Novel Escherichia coli umuD' Mutants: Structure-Function Insights into SOS Mutagenesis

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Journal of Bacteriology, September 1998, p. 4658-4666, Vol. 180, No. 17
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Novel Escherichia coli umuD' Mutants: Structure-Function Insights into SOS Mutagenesis

Mary McLenigan,¹ Thomas S. Peat,²^, Ekaterina G. Frank,¹ John P. McDonald,¹ Martín Gonzalez,¹ Arthur S. Levine,¹ Wayne A. Hendrickson,²^,³ and Roger Woodgate¹^,^*

Section on DNA Replication, Repair and Mutagenesis, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, Maryland 20892¹ and Department of Biochemistry and Molecular Biophysics² and Howard Hughes Medical Institute,³ Columbia University, New York, New York 10032

Received 20 March 1998/Accepted 20 June 1998

	ABSTRACT

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Although it has been 10 years since the discovery that the Escherichia coli UmuD protein undergoes a RecA-mediated cleavagereaction to generate mutagenically active UmuD', the functionof UmuD' has yet to be determined. In an attempt to elucidatethe role of UmuD' in SOS mutagenesis, we have utilized a colorimetricpapillation assay to screen for mutants of a hydroxylamine-treated,low-copy-number umuD' plasmid that are unable to promote SOS-dependentspontaneous mutagenesis. Using such an approach, we have identified14 independent umuD' mutants. Analysis of these mutants revealedthat two resulted from promoter changes which reduced the expressionof wild-type UmuD', three were nonsense mutations that resultedin a truncated UmuD' protein, and the remaining nine were missensealterations. In addition to the hydroxylamine-generated mutants,we have subcloned the mutations found in three chromosomal umuD1,umuD44, and umuD77 alleles into umuD'. All 17 umuD' mutants resultedin lower levels of SOS-dependent spontaneous mutagenesis but variedin the extent to which they promoted methyl methanesulfonate-inducedmutagenesis. We have attempted to correlate these phenotypes withthe potential effect of each mutation on the recently describedstructure of UmuD'.

	INTRODUCTION

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While it has been known for some time that SOS mutagenesis in Escherichia coli is not a passive process (see references 12and 40 for recent reviews), the complexity of the protein-proteininteractions necessary to facilitate error-prone translesion DNAsynthesis is only just being comprehended. Both genetic and biochemicalexperiments have demonstrated that UmuD is functionally inactiveuntil it undergoes a posttranslational cleavage reaction to UmuD'(4, 25, 33). Once generated, UmuD' associates with UmuC,RecA, and DNA polymerase III proteins to form the so-called "mutasome"(30). It was previously thought that this mutasome facilitatedonly translesion replication, but recent data suggest that itcan also promote extension from mispairs generated during normalDNA synthesis (8).

The likelihood of formation of the mutasome depends upon a series of sequential protein-protein interactions that determinethe stability of the Umu mutagenesis proteins (5, 10). Forexample, both the UmuD and UmuC proteins are labile in vivo andare rapidly degraded by the Lon protease (9). Although UmuDcan autodigest (4), an interaction with a RecA nucleoproteinfilament greatly enhances the efficiency of the conversion ofUmuD to UmuD' (33, 39). As a consequence, UmuD' is able toform a complex with UmuC that appears to be much more stable thanthe corresponding UmuDC complex (10, 18).

Despite advances in the understanding of the regulation of SOS mutagenesis, little is known about the function of UmuD' inthe mutagenic process. Potential insights into such activitiescan be gained from the structural analysis of UmuD'. The UmuD'monomer consists of a compact globular head (residues 46 to 135)with an unusual antiparallel $beta$ -structure composed of seven $beta$ -strandswhich associate to form three $beta$ -sheets (27). The remaining residues(25 to 45 and 136 to 139) form long N-terminal and short C-terminalextensions from the body of the protein. Within the crystallizedUmuD' structure, three discrete but interrelated structural formsare observed. The first, termed the "molecular dimer," is primarilyhydrophobic and consists of parts of residues Tyr52, Val54, Ile87,Gly92, Glu93, Phe94, and Phe128, with the Phe94 residues fromeach monomer stacked on top of each other. The second form isthe "filament dimer." The filament dimer interface involves hydrogenbonds between the two short carboxyl-terminal extensions fromeach monomer as well as several hydrophobic interactions betweenthe overlapping extended amino termini. The two dimers were sonamed because of additional molecular and biochemical data whichsuggested that the molecular dimer predominates over the filamentdimer in dilute solution (28). Using nuclear magnetic resonance(NMR), Ferentz et al. have reported strong intersubunit nuclearoverhauser effects at the C terminus of UmuD' (6) and suggestthat only the crystal filament dimer may, in fact, exist in solution.Finally, again within the UmuD' crystal, UmuD' molecular and filamentdimers associate together such that they form an "extended UmuD'filament" (27, 28) that, based upon mutational analysis, ishypothesized to be important for the biological function of UmuD'(28).

Experiments that will, hopefully, resolve the differences in interpretation of dimeric UmuD' structures as defined by crystallographyand NMR spectroscopy are currently in progress. In this work,we continue to use the terms "molecular dimer" to indicate theprotein-protein interactions between the two globular domainsof each UmuD' promoter and "filament dimer" to indicate the interactionsbetween the long and short N- and C-terminal extensions (28).

As part of our continuing studies into the molecular mechanisms of damage-inducible mutagenesis, we were interested in isolatingnovel loss-of-function umuD' mutants that might provide structure-functioninsights into the activities of the UmuD' protein. To do so, wehave taken advantage of a powerful colorimetric papillation assayto screen for randomly mutagenized plasmid-encoded UmuD' proteinsthat are unable to promote SOS-dependent spontaneous mutagenesis.Similar to a previous study in which loss-of-function UmuC proteinswere identified (41), this strategy resulted in the isolationof a number of novel umuD' mutants. While all of the novel umuD'mutants that we have isolated result in a reduced capacity topromote spontaneous SOS mutagenesis, they vary in the extent towhich they promote mutagenesis in damaged cells; we have attemptedto explain these phenotypes based upon the predicted structuralchanges between the mutant and wild-type UmuD' proteins (6,27, 28).

