Antagonism of Ultraviolet-Light Mutagenesis by the Methyl-Directed Mismatch-Repair System of Escherichia coli

Antagonism of Ultraviolet-Light Mutagenesis by the Methyl-Directed Mismatch-Repair System of Escherichia coli

Hongbo Liu^a, Stephen R. Hewitt^a, and John B. Hays^a
^a Department of Environmental and Molecular Toxicology, Oregon State University, Corvallis, Oregon 97331-7301

Corresponding author: John B. Hays, Department of Environmental and Molecular Toxicology, Oregon State University, ALS 1007, Corvallis, OR 97331-7301., haysj{at}bcc.orst.edu (E-mail)

Communicating editor: P. L. FOSTER

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Previous studies have demonstrated that the Escherichia coliMutHLS mismatch-repair system can process UV-irradiated DNAin vivo and that the human MSH2·MSH6 mismatch-repairprotein binds more strongly in vitro to photoproduct/base mismatchesthan to "matched" photoproducts in DNA. We tested the hypothesisthat mismatch repair directed against incorrect bases oppositephotoproducts might reduce UV mutagenesis, using two allelesat E. coli lacZ codon 461, which revert, respectively, via CCC $->$ CTC and CTT $->$ CTC transitions. F' lacZ targets were mated frommut⁺ donors into mutH, mutL, or mutS recipients, once cellswere at substantial densities, to minimize spontaneous mutationprior to irradiation. In umu⁺ mut⁺ recipients, a range of UVfluences induced lac⁺ revertant frequencies of 4–25 x10^-8; these frequencies were consistently 2-fold higher in mutH,mutL, or mutS recipients. Since this effect on mutation frequencywas unaltered by an Mfd^- defect, it appears not to involve transcription-coupledexcision repair. In mut⁺ umuC122::Tn5 bacteria, UV mutagenesis(at 60 J/m²) was very low, but mutH or mutL or mutS mutationsincreased reversion of both lacZ alleles roughly 25-fold, to5–10 x 10^-8. Thus, at UV doses too low to induce SOS functions,such as Umu₂'D, most incorrect bases opposite occasional photoproductsmay be removed by mismatch repair, whereas in heavily irradiated(SOS-induced) cells, mismatch repair may only correct some photoproduct/basemismatches, so UV mutagenesis remains substantial.

IN most prokaryotes, and in all eukaryotes examined, highlyconserved protein systems that recognize DNA mismatches andcertain DNA lesions play critical roles in maintenance of geneticstability. These long-patch mismatch-repair systems decreaseDNA replication error rates 100- to 1000-fold, by recognizingand correcting base/base and (insertion/deletion)-loopout mismatchesthat escape proofreading by DNA polymerase (KORNBERG and BAKER1992 ). Genetic analyses, and subsequent comprehensive biochemicalcharacterization in vitro (LAHUE et al. 1989 ), have elucidatedthe mismatch-repair pathway in Escherichia coli. Homodimersof E. coli MutS protein bind preferentially to mismatches; then,MutS and MutL homodimers activate MutH protein to specificallynick unmethylated DNA strands at the nearest adenine-hemimethylatedd(GATC) sites, during the interval before adenines in newlyreplicated d(GATC) sequences are methylated. The activation/nickingprocess most likely involves a protein/DNA translocation andsearch process driven by ATP hydrolysis (ALLEN et al. 1997 ).Thus, MutH directs incision and subsequent excision to the nascentDNA strand specifically, so replication errors are correctedrather than fixed. In a reconstituted system (LAHUE et al. 1989), excision requires UvrD protein (DNA helicase II) and either3'-5' or 5'-3' single-stranded DNA (ssDNA) endonuclease, dependingon the relative orientations of the mismatch and the nickedd(GATC) site (COOPER et al. 1993 ). The replicative polymerase(E. coli DNA polymerase III) fills the excision gap. Recombinationinvolving partially diverged DNA sequences is antagonized bymismatch-repair systems, which presumably recognize mismatchesin heteroduplex joints (FEINSTEIN and LOW 1986 ; RAYSSIGUIERet al. 1989 ; PETIT et al. 1991 ; WORTH et al. 1994 ). Accumulatingevidence now suggests processing by mismatch-repair systemsof DNA molecules containing various DNA lesions. These includeultraviolet-light (UV) photoproducts (FENG et al. 1991 ; FENGand HAYS 1995 ; MU et al. 1997 ; WANG et al. 1999 ), O⁶meGresidues (KAT et al. 1993 ; DUCKETT et al. 1996 ), cisplatinG-G intrastrand cross-links (DUCKETT et al. 1996 ), adriamycin(DRUMMOND et al. 1996 ) and acetyl-aminofluorene and aminofluorene(AAF/AF) adducts (LI et al. 1996 ), and S⁶-methylthioguanine/basemismatches (SWANN et al. 1996 ). MutS and MutL activities ortheir homologs are required for efficient transcription-couplednucleotide excision repair of cyclobutane pyrimidine dimers(CPDs) in E. coli (MELLON and CHAMPE 1995 ) and human cells(MELLON et al. 1996 ).

The fate of nonreplicating UV-irradiated phage ${lambda}$ chromosomesin E. coli deficient in nucleotide excision repair (Uvr^-) hasprovided direct in vivo evidence for processing of photoproduct-containingDNA by mismatch-repair proteins. Elevation of homologous recombination,from nearly undetectable frequencies to as much as 10%, andphysical breakdown that resulted in duplex DNA breaks and ssDNAgaps and in loss of biological activity required MutS, MutL,and MutH functions and adenine-undermethylated d(GATC) sites(FENG et al. 1991 ). Further work (FENG and HAYS 1995 ) stronglyimplicated helicase and ssDNA exonuclease activities involvedin mismatch repair (COOPER et al. 1993 ). Studies of photoproductbinding by hMutS ${alpha}$ , the human homolog of MutS, have demonstratedspecific binding to a variety of mismatched CPDs and [6-4] photoproducts,but not to matched photoproducts (MU et al. 1997 ; WANG etal. 1999 ).

Mismatch repair, targeted to mismatched photoproducts generatedby translesion synthesis during the interval that d(GATC) siteson nascent strands remained unmethylated, would excise incorrectbases rather than the photoproducts. For such a process to antagonizemutagenesis efficiently, the subsequent ssDNA-gap-filling DNAsynthesis would have to insert the correct base opposite thetemplate photoproduct that originally provoked the repair process.Correct insertion seems the usual result of synthesis past CPDsin phage ssDNA in E. coli (BANERJEE et al. 1988 ; JIANG andTAYLOR 1993 ) and in human nuclear extracts replicating UV-irradiatedSV40-origin plasmids (CARTY et al. 1993 ; THOMAS and KUNKEL1993 ). Alternatively, stalled mismatch-repair resynthesis tractscould be extended by recombinational template-switching or gap-fillingmechanisms. Finally, failed mismatch-repair resynthesis couldlead to DNA degradation, the net result being elimination ofmutant chromosomes. In any event, a prediction of these mutagenesis-antagonismmodels is that UV mutagenesis should be enhanced in E. colimutS, mutL, and mutH mutants, beyond increases in spontaneousmutation.

