©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
Lagging Strand DNA Synthesis at the Eukaryotic Replication Fork Involves Binding and Stimulation of FEN-1 by Proliferating Cell Nuclear Antigen (*)

(Received for publication, July 10, 1995)

Xiangyang Li (1)(§) Jun Li (2) John Harrington (2) Michael R. Lieber (2) Peter M. J. Burgers (1)(¶)

From the  (1)Departments of Biochemistry, Molecular Biophysics, and (2)Pathology, Washington University School of Medicine, St. Louis, Missouri 63110

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

The 5` 3`-exonuclease domain of Escherichia coli DNA polymerase I is required for the completion of lagging strand DNA synthesis, and yet this domain is not present in any of the eukaryotic DNA polymerases. Recently, the gene encoding the functional and evolutionary equivalent of this 5` 3`-exonuclease domain has been identified. It is called FEN-1 in mouse and human cells and RTH1 in Saccharomyces cerevisiae. This 42-kDa enzyme is required for Okazaki fragment processing. Here we report that FEN-1 physically interacts with proliferating cell nuclear antigen (PCNA), the processivity factor for DNA polymerases and . Through protein-protein interactions, PCNA focuses FEN-1 on branched DNA substrates (flap structures) and on nicked DNA substrates, thereby stimulating its activity 10-50-fold but only if PCNA can functionally assemble as a toroidal trimer around the DNA. This interaction is important in the physical orchestration of lagging strand synthesis and may have implications for how PCNA stimulates other members of the FEN-1 nuclease family in a broad range of DNA metabolic transactions.


INTRODUCTION

In eukaryotic cells, a family of structure-specific endonucleases can be defined based on conserved domains within FEN-1 (flap endonuclease), a 42-kDa enzyme that is both a 5` flap DNA endonuclease and a nick specific 5`-exonuclease(1) . The Saccharomyces cerevisiae analog of FEN-1 is encoded by the RTH1 gene (2, 3) . Both human and yeast FEN-1 (yFEN-1) (^1)are highly homologous to the human DNA repair gene XP-G and its yeast homologue RAD2(4) . Various DNA metabolic processes are thought to require processing of intermediates by the FEN-1 endonuclease. The enzyme shows the greatest activity as an endonuclease on nicked double-stranded DNA substrates with the 5`-end of the nick expanded into a single-stranded tail (see structure in Fig. 2A), cutting these so-called flap structures at the base of the tail(5) . These types of DNA intermediates likely occur during end joining reactions in which DNA ends with limited homology are joined. Mammalian FEN-1 has also been identified as DNase IV, or maturation factor I, a nick-specific 5` 3`-exonuclease required for nick translation during Okazaki fragment maturation(6, 7, 8, 9, 10) . Consistent with its corresponding functional activity, mammalian FEN-1 shows sequence homology with the 5` 3`-exonuclease domain present in Escherichia coli DNA polymerase I(10) . The yeast RTH1 gene is dispensable for cell growth, but rth1 deletion mutants are temperature-sensitive for growth and show a terminal phenotype consistent with a defect in DNA replication(2, 3) . Genetic studies with yeast rth1 deletion mutants have also shown that FEN-1 functions in the repair of alkylation damage and in recombinational repair. However, yFEN-1 (RTH1) does not function in nucleotide excision repair(2, 3) . Rather, in vitro studies have shown that the endonucleolytic activity of XP-G (the mammalian homologue of RAD2) is required for this repair process(11) .