	MATERIALS AND METHODS

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Plasmids and bacterial strains. To facilitate the specific identification of E. coli umuD' mutants, we have utilized two compatible plasmids that separatelyencode the genetically engineered umuD' and umuC genes (41).pRW66 is a low-copy-number spectinomycin resistance plasmid thatexpresses UmuD'. pRW124 is a medium-copy-number ampicillin resistanceplasmid that expresses UmuC. Both vectors express the Umu proteinsfrom the native umu promoter, but pRW124 lacks an obvious ribosomebinding site. As a consequence, the level of UmuC protein expressedfrom the medium-copy-number plasmid is comparable to that of UmuD'from the low-copy-number plasmid and is only three- to fivefoldhigher than that expressed chromosomally (41).

Three E. coli K-12 strains were utilized to identify and characterize the novel plasmid-encoded umuD' mutants. Strain RW126[relevant genotype, $Delta$ (umuDC)595::cat recA718 srlC300::Tn10 lexA71(Def)::Tn5hisG4(Oc) galK2(Oc)] was used for the initial screening and principlecharacterization of the plasmid-encoded umuD' mutants. This strainis extremely useful in identifying plasmids that carry eithera gain (15) or loss (41) of Umu-like activity, as it measuresboth Umu-dependent spontaneous mutator activity and damage-inducedUmu-dependent mutagenesis. Strain JL852 [relevant genotype, recA730srlC300::Tn10 lexA71(Def)::Tn5 hisG4(Oc)] (22) was used to determineif any of the plasmid-encoded mutants were phenotypically dominantnegative. This strain expresses the chromosomally encoded UmuDand UmuC proteins, but since the RecA730 protein constitutivelymediates cleavage of UmuD (33, 39) the strain is, in fact,phenotypically UmuD'C. Strain TK614 [relevant genotype, recA⁺ lexA⁺ uvrA6 umuD77 hisG4(Oc)] (19) was used to isolate plasmid DNAfor sequencing (see below).

In vitro mutagenesis of pRW66 and screening for umuD' mutants. Randomly mutagenized pRW66 was obtained following the hydroxylamine mutagenesis procedure described previously (16, 41).Briefly, 2 µg of purified plasmid DNA was incubated in 100 µlof 800 mM hydroxylamine HCl (Sigma), 50 mM sodium phosphate (pH6.0), and 1 mM EDTA for 48 h at 37°C. The mutagenized DNA wasrecovered in TE (10 mM Tris-HCl [pH 8.0], 1 mm EDTA) by repeateddilution and concentration cycles in a Centricon 30 ultrafiltrationcartridge (Amicon). Potential umuD' mutants were identified byintroducing the mutagenized plasmid DNA into the umu tester strainRW126 harboring the medium-copy-number umuC plasmid pRW124. Transformantswere selected on Luria-Bertani plates supplemented with spectinomycin(50 µg/ml) and ampicillin (100 µg/ml) and then restreaked witha sterile toothpick onto MacConkey galactose (1%) indicator platessupplemented with spectinomycin and ampicillin. After 10 daysof incubation at 37°C, colonies that produced less than half ofthe number of Gal⁺ papillae seen with the control strain were analyzed further byusing the qualitative His⁺ mutagenesis assay.

Qualitative mutagenesis assay. Assays were performed essentially as described previously (41). Aliquots (1 ml) from a fresh overnight culture were centrifugedand resuspended in an equal volume of SM buffer (23). The abilityof particular plasmid-bearing strains to promote Umu-dependentSOS mutator activity in the absence of exogenous DNA damage wasjudged by plating 100-µl aliquots on Davis and Mingioli minimalagar plates supplemented with a trace amount of histidine (1 µg/ml)(3). Umu-dependent, chemically induced mutagenesis was determinedessentially as described above, except that 1 µl of methyl methanesulfonate(MMS) (Sigma) was applied to a small sterile disk in the centerof the plate. Both spontaneously arising and MMS-induced His⁺ mutants were scored after 4 days of incubation at 37°C.

Steady-state levels of wild-type and mutant UmuD' proteins. UmuD' protein was detected in whole-cell E. coli extracts by the Western-light chemiluminescence assay (Tropix, Bedford, Mass.),essentially as described previously (39). Briefly, whole-cellextracts from ~10⁸ cells were separated by electrophoresis in an 18% acrylamide-sodiumdodecyl sulfate gel. Proteins were transferred to an ImmobilonP (Millipore) support membrane and incubated overnight with a1:10,000 dilution of affinity-purified polyclonal UmuD' antiserum(10). After appropriate washes, the membranes were incubatedwith a 1:10,000 dilution of a goat anti-rabbit antibody conjugatedwith alkaline phosphatase (Bio-Rad). UmuD' was visualized afterthe membrane was incubated with the CPD-Star chemiluminescentsubstrate (Tropix) and exposed to X-ray film for an appropriateperiod of time. The relative level of UmuD' protein was obtainedby image analysis of films using NIH Image, version 1.59. In mostcases, values were obtained from multiple exposures so that thedesired bands were in the linear range of the film (39).

DNA sequence analysis. Plasmid DNA (pRW66 derivative and pRW124) was isolated from RW126 and transformed into TK614 [relevant genotype, recA⁺ lexA⁺ uvrA6 umuD77 hisG4(Oc)] (19), selecting for spectinomycin-resistant(pRW66) colonies and subsequently screening for ampicillin-sensitive(lacking pRW124) colonies. The pRW66 mutant phenotype was verifiedby using the qualitative His⁺ reversion assay described above. In all cases, plasmids thatfailed to promote any spontaneous or damage-induced mutagenesisin the recA718 strain (RW126) were unable to complement the chromosomallyencoded umuD77 allele in the recA⁺ background. By comparison, those plasmids that were able to promotemodest levels of Umu-dependent spontaneous or damage-induced mutagenesisdid complement the umuD77 allele (data not shown). The entireumuD' gene (including regulatory elements) in plasmid pRW66 (andmutant derivatives) was sequenced by Lark Sequencing TechnologiesInc. (Houston, Tex.), using standard dideoxy sequencing protocolsand four unique oligonucleotide primers spaced about 150 bp apart.

Subcloning of the previously identified chromosomal umuD1, umuD44, and umuD77 mutations into umuD'. The umuD44 and umuD77 mutations (2, 21) were subcloned into umuD' by isolating a ClaI-HindIII fragment from pGW2055 andpGW2051, respectively, and cloning the fragment into the similarlydigested umuD' vector pRW66. The umuD1 mutation (2, 21) wasgenerated in umuD' by synthesizing four synthetic oligonucleotidesthat, when annealed together, generated approximately 100 bp ofdouble-stranded DNA with EcoRI and ClaI ends. This fragment encodesthe wild-type umuDC promoter-operator regulatory sequences butalso introduces a unique NdeI restriction enzyme site at the 5'end of the mutant umuD'1 gene. Plasmid pRW368, which carries theentire umuD'1 gene, was constructed by ligating the syntheticoligonucleotides into the EcoRI-ClaI-digested vector pRW66.

