Mutations Affecting the Ability of the Escherichia coli UmuD' Protein To Participate in SOS Mutagenesis

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Journal of Bacteriology, January 1999, p. 177-185, Vol. 181, No. 1
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Mutations Affecting the Ability of the Escherichia coli UmuD' Protein To Participate in SOS Mutagenesis

Toshihiro Ohta,¹^, Mark D. Sutton,¹ Angelina Guzzo,¹ Shannon Cole,¹ Ann E. Ferentz,² and Graham C. Walker¹^,^*

Department of Biology, Massachusetts Institute of Technology, Cambridge, Massachusetts 02139,¹ and Department of Biological Chemistry and Molecular Pharmacology, Harvard Medical School, Boston, Massachusetts 02115²

Received 13 August 1998/Accepted 23 October 1998

	ABSTRACT

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The products of the SOS-regulated umuDC operon are required for most UV and chemical mutagenesis in Escherichia coli, a processthat results from a translesion synthesis mechanism. The UmuDprotein is activated for its role in mutagenesis by a RecA-facilitatedautodigestion that removes the N-terminal 24 amino acids. A previousgenetic screen for nonmutable umuD mutants had resulted in theisolation of a set of missense mutants that produced UmuD proteinsthat were deficient in RecA-mediated cleavage (J. R. Battista,T. Ohta, T. Nohmi, W. Sun, and G. C. Walker, Proc. Natl. Acad.Sci. USA 87:7190-7194, 1990). To identify elements of the UmuD'protein necessary for its role in translesion synthesis, we beganwith umuD', a modified form of the umuD gene that directly encodesthe UmuD' protein, and obtained missense umuD' mutants deficientin UV and methyl methanesulfonate mutagenesis. The D39G, L40R,and T51I mutations affect residues located at the UmuD'₂ homodimerinterface and interfere with homodimer formation in vivo. TheD75A mutation affects a highly conserved residue located at oneend of the central strand in a three-stranded $beta$ -sheet and appearsto interfere with UmuD'₂ homodimer formation indirectly by affectingthe structure of the UmuD' monomer. When expressed from a multicopyplasmid, the L40R umuD' mutant gene exhibited a dominant negativeeffect on a chromosomal umuD⁺ gene with respect to UV mutagenesis, suggesting that the mutationhas an effect on UmuD' function that goes beyond its impairmentof homodimer formation. The G129D mutation affects a highly conservedresidue that lies at the end of the long C-terminal $beta$ -strand andresults in a mutant UmuD' protein that exhibits a strongly dominantnegative effect on UV mutagenesis in a umuD⁺ strain. The A30V and E35K mutations alter residues in the N-terminalarms of the UmuD'₂ homodimer, which are mobile insolution.

	INTRODUCTION

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The gene products of the umuDC operon play important roles in the ability of Escherichia coli to tolerate damage to its DNA(10, 17, 30, 35, 36, 41). umuDC mutants were originallyidentified by screening directly for derivatives of E. coli thatare nonmutable by treatment with UV and various other chemicals(13, 32). Mutagenesis by such agents occurs as the resultof a translesion synthesis mechanism in which an incorrect nucleotideis inserted opposite the lesion and the chain is then subsequentlyextended (10, 24, 26, 33, 38).

Expression of the umuDC gene products is elaborately regulated, both transcriptionally and posttranslationally. The umuDCoperon is expressed at a low basal level and is induced in responseto DNA damage (1) as part of the cellular SOS response (10,14, 30, 35, 37). A cell's attempts to replicate damagedDNA generate regions of single-stranded DNA, which then permitthe formation of RecA nucleoprotein filaments (RecA*). Interactionof LexA with RecA* then facilitates a latent capacity of LexAto autodigest. The resulting proteolytic inactivation of LexAleads to increased levels of expression of the umuDC operon andother LexA-repressed loci. The full-length UmuD protein that resultsfrom translation of the umuD gene is inactive in mutagenesis (19)and is converted to the form that is active in mutagenesis, UmuD',by RecA*-mediated cleavage (5, 19, 27). This cleavage ismechanistically similar to the RecA*-mediated cleavage of LexA(16) and results in the removal of the N-terminal 24 amino acidsof UmuD. Until recently, it appeared that intact UmuD was simplyan inactive precursor of UmuD' with respect to SOS mutagenesis.However, recent evidence suggests the possibility that UmuD, actingtogether with UmuC, may play a role that is functionally equivalentto a eukaryotic DNA damage checkpoint control system by regulatingprogression through the cell cycle after DNA damage (20, 21).Both UmuD and UmuD' form homodimers (40), and the UmuD-UmuD'heterodimer is more stable than either of the homodimers (2).The three dimeric forms of the umuD gene product differ from oneanother with respect to their susceptibility to specific cytoplasmicproteases (8). The UmuD'₂ homodimer interacts with UmuC toform a UmuD'₂C complex (4). After UmuD is cleaved to generateUmuD', the UmuD' and UmuC proteins participate in translesionsynthesis (24, 26, 33) and may also play a role in modulatingrecombinational repair of damaged DNA (3, 31).

The crystal structure of the UmuD' protein was recently determined, and the UmuD' monomer was found to consist of a globularC-terminal domain with an extended N-terminal region (22). Inthe crystal structure that was determined, the UmuD' monomerswere arranged in a filament in which there were two differentinterfaces between UmuD monomers, one rich in aliphatic residuesthat involves interactions between the C termini (referred toby Peat et al. [22, 23] as the filament dimer interface) andone rich in aromatic residues (referred to by Peat et al. [22,23] as the molecular dimer interface). Nuclear magnetic resonance(NMR) analyses of the UmuD'₂ homodimer in solution (7) haveindicated that the actual homodimer interface is the one involvingcontacts between the C termini as well as interactions involvingN41 and L44 (using the same numbering system as for intact UmuD)rather than the interface rich in aromatic residues that was originallyassigned on the basis of the crystallographic analyses. No evidencewas seen in the NMR studies (7) for the UmuD filaments thathave been hypothesized to be important for the role of UmuD' inmutagenesis (22, 23). Structural information is not yet availablefor the UmuD₂ homodimer, but cross-linking studies of monocysteinederivatives of UmuD (15) are consistent with the UmuD₂ homodimerinterface resembling the interface of the UmuD'₂ homodimer. However,the UmuD'₂ and UmuD₂ homodimers differ in other respects. Forexample, monocysteine substitutions at positions 37 and 38 seemto be particularly well positioned to form disulfide bonds acrossthe interface of the UmuD₂ homodimer (11), while the N-terminalarms that contain the residues at positions 37 and 38 are freein solution in the UmuD'₂ homodimer (7).

