by basic amino acids. In this model, acidic amino acids are
excluded from the hydrophobic core and disfavored in flanking regions
(24, 25). Analysis of the NQO1*1 amino acid sequence revealed a
potential Hsp70 binding site located near the N terminus of the NQO1
protein (Fig. 7A). Using
site-directed mutagenesis we introduced an amino acid substitution (aspartic acid for isoleucine) at position 8 in the NQO1 protein. The
plasmid encoding mutant NQO1*1/I8D was efficiently transcribed and
translated in RRLs with almost equal efficiency to that of wild-type
NQO1*1 (Fig. 7B). The mutant NQO1 protein, however, failed
to interact with Hsp70 in vitro as demonstrated by
co-immunoprecipitation studies (Fig. 7C).
Catalytic Activity of RRL-generated NQO1 Proteins--
The
catalytic activity of in vitro transcribed/translated
NQO1*1, NQO1*2, and NQO1*1/I8D proteins was measured
spectrophotometrically by following the reduction of
2,6-dicholorphenol-indophenol at 600 nm. Aliquots (5 µl) of RRL
reactions were removed at regular intervals over 60 min and assayed for
NQO1 catalytic activity. NQO1 protein expression was confirmed by
immunoblot analysis as described previously (data not shown).
Transcription/translation of the wild-type NQO1*1 coding region
resulted in a time-dependent increase in NQO1 activity
(Fig. 7D). Although RRL-mediated transcription/translation of either the NQO1*2 or NQO1*1/I8D coding regions produced full-length NQO1 products, both proteins failed to demonstrate catalytic activity, suggesting the functional role of Hsp70 interaction with NQO1*1 protein. The NQO1*1/I8D protein also underwent RRL-mediated
degradation, and protein degradation was inhibited by the addition of
MG132, suggesting that NQO1*1/I8D was degraded by the UPP (Fig.
7E).
Hsp40 and Hsp90 Interactions with NQO1*1 and NQO1*2
Proteins--
Since Hsp40 and Hsp90 are known to be co-chaperones of
Hsp70 in the Hsp family, we also investigated the interactions of these chaperones with the NQO1*1 and NQO1*2 proteins. Co-immunoprecipitation studies were performed in HT-29 and MDA-MB 231 cells. Sonicated samples
were immunoprecipitated using anti-Hsp40 antibodies followed by
immunoblot analysis with anti-NQO1 antibodies. These co-IP experiments
demonstrated an association between wild-type NQO1*1 protein and Hsp40,
but no association was observed between Hsp40 and mutant NQO1*2 protein
(Fig. 8A). These results are
similar to data obtained for the interaction between Hsp70 and
wild-type NQO1*1 protein, suggesting that Hsp40 may complex together
with Hsp70 in their association with NQO1*1. The ternary complex of NQO1, Hsp40, and Hsp70 was confirmed by stripping the membrane shown in
Fig. 8A and re-probing with anti-Hsp70 antibodies. The presence of Hsp70 in the immunoprecipitated complex could be observed in HT-29 cells but not MDA-MB 231 cells (Fig. 8B). The
absence of an association of Hsp40 with NQO1 in MDA-MB 231 cells could not be explained by the cellular levels of Hsp40, since greater levels
of Hsp40 could be detected in MDA-MB 231 cells than in HT-29 cells
(Fig. 8C). Using similar co-IP studies, however, we failed
to detect an association of NQO1*1 or NQO1*2 proteins with Hsp90 in
HT-29 and MDA-MB 231 cell lines or RRLs (data not shown).
It is well known that misfolded proteins are substrates for the
UPP. Inhibition of the 26 S proteasome results in an increase in the
amount of NQO1*2 protein and a build up of higher molecular weight NQO1
immunoreactive species consistent with the formation of
polyubiquitinated NQO1 proteins. Treatment of MDA-MB 231 cells with
inbibitors of the 26 S proteasome also results in an increase in the
half-life of the NQO1*2 protein, clearly demonstrating the role of the
UPP in degradation of the mutant NQO1*2 protein. The shortened
half-life of the mutant NQO1*2 protein (1.5 h) is in contrast to the
stability of wild-type NQO1*1 protein, which has a half-life of greater
than 18 h (18).