To test this prediction we analyzed UV-induced reversion oftwo E. coli lacZ codon-461 alleles, constructed by CUPPLESand MILLER 1989 to revert to lac⁺ only by CCC $->$ CTC or CTT $->$ CTC transitions. The targets are thus 3' pyrimidines in potentialphotoproduct sites. To minimize culture-to-culture fluctuationsin spontaneous mutant frequencies, we mated the F' lacZ targetsinto mut^- cells just before irradiation, when cell densitieswere already substantial. We find a consistent twofold increasein UV mutagenesis in mismatch-repair-deficient (umu⁺) bacteriaand also hitherto unsuspected substantial UmuC-independent UVmutagenesis, which is readily detectable only in mut^- cells.

MATERIALS AND METHODS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Bacterial strains and plasmids:
E. coli K-12 strains employed in the mutation studies are describedin Table 1. Transduction with P1 phage employed standard techniques(MILLER 1972 ). Transposon-insertion alleles encoding cat, Tn5,and Tn10 were selected on Luria broth (LB) plates containing,respectively, chloramphenicol (35 µg/ml), kanamycin (50µg/ml), or tetracycline (15 µg/ml). MutS^-, MutH^-,and MutL^- phenotypes were identified by increased spontaneousresistance to rifampicin (100 µg/ml) in LB plates, andthe UmuC^- phenotype was recognized by increased UV sensitivity.Plasmid pMQ315 contains the mutS⁺-encoding BglII restrictionfragment of E. coli DNA, inserted into the BamHI site of plasmidpBR322 (WU and MARINUS 1994 ).

View this table:
In this window
In a new window

Table 1. Bacterial strains

Media and antibiotics:
M9 minimal media contained 6 g/liter K₂HPO₄ plus 3 g/liter KH₂PO₄(pH 7.0), 1 g/liter (19 mM) NH₄Cl, 0.1 mM CaCl₂, 1 mM MgSO₄,and 0.001% thiamine, plus glucose (0.2%), glycerol (0.2%), orlactose (0.2%). LB plates have been described (MILLER 1972 ).Plates were solidified with 1.5% agar (glucose plates; Difco,Detroit) or 1.5% noble agar (lactose plates; United States Biochemical,Swampscott, MA).

Growth, mating, and irradiation of bacteria:
For mutagenesis experiments, bacteria were streaked from frozen-glycerolcultures onto LB plates, and single colonies were used, afterno more than 36 hr of growth, to inoculate glycerol-minimal-mediumcultures, typically 30 ml, containing 60 µg/ml proline.(Inoculation with older colonies resulted in significantly higherfinal levels of spontaneous lac⁺ revertants in cultures of mut^-strains.) After overnight growth at 37°, cultures of variousF^- (mut⁺ or mut^-) phr::cat ${Delta}$ (lac-pro) recipients and mut⁺ F'(pro⁺ lacI^- lacZ^-) donors were both diluted 1.5-fold with freshmedium, or grown without dilution, to ~3.5 x 10⁸ cells/ml, mixedtogether, and incubated at 37° with very gentle swirling.(All cultures of F^- recipients contained 60 µg/ml proline.)After a 2-hr mating period, mixtures were washed with glycerol-minimalmedium containing chloramphenicol, but no proline, resuspendedto 1 x 10⁸ cells/ml in the same medium, and grown for 6–8hr, to select for phr::cat F' (pro⁺ lacI^- lacZ^-) transconjugants.At the end of selective growth, transconjugants typically represented80% of the total colony-forming units in the mating mixture,as determined by selective vs. nonselective plating.

For UV irradiation, mixtures were diluted with glycerol-minimalmedium plus chloramphenicol to yield 2.5 x 10⁸ transconjugants/ml,and 10-ml aliquots were added to uncovered 10-cm plastic petridishes and irradiated at 2 W/m², using 254-nm lamps attenuatedby window screen. Unirradiated aliquots were used as controls.Lamp fluences were checked using a Spectronics DRC-100X meterand/or an International Light IL1700 radiometer. To determinesurviving fractions, irradiated and unirradiated control cellswere spread immediately on glucose-minimal plates containingchloramphenicol, and colonies were scored after 48 hr incubation.Under these conditions, survival frequencies of (unmated) mutS-,mut⁺-, and mutS⁺-overproducing (mutS⁺⁺⁺) bacteria (strains LH2519,LH3179, and LH2536, respectively) were very similar to one another:~25, 17, 10, 5, and 1.3%, at 20, 30, 45, 60, and 90 J/m², respectively.

Analysis of mutation in UV-irradiated bacteria:
For initial screening of all six lacZ461 alleles for effectsof mismatch repair on UV mutagenesis, mut⁺ and mutS201::Tn5F' (lacZ) strains were grown as described above without matingand were irradiated and analyzed. In all other experiments,irradiated and unirradiated transconjugant cells were dilutedwith equal volumes of glycerol-minimal medium containing chloramphenicoland were incubated at 37° with shaking. Cultures were incubatedin minimal medium rather than broth to reduce carryover of tracenutrients onto the selective plates, and glycerol was used ratherthan glucose to ensure maximal expression of the lacZ gene.Cells were harvested by centrifugation after 8–10 hr (logarithmicgrowth was fully restored by 4 hr), resuspended in 0.2 vol ofM9 minimal salts, diluted appropriately, and spread on glucose-minimal/chloramphenicolplates to score total (transconjugant) bacteria, or cells werespread directly on scavenged lactose-minimal/chloramphenicolplates to score revertants and were incubated for 48 hr at 37°.[Plates were scavenged 1 day before initiation of experimentsby spreading 5 x 10⁷ bacteria of strain LH3302 (phr::cat transductantof ${Delta}$ lac strain FC755) and incubating overnight at 37°. Thisprevents further mutagenesis on the plates (see RESULTS).] Throughoutthe text, "UV-induced revertant frequencies" implies that lac⁺revertant frequencies were determined for parallel unirradiatedcultures and were subtracted from apparent frequencies for UV-irradiatedcells. Since unirradiated cultures grew (increased in turbidity)about four times as well as irradiated cultures during the 8-hrpostirradiation period, this subtraction may overcorrect slightlyfor background spontaneous mutant frequencies in the irradiatedcells. Revertant frequencies determined after as much as 24hr of postirradiation growth in liquid medium were the sameas 8-hr frequencies.

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Design and evaluation of experimental approaches:
Our aims were (i) to ensure that most UV mutagenesis (here reversionof lacZ^- alleles to lac⁺) took place during a defined periodof postirradiation growth in liquid culture, rather than onselective plates, and (ii) to minimize fluctuations in the backgroundspontaneous mutant frequencies in cultures of mismatch-repair-defective(mut^-) bacteria.

To determine the time required for recovery from UV irradiationand concomitant mutagenesis, we incubated irradiated cells inglycerol-minimal medium and measured total cell masses (turbidityunits; Figure 1) and numbers of viable bacteria (data not shown).After a 4-hr recovery period these both began to increase exponentially.However, frequencies of lac⁺ revertants after recovery couldnot be determined unequivocally by spreading on lactose-minimalplates, even when cells were washed several times: the numberof visible Lac⁺ colonies increased every day for at least 5days, and their number was not proportional to the number ofcells spread. These problems were most severe for mut^- bacteria.We suspected that trace carbon sources in the lactose-minimalplates were supporting limited slow growth by lacZ^- bacteria,the final numbers of cells being more dependent on the amountsof trace nutrients than on the initial numbers of cells, asobserved previously (ZIEG and KUSHNER 1977 ). We also suspectedthat lac⁺ revertants continued to arise during this slow growth.To eliminate trace nutrients in the plates, we used purified("noble") agar, high-purity (glucose-free) lactose and scavengedthe plates by spreading with 5 x 10⁷ ${Delta}$ lac bacteria and incubatingovernight, just before UV mutagenesis experiments. Under theseconditions, the number of Lac⁺ colonies arising was directlyproportional to the number of cells spread, and did not changeduring 2–7 days of incubation on plates.