Yeast two-hybrid interactions. The wild-type umuD' gene was obtained from plasmid pEC42 (11) and subcloned as an EcoRI-to-BglII fragment into the yeasttwo-hybrid vectors pGAD424 and pGBT9 (1) in such a way as tocreate in-frame fusions with the GAL4 activating domain and theGAL4 binding domain. These plasmids were designated pJM8 (pGAD424derivative) and pJM10 (pGBT9 derivative), respectively. Variousmutant umuD' genes were subcloned from pRW66 into pJM10 by usingthe unique ClaI and AgeI sites in the plasmid. The umuD' mutantderivatives of pJM10 were designated pJM50 to pJM60, and eachwas sequenced to ensure that it contained the correct allele ofumuD'. These mutant umuD' genes were then subcloned from the pJM10-derivativeplasmids, by utilizing the unique restriction enzymes sites forEcoRI and PstI, into pGAD424 and were designated pJM61-71. Thevarious wild-type and mutant pGAD424-umuD' derivatives were thencotransformed with the corresponding pGBT9-umuD' derivatives intoSaccharomyces cerevisiae SFY526 (1, 14, 17, 31). Transformantswere selected on synthetic medium lacking both leucine and tryptophan( $-$ leu $-$ trp) (32). These transformants, designated T13 (wild-typeumuD') or T125 to T135 (mutant umuD'), were inoculated into 5-mlcultures of liquid $-$ leu $-$ trp medium, supplemented with 40 µl ofYPD (2% peptone, 1% yeast extract, and 2% dextrose) per ml toenhance growth, and grown to mid-log phase (optical density at600 nm [OD₆₀₀], approximately 1.0). These cultures were then usedto perform liquid $beta$ -galactosidase assays. Briefly, 0.1 ml of culture,0.7 ml of Z buffer (60 mM Na₂HPO₄, 40 mM NaH₂PO₄, 10 mM KCl, and1 mM MgSO₄ [pH 7.0]), 50 µl of CHCl₃, and 50 µl of 0.1% sodiumdodecyl sulfate were vortexed for 30 s in a 1.5-ml microcentrifugetube. One hundred sixty microliters of ONPG solution (4 mg ofo-nitrophenylgalactoside per ml in 0.1 M phosphate buffer, pH7.0) was added, and the tube was vortexed. After 1 h of incubationat 30°C, the reactions were quenched by adding 0.4 ml of 1 M Na₂CO₃.The microcentrifuge tubes were then centrifuged for 10 min at14,000 rpm. The absorbance of 1 ml of the supernatant was thendetermined at 420 nm. $beta$ -Galactosidase units were calculated withthe following equation: 1,000(OD₄₂₀/t × V × OD₆₀₀) where t isthe time (in minutes) of incubation and V is the volume (in milliliters)of culture added to Z buffer (23).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Isolation of novel plasmid-encoded E. coli umuD' mutants. recA718 lexA(Def) strains that carry functional chromosomally encoded or plasmid-encoded umu genes normally exhibit modestUmu-dependent spontaneous mutator activity (15, 37, 41).This spontaneous mutator activity can be conveniently monitoredby assaying for the reversion of either the hisG4(Oc) or galK2(Oc)(26) mutations, the latter being monitored by a colorimetricpapillation assay. Since we were interested in specifically obtainingumuD' mutants, we utilized the compatible two-plasmid system thatwe have previously employed to identify umuC mutants (41). Inthis case, however, the umuD' plasmid, pRW66, was mutagenizedin vitro with hydroxylamine and introduced into the tester strainharboring the wild-type umuC plasmid pRW124.

Approximately 7,000 transformants were screened for reduced abilities to promote Umu-dependent spontaneous mutagenesis. Anumber of potential mutants were identified, of which 17 werechosen for further characterization. Subsequent DNA analysis revealedthat 3 of the mutants had been independently identified twice(Table 1), leaving 14 novel mutants. Of these mutants, two carriedpromoter mutations, three were nonsense mutations, and the remainingnine were missense mutations (Table 1). As would be expectedwith hydroxylamine mutagenesis, most of these changes correlatedwith a C $right-arrow$ T transition in either the coding or noncoding DNA strand.The exception was a G $right-arrow$ T transversion mutation found in the promoterregion of pRW66-42, which presumably arose spontaneously.

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TABLE 1. Promoter, nonsense, and missense umuD' mutants

Effects of plasmid-encoded umuD' mutations on the ability to promote SOS mutagenesis. Most of the plasmid-encoded umuD' mutations generated by the hydroxylamine treatment resulted in a strain that phenotypicallyexhibited 5 to 10% of the level of spontaneous SOS mutagenesisof the wild-type counterpart. The exceptions were plasmids thatexhibited approximately 20% (pRW66-13 [M61I] and pRW66-42 [ $-$ 35promoter mutation]) and approximately 50% (pRW66-19 [G64D]) ofthe spontaneous mutagenesis activity promoted by the wild-typeprotein. In contrast, many of the umuD' mutants were able to promoteMMS-induced mutagenesis, albeit to varying degrees (Table 1),indicating that under experimental conditions in which cells areexposed to continuous exogenous DNA damage, the mutant UmuD' proteinsare at least partially active. Such observations were confirmedby the fact that these mutants were able to complement a umuD77allele in a damage-induced recA⁺ lexA⁺ background (data not shown). The notable exceptions were plasmidswith ochre nonsense mutations {pRW66-31 [Q100X(Oc)] and pRW66-48[Q42X(Oc)]} and a plasmid with a missense mutation resulting inG129D (pRW66-20) that failed to promote any Umu-dependent mutagenesis(Table 1). The latter observation correlates with the fact thatthe Gly129 residue is critical to UmuD and UmuD' structure, asit is absolutely conserved in 14 of the UmuD/LexA homologs identifiedto date (28).

By comparison, the three chromosomal umuD alleles, umuD1 (P27S), umuD44 (G65R), and umuD77 (G92D) (which normally render UmuDnoncleavable and the strain concomitantly nonmutable [2, 19,21, 35]), all promoted significant levels of spontaneous andMMS-induced mutagenesis when cloned into umuD' (Table 1). Itwould appear, therefore, that these mutations affect the abilityof UmuD to undergo posttranslational processing but do not seemto have a major role in any subsequent activity of UmuD'.

