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J. Biol. Chem., Vol. 277, Issue 18, 15807-15812, May 3, 2002
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From the Department of Biochemistry and Biophysics, Oregon
State University, Corvallis, Oregon 97331-7305
Received for publication, January 29, 2002, and in revised form, February 13, 2002
In Escherichia coli the
mutT gene is one of several that acts to minimize
mutagenesis by reactive oxygen species. The bacterial MutT protein and
its mammalian homolog have been shown to catalyze in vitro
the hydrolysis of the oxidized deoxyguanosine nucleotide, 8-oxo-dGTP,
to its corresponding monophosphate. Thus, the protein is thought to
"sanitize" the nucleotide pool by ridding the cell of a nucleotide
whose incorporation into DNA would be intensely mutagenic. However,
because others have shown mutT mutations to be mutagenic
under some conditions of anaerobic growth, and have shown 8-oxo-dGTP to
be a poor DNA polymerase substrate, there is reason to question this
model. We have devised an assay for 8-oxo-dGTP in bacterial extracts.
Using this assay, which involves reversed-phase high-performance liquid
chromatography and electrochemical detection, we have been unable to
detect 8-oxo-dGTP in extracts of three different mutT
mutants of E. coli, even after growth of the bacteria in
the presence of hydrogen peroxide. Our estimated upper limit for
8-oxo-dGTP content of these bacteria is about 200 molecules/cell,
corresponding to a concentration of about 0.34 µM. When
8-oxo-dGTP was added at 0.34 µM to an in
vitro DNA replication system primed with a DNA template that
permits scoring of replication errors and with the four normal dNTPs at
their estimated intracellular concentrations, there was no detectable effect upon the frequency of replication errors. These findings lead us
to question the conclusion that 8-oxo-dGTP is the most significant
physiological substrate for the MutT protein.
The action of reactive oxygen species upon cells stimulates
mutagenesis in large part by increasing the abundance in DNA of the
oxidized guanine derivative, 7,8-dihydro-8-oxoguanine
(8-oxoG).1 This base
efficiently pairs with adenine, leading, if unrepaired, to a
transversion mutation (1). In Escherichia coli the products of three genes play particularly prominent roles in counteracting this
genotoxicity, and all three have homologs in mammalian cells. Two of
these genes, mutM and mutY, encode DNA
glycosylases, and their actions initiate base excision repair processes
at sites occupied by oxoG (1). The third gene, mutT, encodes
a nucleotidase, which cleaves dGTP to dGMP and pyrophosphate (2) but
which Maki and Sekiguchi (3) showed to have much lower
Km for the oxidized dGTP derivative, 8-oxo-dGTP.
This finding plus subsequent publications from the same laboratory
(4-9) support the concept that the action of the MutT protein is to
"sanitize" the nucleotide pool by removing from cells a damaged
nucleotide that, if incorporated into DNA, would be strongly
mutagenic. In agreement with this model, several investigators (10-12)
have shown that addition of 8-oxo-dGTP to an in vitro DNA
replication system in which replication errors could be scored as
mutations stimulated replication errors that were shown by sequence
analysis to be transversions.
The human homolog of MutT, hMTH1, has been expressed in mutT
mutant E. coli and shown to suppress the mutator phenotype
(5, 8). Thus, both bacterial and mammalian proteins are thought to play
the same role in sanitizing the nucleotide pool. The bacterial and
human enzymes differ somewhat in substrate specificity; hMTH1 acts upon
two oxidized dATP derivatives as well as upon 8-oxo-dGTP (13), and the
bacterial enzyme acts upon 8-oxo-GTP, the ribonucleotide analog of
8-oxo-dGTP (14).
Although most published data support the nucleotide pool cleansing role
for MutT in ridding the cell of 8-oxo-dGTP, two puzzling observations
have been made. First, Fowler et al. (15) showed that under
certain growth conditions for E. coli the mutT
mutator phenotype is expressed even when cells are grown anaerobically, and this is under conditions where no appreciable dGTP oxidation should be taking place. Second, Einolf et al. (16, 17)
showed 8-oxo-dGTP to be a poor substrate for several DNA polymerases when compared with dGTP. For four different polymerases (16), the
kcat/Km was
~105-fold higher for dGTP:C than for either 8-oxo-dGTP:A
or 8-oxo-dGTP:C, suggesting that 8-oxo-dGTP levels in cells would have
to be quite high in order for it to substitute for dGTP to a
significant extent and hence to play a significant role in mutagenesis.
