A Uve1p-Mediated Mismatch Repair Pathway in Schizosaccharomyces pombe

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Molecular and Cellular Biology, July 1999, p. 4703-4710, Vol. 19, No. 7
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

A Uve1p-Mediated Mismatch Repair Pathway in Schizosaccharomyces pombe

Balveen Kaur,¹^,² J. Lee A. Fraser,³ Greg A. Freyer,⁴ Scott Davey,³^,⁵ and Paul W. Doetsch¹^,⁶^,^*

Department of Biochemistry¹ and Division of Biological and Biomedical Sciences,² Graduate Program in Biochemistry and Cell and Developmental Biology, and Division of Cancer Biology, Department of Radiation Oncology,⁶ Emory University, School of Medicine, Atlanta, Georgia 30322; Department of Pathology³ and Departments of Oncology and Biochemistry,⁵ Queen's University, Kingston, Ontario K7L 3N6, Canada; and Department of Environmental Health Sciences, School of Public Health, and Department of Anatomy and Cell Biology, Columbia University, New York, New York 10032⁴

Received 11 January 1999/Returned for modification 10 March 1999/Accepted 8 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

UV damage endonuclease (Uve1p) from Schizosaccharomyces pombe was initially described as a DNA repair enzyme specific forthe repair of UV light-induced photoproducts and proposed as theinitial step in an alternative excision repair pathway. Here wepresent biochemical and genetic evidence demonstrating that Uve1pis also a mismatch repair endonuclease which recognizes and cleavesDNA 5' to the mispaired base in a strand-specific manner. Thebiochemical properties of the Uve1p-mediated mismatch endonucleaseactivity are similar to those of the Uve1p-mediated UV photoproductendonuclease. Mutants lacking Uve1p display a spontaneous mutatorphenotype, further confirming the notion that Uve1p plays a rolein mismatch repair. These results suggest that Uve1p has a surprisinglybroad substrate specificity and may function as a general typeof DNA repair protein with the capacity to initiate mismatch repairin certainorganisms.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

There are multiple processes by which DNA single-base mismatches are produced in cells. The most common of these is the misincorporationof nucleotides by DNA polymerase during replication. Mismatchescan also arise following deamination of cytosine to uracil, formingU/G mispairs, or upon recombination between homeologous sequences(30). To correct this type of DNA anomaly, cells have developedseveral mechanisms for mismatch repair (MMR) that are essentialfor maintaining the integrity of the genome. In addition to mediatingthe repair of single base mismatches, MMR functions in maintainingthe stability of simple DNA repeat tracts during replication includinginsertions caused by slippage loops in the primer strand and deletionscaused by failure to repair loops in the template strand. In Escherichiacoli, several different MMR pathways have been identified, andthese have served as models in other organisms. The E. coli MutHLS(long-patch MMR) system repairs all single-base mispairs exceptC/C mismatches (28). Repair is initiated by binding of MutSand MutL to the mismatch, followed by a MutH-mediated incisionof the nonmethylated DNA strand at hemimethylated GATC sites.The nicked strand is then degraded past the site of mismatch,and DNA polymerase fills in the resulting gap (28, 33, 37).The very short patch MMR system of E. coli recognizes G/T mismatchesat sites where cytosine is methylated by the Dcm methylase andrestores them to G/C pairs (25, 26, 49). This pathway requiresthe Vsr endonuclease in addition to MutS and MutL (18). A thirdtype of mismatch correction in E. coli is mediated by the MutYprotein, which initiates conversion of A/G mispairs to C/G pairsby an N-glycosylase and an associated apurinic/apyrimidinic lyaseactivity (32).

Biochemical and genetic studies have demonstrated that eukaryotes possess nick-directed MMR capabilities which appear to besimilar in a number of respects to the E. coli long-patch MMRsystem (11, 29). Most of our current information concerningeukaryotic MMR has come from studies of Saccharomyces cerevisiaeand humans. S. cerevisiae possesses numerous genes encoding proteinswith similarities to E. coli MutS and MutL, but only a subsetof these (MSH2, MSH6, PMS1, and MLH1) are thought to functionas bona fide base MMR proteins (7). Other S. cerevisiae homologs,such as MSH3, MSH4, and MSH5, are thought to function in looprepair and/or recombination. In addition, non-MutS/MutL homologssuch as RTH1 (RAD27) and EXO1 appear to function in loop repair(7). In humans, at least six different genes have been identifiedthat encode proteins related to the bacterial MutS and MutL proteins.The products of inherited mutations in four of these genes (MSH2,MLH1, PMS1, and PMS2) are associated with hereditary nonpolyposiscolon cancer and confer microsatellite sequence instability incells containing such mutations (5, 13, 22, 31). Thus,in both S. cerevisiae and humans, there are a variety of proteinswhich likely function in several different pathways for the repairof single-base mismatches and loops for the maintenance of genomicstability.

The fission yeast Schizosaccharomyces pombe has also served as a useful model system for eukaryotic DNA repair systems. Incontrast to S. cerevisiae and humans, much less is known aboutMMR in S. pombe. The mutL homolog pms1 has been recently identified(14, 36). Disruption of the S. pombe pms1 gene confers a spontaneousmutator phenotype, reduction of spore viability, and a increasein postmeiotic segregation, indicating that it plays a role inMMR (36). Two other genes, swi4 and swi8, are homologs of S.cerevisiae MSH3 and MSH2, respectively, and it has been proposedthat they may mediate roles in loop repair and, in the case ofswi8, correction of single-base mismatches (7). S. pombe exonuclease1 (encoded by the exo1 gene) is a meiotically induced 5'-to-3'double-stranded DNA exonuclease, is a homolog of the S. cerevisiaeEXO1 gene product, and has been proposed to play a role in mutationavoidance and MMR (38-40). Genetic analysis of meiotic recombinationevents has indicated the existence of at least two pathways responsiblefor MMR in S. pombe: a major, long-patch MMR system (mediatedby msh1 and pms1) which recognizes all mismatch combinations exceptC/C; and a minor, short-patch MMR system which recognizes allcombinations, including C/C mismatches (34, 35). Further supportfor these observations was provided by the discovery of two distinctmismatch-binding activities in S. pombe crude cell extracts (15).Recently, the S. pombe nucleotide excision repair (NER) genesrhp14, swi10, and rad16 (homologs of the S. cerevisiae RAD14,RAD10, and RAD1 genes, respectively) have been identified as componentsof the short-patch MMR system and function independently of msh2pms1 (16). Taken together, the available genetic and limitedbiochemical data suggest that S. pombe possesses multiple pathwaysfor conductingMMR.