Figure 2: PCNA stimulates yFEN-1 endonuclease activity on a flap substrate. A, diagram of a DNA flap substrate. The position of the label is indicated by the asterisk on the flap strand, SC5. Oligonucleotides are: SC1, CAGCAACGCAAGCTTG (strand adjacent to the flap strand); SC3, GTCGACCTGCAGCCCAAGCTTGCGTTGCTG (strand annealed to the flap and the adjacent strand); and SC5, ATGTGGAAAATCTCTAGCAGGCTGCAGGTCGAC (flap strand, which is the one labeled) (see (1) for a full description). The 5` ends are indicated. B, stimulation of yFEN-1 endonuclease by PCNA. The endonuclease assay was done in a 15-µl total volume containing 50 mM Tris-HCl, pH 8.0, 10 mM MgCl(2), 0.5 mM beta-mercaptoethanol, 500 µg/ml BSA, 10 fmol of flap substrate, 50 fmol of FEN-1, and, when present, 26,000 fmol as trimer of PCNA (2.3 µg), 30 fmol of RF-C, and 100 µM ATP. C, mutant PCNA fails to stimulate. The assay was done as in panelB, but the PCNA concentration was varied as indicated. pcna-52, which is a monomer in solution, was added at the indicated level. Products of the reaction were separated on a denaturing 15% polyacrylamide gel and visualized on a PhosphorImager. The mobility of the top band is 33 nucleotides and that of the cleaved product is 20 nucleotides. Control experiments showed no detectable nuclease activity by PCNA alone (data not shown).



The yeast proliferating cell nuclear antigen (PCNA) is the processivity factor for DNA polymerases and . It is a homotrimer with a subunit molecular mass of 29 kDa and is highly conserved from yeast to mammalian cells. The crystal structure of yeast PCNA shows that the trimer forms a closed ring with the appropriate dimensions and electrostatic properties to encircle double-stranded DNA and to interact with it using nonspecific contacts(12) . Processivity in DNA synthesis is achieved by protein-protein interactions between PCNA and the polymerase, thereby tethering the DNA polymerase at the primer terminus(13) . In addition to this structural function during the elongation phase of DNA replication, mammalian PCNA, through its interactions with the cyclin-dependent protein kinase inhibitor p21 (CIP1/WAF1/SDI1), has also been implicated in cell cycle control(14, 15) . In this communication we show that PCNA physically interacts with FEN-1 and sequesters it to its site of action, thereby stimulating the activity of FEN-1 10-50-fold.


EXPERIMENTAL PROCEDURES

Materials

The yeast strains used were PY26 (Mata, ura3-52, leu2-3, 112,trp1Delta, prb1-1122, prc1-407, pep4-3, Deltanuc1::LEU2) and its Deltarth1 derivative PY59 (as PY26, but Deltarth1::hisG), which was made by insertional activation of the RTH1 gene using plasmid pR2.10(3) . Strains were grown and extracts prepared and concentrated with 0.35 g/ml ammonium sulfate as described(16) . E. coli single-stranded DNA binding protein, yeast FEN-1, and yeast PCNA were overproduced in E. coli and purified as described(1, 17) . Yeast replication factor C (RF-C) was purified as described(18) . PCNA or bovine serum albumin was coupled to Affi-Gel 10 (Bio-Rad) according to the manufacturer's protocol. Beads contained 3 mg of PCNA/ml of beads or 4 mg of BSA/ml of beads.

Two-hybrid Analysis

The entire POL30 gene or pol30-52 gene (containing the S115P mutation) was fused to the bacterial lexA DNA binding domain in vector pCH435(17) . Screening of a library of yeast cDNAs fused to the GAL4 activation domain using the lexA-pol30-52 construct as bait was carried out essentially as described(19) . In the one positive RTH1 isolate obtained, fusion with the activation domain of GAL4 occurred at amino acid 81. The strength of the interaction was 2.5 units of beta-galactosidase activity for lexA-POL30 and 2.2 units for lexA-pol30-52, whereas negative controls were 0.5-0.8 units of beta-galactosidase activity.