View larger version (18K):
In this window
In a new window
Download PPT slide

Figure 1. Time course of UV mutagenesis and recovery from irradiation. Cultures of phr::cat F' (lacZ461-6) bacteria (strain LH3140) were grown and irradiated to 60 J/m² in glycerol-minimal medium, diluted to a turbidity of 15 Klett units (~1 x 10⁸ cfu/ml, for unirradiated bacteria), and shaken at 37°. Data correspond to means of turbidity measurements (•) for two independent experiments. Measurements of frequencies of UV-induced lac⁺ revertants ( ${triangleup}$ ) were essentially as described in MATERIALS AND METHODS; data correspond to means for four independent experiments, with standard deviations indicated.

The low frequency of lac⁺ revertants among cells that were spreadimmediately on selective plates (Figure 1) indicates that thetechnique mostly scores mutants that arise during postirradiationincubation in liquid culture. The maximum in revertant frequencyafter ~4 hr suggests that mutation fixation is nearly completeby then, but that chromosome replication and/or segregationof lac⁺ and lacZ^- alleles into daughter cells has not occurredyet. The subsequent 50% decrease in apparent revertant frequencyindicates that few additional mutations arise during subsequentrounds of replication. Segregation of parental and daughterstrands and cells after mutation of DNA strands would thus doublethe number of survivors without increasing the number of revertants,as suggested previously (BRIDGES and MUNSON 1968 ). After 6hr of growth in culture, numbers of both lac⁺ and total cellsincrease exponentially in parallel, providing a stable mutantfrequency (Figure 1 and data not shown).

To screen for effects of mismatch-repair deficiency on UV mutagenesisvia different transition and transversion pathways, we employedbacteria encoding on respective F' episomes the six lacZ codon-461alleles constructed by CUPPLES and MILLER 1989 ; the designationslacZ461-1, lacZ461-2 ... lacZ461-6 used here correspond to theirstrains CC101, CC102 ... CC106. Each different allele revertsto a (GAG) codon for glutamate, the only amino acid compatiblewith ß-galactosidase activity (CUPPLES and MILLER 1988), by a different single base substitution. Table 2 shows lac⁺revertant frequencies (corrected for spontaneous frequenciesin the same cultures) induced by a UV dose of 45 J/m², in mut⁺and mutS201 bacteria bearing each of the six F'(lacZ) episomes.For the two lacZ alleles where target bases are not in potentialdipyrimidine-photoproduct sites, the revertant frequencies (x10⁸) in mut⁺ and mutS201 derivatives were 48 vs. 56 for lacZ461-4,and 14 vs. 16 for lacZ461-5 (sense-strand GCG $->$ GAG and GTG $->$ GAG transversions, respectively; Table 2, lines 7–10).Thus, neither of these (presumably untargeted) transversionsshowed a mismatch-repair effect. The two other transversionalleles showed low UV-induced reversion frequencies, althoughtarget bases were in potential photoproduct sites, and low mismatch-repaireffects: frequencies (x 10⁸) in mut⁺ and mutS201 derivativeswere 2.8 vs. 4.5 for lacZ461-1 and 1.6 vs. 2.0 for lacZ461-3(sense-strand T TAG $->$ T GAG and T CAG $->$ T GAG reversions, respectively; Table 2, lines 1 and 2, 5 and 6). However, where the mutationtargets were 3' bases in dipyrimidines, reverting via transitions,revertant frequencies (x 10⁸) were high and were consistentlytwofold higher in mutS201 derivatives: 73 vs. 131 for lacZ461-2and 71 vs. 159 for lacZ461-6 (template strand CCC $->$ CTC and CTT $->$ CTC reversions, respectively; Table 2, lines 3 and 4, 11 and12). The lacZ461-2 and lacZ461-6 alleles were employed in allsubsequent experiments.

View this table:
In this window
In a new window

Table 2. UV-induced reversion of lacZ461 alleles

Revertant frequencies among unirradiated mutS F' (lacZ461-2)and mutS F' (lacZ461-6) bacteria fluctuated considerably fromculture to culture, perhaps reflecting spontaneous reversionrelatively early in colony isolation or culture growth (beforeirradiation). When the spreads in the respective sets of revertantfrequencies observed for a particular strain were measured bycalculating the standard deviations from the mean, large culture-to-culturefluctuations in spontaneous mutation frequencies for mut^- strainswere apparent. Thus, in the experiments shown in Table 2, thestandard deviations of the sets of spontaneous-reversion frequenciesfor mutS201 strains bearing F'(lacZ461-1) ... F'(lacZ461-6)episomes were, respectively, 94, 110, 36, 63, 89, and 88% ofthe corresponding means. In other experiments, with umuC122mutL96 F'(lacZ461-6) bacteria (strain LH3290), the set of spontaneousrevertant frequencies (x 10⁸) combined from several experiments(total n = 16), showed a mean of 50 and a standard deviationof 88, 176% of the mean. In subsequent experiments, therefore,we propagated parallel cultures of F^- mutS bacteria or otherrecipients of interest, and mut⁺ umuC122 (F' lacZ^-) donors,and mated F⁺ to F^- cultures for 2 hr. Selection for 6–8hr yielded ~80% pro⁺ chloramphenicol-resistant transconjugants.These were irradiated, grown out, and plated, with continuedselection, which increased the transconjugant fraction to 90–95%.When umu⁺ mut^- recipients were mated with F'(lac-Z461-6) donors(see Figure 2 and Figure 3), the set of all spontaneous revertantfrequencies (x 10⁸) of transconjugant cultures (n = 26 for allcultures of all experiments with mutS, mutL, and mutH recipients)showed a mean of 3.3 and standard deviation 1.0, only 30% ofthe mean. For F'(lacZ461-2) donors, the set of all spontaneousrevertant frequencies (x 10⁸) for all umu⁺ mut^- transconjugantcultures (n = 7) showed mean 3.9 and standard deviation 1.0,only 25% of the mean. In experiments with umuC122 mut^- recipients(see Figure 4), the set of all transconjugant spontaneous revertantfrequencies (x 10⁸) for lacZ461-6 donors (n = 17) showed mean2.9, standard deviation 1.5 (52%), and for lacZ461-2 donors(n = 17), mean 2.7, standard deviation 1.0 (37%).