We (4, 10, 17) and others (45, 48) have described an alternative excision repair pathway which exists in S. pombeand was proposed to be highly specific for cyclobutane pyrimidinedimers (CPDs) and 6-4 photoproducts (6-4PPs), the major toxicand mutagenic UV light-induced DNA photoproducts. UV damage endonuclease(Uve1p; also called UVDE), the enzyme initiating this alternativeexcision repair pathway, incises duplex DNA immediately 5' tothe sites of damage (4, 20). The S. pombe gene uve1, encodingthis protein, as well as two similar genes from Neurospora crassaand Bacillus subtilis have been identified, indicating that thisrepair pathway exists in both prokaryotes and eukaryotes (8,41, 42). Recently, we reported the overexpression, purification,and initial enzymological characterization of G $Delta$ 228-Uve1p, a fullyactive, truncated form of Uve1p (20). Because CPDs and 6-4PPsdiffer significantly with respect to the structural distortionsthat they induce in duplex DNA, it seemed reasonable to expectthat Uve1p might recognize other types of DNA damage. A recentreport on the thermodynamic and base-pairing properties of DNAdodecamer duplexes containing CPDs and 6-4PPs at sites of adjacentthymines (TT) indicate that proper Watson-Crick base pairing withthe opposite AA is disrupted for both of these photoproducts (19).These observations raised the possibility that Uve1p recognizessingle base mismatches resulting in disruption of normal Watson-Crickbase pairing in duplexDNA.

In the present study, we report a novel mismatch endonuclease activity in S. pombe mediated by Uve1p. We present biochemicaland genetic evidence indicating that Uve1p, an enzyme previouslyconsidered to be involved exclusively in the repair of UV-inducedDNA photoproducts, is an initiating enzyme in an S. pombe MMRpathway. These results suggest that Uve1p (i) has a broad substratespecificity range, (ii) may be the initiating repair enzyme fora general excision repair pathway, and (iii) is likely to be acomponent of MMR pathways that exist in both prokaryotes andeukaryotes.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Strains and vectors. S. cerevisiae DY150 (Clontech) was used for protein expression. The S. cerevisiae expression vector pYEX4T-1 was obtainedfrom Clontech. S. pombe strains used in this study were 972 (h^S) (24), PRS301 (h^S pms1::ura4⁺) (36), and Sp30 (h^S ade6-210 leu-32 ura4-D18) (9). Sp362 (h^S ade6-210 leu1-32 ura4-D18 uve1::ura4⁺) was constructed by transforming Sp30 with a linearized, genomicuve1⁺ fragment derived from pgUV2 (8) in which nucleotides 215 (EcoRI)to 1045 (ClaI) of uve1⁺ were replaced with the ura4⁺ gene. Extracts of Sp362 contained no detectable Uve1p activityagainst CPD-30mer (data not shown). Cultures were grown in pombeminimal medium (24) with glutamate (3.75 g/liter) replacingammonium chloride as the nitrogen source (12) supplemented with150 mg each of adenine, leucine, and uracil per liter (PMALU^g). Solid medium was prepared by addition of agar (20 g/liter).L-Canavanine sulfate was sterilized prior to addition to themedium.

Purification of Uve1p and other mismatch endonucleases. GFL-Uve1p and G $Delta$ 228-Uve1p (full-length and truncated Uve1p fused to glutathione S-transferase [GST]) were cloned and expressedin the pYEX4T-1 S. cerevisiae expression system to generate N-terminalGST-Uve1p fusion proteins as previously described (20). G $Delta$ 228-Uve1pwas purified by glutathione-Sepharose affinity chromatographyas previously described (20). GFL-Uve1p was found to rapidlylose activity following this purification step and was subsequentlyused in experiments as a crude extract preparation which showedgreater stability. S. cerevisiae cells transformed with vectoralone (expressing the GST tag only) were subjected to a parallelpurification procedure, with the resulting GST used as a controlfor possible contaminating activities copurified from the expressionsystem. Thrombin cleavage of G $Delta$ 228-Uve1p to generate $Delta$ 228-Uve1pfollowed by purification was carried out as previously described(20). Purified mismatch repair endonuclease, E. coli endonucleaseV (44), was a gift from Yoke Wah Kow (Atlanta, Ga.).

Uve1p substrate preparations. The CPD-30mer Uve1p substrate (20) containing a centrally embedded, cis-syn TT CPD was a gift from John-Stephen Taylor (St.Louis, Mo.). All other oligonucleotide substrates (Table 1) formismatch endonuclease experiments were synthesized by Operon,Inc. (Alameda, Calif.), or IDT, Inc. (Coralville, Iowa). All oligonucleotideswere gel purified and subjected to DNA sequence analysis for sequenceconfirmation. Oligonucleotides were 5' end labeled with polynucleotidekinase (PNK) by using 50 µCi of [ $gamma$ -³²P]ATP (3,000 Ci/mmol; Amersham) as previously described (4).3'-end-labeled oligonucleotides were prepared by incubating 10pmol of the indicated oligonucleotide with 10 U of terminal deoxynucleotidyltransferase(TdT; Promega) and 50 µCi of [ $alpha$ -³²P]ddATP (3,000 Ci/mmol; Amersham) as previously described (4).

