(Received for publication, March 26, 1997)
From the Department of Biology and the
§ Curriculum in Genetics and Molecular Biology, University
of North Carolina, Chapel Hill, North Carolina 27599
A site-directed mutation in motif IV of Escherichia coli DNA helicase II (UvrD) was generated to examine the functional significance of this region. The highly conserved arginine at position 284 was replaced with alanine to construct UvrD-R284A. The ability of the mutant allele to function in methyl-directed mismatch repair and UvrABC-mediated nucleotide excision repair was examined by genetic complementation assays. The R284A substitution abolished function in both DNA repair pathways. To identify the biochemical defects responsible for the loss of biological function, UvrD-R284A was purified to apparent homogeneity, and its biochemical properties were compared with wild-type UvrD. UvrD-R284A failed to unwind a 92-base pair duplex region and was severely compromised in unwinding a 20-base pair duplex region. The Km of UvrD-R284A for ATP was significantly greater than 3 mM compared with 80 µM for UvrD. A large decrease in ATP binding was confirmed using a nitrocellulose filter binding assay. These data suggested that the R284A mutation severely reduced the affinity of helicase II for ATP. The reduced unwinding activity and loss of biological function of UvrD-R284A was probably the result of decreased affinity for ATP. These results implicate motif IV of superfamily I helicases in nucleotide binding and represent the first characterization of a helicase mutation outside motifs I and II that severely impacted the Km for ATP.
Helicase-catalyzed unwinding of double-stranded nucleic acid
molecules is required in all aspects of DNA and RNA metabolism including replication, DNA repair, recombination, transcription, translation, RNA processing, and bacterial conjugation (1-10). Helicases couple the energy derived from hydrolysis of nucleoside 5-triphosphates (NTPs)1 to the disruption
of hydrogen bonds between the complementary bases of a double helix.
The mechanism of unwinding is not known although models have been
proposed and are currently being tested (7, 11, 12). These models are
based on the formation of active oligomers, which provide multiple DNA
binding sites for the helicase. Most, if not all, helicases appear
capable of forming either a dimer or hexamer, and evidence suggests
that the oligomer is an active species (7).
Helicases are ubiquitous in nature, with numerous examples in viral, prokaryotic, and eukaryotic organisms. Extensive computer-assisted sequence analysis of numerous helicases has uncovered a series of short, conserved amino acid motifs (13-15). This has allowed grouping of helicases into four families based on the extent of amino acid similarity and on the organization of these conserved regions. These families presumably represent evolutionary relationships. Superfamilies I and II are the largest and most closely related groups, whereas superfamily III and family IV have unique motif compositions that differ considerably from those in superfamilies I and II and from each other (16).
Analysis of helicases with mutations in highly conserved residues in several of the so-called "helicase motifs" has suggested a biochemical role of some of these regions in helicase function. For example, motifs I and II, first described as the Walker A and B sequences in a large family of NTP binding proteins (17), have been directly implicated in NTP binding and/or hydrolysis (18-22). The function of the remaining helicase motifs is less clear. Roles for motif VI in nucleic acid binding and ATP hydrolysis have been proposed for various superfamily II RNA helicases (23-25). Motif V has been implicated in single-stranded DNA (ssDNA) binding (26) and motif III in coordination of ATP and ssDNA binding (27) for superfamily I helicases. The recent crystal structure of PcrA, a superfamily I DNA helicase from Bacillus stearothermophilus, suggested that all seven of the conserved helicase motifs are clustered together in the vicinity of the ATP binding site (28). Thus, all of the motifs may be involved in ATP binding and/or hydrolysis, at least for those enzymes with structures similar to PcrA.
Escherichia coli DNA helicase II, the product of the
uvrD gene, is a well characterized DNA helicase. This enzyme
is a required component of the UvrABC-mediated nucleotide excision
repair pathway (29, 30) and the methyl-directed mismatch repair pathway
(31). Less defined roles in recombination and DNA replication have also been suggested (18, 19, 32-40). The purified enzyme unwinds DNA with
3 to 5
polarity (41) and is capable of initiating unwinding from a
nick, its presumed biological substrate in the repair pathways
(42-44). UvrD belongs to helicase superfamily I along with other
E. coli helicases such as Rep, RecB, RecD, TraI, and
helicase IV (helD gene product) (13, 16), as well as a large
number of eukaryotic viral helicases and several yeast helicases.