As part of an effort to understand the mechanism by which the umuD gene product exerts its biological roles, we had previouslyscreened for umuD mutants that were defective in their abilityto participate in SOS mutagenesis (2). However, the mutantsobtained in that screen were found to produce derivatives of UmuDthat were deficient in their ability to undergo the RecA*-facilitatedautodigestion that gives rise to UmuD', the form active in mutagenesis.Earlier examples of mutants of this class had been obtained byaltering the Ser60 and Lys97 residues of UmuD (19), which playroles in UmuD cleavage that are analogous to those played by Ser119and Lys156 in LexA cleavage (29). To gain insights into whichresidues of UmuD' are required for its actual role in UV mutagenesis,we adopted an alternative strategy, namely mutagenizing a modifiedform of the umuD gene that directly encodes UmuD' (19) and screeningfor umuD' mutants with deficiencies in UV mutagenesis. While thispaper was under review, a related study in which umuD' mutantswere identified on the basis of their deficiencies in promotingthe umuD'C-dependent spontaneous mutagenesis observed in a lexA(Def)recA718 mutant was reported (18).

	MATERIALS AND METHODS

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Bacterial strains and plasmids. The bacterial strains and the plasmid used in this study have been described previously. E. coli GW3200 (6) is a umuD44derivative of AB1157 (thr-1 leu-6 proA2 hisG4 thi-1 argE3 lacY1galK2 ara-14 xyl-5 mtl-1 tsx-33 rpsL31 supE44). GW8025 (21)is a lexA300(Def)::spc $Delta$ (umuDC)595::cat derivative of GW1000 [recA441sulA11 $Delta$ lacU169 thr-1 leu-6 hisG4 argE3 ilv(Ts) galK2 rpsL31].The plasmid pGW2122 (19) carries the umuD' gene under the controlof the umuDC promoter. pGW2122 was constructed from the correspondingumuD⁺ plasmid pGW2020 (19) by using site-directed oligonucleotidemutagenesis to remove the nucleotides that encode amino acids2 to 24 ofUmuD.

Isolation of umuD' mutants. Plasmid pGW2122 DNA was purified by CsCl density gradient centrifugation and then treated with hydroxylamine as previouslydescribed (2). Mutagenized plasmids were transformed into theumuD44 strain GW3200 (19), and the resulting transformants werescreened for failure to fully complement the deficiency of GW3200in UV-induced argE3 reversion to an Arg⁺ phenotype (argE3 $right-arrow$ Arg⁺ reversion). Screening was carried out by patching colonies ofGW3200 derivatives carrying the mutagenized plasmids in duplicateonto supplemented M9-glucose plates containing a trace of arginine(2), irradiating with a dose of 20 J of UV light/m² and then incubating at 37°C for 2 days before scoring for Arg⁺ papillae. For plasmids encoding UmuD' derivatives with deficienciesin UV mutagenesis, the umuD' coding region and the upstream regionwere determined by dideoxynucleotide sequencing (19). In addition,several umuD' mutants were isolated by site-directed oligonucleotidemutagenesis of pGW2122. All site-directed mutants were sequencedto confirm that the desired mutation had been successfullyintroduced.

UV and MMS mutagenesis. The methods used to determine the susceptibility of various strains to mutagenesis by UV light (6) and methyl methanesulfonate(MMS) (34) have been describedpreviously.

Measurements of UmuD' in vivo levels and UmuD'₂ homodimer formation. Levels of UmuD' in vivo were assessed by the following method. Overnight cultures of GW3200 bearing the mutant umuD' plasmidswere diluted 1:20 in M9 medium (39) supplemented with 0.1 mMCaCl₂, 2 mM MgSO₄, 0.2% glucose, 0.4% Casamino Acids, and 5 µgof thiamine per ml. At an optical density at 600 nm (OD₆₀₀) ofca. 0.4, the cells were UV irradiated at 20 J/m² after which they were grown at 37°C for 1 h. The cells were thenpelleted and resuspended in sodium dodecyl sulfate (SDS) samplebuffer (50 mM Tris-Cl [pH 6.8], 100 mM dithiothreitol, 2% SDS,0.2% bromophenol blue, 10% glycerol), and 0.1 OD₆₀₀ unit of cellswas subjected to electrophoresis on an SDS-15% polyacrylamidegel. The proteins were then transferred to a polyvinylidene difluoridemembrane (Immobilon-P). The membrane was incubated with affinity-purifiedantibodies raised against UmuD, and cross-reacting material wasvisualized by using chemiluminescence (Tropix). Homodimer formationwas measured in vivo by formaldehyde cross-linking (28). GW8025derivatives bearing the respective umuD'-expressing plasmids weregrown in LB medium (39) at 42°C to an OD₆₀₀ of ca. 0.8. Thecells were harvested and resuspended in 100 mM sodium phosphate,pH 6.8, and the OD₆₀₀ was adjusted to 0.5. Formaldehyde (Mallinckrodt)was added to a final concentration of 1%, and samples were incubatedat room temperature for 30 min. After incubation, the cells wereconcentrated by centrifugation, lysed by addition of SDS samplebuffer, and then subjected to electrophoresis and chemiluminescencedetection as describedabove.

	RESULTS

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Isolation and generation of umuD' mutants that are deficient in UV mutagenesis. To identify mutations that affected the ability of the UmuD' protein to participate in UV mutagenesis, the plasmid pGW2122(19), which carries a modified form of the umuD gene that directlyencodes UmuD', was mutagenized with hydroxylamine and transformedinto a umuD44 mutant. The resulting transformants were patchedon minimal medium containing a trace of arginine, irradiated withUV light, and then screened for their proficiency in UV mutagenesisby a papillation assay based on argE3 $right-arrow$ Arg⁺ reversion. After screening several thousand derivatives, we identified19 candidates that showed a significant reduction in the numberof UV-induced Arg⁺ papillae relative to that of the umuD44 derivative carrying theparental umuD' plasmid, pGW2122. Two of these grew slowly on supplementedminimal medium and were not characterized further, while restrictionendonuclease analysis of the plasmid in a third derivative showedclearly that it had undergone a deletion of part of the umuD'gene. The umuD' coding and upstream regions of the remaining 16plasmids were then sequenced, and the results are summarized inTable 1. Two independently isolated derivatives altered the $-$ 35region of the umuDC promoter from TTGATA to TTAATA, and a mutantcarrying this same promoter mutation was also isolated by McLeniganet al. (18) in a related study. The change of this criticalpromoter residue (25) severely reduces umuD' expression (18).Another plasmid altered the initial ATG codon of umuD', a changethat would prevent translation of the umuD' message. Two nonsensemutants were isolated, one with an ochre mutation affecting codon100 and the other with an amber mutation affecting codon 52. Sincethe strain employed in our study carries the supE44 amber suppressor,which would lead to a substitution of glutamine for tyrosine 52(12), it seems most likely that this substitution results inan inactive or unstable UmuD' protein.

