©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
Structure-Function Relationship of the Eukaryotic DNA Replication Factor, Proliferating Cell Nuclear Antigen (*)

(Received for publication, February 2, 1995; and in revised form, May 25, 1995)

Kotaro Fukuda (1) (2) Hiroshi Morioka (1) Sayuri Imajou (1)(§) Soichiro Ikeda (1) Eiko Ohtsuka (1) Toshiki Tsurimoto (2)(§)(¶)

From the  (1)Faculty of Pharmaceutical Sciences, Hokkaido University, Sapporo 060, Japan and the (2)Institute for Molecular and Cellular Biology, Osaka University, Yamada-oka, Suita, Osaka 565, Japan

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS and DISCUSSION
CONCLUSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

Proliferating cell nuclear antigen (PCNA) is essential for eukaryotic DNA replication and functions as a processivity factor of DNA polymerase (pol ). Due to the functional and structural similarity with the beta-subunit of Escherichia coli DNA polymerase III, it has been proposed that PCNA would act as a molecular clamp during DNA synthesis. By site-directed mutagenesis and biochemical analyses, we have studied the functional domains of human PCNA required for stimulation of replication factor C (RF-C) ATPase and DNA synthesis by pol . Short deletions from either the N or C termini caused drastic changes in extraction and chromatographic behaviors, suggesting that both of these terminal regions are crucial to fold the tertiary structure of PCNA. The short C-terminal stretch from Lys to Glu is necessary for stimulation of RF-C ATPase activity, but not for stimulation of DNA synthesis by pol . Nine basic amino acids that are essential for activating DNA synthesis by pol are positioned at the internal alpha-helices of PCNA. This result is in good agreement with the observation that PCNA has a ring structure similar to the beta-subunit and clamps a template DNA through this positively charged internal surface. Several other charged amino acids are also required to stimulate either RF-C ATPase or pol DNA synthesis. Some of them are positioned at loops which are exposed on one of the side surface of PCNA adjacent to the C-terminal loop. In addition, the beta-sheets composing the intermolecular interface of the trimeric PCNA are important for interaction with pol . Therefore, the outer surface of PCNA has multiple functional surfaces which are responsible for the interaction with multiple factors. Furthermore, the two side surfaces seem to be functionally distinguishable, and this may determine the orientation of tracking PCNA along the DNA.


INTRODUCTION

The proliferating cell nuclear antigen (PCNA) (^1)is an essential replication factor for simian virus 40 (SV40) DNA replication in vitro and is involved in the elongation stages of DNA replication(1, 2, 3, 4) . Recent studies have further demonstrated the involvement of PCNA in cellular chromosomal DNA replication in vivo(5, 6, 7) . In addition to its essential role in DNA replication, PCNA is required for nucleotide excision repair of DNA (8, 9, 10) and also may participate in the cell cycle control as demonstrated by an interaction with a cyclin dependent kinase complex(11) . Therefore, PCNA is multifunctional through the interaction with several specific partners, and all of the functions are crucial for cell proliferation.

Genes encoding PCNA have been isolated from various eukaryotes and are composed of highly conserved amino acid sequences of around 260 residues. The functions of PCNA during DNA replication have been elucidated by studies of SV40 DNA replication in vitro. In this reaction, three protein components, PCNA, DNA polymerase (pol) , and replication factor C (RF-C) are required for leading strand DNA synthesis following the initiation of DNA synthesis by DNA pol alpha at the SV40 origin(12) . PCNA and RF-C form a complex at a primer-template junction(13) , and consequently, the DNA synthesizing DNA polymerase switches from pol alpha to pol (14) . In this process, PCNA makes connections between the primer-end recognition reaction and the DNA synthesis reaction through physical interactions with RF-C and pol . These interactions have been demonstrated as the stimulation of RF-C ATPase and pol DNA synthesis by PCNA(15) . However, little is known about the detailed mechanism of how such a complex is formed and which structures are responsible for these interactions.