View larger version (16K):
In this window
In a new window
Download PPT slide

Figure 2. Dependence of mutant frequency in umu⁺ bacteria on UV dose. Growth and mating of umu⁺ phr::cat ${Delta}$ (lac-pro) recipients with F' (lacZ461-6 pro⁺) donors (strain LH3305), selection for transconjugants, UV irradiation to indicated fluences, further growth and plating, and analysis of UV-induced lac⁺ revertant frequencies were as described in MATERIALS AND METHODS. For each UV fluence, each open, filled, or crossed symbol corresponds to an independent experiment employing typically three parallel cultures of a particular strain: (open, solid, and crossed circles) mutS97, strain LH2519; (open, solid, and crossed squares) mut⁺, strain LH3279; (open, solid, and crossed triangles) mutS⁺⁺⁺, strain LH23305. (For crossed and solid symbols at 45 J/m² there were only one or two independent cultures.) Values represent means for the multiple independent cultures for each strain. Some symbols at each UV fluence are off-set for clarity. Solid lines are drawn through means of values corresponding to circles, and dashed lines are drawn through means of triangle values. To estimate standard errors of the mean (SEMs), the set of all values for a particular strain and UV dose, for all cultures and experiments, were combined and analyzed, since experiment-to-experiment variations were not consistently markedly different from culture-to-culture variations. Revertant frequency means (± SEM) (x 10⁸) for mutS97, mut⁺, and mutS⁺⁺⁺ bacteria, respectively, were as follows: 20 J/m², 14.4 (± 0.9), 5.7 (± 0.2), 3.4 (± 0.6); 30 J/m², 28.0 (± 3.4), 10.2 (± 0.9), (7.1 ± 1.6); 45 J/m², 55.0 (± 1.0), 24.4 (± 4.2), 20.5 (± 2.7). For the set of all data for unirradiated mutS97 bacteria (n = 14), mean (SEM) was 3.9 (± 0.3) x 10^-8 (frequencies for unirradiated mut⁺ and mutS⁺⁺⁺ bacteria were negligible).

View larger version (15K):
In this window
In a new window
Download PPT slide

Figure 3. UV-induced mutation in umu⁺ bacteria. Indicated umu⁺ phr::cat ${Delta}$ (lac-pro) recipients and mut⁺ donors of F' (lacZ-pro⁺) episomes were grown and mated, and transconjugants were selected, irradiated to 60 J/m², grown 8 hr, and scored for frequencies of UV-induced lac⁺ revertants, as described in MATERIALS AND METHODS. For each indicated genotype, each individual symbol refers to an independent experiment, in which mutant frequencies for two to three parallel cultures of mut⁺ recipients (strain LH3179) were, respectively, compared to frequencies for two to three parallel cultures of one particular mutant recipient: mutS (•), strain LH2519; mutL ( ${blacksquare}$ ), LH3183; mutH ( ${blacksquare}$ ), LH2520; mutS⁺⁺⁺ ( ${circ}$ ), LH2536. [mut⁺ mfd recipients (strain LH2548) were compared to mutS mfd ( ${blacktriangleup}$ ) recipients (strain LH2549).] For each independent experiment (independent symbol), relative mutant frequency equals mean of mutant frequencies for the mut^- (or mutS⁺⁺⁺) cultures divided by the mean for the mut⁺ cultures. Expected reversion pathways for the two F' (lacZ^- pro⁺) donors employed are indicated: C $->$ T, lacZ461-2 (strain LH3303); T $->$ C, lacZ461-6 (strain LH3305). For the experiments employing mut^- vs. mut⁺ bacteria (solid symbols), mean (± SEM) UV-induced revertant frequencies (x 10⁸), of transconjugants for sets of pooled data from all cultures in all repetitions of each particular experiment, were as follows for mut⁺ and mut^- strains, respectively: mutS C $->$ T, 24.3 (± 1.3) and 13.4 (± 0.3); mutS T $->$ C, 28.0 (± 3.4) and 10.2 (± 0.9); mutL T $->$ C, 24.8 (± 1.3) and 12.0 (± 0.3); mutH T $->$ C, 23.9 (± 1.4) and 11.6 (± 1.0); mutS mfd T $->$ C, 30.4 (± 5.3) and 19.2 (± 1.4). Corresponding frequencies (± SEM) (x 10⁸) for pooled data for unirradiated mut^- bacteria were 3.3 (± 0.4), 4.7 (± 0.3), 3.4 (± 0.4), 4.1 (± 0.4), and 4.4 (± 0.4). Corresponding mean revertant frequencies (± SEM) x 10⁸ for mutS⁺⁺⁺ C $->$ T and mutS⁺⁺⁺ T $->$ C were 12.6 ± 1.3 and 7.1 ± 1.6.

View larger version (19K):
In this window
In a new window
Download PPT slide

Figure 4. UV-induced mutation in umuC122 bacteria. Indicated umuC122 phr::cat ${Delta}$ (lac-pro) recipients and mut⁺ donors of F' (lacZ461-2 pro⁺) [strain LH3303, open bars (C $->$ T reversion)] or F' (lacZ461-6 pro⁺) [strain LH3305, shaded bars (T $->$ C reversion)] were grown and mated, and transconjugants were selected, irradiated to 60 J/m², grown 8 hr, and scored for frequencies of lac⁺ revertants, as described in MATERIALS AND METHODS. Individual symbols correspond to individual cultures, and different symbol shapes ( ${blacksquare}$ , •, ${blacktriangleup}$ ), respectively, correspond to different independent experiments each employing two or three cultures of the particular indicated strains in parallel. Recipient genotypes indicated: mut⁺, strain LH3265; mutS, LH2534; mutL, LH3269; mutH, LH2535. For the experiments employing mut^- bacteria (bars 3–8), respective mean (± SEM) UV-induced and spontaneous transconjugant revertant frequencies (x 10⁸) were as follows: mutS C $->$ T, 5.0 (± 0.5) and 2.6 (± 0.1); mutS T $->$ C, 5.9 (± 0.1) and 2.8 (± 0.6); mutL C $->$ T, 5.0 (± 0.4) and 2.7 (± 0.4); mutL T $->$ C, 5.6 (± 1.0) and 3.3 (± 0.5); mutH C $->$ T, 5.8 (± 1.3) and 1.7 (± 0.5); mutH T $->$ C, 5.9 (± 0.8) and 2.9 (± 0.8).

UV mutagenesis in umu⁺ mut^- bacteria:
We used the mating technique to compare reversion of lacZ461-6mutations in mutS vs. mut⁺ transconjugants at three UV fluences(Figure 2). Revertant frequencies increased with fluence inboth strains, but averaged 2.6-fold higher in mutS97 than inmut⁺ bacteria, in good agreement with the mutS/mut⁺ ratio of2.2 obtained in experiments with single cultures of F' (lacZ)bacteria (no mating; see above). In mut⁺ bacteria harboringa mutS⁺-encoding plasmid, there was a small trend to even lowerrevertant frequencies.

Figure 3 shows the effects of mismatch-repair deficiencieson lac461-2 and lacZ461-6 reversions at a single UV fluenceof 30 J/m². Revertant frequencies for mutH, mutL, and mutS bacteriawere again consistently twice as high as for mut⁺. Both theMutS^- and MutL^- effects might reflect reductions in transcription-couplednucleotide excision repair (MELLON and CHAMPE 1995 ), sincethe lacZ gene should be derepressed in these lacI-defectivebacteria growing in glycerol. However, in strains defectivein Mfd activity, which normally couples transcription blockageto template-strand-specific excision repair (SELBY et al. 1991; SELBY and SANCAR 1993 ), a mutS mutation again increasedlacZ461-6 T $->$ C reversion, to 2.2 times the mut⁺ value (Figure 4,triangles). The Mfd^- phenotype was confirmed by lower survivalat 30 J/m² (5% vs. 18% for Mfd⁺) and by transduction of themfd::Tn5 marker into strain WU3610 and verification of lossof the mutation-frequency-decline phenotype (WITKIN 1966 ).