UvrD has previously been the subject of biochemical and genetic studies involving mutation of highly conserved residues in motifs I, II, and III (18, 19, 27, 44). Currently, very little biochemical information exists on the specific role of motif IV in superfamily I and II helicases although its importance for biological function has been demonstrated in genetic studies (45-47). In this report, the functional significance of motif IV in E. coli DNA helicase II was addressed by site-directed mutagenesis of arginine residue 284, which is invariant among superfamily I helicases. The results indicated that the mutant protein had a significant decrease in affinity for ATP, implicating motif IV in nucleotide binding. This represents the first helicase mutation outside of motifs I and II that exhibits a severe defect in nucleotide binding.
Materials
Bacterial StrainsE. coli BL21(DE3)
(F ompT [lon] hsdSB
rB
mB
gal dcm
DE3) was from Novagen, Inc. E. coli JH137 (K91
lacZ dinD1::MudI (Apr lac)) was
obtained from Dr. P. Model (Rockefeller University). BL21(DE3)
uvrD and JH137
uvrD were
constructed previously in this laboratory (18).
pET81F1+ was from Dr. P. J. Laipis (University of Florida), and pET9d, pET11d, and pLysS were from Novagen, Inc. M13mp7 ssDNA was prepared as described previously (48). Unlabeled nucleotides were from U. S. Biochemicals Corp. Radioactively labeled nucleotides were from Amersham Corp. pET9d-UvrD and pET11d-UvrD were constructed previously in this laboratory (18).
EnzymesRestriction endonucleases, DNA polymerase I (large fragment), phage T4 DNA ligase, phage T7 DNA polymerase, and phage T7 polynucleotide kinase were from New England Biolabs Inc. and used as recommended by the supplier.
To overexpress helicase II prior to purification, a 10-liter culture of
mid-log phase BL21(DE3)/pLysS cells containing pET11d-UvrD or a 2-liter
culture of mid-log phase BL21(DE3)uvrD/pLysS cells containing pET9d-UvrD-R284A were induced for protein expression by
adding isopropyl
-D-thiogalactopyranoside to 0.5 mM. Growth was continued for 4 h at 37 °C.
Wild-type and mutant helicase II proteins were purified using a
procedure described previously (49). The concentration of purified
protein was determined by spectrophotometric absorbance readings at 280 nm using the previously published helicase II extinction coefficient of
1.29 ml mg
1 cm
1 (49). Storage buffer for
helicase II was 20 mM Tris-HCl (pH 8.3), 200 mM
NaCl, 25 mM 2-mercaptoethanol, 1 mM EDTA, 0.5 mM EGTA, and 50% glycerol.
Methods
Site-directed MutagenesisThe plasmid pET81F1-UvrD (27),
containing the full-length helicase II coding sequence cloned behind a
T7 promoter, as well as the phage F1 origin of replication, was the
template for site-directed mutagenesis by standard procedures (50). The
oligonucleotide 5-GCTGGTAGAGGCGTAGTTTTGCTCC-3
altered codon 284 of
helicase II from CGC(arginine) to GCC(alanine) and disrupted a
BsrBI restriction site, allowing the initial screening of
mutants by restriction digest. After mutagenesis, a 2.0-kilobase pair
NcoI-BsiWI DNA fragment containing the desired
mutation was sub-cloned into pET9d-UvrD, replacing the wild-type
NcoI-BsiWI fragment in this plasmid and generating pET9d-UvrD-R284A. The presence of a single mutation at the
correct location was verified by sequence analysis of the entire
helicase II gene in pET9d-UvrD-R284A using an Applied Biosystems 373A
DNA Sequencer.