Ability of mutant UmuD' proteins to form dimers: the two-hybrid assay. Since we believe that the mutagenically active form of UmuD' protein is a dimer, we were interested in determining if we couldcorrelate the level of mutagenesis promoted by each mutant proteinwith the extent to which it dimerized. One way to assess the strengthof such protein-protein interactions is to use the yeast two-hybridassay (7). Indeed, such an approach has been useful in determiningthe strength of UmuD-UmuD' interactions in vivo (18). We thereforesubcloned many of the umuD' missense mutations into the appropriatetwo-hybrid vectors and determined the ability of the mutant proteinsto interact with themselves. The two-hybrid fusion is at the N-terminalend of UmuD' (and mutant derivatives). Since the N-terminal tailof UmuD' makes extensive protein-protein contacts within the filamentdimer (28), as well as additional UmuD' promoters within thecrystallized extended UmuD' filament (28), we believe that simplesteric hindrance of the fusion protein will preclude such N-terminalinteractions. Any detectable protein-protein interactions are,therefore, thought to represent either molecular dimer (27)or filament dimer interactions through the short C-terminal extension(6, 28).

Based upon the levels of $beta$ -galactosidase expressed by these plasmids (Fig. 1A), it appeared that in the heterologous S. cerevisiaebackground, the mutational changes in 7 of the 11 mutant proteinsresulted in a protein with a reduced ability to interact withitself (Fig. 1A). In many cases, this inability to interact didindeed correlate with the level of spontaneous SOS mutagenesispromoted by the mutant proteins (Table 1). In general, thosemutants that produced $beta$ -galactosidase levels of $<=$ 1 Miller units(A50V, T51I) were generally the most deficient in spontaneousand damage-induced mutagenesis. One exception was the V130M mutation,which also produced $<=$ 1 Miller units but resulted in intermediatelevels of mutagenesis. We believe that the lower level of $beta$ -galactosidaseproduced by this mutant most likely reflects the inherent instabilityof the mutant protein (see below) rather than its inability todimerize. Mutants that produced ~2.3 to 5.3 Miller units of $beta$ -galactosidase(A50T, M61I, H82Y, G129S) all gave intermediate levels of spontaneousand induced mutagenesis, indicating that dimerization of thesemutants is impaired but not completely abolished. Further comparisonrevealed that two of the mutants, G64D and G92D, exhibited levelsof $beta$ -galactosidase somewhat similar to the wild-type construct(Fig. 1A) and both of these mutants gave high levels of spontaneousand induced mutagenesis. The G65R mutant and especially the G129Dmutant produced approximately four- to fivefold-higher levelsof $beta$ -galactosidase than the wild-type control. We interpret theseresults to indicate that both the G65R and G129D mutations increasethe ability of the mutant protein to dimerize. While the G65Rmutant was moderately proficient for mutagenesis, the G129D mutantwas completely defective for both spontaneous and damage-inducedmutagenesis.

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FIG. 1. Abilities of various missense mutants to interact with each other and wild-type UmuD'C. (A) Abilities of missense mutants to interact with themselves when expressed as two-hybrid fusion proteins in a heterologous S. cerevisiae background. This fusion is at the N-terminal end of UmuD' (and mutant derivatives) and presumably precludes any filament dimer interactions via the N-terminal extension of UmuD'. Any interactions are, therefore, thought to represent either molecular dimer or filament dimer interactions through the short C-terminal extension. The amount of $beta$ -galactosidase produced by each construct is expressed in Miller units, and the amino acid substitution in each mutant protein is indicated in single-letter amino acid code. (B) Effects on cellular mutagenesis of missense UmuD' mutants in JL852, a strain that constitutively expresses UmuD'C. As in panel A, the amino acid substitution in each mutant protein is indicated in single-letter amino acid code. WT is the level of mutagenesis in the presence of pRW66, while NP is the level of mutagenesis in its absence. Since none of the mutants appear to exhibit a dramatic dominant-negative phenotype, we assume that they are all recessive to the wild-type UmuD' protein.

Dominant/recessive nature of umuD' mutants. All of our initial mutational studies were performed in a $Delta$ umuDC background in which the mutant protein can interact onlywith itself. To determine if any of the missense mutants might,in fact, be dominant mutations, we introduced each of the missensemutations into E. coli JL852 (22). This strain expresses thechromosomally encoded UmuD and UmuC proteins, but since the RecA730protein constitutively mediates cleavage of UmuD (33, 39)the strain is, in fact, phenotypically UmuD'C. As a consequence,the strain exhibits a greatly elevated spontaneous mutation ratecompared to recA⁺ lexA(Def) cells, with approximately 210 His⁺ revertants appearing on each plate (Fig. 1B). Introduction ofthe wild-type UmuD' plasmid pRW66 into the cells increased thelevel to approximately 300 His⁺ mutants per plate, suggesting that the normal cellular levelsof UmuD'(C) are, in fact, limiting for optimal SOS-dependent spontaneousmutagenesis. Strictly speaking, dominance of a particular alleleover the wild-type gene should be determined when the cellularlevels of both proteins are approximately equal. In this experiment,however, the mutant proteins are expressed from a low-copy-numberplasmid while the wild-type UmuD'(C) proteins are chromosomallyexpressed. If any of the missense mutants are dominant negative,one would expect that they would reduce the level of spontaneousmutagenesis promoted by the chromosomally expressed UmuD'C complex.Despite the disparity in the levels of protein expression, analysisof the missense mutants identified here, including the G129D andG65R mutants (which we predict to at least homodimerize more efficientlythat the wild-type protein), revealed that they failed to significantlyreduce the level of spontaneous mutagenesis (Fig. 1B). These observationssuggest that under our experimental conditions, all of the mutantsare, in fact, recessive to the wild-type protein.

Steady-state levels of plasmid-encoded UmuD' mutants. Another obvious explanation for the inability of various umuD' mutants to promote mutagenesis is that the mutant protein isunstable and rapidly degraded in vivo. We have previously shownthat analysis of the steady-state levels of the Umu proteins isoften an accurate reflection of the relative stability of theprotein in vivo (10). In a $Delta$ umuDC background (as employed here),the wild-type UmuD' protein is relatively stable in vivo (10).Analysis of the steady-state levels of the missense mutant UmuD'proteins (with UmuC coexpressed in trans from pRW124) revealedthat most mutant proteins exhibited 30 to 100% of the steady-statelevel of the wild-type protein (Table 1). These observationssuggest that the various missense mutations have only negligibleto moderate effects on the stability of the mutant UmuD' proteinor that if they do affect its stability, such a phenotype is suppressedby coexpression with UmuC (Fig. 2). One obvious exception wasthe V130M protein, which was judged to be present at only 4% ofthe level of the wild-type protein.