The assembly of a functional replication DNA polymerase holoenzyme through protein-protein interaction has been reported for Escherichia coli DNA pol III and bacteriophage T4 DNA polymerase (for a review, see (16) and (17) ). The first step is a binding of an ATPase complex (E. coli complex and bacteriophage T4 gene 44/62 protein complex) to a primer-template junction. Following this process, a processivity factor (E. coli beta-subunit and bacteriophage T4 gene 45 protein) forms a secondary complex with the ATPase. This complex tethers its specific core DNA polymerase (E. coli alpha, , , and bacteriophage T4 gene 43 protein) onto a DNA template mediated by hydrolysis of ATP, and a processive DNA polymerase holoenzyme is formed. Judging from the highly conserved reaction processes, there should be close structural and functional relationships between these bacterial and eukaryotic replication factors. The three-dimensional structure of pol III beta-subunit has been determined by x-ray crystallography(18) . The tertiary structure of beta-subunit is a characteristic ring or torus-like structure composed of two homologous subunits that combine to form a DNA tracking protein (for a review, see (19, 20, 21) ). The central hole in the structure has a highly positively charged surface containing six alpha-helices which are thought to be important for interaction with the DNA template. The outer surface has several beta-sheet structures that may interact with other protein components. This model proposes three structurally related units in each monomer subunit and therefore, the whole beta-subunit dimer consists of six of these units. Structural similarity between PCNA and the beta-subunit has been suggested, even though their primary sequences are not related(18) . The prediction has been realized to be essentially correct by a recent study of the crystal structure of PCNA from Saccharomyces cerevisiae(22) . Based on the crystallography results, each PCNA monomer consists of two structurally related domains and the whole molecule contains three PCNA subunits. Thus, like the beta-subunit of pol III, the PCNA clamp has six structurally related units.

To study the assembly of these important eukaryotic replication factors into a functional complex, detailed information on the molecular structure and function of PCNA and the mechanism of protein-protein interactions with RF-C and pol is necessary. We therefore constructed mutations covering the whole PCNA gene by site-directed mutagenesis. Each mutant PCNA protein was expressed in E. coli cells and purified. Stimulation of RF-C ATPase and pol activity was then compared to the wild type protein.


MATERIALS AND METHODS

Oligonucleotides

Oligonucleotides for polymerase chain reaction (PCR) primers were synthesized with an Applied Biosystems model 394 DNA synthesizer (Applied Biosystems, Foster City, CA) or purchased from Biologica Co. (Nagoya, Japan).

Construction of a Plasmid Carrying the Wild Type PCNA

pT7PCNA which allows expression of human PCNA protein was constructed by inserting human PCNA cDNA sequence into pGEMEX-1 (Promega, Madison, Wl). The 900-base pair cDNA fragment was isolated from a human PCNA expression plasmid, pT7hPCNA(23) , a generous gift from Dr. Bruce Stillman (Cold Spring Harbor Laboratory, Cold Spring Harbor, NY), and inserted into NotI and XbaI sites in pGEMEX-1. The resulted plasmid, pT7PCNA, has the intact PCNA gene between the T7 RNA polymerase promoter and the terminator sequences similarly as the parental plasmid. pT7PCNA was harbored in E. coli BL21 (DE3) carrying the T7 RNA polymerase gene under the control of the lac UV 5 promoter.

Mutant Construction of the PCNA Gene

Mutations were introduced by PCR-mediated, site-directed mutagenesis(24) . Four deletion mutants, Delta2-9, Delta257-261, Delta254-261, and Delta250-261 lack 8 amino acids from the second Phe and 5, 8, and 12 amino acids from the C-terminal end, respectively. 29 amino acid substitution mutants were constructed by altering the charged amino acids, Glu^3, Lys, Lys^14, Lys, Asp, Asp, Glu, Asp, Arg, Lys, Lys, Asp, Asp, Lys, Asp, Glu, Arg, Arg, Lys, Lys, Glu, Asp, Glu, Arg, Lys, Asp, Lys, Glu, and Asp to alanine as indicated in Fig. 1. Specific base substitutions were introduced as a mismatch between a PCR primer and a target sequence. Two mutagenic primers were prepared for each mutant construction. The first PCR was performed with a set of primers at 25 pmol each in a 50-µl reaction mixture containing 10 mM KCl, 20 mM Tris-HCl (pH 8.8), 1 mM (NH(4))(2)SO(4), 2 mM MgSO(4), 0.1% Triton X-100, 10 ng of pT7PCNA, 10 pmol of dNTP, 5 µg of bovine serum albumin, and 1-2 units of Vent DNA polymerase (New England Biolabs, Beverley, MA) by 30-35 cycles of 94 °C for 1 min, 45 °C for 1 min and 72 °C for 2 min after heating at 94 °C for 10 min. For some reactions, Pfu DNA polymerase (Stratagene, LaJolla, CA) was used instead of Vent DNA polymerase under the same condition except for the addition of 6 mM (NH(4))(2)SO(4) and 1.5 mM MgCl(2). The second PCR was performed by 35-40 cycles with the first PCR products in 50 µl of reaction mixture similar to the first PCR reaction in the presence of 1 unit of Perfect Match DNA polymerase enhancer (Stratagene). The product was purified after trimming with restriction enzymes and ligated with pT7PCNA digested with the same restriction enzymes.