UV irradiation survival was determined as described (19). The frequency of spontaneous mutant formation was determined as follows. Eleven independent transformants of each of the appropriate cell strains were grown overnight under antibiotic selection at 37 °C. Serial dilutions of each of the saturated cultures were made in M9 minimal media salts. Appropriate dilutions were plated on LB agar to determine cell titer and on LB agar plus 100 µg/ml rifampicin to determine the number of spontaneously arising rifampicin-resistant cells. After incubation at 37 °C for at least 24 h, colonies were counted, and the spontaneous mutant frequency was calculated for each strain by dividing the median value of rifampicin-resistant cells by the average total viable cells.
Proteolytic DigestionLimited chymotrypsin cleavage of UvrD
and UvrD-R284A was performed as described previously (51).
-Chymotrypsin (5 ng) was added to reactions (15 µl) containing
either 2 µM UvrD (monomer) or 1.8 µM
UvrD-R284A (monomer), and the reaction was incubated for 2 min at room
temperature (25 °C). Where indicated, 2 µM M13mp7 ssDNA was included. Reactions were stopped with 15 µl of gel loading buffer (250 mM Tris-HCl (pH 6.8), 3.4% SDS, 1.1 M 2-mercaptoethanol, 20% glycerol, 0.01% bromphenol blue)
and boiled for 2 min. Products were resolved on a 12% polyacrylamide
gel (32:1 cross-linking ratio) in the presence of 0.1% SDS and
visualized by staining with Coomassie Brilliant Blue R-250 (Sigma).
The binding of UvrD
and UvrD-R284A to ssDNA was determined by measuring the retention of
[32P]DNA on nitrocellulose filters as described
previously (52). Reactions (20 µl) contained 25 mM
Tris-HCl (pH 7.5), 3 mM MgCl2, 20 mM NaCl, 5 mM 2-mercaptoethanol, 50 µg/ml
bovine serum albumin, and a [32P]-labeled 92-bp partial
duplex helicase substrate (approximately 1.3 µM
nucleotide phosphate) (1.86 × 108 cpm
µmol1). Binding reactions were initiated with UvrD or
UvrD-R284A over a concentration range of 0.7-84 nM
(monomer). After incubation at 37 °C for 10 min, 1 ml of reaction
buffer (pre-warmed at 37 °C) was mixed with each sample, and the
entire volume was passed through a nitrocellulose filter at a flow rate
of 4 ml/min. Filters were washed twice with 1 ml of pre-warmed reaction
buffer, dried, and subjected to liquid scintillation counting.
Background binding in the absence of enzyme represented less than 0.5%
of the total signal and was subtracted from the experimental data.
Apparent Kd values were calculated as described
previously (27, 53).
Binding of [3H]ATP to UvrD was also examined by nitrocellulose filter binding. Reactions (20 µl) contained 25 mM Tris-HCl (pH 7.5), 3 mM MgCl2, 50 mM NaCl, 6.3 mM 2-mercaptoethanol, 100 µg/ml bovine serum albumin, 12.5% glycerol, and 2.3 µM UvrD or UvrD-R284A (monomer). Binding was initiated by addition of [3H]ATP (1.1 Ci/mmol) to a final concentration of 200 µM at 0 °C. After 4 min, 15 µl of each reaction was applied directly to a nitrocellulose filter presoaked in reaction buffer at 4 °C. Filters were rinsed once with 750 µl of reaction buffer at a flow rate of 4 ml/min, dried, and subjected to liquid scintillation counting. Background binding in the absence of enzyme represented less than 1% of the total signal and was subtracted from the experimental data. The nitrocellulose filters used in the DNA and ATP binding experiments (0.45 µM type HA, Millipore Corp.) were pre-treated by soaking in 0.4 M KOH for 40 min followed by extensive washing with deionized, distilled water.