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FIG. 2. Steady-state levels of missense mutants. The levels of UmuD' protein expressed from pRW66 and missense derivatives were analyzed in whole-cell E. coli extracts (RW126/pRW124) by chemiluminescence immunoassay. The amino acid substitution in each mutant protein is indicated in single-letter code above the individual lanes. The position of wild-type UmuD' is indicated on the left. As noted previously (21), some of the missense mutations result in a protein that migrates anomalously compared to the wild-type UmuD' protein.

Plasmids with nonsense mutations {pRW66-11 [Q36X(Am)], pRW66-31 [Q42X(Oc)], and pRW66-48 [Q100X(Oc)]} failed to yield a detectableUmuD' protein under a variety of conditions (data not shown).

We were also unable to detect the wild-type UmuD' protein expressed from plasmid pRW66-17 (which contains the $-$ 35 promotermutation TTGATA $right-arrow$ TTAATA). By comparison, however, we were ableto detect steady-state levels of the wild-type UmuD' protein expressedfrom the TTGATA $right-arrow$ TTTATA $-$ 35 promoter mutation in plasmid pRW66-42,but only if we increased the amount of cell extract normally appliedto the gel from 40 to 200 µg per track (data not shown).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Molecular basis for the phenotypes of E. coli umuD' mutants. (i) Promoter mutations. Two mutations that caused G $right-arrow$ A or G $right-arrow$ T changes in the $-$ 35 region of the umu promoter (TTGATA) were recovered. Previous studieshave suggested that this guanine residue within the $-$ 35 promoterregion is critical for efficient promoter activity (20). Consistentwith this suggestion, both mutations reduced the expression ofUmuD' (based upon the steady-state levels of UmuD' protein). Ourstudies demonstrated that the G $right-arrow$ A mutation caused the greatestphenotypic defect, while the G $right-arrow$ T mutation resulted in levels ofUmuD' that were apparently suboptimal for both spontaneous andMMS-induced mutagenesis (Table 1). Such observations are thereforeconsistent with mutational studies of the lacUV5 $-$ 35 promoterregion (20).

(ii) Nonsense mutations. Three nonsense mutations were recovered. Two were ochre stop codons that resulted in truncated UmuD' proteins of 16 and 74amino acids. Neither truncated protein was detected by Westernanalysis, suggesting either that the peptide fragments were notrecognized by the polyclonal UmuD' antiserum or that the peptideproduced was perhaps more rapidly degraded in vivo. In addition,neither mutant protein possessed any ability to promote eitherspontaneous or MMS-induced mutagenesis. The third nonsense mutationoccurred when the Glu36 codon was changed to an amber codon (Table1). As previously noted (41), strain RW126 carries the amber-suppressingmutation supE44, which inserts a Glu residue instead of terminatingprotein synthesis. Thus, if suppressed, the Q36X(Am) mutationshould, in fact, produce a full-length wild-type protein. Similarto previous results obtained with an amber mutation in umuC (41),the levels of wild-type UmuD' produced by the suppressed Q36X(Am)mutation were insufficient to promote spontaneous mutagenesisand were obviously limiting for MMS-induced mutagenesis (Table1).

(iii) Missense mutations. Most of the loss-of-function mutations identified here were missense mutations. We have also cloned the three previously identifiedchromosomal missense umuD mutations into umuD'. We were thereforeinterested in determining the molecular basis for the observedphenotypes of these novel umuD' mutants. This goal has been greatlyfacilitated by the recent determination of the three-dimensionalstructure of UmuD' (6, 27, 28). As noted in the introduction,based upon the crystallized structure of UmuD', we have previouslysuggested that the UmuD' protein might exist in several forms(27, 28). In this article we use the terms "molecular dimer"to indicate the protein-protein interactions between the two globulardomains of each UmuD' promoter, "filament dimer" for the interactionsbetween the long and short N- and C-terminal extensions, respectively,and "extended filaments" for the higher-order protein-proteininteractions observed between molecular and filament dimers.

The phenotypes of all of these missense umuD' mutants are therefore discussed in light of the effects that the changes mighthave on the structural integrity of the UmuD' protein. A wormdiagram of a UmuD' monomer and the position of the various missensemutations are shown in Fig. 3. Over half of the missense mutations(A50T, A50V, G64D, G65R, H82Y, G92D, and probably P27S) resultedin amino acid substitutions at residues that are solvent accessiblein a UmuD' monomer. The remaining mutations were at residues normallyburied within the body of the protein.

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FIG. 3. Worm diagram of a UmuD' promoter with mutations labeled. The N and C termini are labeled, as well as each of the mutations described in this study. Wild-type amino acids are identified as follows: hydrophobic residues are colored green, hydrophilic residues are colored yellow, and glycines are colored cyan. Each residue is labeled along with the change found in the mutant protein. This figure was generated with the program GRASP (24).

P27S(pRW368/umuD'1). The P27S mutant was generated by subcloning the umuD1 mutation into umuD'. The Pro27 residue is absolutely conserved in all10 UmuD-like proteins identified to date but is somewhat morevariable in the structurally related repressor proteins (28,40). While this mutation blocks cleavage of UmuD and resultsin a nonmutable phenotype (2, 21, 35), when cloned intoumuD' the mutant was moderately proficient at promoting both SOS-dependentspontaneous and MMS-induced mutagenesis (Table 1). Unfortunately,the P27S mutation is in a region of the UmuD' protein that isdisordered within the UmuD' crystal and cannot be accurately determined(27, 28). We speculate, however, that the phenotypic differencesseen when the mutation is expressed in UmuD' compared to UmuDsupport the hypothesis that the amino terminus of UmuD undergoesa conformational change during its conversion to the mutagenicallyactive UmuD' protein (6, 13, 28). We hypothesize that theP27S mutation somehow prevents the amino terminus of UmuD fromentering the catalytic active site of UmuD yet is less importantfor the subsequent activity of UmuD'.