Figure 1: Mutation sites in aligned amino acid sequences of human(32) , rice(33) , Drosophila melanogaster (34), yeast (S. cerevisiae) (6) PCNA. Conserved amino acids, which were substituted to alanine in this study, were indicated by filled boxes for basic amino acids and shaded boxes for acidic amino acids. Regions corresponding to beta-sheets and alpha-helices (betaA1 to betaI2, and alphaA1 to alphaB2, respectively) follow the labeling of the crystal structure of yeast PCNA(22) .



The mutated DNA sequences were confirmed with an Applied Biosystems model 373A automatic DNA sequencer (Applied Biosystems) or a conventional electrophoresis method with T7 DNA polymerase Version 2.0 Kit (U. S. Biochemical Corp., Cleveland, OH).

Expression and Extraction of PCNA

BL21 (DE3) cells harboring the PCNA expression plasmid were incubated in 1 liter of L-broth with 30 µg/ml methicillin and 10 µg/ml ampicillin at 30 °C until the absorbance reached 0.5 at 600 nm. Then, isopropyl-beta-D-thiogalactopyranoside (IPTG) was added at a final concentration of 1 mM, and the culture was successively incubated at 30 °C overnight. The following procedures were carried out at 4 °C. The induced E. coli cells were collected at 6,000 rpm for 15 min, suspended with a 5 ml of lysis buffer (25 mM Tris-HCl (pH 7.7), 25 mM NaCl, 1 mM EDTA, 0.01% Nonidet P-40, 4 mM bezamidine, 4 mM pepstatin A, 20 mM NaHSO(3), 2 µg/ml leupeptin, 1 mM phenylmethylsulfonyl fluoride (PMSF), and 1 mM dithiothreitol (DTT)), and sonicated with a microtip-horn at 0 °C for 15 s, 16 times with 2-min intervals. The sample was centrifuged at 32,000 rpm for 30 min, and the cleared lysate was obtained (sonic lysate). For Delta2-9 and Delta250-261 mutants, PCNA proteins could not be extracted in the sonic lysate due to the formation of inclusion bodies. Thus, the following extraction procedure was performed. The precipitate was suspended in buffer A (25 mM Tris-HCl (pH 7.9), 1 mM EDTA, 0.01% Nonidet P-40, 10% glycerol, 2 µg/ml leupeptin, 1 mM PMSF, and 1 mM DTT) containing 4 M urea at 0 °C for 30 min, and the lysate was obtained by a ultracentrifugation as above (urea lysate).

Purification of PCNAs

The sonic lysate containing about 100 mg of protein was loaded onto 10 ml of Econo-pac Q cartridge (Bio-Rad) equilibrated with buffer A containing 0.1 M NaCl. After washing the column with 20 ml of the same buffer, proteins were eluted with a 80-ml linear gradient from 0.1 to 0.6 M NaCl in buffer A. Presence of PCNA in fractions was monitored by SDS-polyacrylamide gel electrophoresis and Coomassie Brilliant Blue staining. A contaminated nuclease activity was monitored by incubating 0.5 µg of pUC118 DNA with an aliquot of each fraction at 37 °C. PCNA-containing fractions were pooled and loaded onto a Sephacryl S-300HR column (5 times 75 cm; Pharmacia Biotech, Inc.) in buffer A with 0.1 M NaCl. PCNA fractions eluted around 120 kDa were pooled and loaded onto a Mono Q (HR 5/5; Pharmacia) equilibrated with buffer A containing 0.1 M NaCl. The column was washed with the same buffer, and PCNA was eluted with a 8-ml linear gradient from 0.1 to 0.6 M NaCl in buffer A. PCNA exhibited a discrete peak at 0.55 M NaCl. When a contaminated nuclease existed, the pooled fractions were loaded onto a second Sephacryl S-300HR column (1.8 times 50 cm) and a second Mono Q (HR 5/5). Purified PCNA was aliquoted and stored at -70 °C.

For mutant PCNAs, K20A, D189A, E192A, R210A, and D257A, the pooled Econo-pac Q cartridge fractions was loaded onto a 5-ml Econo-pac HTP cartridge (Bio-Rad) equilibrated with buffer H (20 mM KPO(4) (pH 6.9), 0.01% Nonidet P-40, 10% glycerol, 2 µg/ml leupeptin, 1 mM PMSF, and 1 mM DTT). Proteins were eluted with a 30-ml gradient of 0.02 to 0.6 M KPO(4). PCNA-containing fractions were pooled, mixed with an equal volume of 4 M (NH(4))(2)SO(4), and loaded onto a 5-ml Econo-pac methyl HIC cartridge (Bio-Rad) equilibrated with buffer A containing 2 M (NH(4))(2)SO(4). Proteins were eluted with a 30-ml linear gradient from 2 to 0 M (NH(4))(2)SO(4) in buffer A. PCNA-containing fractions around 0.3 M (NH(4))(2)SO(4) were pooled and dialyzed against buffer A with 50 or 100 mM NaCl and loaded onto a Mono Q (HR 5/5) as above.