Glutaraldehyde Cross-linkingThe presence of a dimeric
helicase II species was monitored by glutaraldehyde cross-linking as
described previously (27, 49). Reactions (20 µl) contained 20 mM Tricine (pH 8.3), 50 mM NaCl, 5 mM MgCl2, 5 mM 2-mercaptoethanol,
18% glycerol, and either 1.5 µM UvrD (monomer) or 1.4 µM UvrD-R284A (monomer). When present, the
oligonucleotide (dT)10 and ATPS were included at a
concentration of 1.7 µM and 3 mM,
respectively. Cross-linking was initiated by the addition of
glutaraldehyde (EM grade, Electron Microscopy Sciences) to a final
concentration of 0.01%. Reactions were incubated at room temperature
for 30 min and then quenched with 2 µl of 100 mM lysine
acetate and 20 µl of gel-loading buffer (see above). Samples were
boiled for 2 min, and the products were resolved on a 9.6%
polyacrylamide gel (32:1 cross-linking ratio) in the presence of 0.1%
SDS.
The DNA unwinding activity of UvrD and
UvrD-R284A was determined with 92- and 20-bp partial duplex
[32P]DNA substrates prepared as described previously (19,
41). Both substrates were purified by gel filtration on a Bio-Gel A5M column (Bio-Rad) prior to use. Helicase reactions (20 µl) contained 25 mM Tris-HCl (pH 7.5), 3 mM
MgCl2, 20 mM NaCl, 5 mM
2-mercaptoethanol, 3 mM ATP, and the indicated partial
duplex DNA substrate (approximately 1.3 µM nucleotide
phosphate) (1.8 × 108 cpm µmol1 for
the 92-bp substrate and 1.6 × 108 cpm
µmol
1 for the 20-bp substrate). Reactions were
pre-warmed at 37 °C and initiated with the indicated amount of UvrD
or UvrD-R284A. After incubation at 37 °C for 10 min, the reactions
were quenched with 10 µl of stop solution (37.5% glycerol, 50 mM EDTA, 0.05% each of xylene cyanol and bromphenol blue,
and 0.3% SDS). Products were resolved on an 8% non-denaturing
polyacrylamide gel, and the results were quantified using phosphor
storage technology and ImageQuant software (Molecular Dynamics).
The DNA-stimulated hydrolysis of ATP by UvrD and UvrD-R284A was measured as described previously (54). ATPase reaction mixtures were identical to those for the helicase reactions with the following exceptions. M13mp7 ssDNA (30 µM nucleotide phosphate) was substituted for the partial duplex helicase substrate, and [3H]ATP was substituted for unlabeled ATP. Reactions (20 µl) were pre-warmed at 37 °C and initiated with the indicated amount of [3H]ATP. Reactions were incubated at 37 °C, and duplicate samples (5 µl) were removed and quenched with 5 µl of stop solution (33 mM EDTA, 7 mM ATP, and 7 mM ADP) after 5 min for UvrD or 10 min for UvrD-R284A. Products were processed as described previously (54).
DNA helicase II (also called UvrD) has been included, along with a
large number of other helicases and putative helicases, in a group
designated helicase superfamily I based on conservation of amino acid
sequence in seven distinct motifs (13, 15). Presumably, these motifs
represent sites of functional significance that have been
evolutionarily conserved. The amino acid sequences of motif IV from the
E. coli superfamily I helicases, including UvrD, are shown
in Fig. 1. To evaluate the functional significance of
motif IV, a mutant uvrD allele was constructed containing an arginine to alanine substitution at position 284 (uvrD-R284A). This arginine is the most highly conserved
residue in motif IV. It is found in all identified members of
superfamily I. The ability of the mutant protein to substitute for the
wild-type protein in two DNA repair pathways was examined in genetic
complementation studies. In addition, the UvrD-R284A protein was
purified and biochemically characterized.
Genetic Characterization of UvrD-R284A
DNA helicase II is an essential component of two DNA repair
pathways, methyl-directed mismatch repair and UvrABC-mediated nucleotide excision repair (29-31). The ability of UvrD-R284A to function in each pathway was tested using genetic complementation assays. The frequency of spontaneous mutant formation in E. coli strain JH137uvrD was 161-fold higher than its
parent strain JH137 due to loss of a functional methyl-directed
mismatch repair system (55, 56). JH137
uvrD was also
highly sensitive to UV light due to loss of UvrABC-mediated nucleotide
excision repair (57). Plasmids pET9d-UvrD and pET9d-UvrD-R284A were
transformed into JH137
uvrD to examine the ability of UvrD
and UvrD-R284A to restore the wild-type spontaneous mutant frequency
and UV resistance. The level of uninduced expression of the
uvrD gene from pET9d-UvrD in JH137
uvrD was
determined previously and was only slightly less than expression from
the JH137 chromosome (18). This was confirmed in this study (data not
shown).