In an attempt to understand possible mechanisms underlying the
differential stability of NQO1*1 and NQO1*2 proteins, we have investigated a potential role for the involvement of molecular chaperones of the heat shock protein family (Hsp). Molecular chaperones have been implicated in a wide variety of cellular processes including protein folding, protein transport, and protein degradation
(26-29).
In co-immunoprecipitation studies using cellular systems, we found that
Hsp70 associated with the wild-type NQO1*1 protein but not with the
mutant NQO1*2 protein. To confirm these observations in a cell-free
system, we performed similar experiments employing RRLs in an in
vitro coupled transcription/translation system. Our results
demonstrated that although approximately equivalent amounts of NQO1*1
and NQO1*2 proteins were generated in RRLs, interaction of Hsp70 could
only be observed with wild-type NQO1*1 but not with mutant NQO1*2
protein. Hsp70-catalyzed protein folding requires ATP hydrolysis and
often involves the presence of co-chaperones such as Hsp40 and Hsp90
(19, 30). In the co-immunoprecipitated complex of NQO1 and Hsp70, Hsp40
could also be detected, suggesting the presence of a ternary complex.
No interaction, however, could be observed between NQO1*1 or NQO1*2
proteins and Hsp90, demonstrating that there is some degree of
specificity to the interactions of NQO1 and the proteins of the Hsp family.
In protein folding interactions, molecular chaperones such as Hsp70 are
believed to bind with the target substrate, facilitate correct folding,
and then dissociate from the complex (19, 28). In HT-29 cells, time
course studies demonstrated that the Hsp70·NQO1 complex was greatly
reduced after 4 h following the inhibition of protein synthesis.
In addition, RRL experiments using in vitro transcription/translation demonstrated that Hsp70 did associate with
newly synthesized NQO1*1 protein; however, Hsp70 failed to interact
with mature recombinant NQO1*1. The association of Hsp70 and NQO1*1 in
cells and in cell-free systems, therefore, most probably reflects the
association of Hsp70 with a precursor form of the mature NQO1 protein
that has not been fully and completely folded (Fig.
9). These results are consistent with the
proposed role of Hsp70 in protein folding (30) and are the first
demonstration that chaperones interact with NQO1.
Additional evidence linking Hsp70 with NQO1 has come from
site-directed mutagenesis studies of a proposed Hsp70 binding motif located near the N terminus of the NQO1 protein. Studies with Dna K,
the E. coli homologue of human Hsp70, has identified binding motifs in the substrate proteins that associate with Dna K (25, 30).
The binding motifs consist of a hydrophobic core of four to five
residues enriched in leucine, isoleucine, and valine and two flanking
regions enriched in basic residues. Acidic residues are excluded from
the core and disfavored in the flanking regions. A search of the human,
mouse, and rat NQO1 amino acid sequences revealed the presence of an
identical Dna K binding site
(R4R5A6L7I8V9L10A11H12) located near the N terminus of the protein. Site-directed mutagenesis was used in combination with in vitro
transcription/translation to generate a human NQO1*1 protein where
isoleucine was replaced with aspartic acid at position 8 of the amino
acid sequence (NQO1*1/I8D). As predicted from the proposed model, the
insertion of an acidic residue into the hydrophobic core resulted in
the loss of binding of NQO1*1/I8D to Hsp70. The resultant in
vitro translated NQO1*1/I8D protein had no measurable catalytic
activity and was degraded by the UPP system demonstrating the
functional role of the interaction of Hsp70 with NQO1. In addition, an
examination of the x-ray crystal structure of recombinant human NQO1
has revealed that the Dna K binding site is not directly exposed to the
surface in the mature protein (31). This is confirmed by the absence of
an association between mature NQO1*1 and Hsp70. These data further
implicate a role for Hsp70 in the folding of immature NQO1 into an
active protein. It is also possible that introduction of an acidic
amino acid residue into the N terminus of the NQO1 amino acid sequence might have interfered with the catalytic function of the enzyme. This
seems unlikely, however, since the addition of positively charged
residues to the N terminus of NQO1 in the form of a 6×-His-tag did not
result in significant loss of enzymatic activity as compared with the
NQO1*1 protein (32).2 The
His-tagged NQO1*1 protein had ~70% of the catalytic activity of the
wild-type NQO1*1 protein and was not degraded by the UPP, while in
contrast the NQO1*1/I8D protein was a target of UPP-mediated degradation.