RF-C and Pol Preparation

RF-C was prepared from 293 human cells following a published method with slight modifications (13) . Pol was prepared from calf thymus also by a slight modification from a previously published method(13) .

ATPase Assay

The assay for RF-C ATPase was essentially the same as described elsewhere(15, 25) . The reaction mixture (20 µl) contained 30 mM HEPES (pH 7.5), 7 mM MgCl(2), 0.5 mM DTT, 0.1 mg/ml bovine serum albumin, 40 or 100 mM NaCl, 200 pmol of poly(dA)bulletoligo(dT) (5:1), 0.1 mM [-P]ATP or 0.1 mM [alpha-P]ATP, RF-C (4 ng), and PCNAs (280 ng). The mixture was incubated at 37 °C for the indicated periods, and P(i) or ADP produced from ATP was measured by a Norit A charcoal adsorption or a chromatography with a POLYGRAM cel 300 pei/uv 254 0.1-mm layer plate, respectively (Macherey-Nagel, Doren, Germany).

DNA Polymerase Assay

The DNA synthesis assay with pol was carried out as described elsewhere(14) . A reaction mixture (5 µl) containing 30 mM HEPES (pH 7.5), 7 mM MgCl(2), 0.5 mM DTT, 0.1 mg/ml bovine serum albumin, 250 pmol poly(dA)bulletoligo(dT) (20:1), 0.05 mM [alpha-P]TTP (3000 cpm/pmol), calf thymus pol (0.2 unit), and various amounts of PCNA was incubated at 37 °C for 15 min. The incorporated dTMP was measured as a DE81 paper-adsorbed count after washing with 0.5 M Na(2)HPO(4).


RESULTS and DISCUSSION

Expression and Extraction of Mutant PCNAs

Construction of a plasmid, pT7hPCNA which expresses human PCNA efficiently in E. coli has been described by Fien and Stillman(23) . We have constructed a similar expression plasmid, pT7PCNA, suitable for the site-directed mutagenesis in the PCNA gene using pT7hPCNA as a parental plasmid. In this construct, the PCNA gene obtained from the cDNA was placed under the control of the strong T7 RNA polymerase promoter. After the induction of the promoter with IPTG, a 36-kDa PCNA polypeptide became a major protein component in an E. coli extract and was easily purified by conventional column chromatography.

In order to investigate functional regions of PCNA, 33 mutations were introduced into the PCNA gene in the plasmid pT7PCNA, and the mutant PCNA proteins were expressed as for the wild type. Several N- or C-terminal truncations and amino acid substitution mutations at highly conserved amino acids were designed to study. Terminal deletions were designed to determine which region of the PCNA was functionally important. An N-terminal deletion mutant, Delta2-9 that lacks 8 amino acids from the second codon, and three C-terminal deletion mutants, Delta257-261, Delta254-261, and Delta250-261 lack 5, 8, and 12 amino acids from the C terminus, respectively, were constructed. The amino acids in PCNA highly conserved among several species were expected to be involved in its indispensable functions. Furthermore, since a substitution of a charged amino acid to a noncharged one will have a minimal effect on the whole structure of PCNA, any altered phenotype may simply represent an altered function rather than the denaturation of the whole protein. Twenty-nine charged amino acids as indicated in Fig. 1were individually substituted with the noncharged amino acid, alanine.

In all cases, the mutant PCNA proteins accumulated to high amounts in the E. coli cells after the induction of the T7 promoter and became major components as observed for the wild type PCNA. Most of the mutant PCNAs, except for Delta2-9 and Delta250-261, were extracted efficiently from the E. coli cells by a sonic extraction and behaved as a single component of native molecular mass of around 120 kDa, as determined by size fractionation chromatography during the purification. This molecular mass is in good agreement with the prediction that PCNA is in a trimeric state(22) .

Importance of N- or C-terminal Stretches for the Structure

In contrast to most of the altered proteins, Delta2-9 and Delta250-261 remained in an insoluble fraction after the sonic extraction, and an additional 4 M urea treatment was necessary to solubilize them. The insolubility of Delta2-9 and Delta250-261 in the sonic lysate may be due to formation of inclusion bodies in the E. coli cells. A drastic change in the mode of extraction from E. coli cells observed with two deletion mutant PCNAs probably indicates a loss of their native configuration. Indeed, they showed a heterogeneous size distribution in which the majority of the protein was eluted in fractions smaller than 100 kDa during the size fractionation step, after the removal of urea (data not shown). These results suggest that the 8 and 12 amino acid stretches from N- and C-terminal end of PCNA may be crucial to maintain a trimeric native structure. The crystal structure of yeast PCNA shows a characteristic ring structure, and its array of antiparallel beta-sheets comprises the framework of the ring(22) . These terminal deletions eliminate one of these beta-sheets which disrupt the ordered alignment of beta-sheets, and consequently the native molecular structure is lost.