UV mutagenesis in UmuC^- Mut^- bacteria:
The defining phenotype of umuC mutations is a drastic decreasein UV mutagenesis (KATO and SHINOURA 1977 ; STEINBORN 1978). Figure 4 shows that UV-induced reversions of lacZ461-2 andlacZ461-6 alleles in umuC::Tn5 mut⁺ bacteria were almost undetectable(Figure 4), but that inactivation of mismatch repair unmaskedsubstantial UmuC-independent UV mutagenesis: UV-induced frequenciesof both T $->$ C and C $->$ T reversion induced by 30 J/m² were roughly5 x 10^-8, in mutS, mutL, and mutH bacteria. These experimentswere repeated, using 100 plates each to analyze revertant frequenciesamong irradiated umuC122 mut⁺ recipients (strain LH3266) containingF' lacZ461-2 or F' lacZ461-6 episomes. On the basis of 135 and121 total Lac⁺ colonies, respectively, revertant frequencieswere 4.0 x 10^-9 and 2.7 x 10^-9; the respective revertant frequenciesfor umuC122 mutS::Tn10 recipients (strain LH2534) containingthe same episomes were 10.7 x 10^-8 and 7 x 10^-8, a 25-fold increasein each case. In earlier experiments not using the mating technique,mutL umuC122 (F' lacZ461-6) bacteria showed wide fluctuationsin spontaneous reversion frequency (see above). Here we analyzedUV mutagenesis only for 7 (of 17) cultures that showed spontaneousrevertant frequencies of <10 x 10^-8 before irradiation; themean (standard deviation) revertant frequency was 6.7 (±2.2) x 10^-8. UV irradiation of each of these cultures to 60J/m² increased revertant frequencies; the mean was 12.1 (±6) x 10^-8. The apparent UV-specific component, 5.4 x 10^-8, wasthus in good agreement with values obtained using the matingtechnique (see above). Revertant frequencies for mut⁺ umuC122(F' lacZ461-6) bacteria (no mating) were again <5 x 10^-9.

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The experiments described here support a hypothesis that mismatch-repairsystems antagonize UV mutagenesis by excising incorrect basesinserted in nascent strands opposite photoproducts during thecourse of DNA replication, and replacing them, some or mostof the time, with the correct bases. This hypothesis was motivatedby observations that human MSH2 · MSH6 protein boundspecifically to DNA containing a mismatched cyclobutane pyrimidinedimer (CPD, Py<>Py), e.g., T<>T/AG, or a mismatched pyrimidine-(6-4')-pyrimidinonephotoproduct ([6-4] photoproduct, Py[6-4]Py), e.g., T[6-4]T/AG,but not to DNA containing T<>T/AA or T[6-4]T/AA pairs (MUet al. 1997 ; WANG et al. 1999 ). Other explanations for theseresults, especially for the twofold difference between mut⁺and mut^- bacteria seen in umu⁺ strains, might be more efficientexcision repair in mut⁺ bacteria, or faster replication (relativeto repair) in mut^- cells. DNA replication might in principlebe faster if not delayed by binding and/or processing of mismatchedbases or photoproducts by mismatch-repair proteins, but we arenot aware of any reports of faster replication in mut^- bacteria.We think it is unlikely that the antagonism of UV mutagenesisby mismatch repair described here simply reflects removal, byMutSL-assisted transcription-coupled excision repair, of premutagenicphotoproducts at the CCC and TT targets in the lacZ461-2 andlacZ461-6 template strands, because we observed MutH-dependentand Mfd-independent antagonism of mutagenesis, in contradistinctionto the requirements for transcription-coupled repair. Furthermore,the previously reported MutHLS-dependent recombination of repressor-blockedUV-irradiated phage DNA occurred in excision-repair-deficient(Uvr^-) bacteria (FENG et al. 1991 ). Clearly, it would be ofinterest to analyze mismatch-repair effects on UV mutagenesisin Uvr^- bacteria. UV mutagenesis might occur in Uvr⁺ bacteriaduring replication, or by insertion of an incorrect nucleotideopposite a nearby second UV photoproduct during DNA synthesisto fill a gap created by excision repair of a first photoproductin the opposite strand. In the latter case, mismatch repairmight prevent fixation of mutations during subsequent excisionrepair of the second photoproduct. In any event, the constantratio between UV-induced revertant frequencies for mut^- andmut⁺ bacteria seen in Figure 2 as the UV dose increases seemsmost consistent with a constant efficiency of mismatch repair.

Mismatch repair provoked by photoproduct/base mismatches, asby base/base mismatches, would be expected only in the vicinityof replication forks, where unmethylated d(GATC) sites werestill present (LAHUE et al. 1989 ). In unreplicated DNA, therefore,Py<>U/PuG mismatches resulting from the relatively rapiddeamination of cytosines in CPDs (PENG and SHAW 1996 ) wouldnot be processed, whereas Py<>U/PuG mismatches arising innewly replicated DNA might be "corrected" to Py<>U/PuA, actuallyfixing C $->$ T transitions. Also, if progress of replication forkspast template Py<>C photoproducts depended on deaminationto Py<>U, so as to facilitate insertion of an adenine nucleotide(TESSMAN et al. 1992 ), the resulting Py<>U/PuA moiety wouldnot be recognized by MutS (WANG et al. 1999 ). Thus, if deaminationof cytosines in CPDs played a major role in UV mutagenesis inthe experiments described here, mismatch repair might antagonizeUV-induced T $->$ C transitions more efficiently than C $->$ T. However,the apparent mutation-removal efficiencies were approximatelythe same for UV-induced mutation of the two alleles tested,roughly 50% in umu⁺ and 96% in umuC122 bacteria. Therefore,most C $->$ T reversions as measured here in mut^- lacZ461-2 bacteriawould appear not to have arisen by cytosine-deamination mechanisms,but rather by insertion during DNA replication of adenines oppositephotoproducts containing cytosines [perhaps their imino tautomers(PERSON et al. 1974 ; JIANG and TAYLOR 1993 )]. (Although [6-4]photoproducts may be responsible for some or all of the MutHLS-sensitiveUV mutagenesis described here, cytosine deamination is not enhancedin these photoproducts.)

In comparisons among different studies of UV mutagenesis, thespecific circumstances under which UV-induced mutations ariseand are fixed may be important. In our experiments irradiatedcells were diluted and shaken in liquid glycerol-minimal medium,under conditions such that parallel unirradiated cultures grewexponentially. Irradiated cultures resumed exponential growthafter ~4 hr, at which time fixation of mutations appeared complete(Figure 1). In the scavenged lactose-minimal plates trace carbonsources appeared not to be available to the lacZ^- bacteria foreven limited growth and further mutagenesis, since very fewLac⁺ colonies arose when bacteria were plated immediately afterirradiation. Most mutations appeared to arise 2–4 hr afterirradiation, although the cultures did not show appreciablegrowth until 6 hr (Figure 1). Other workers (CROWLEY and HANAWALT1998 ) have shown that for excision-repair-proficient bacteriagrowing in glucose-minimal medium, removal from the genome overallof CPDs induced by 40 J/m² of 254-nm irradiation is essentiallycomplete within 60 min; repair of [6-4] photoproducts is completein 20 min. Thus, factors other than photoproduct removal wouldappear to be rate limiting here for resumption of growth andcolony-forming proficiency.