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TABLE 1. Base mismatch- and CPD-containing oligonucleotides used in this study

Uve1p activity assays. Reactions with G $Delta$ 228-Uve1p were carried out by incubating approximately 100 fmol of labeled oligonucleotide substrate with100 to 150 ng of purified G $Delta$ 228-Uve1p in 20 mM HEPES (pH 6.5)-10mM MgCl₂-1 mM MnCl₂-150 mM NaCl for 20 min at 37°C (10 to 20 µl,final volume). Reactions with crude preparations of GFL-Uve1pwere carried out with 20 to 30 µg of cell extract incubated withthe appropriate substrate in 20 mM HEPES (pH 7.5)-100 mM NaCl-10mM MgCl₂-1 mM MnCl₂ at 37°C for 20 min. The reaction productswere processed by extraction with an equal volume of phenol-chloroform-isoamylalcohol (25:24:1), ethanol precipitation, resuspension, and analysison 20% denaturing (7 M urea) polyacrylamide (DNA sequencing) gelsas previously described (20). The DNA species correspondingto the uncleaved substrate and Uve1p-mediated DNA strand scissionproducts were analyzed and quantified by PhosphorImager (MolecularDynamics model 445SI) analysis andautoradiography.

Kinetics experiments were carried out with 331 nM G $Delta$ 228-Uve1p and 5 to 50 nM *CX/AY-31mer under otherwise standard reactionconditions (described above) for 0 to 5 min at 37°C. The apparentK_m and K_cat values were determined from Lineweaver-Burk plotsof averaged data from three individualexperiments.

5'-terminal analysis. G $Delta$ 228-Uve1p was incubated with 3'-end-labeled *CX/AY-31mer under standard reaction conditions at 37°C for 20 min. The ethanol-precipitatedreaction products were incubated with 10 U of calf intestinalphosphatase (CIP; Promega) at 37°C for 30 min or with 10 U ofT4 PNK (New England Biolabs) and 50 pmol of ATP as previouslydescribed (4). The reaction products were analyzed on 20% denaturingpolyacrylamide gels as described above for Uve1p activity assays.Differences in electrophoretic mobilities between kinase-treatedand untreated DNA strand scission products indicated the presenceor absence of a preexisting 5'-phosphoryl group (4).

3'-terminal analysis. To determine the chemical nature of the 3' terminus of GST $Delta$ 228-Uve1p-mediated DNA strand scission products, 5'-end-labeled*CX/AY-31mer was incubated with G $Delta$ 228-Uve1p as described above.The ethanol-precipitated, resuspended reaction products were thentreated with 10 U of TdT and ddATP as previously described (4).Samples were processed and analyzed on polyacrylamide gels asdescribed above for 5'-terminalanalysis.

Establishment of optimal pH for mismatch endonuclease activity. To determine the pH optimum for Uve1p-mediated mismatch cleavage, 100 fmol of 3'-end-labeled *CX/AY-31mer was incubated withapproximately 100 ng of G $Delta$ 228-Uve1p plus 10 mM MgCl₂ and 1 mMMnCl₂ in 20 mM reaction buffers varying in pH sodium citrate (pH3.0 to 6.0), HEPES KOH (pH 6.5 to 8.0), and sodium carbonate (pH9.0 to 10.6). The reaction products were analyzed on a 20% denaturingpolyacrylamide gel, and the optimal pH was calculated as previouslydescribed for Uve1p cleavage of CPD-30mer (20).

Substrate competition assay. End-labeled *CX/AY-31mer was generated by annealing 3'-end-labeled CX with unlabeled strand AY. Unlabeled nonspecific (nonmismatch)competitor GX/CY-31mer was made by annealing strand GX to strandCY, resulting in a duplex oligonucleotide with a G/C base pairinstead of a C/A mispair. Unlabeled CX/AY-31mer, a mismatch-containingspecific competitor, was generated as described above. CPD-30mer,a well-characterized substrate for Uve1p, was used as an additionalunlabeled, putative specific competitor. 3'-end-labeled *CX/AY-31mer(0.1 pmol) was incubated with 100 ng of purified G $Delta$ 228-Uve1p andincreasing amounts (0.1 to 2.0 pmol) of either putative specific(CX/AY-31mer or CPD-30mer) or nonspecific (GX/CY-31mer) competitor.The competition reactions were processed and analyzed on 20% denaturinggels as described above. The DNA species corresponding to theuncleaved *CX/AY-31mer and the DNA strand scission products werequantified by PhosphorImager (Molecular Dynamics model 445SI)analysis.

Colony formation assays for canavanine resistance. To determine sensitivity to L-canavanine, 10 ml of PMALU^g was inoculated with 100 µl of the indicated saturated culture andgrown to mid-log phase at 25°C; 200 cells were plated onto PMALU^g plates with various concentrations of L-canavanine sulfate (0,0.075, 0.22, 0.75, 2.2, 7.5, 22, and 75 µg/ml), and incubatedat 30°C. Colonies were counted after 4 days, and viability wasnormalized against the 0-g/ml plate for each strain. Colony formationassays (mutation frequency) were conducted for each strain byplating 10⁷ cells from saturated cultures onto 24 PMALU^g plates supplemented with L-canavanine sulfate (75 µg/ml). Colonieswere counted after 8 days of incubation at 30°C. Mean mutationfrequencies were calculated by the method of the median (23).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