Stimulation of RF-C ATPase and Pol DNA Synthesis

As mentioned above, processive DNA synthesis by pol requires the formation of a complex among pol , PCNA, and RF-C. We employed two assays, stimulation of RF-C ATPase activity and stimulation of pol DNA synthesis to examine the ability of each of the altered PCNA protein to function. The results with 33 mutant PCNAs are shown in Fig. 2and Fig. 3. Five and 16 mutations out of the 33 affected the stimulatory activities for RF-C ATPase and pol DNA synthesis, respectively. Since ATP promotes the formation of the complex between RF-C and PCNA(13) , the level of stimulated RF-C ATPase activity with PCNA may reflect directly the extent of interaction between the two components.


Figure 2: RF-C ATPase assay with mutant PCNAs. Time course of P(i) production with 4 ng of RF-C and 280 ng of mutant PCNAs is shown. Mutant PCNAs are shown with symbols in the inset. Each graph (A-E) demonstrates a result of an independent experiment with controls with and without wild type PCNA (filled and open circles, respectively).




Figure 3: Pol activity with mutant PCNAs. DNA synthesis was measured with 0.2 unit of pol and increasing amounts of wild or mutant PCNAs as described under ``Materials and Methods.'' The incorporated [alpha-P]TMP after an incubation at 37 °C for 15 min is shown. Mutant PCNAs added are indicated with symbols in each inset. Each graph shows a result of an independent experiment and has an activity with wild type PCNA (filled circles). Picomoles of the incorporated dTMP in 1 µl of a reaction mixture are shown.



The activity pol DNA synthesis was assayed with the DNA polymerase, PCNA, and a template DNA, poly(dA)bulletoligo(dT). Under our assay condition, due to the presence of excess primer ends on poly(dA)bulletoligo(dT), pol is able to carry out processive DNA synthesis without RF-C, and the pol activity may be dependent on one or two of the following functions of PCNA, direct protein-protein interaction between PCNA and pol and the DNA clamping activity by PCNA. The mutant data do not discriminate between these two functions.

In the case of deletion mutants Delta2-9 and Delta250-261, which have lost the native configuration, they did not exhibit the stimulative activities for RF-C ATPase and pol DNA synthesis (Fig. 2A and Fig. 3A for Delta250-261, but data is not shown for Delta2-9). The loss of the stimulative activity was not simply due to the denaturation of this protein with urea during extraction, but because of an inability to fold into the native structure by these truncations, inasmuch as the wild type PCNA could be renatured and become fully active by removing urea after being extracted by the same procedure as these mutants (data not shown). Therefore, the native trimeric structure is necessary for both the functions.

The C-terminal Loop Interacts with RF-C

A deletion mutant Delta257-261 showed similar activity in the stimulation of RF-C ATPase as that of wild type, but Delta254-261 did not stimulate RF-C ATPase activity at all (Fig. 2A). In contrast, both Delta254-261 and Delta257-261 exhibit a full stimulatory activity for pol DNA synthesis (Fig. 3A). Therefore, the C-terminal region from Asp to the end is dispensable for the stimulation of both activities, and an internal few amino acids from Glu is necessary to stimulate RF-C ATPase activity specifically. Since an eight amino acids stretch between Lys to Ser has conserved charged residues at Lys, Glu, Asp, Glu, and Glu, these may play a role in interaction with RF-C. Indeed, this region is exposed as a loop in the yeast PCNA structure and a role in interaction with other molecules has been suggested(22) . To test the importance of the charged residues in this region, we substituted the basic residue, Lys and two of the acidic residues, Glu and Asp, with alanine individually, and assayed their stimulative activity for RF-C ATPase. However, all of the mutants have full activity (data not shown). Of course, they also have a full stimulation for pol DNA synthesis activity (Fig. 3F shows K254A and E256A; D257A is not shown). Thus, elimination of one charged residue from the charged amino acid stretch may be insufficient to observe an effect. This must be further tested by construction of multiple amino acids substitution mutants.

Interaction with DNA at the Inner alpha-Helices

The terminal deletion mutants were not very informative about the structure and function of PCNA, since even very short deletions completely eliminate the native structure. Thus, we focused attention on determining which amino acids in the internal coding region were important for function.