The frequency of formation of spontaneous mutants at the
rpoB locus (Rifr phenotype) was determined as
described under "Experimental Procedures." Wild-type
uvrD, when introduced on the pET9d plasmid, fully restored methyl-directed mismatch repair function as indicated by a relative mutability of 0.6 compared with 1.0 for the parental strain JH137 (Table I). In contrast, the presence of the
uvrD-R284A allele in JH137uvrD resulted in a
relative mutability of 121, suggesting that the mutant protein did not
function in the methyl-directed mismatch repair pathway.
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The ability of UvrD-R284A to function in UvrABC-mediated nucleotide
excision repair was assessed by exposing cells to UV light and
determining survival at increasing UV fluences. Strains JH137, JH137uvrD, JH137
uvrD/pET9d,
JH137
uvrD/pET9d-UvrD, and
JH137
uvrD/pET9d-UvrD-R284A were compared as shown in Fig.
2. pET9d-UvrD completely restored the wild-type level of
UV resistance. The mutant allele did not restore wild-type UV
resistance and appeared to make the cells slightly hypersensitive to UV
light as compared with JH137
uvrD. The significance of the
latter observation was not explored. It was clear that UvrD-R284A was
not able to substitute for UvrD in UvrABC-mediated nucleotide excision
repair.
Biochemical Characterization of UvrD-R284A
To identify the biochemical defects responsible for the loss of
biological function of UvrD-R284A, mutant and wild-type helicase II
were purified as described previously (49). UvrD was purified to
apparent homogeneity as evidenced by the presence of a single protein
species on an SDS-polyacrylamide gel (Fig. 3, lane
A). Purified UvrD-R284A was contaminated by three faint species
migrating slightly faster than UvrD-R284A (Fig. 3, lane D).
These species appeared to be proteolytic products of UvrD-R284A because
they all reacted strongly with anti-helicase II antibody (data not shown). This suggested that the mutant enzyme was somewhat less stable
than the wild-type enzyme. However, UvrD-R284A folded normally as
indicated by a chymotrypsin cleavage pattern that was identical to that
of UvrD (Fig. 3, lanes B and E). In the presence
of ssDNA, both UvrD-R284A and UvrD were protected from chymotrypsin
cleavage (Fig. 3, lanes C and F). Furthermore,
proteolytic products did not accumulate with long term enzyme storage.
Given these results and the minimal representation of the smaller
species in the total protein, it was unlikely that their presence
influenced the data presented in this study.
DNA Binding
The ability of UvrD-R284A to bind to DNA was
tested using a nitrocellulose filter binding assay and the 92-bp
partial duplex helicase substrate. Although the substrate contains a
short duplex region, the assay measured primarily the affinity of the
protein for ssDNA due to the lack of significant binding of helicase II to double-stranded DNA. DNA binding isotherms were generated using a
constant ligand concentration and varying concentrations of helicase II
(Fig. 4). A Hill plot was used to calculate apparent equilibrium dissociation constants from these data as described previously (27, 53). There was no significant difference between the
DNA binding properties of UvrD-R284A and UvrD (apparent
Kd of 11 and 17 nM, respectively). Thus,
the highly conserved arginine residue in motif IV was not required for
nucleic acid binding. This conclusion was further supported by the
results of limited proteolysis experiments (see Fig. 3), which
demonstrated that both UvrD and UvrD-R284A were protected from
chymotrypsin cleavage when an ssDNA ligand was present and presumably
bound by the enzyme.