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TABLE 1. DNA sequence changes of umuD' mutants

The remaining mutated plasmids carried missense alleles that affect the ability of the UmuD' protein to participate in UVmutagenesis. All caused single amino acid changes except for adouble mutation that affected two adjacent amino acids (S49N A50T).The A30V mutant was isolated twice independently, but the otherduplications in our collection of 16 mutants may not have beenindependent and are not listed in Table 1. As in our previousstudy (2), which also used hydroxylamine as a mutagen, themajority of the mutations resulted from G:C $right-arrow$ A:T transitions. Withthe exception of the G129D mutation, all of the mutations affectedamino acids in the N-terminal portion of the UmuD' protein. Byusing site-directed mutagenesis, a few mutations that affectedparticular residues in the C-terminal portion of UmuD were alsointroduced (Table 1). A mutation resulting in the L40R changewas also constructed because L40 is a highly conserved residuethat lies within the UmuD'₂ homodimer interface identified inour NMR studies (7).

Deficiencies of umuD' mutants in mutagenesis induced by UV light and MMS. Derivatives of the umuD44 strain GW3200 carrying the umuD' mutant plasmids described above were assayed for their abilitiesto be mutated in response to UV irradiation. Figure 1A comparesthe UV mutabilities of umuD44 derivatives carrying these missensemutant umuD' plasmids to that of a derivative carrying the parentalumuD' plasmid. All of the mutants isolated in our screen had significantdeficiencies in UV mutagenesis, with the G129D mutant being themost defective. Of the mutants constructed by site-directed mutagenesis,the L40R mutant had a severe deficiency in UV mutagenesis andthe D75A mutant also was very significantly impaired; the othersite-directed mutants showed less than a twofold reduction inUV mutagenesis (data not shown) and were not characterized further.These same derivatives were also tested for their ability to undergothe argE3 $right-arrow$ Arg⁺ reversion induced by the alkylating agent MMS (Fig. 2). The L40Rand G129D mutants showed the most severe deficiencies in MMS mutagenesis,with the D75A and T51I mutants showing the next most severe. Asmentioned above, one mutant umuD' plasmid encodes two mutations,S49N and A50T, and was substantially deficient in MMS mutagenesis(Fig. 2). From our data alone, it is not possible to assess therelative contributions of the two alterations of UmuD' towardsthe deficiency in MMS mutagenesis. However, in a related study,McLenigen et al. (18) isolated an A50T single mutant and foundthat it reduced MMS mutagenesis by less than a factor of two.Since we observed considerably more than a twofold reduction inMMS mutagenesis with the S49N A50T double mutant, the S49N alterationmust also result in a reduction in mutagenesis proficiency. Infact, it seems likely that the reason that this derivative wasdetected in our screen was because the S49N and the A50T mutationscombined to cause a phenotype that was readily detectable. Overall,the deficiencies of the mutant umuD' strains in UV mutagenesislargely paralleled their deficiencies in MMS mutagenesis.

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FIG. 1. Effect of plasmids carrying umuD' mutations on UV-induced (20 J/m²) reversion of argE3 $right-arrow$ Arg⁺ in an AB1157 umuD44 strain (GW3200) (A) and an isogenic umuD⁺ strain (AB1157) (B). UV mutability is expressed relative to the umuD44 strain carrying the umuD' plasmid pGW2122 (17.8 induced Arg⁺ revertants/10⁶ survivors) (A) and relative to the umuD⁺ strain AB1157 (8.3 induced Arg⁺ revertants/10⁶ survivors) (B).

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FIG. 2. Effect of plasmids carrying umuD' mutations on MMS-induced reversion of argE3 $right-arrow$ Arg⁺ in the AB1157 umuD44 strain, GW3200.

The plasmids producing umuD' derivatives that were significantly impaired in UV and MMS mutagenesis were also introduced intoan isogenic umuD⁺ strain to test whether the UmuD' proteins they encoded were capableof interfering with the UV mutagenesis that is dependent on thechromosomal copy of the umuD⁺ gene. As shown in Fig. 1B, the introduction of the umuD' derivative-producingplasmid into the umuD⁺C⁺ strain AB1157 substantially increases the level of UV mutagenesisthat is observed, a finding indicating that UmuD' is normallya limiting component for UV mutagenesis in UV-irradiated wild-typecells. In Fig. 1B, the level of UV mutagenesis observed with AB1157derivatives carrying the various mutant umuD' plasmids is expressedrelative to that observed with the umuD⁺ strain, AB1157. Only two alleles, those encoding the L40R andG129D changes, exhibited a dominant negative effect over the chromosomalumuD⁺ allele even though the mutant UmuD' derivatives were expressedat elevated levels from multicopy plasmids. Of the two, the G129D-encodingallele exhibited the strongest dominant negative effect. The somewhathigher level of UV mutagenesis observed in some other cases, forexample with the plasmid carrying the D39G-encoding allele, ispresumably due to the expression of elevated levels of a partiallyactive UmuD'protein.

In vivo levels of mutant UmuD' derivatives. One possible explanation for the lack of activity of some of the UmuD' mutants in UV and MMS mutagenesis could be that themutant proteins were misfolded or structurally unstable and thereforesubject to proteolytic degradation. To ascertain whether the UmuD'mutants were present at levels sufficient to promote induced mutagenesis,their steady-state levels were compared to that of the plasmid-encodedwild-type UmuD' in a lexA⁺ umuD44 strain (GW3200) following UV irradiation. No UmuD or UmuD'was detected in the umuD44 strain in the absence of a umuD-expressingplasmid (data not shown). Repeated analyses indicated that withthe exception of the mutants D39G and D75A and, possibly, T51I,all of the mutant UmuD' proteins were present at levels comparableto or greater than that of wild-type UmuD' (Fig. 3A).