G $Delta$ 228-Uve1p recognizes 12 possible base mismatch combinations. Previously, we reported that an overexpressed, GST-tagged version of Uve1p (G $Delta$ 228-Uve1p) containing an N-terminal 228-amino-aciddeletion is active on UV photoproducts (CPDs and 6-4PPs) and stablein a purified form (20). In contrast, overexpressed GST-tagged,full length Uve1p (GFL-Uve1p) was found to be active and stablein crude preparations but rapidly lost activity following purification.Because of substantial structural differences between CPDs and6-4PPs, it is not obvious what features of damaged DNA Uve1p recognizes.One possibility is that Watson-Crick base pairing is disruptedfor the 3' pyrimidines in both CPDs and 6-4PPs, suggesting thatUve1p might target its activity to mispaired bases in duplex DNA(19). We therefore investigated the ability of purified G $Delta$ 228-Uve1pto cleave duplex oligonucleotides containing all possible combinationsof single-base mispairs embedded within the same flanking sequencecontext. For these studies, we used a collection of mismatch-containingoligonucleotides (series XY-31mer) which were designed so as togenerate all possible mismatch combinations (Table 1). StrandsGX, AX, TX, and CX were 3' end labeled and then annealed to strandGY, AY, TY, or CY prior to incubation with purified G $Delta$ 228-Uve1p.Reaction products were analyzed on DNA sequencing-type gels (Materialsand Methods). The ability of G $Delta$ 228-Uve1p to cleave all 12 possiblemispair combinations is shown in Fig. 1. No DNA strand cleavagewas observed for duplex substrates containing normal Watson-CrickG/C or A/T base pairs.

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FIG. 1. G $Delta$ 228-Uve1p recognizes 12 different base mismatch combinations. The 3'-end-labeled oligonucleotide series X/Y-31mer (sequence given at bottom; asterisk indicates labeled strand and labeled terminus) was used to assess Uve1p cleavage activity on 16 different base pair and base mispair combinations (Table 1). Base mispairs are indicated above numbered lanes, with asterisks denoting bases on the labeled strand for G series (A), A series (B), C series (C), and T series (D) treated with purified G $Delta$ 228-Uve1p (odd-numbered lanes) or mock reactions (even-numbered lanes). Reaction products were analyzed on DNA sequencing-type gels. Arrows indicate Uve1p cleavage sites immediately (arrow a) and one (arrow b) and two (arrow c) nucleotides 5' to the mismatch site. G and C+T base-specific chemical cleavage DNA sequencing ladders were run in adjacent lanes as nucleotide position markers.

The sites of G $Delta$ 228-Uve1p-mediated mismatch-specific DNA cleavage were identified in each case by comparing the electrophoreticmobilities of the DNA strand scission products to those of a DNAsequencing ladder obtained by base-specific chemical cleavage.Arrows a, b, and c indicate the DNA strand scission products correspondingto cleavage by G $Delta$ 228-Uve1p immediately (position 0), one (position $-$ 1), or two (position $-$ 2) nucleotides 5' to the site of the mismatch,respectively (Fig. 1). These sites of G $Delta$ 228-Uve1p-mediated endonucleolyticcleavage were confirmed in similar experiments using 5'-end-labeledGX, AX, TX, and CX strands in the mismatch substrates (not shown).In addition, GFL-Uve1p (in crude cell extracts) recognized andcleaved *CX-AY-31mer in the same manner as G $Delta$ 228-Uve1p (Fig. 2B).The preferred sites of cleavage and the efficiency with whicheach mismatch is recognized by G $Delta$ 228-Uve1p is variable and dependson the type of base mispair presented to the enzyme. Within thesequence context examined, G $Delta$ 228-Uve1p exhibited strong cleavageat the *C/C (asterisk denotes labeled strand base) site and at*C/A and *G/G sites (30 to 40% cleavage of substrate relativeto that observed for CPD-30mer), moderate cleavage at *G/A, *A/G,and *T/G sites (10 to 25% cleavage relative to CPD-30mer), andweak cleavage at *G/T, *A/A, *A/C, *C/T, *T/T, and *T/C sites(5 to 10% cleavage relative to CPD-30mer). These differences inthe extent of cleavage were reproducible and observed in threeseparate experiments. These results suggest that the G $Delta$ 228-Uve1pmismatch endonuclease activity may have a preference for certainbase mismatch combinations (e.g., *C/A) over others (e.g., *T/C).However, these experiments do not rule out the possibility thatthe extent of cleavage observed is also influenced by the sequenceflanking the mismatch.

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FIG. 2. Nature of Uve1p-generated DNA strand scission products and activity of full-length Uve1p. (A) Analysis of 5' termini of Uve1p-generated DNA cleavage products with *CX/AY-31mer. 3'-end-labeled oligonucleotide with C/A mismatch (sequence on bottom) was reacted with G $Delta$ 228-Uve1p and then further treated with PNK or CIP as indicated. Lane 1 represents buffer treatment only. X* indicates base mismatch site. Arrows a and b indicate sites of Uve1p cleavage. (B) Full-length Uve1p possesses mismatch endonuclease activity. 5'-end-labeled duplex *CX/AY-31mer was incubated with crude extracts of cells expressing either GFL-Uve1p (lane 1) or G $Delta$ 228-Uve1p (lane 2) and cells expressing the GST tag alone (lane 3) or with E. coli endonuclease (Endo) V, a known mismatch endonuclease (lane 4). Arrows indicate cleavage sites immediately (arrow a) and one nucleotide (arrow b) 5' to the mismatch site. Arrow V indicates E. coli endonuclease V cleavage 3' to the mismatch site and was used as a position reference. Bands below arrows (indicated by asterisks) correspond to shortened products due to a weak 3'-to-5' exonuclease activity present in the Uve1p preparations (see text for details). Reaction products on DNA sequencing-type gels were analyzed as described for Fig. 1.