Among the conserved amino acids in the PCNA gene, 14 basic residues were substituted with Ala individually. Mutants K13A, K14A, K20A, K77A, R146A, R149A, and K217A lost the stimulation of pol activity and exhibited only a basal level DNA synthesis. The addition of K80A, K110A, or R210A to the pol DNA synthesis reaction caused a limited stimulation in pol activity at less than 50% of wild type (Fig. 3D). With mutants R64A and K168A, a partial decrease in stimulation, corresponding to 50-80% of wild type activity, was observed (Fig. 3, C and E). The rest of the basic amino acid substitutions did not affect the stimulatory activity for pol DNA synthesis, showing that these residues were not required for the activity (data not shown except for K254A in Fig. 3).

One characteristic feature of both the pol III beta-subunit and yeast PCNA is the presence of alpha-helices with positively charged amino acids at the inner surface of the ring(18, 22) . This structural feature may be responsible for the DNA clamping activity of these DNA tracking proteins. One subunit of PCNA has 4 alpha-helices, and each has 2 or 3 basic residues which are highly conserved from human to yeast (Fig. 1). Lys, Lys^14, Lys, Lys, Lys, Arg, Arg, and Lys are exactly positioned at each alpha-helix and all are necessary to stimulate pol activity. These contribute to the positive electrostatic potential in the center of the ring and are suggested to be necessary for an interaction with DNA. Thus, their requirement for pol activity may be a reflection of such an interaction with the template DNA. It is of interest that the elimination of only 1 residue out of 9 positively charged residues reduces drastically the ability of PCNA to stimulate pol activity. Probably, a certain positive electrostatic distribution on the inner surface is important to maintain the DNA clamping activity.

The inability to stimulate pol DNA synthesis with these mutant PCNAs may due to the decrease in either the initial DNA clamping activity or the sliding activity on DNA. To distinguish the mechanisms, we analyzed the products from DNA synthesis by pol using denatured alkaline agarose gel electrophoresis (Fig. 4). A full-length product of 200-300 nucleotides long was synthesized with wild type PCNA but DNA shorter than 20 nucleotides was produced without PCNA. If we analyzed the reaction products with mutants K13A, K14A, K20A, K77A, and K217A, all of them were significantly processive, although their incorporation of dTMP was only a few percent of the fully stimulated pol DNA synthesis ( Fig. 3and Fig. 4). Since the incorporation is corresponding to a DNA synthesis of less than 0.3 nucleotide from each primer end, length of the product represents the processivity of DNA synthesis. Therefore, these mutants block mainly the initiation of pol DNA synthesis but not the processivity of the DNA synthesis. This implies that the elimination of positive charges in the alpha-helices may decrease the DNA clamping activity of PCNA but not the sliding activity, leading to inefficient initiation of pol DNA synthesis.


Figure 4: Product analysis of pol DNA synthesis with mutant PCNAs by alkaline agarose gel electrophoresis. DNA synthesis reaction was carried out as described under ``Materials and Methods'' with indicated mutant PCNA proteins. In reactions from minus to K217A and from K80A to R210A, TMP of 10 times and five times higher specific activities than that of the rest were used, respectively. The products of roughly same radioactivity were loaded onto a 1% agarose gel and separated in an alkaline condition as described in Tsurimoto and Stillman(14) . Length of DNA (bases) obtained from a size marker is shown at the left side.



None of the basic amino acids in the internal alpha-helices affected stimulation of RF-C ATPase ( Fig. 2and data not shown). Taking the complex formation among RF-C, PCNA, and a DNA template into consideration, the DNA clamping activity might potentially affect the RF-C/PCNA interaction. However, the stimulation of RF-C ATPase was independent of the DNA clamping of PCNA, implying that the initial contact between RF-C and PCNA seems to occur in the absence of DNA, or the DNA binding of RF-C alone may have primary significance for the complex formation.

Interaction with Pol

Other positively charged mutants, K64A, K110A, and K168A, which were severely affected the stimulation of pol activity, are separated from the internal alpha-helices and are located at the outer surface of the PCNA ring(22) . This suggests that their outer surface is probably involved in interacting with pol . There are also several highly conserved acidic amino acids on the protein outer surface. We have constructed mutants, E3A, D21A, D41A, E55A, D63A, D86A, D97A, D122A, E143A, E174A, D189A, E192A, and D232A (Fig. 5). Among them, less than 50% of the pol activity found in the presence of wild type PCNA was observed with the D41A mutant and between 50-80% of that with the D122A mutant (Fig. 3C). The other acidic amino acid mutations allowed a full stimulatory activity at wild type level (data not shown except for D232A in Fig. 3).


Figure 5: The mutation sites and their activities to stimulate RF-C ATPase or pol DNA synthesis. Filled circles indicate locations of mutations. Arrowheads indicate the end points of deletions. Symbols in each stimulatory activity represent extents of the activity by mutant PCNAs. +++, more than 80% activity of the wild type; ++, between 80 and 50% of the activity; +, between 50 and 20% of the activity; and -, less than 20% of the activity, respectively.