Note that in studies with the in vitro DNA replication
systems (10-12), 8-oxo-dGTP was present at concentrations equal to or
greater than those of dGTP, conditions that are unlikely to hold in
living cells.
To better understand the role of 8-oxo-dGTP in mutagenesis and the
mechanism by which MutT minimizes the effects of oxidative DNA damage,
it seemed important for intracellular levels of 8-oxo-dGTP to be
measured directly under various conditions. For example, we would
expect to see higher levels of 8-oxo-dGTP in mutT mutator mutant bacteria than in wild-type cells and lower levels in
anaerobic than in aerobic growth conditions. Developing a protocol for
extracting and analyzing the 8-oxo-dGTP pool in E. coli and
carrying out such analyses were the goals of this investigation.
Mutant E. coli Strains and Culture Conditions--
E.
coli strains used included strain B, the wild-type control from
our collection, and three mutT mutants obtained from the E. coli Genetic Stock Center, New Haven, CT. These strains
are ES1580, 58-278M, and T-198. All bacteria were grown in LB medium, and 50-ml cultures were grown to mid-logarithmic phase for extraction and assays of dNTPs.
Extraction of Nucleotides--
Bacterial cultures (50 ml each)
were extracted for nucleotide analysis by a modification of the dual
extraction procedure using methanol and acid as described in an earlier
paper from this laboratory (18). Briefly, bacteria were collected by
rapid filtration and extracted with cold 60% methanol, 1% toluene at HPLC Nucleotide Analyses--
The HPLC method of DiPierro
et al. (20) was modified to develop an HPLC assay for
simultaneous measurement of 8-oxo-dGTP and the four standard dNTPs. The
chromatographic system consisted of a Beckman 126 analytical pump
system with a Beckman 166 UV detector. Standard dNTPs and other
nucleotides were detected and quantitated by UV absorbance at a
wavelength of 267 nm. Analysis of 8-oxo-dGTP used a Bioanalytical
Systems LC-4B amperometric detector with a CC4 flow cell, which was
connected in series with the UV detector. 8-Oxo-dGTP was detected using
a glassy carbon electrode set at a potential of +900 mV
versus the Ag/AgCl reference electrode. We obtained
8-oxo-dGTP from Amersham Biosciences, who reported its purity at
greater than 99% as determined by HPLC. Our HPLC analysis of the
product confirmed this estimate (data not shown).
Chromatographic separation of nucleotides was achieved by using an
Alltima C18 column (Alltech Inc., Nicholasville, KY) with a Phenomenex
C18 guard cartridge or Discovery C18 (Supelco, Sigma-Aldrich) column
with C18 guard column (Supelco). All analytical columns were 250 × 4.6 mm, with a 5-µm particle size. The mobile phase consisted of
Buffer A (10 mM tetrabutylammonium hydroxide, 10 mM KH2PO4, 0.25% methanol, pH 7.0)
and Buffer B (2.8 mM tetrabutylammonium hydroxide, 100 mM KH2PO4, 30% methanol, pH 5.5).
All mobile phase buffers were filtered and degassed. Separation was
achieved with the Alltima C18 column using a 40-min linear gradient of
50% buffer A, 50% buffer B to 30% buffer A, 70% buffer B followed
by a wash with 100% buffer B. It was necessary to re-equilibrate the
column in 50% buffer A, 50% buffer B for at least 30 min after each
run to achieve reproducible retention times for all nucleotides on subsequent runs. With the Discovery C18 column, separation of all
nucleotides could be achieved in a 25-min linear gradient of 50%
buffer A, 50% buffer B to 40% buffer A, 60% buffer B, with buffer B
containing 6% acetonitrile in addition to the substances listed above.
All separations were performed at a flow rate of 1.5 ml/min. Authentic
nucleotide standards were used to identify nucleotides in the elution
profile and develop calibration curves for all nucleotides. Injections
(50 µl each) of bacterial extract were performed in duplicate with
material in the second injection containing internal standards of dATP,
dCTP, dGTP, dTTP, and 8-oxo-dGTP. Data from these second runs were used
to verify identifications made from elution times, as well as to
calculate recoveries of each nucleotide and apply these figures to
correct nucleotide data from the extract for variable losses of
material during nucleotide extraction and separation.