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FIG. 3. The in vivo levels of the UmuD' mutants (A) and their ability to form UmuD' homodimers (B) were measured in crude lysates by using chemiluminescence immunodetection as described in Materials and Methods. (A) In vivo levels of the UmuD' mutants relative to that of wild-type UmuD' in a lexA⁺ strain (GW3200) following a 20-J/m² UV dose are shown. (B) The abilities of the various UmuD' mutants to be cross-linked as homodimers in vivo by formaldehyde are shown. The UmuD' mutant proteins were expressed constitutively because of the lexA(Def) allele in strain GW8025. The positions of the UmuD' monomer and UmuD'₂ homodimer are indicated.

As is evident from the cross-linking experiments described in the next section, a strikingly different result was obtainedwhen the levels of the mutant UmuD' proteins were measured ina lexA(Def) strain. In this case, the SOS regulon is constitutivelyderepressed due to disruption of the lexA gene encoding the repressorof the SOS regulon. Whereas the D39G and D75A mutant proteinswere barely detectable following UV irradiation of a lexA⁺ strain, they were nearly as abundant as wild-type UmuD' whenmeasured in a lexA(Def) strain (Fig. 3B). It is possible thatthe higher levels of RecA protein in the lexA(Def) strain areresponsible for the stabilization of the mutant proteins (9).These results suggest that the poor activity of the mutants D39G,D75A, and, possibly, T51I in UV and MMS mutagenesis is due, atleast in part, to their reduced abundance relative to that ofwild-type UmuD', whereas the poor mutability of the other UmuD'mutants is due to a specific biochemicaldefect.

Ability of the mutant UmuD' derivatives to form homodimers in vivo. In addition to their in vivo levels, another explanation for the poor mutability of some of the UmuD' mutants in UV and MMSmutagenesis could be that they have a defect in UmuD'₂ homodimerformation. To determine if any of the UmuD' mutants were poorlyactive in induced mutagenesis due to a defect in their abilityto form UmuD'₂ homodimers, we measured homodimerization in vivoby formaldehyde cross-linking. In these experiments, a lexA(Def)strain was used so that expression of the plasmid-encoded UmuD'mutants was constitutive. Whereas the A30V, E35K, S49N, A50T,and G129D derivatives were comparable to wild-type UmuD' withrespect to their ability to form homodimers, the D39G, L40R, T51I,and D75A derivatives were severely impaired in this regard (Fig.3B). Similar results were obtained when the plasmids carryingthe mutant umuD' alleles were examined in a lexA⁺ host in which umuD' expression had been induced by a 20-J/m² UV dose (data not shown), the only difference being that theD39G, T51I, and D75A derivatives were present at lower levelsin the UV-irradiated cells. In light of these results, the impairedabilities of the D39G, L40R, T51I, and D75A derivatives to participatein UV and MMS mutagenesis are likely due, at least in part, totheir reduced ability to form homodimers. With respect to themutants D39G and D75A, their severely reduced steady-state levelsrelative to that of wild-type UmuD' may be related to their reducedability to formhomodimers.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

By a combination of direct screening and site-directed mutagenesis, we have identified several missense umuD' mutants thatare deficient in their ability to participate in UV-induced mutagenesis.By starting with an altered umuD gene that directly encodes UmuD',we were able to obtain mutants that affect the role of UmuD' inUV mutagenesis rather than mutants that interfere with UV mutagenesisindirectly by causing deficiencies in the RecA*-facilitated cleavageof UmuD, as in our earlier study (2). All of the mutants thatwe characterized had deficiencies in MMS mutagenesis that werelargely similar to their deficiencies in UV mutagenesis, consistentwith the UmuD' protein playing similar mechanistic roles in themutagenesis induced by both of these agents. Our observation thatall of the mutants isolated by screening for deficiencies in UVmutagenesis were also deficient in MMS mutagenesis contrasts withthe situation described by McLenigan et al. (18). Their primaryscreen was for plasmid-borne alleles of umuD' that reduced thelevel of spontaneous mutagenesis observed in a lexA(Def) recA718 $Delta$ umuDC strain that expressed UmuC from a medium-copy-number plasmid.In their case, only some of the umuD' alleles that they identifiedexhibited substantial reductions in MMS mutagenesis; UV mutagenesiswas not examined. Taken together, these two studies suggest thatthere are elements of UmuD' structure that are important for theelevated umuD'C-dependent spontaneous mutation rate observed ina lexA(Def) recA718 genetic background that are unimportant, orof lesser importance, for the mutagenesis observed in wild-typecells whose DNA has been damaged by UV light orMMS.

Before discussing how particular amino acid changes might reduce the ability of the UmuD' protein to participate in UV andMMS mutagenesis, it is worth pointing out that a mutationallyinduced change might (i) alter the core structure of the protein,rendering it nonfunctional or unable to bind to other proteinsrequired for mutagenesis, or (ii) change the surface of the proteinin a region that is involved in interactions with other proteinsinvolved in the translesion synthesis mechanism that underliesSOS mutagenesis without substantially altering the overall structureof the protein. In some cases, a residue might be important forthe structural integrity of UmuD' and also lie on the surface,in which case either or both explanations for reduced functionalitywouldapply.

Four of the mutations that resulted in defective UV and MMS mutagenesis produced mutant UmuD' proteins that had severe deficienciesin their abilities to form homodimers in vivo as determined byformaldehyde cross-linking: D39G, L40R, T51I, and D75A (Fig. 4and 5). Three of these changes (D39G, L40R, and T51I) alter residuesthat are located at the homodimer interface that was identifiedby NMR studies of UmuD'₂ in solution (7) and are not near thehomodimer interface that had been assigned on the basis of crystallographicstudies (22, 23). Thus, these mutant proteins provide additionalsupport for our conclusion that the interface of the UmuD'₂ homodimerin solution is the one involving contacts between the C terminiand interactions involving N41 and L44 (7). As discussed below,the fourth alteration, D75A, appears to indirectly affect homodimerformation by causing a significant structural alteration of theUmuD' monomer that interferes with its ability to dimerize. Furthermore,our observation that the mutant UmuD' proteins displaying themost substantial reductions in homodimer formation in vivo alsoexhibited the lowest levels of UmuD' protein in UV-irradiatedlexA⁺ cells suggests that homodimer formation is an important factorin UmuD' stability in vivo.