A50T(pRW66-1/umuD'312), A50V(pRW66-52/umuD'313), and T51I(pRW66-38/umuD'314). The Ala50 residue is highly conserved in the UmuD-like mutagenesis proteins and is invariant with the exceptions of the Salmonellatyphimurium UmuD protein (which has a serine) (34, 38) andRulA (which has a histidine at residue 50) (36). Thr51 is alsohighly conserved in 9 of the 10 UmuD-like proteins. Interestingly,isoleucine is naturally found at this position in RulA (36).Ala50 and Thr51 are located at the N-terminal end of the first $beta$ -strand of UmuD' (Fig. 3). The Ala50 residue is about 3.5 to4.5 Å from Ala77, Ser76, and His47. It is relatively exposed tosolvent in the UmuD' monomer and is at the start of the turn thatcomes from the extended N terminus. Substituting a Val or Thrat this position puts a larger side chain in the space. Thr51points toward the N-terminal extended strand and is relativelyclose to Ile38 of the symmetrically related molecule in the UmuD'filament dimer (6, 28). Based upon the two-hybrid assay (Fig.1A), mutational changes at both Ala50 and Thr51 appear to affectthe ability of UmuD' to dimerize, the T51I mutation being moresevere than the A50V or A50T mutation. One hypothesis that explainsthese observations is that Thr51 may be important, along withAla50, in keeping the N terminus in an appropriate orientationfor filament dimer formation (6, 28). While not at the filamentdimer interface per se, we hypothesize that the defects associatedwith the T51I, A50V, and A50T mutations result from a reducedability of the mutant proteins to form filament dimers.

M61I(pRW66-13/umuD'315). The Met61 residue is conserved in virtually all UmuD-like mutagenesis proteins and repressor proteins (13 of 14 homologs),with the only exception being the bacteriophage P1 HumD protein,which has a histidine at the corresponding position (40). Met61is juxtaposed to Ser60 of the catalytic active site and is normallyburied within the body of the protein at the end of the catalyticcrevice (Fig. 4). Interestingly, the M61I substitution would createa hole, which we speculate that Ile85 may move to fill. This,in turn, could pull on the $beta$ -strand to which it is attached andthereby affect the filament dimer interface (Fig. 5) (6, 28).The M61I protein did not appear to dimerize quite as efficientlyas the wild-type protein and exhibited intermediate levels ofspontaneous SOS mutagenesis but normal levels of damage-inducedmutagenesis. Thus, the mild phenotype of the mutant appears tobe suppressed in damaged cells, presumably because of interactionsbetween the M61I mutant protein and activated RecA in vivo.

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FIG. 4. Surface representation of the UmuD' promoter. This orientation is approximately the same as that of the worm diagram of Fig. 3. The surface areas of residues involved in the molecular dimer interface (27, 28) are colored blue, except Gly92, which is colored red. The surface areas of residues that were mutated, other than Gly92, are colored green. Also seen in this view are Met61, Ala50, and Thr51. This figure was generated with the program GRASP (24).

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FIG. 5. Position of UmuD' mutants in a filament dimer. (A) Overall view of a UmuD' filament dimer. The view presented here is similar to that previously reported (28) and is shown for orientation purposes. One promoter is colored magenta, while the other is peach. (B) Close-up of the positions of the various UmuD' mutants and their locations with respect to the filament dimer interface. This view is identical to that of panel A. The side chains of the mutant residues are colored violet. Although the mutant residues are found in each protomer, for the sake of clarity only the mutant residues in the peach-colored protomer are identified. This figure was generated with the program GRASP (24).

G64D(pRW66-19/umuD'316). The G64D mutation also resulted in a mild phenotype, with approximately half the normal levels of spontaneous and MMS-inducedmutagenesis, and appeared to interact with itself to the sameextent as the wild-type protein. Gly64 is located in the short3₁₀ helix of UmuD' and is variable among UmuD-like proteins. Thisresidue is on the surface of the UmuD' protein and would be predictedto be in close proximity to the carboxyl-terminal tail of anotherpromoter in the filament dimer (Fig. 5). Presumably, the G64Dmutation moderately affects filament dimer formation, but as withthe M61I mutation, this effect is suppressed in a damaged cell,where we hypothesize that activated RecA acts as a scaffold tocorrectly position UmuD' for its subsequent role in translesionreplication (28).

G65R(pRW356/umuD'44). The G65R mutation was originally identified on the basis of its nonmutable phenotype when expressed in UmuD (2, 19, 21).In contrast, however, when subcloned into umuD', G65R can apparentlypromote significant levels of spontaneous and damage-induced mutagenesis(Table 1). Clearly, such a mutational change has dramatic andspecific effects on the ability of E. coli UmuD to undergo posttranslationalprocessing but much less effect on the subsequent mutagenic functionof UmuD'. The G65R residue is solvent exposed and is located inthe short 3₁₀ helix of UmuD' (Fig. 3 and 5). The C $alpha$ of Gly65 is~4 Å from the N $zeta$ of Lys136 in the same molecule and ~5 Å fromthe N $zeta$ of Lys136 of the symmetrically related filament dimer molecule(Fig. 5). Thus, one hypothesis to explain the defect in mutagenesisof the G65R UmuD' substitution is that it results in a positivelycharged area that subsequently affects efficient filament dimerformation.

H82Y(pRW66-30/umuD'305). The His82 residue is highly conserved in 7 of the 10 UmuD-like proteins. This residue is located on a ridge on the surfaceof UmuD', and we have previously hypothesized that it could makecontact with the amino-terminal tail of another promoter in theextended UmuD' filament (28). His82, like Gly64 and Gly65, isalso in the vicinity of the C terminus of a filament dimer mate(Fig. 5), but at its closest approach of 9 to 10 Å, it would beless likely to affect filament dimer formation. Either way, theH82Y substitution appears to result in a more severe defect thanG64D, as both spontaneous and MMS-induced mutagenesis rates werelower than those seen with the G64D substitution.

G92D(pRW358/umuD'77). Like the G65R mutation, the G92D mutation was originally identified on the basis of its nonmutable phenotype when expressedin UmuD (2, 19, 21). The molecular basis for this phenotypeis not immediately clear, as two structurally related proteins(LexA and bacteriophage 434 CI) have an aspartate at a positionequivalent to residue 92 (21, 28). The G92D residue is foundat the crystallized molecular dimer interface of UmuD' (Fig. 4).The G92D mutant was phenotypically indistinguishable from wild-typeUmuD', and had we not subcloned the mutation from umuD77, thischange would not have been identified in our colorimetric screenfor loss-of-function umuD' mutants. If, however, UmuD and UmuD'have the same general structure, as is now hypothesized (6),one could easily explain the nonmutable phenotype of UmuD G92Dby the fact that it might favor molecular dimer formation. Suchan interaction is predicted to occlude the catalytic active siteof UmuD and thereby exclude the possibility of UmuD cleavage (27).