8-Oxo-dGTPase Assay--
The assay for 8-oxo-dGTPase activity
was performed as described by Bialkowski and Kasprzak (21). To prepare
cell extracts for determination of enzyme activity, 50-ml bacterial
cultures were grown to mid-log phase and then centrifuged to pellet the cells. After washing the cell pellet in 20 mM Tris-buffered
saline, the cells were once again recovered by centrifugation and
resuspended in 500 µl of 20 mM Tris-HCl, pH 7.4. Cells
were lysed by sonication followed by centrifugation to pellet cell
debris. A sample of the resulting supernatant was used to determine
protein concentration, and the rest was transferred to chilled
polycarbonate Ultracentrifuge tubes (Beckman No. 343778) and
centrifuged for 1 h at 49,000 rpm, 4 °C, in a Beckman TL-100
Ultracentrifuge. Three fractions of the supernatant (100 µl each)
with protein concentrations of more than 4 mg/ml were filtered through
individual 30 K Nanosep filters until passage was complete. The
8-oxo-dGTPase activity of the resulting ultrafiltrates was determined
by incubating the ultrafiltrate (5 µl) in a reaction mix (total
volume = 60 µl) containing 40 µM 8-oxo-dGTP, 5 mM MgCl2, and 100 mM Tris-HCl, pH
8.5, at 37 °C for 4 h; this was followed by the addition of 20 µl of 50 mM Na2EDTA to terminate the
enzymatic activity. The reaction mixture was analyzed by HPLC using an
Alltima C18 column (5 µm, 250 × 4.6 mm, Alltech Inc.) at a flow
rate of 1.0 ml/min, with nucleotides detected by UV absorbance at 293 nm. Aliquots (50 µl) of the reaction mixture were chromatographed
isocratically with 100 mM NaH2PO4, methanol (95:5) at a flow rate of 1 ml/min. 8-oxo-dGTP (Amersham Biosciences) and 8-oxo-dGMP (prepared as described by Bialkowski and
Kasprzak (21)) were used for calibration. The enzymatic activity in
each extract is described as pmol of 8-oxo-dGMP formed/min/mg of protein.
Analysis of Replication Errors by in Vitro DNA Synthesis--
We
analyzed replication errors during DNA synthesis in vitro by
the method of Roberts and Kunkel (22), in which a cytosolic extract of
HeLa cells is programmed with a modified M13 phage replicative form DNA
containing an SV40 replication origin and part of the E. coli
lacZ gene capable of
Replication reaction mixtures were treated with DpnI
endonuclease to eliminate unreplicated DNA molecules (22), and DNA in
the mixtures was transferred by electroporation into E. coli NR9162 (mutS). This mixture was plated on E. coli
CSH50, an Electrochemical Detection of 8-Oxo-dGTP--
Because
electrochemical detection is routinely used to assay 8-oxo-dGMP levels
in DNA, and because it is more sensitive than UV absorbance-based
methods, we established an electrochemical detection and quantitation
protocol for 8-oxo-dGTP. Fig. 1 shows a
voltammogram for a solution of authentic 8-oxo-dGTP. A strong signal
with a midpoint potential of about +700 mV was seen. No such signal was
seen with dGTP. For detection of 8-oxo-dGTP, thereafter in HPLC
streams we applied +900 mV. Fig. 2 shows
separation of a mixture of standard nucleotides, detected by
ultraviolet absorbance, plus an 8-oxo-dGTP standard detected
electrochemically at + 900 mV when subjected to identical
chromatographic conditions. With this elution protocol, 8-oxo-dGTP,
with a retention time of ~37 min, was clearly separated from the
eight common ribo- and deoxyribonucleoside triphosphates. In separate
experiments (not shown) we found that none of the standard ribo- or
deoxyribonucleoside triphosphates showed a discernible peak when
analyzed by HPLC and electrochemical detection at +900 mV. We conclude,
therefore, that 8-oxo-dGTP can be detected and quantitated in the
presence of an excess of each of the standard nucleoside
triphosphates.
8-Oxo-dGTP in Bacterial Extracts--
Next we attempted to detect
and quantitate 8-oxo-dGTP in E. coli extracts. Fig.
3 shows the elution profile analyzed by
electrochemical detection for extracts of E. coli B and a
mutT mutant, T-198. No signal was seen in either extract at
37 min. The mutT mutant showed a peak at about 39 min, but
that peak did not represent 8-oxo-dGTP, as revealed by mixing 50 pmol
of authentic 8-oxo-dGTP with the extract prior to analysis and seeing a
peak corresponding to that added material at 37 min.