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FIG. 4. Worm representation of the UmuD'₂ homodimer. Residues critical for UV mutagenesis are shown in red; those in pink are sites of missense mutations that caused less than a twofold reduction in UV mutagenesis.

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FIG. 5. Close-up view of the dimerization interface showing interactions of side chains that may be important for dimerization.

Although the UmuD'₂ homodimer interface in solution may not exactly match the interface seen in the crystal that is rich inaliphatic contacts and involves interactions between the C termini(the one originally designated the filament dimer [22, 23]),it nevertheless appears to be a good approximation of the UmuD'₂homodimer interface that exists in solution (7). Part of thisinterface consists of interactions between the $alpha$ -helices formedby residues 40 to 45 (Fig. 5). L40, the first amino acid of thishelix, makes hydrophobic contacts with L44 of the other monomerso that the L40R mutation would be expected to disrupt these contactsand interfere with homodimer formation. Similarly, it appearsthat the D39G change also directly affects the homodimer interfacesince D39 normally hydrogen bonds to the amide of D41 in the oppositemonomer. Residues 49 to 51 lie near the turn at residues 48 and49 that poises the 40 to 45 $alpha$ -helices so that they can interactwith each other across the dimerization interface. The hydroxylof T51 forms a hydrogen bond with the backbone carbonyl of H47that is important for this turn. Mutating this residue to I51would eliminate this bond and potentially be detrimental to thestructure.

It is interesting that although in vivo formaldehyde cross-linking analyses indicated that the L40R UmuD' derivative was impairedin UmuD'₂ homodimer formation to approximately the same extentas the D39G, T51A, and D75A derivatives and is present in thecells at a higher level, it was markedly less proficient in UVand MMS mutagenesis. This observation suggests that the L40R mutationhas an effect on UmuD' function that goes beyond its influenceon homodimer formation. This inference is additionally supportedby our observation that the L40R derivative was only one of twoumuD' mutants that, when expressed from a multicopy-number plasmid,exerted a dominant negative effect on a chromosomal umuD⁺ gene with respect to UV mutagenesis. Thus, some feature of thestructure of the L40R UmuD' derivative enables it to interferewith the function of a wild-typeprotein.

The D75A alteration apparently interferes with homodimer formation indirectly by affecting the structure of the UmuD' monomerand results in a UmuD' derivative that is strikingly unstablein a UV-irradiated lexA⁺ host. D75 is located at one end of the central strand in a three-stranded $beta$ -sheet (Fig. 4) and is highly conserved across the family ofmutagenesis and repressor proteins (10). Disruption of thisthree-stranded sheet by mutating D75 could prevent the proteinfrom folding correctly and make it highly susceptible to proteolysis.In addition, the D75 side chain normally forms a hydrogen bondwith the side chain of H47. A change of this residue to A75 wouldeliminate this interaction, which may be critical for holdingtogether another part of theprotein.

The G129D mutant protein, which was also identified by McLenigan et al. (18), is of particular interest because it is presentin cells at levels comparable to that of the parental UmuD' proteinyet is severely deficient in its ability to participate in UVand MMS mutagenesis. Furthermore, the G129D mutant was the onlyderivative identified in our study that exerted a strongly dominanteffect over a chromosomal umuD⁺ allele with respect to UV mutagenesis when it was expressed froma multicopy plasmid. Finally, the G129D mutant was identifiedin our earlier screen for umuD⁺ derivatives that were deficient in UV mutagenesis (2). Inthe context of the intact UmuD protein, the G129D mutation wasfound to cause a very severe defect in RecA*-mediated UmuD cleavageand to exert a strongly dominant negative effect on a chromosomalumuD⁺ allele with respect to UV mutagenesis (2). G129 is a criticalstructural residue, lying at the end of the long C-terminal $beta$ -strandand making hydrophobic contacts to residue V74 in the $beta$ -strandat positions 70 to 75 (Fig. 4). It is conserved across the familyof mutagenesis proteins and repressors (10). Mutating the glycineto an aspartic acid would be expected to disrupt this interaction,causing some perturbation of the structure. It is intriguing thatMcLenigan et al. (18) found that the G129D UmuD' derivativedid not exert a dominant negative effect on the elevated levelsof spontaneous mutagenesis observed in a recA730 mutant, a geneticbackground in which UmuD is constitutively cleaved to UmuD' inthe absence of exogenously induced DNA damage. One possible explanationis that there are requirements for UmuD' function for the elevatedspontaneous mutagenesis observed in a recA730 strain that arenot identical to those required for UV and MMS mutagenesis ina wild-type strain, a possibility consistent with the propertiesof certain of the mutants identified by McLenigan et al. (18).An alternative explanation would be that the G129D UmuD' derivativeinterferes with the RecA-mediated cleavage observed in a UV-irradiatedcell but not with the RecA-mediated cleavage that occurs in arecA730strain.

As discussed above, it appears that both the S49N and A50T mutations cause partial deficiencies in the ability of UmuD' toparticipate in UV and MMS mutagenesis. S49 and A50 are locatedimmediately next to the turn at residues 48 and 49 that positionsthe 40 to 45 $alpha$ -helices at the homodimer interface, yet they donot cause an obvious impairment in homodimer formation. It isinteresting that residues S49, A50, and T51 lie very near G129,with only residue D76 in between (Fig. 6). Thus, it seems thatthis region of UmuD' is a likely candidate for a binding sitefor another protein.

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FIG. 6. Space-filling model of the UmuD' dimer, rotated by 90° relative to the view shown in Fig. 4, and illustrating the spatial relationship of residues S49, A50, T51, S76, and G129.

Two of the most interesting mutants isolated in our screen for those deficient in UV mutagenesis were the ones that causethe A30V and E35K alterations in the N-terminal arms of the UmuD'₂homodimer. These arms have been shown to be mobile in solution(7). We have previously reported that derivatives of intactUmuD that carry monocysteine substitutions at positions 37 and38 can be cross-linked by a disulfide bond with very high efficiencyafter oxidation with I₂ (11), an observation suggesting that,in UmuD₂, at least residues at these positions on the arms areconstrained in a fashion that optimally positions them for rapiddisulfide bond formation across the homodimer interface when I₂is added. Taken together with our observation that amino acidsin the mobile N-terminal arms of UmuD' are important for UV mutagenesis,these observations suggest that at least one purpose of RecA*-mediatedcleavage of UmuD is to free up these arms so that they are ableto interact with another protein in a fashion that was not possiblewhile they were part of the UmuD₂ homodimer. It will be interestingto learn how the changes in protein structure that occur afterRecA*-mediated cleavage enable UmuD' to participate in the processof translesion synthesis that is currently being analyzed in vitro(26, 33, 38).