Mismatch repair might reduce UV mutagenesis by removing incorrectbases inserted opposite photoproducts during translesion synthesisand/or correcting mismatches from "untargeted" SOS mutagenesis(KUNZ and GLICKMAN 1984 ; CHRISTENSEN et al. 1985 ; MILLER1985 ; CAILLET-FAUQUET and MAENHAUT-MICHEL 1988 ). Severalconsiderations argue against a hypothesis that most of the UVmutagenesis seen here in mut^- umuC122 bacteria is untargeted.

CAILLET-FAUQUET and MAENHAUT-MICHEL 1988 reported no significantdifference between the frequencies of spontaneous reversionto rifampicin resistance of umuC122 mutS bacteria that wererecA⁺ or those that carried the recA730 mutation, known to causean SOS-like activation of RecA protein that increases (untargeted)spontaneous mutation ("SOS mutagenesis"), whereas a recA270mutation in umu⁺ mutS/L backgrounds increased the mutation frequency2.5-fold. This is consistent with other reports that SOS mutagenesisrequires UmuC function.
FIJALKOWSKA et al. 1997 observedthat a recA730 mutation increasedtransversion frequencies (reversionsof lacZ461-4 and lacZ461-5mutations) much more than transitionfrequencies (lacZ461-2and lacZ461-6 reversions), respectively,2–6-fold vs.20–70-fold, in both mut⁺ and mutS bacteria(both umuC⁺).There is no evidence to suggest that this preferencemight bereversed in umuC122 bacteria.
Previous studies suggestthat untargeted mutations amount toonly 3–10% of allUV-induced mutations, including thoseat both putative photoproductand nonphotoproduct sites (KUNZand GLICKMAN 1984 ; CHRISTENSENet al. 1985 ; MILLER 1985).

Thus, although we cannot rule out some contribution of untargetedevents to the greatly increased UV-induced transition frequenciesseen in mut^- derivatives of umuC122 bacteria, it seems likelythat much of this reflects photoproduct-targeted events. Inumu⁺ bacteria, the greater-than-first-power dependence of mutantfrequency on dose seen in both mut⁺ and mutS derivatives (Figure 2)argues in favor of targeted mutagenesis in both strains,since untargeted mutation would be expected to level off athigher doses, once SOS induction was maximal.

Some previous descriptions of UmuC-independent UV mutagenesisin mismatch-repair-proficient bacteria represent special casesnot applicable here. Fuchs and co-workers (NAPOLITANO et al.1997 ) have described SOS-dependent, but UmuC-independent, frameshiftmutagenesis at certain hotspots, targeted by 2-acetylaminofluoreneadducts, that involves slip mispairing at mononucleotide ordinucleotide repeats at these sequences. The UVM pathway, studiedextensively by HUMAYUN 1998 , specifically causes mutationsby inserting thymine nucleotides opposite etheno-cytosine residues.Although inducible by other kinds of DNA damage, it is independentof RecA and UmuD₂'C.

Lawrence and co-workers (CHRISTENSEN et al. 1988 ) observedsubstantial UmuC-independent UV mutagenesis when they spreadcultures of mut⁺ uvrA6 umuC122 bacteria, after post-UV-irradiationgrowth, on nonselective plates, and identified lacI^- mutantsamong other survivors by colony color. However, when they spreadthe same cultures on scavenged selective (phenyl-galactosidase)plates, similar to the procedure used here, very few colonies(lacI^- mutants) were seen. On nonselective plates, mismatch-repairproteins might have declined during colony growth, making cells(umuC122) Mut^- phenocopies, as has been reported for stationary-phase(FENG et al. 1996 ) or carbon-starved (HARRIS et al. 1997 )bacteria. [P. L. Foster has argued against a hypothesis of lowmismatch repair under starvation conditions, however (FOSTER1999 ).] Alternatively, some of these irradiated uvrA umuC122bacteria might have become Mut^- phenocopies eventually duringincubation on the nonselective plates, due to saturation ofmismatch repair (SCHAAPER and RADMAN 1989 ; CUPPLES et al.1990 ) by uracil/base mismatches arising from deamination ofunrepaired CPD cytosines (WANG et al. 1999 ).

Another source of UmuC-independent UV mutagenesis might be theproduct of the dinB (dinP) gene (OHMORI et al. 1995 ), whichmaps close to lacZ and would thus be present in the F' episomesused here. Although the DinB protein is a UmuC homolog, it isnot known whether it interacts with UmuD protein, which shouldbe present at some level in umuC122 bacteria. It would be ofinterest to analyze UV mutagenesis in ${Delta}$ umuCD mutS bacteria.

Why is antagonism of UV mutagenesis apparently more completein umuC122 than in umu⁺ bacteria? One possibility is that thehigh numbers of misinsertions in umu⁺ bacteria (correspondingto revertant frequencies of ~50 x 10^-8 in mut^- umu⁺ cells irradiatedto 45 J/m²) saturate the mismatch-repair system, as observedpreviously in other contexts (SCHAAPER and RADMAN 1989 ; CUPPLESet al. 1990 ). By this hypothesis, the revertant frequenciesin umuC122 mut^- cells at 60 J/m² (~5 x 10^-8) would correspondto misinsertion levels below the saturation threshold. However,the apparent constant efficiency of antagonism of UV mutagenesisby mismatch repair in umu⁺ bacteria, as fluences increase from20 to 45 J/m² (Figure 2), argues against this. Since MutS proteinshows lower affinity for photoproduct/base mismatches than forcorresponding base/base mismatches (WANG et al. 1999 ; H. WANGand J. B. HAYS, unpublished data), high concentrations of MutSmight be needed for efficient antagonism of UV mutagenesis.However, a multicopy plasmid encoding the mutS⁺ gene had littleeffect on mutant frequencies (Figure 2 and Figure 3); simultaneousoverproduction of MutS, MutL, and MutH activities has not beentested. A second explanation would be that one class of photoproducts,perhaps CPDs, is responsible for UV mutagenesis in umuC^- bacteria,whereas both CPDs and [6-4] photoproducts might target mutationsin umu⁺ bacteria. Only mutations targeted by one class mightbe subject to mismatch repair. However, both T-T CPDs and T-T[6-4] photoproducts mismatched opposite A-G are recognized byMutS or its human homolog hMutS ${alpha}$ , and neither photoproduct oppositeA-A is recognized (H. WANG and J. B. HAYS, unpublished data; WANG et al. 1999 ); i.e., there is no evidence for MutS/hMutS ${alpha}$ preference for one mismatched photoproduct over the other. Athird explanation might be that in UV-irradiated umu⁺ bacteria,DNA resynthesis associated with mismatch repair triggered byphotoproducts might itself result in new misinsertions, oppositephotoproducts or at nonphotoproduct sites, by DNA polymeraseIII (LAHUE et al. 1989 ) associated with UmuD'₂C and RecA protein.