So far we have not identified the material in the T-198 extract that
elutes at 39 min, but we note that a similar peak was seen in the
analysis of extracts of two other mutT mutants (data not
shown). In preliminary attempts to identify this material, we treated
standard nucleotides with H2O2 and ascorbate
and analyzed these reaction mixtures by HPLC and electrochemical
detection. dCTP and GTP were the only nucleotides to yield
electrochemically active material under these conditions. The oxidized
dCTP eluted shortly after authentic dCTP, and the GTP oxidation product
eluted immediately before authentic GTP. These preliminary experiments suggest that the unknown material, which may provide a clue to the MutT
function, is not an oxidized derivative of a standard nucleoside triphosphate.
In our analyses of the other two mutT mutants we were
similarly unable to detect material with an elution time of 37 min, corresponding to 8-oxo-dGTP (data not shown). As expected for mutT mutants, all three strains that we studied lacked
detectable 8-oxo-dGTPase activity (Fig.
4). This was true whether the cells were
grown aerobically, anaerobically, or aerobically in the presence of 2.5 mM hydrogen peroxide.
Next we asked whether 8-oxo-dGTP could be detected in bacteria, either
wild-type or mutT-negative, that were oxygen-stressed by
growth in the presence of 2.5 mM hydrogen peroxide. For
this experiment we analyzed extracts from larger numbers of cells than depicted in Fig. 3. This allowed the visualization of a number of peaks
in the elution profiles (Fig. 5), but
none of them increased significantly in peroxide-stressed as compared
with normal bacterial cultures. Although one of the peaks was seen at
an elution time of 37 min in this experiment, it did not represent
8-oxo-dGTP, because addition of authentic 8-oxo-dGTP to one of the
extracts generated a distinct peak at 36 min (elution times for
8-oxo-dGTP varied slightly depending upon the age of the column). We
conclude that 8-oxo-dGTP levels are below the limits of detection by
our method, whether the bacteria are mutT-plus or -minus and
whether or not the cells are stressed by growth in hydrogen
peroxide.
Replication Errors Analyzed by in Vitro DNA Replication--
Using
standard 8-oxo-dGTP and extracts representing as many as 1.5 × 109 bacterial cells, we determined that we could have
detected as little as 6 pmol in a bacterial extract using our
electrochemical detection method (data not shown). Given the number of
bacterial cells represented by each extract we assayed, this lower
limit of detection would correspond to about 240 molecules/cell. Based upon previous dNTP pool size measurements from this laboratory (24),
240 molecules/E. coli cell would correspond to an
approximate intracellular concentration of 0.34 µM. We
then asked whether 8-oxo-dGTP at this concentration is significantly
mutagenic in an in vitro replication system containing the
four standard dNTPs at their approximate intracellular concentrations.
For this experiment we used the system of Roberts and Kunkel (22), in
which a cytosolic extract of HeLa cells is programmed with a modified
M13 phage replicative form DNA containing part of the E. coli
lacZ gene capable of
Thus, 8-oxo-dGTP appears not to be significantly mutagenic when exposed
to a replication system at its highest possible intracellular concentration in the presence of dGTP at 10 µM, the
estimated concentration in a HeLa cell nucleus. E. coli
contains dGTP at an estimated concentration of 100 µM
(24), which is 10-fold higher. If 0.34 µM
8-oxo-dGTP is not detectably mutagenic in the presence of dGTP at 10 µM, it seems unlikely that the oxidized nucleotide would
be mutagenic in the presence of dGTP at a 10-fold higher concentration.
We have developed a separation and analytical system that allows
the detection of as little as 6 pmol of 8-oxo-dGTP in a bacterial extract containing the normal nucleotides at their ordinary
concentrations. However, when extracts of wild-type and mutT
bacteria were compared, we were not able to detect the oxidized
nucleotide even at this level in either wild-type or mutant cell
extracts, whether or not the bacteria had been oxidatively stressed
beforehand by exposure to hydrogen peroxide. To be sure, our
electrochemical detection profiles did reveal the presence in mutant
cell extracts of at least one electrochemically active substance (Fig.
3, C and D) that is distinct from 8-oxo-dGTP.
Identification of this material might provide a clue to understanding
the mutator phenotype of mutT mutants. However, at present
we do not even know whether the unknown material is a nucleotide;
preliminary data indicate that it is not an oxidized derivative of one
of the standard ribo- or deoxyribonucleoside triphosphates. Clearly,
identification of this material, which is apparently present in quite
small amounts, might provide a clue to additional biochemical functions
of the MutT protein, and that is one of the directions our
future research will take.