Dimerization
A glutaraldehyde cross-linking procedure was
used to detect dimerization of UvrD and UvrD-R284A (49). Glutaraldehyde
catalyzes the formation of a covalent bond between primary amines in
close proximity, providing a simple method for detecting
protein-protein interactions in solution. UvrD and UvrD-R284A, at a
relatively high concentration, were each exposed to a low concentration
of glutaraldehyde in the absence or presence of ATPS or
oligonucleotide (dT)10. The products were resolved on an
SDS-polyacrylamide gel and stained with Coomassie Blue. No difference
in the dimerization of UvrD and UvrD-R284A was observed in the absence
or presence of ATP
S or oligo(dT)10 (data not shown).
Helicase II catalyzes a DNA-stimulated ATP
hydrolysis reaction that is coupled to the unwinding reaction. To begin
to evaluate the ATPase activity of UvrD-R284A, we attempted to measure
a Km for ATP. Wild-type UvrD exhibited a standard
hyperbolic saturation curve as a function of increasing ATP
concentration with a Km of 80 ± 7 µM (Fig. 5A). The
Km value of UvrD-R284A for ATP was too high to be
determined because the maximal velocity could not be approached. The
velocity of ATP hydrolysis catalyzed by UvrD-R284A was a linear
function of ATP concentration up to 3 mM (Fig.
5B). Apparent substrate inhibition of the wild-type enzyme
prevented accurate measurement of ATP hydrolysis velocities at
substantially higher ATP concentrations (data not shown). The inability
to saturate UvrD-R284A with ATP suggested that it was defective in
nucleotide binding.
ATP Binding
To directly measure the affinity of helicase II
for ATP, an initial attempt was made to determine the equilibrium
dissociation constant, Kd. Several techniques were
used without success, including fluorescence spectroscopy and
nitrocellulose filter binding. Failure to determine a
Kd was the result of the limited solubility of
helicase II and its relatively low affinity for ATP, which made it
impossible to generate a complete and reproducible binding curve using
these assays. In addition, we did not observe an intrinsic fluorescence
change in helicase II upon ATP binding. However, having a
Kd for the UvrD-ATP interaction would not be useful
for comparative purposes if we were unable to measure this value for
UvrD-R284A. Instead, nitrocellulose filter binding assays were used as
a qualitative comparison of ATP binding between UvrD and UvrD-R284A by
measuring the amount of [3H]ATP bound at a single
nucleotide concentration. These assays were performed at 0 °C and in
the absence of DNA. Under these conditions, the turnover number for
wild-type helicase II was approximately 0.002 s1 (data
not shown). Table II shows that at 200 µM
[3H]ATP, UvrD bound 0.92 pmol of ATP/pmol of enzyme. This
fraction of ATP-bound enzyme was fairly consistent with a
Km of 80 µM ATP. In contrast,
UvrD-R284A bound only 0.015 pmol of ATP/pmol of enzyme, 1.6% of the
wild-type value. These results suggested that UvrD-R284A was defective
in its association with ATP.
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The lack of genetic complementation in both
DNA repair pathways suggested that the mutant protein was severely
compromised in its DNA unwinding activity. The unwinding activity of
UvrD-R284A was measured using two short partial duplex DNA substrates
and was compared with UvrD (Fig. 6). The mutant enzyme
failed to catalyze unwinding of a 92-bp duplex region and catalyzed
feeble unwinding of a 20-bp duplex region in a 10-min incubation. At a
UvrD-R284A concentration of 344 nM, there was no detectable
unwinding of the 92-bp partial duplex substrate and less than 10 percent unwinding of the 20-bp partial duplex substrate. In contrast,
wild-type helicase II unwound 50% of the 92-bp partial duplex
substrate at a protein concentration of 25 nM and 50% of
the 20-bp partial duplex substrate at a protein concentration of 0.5 nM. In a 100-min incubation, 197 nM UvrD-R284A
unwound 39% of the 20-bp partial duplex. Under the same conditions,
344 nM mutant enzyme did not unwind a detectable fraction
of the 92-bp substrate (data not shown).