Kinetic studies were carried out with G $Delta$ 228-Uve1p and *CX/AY-31mer (Materials and Methods). The K_m and K_cat values were determinedto be 390 nM and 2.2 min¹, respectively. In comparison to the kinetic parameters of G $Delta$ 228-Uve1pfor CPD-30mer (20), the K_m for *CX/AY-31mer is 8-fold higherand the K_cat is 10-fold higher, indicating that although G $Delta$ 228-Uve1pbinding to the mismatch-containing substrate is weaker than bindingto a CPD-containing substrate, the catalytic efficiency of theenzyme is higher for the *CX/AY-31mersubstrate.

Nature of the Uve1p mismatch endonuclease-generated DNA cleavage products. Uve1p has been shown to incise DNA containing CPDs and 6-4PPs directly 5' to the photoproduct site, generating products containing3'-hydroxyl and 5'-phosphoryl groups (4). We wished to determinewhether similar 3' and 5' termini were produced following Uve1p-mediatedcleavage of base mismatch-containing substrates. To study this,the DNA strand scission products generated by G $Delta$ 228-Uve1p cleavageof 3'-end-labeled *CX/AY-31mer (CX strand labeled) (Table 1)were further treated with CIP, which removes 5'-terminal phosphorylgroups from substrate DNA. The major sites of Uve1p-mediated DNAcleavage relative to the base mispair site were found to be atpositions 0 and $-$ 1 (Fig. 2A, lane 2). CIP treatment of these DNAcleavage products resulted in species that had retarded electrophoreticmobilities compared to non-CIP-treated DNA cleavage products,indicating a decrease in charge corresponding to removal of 5'-terminalphosphoryl groups (Fig. 2A, lanes 2 and 3). In addition, G $Delta$ 228-Uve1pmismatch endonuclease-generated DNA cleavage products were resistantto phosphorylation by PNK, an expected result if the 5' terminialready contain phosphoryl groups (Fig. 2A, lane 4). Electrophoreticmobility shift analysis utilizing 5'-end-labeled *CX/AY-31mer,TdT, and [ $alpha$ -³²P]ddATP) resulted in addition of a single ddAMP to the 3' endof G $Delta$ 228-Uve1p-generated DNA cleavage products and indicates thepresence of a 3'-hydroxyl terminus (data not shown). We concludefrom these results that the 3' and 5' termini of the productsof G $Delta$ 228-Uve1p-mediated cleavage of substrates containing single-basemismatches are identical to those generated following cleavageof substrates containing CPDs or 6-4PPs.

To verify that the Uve1p mismatch endonuclease activity observed was not the result of trace endonucleolytic contaminationfrom the S. cerevisiae expression system and to determine whetherfull-length Uve1p was also capable of mismatch endonuclease activity,extracts from cells overexpressing GFL-Uve1p, G $Delta$ 228-Uve1p, andGST tag alone were tested for their abilities to cleave 5'-end-labeled*CX/AY-31mer. Both GFL-Uve1p and G $Delta$ 228-Uve1p cleaved the basemismatch-containing substrate at positions 0, $-$ 1, and $-$ 2 (Fig.2B). We also observed a weak 3'-to-5' exonucleolytic activityassociated with both crude GFL-Uve1p preparations and purifiedG $Delta$ 228-Uve1p which shortened the Uve1p-mediated cleavage productsby one to three nucleotides (Fig. 2B, lanes 1 and 2). These shorterproducts are not due to additional cleavages by Uve1p mismatchendonuclease activity, as they are not observed in identical experimentswith 3'-end-labeled substrates (not shown). Purified $Delta$ 228-Uve1pobtained following thrombin cleavage of the GST tag also possessedmismatch endonuclease activity (data not shown). In contrast,no cleavage of mismatch-containing substrates was observed whenextracts from cells transfected with vector expressing only theGST tag were tested. We conclude from these results that GFL-Uve1pand its more stable, truncated version, G $Delta$ 228-Uve1p, both possessmismatch endonucleaseactivities.

G $Delta$ 228-Uve1p mismatch endonuclease and G $Delta$ 228-Uve1p UV photoproduct endonuclease exhibit similar properties and compete for the same substrates. We have previously reported that G $Delta$ 228-Uve1p requires divalent cations for activity and exhibits optimal activity againstUV photoproducts in the presence of 10 mM MgCl₂ and 1 mM MnCl₂(19). Omission of divalent cations from the reaction bufferresulted in abolishing G $Delta$ 228-Uve1p mismatch endonuclease activityon 5'-end-labeled *CX/AY-31mer (Fig. 3). The pH optimum for G $Delta$ 228-Uve1pmismatch endonuclease activity on this same substrate was foundto be 6.5 (not shown), which corresponds to the pH where optimalactivity is observed against UV photoproducts (20).

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FIG. 3. G $Delta$ 228-Uve1p requires divalent cations for mismatch recognition. 5'-end-labeled duplex *CX/AY-31mer was incubated with G $Delta$ 228-Uve1p (lanes 1 and 4) or buffer only (control [CON]; lanes 2 and 5) in the presence (lanes 1 and 2) or absence (lanes 4 and 5) of Mn²⁺. C* indicates base mismatch site. Arrows a and b indicate Uve1p cleavage positions. E. coli endonuclease (Endo) V-reacted oligonucleotide (arrow v, lane 3) and C+T and G+A sequencing ladders included as nucleotide position markers are marked. Bands below arrow b (indicated by asterisks) correspond to shortened products due to 3'-to-5' exonuclease activity (described in the legend to Fig. 2).

To further confirm that the mismatch endonuclease activity was mediated by G $Delta$ 228-Uve1p, a substrate competition experimentwas performed with CPD-30mer, a known Uve1p substrate which containsa centrally located UV photoproduct (CPD). Addition of increasingamounts of unlabeled CPD-30mer resulted in a significant, concentration-dependentdecrease in G $Delta$ 228-Uve1p-mediated mismatch endonuclease activityagainst 3'-end-labeled *CX/AY-31mer (C/A mispair) (Fig. 4). Incontrast, increasing amounts of the undamaged GX/CY-31mer (G/Cbase pair) had only a modest inhibitory effect and did not increasewith increasing amounts of added oligonucleotide, indicating nonspecificbinding to Uve1p within this concentration range. Increasing amountsof added, unlabeled CX/AY-31mer showed a moderate inhibition butwas not as effective as CPD-30mer. The effective competition byCPD-30mer for mismatch endonuclease activity suggests that bothbase mismatch and UV photoproduct endonuclease activities areassociated with G $Delta$ 228-Uve1p.