If these affected mutation sites are placed on the crystal structure of PCNA, they are positioned in several specific structures. Lys and Lys are in two beta-sheets (betaI1 and betaC2, respectively; see Fig. 6) corresponding to the intermolecular interface of the PCNA trimer(22) . It has been suggested that the interface may be necessary to hold the trimeric structure. However, since these mutant proteins behave as a native trimer during gel filtration chromatography (data not shown), this does not appear to be the explanation of why these mutants are defective. Thus, the mutation effects may be due to some local structural changes which influence the DNA clamping activity or the contact with pol . Asp, Lys, and Asp are in the loop between sets of beta-sheets. These loops are exposed on the outside of the protein and we suggest that they provide a structure to contact directly with pol .


Figure 6: Summary of PCNA regions necessary for the stimulation of RF-C ATPase and pol DNA synthesis. Boxed regions indicate the mutation sites where the stimulatory activity of RF-C ATPase and pol DNA synthesis were affected. The height of each box demonstrates the extent of the effect on each activity by mutations according the results in Fig. 5. Neighboring mutation sites of a similar result are included in a same box to indicate that they may compose a functional region. Ambiguity for deletion ends of the terminal functional region is indicated by slant lines with amino acid positions. The internal borders of functional region of each terminal deletions have not been obtained by this study and are indicated by broken lines. Bars with betaA1 to betaI2 indicate the structure units of yeast PCNA(22) .



Interaction with RF-C

Using the same set of mutants, we studied their effect on RF-C ATPase stimulation. Mutant D41A is severely affected for the stimulatory activity on RF-C ATPase and another mutant, D97A, showed only a small but reproducible decrease in the activity (Fig. 2, B and C). The other mutations had no effect on this stimulation ( Fig. 2shows D63A, D86A, and D122A, but the others are not shown). Therefore, only two out of 29 mutated amino acids exhibited an apparent effect on the RF-C ATPase stimulation (Fig. 5). This may indicate that a very limited surface of the protein is used to contact with RF-C. As mentioned above, the C-terminal loop of PCNA is required for the specific interaction with RF-C. The crystal structure of yeast PCNA shows that both Asp and Asp are exposed to a surface on the same side of PCNA as the C-terminal loop. This implies that the three clustered loops projecting to one side of PCNA compose a pocket to contact RF-C.

Interestingly, D41A affects both RF-C ATPase stimulation and pol DNA synthesis. To exclude the possibility that the D41A mutation would change the protein structure, we analyzed the circular dichroism profile of D41A. The signals of short wave range (200-250 nm) which represent peptide secondary structure were completely same between wild PCNA and D41A. This indicates that D41A has the same structure as wild PCNA. Thus, Asp is required to interact with both RF-C and pol , and this loop has two targets for interaction. But it is unclear whether or not this amino acid is able to interact with pol and RF-C simultaneously.

The CDC44 gene in S. cerevisiae encodes the large subunit of RF-C, and five independent suppressors of its cold sensitive mutations were isolated. All of them were mapped to the PCNA gene (pol 30), suggesting that the 140-kDa subunit interacts directly with PCNA(26) . (^2)These mutations occurred at positions completely or partially buried in the structure and are likely to cause changes in the structure of PCNA(22) . Although these suppressor mutation sites are involved in interacting with RF-C, they are physically close to sites which we have shown to be involved in interacting with pol , but not with RF-C. This discrepancy may due to a difference of the assay system. In our system, interaction of RF-C and PCNA is studied by a biochemical assay and only strongly affected mutations may have been appeared. In the case of suppressor mutation, such strong mutations might not be isolated, but rather, mutations that only moderately affect the protein could be isolated, for example, those which alter the partial molecular structure will be selected. It is therefore likely that the amino acid residues involved in maintaining the tertiary structure may contribute to interaction with RF-C as well as pol , but their effect may not be detected in our biochemical assay.

Asymmetrical Sides of PCNA

Our studies indicate the importance of exposed loop structures for interacting with RF-C and pol . Some of them containing Arg and Asp that may be involved in interaction with pol are located at the peripheral surface of the ring and do not contribute much to its orientation. But other loops containing Asp, Asp, and the C-terminal loop that may interact with both RF-C and pol or RF-C alone are of interest. These are projected to a common side of the PCNA trimer, implying that PCNA has an orientation for the function where one side is used to interact with RF-C and pol . This side should face to a primer/template junction and the other should face to a double stranded DNA region (Fig. 7). Are there any functions on the other free side? PCNA has multiple target proteins to interact with in addition to replication proteins, for example the interactions of PCNA with cell cycle proteins, cyclin-dependent kinase, cyclins, and p21 and with a DNA damage-induced protein, Gadd45, have been reported(11, 27, 28) . It is therefore possible that the free side may provide a structure to contact with such proteins. Mapping of PCNA regions interact with cyclin D has been reported using deletion constructs of PCNA, but it is difficult to localize finely the regions for the interaction on the crystal structure, since relatively large deletions were used(29) . This will be tested in future studies using our mutant PCNA proteins.