The absence of an association between Hsp70/40 and mutant NQO1*2
protein suggests that the proline to serine amino acid substitution in
the NQO1*2 protein prevents binding of Hsp70 to the mutant protein.
X-ray crystallographic studies have shown that this substitution is
located near the transition of a In summary, we have demonstrated an association of Hsp70 and Hsp40 with
wild-type NQO1 but not mutant NQO1*2 protein. Given the documented role
for Hsp70/40 in protein folding (30, 34), we hypothesize a role for
Hsp70/40 in the differential stability of NQO1*1 and NQO1*2 proteins
(Fig. 9). This proposed model will allow for the design of future
experiments to characterize the structural motifs that govern the
interaction of Hsp and NQO1 proteins.
*
This work was supported by Health and Human Services
Grant RO1CA51210.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.
Published, JBC Papers in Press, January 30, 2002, DOI 10.1074/jbc.M111576200
2
D. Siegel and J. K. Kepa, unpublished data.
The abbreviations used are:
NQO1, NAD(P)H:quinone oxidoreductase 1;
UPP, ubiquitin-proteasomal
pathway;
RRL, rabbit reticulocyte lysate;
MG132, Z-Leu-Leu-Leu-CHO;
LC, clasto-lactacystin-
Interaction of the Molecular Chaperone Hsp70 with
Human NAD(P)H:Quinone Oxidoreductase 1*
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-lactone were obtained
from Calbiochem. MG132 was purchased from Biomol Research Laboratories
(Plymouth Meeting, PA). RIPA (protease inhibitor mixture) was obtained
from Roche Diagnostics GmbH (Mannheim, Germany). Human recombinant NQO1
standard was purified from Escherichia coli by Cibacron blue
affinity chromatography as described previously (11, 20). All other
chemicals and reagents used in this study were of the highest purity
grade available commercially.
aspartic acid mutation (I8D) into the human NQO1 coding region at amino
acid position 8 are as follows: Primer 1, 5'-cccaagcttATGGTCGGCAGGAAAGAGCACTGACGTAGCTGGCTCAC-3'; Primer 2, 5'-tgctctagaTCATTTTCTAGCTTTGATCTG-3'.
-lactone (LC), E-64, and PMSF were
added to each plate, and the medium replaced with fresh inhibitor 3 h later. After 6 h of incubation with inhibitor,
cells were washed with PBS and then lysed in ice-cold RIPA buffer.
Protein concentrations were determined (22), and NQO1 levels were
analyzed by immunoblot analysis.
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-lactone or
non-proteasomal inhibitors PMSF (serine protease inhibitor) and E-64
(cysteine protease inhibitor) on NQO1 stability was examined in MDA-MB
231 human breast carcinoma cells, which have previously been genotyped
as homozygous for the NQO1*2 allele (17). NQO1 degradation was
inhibited by the addition of MG132 or LC (Fig. 1A). In contrast, PMSF or E-64
had no effect on the degradation of NQO1. Several higher molecular
weight, anti-NQO1 immunoreactive proteins could be observed after
pretreatment with UPP inhibitors but not after pretreatment with PMSF
or E-64 (Fig. 1B). The presence of higher molecular weight
products after pretreatment with UPP inhibitors was consistent with the
accumulation of polyubiquitinated forms of NQO1. Confirmation of the
build up of high molecular weight polyubiquitinated proteins in samples
treated with proteasomal inhibitors was demonstrated using an
anti-ubiquitin antibody (Fig. 1C). The abundance of
polyubiquitinated species was greatly enhanced when UPP was blocked by
MG132 or LC (Fig. 1C, lanes 2-5). No
accumulation of polyubiquitinated proteins could be detected following
treatment with PMSF or E-64 (Fig. 1C, lanes 6 and
7). In agreement with UPP-mediated degradation of NQO1*2,
immunoprecipitation analysis using an anti-NQO1 monoclonal antibody
followed by anti-ubiquitin immunoblot analysis confirmed the presence
of polyubiquitinated NQO1*2 proteins in sonicates from MDA-MB 231 cells
treated with proteasome inhibitors (Fig. 1D).
View larger version (45K):
[in a new window]
Fig. 1.