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FIG. 4. G $Delta$ 228-Uve1p mismatch endonuclease and G $Delta$ 228-Uve1p UV photoproduct endonuclease compete for the same substrates. G $Delta$ 228-Uve1p was incubated with 3'-end-labeled duplex *CX/AY-31mer (Table 1) in the presence of increasing amounts of unlabeled duplex CPD-30mer (squares), duplex GX/CY-31mer (triangles), or duplex CX/AY-31mer (circles). The Uve1p-mediated DNA cleavage products were analyzed on DNA sequencing gels, and the extent of strand scission was quantified by PhosphorImager analysis (Materials and Methods). Uve1p activity is expressed as percentage of the cleavage observed relative to that observed in the absence of any competitor (defined as 100% activity). The error bars indicate the mean ± standard deviation from three separate experiments.

Uve1p incises only one strand of a duplex containing a base mismatch. Since Uve1p recognizes all possible base mismatch combinations, it was of interest to determine whether the enzyme could inciseboth strands on the same molecule, resulting in a DNA double-strandbreak. To investigate this, an oligonucleotide (*CX/AY-41mer)was designed such that the base mispair was placed in the centerof the oligonucleotide. G $Delta$ 228-Uve1p was incubated with 3'-end-labeled*CX/AY-41mer under standard conditions, and the DNA strand scissionproducts were analyzed on both nondenaturing and denaturing gels(Fig. 5). In the event that G $Delta$ 228-Uve1p created a DNA double-strandbreak by incising 5' to the base mismatch site on the two complementarystrands, the resulting products would be similar in electrophoreticmobility to those created by the restriction enzyme DdeI (whichcleaves adjacent to the mismatch) when analyzed on a nondenaturingpolyacrylamide gel. In contrast, if G $Delta$ 228-Uve1p incises on either(but not both) complementary strand, then the resulting productwould be a full-length duplex containing a single-strand nickwhich would comigrate with uncut duplex *CX/AY-41mer on a nondenaturinggel. Nondenaturing gel analysis of G $Delta$ 228-Uve1p-treated *CX/AY-41mergenerated a product with an electrophoretic mobility identicalto that of the untreated duplex with no products detected, correspondingto those created by a double-strand break (Fig. 5A). Denaturinggel analysis revealed a G $Delta$ 228-Uve1p-generated DNA strand scissionproduct resulting from a single-strand break of the labeled strandof either *CX/AY-41mer or CX/*AY-41mer. Together with the nondenaturinggel analysis, these results indicate that within the G $Delta$ 228-Uve1psubstrate population, nicks occur on one or the other strand butnot both strands (Fig. 5B). We conclude from these results thatG $Delta$ 228-Uve1p is capable of nicking only one of the two strandscontaining a base mismatch and does not make double-strand breaksin duplex DNA.

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FIG. 5. Uve1p incises only one strand of a duplex containing a base mismatch. (A) 3'-end-labeled *CX/AY-41mer was incubated with restriction enzyme DdeI (lane 1), G $Delta$ 228-Uve1p (lane 2), or buffer (lane 3). The reaction products were analyzed on a nondenaturing gel as described in the text for the presence of DNA double-strand break products (arrow dsb). Arrows b and c indicate the primary cleavage site for Uve1p on this substrate. (B) 3'-end-labeled *CX/AY-41mer or CX/*AY-41mer was incubated with G $Delta$ 228-Uve1p (+ lanes) or buffer ( $-$ lanes) and analyzed on denaturing, DNA sequencing-type gels as described in the text. Arrows b and c indicate positions of major Uve1p cleavage events relative to the mismatched base (asterisk) position. G+A and C+T base-specific sequencing ladders are included in outside lanes as nucleotide position markers.

uve1 null mutants exhibit a mutator phenotype. We have examined the spontaneous mutation rate of uve1::ura4⁺ disruption mutants as assayed by the ability to form coloniesresistant to the toxic arginine analog L-canavanine. Uptake ofL-canavanine in S. pombe is mediated by an arginine permease encodedby the can1⁺ gene (12). Mutations in can1⁺ eliminate the uptake of L-canavanine, and mutant cells are ableto form colonies on medium supplemented with L-canavanine, whereaswild-type cells cannot. We have compared the rates of spontaneousmutagenesis at the can1⁺ locus in uve1::ura4⁺ disruption mutants (Sp362) to those of both a negative control(wild-type strain 972) and a positive control, pms1::ura4⁺ (Materials and Methods). The pms1 gene product is a homolog ofE. coli MutL, and loss of pms1 causes a strong mitotic mutatorphenotype and increased postmeiotic segregation (36).

To determine the relative sensitivity of each yeast strain to L-canavanine, 200 cells from mid-log-phase cultures were platedonto PMALU^g plates supplemented with increasing concentrations of L-canavanine.The strains were equally sensitive to L-canavanine (not shown).All strains were viable in the presence of lower concentrationsof L-canavanine up to and including 2.2 µg/ml, while concentrationshigher than this were toxic to all strains. However, the colonieswhich grew in the presence of 2.2 µg of L-canavanine per ml weresmaller in diameter than the colonies which grew in the presenceof lowerconcentrations.