Our observations with an in vitro replication error
detection system are consistent with the results of Einolf et
al. (16), who reported that 8-oxo-dGTP is a very poor substrate,
as compared with dGTP, for four different DNA polymerases: E. coli polymerases I and II, T7 polymerase, and HIV reverse
transcriptase. Three of those polymerases do not play their primary
roles in chromosomal DNA replication. However, more recently Einolf and
Guengerich (17) observed the same result when they analyzed 8-oxo-dGTP as a substrate for a mammalian replicative polymerase, DNA polymerase We thank our colleague Dr. William Baird and
the Center for Gene Research and Biotechnology for the long-term loan
of an HPLC electrochemical detector and a Beckman HPLC unit,
respectively, and we thank members of Dr. Baird's laboratory for
instructions in use of the electrochemical detector. We thank Stella
Martomo of this laboratory for assistance with the in vitro
DNA replication reactions. Special thanks are due to Dr. Michael
Tassotto for technical support.
*
This work was supported by grants from the National Science
Foundation (MCB 9906576) and the National Institutes of Health (GM 55134).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, February 20, 2002, DOI 10.1074/jbc.M200965200
The abbreviations used are:
oxoG, 7,8-dihydro-8-oxoguanine;
oxo-dGTP, 8-oxodeoxyguanosine triphosphate;
dNTP, deoxyribonucleoside 5'-triphosphate;
HPLC, high-performance
liquid chromatography;
X-gal, 5-bromo-4-chloro-3-indoyl-
Assessing the Metabolic Function of the MutT 8-Oxodeoxyguanosine
Triphosphatase in Escherichia coli by Nucleotide Pool
Analysis*
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
20 °C followed by drying under vacuum, re-extraction in 5%
trichloroacetic acid, centrifugation, extraction of the supernatant
with 0.5 M tri-N-octylamine-Freon, drying
of the aqueous phase, and dissolution of the solid residue in 100 µl
of HPLC buffer (50% buffer A, 50% buffer B; see below). One
modification was that all solutions used for nucleotide extraction
contained 0.1 mM desferrioxamine mesylate
(Sigma-Aldrich), to prevent oxidation during the extraction procedure (19). The yield of dNTP extracted was determined by subjecting standard dNTPs to identical extraction conditions and then
subjecting them to the same HPLC analysis as the extracts. A typical
recovery for 8-oxo-dGTP was 64%, and for the standard dNTPs,
recoveries ranged from 50 to 80%.
-complementation. The lacZ gene
contains an opal mutation in codon 7 of the gene for the
-complementing peptide. Most substitution mutations at this site
generate a peptide in which -complementation is readily detected by
plating in the presence of X-gal, a chromogenic 
-galactosidase substrate. The specific DNA construct used in these experiments is
identified as M13mp2SV/opal-7 in another paper from this laboratory (23), and the specific methods we used are as described in that reference. DNA synthesis reactions were carried out using HeLa S3 cell
cytoplasmic extract (75 µg protein), 1 µg of SV40 T antigen (Molecular Biology Resources, Milwaukee, WI), 80 ng of DNA template, and nucleotides at the following concentrations: dATP, 60 µM; dCTP, 30 µM; dGTP, 10 µM;
dTTP, 60 µM; and 8-oxo-dGTP (Amersham Biosciences);
concentrations varied as indicated. Additional reaction components included 30 mM HEPES buffer, pH 7.8, 7 mM MgCl2, 200 µM each of CTP,
GTP, and UTP, 4 mM ATP, 0.5 mM dithiothreitol, and 25 µg of bovine serum albumin. Reaction mixtures were incubated for 4 h at 37 °C.
-complementing host (22), in the presence of X-gal at a
density sufficient to give about 2000 plaques/plate. Mutant plaques
were identified by their blue color.
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
View larger version (13K):
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Fig. 1.
Voltammograms of 8-oxo-dGTP and dGTP at a
glassy carbon electrode. Maximal oxidation of 8-oxo-dGTP occurs at
an applied potential of +900 mV. 120 pmol of each nucleotide was
injected for each chromatographic run.
View larger version (17K):
[in a new window]
Fig. 2.
HPLC and electrochemical detection of
8-oxo-dGTP. Top panel, elution profile of a mixture of
250 pmol of each standard ribo- and deoxyribonucleoside triphosphate.
The standard nucleotides were detected by UV absorbance at 267 nm.