	ACKNOWLEDGMENTS

We thank the members of our laboratory, particularly Brad Smith, for their many helpful discussions and Leticia Vega and LisaLee for their assistance with the genetic screening. We also thankRoger Woodgate and his colleagues for sharing information withus in advance ofpublication.

This work was supported by Public Health Service grant CA21615 from the National Cancer Institute. A.E.F. was supported byan American Cancer Society postdoctoral fellowship and by theONR Science Scholar program at the Bunting Institute of RadcliffeCollege. A.G. was supported by a postdoctoral fellowship fromthe Medical Research Council of Canada. S.C. carried out her researchas part of the Undergraduate Research Opportunities Program (UROP)at the Massachusetts Institute ofTechnology.

	FOOTNOTES

^* Corresponding author. Mailing address: 68-633, Department of Biology, Massachusetts Institute of Technology, Cambridge, MA02139. Phone: (617) 253-6716. Fax: (617) 253-2643. E-mail: gwalker{at}mit.edu.

Present address: School of Life Science, Tokyo University of Pharmacy and Life Science, 1432-1 Horinouchi, Hachioji, Tokyo192-03,Japan.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Bagg, A., C. J. Kenyon, and G. C. Walker. 1981. Inducibility of a gene product required for UV and chemical mutagenesis in Escherichia coli. Proc. Natl. Acad. Sci. USA 78:5749-5753[Abstract/Free Full Text].

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. Boudsocq, F., M. Campbell, R. Devoret, and A. Bailone. 1997. Quantitation of the inhibition of Hfr x F $-$ recombination by the mutagenesis complex UmuD'C. J. Mol. Biol. 270:201-211[Medline].

4. Bruck, I., R. Woodgate, K. McEntee, and M. F. Goodman. 1996. Purification of a soluble UmuD'C from Escherichia coli: cooperative binding of UmuD'C to single-stranded DNA. J. Biol. Chem. 271:10767-10774[Abstract/Free Full Text].

5. 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].

6. Elledge, S. J., and G. C. Walker. 1983. Proteins required for ultraviolet light and chemical mutagenesis: identification of the products of the umuC locus of Escherichia coli. J. Mol. Biol. 164:175-192[Medline].

7. 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].

8. 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].

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

10. Friedberg, E. C., G. C. Walker, and W. Siede. 1995. DNA repair and mutagenesis. The American Society for Microbiology, Washington, D.C.

11. 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].

12. Inokuchi, H., F. Yamao, H. Sakano, and H. Ozeki. 1979. Identification of transfer tRNA suppressors in Escherichia coli. J. Mol. Biol. 132:649-662[Medline].

13. 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].

14. Koch, H. K., and R. Woodgate. 1998. The SOS response, p. 107-134. In J. A. Nickoloff, and M. F. Hoekstra (ed.), DNA damage and repair, vol. 1. DNA repair in prokaryotes and lower eukaryotes. Humana Press, Totowa, N.J.

15. Lee, M. H., T. Ohta, and G. C. Walker. 1994. A monocysteine approach for probing the structure and interactions of the UmuD protein. J. Bacteriol. 176:4825-4837[Abstract/Free Full Text].

16. Little, J. W. 1993. LexA cleavage and other self-processing reactions. J. Bacteriol. 175:4943-4950[Free Full Text].

17. Livneh, Z., O. Cohen-Fix, R. Skaliter, and T. Elizur. 1993. Replication of damaged DNA and the molecular mechanism of ultraviolet light mutagenesis. Crit. Rev. Biochem. Mol. Biol. 28:465-513[Medline].

18. McLenigan, M., T. S. Peat, E. G. Frank, J. P. McDonald, M. Gonzalez, A. S. Levine, W. A. Hendrickson, and R. Woodgate. 1998. Novel Escherichia coli umuD' mutants: structure-function insights into SOS mutagenesis. J. Bacteriol. 180:4658-4666[Abstract/Free Full Text].

19. Nohmi, T., J. R. Battista, L. A. Dodson, and G. C. Walker. 1988. RecA-mediated cleavage activates UmuD for mutagenesis: mechanistic relationship between transcriptional derepression and posttranslational activation. Proc. Natl. Acad. Sci. USA 85:1816-1820[Abstract/Free Full Text].

20. Opperman, T., S. Murli, and G. C. Walker. A DNA damage checkpoint control mechanism that regulates DNA synthesis and growth. Submitted for publication.

21. Opperman, T., S. Murli, and G. C. Walker. 1996. The genetic requirements for UmuDC-mediated cold sensitivity are distinct from those for SOS mutagenesis. J. Bacteriol. 178:4400-4411[Abstract/Free Full Text].

22. Peat, T. S., E. G. Frank, J. P. McDonald, A. S. Levine, R. Woodgate, and W. A. Hendrickson. 1996. Structure of the UmuD' protein and its regulation in response to DNA damage. Nature 380:727-730[Medline].

23. Peat, T. S., E. G. Frank, J. P. McDonald, A. S. Levine, R. Woodgate, and W. A. Hendrickson. 1996. The UmuD' protein filament and its potential role in damage-induced mutagenesis. Structure 4:1401-1412[Medline].

24. Rajagopalan, M., C. Lu, R. Woodgate, M. O'Donnell, M. F. Goodman, and H. Echols. 1992. Activity of the purified mutagenesis proteins UmuC, UmuD', and RecA in replicative bypass of an abasic DNA lesion by DNA polymerase III. Proc. Natl. Acad. Sci. USA 89:10777-10781[Abstract/Free Full Text].

25. Record, M. T., Jr., W. S. Reznikoff, M. L. Craig, K. L. McQuade, and P. J. Schlax. 1998. Escherichia coli RNA polymerase (E $sigma$ ⁷⁰) promoters, and the kinetics of the steps of transcription initiation, p. 792-821. In F. Neidhardt, R. Curtiss, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. Reznikoff, M. Riley, M. Schaecter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed., vol. 1. American Society for Microbiology, Washington, D.C.