The mean mutation rate of each of these strains was examined by fluctuation analysis. Single colonies from PMALU^g medium were used to inoculate liquid cultures which were grownto saturation; 10⁷ cells were plated onto PMALU^g plates containing 75 µg of L-canavanine sulfate per ml, and thecanavanine-resistant colonies were counted after incubation at30°C for 8 days. We determined the number of colonies on 12 separateplates for each of three experiments; the data are summarizedin Table 2. Both uve::ura4⁺ and pms::ura4⁺ strains showed an elevated number of resistant colonies comparedto the wild type. The mutation rates (Table 2) for wild-type,uve1::ura4⁺, and pms::ura4⁺ strains were calculated by the method of the median (23). Theuve1::ura4⁺ mutants have a mutation rate approximately 6.5-fold higher thanthat of the wild type and 2-fold lower than that of the pms::ura4⁺ strain, indicating that loss of Uve1p confers a mutator phenotypeupon cells.

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TABLE 2. Spontaneous mutation rates of uve1 and pms1 null mutants

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

It has been recognized for a number of years that the repair of the major UV photoproducts, CPDs and 6-4PPs, in S. pombe ismediated by more than one excision repair pathway. The evidencefor this was initially based on the finding that S. pombe NERmutants were still proficient in the removal of both CPDs and6-4PPs from genomic DNA (27). The discovery of the Uve1p-mediatedexcision repair pathway provided a biochemical basis for theseobservations (4, 41). Subsequent investigations showed thatmutants lacking NER and Uve1p were highly sensitive to UV lightand were deficient for removal of CPDs and 6-4PPs from DNA (48).The discovery that Uve1p could recognize both CPDs and 6-4PPs,DNA lesions which induce quite different structural distortionsin duplex DNA, raised the issue of the structural basis for DNAdamage recognition by Uve1p. One possible explanation came froma recent thermodynamic and base-pairing study that compared structuresof matched and mismatched DNA dodecamer duplexes containing cis-synCPD and 6-4PP of TT (19). The covalent interaction between adjacentbases in the dimer pair prevents the 3' pyrimidine from pairingcorrectly with the complementary base. Such disruption of Watson-Crickbase pairing provided a possible explanation for the structuraldistortion recognized by Uve1p. Hence we tested the ability ofUve1p to incise DNA containing all 12 possible base mismatch combinationsand found that each was a substrate for thisenzyme.

The finding that Uve1p recognizes all potential DNA base mispair combinations indicates that, in addition to its UV photoproductcleavage activity, it is a diverse mismatch endonuclease withbroad substrate specificity. In this regard, Uve1p is similarto E. coli endonuclease V (43), an S. cerevisiae and human "all-type"mismatch endonuclease (6, 46), and calf thymus topoisomeraseI (47), which also recognize all potential base mismatch combinations.These enzymes incise DNA at each of the 12 base mispairs withvariable efficiencies and either to the 5' (human all-type mismatchendonuclease) or 3' (E. coli endonuclease V) sides of a mismatch.Uve1p shows a preference for *C/C and *C/A mispairs, a propertysimilar to that of the human all-type mismatch endonuclease (46).In contrast, the strong preference of Uve1p for *G/G mispairsis a property which distinguishes Uve1p from all other mismatchendonucleases identified to date. The biochemical properties ofUve1p-mediated mismatch cleavage and the spontaneous mutator phenotypedisplayed by uve1 null mutants suggest that Uve1p is involvedin MMR in vivo. Uve1p-generated incision 5' to the base mismatchsite could be followed by a 5'-to-3' exonuclease activity suchas that mediated by S. pombe exonuclease I (40) or the FEN-1homolog Rad2p (1), followed by resynthesis andligation.

S. pombe possesses at least two distinct MMR systems; the relationship of Uve1p to either of these is not known at present,nor is it known whether Uve1p functions in a distinct MMR system.The proposed major MMR pathway does not recognize C/C mismatchesand has relatively long (approximately 100-nucleotide) repairtracts (34). Uve1p is thought to participate in a relativelyshort patch repair process which utilizes Rad2p (a FEN-1 homolog)DNA polymerase $delta$ , DNA ligase, and accessory factors (1, 2).Based on these properties, it is unlikely that Uve1p is involvedin a long-tract MMR system. The second, presumably less frequentlyutilized pathway recognizes all potential base mismatch combinationsand has a repair tract length of about 10 nucleotides (34).Recently, this second pathway, which recognizes C/C mismatches,was shown to be mediated by the NER proteins Rhp14p, Swi10p, andRad16p, which function in damage recognition and incision (16).Based on these observations, our results suggest that Uve1p maymediate a third, distinct MMR system in S. pombe.

To further address the role of Uve1p in MMR, we tested whether a mutant lacking Uve1p activity had an increased spontaneousmutation frequency, a predictable phenotype associated with MMRdeficiencies (22). A uve1::ura4⁺ disruption strain was found to possess a mutator phenotype inthe L-canavanine resistance assay, although at levels slightlylower than that observed for a pms1::ura4⁺ disruption strain. In the mutation fluctuation analysis, a widerrange of mutant colonies was observed for uve1::ura4⁺ than for pms1::ura4⁺, suggesting that the pathways leading to mutation due to eliminationof uve1 and pms1 are likely to be mechanisticallydifferent.

What is the structural basis for lesion recognition by Uve1p? Previous studies with Uve1p have focused exclusively on itsrole in the repair of UV light-induced DNA damage, resulting inthe notion that this enzyme functions in the repair of UV photoproductsexclusively. In view of the findings reported here, it might bedesirable to consider renaming this enzyme to reflect its overallproperties. The results of this study clearly indicate a muchbroader involvement of Uve1p in S. pombe DNA repair and suggestthat many other types of DNA lesions may be recognized by thisversatile repair protein. For example, we have recently foundthat Uve1p recognizes and incises DNA substrates containing uracil,dihydrouracil, cis-platinum-induced adducts, as well as smallbase bulges (3, 21). The molecular basis for substrate recognitionby Uve1p is not obvious but could in part be due to disruptionof normal Watson-Crick base pairing and the corresponding changesexpected in the electronic characteristics of the major and minorgrooves of B-DNA. Structural studies of Uve1p associated withits substrates would provide important information regarding howthis enzyme recognizes and accesses DNAdamage.