G129D(pRW66-20/umuD'318), G129S(pRW66-44/umuD'317), and V130M(pRW66-18/umuD'319). Residues 129 and 130 are highly conserved in all of the structurally related proteins. Gly129 is invariant in both the UmuD-likemutagenesis proteins and the LexA and CI repressor proteins (28,40); Val130 is strictly conserved in the mutagenesis proteinbut not the repressor proteins. Interestingly, two mutations wererecovered at residue 129. Both substitutions dramatically reducethe ability of the mutant protein to perform both spontaneousand MMS-induced mutagenesis (Table 1). The G129D substitutionis also unique in that the same substitution renders UmuD noncleavable(2). Both the Gly129 and Val130 residues are found in a tightlypacked area in the last $beta$ -strand of UmuD' (Fig. 3). Indeed, Gly129is packed closely (less than 4Å away) to the backbone of residuesAsp75 and Ser76, and any side chain would impinge on these residues(Fig. 5). Glycine is normally invariant at position 129, as itis presumably the only amino acid small enough to fit into theavailable space. Substitution with either serine or aspartatepresumably affects the overall structure of UmuD', but these changeslead only to a modest increase in susceptibility to proteolysis.In contrast, they clearly have dramatic effects on the mutantprotein's ability to perform mutagenesis functions. Based uponthe two-hybrid assay, it appeared that the G129D mutant proteinis very efficient at forming dimers, presumably because the mutationsomehow affects filament dimer formation, but we cannot excludethe possibility that it also affects the molecular dimer. As notedfor the G92D mutation, if G129D does promote molecular dimerization,an inability of the UmuDG129D molecular dimer to dissociate mightexplain why the UmuDG129D protein is rendered noncleavable (2).

The V130M mutant performs mutagenesis functions moderately efficiently, but this mutation dramatically increases the susceptibilityof the protein to proteolysis (Fig. 2). Val130 is close to thevery C terminus of the symmetrically related filament dimer moleculeand is about 4 Å away from Asp84, Ala80, and Ile78 (Fig. 5). Inthe case of the V130M mutant protein, we hypothesize that thedefect in mutagenesis functions is more likely attributed to theinstability of the mutant protein than to any gross defect infunction.

Concluding remarks. Based upon the crystal structure of UmuD' (27, 28), we hypothesized that UmuD' might interact with itself in two ways:by the formation of a molecular dimer and by the formation ofa filament dimer. The filament dimer gained its name from theextended filament structures seen in the UmuD' crystal (27,28) as well as the multimeric (dimer, tetramer, hexamer) complexesseen at physiological concentrations in solution (28). Theseobservations suggested to us that both dimer interactions occurin the crystal and in solution. Very recently, Ferentz et al.(6) reported that they see strong nuclear overhauser effectsacross the carboxyl termini of UmuD', concluding that only thefilament dimer exists in solution. Indeed, filament dimer interactionappears to be important for the in vivo mutagenesis-promotingactivity of UmuD', as N-terminal and C-terminal deletion mutantsof UmuD' that exhibit reduced abilities to form multimeric complexesare also rendered phenotypically nonmutable (28). At present,we cannot rule out the possibility that a molecular dimer alsoexists, however, as the C-terminal deletion mutant (28) which,based upon the NMR-derived structure of UmuD' would be predictedto be unable to form a filament dimer, still apparently formsa chemically cross-linkable dimer (unpublished observations).What is clear, however, is that our screen for loss-of-functionumuD' mutants appears to yield predominantly filament dimer mutants.Based upon these observations, it would seem that mutations whichdisrupt the UmuD' filament dimer have a significant effect onthe ability of the mutant protein to promote mutagenesis, whereasthose at the putative molecular dimer interface are much lesspronounced.

We previously hypothesized that, as part of the mutagenic process, a RecA nucleoprotein filament would act as a scaffold forthe assembly of UmuD' filaments (28). Further support for sucha model comes from our observations that many of the loss-of-functionmutants were defective for spontaneous mutagenesis but that underconditions of DNA damage, where one would predict more extensiveRecA nucleoprotein filament formation, the phenotypes of manyUmuD' mutants were much less pronounced. To explain such observations,we favor the hypothesis that the various UmuD' mutants have reducedabilities to form UmuD' filament dimers per se, but by bindingto a RecA nucleoprotein filament the UmuD' filament dimer (andperhaps the higher-order filament structures) is sufficientlystabilized for error-prone repair to occur with roughly normalefficiency.

Further experiments with site-directed mutants of UmuD' are currently in progress to address the role of the molecular andfilament UmuD' dimers in damage-induced mutagenesis and how suchstructures might affect the ability of UmuD' to interact withUmuC, RecA, and, potentially, DNA polymerase III holoenzyme.

	ACKNOWLEDGMENT

We thank Brian Meffle for help with the yeast two-hybrid assays.

	FOOTNOTES

^* Corresponding author. Mailing address: Building 6, Room 1A13, NICHD, NIH, 9000 Rockville Pike, Bethesda, MD 20892-2725. Phone:(301) 496-6175. Fax: (301) 594-1135. E-mail: woodgate{at}helix.nih.gov.

Present address: Los Alamos National Laboratory, Los Alamos, NM 87545.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Bartel, P. L., and S. Fields. 1995. Analyzing protein-protein interactions using two-hybrid system. Methods Enzymol. 254:241-263[Medline].

2. Battista, J. R., T. Ohta, T. Nohmi, W. Sun, and G. C. Walker. 1990. Dominant negative umuD mutations decreasing RecA-mediated cleavage suggest roles for intact UmuD in modulation of SOS mutagenesis. Proc. Natl. Acad. Sci. USA 87:7190-7194[Abstract/Free Full Text].

3. Bridges, B. A., and R. Woodgate. 1985. Mutagenic repair in Escherichia coli: products of the recA gene and of the umuD and umuC genes act at different steps in UV-induced mutagenesis. Proc. Natl. Acad. Sci. USA 82:4193-4197[Abstract/Free Full Text].

4. Burckhardt, S. E., R. Woodgate, R. H. Scheuermann, and H. Echols. 1988. UmuD mutagenesis protein of Escherichia coli: overproduction, purification and cleavage by RecA. Proc. Natl. Acad. Sci. USA 85:1811-1815[Abstract/Free Full Text].

5. Donnelly, C. E., and G. C. Walker. 1992. Coexpression of UmuD' with UmuC suppresses the UV mutagenesis deficiency of groE mutants. J. Bacteriol. 174:3133-3139[Abstract/Free Full Text].