26. Reuven, N. B., G. Tomer, and Z. Livneh. 1998. The mutagenesis proteins UmuD' and UmuC prevent lethal frameshifts while increasing base substitution mutations. Mol. Cell 2:191-199[Medline].

27. Shinagawa, H., H. Iwasaki, T. Kato, and A. Nakata. 1988. RecA protein-dependent cleavage of UmuD protein and SOS mutagenesis. Proc. Natl. Acad. Sci. USA 85:1806-1810[Abstract/Free Full Text].

28. Skare, J. T., B. M. Ahmer, C. L. Seachord, R. P. Darveau, and K. Postle. 1993. Energy transduction between membranes. TonB, a cytoplasmic membrane protein, can be chemically cross-linked in vivo to the outer membrane receptor FepA. J. Biol. Chem. 268:16302-16308[Abstract/Free Full Text].

29. Slilaty, S. N., and J. W. Little. 1987. Lysine-156 and serine-119 are required for LexA repressor cleavage: a possible mechanism. Proc. Natl. Acad. Sci. USA 84:3987-3991[Abstract/Free Full Text].

30. Smith, B. T., and G. C. Walker. 1998. Mutagenesis and more: umuDC and the Escherichia coli SOS response. Genetics 148:1599-1610[Abstract/Free Full Text].

31. Sommer, S., A. Bailone, and R. Devoret. 1993. The appearance of the UmuD'C protein complex in Escherichia coli switches repair from homologous recombination to SOS mutagenesis. Mol. Microbiol. 10:963-971[Medline].

32. Steinborn, G. 1978. Uvm mutants of Escherichia coli K12 deficient in UV mutagenesis. I. Isolation of uvm mutants and their phenotypical characterization in DNA repair and mutagenesis. Mol. Gen. Genet. 165:87-93[Medline].

33. Tang, M., I. Bruck, R. Eritja, J. Turner, E. G. Frank, R. Woodgate, M. O'Donnell, and M. F. Goodman. 1998. Biochemical basis of SOS-mutagenesis in Escherichia coli: reconstitution of in vitro lesion bypass dependent on the UmuD'₂C mutagenic complex and RecA protein. Proc. Natl. Acad. Sci. USA 95:9755-9760[Abstract/Free Full Text].

34. Walker, G. C. 1977. Plasmid (pKM101)-mediated enhancement of repair and mutagenesis: dependence on chromosomal genes in Escherichia coli K-12. Mol. Gen. Genet. 152:93-103[Medline].

35. Walker, G. C. 1984. Mutagenesis and inducible responses to deoxyribonucleic acid damage in Escherichia coli. Microbiol. Rev. 48:60-93[Free Full Text].

36. Walker, G. C. 1995. SOS-regulated proteins in translesion synthesis and mutagenesis. Trends Biochem. Sci. 10:416-420.

37. Walker, G. C. 1996. The SOS response of Escherichia coli, p. 1400-1416. In F. Neidhardt, R. Curtiss, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. Reznikoff, M. Riley, M. Schaecter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed., vol. 1. American Society for Microbiology, Washington, D.C.

38. Walker, G. C. 1998. Skiing the black diamond slope: progress on the biochemistry of translesion synthesis. Proc. Natl. Acad. Sci. USA 95:10348-10350[Free Full Text].

39. Walker, G. C., and P. P. Dobson. 1979. Mutagenesis and repair deficiencies of Escherichia coli umuC mutants are suppressed by the plasmid pKM101. Mol. Gen. Genet. 172:17-24[Medline].

40. Woodgate, R., M. Rajagopalan, C. Lu, and H. Echols. 1989. UmuC mutagenesis protein of Escherichia coli: purification and interaction with UmuD and UmuD'. Proc. Natl. Acad. Sci. USA 86:7301-7305[Abstract/Free Full Text].

41. Woodgate, R., and S. Sedgwick. 1992. Mutagenesis induced by bacterial UmuDC proteins and their plasmid homologues. Mol. Microbiol. 6:2213-2218[Medline].