Affinity Binding to Beads

BSA or PCNA beads (3 µl) were gently agitated in a thin walled 0.5-ml microcentrifuge tube with 10 ng of yFEN-1 in 100 µl of 40 mM Hepes-NaOH, pH 7.4, 2 mM MgCl(2), 150 mM NaCl (buffer A) at 4 °C for 1 h. The bottom of the tube was pierced with a 27-gauge needle and the solvent gently spun out in a clinical centrifuge. The beads were washed with 2 times 10 µl of buffer A and eluted with 2 times 3 µl of buffer A containing 0.3 M NaCl, 2 times 3 µl of buffer A containing 0.6 M NaCl, and finally 2 times 3 µl of buffer A containing 1% SDS, each time by pipetting the buffer on top of the beads and after 5 min at 0 °C, gently spinning through. Proteins in the fractions were separated on a 10% polyacrylamide gel containing sodium dodecyl sulfate and subjected to immunoblot analysis using immunopurified rabbit antisera to yFEN-1 for detection.


RESULTS AND DISCUSSION

The RTH1 gene was isolated by us as a PCNA-interacting gene using the yeast two-hybrid method(20) . In this search for interacting genes, the bacterial lexA DNA binding domain was fused to a cold-sensitive PCNA mutant (pol30-52) rather than to the wild-type POL30 gene as strains with the latter construct grew poorly and had a very low transformation frequency(17) . The measured interaction signals between POL30-lexA or pol30-52-lexA and RTH1 fused to the GAL4 activation domain were identical and weak (see ``Experimental Procedures''). As the two-hybrid method may detect both direct and indirect interactions, we turned to biochemical methods to investigate a possible interaction between yFEN-1 and PCNA.

The existence of a specific protein-protein interaction between yFEN-1 and PCNA was confirmed by affinity chromatography on PCNA beads. Yeast FEN-1 bound specifically to PCNA beads but not to control BSA beads (Fig. 1A). Elution from the PCNA beads was accomplished at 0.6 M NaCl, indicating that salt bridges contribute substantially to the PCNA-FEN-1 interaction. Subsequent treatment with ionic detergents did not release additional yFEN-1 (Fig. 1A). The specificity of the interaction was demonstrated by the observation that an excess of PCNA blocked binding of yFEN-1 to the beads (Fig. 1B). As expected from the observed in vivo interaction between yFEN-1 and the mutant pcna-52 by the two-hybrid method, an excess of the latter mutant protein also blocked the binding of yFEN-1 to PCNA beads. Finally, we showed that the beads can bind yFEN-1 from crude yeast extracts. That the species detected on the Western blot is yFEN-1 follows from its comigration with purified yFEN-1 and the absence of a signal with Deltarth1 extracts (Fig. 1C). Although yFEN-1 is not the major polypeptide species from crude extracts bound to PCNA beads, it can be detected as a distinct band on silver stained gels, which is absent when extracts are used from an isogenic Deltarth1 strain (data not shown).


Figure 1: Immunoblot analysis of yFEN-1 binding to PCNA beads. A, fractionation of yFEN-1 on BSA or PCNA beads. See ``Experimental Procedures'' for details. B, competition assay. The assay was as described, except that yFEN-1 was preincubated for 10 min at 4 °C with 100 µg of BSA (lane1) or 30 or 100 µg of PCNA (lanes2 and 4) or 30 or 100 µg of pcna-52 (lanes3 and 5) in 100 µl of buffer A prior to addition of PCNA beads. The 0.6 M NaCl eluate was analyzed. C, PCNA beads bind yFEN-1 in crude extracts. Extracts (500 µg) were incubated with 10 µl of PCNA beads in 200 µl of buffer A, washed, and eluted with a total of 20 µl of buffer A containing 0.6 M NaCl as described. Lane1, 15 ng of purified FEN-1; lane2, 10 ng of FEN-1 plus 10 µl of 0.6 M NaCl eluate from strain PY26; lane3, 10 µl of eluate from strain PY26; lane4, 10 µl of eluate from strain PY59.