Bottom panel, analysis by electrochemical detection of a
250-pmol sample of authentic 8-oxo-dGTP eluted under identical
conditions. Electrochemical detection was carried out at an applied
potential of +900 mV. A separate analysis of the standard triphosphate
mixture by electrochemical detection showed no peaks (not shown).
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Fig. 3.
Analysis of E. coli
nucleotide extracts by electrochemical detection. Panel
A shows the detection of 50 pmol of authentic 8-oxo-dGTP standard
at an applied potential of +900 mV. Nucleotide extracts (50 µl each)
from E. coli B (B) and the
mutT 
strain, ES1580 (C), were
separated by HPLC and detected electrochemically at +900 mV.
Panel D shows the HPLC separation and electrochemical
detection of nucleotides extracted from ES1580 with 50 pmol of
authentic 8-oxo-dGTP standard added to the extract. Each
chromatographic run represents the nucleotides extracted from
~109 cells.
View larger version (27K):
[in a new window]
Fig. 4.
Lack of detectable 8-oxo-dGTPase activity in
extracts of wild-type and mutT mutant E. coli strains. Anaerobic cultures were grown to mid-log
phase in a Bactron anaerobic chamber (Sheldon Mfg.). Error
bars represent the standard error for three independent cultures
treated identically. To each H2O2-treated
culture (50 ml each) was added H2O2 to 5 mM every 20 min for 2 h until the cultures were in
mid-log phase. Measurements of H2O2 levels in
the cultures established that frequent additions were necessary to
maintain levels close to 5 mM.
View larger version (16K):
[in a new window]
Fig. 5.
Effect of bacterial growth in hydrogen
peroxide upon HPLC profile. Cells were exposed to 2.5 mM H2O2 for 15 min prior to
nucleotide extraction (A, C, and
D). Nucleotide extracts were prepared as described under
"Experimental Procedures" except that desferrioxamine mesylate was
not added during the extraction. Nucleotides were detected
electrochemically at an applied potential of +900 mV, and each
chromatogram represents nucleotides extracted from ~7 × 109 cells. Panel B depicts an extract of T-198
(mutT) bacteria grown in the absence of
H2O2. Panel D depicts an extract of
mutT mutant bacteria grown in H2O2
to which was added 100 pmol of authentic 8-oxo-dGTP immediately prior
to HPLC analysis.
-complementation and an SV40 replication
origin. The lacZ gene contains an opal mutation in codon 7 of the gene for the -complementing peptide. Most substitution
mutations at this site generate a peptide in which -complementation
is readily detected by plating in the presence of a chromogenic
-galactosidase substrate. In the presence of supercoiled RF DNA from
this phagemid and SV40 T-antigen, replication in this system initiates
at the SV40 origin and is semiconservative (22). For this experiment we
provided the standard dNTPs at concentrations estimated to exist inside
a HeLa cell nucleus: 60 µM dATP, 60 µM
dTTP, 30 µM dCTP, and 10 µM dGTP (25). As
shown in Table I, the addition of
8-oxo-dGTP to this system at 0.34 µM yielded, after
replication and analysis, a mutant fraction indistinguishable from that
seen with an otherwise identical replication mixture containing no 8-oxo-dGTP. The mutant fraction increased slightly as the 8-oxo-dGTP concentration was increased to 10 µM, but as the numbers
of mutant plaques counted were quite small, the calculated increases in mutant fraction are probably not statistically significant.
Effect of 8-oxo-dGTP upon mutation frequency during in vitro DNA
replication
-complementing host in the presence of X-gal. Mutant
plaques were identified by their blue color. Background refers to
pre-existing mutants present in the phagemid preparations that were not
subjected to in vitro replication.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
, in the presence of proliferating cell nuclear antigen. Our in vitro experiments were done with a human cell extract
system (22) that carries out semiconservative replication
initiating at normal replication origins. Using a mutational target in
which most or all substitution mutations can be detected, we saw no significant increase over the control mutant fraction when replication was carried out in the presence of standard 8-oxo-dGTP at the experimentally determined upper limit of its intracellular
concentration. These observations, coupled with expression of the
mutT mutator phenotype under anaerobic growth conditions
(15), suggest that the mechanism by which the MutT protein counteracts
oxidative mutagenesis needs to be re-evaluated.
ACKNOWLEDGEMENTS
FOOTNOTES
To whom correspondence should be addressed. Tel.: 541-737-1865;
Fax: 541-754-0481; E-mail: mathewsc@ucs.orst.edu.
ABBREVIATIONS
-D-galactoside;
HIV, human
immunodeficiency virus.
REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
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