In bacteria subjected to UV fluences insufficient to inducethe SOS response, occasional photoproduct/base mismatches mightarise from DNA replication past UV photoproducts, perhaps facilitatedby low-level UmuC-independent constitutive activities that allowederror-prone translesion synthesis. If so, these mismatches wouldappear to be almost all corrected by the MutHLS system. In heavilyDNA-damaged SOS-induced bacteria, however, where a burst ofmutagenesis to increase genetic variability has been hypothesizedto promote species survival (ECHOLS 1982 ), inefficient correctionof photoproduct/base mismatches, because of error-prone mismatch-repairresynthesis or for other reasons, might be of less concern.One testable prediction of this model is that UV mutagenesisin mut^- strains independent of UmuC function should not requireother SOS functions. Another prediction, that MutS-like proteinsspecifically bind to mismatched but not to matched photoproducts,has been confirmed for both human hMutS ${alpha}$ protein (MU et al. 1997; WANG et al. 1999 ) and E. coli MutS protein (H. WANG andJ. B. HAYS, unpublished observations).

ACKNOWLEDGMENTS

We thank Claire Cupples, Patricia Foster, Martin Marinus, JeffreyMiller, and Roger Woodgate for providing bacterial strains,Rick Bockrath, Chris Lawrence, and Roger Woodgate for adviceon the manuscript, and Cliff Pereira, Oregon State University,for valuable help with statistical analyses. This work was supportedby American Cancer Society grant RPG-96-074-03-CNE to J.B.H.This is technical report 11552 from the Oregon AgriculturalExperiment Station.

Manuscript received April 13, 1999; Accepted for publication October 1, 1999.

LITERATURE CITED

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

ALLEN, D. J., A. MAKHOV, M. GRILLEY, J. TAYLOR, and R. THRESHER et al., 1997 MutS mediates heteroduplex formation by a translocation mechanism. EMBO J. 14:4467-4470.

BANERJEE, S. K., R. B. CHRISTENSEN, C. W. LAWRENCE, and J. E. LECLERC, 1988 Frequency and spectrum of mutations produced by a single cis-syn thymine-thymine cyclobutane dimer in a single-stranded vector. Proc. Natl. Acad. Sci. USA 85:8141-8145[Abstract/Free Full Text].

BRIDGES, B. A. and R. J. MUNSON, 1968 Evidence for the mechanism of base change mutation by ultraviolet light in a strain deficient in excision-repair. Proc. R. Soc. Lond. Ser B 171:213-226[Medline].

CAILLET-FAUQUET, P. and G. MAENHAUT-MICHEL, 1988 Nature of the SOS mutator activity: genetic characterization of untargeted mutagenesis in Escherichia coli.. Mol. Gen. Genet. 213:491-498[Medline].

CARTY, M. P., J. HAUSER, A. S. LEVINE, and K. DIXON, 1993 Replication and mutagenesis of UV-damaged DNA templates in human and monkey cell extracts. Mol. Cell. Biol. 13:533-547[Abstract/Free Full Text].

CHRISTENSEN, J. R., J. E. LECLERC, P. V. TATA, R. B. CHRISTENSEN, and C. W. LAWRENCE, 1988 UmuC function is not essential for the production of all targeted lacI mutations induced by ultraviolet light. J. Mol. Biol. 203:635-641[Medline].

CHRISTENSEN, R. B., J. R. CHRISTENSEN, I. KOENIG, and C. W. LAWRENCE, 1985 Untargeted mutagenesis induced by UV in the lacI gene of Escherichia coli.. Mol. Gen. Genet. 201:30-34[Medline].

COOPER, D. L., R. S. LAHUE, and P. MODRICH, 1993 Methyl-directed mismatch repair is bidirectional. J. Biol. Chem. 268:11823-11829[Abstract/Free Full Text].

CROWLEY, D. J. and P. C. HANAWALT, 1998 Induction of the SOS response increases the efficiency of global nucleotide excision repair of cyclobutane pyrimidine dimers, but not 6-4 photoproducts, in UV-irradiated Escherichia coli.. J. Bacteriol. 180:3345-3352[Abstract/Free Full Text].

CUPPLES, C. G. and J. H. MILLER, 1988 Effects of amino acid substitutions at the active site in Escherichia coli ß-galactosidase. Genetics 120:637-644[Abstract/Free Full Text].

CUPPLES, C. G. and J. H. MILLER, 1989 A set of lacZ mutations in Escherichia coli that allow rapid detection of each of the six base substitutions. Proc. Natl. Acad. Sci. USA 86:5345-5349[Abstract/Free Full Text].

CUPPLES, C. G., M. CABRERA, C. CRUZ, and J. H. MILLER, 1990 A set of lacZ mutations in Escherichia coli that allow rapid detection of specific frameshift mutations. Genetics 125:275-280[Abstract].

DRUMMOND, J. T., A. ANTHONEY, R. BROWN, and P. MODRICH, 1996 Cisplatin and adriamycin resistance are associated with MutL ${alpha}$ and mismatch repair deficiency in an ovarian tumor cell line. J. Biol. Chem. 271:19645-19648[Abstract/Free Full Text].

DUCKETT, D. R., J. T. DRUMMOND, A. I. H. MURCHIE, J. T. REARDON, and A. SANCAR et al., 1996 Human MutS ${alpha}$ recognizes damaged DNA basepairs containing O⁶-methylguanine, O⁴-methylthymine, or the cisplatin-d(GPG) adduct. Proc. Natl. Acad. Sci. USA 93:6443-6447[Abstract/Free Full Text].

ECHOLS, H., 1982 Mutation rate: some biological and biochemical considerations. Biochemie 64:571-575[Medline].

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].

FEINSTEIN, S. I. and K. B. LOW, 1986 Hyper-recombining recipient strains in bacterial conjugation. Genetics 113:13-33[Abstract/Free Full Text].

FENG, G., H.-C. T. TSUI, and M. WINKLER, 1996 Depletion of the cellular amounts of MutS and MutH methyl-directed mismatch-repair proteins in stationary-phase Escherichia coli K-12 cells. J. Bacteriol. 178:2388-2396[Abstract/Free Full Text].

FENG, W.-Y. and J. B. HAYS, 1995 DNA structures generated during mismatch repair of nonreplicating phage DNA in Escherichia coli: requirements for helicase, exonuclease, RecF and RecBCD functions. Genetics 140:1175-1186[Abstract].

FENG, W.-Y., E. LEE, and J. B. HAYS, 1991 Recombinagenic processing of UV-light photoproducts in nonreplicating phage DNA by the Escherichia coli methyl-directed mismatch repair system. Genetics 129:1007-1020[Abstract].

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].

FOSTER, P. L., 1999 Are adaptive mutations due to a decline in mismatch repair? The evidence is lacking. Mutat. Res. 436:179-184[Medline].

HARRIS, R. S., G. FENG, K. J. ROSS, R. SIDHU, and C. THULIN et al., 1997 Mismatch repair protein MutL becomes limiting during stationary-phase mutation. Genes Dev. 11:2426-2437[Abstract/Free Full Text].

HUMAYUN, M. Z., 1998 SOS and Mayday: multiple inducible mutagenic pathways in Escherichia coli. Mol. Microbiol. 30:905-910[Medline].