The functional interaction between yFEN-1 and PCNA was probed with DNA substrates that are probable intermediates in DNA end joining (flap structures, Fig. 2A) and in DNA replication (nicked duplexes). On a model flap structure, PCNA stimulated the activity of yFEN-1 about 10-fold (Fig. 2B) based on PhosphorImager quantitation. It is important to note that, in contrast to assays with nicked substrates described below, only PCNA and yFEN-1 were added in this assay. Therefore, stimulation of yFEN-1 activity can be directly attributed to its interaction with PCNA rather than with other accessory factors. Stimulation requires that PCNA is a trimer. The pcna-52 mutant exists as a monomer in solution(17) . Despite the fact that this mutant protein exhibits a similar affinity for yFEN-1 as wild-type PCNA, it failed to stimulate yFEN-1 activity (Fig. 2C; see also Fig. 1B). The most straightforward conclusion of these experiments is that PCNA must encircle the double-stranded DNA in order to stimulate yFEN-1, and the mutant form is unable to do so. Because this mode of PCNA loading occurs by nonspecific diffusion onto DNA ends, a large excess is required to observe substantial stimulation(21) . Thus, at the lowest concentration of PCNA tested (0.02 µg), which represents a 20-fold molar excess over DNA substrate, very little stimulation was observed (Fig. 2C). RF-C is required for the efficient loading of PCNA at primer termini in an ATP-dependent manner(18, 22, 23, 24) . If RF-C would efficiently and appropriately load PCNA at flap structures one would expect to observe stimulation of yFEN-1 activity at PCNA levels stoichiometric with DNA substrate. However, inclusion of RF-C and ATP in the nuclease assay did not give a significant further stimulation of yFEN-1 beyond that observed by PCNA alone, either at high concentrations of PCNA (Fig. 2B) or at low concentrations of PCNA, which show only minimal stimulation (data not shown). Possibly, RF-C fails to recognize the flap structure as a docking site for PCNA. Or, alternatively, PCNA loaded by RF-C is on the wrong double-stranded side of the flap structure necessary for yFEN-1 stimulation. These observations with the yeast enzymes were extended to the human system. Human PCNA stimulated the endonucleolytic activity of human FEN-1 on the flap structure substrate to a similar degree (data not shown).

In contrast to these results with flap substrates, we observed no obvious stimulation of yFEN-1 activity by PCNA on model oligonucleotides containing a nick (data not shown). (^2)PCNA is known to slide rapidly across linear DNA molecules(25) . As the more rapid sliding of PCNA across these small linear double-stranded DNA substrates, in comparison to the sterically hindered flap substrates, might not provide a significant mean residence time for PCNA in order to interact productively with yFEN-1, we turned to circular DNA substrates from which PCNA, once loaded, would not be able to dissociate (Fig. 3). RF-C and ATP are absolutely required to load PCNA at primer termini of circular substrates(21) . In agreement with these known properties of PCNA, we observed stimulation of yFEN-1 activity by PCNA but only if RF-C and ATP were also present. Interestingly, the inclusion of salt (75 mM NaCl) in the assay revealed the functional interaction between PCNA and yFEN-1 most profoundly. As PCNA is efficiently loaded by RF-C onto the DNA at physiological salt levels, it in turn is capable of loading yFEN-1 and hence stimulating its activity (Fig. 3). In the absence of PCNA, yFEN-1 fails to interact with the DNA at these salt concentrations, and a modification of the assay to very low salt and magnesium concentrations is essential to detect yFEN-1 activity at nicks(5) . No stimulation was observed with the monomeric mutant pcna-52 (data not shown).