6. Ferentz, A. E., T. Opperman, G. C. Walker, and G. Wagner. 1997. Dimerization of the UmuD' protein in solution and its implications for regulation of SOS mutagenesis. Nat. Struct. Biol. 4:979-983[Medline].

7. Fields, S., and O. K. Song. 1989. A novel genetic system to detect protein-protein interactions. Nature 340:245-246[Medline].

8. Fijalkowska, I. J., R. L. Dunn, and R. M. Schaaper. 1997. Genetic requirements and mutational specificity of the Escherichia coli SOS mutator activity. J. Bacteriol. 179:7435-7445[Abstract/Free Full Text].

9. Frank, E. G., D. G. Ennis, M. Gonzalez, A. S. Levine, and R. Woodgate. 1996. Regulation of SOS mutagenesis by proteolysis. Proc. Natl. Acad. Sci. USA 93:10291-10296[Abstract/Free Full Text].

10. Frank, E. G., M. Gonzalez, D. G. Ennis, A. S. Levine, and R. Woodgate. 1996. In vivo stability of the Umu mutagenesis proteins: a major role for RecA. J. Bacteriol. 178:3550-3556[Abstract/Free Full Text].

11. Frank, E. G., J. Hauser, A. S. Levine, and R. Woodgate. 1993. Targeting of the UmuD, UmuD' and MucA' mutagenesis proteins to DNA by RecA protein. Proc. Natl. Acad. Sci. USA 90:8169-8173[Abstract/Free Full Text].

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Appl. Environ. Microbiol.	Infect. Immun.	Eukaryot. Cell
Mol. Cell. Biol.	J. Virol.	Microbiol. Mol. Biol. Rev.

1.	Bartel, P. L., and S. Fields. 1995. Analyzing protein-protein interactions using two-hybrid system. Methods Enzymol. 254:241-263[Medline].
2.	Battista, J. R., T. Ohta, T. Nohmi, W. Sun, and G. C. Walker. 1990. Dominant negative umuD mutations decreasing RecA-mediated cleavage suggest roles for intact UmuD in modulation of SOS mutagenesis. Proc. Natl. Acad. Sci. USA 87:7190-7194[Abstract/Free Full Text].
3.	Bridges, B. A., and R. Woodgate. 1985. Mutagenic repair in Escherichia coli: products of the recA gene and of the umuD and umuC genes act at different steps in UV-induced mutagenesis. Proc. Natl. Acad. Sci. USA 82:4193-4197[Abstract/Free Full Text].
4.	Burckhardt, S. E., R. Woodgate, R. H. Scheuermann, and H. Echols. 1988. UmuD mutagenesis protein of Escherichia coli: overproduction, purification and cleavage by RecA. Proc. Natl. Acad. Sci. USA 85:1811-1815[Abstract/Free Full Text].
5.	Donnelly, C. E., and G. C. Walker. 1992. Coexpression of UmuD' with UmuC suppresses the UV mutagenesis deficiency of groE mutants. J. Bacteriol. 174:3133-3139[Abstract/Free Full Text].
6.	Ferentz, A. E., T. Opperman, G. C. Walker, and G. Wagner. 1997. Dimerization of the UmuD' protein in solution and its implications for regulation of SOS mutagenesis. Nat. Struct. Biol. 4:979-983[Medline].
7.	Fields, S., and O. K. Song. 1989. A novel genetic system to detect protein-protein interactions. Nature 340:245-246[Medline].
8.	Fijalkowska, I. J., R. L. Dunn, and R. M. Schaaper. 1997. Genetic requirements and mutational specificity of the Escherichia coli SOS mutator activity. J. Bacteriol. 179:7435-7445[Abstract/Free Full Text].
9.	Frank, E. G., D. G. Ennis, M. Gonzalez, A. S. Levine, and R. Woodgate. 1996. Regulation of SOS mutagenesis by proteolysis. Proc. Natl. Acad. Sci. USA 93:10291-10296[Abstract/Free Full Text].
10.	Frank, E. G., M. Gonzalez, D. G. Ennis, A. S. Levine, and R. Woodgate. 1996. In vivo stability of the Umu mutagenesis proteins: a major role for RecA. J. Bacteriol. 178:3550-3556[Abstract/Free Full Text].
11.	Frank, E. G., J. Hauser, A. S. Levine, and R. Woodgate. 1993. Targeting of the UmuD, UmuD' and MucA' mutagenesis proteins to DNA by RecA protein. Proc. Natl. Acad. Sci. USA 90:8169-8173[Abstract/Free Full Text].
12.	Friedberg, E. C., G. C. Walker, and W. Siede. 1995. DNA repair and mutagenesis. American Society for Microbiology, Washington, D.C.
13.	Guzzo, A., M. H. Lee, K. Oda, and G. C. Walker. 1996. Analysis of the region between amino acids 30 and 42 of intact UmuD by a monocysteine approach. J. Bacteriol. 178:7295-7303[Abstract/Free Full Text].
14.	Hill, J., K. A. G. Donald, and D. E. Griffiths. 1991. DMSO-enhanced whole cell yeast transformation. Nucleic Acids Res. 19:5791[Free Full Text].
15.	Ho, C., O. I. Kulaeva, A. S. Levine, and R. Woodgate. 1993. A rapid method for cloning mutagenic DNA repair genes: isolation of umu-complementing genes from multidrug resistance plasmids R391, R446b, and R471a. J. Bacteriol. 175:5411-5419[Abstract/Free Full Text].
16.	Isackson, P. J., and K. P. Bertrand. 1985. Dominant negative mutations in the Tn10 tet repressor: evidence for use of the conserved helix-turn-helix motif in DNA binding. Proc. Natl. Acad. Sci. USA 82:6226-6230[Abstract/Free Full Text].
17.	Ito, H., Y. Fukuda, K. Murata, and A. Kimura. 1983. Transformation of intact yeast cells treated with alkali cations. J. Bacteriol. 153:163-168[Abstract/Free Full Text].
18.	Jonczyk, P., and A. Nowicka. 1996. Specific in vivo protein-protein interactions between Escherichia coli SOS mutagenesis proteins. J. Bacteriol. 178:2580-2585[Abstract/Free Full Text].
19.	Kato, T., and Y. Shinoura. 1977. Isolation and characterization of mutants of Escherichia coli deficient in induction of mutations by ultraviolet light. Mol. Gen. Genet. 156:121-131[Medline].
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