Figure 7: A model for the assembly of pol complex. A monomer of PCNA is indicated at the top. The four alpha-helices with nine basic amino acids are shown at the internal surface. The C-terminal stretch with acidic amino acids is projected from the molecule to emphasize the interaction site with RF-C. Shaded areas indicate the 6 predicted sites which may interact with RF-C and pol . The trimer PCNA molecule with a ring structure is shown (second row), and the internal positive charges provide interaction surface with DNA duplex. In the presence of RF-C and ATP, PCNA is transferred onto the template/primer and forms the primer recognition complex (third row). The large subunit (140 kDa) at the center and four small subunits (40, 38, 37, 36.5 kDa) of RF-C are indicated in the elliptic shape. Subsequently, pol is incorporated and a highly processive DNA polymerase complex is formed (forth row).




CONCLUSION

We have introduced 33 mutations into the human PCNA gene and studied their effects on the functions of PCNA. Stimulatory effects on RF-C ATPase activity and pol DNA synthesis activity were examined and the results are summarized in Fig. 5and Fig. 6. Amino acid substitution at residues Lys, Lys^14, Lys, Lys, Lys, Arg, Arg, Arg, and Lys in PCNA, which are located at the alpha-helices, exhibited a limited stimulation of pol activity. The alpha-helices provide an internal surface to clamp a DNA template through their highly positive charges facing to the same side of each alpha-helix (Fig. 7). In addition to the internal surface, the beta-sheets at the intermolecular interface and the exposed loops have a significant role in interaction with pol . The assay to stimulate RF-C ATPase with mutant PCNAs demonstrates a strict requirement for specific residues that are located at the loops projecting to one side of the PCNA trimer. PCNA has 6 redundant units in the trimeric structure, each of which may have surfaces to interact with either pol or RF-C, or both.

How do pol and RF-C share the redundant structures of PCNA? RF-C consists of five subunits, and their cDNA sequences have demonstrated a significant structural redundancy among them(30, 31) . Thus, we propose a model to assemble the processive DNA polymerase complex as described in Fig. 7. At least three pockets of the side loops may interact with three subunits of RF-C specifically. Other structures, such as the intermolecular interface, may also contribute to interactions with RF-C, as suggested by the yeast genetics. This means that the five subunits of RF-C may occupy five out of six units of PCNA trimer. Interaction between RF-C and PCNA in the presence of ATP may induce a conformational change in PCNA, which could then open one of the interfaces and pass a DNA helix through the PCNA ring. Then pol may be recruited onto the template DNA using one free unit of PCNA as a contact site.

Our study with single amino acid mutations and deletion mutations in PCNA demonstrates the presence of multiple functional surfaces in the characteristic ring structure of PCNA. In addition, several loops projected from one specific side provides the orientation which is important for the function of PCNA as a tracking molecule.


FOOTNOTES

*
This work was supported by grants from the Ministry of Education, Science and Culture, Japan. 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: Nara Institute of Science and Technology, 8916-5 Takayama, Ikoma, Nara 630-01, Japan.

To whom correspondence should be addressed: Nara Institute of Science and Technology, 8916-5 Takayama, Ikoma, Nara 630-01, Japan. Tel.: 07437-2-5511; Fax: 07437-2-5519.

(^1)
The abbreviations used are: PCNA, proliferating cell nuclear antigen; pol, polymerase; RF-C, replication factor C; PCR, polymerase chain reaction; IPTG, isopropyl-beta-D-thiogalactopyranoside; PMSF, phenylmethylsulfonyl fluoride; DTT, dithiothreitol.

(^2)
K. Fien and B. Stillman, personal communication.


ACKNOWLEDGEMENTS

We are grateful to Dr. Bruce Stillman (Cold Spring Harbor Laboratory, Cold Spring Harbor, NY) for his generous gift of the human PCNA cDNA and for his critical reading of the manuscript, Dr. John Kuriyan (The Rockefeller University, New York, NY) for his kind communication of the crystal structure of yeast PCNA prior to publication. We also thank Dr. Hisao Masukata (Nagoya University, Nagoya, Japan) and Dr. Hiroshi Yoshikawa (NAIST, Ikoma, Japan) for their valuable comments in preparing the manuscript and Takashi Oku for his technical assistance.


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