	ACKNOWLEDGMENTS

We thank Angela Avery, Yoke Wah Kow, and Gerald Shadel for helpfuldiscussions.

This work was supported by NIH grants CA73041 (P.W.D.), CA72647 (G.A.F.), and ES07940 (G.A.F. and S.D.) and by Medical ResearchCouncil of Canada grant MT-14352 (S.D.) S.D. is a Cancer CareOntario Scientist. J.L.A.F. is a Queen's University R. S. McLaughlinFellow.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry, 4123 Rollins Research Center, Emory University, Schoolof Medicine, Atlanta, GA 30322. Phone: (404) 727-0409. Fax: (404)727-3954. E-mail: medpwd{at}emory.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Alleva, J. L., and P. W. Doetsch. 1998. Characterization of Schizosaccharomyces pombe Rad2 protein, a FEN-1 homolog. Nucleic Acids Res. 26:3645-3650[Abstract/Free Full Text].
2.	Alleva, J. L., and P. W. Doetsch. Unpublished data.
3.	Avery, A. M., B. Kaur, J. S. Taylor, J. A. Mello, J. M. Essigmann, and P. W. Doetsch. Substrate specificity of ultraviolet DNA endonuclease (UVDE/Uve1p) from Schizosaccharomyces pombe. Nucleic Acids Res., in press.
4.	Bowman, K. K., K. Sidik, C. A. Smith, J. S. Taylor, P. W. Doetsch, and G. A. Freyer. 1994. A new ATP-independent DNA endonuclease from Schizosaccharomyces pombe that recognizes cyclobutane pyrimidine dimers and 6-4 photoproducts. Nucleic Acids Res. 22:3026-3032[Abstract/Free Full Text].
5.	Bronner, C. E., S. M. Baker, P. T. Morrison, G. Warren, L. G. Smith, M. K. Lescoe, M. Kane, C. Earabino, J. Lipford, and A. Lindblom. 1994. Mutation in the DNA mismatch repair gene homologue hMLH1 is associated with hereditary non-polyposis colon cancer. Nature 368:258-261[Medline].
6.	Chang, D. Y., and A. L. Lu. 1991. Base mismatch-specific endonuclease activity in extracts from Saccharomyces cerevisiae. Nucleic Acids Res. 19:4761-4766[Abstract/Free Full Text].
7.	Crouse, G. F. 1998. Mismatch repair systems in Saccharomyces cerevisiae, p. 411-448. In J. A. Nickoloff, and M. F. Hoekstra (ed.), DNA repair in prokaryotes and lower eukaryotes, vol. 1. DNA damage and repair. Humana Press, Inc., Totowa, N.J.
8.	Davey, S., M. L. Nass, J. V. Ferrer, K. Sidik, A. Eisenberger, D. L. Mitchell, and G. A. Freyer. 1997. The fission yeast UVDR DNA repair pathway is inducible. Nucleic Acids Res. 25:1002-1008[Abstract/Free Full Text].
9.	Davey, S., C. S. Han, S. A. Ramer, J. C. Klassen, A. Jacobsen, A. Eisenberger, K. M. Hopkins, H. B. Lieberman, and G. A. Freyer. 1998. Fission yeast rad12⁺ regulates cell cycle checkpoint control and is homologous to the Bloom's syndrome disease gene. Mol. Cell. Biol. 18:2721-2728[Abstract/Free Full Text].
10.	Doetsch, P. W. 1994. What's old is new: an alternative DNA excision repair pathway. Trends Biochem. Sci. 20:384-386.
11.	Fang, W. H., and P. Modrich. 1993. Human strand-specific mismatch repair occurs by a bidirectional mechanism similar to that of the bacterial reaction. J. Biol. Chem. 268:11838-11844[Abstract/Free Full Text].
12.	Fantes, P., and J. Creanor. 1984. Canavanine resistance and the mechanism of arginine uptake in the fission yeast Schizosaccharomyces pombe. J. Gen. Microbiol. 130:3265-3273.
13.	Fishel, R., M. K. Lescoe, M. R. Rao, N. G. Copeland, N. A. Jenkins, J. Garber, M. Kane, and R. Kolodner. 1993. The human mutator gene homolog MSH2 and its association with hereditary nonpolyposis colon cancer. Cell 75:1027-1038[Medline].
14.	Fleck, O., H. Michael, and L. Heim. 1992. The swi4⁺ gene of Schizosaccharomyces pombe encodes a homologue of mismatch repair enzymes. Nucleic Acids Res. 20:2271-2278[Abstract/Free Full Text].
15.	Fleck, O., P. Schar, and J. Kohli. 1994. Identification of two mismatch-binding activities in protein extracts of Schizosaccharomyces pombe. Nucleic Acids Res. 22:5289-5295[Abstract/Free Full Text].
16.	Fleck, O., E. Lehmann, P. Schar, and J. Kohli. 1999. Involvement of nucleotide excision repair in msh2 pms1-independent mismatch repair. Nat. Genet. 21:314-317[Medline].
17.	Freyer, G. A., S. Davey, J. V. Ferrer, A. M. Martin, D. Beach, and P. W. Doetsch. 1995. An alternative eukaryotic DNA excision repair pathway. Mol. Cell. Biol. 15:4572-4577[Abstract].
18.	Hennecke, F., H. Kolmar, K. Brundl, and H. J. Fritz. 1991. The vsr gene product of E. coli K-12 is a strand- and sequence-specific DNA mismatch endonuclease. Nature 353:776-778[Medline].
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