The results presented here indicate that arginine 284 is required for high affinity binding of ATP, which suggests that motif IV is an integral part of the nucleotide binding site on DNA helicase II. This was initially surprising since it is generally believed that helicase motifs I and II are involved in NTP binding and/or hydrolysis. This notion stems from the fact that motifs I and II are common to a large population of NTP-binding proteins, including the DNA helicases (17). Moreover, biochemical studies on mutants of a wide range of helicases have generally supported a role for motifs I and II in NTP hydrolysis (18-22). Most of the mutations, however, did not affect NTP binding. Helicase motif IV is not conserved among all NTP binding proteins, which suggested that it might be important for a biochemical property common to helicases. However, UvrD-R284A exhibited a significant defect in ATP binding, and in light of the recent crystal structure of PcrA, this result can be readily explained (see below).
Efforts to define the kinetic parameters Km and kcat for the DNA-stimulated ATP hydrolysis reaction revealed an inability to saturate UvrD-R284A with ATP. Since the ATPase reaction velocity was a linear function of ATP concentration up to 3 mM, the Km for ATP must be much greater than 3 mM. Km is defined as the concentration of substrate that provides half-maximal reaction velocity. If it is assumed that the ATPase reaction catalyzed by helicase II can be described by simple Michaelis-Menten kinetics and that a minimal reaction is represented by the following scheme, where S is ATP,
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To isolate and evaluate the initial ATP binding event, conditions were
sought under which a negligible amount of ATP hydrolysis occurred. At
0 °C in the absence of DNA, the turnover number for ATP by UvrD was
approximately 0.002 s1. No hydrolysis was detected under
these conditions using UvrD-R284A. Thus, the nitrocellulose filter
binding assay likely measured only E + S
ES, again assuming the simple Michaelis-Menten scheme depicted above. Since the amount of ATP bound by UvrD-R284A was significantly decreased under these conditions, a decreased affinity for ATP was likely the primary defect in the mutant protein. Thus, the
large increase in Km for ATP was the result of a decreased affinity for the substrate.
A defect in ATP binding would seem to be at odds with the results of
proteolysis protection experiments (data not shown). The presence of
ATP, like ssDNA, protects wild-type helicase II from cleavage by
chymotrypsin (51). Based on the decreased binding of ATP by UvrD-R284A,
we expected to see a large difference in the amount of ATP required to
protect UvrD versus UvrD-R284A from proteolytic cleavage. In
fact, the increase in the concentration of ATP required for protection
of UvrD-R284A compared with UvrD was relatively small (less than
2-fold, data not shown). However, the structural changes responsible
for proteolysis protection when ligands are present are not known. This
fact, coupled with the lack of information on the kinetic mechanism for
ATP hydrolysis catalyzed by helicase II, makes it possible that the
proteolysis protection assay does not directly measure ATP binding. For
example, an ATP concentration of 1.5-2.0 mM was required
for significant protection of UvrD from cleavage by chymotrypsin. This
is clearly inconsistent with a Km for ATP of 80 µM. This fact alone indicates that this assay measures
something more complex than simple ATP binding. Furthermore, when the
poorly hydrolyzed ATP analog ATPS was used as a ligand, there was a
more substantial increase in the concentration required for proteolytic
protection of UvrD-R284A compared with UvrD (approximately 6-fold, data
not shown). The results of the proteolysis protection study likely reflected a combination of processes such as ATP hydrolysis and conformational changes in the protein, in addition to nucleotide binding. Thus, the results of this series of experiments, while not
fully explained, cannot be interpreted as evidence for a normal interaction with ATP.
Although there was clearly a serious defect in nucleotide binding, it
was also possible that an additional defect existed in the hydrolytic
mechanism. Such a defect would also have contributed to the inability
of UvrD-R284A to unwind DNA and function in DNA repair pathways. It was
possible to estimate a Km for UvrD-R284A from the
data in Fig. 5 if we assumed the hydrolytic mechanism was unaffected.
The initial slope of a reaction velocity versus substrate
concentration graph, such as the one depicted in Fig. 5, is equal to
kcat/Km × ET, where ET is the total
enzyme concentration. If the hydrolytic mechanism of UvrD-R284A were
unaffected by the mutation, then kcat should
have been equal to that of UvrD. From the slope of the line in Fig.