Inhibition of mutant NQO1*2 protein
degradation in MDA-MB 231 breast cancer cells. MDA-MB 231 cells
were treated with proteasome inhibitors (MG132,
LC) or non-proteasomal inhibitors (PMSF,
E-64) at the indicated concentrations for 6 h.
A, crude sonicate (50 µg) was subjected to SDS-PAGE and
immunoblot analysis. Membranes were probed with anti-NQO1 antibodies.
Treatment of MDA-MB 231 cells with proteasome inhibitors generates
higher molecular weight NQO1 immunoreactive products. B,
experimental conditions were identical as described in A,
except 100 µg of crude sonicate was analyzed by SDS-PAGE and
immunoblot analysis, and film was exposed or 1 h. Treatment of
MDA-MB 231 cells with proteasome inhibitors generates higher molecular
weight ubiquitin immunoreactive products. C, experimental
conditions were identical as described in A, except
membranes were probed with anti-ubiquitin antibodies. D,
MDA-MB 231 cells were treated with either MG132 or LC (10 µM) for 6 h. Samples were then immunoprecipitated
with anti-NQO1 antibodies followed by SDS-PAGE and immunoblot analysis
with anti-ubiquitin antibodies.
View larger version (65K):
[in a new window]
Fig. 2.
The effect of proteasome inhibitor MG132 on
the stability of mutant NQO1*2 protein in MDA-MB 231 cells. At the
indicated time following cycloheximide treatment, cells were processed
for immunoprecipitation, SDS-PAGE, and immunoblot analysis. Membranes
were probed with anti-NQO1 antibodies. A, in the absence of
proteasome inhibitor MG132. B, in the presence of MG132 (10 µM). IgG (H), immunoglobin heavy chain;
IgG (L), immunoglobin light chain.
View larger version (71K):
[in a new window]
Fig. 3.
The association of NQO1 with Hsp70 in
cells. Co-immunoprecipitation was carried out to examine sonicates
from HT-29 and MDA-MB 231 cells for an association of NQO1 with Hsp70.
A, sonicated samples were immunoprecipitated with anti-NQO1
antibodies followed by SDS-PAGE and immunoblot analysis with anti-Hsp70
antibodies. HT-29 sonicate (50 µg) was used as a molecular weight
standard for Hsp70. B, samples were immunoprecipitated with
anti-Hsp70 antibodies followed by SDS-PAGE and immunoblot analysis with
anti-NQO1 antibodies. NQO1 Std, purified human recombinant
NQO1 (5 ng).
View larger version (52K):
[in a new window]
Fig. 4.
Effect of proteasome inhibitors on the
association of NQO1 with Hsp70 in cells. Co-immunoprecipitation
was carried out to examine sonicates prepared from HT-29 and MDA-MB 231 cells pretreated with proteasome inhibitors (MG132,
LC, 10 µM) for an association of NQO1 with
Hsp70. A, samples were immunoprecipitated with anti-NQO1
antibodies followed by SDS-PAGE and immunoblot analysis with anti-Hsp70
antibodies. B, cellular levels of Hsp70 in HT-29 and MDA-MB
231 cells. Sonicates prepared from HT-29 and MDA-MB 231 cells (50 µg)
were examined by SDS-PAGE and immunoblot analysis with anti-Hsp70
antibodies.
View larger version (61K):
[in a new window]
Fig. 5.
The effect of de novo
protein synthesis inhibition on the association of NQO1 with
Hsp70. A, HT-29 cells were treated with cycloheximide,
and at the indicated times samples were immunoprecipitated with
anti-NQO1 antibodies followed by SDS-PAGE and immunoblot analysis with
anti-Hsp70 antibodies. HT-29 sonicate (50 µg) was used as a molecular
weight standard for Hsp70. B, prior to immunoprecipitation,
sonicate (50 µg) was removed and analyzed by SDS-PAGE and immunoblot
analysis with anti-Hsp70 antibodies. C, the membrane
utilized in B was stripped and reprobed with anti-NQO1
antibodies. NQO1 Std, purified human recombinant NQO1 (5 ng).
View larger version (39K):
[in a new window]
Fig. 6.