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	ALL ASM JOURNALS

1.	Bagg, A., C. J. Kenyon, and G. C. Walker. 1981. Inducibility of a gene product required for UV and chemical mutagenesis in Escherichia coli. Proc. Natl. Acad. Sci. USA 78:5749-5753[Abstract/Free Full Text].
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.	Boudsocq, F., M. Campbell, R. Devoret, and A. Bailone. 1997. Quantitation of the inhibition of Hfr x F $-$ recombination by the mutagenesis complex UmuD'C. J. Mol. Biol. 270:201-211[Medline].
4.	Bruck, I., R. Woodgate, K. McEntee, and M. F. Goodman. 1996. Purification of a soluble UmuD'C from Escherichia coli: cooperative binding of UmuD'C to single-stranded DNA. J. Biol. Chem. 271:10767-10774[Abstract/Free Full Text].
5.	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].
6.	Elledge, S. J., and G. C. Walker. 1983. Proteins required for ultraviolet light and chemical mutagenesis: identification of the products of the umuC locus of Escherichia coli. J. Mol. Biol. 164:175-192[Medline].
7.	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].
8.	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].
9.	Frank, E. G., J. Hauser, A. S. Levine, and R. Woodgate. 1993. Targeting of the UmuD, UmuD' and MucA' mutagenesis proteins to DNA by the RecA protein. Proc. Natl. Acad. Sci. USA 90:8169-8173[Abstract/Free Full Text].
10.	Friedberg, E. C., G. C. Walker, and W. Siede. 1995. DNA repair and mutagenesis. The American Society for Microbiology, Washington, D.C.
11.	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].
12.	Inokuchi, H., F. Yamao, H. Sakano, and H. Ozeki. 1979. Identification of transfer tRNA suppressors in Escherichia coli. J. Mol. Biol. 132:649-662[Medline].
13.	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].
14.	Koch, H. K., and R. Woodgate. 1998. The SOS response, p. 107-134. In J. A. Nickoloff, and M. F. Hoekstra (ed.), DNA damage and repair, vol. 1. DNA repair in prokaryotes and lower eukaryotes. Humana Press, Totowa, N.J.
15.	Lee, M. H., T. Ohta, and G. C. Walker. 1994. A monocysteine approach for probing the structure and interactions of the UmuD protein. J. Bacteriol. 176:4825-4837[Abstract/Free Full Text].
16.	Little, J. W. 1993. LexA cleavage and other self-processing reactions. J. Bacteriol. 175:4943-4950[Free Full Text].
17.	Livneh, Z., O. Cohen-Fix, R. Skaliter, and T. Elizur. 1993. Replication of damaged DNA and the molecular mechanism of ultraviolet light mutagenesis. Crit. Rev. Biochem. Mol. Biol. 28:465-513[Medline].
18.	McLenigan, M., T. S. Peat, E. G. Frank, J. P. McDonald, M. Gonzalez, A. S. Levine, W. A. Hendrickson, and R. Woodgate. 1998. Novel Escherichia coli umuD' mutants: structure-function insights into SOS mutagenesis. J. Bacteriol. 180:4658-4666[Abstract/Free Full Text].
19.	Nohmi, T., J. R. Battista, L. A. Dodson, and G. C. Walker. 1988. RecA-mediated cleavage activates UmuD for mutagenesis: mechanistic relationship between transcriptional derepression and posttranslational activation. Proc. Natl. Acad. Sci. USA 85:1816-1820[Abstract/Free Full Text].
20.	Opperman, T., S. Murli, and G. C. Walker. A DNA damage checkpoint control mechanism that regulates DNA synthesis and growth. Submitted for publication.
21.	Opperman, T., S. Murli, and G. C. Walker. 1996. The genetic requirements for UmuDC-mediated cold sensitivity are distinct from those for SOS mutagenesis. J. Bacteriol. 178:4400-4411[Abstract/Free Full Text].
22.	Peat, T. S., E. G. Frank, J. P. McDonald, A. S. Levine, R. Woodgate, and W. A. Hendrickson. 1996. Structure of the UmuD' protein and its regulation in response to DNA damage. Nature 380:727-730[Medline].
23.	Peat, T. S., E. G. Frank, J. P. McDonald, A. S. Levine, R. Woodgate, and W. A. Hendrickson. 1996. The UmuD' protein filament and its potential role in damage-induced mutagenesis. Structure 4:1401-1412[Medline].
24.	Rajagopalan, M., C. Lu, R. Woodgate, M. O'Donnell, M. F. Goodman, and H. Echols. 1992. Activity of the purified mutagenesis proteins UmuC, UmuD', and RecA in replicative bypass of an abasic DNA lesion by DNA polymerase III. Proc. Natl. Acad. Sci. USA 89:10777-10781[Abstract/Free Full Text].
25.	Record, M. T., Jr., W. S. Reznikoff, M. L. Craig, K. L. McQuade, and P. J. Schlax. 1998. Escherichia coli RNA polymerase (E $sigma$ ⁷⁰) promoters, and the kinetics of the steps of transcription initiation, p. 792-821. In F. Neidhardt, R. Curtiss, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. Reznikoff, M. Riley, M. Schaecter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed., vol. 1. American Society for Microbiology, Washington, D.C.
26.	Reuven, N. B., G. Tomer, and Z. Livneh. 1998. The mutagenesis proteins UmuD' and UmuC prevent lethal frameshifts while increasing base substitution mutations. Mol. Cell 2:191-199[Medline].
27.	Shinagawa, H., H. Iwasaki, T. Kato, and A. Nakata. 1988. RecA protein-dependent cleavage of UmuD protein and SOS mutagenesis. Proc. Natl. Acad. Sci. USA 85:1806-1810[Abstract/Free Full Text].
28.	Skare, J. T., B. M. Ahmer, C. L. Seachord, R. P. Darveau, and K. Postle. 1993. Energy transduction between membranes. TonB, a cytoplasmic membrane protein, can be chemically cross-linked in vivo to the outer membrane receptor FepA. J. Biol. Chem. 268:16302-16308[Abstract/Free Full Text].
29.	Slilaty, S. N., and J. W. Little. 1987. Lysine-156 and serine-119 are required for LexA repressor cleavage: a possible mechanism. Proc. Natl. Acad. Sci. USA 84:3987-3991[Abstract/Free Full Text].
30.	Smith, B. T., and G. C. Walker. 1998. Mutagenesis and more: umuDC and the Escherichia coli SOS response. Genetics 148:1599-1610[Abstract/Free Full Text].
31.	Sommer, S., A. Bailone, and R. Devoret. 1993. The appearance of the UmuD'C protein complex in Escherichia coli switches repair from homologous recombination to SOS mutagenesis. Mol. Microbiol. 10:963-971[Medline].
32.	Steinborn, G. 1978. Uvm mutants of Escherichia coli K12 deficient in UV mutagenesis. I. Isolation of uvm mutants and their phenotypical characterization in DNA repair and mutagenesis. Mol. Gen. Genet. 165:87-93[Medline].
33.	Tang, M., I. Bruck, R. Eritja, J. Turner, E. G. Frank, R. Woodgate, M. O'Donnell, and M. F. Goodman. 1998. Biochemical basis of SOS-mutagenesis in Escherichia coli: reconstitution of in vitro lesion bypass dependent on the UmuD'₂C mutagenic complex and RecA protein. Proc. Natl. Acad. Sci. USA 95:9755-9760[Abstract/Free Full Text].
34.	Walker, G. C. 1977. Plasmid (pKM101)-mediated enhancement of repair and mutagenesis: dependence on chromosomal genes in Escherichia coli K-12. Mol. Gen. Genet. 152:93-103[Medline].
35.	Walker, G. C. 1984. Mutagenesis and inducible responses to deoxyribonucleic acid damage in Escherichia coli. Microbiol. Rev. 48:60-93[Free Full Text].
36.	Walker, G. C. 1995. SOS-regulated proteins in translesion synthesis and mutagenesis. Trends Biochem. Sci. 10:416-420.
37.	Walker, G. C. 1996. The SOS response of Escherichia coli, p. 1400-1416. In F. Neidhardt, R. Curtiss, J. L. Ingraham, E. C. C. Lin, K. B. Low, B. Magasanik, W. Reznikoff, M. Riley, M. Schaecter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella: cellular and molecular biology, 2nd ed., vol. 1. American Society for Microbiology, Washington, D.C.
38.	Walker, G. C. 1998. Skiing the black diamond slope: progress on the biochemistry of translesion synthesis. Proc. Natl. Acad. Sci. USA 95:10348-10350[Free Full Text].
39.	Walker, G. C., and P. P. Dobson. 1979. Mutagenesis and repair deficiencies of Escherichia coli umuC mutants are suppressed by the plasmid pKM101. Mol. Gen. Genet. 172:17-24[Medline].
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