5B and the UvrD kcat of 162 s1, an estimated Km for ATP for
UvrD-R284A was 143 mM. The plot of initial velocity
versus substrate concentration for UvrD-R284A was linear to
at least 3 mM ATP. Since there was no deviation from
linearity, it was concluded that the actual Km was
significantly higher than 3 mM. Apparent substrate
inhibition with wild-type helicase II at high ATP concentrations,
coupled with the necessary modifications in reaction conditions, made it impossible to accurately measure hydrolysis at ATP concentrations significantly higher than 3 mM. Therefore, the relationship
between the apparent Km for ATP and the 143 mM value estimated above was not determined. In light of
these results, it remains possible that there was a defect in the
hydrolytic mechanism of UvrD-R284A in addition to the severe defect in
ATP binding.
The helicase activity of the UvrD-R284A mutant was significantly compromised, and the protein failed to function in vivo. Helicase activity is dependent on ATP hydrolysis, and it seemed reasonable to conclude that the lack of unwinding was due to the tremendous decrease in ATP hydrolysis that, in turn, was due to a decreased affinity of the mutant enzyme for ATP. However, the possibility that the R284A substitution also directly impaired the unwinding mechanism or the coupling between hydrolysis and unwinding cannot formally be ruled out. Based on the results presented here, the lack of biological function in both DNA repair pathways was probably a result of the ATP binding defect. With a Km for ATP significantly greater than 3 mM, it is unlikely that an intracellular ATP concentration of 3 mM (59) would be sufficient to adequately populate the active helicase II pool and allow the enzyme to function properly in vivo.
To the best of our knowledge, UvrD-R284A represents the first helicase mutant, outside of motifs I and II, whose primary defect is in nucleotide binding. A helicase II mutant in motif III was defective in binding ATP but only in the absence of ssDNA (27). This mutant was also defective in binding ssDNA in the absence of ATP. In the presence of ssDNA, the motif III mutant bound ATP with normal affinity, and it was concluded that the motif III mutant was compromised in the ability to form stable binary complexes with its two ligands.
The ATP binding defect described in this study is consistent with the recently published crystal structure of the PcrA helicase (28). The overall amino acid sequence of the PcrA helicase from B. stearothermophilus is 44% identical to UvrD and 90% identical within the seven conserved helicase motifs. Notably, these seven motifs are clustered together at the base of the enzyme, forming the ATP-binding pocket. In view of the extensive amino acid identity, particularly among the conserved motifs, it is likely that the structure of the nucleotide binding sites of PcrA and UvrD closely resemble one another. From this structure, it seems likely that all seven motifs may be involved in nucleotide binding and/or hydrolysis, and thus, a role for motif IV in ATP binding is not surprising.
The PcrA structure indicates that motif IV forms a bridge connecting the two large domains of the protein at the bottom of the nucleotide binding pocket. This region lies near the adenine base of the bound nucleotide, and the authors suggest that a conserved tyrosine in motif IV makes a stacking interaction with the bound NTP. This tyrosine, which is not conserved in all superfamily I helicases, is immediately followed by the invariant arginine that was altered in this study (see Fig. 1). The apparent absence of additional specific interactions between the adenine base and nearby amino acid residues was suggested as an explanation for the lack of nucleotide specificity in reactions catalyzed by the PcrA helicase. UvrD, on the other hand, exhibits a strong preference for ATP or dATP (60), and it is possible that arginine 284 is involved in a specific interaction with the adenine base on ATP and dATP, whereas its counterpart in PcrA contributes less to specificity. Alternatively, arginine 284 may not directly contact the nucleotide but might mediate a local conformational change that places other residues, such as tyrosine 283, in proper position to interact with the NTP. Yet another possibility is that motif IV, acting as a bridge between the two large domains of the helicase, might mediate a global conformational change in the protein that is required for high affinity NTP binding. A more detailed description of the role of arginine 284 in ATP binding must await a high resolution structure for ATP-bound helicase II.
We thank Dr. Thomas Kunkel, Dr. David Porter, and Leah Mechanic for critical reading of the manuscript and Susan Whitfield for preparation of figures. We are especially grateful to Dr. David Porter for assistance with analyzing the steady-state kinetic data.