Figure 3: Stimulation of FEN-1 by PCNA at DNA nicks. A 5`-labeled 24-mer oligonucleotide and a 36-mer oligonucleotide, representing positions 6353-6330 and 6329-6294, respectively, were hybridized to single-stranded mp18 DNA (upperstructure). Assays were as described in the legend to Fig. 2, except for adjustment to 10 mM Tris, pH 8, 5 mM MgCl(2), and 75 mM NaCl. In a 15-µl total volume, 20 fmol of substrate coated with 400 ng of E. coli single-stranded DNA binding protein and, where indicated, 100 fmol of FEN-1, 1300 fmol of PCNA, 30 fmol of RF-C, and 100 µM ATP were incubated for 10 min at 30 °C. Analysis was as described in the legend to Fig. 2. The topband is the labeled 24-nucleotide oligonucleotide. The bottomband (arrow) is the released 5` mononucleotide. Control experiments showed no nuclease activity in all analogous experiments lacking FEN-1 (data not shown).



The interaction between FEN-1 and PCNA may have bearing on the structure of the lagging strand DNA replication complex. Because FEN-1 does not negatively affect DNA synthesis by DNA polymerase or holoenzyme (i.e. does not compete with these polymerases for binding to PCNA), (^3)it may form an integral part of this complex and mediate coupled synthesis and maturation of Okazaki fragments (Fig. 4). In the presence of DNA polymerase or , the complex would carry out nick translation until DNA ligase I seals the nick(9) . In mammalian cells, an RNase H is also required for in vitro Okazaki fragment maturation(7, 26) . However, it is not known at this time whether this enzyme forms an integral component of this maturation complex.


Figure 4: Hypothetical positioning of PCNA and FEN-1 at recombinational flap intermediates (left) and during Okazaki fragment maturation (right). RF-C and polymerase are also shown in the Okazaki fragment model. Indicated contacts with PCNA are based on physical and functional interaction studies.



In addition to replication, the interaction between FEN-1 and PCNA may have broader implications in DNA metabolism as well. In nucleotide excision repair, for example, PCNA has been shown to play an important role(27, 28) . Although FEN-1 likely is not involved in this reaction, a highly homologous structure-specific nuclease, XP-G or RAD2, is absolutely required. Based on the involvement of PCNA in nucleotide excision repair and the presence of homology between FEN-1 and RAD2, it is possible that PCNA may also interact with RAD2 to facilitate its loading and thereby excision of damaged nucleotides. Thus, there may be a common theme in various aspects of DNA metabolism, in addition to DNA replication, in which a processivity factor stimulates a structure-specific nuclease in processing nicked and branched DNA intermediates.

Based on the studies here, we conclude that the functional interaction between PCNA and FEN-1 is important in the orchestration of lagging strand processing at the eukaryotic DNA replication fork. The interaction of PCNA with other FEN-1 family members may be generally important to a wide variety of transactions involving branched DNA intermediates.


FOOTNOTES

*
This work was supported in part by Grants GM32431 (to P. M. J. B.) and CA51105 and GM43236 (to M. R. L.) from the National Institutes of Health. The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
Present address: Dept. of Biochemistry, University of Washington School of Medicine, Seattle, WA.

To whom correspondence should be addressed. Tel.: 314-362-3872; Fax: 314-362-7183; burgers{at}bcserv.wustl.edu.

(^1)
The abbreviations used are: yFEN-1, yeast FEN-1; PCNA, proliferating cell nuclear antigen; RF, replication factor; BSA, bovine serum albumin.

(^2)
PCNA stimulation assays were carried out at various salt levels, either with or without RF-C and ATP. The maximum observed stimulation was about 1.5-fold.

(^3)
DNA polymerase holoenzyme assays were carried out as described in (18) with subsaturating levels of PCNA (3 ng, 35 fmol). Addition of a 20-fold molar excess of FEN-1 (30 ng, 700 fmol) inhibited the reaction by about 10%.


ACKNOWLEDGEMENTS

We thank John Majors and Tim Lohman for critical discussions, and Louise and Satya Prakash for a gift of plasmid pR2.10 for making a RTH1 deletion strain.


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©1995 by The American Society for Biochemistry and Molecular Biology, Inc.