JIANG, N. and J.-S. TAYLOR, 1993 In vivo evidence that UV induced C $->$ T mutations at dipyrimidine sites could result from the replicative bypass of cis-syn cyclobutane dimers or their deamination products. Biochemistry 32:472-481[Medline].

KAT, A., W. G. THILLY, W.-H. FANG, M. J. LONGLEY, and G.-M. LI et al., 1993 An alkylation-tolerant mutator cell line is deficient in strand-specific mismatch repair. Proc. Natl. Acad. Sci. USA 90:6424-6428[Abstract/Free Full Text].

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].

KORNBERG, A., and T. A. BAKER, 1992 DNA Replication. W. H. Freeman and Company, New York.

KUNZ, B. A. and B. W. GLICKMAN, 1984 The role of pyrimidine dimers as premutagenic lesions: a study of targeted vs. untargeted mutagenesis in the lacI gene of Escherichia coli. Genetics 106:347-364[Abstract/Free Full Text].

LAHUE, R. S., K. G. AU, and P. MODRICH, 1989 DNA mismatch correction in a defined system. Science 245:160-164[Abstract/Free Full Text].

LI, G.-M., H. WANG, and L. J. ROMANO, 1996 Human MutS ${alpha}$ specifically binds to DNA containing aminofluorene and acetylaminofluorene adducts. J. Biol. Chem. 271:24084-24088[Abstract/Free Full Text].

MELLON, I. and G. N. CHAMPE, 1995 Products of DNA mismatch repair genes mutS and mutL are required for transcription-coupled nucleotide excision repair of the lactose operon in Escherichia coli.. Proc. Natl. Acad. Sci. USA 93:1292-1297[Abstract/Free Full Text].

MELLON, I., D. K. RAJPAL, M. KOI, C. R. BOLAND, and G. N. CHAMPE, 1996 Transcription-coupled repair deficiency and mutations in human mismatch repair genes. Science 272:557-560[Abstract].

MILLER, J. H., (Editor), 1972 Experiments in Molecular Genetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, NY.

MILLER, J. H., 1985 Mutational specificity of ultraviolet light. J. Mol. Biol. 182:45-68[Medline].

MU, D., M. TURSUN, D. R. DUCKETT, J. T. DRUMMOND, and P. MODRICH et al., 1997 Recognition and repair of compound DNA lesions (base damage and mismatch) by human mismatch repair and excision repair systems. Mol. Cell. Biol. 17:760-769[Abstract].

NAPOLITANO, R. L., I. B. LAMBERT, and R. P. P. FUCHS, 1997 SOS factors involved in translesion synthesis. Proc. Natl. Acad. Sci. USA 94:5733-5738[Abstract/Free Full Text].

OHMORI, H., E. HATADA, Y. QIAO, M. TSUJI, and R. FUKUDA, 1995 dinP, a new gene in Escherichia coli, whose product shows similarities to UmuC and its homologs. Mutat. Res. 347:1-7[Medline].

PENG, W. and B. R. SHAW, 1996 Accelerated deamination of cytosine residue in UV-induced cyclobutane dimers leads to CC $->$ TT transitions. Biochemistry 35:10172-10181[Medline].

PERSON, S., W. MCCLOSKEY, W. SNIPES, and R. BOCKRATH, 1974 Ultraviolet mutagenesis and its repair in Escherichia coli strain containing a nonsense codon. Genetics 78:1035-1049[Abstract/Free Full Text].

PETIT, M. A., J. DIMPFL, M. RADMAN, and H. E. ECHOLS, 1991 Control of large chromosomal duplications in E. coli by the mismatch repair system. Genetics 129:327-332[Abstract].

RAYSSIGUIER, C., D. S. THALER, and M. RADMAN, 1989 The barrier to recombination between Escherichia coli and Salmonella typhimurium is disrupted in mismatch-repair mutants. Nature 342:396-401[Medline].

SCHAAPER, R. M. and M. RADMAN, 1989 The extreme mutator effect of Escherichia coli mutD5 results from saturation of mismatch repair by excessive DNA replication errors. EMBO J. 8:3511-3516[Medline].

SELBY, C. P. and A. SANCAR, 1993 Molecular mechanism of transcription-repair coupling. Science 260:53-58[Abstract/Free Full Text].

SELBY, C. P. and A. SANCAR, 1995 Structure and function of transcription-repair coupling factor. I. Structural domains and binding properties. J. Biol. Chem. 270:4882-4889[Abstract/Free Full Text].

SELBY, C. P., E. M. WITKIN, and A. SANCAR, 1991 Escherichia coli mutant deficient in "mutation frequency decline" lacks strand-specific repair: in vitro complementation with purified coupling factor. Proc. Natl. Acad. Sci. USA 88:11574-11578[Abstract/Free Full Text].

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].

SWANN, P., T. R. WATERS, D. C. MOULTON, Y.-Z. XU, and M. EDWARDS et al., 1996 Role of postreplicative DNA mismatch repair in cytotoxic action of thioguanine. Science 273:1109-1111[Abstract].

TESSMAN, I., S.-K. LIU, and M. A. KENNEDY, 1992 Mechanism of SOS mutagenesis of UV-irradiated DNA: mostly error-free processing of deaminated cytosine. Proc. Natl. Acad. Sci. USA 89:1159-1163[Abstract/Free Full Text].

THOMAS, D. C. and T. A. KUNKEL, 1993 Replication of UV-irradiated DNA in human cell extracts—evidence for mutagenic bypass of pyrimidine dimers. Proc. Natl. Acad. Sci. USA 90:7744-7753[Abstract/Free Full Text].

WANG, H., C. W. LAWRENCE, G.-M. LI, and J. B. HAYS, 1999 Specific binding of human MSH2·MSH6 mismatch-repair protein heterodimers to DNA incorporating thymine- or uracil-containing UV-light photoproducts opposite mismatched bases. J. Biol. Chem. 274:16894-16900[Abstract/Free Full Text].

WITKIN, E. M., 1966 Radiation-induced mutations and their repair. Science 252:1345-1353.

WORTH, L. J., S. CLARK, M. RADMAN, and P. MODRICH, 1994 Mismatch repair proteins MutS and MutL inhibit RecA-catalyzed strand transfer between diverged DNAs. Proc. Natl. Acad. Sci. USA 91:3238-3241[Abstract/Free Full Text].

WU, T. H. and M. G. MARINUS, 1994 Dominant-negative mutations in the mutS gene of Escherichia coli.. J. Bacteriol. 176:5393-5400[Abstract/Free Full Text].

YAJIMA, H., M. TAKO, S. YASUHIRA, J. H. ZHAO, and C. ISCHII et al., 1995 A eukaryotic gene encoding an endonuclease that specifically repairs DNA damaged by ultraviolet light. EMBO J. 14:2393-2399[Medline].

ZIEG, J. and S. R. KUSHNER, 1977 Analysis of recombination between two partially deleted lactose operons of Escherichia coli K-12. J. Bacteriol. 131:123-132[Abstract/Free Full Text].

This article has been cited by other articles:

H. Park, K. Zhang, Y. Ren, S. Nadji, N. Sinha, J.-S. Taylor, and C. Kang
Crystal structure of a DNA decamer containing a cis-syn thymine dimer
PNAS, December 10, 2002; 99(25): 15965 - 15970.
[Abstract] [Full Text] [PDF]