The association of Hsp70 with NQO1 generated
in an in vitro transcription/translation system
(RRL). A, following in vitro
transcription/translation of the wild-type (NQO1*1) and
mutant (NQO1*2) coding regions, samples were
immunoprecipitated with anti-NQO1 antibodies followed by SDS-PAGE and
immunoblot analysis with anti-Hsp70 antibodies. Lane 1, RRLs
only; lane 2, RRLs plus 1 µg of purified human recombinant
NQO1; lane 3, RRLs plus mutant NQO1*2 coding region;
lane 4, RRLs plus wild-type NQO1*1 coding region.
B, immunoblot analysis for NQO1 translation products just
prior to immunoprecipitation (A). NQO1 Std,
purified human recombinant NQO1 (5 ng).
View larger version (27K):
[in a new window]
Fig. 7.
Mutation of a Hsp70 binding motif in NQO1
results in the generation of a NQO1 protein with no catalytic
activity. A, diagram representing the Hsp
binding motif (underlined) located near the N terminus of
the human NQO1 protein. Hydrophobic core amino acids are in
red, and basic flanking amino acids are in green.
Introduction of an aspartic acid residue (blue) at position
8 is shown in the lower diagram (NQO1*1/I8D). B,
immunoblot analysis for NQO1 translation products just prior to
immunoprecipitation (C). C, following in
vitro transcription/translation of wild-type (NQO1*1)
and mutated (NQO1*1/I8D) coding regions, samples were
immunoprecipitated with anti-NQO1 antibodies followed by SDS-PAGE and
immunoblot analysis with anti-Hsp70 antibodies. RRL (50 µg) was
utilized as a molecular weight standard for Hsp70. D, NQO1
catalytic activity was measured at the indicated times in an in
vitro transcription/translation system (RRLs) supplemented with
the following NQO1 coding regions. Open circles, wild-type
NQO1*1; open triangles, mutant NQO1*2; closed
squares, mutated NQO1*1/I8D. E, immunoblot analysis of
RRL-mediated degradation of NQO1*1/I8D in the presence and absence of
25 µM MG132. The NQO1*1/I8D protein was generated in the
TNT-RRL system and then transferred into untreated RRLs as described
previously (18).
View larger version (44K):
[in a new window]
Fig. 8.
The association of NQO1 with Hsp40 in
cells. Co-immunoprecipitation was used to examine sonicates from
HT-29 and MDA-MB 231 cells for an association of NQO1 with Hsp40.
A, samples were immunoprecipitated with anti-Hsp40
antibodies followed by SDS-PAGE and immunoblot analysis with anti-NQO1
antibodies. HT-29 sonicate (50 µg) was utilized as a molecular weight
standard for NQO1 (lane 1). B, membrane in
A was stripped and reprobed with anti-Hsp70 antibodies.
HT-29 sonicate (50 µg) was utilized as a molecular weight standard
for Hsp70 (lane 1). C, levels of Hsp40 in HT-29
and MDA-MB 231 cells. Sonicates prepared from HT-29 and MDA-MB 231 cells (50 µg) were examined by SDS-PAGE and immunoblot analysis with
anti-Hsp40 antibodies.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
View larger version (11K):
[in a new window]
Fig. 9.
Proposed mechanism for the difference in
stability between wild-type NQO1*1 and mutant NQO1*2
proteins.
-sheet and an 
-helical bend. The
proline to serine substitution may disrupt the confirmation of the
NQO1*2 protein preventing recognition and association with Hsp70/40,
resulting in misfolding and subsequent UPP-meditated degradation.
Alternatively, it has been proposed that the proline to serine amino
acid change results in disruption of the central parallel -sheet,
resulting in a decreased affinity of the protein for the FAD cofactor
(33). It is conceivable that the inability of NQO1*2 protein to
efficiently bind FAD prevents the association of the mutant protein
with Hsp70/40. Studies are under way to determine whether an
association with Hsp70/40 facilitates incorporation of FAD into NQO1 proteins.
FOOTNOTES
To whom correspondence should be addressed: Dept. of
Pharmaceutical Sciences, Box C-238, School of Pharmacy, UCHSC, 4200 East 9th Ave., Denver, CO 80262. Tel.: 303-315-6077; Fax: 303-315-0274; E-mail: david.ross@uchsc.edu.
ABBREVIATIONS
-lactone;
E-64, trans-epoxysuccinyl-L-leucylamido-(4-guanidino)butane;
PMSF, phenylmethylsulfonyl fluoride;
RIPA, radioimmune precipitation;
PBS, phosphate-buffered saline.
REFERENCES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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