Replicative Functions of Minute Virus of Mice NS1 Protein Are Regulated In Vitro by Phosphorylation through Protein Kinase C

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Journal of Virology, December 1998, p. 9966-9977, Vol. 72, No. 12
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Replicative Functions of Minute Virus of Mice NS1 Protein Are Regulated In Vitro by Phosphorylation through Protein Kinase C

Jürg P. F. Nüesch,^* Sabine Dettwiler, Romuald Corbau, and Jean Rommelaere

Applied Tumor Virology and Institut National de la Santé et de la Recherche Médicale U375, Deutsches Krebsforschungszentrum, Heidelberg, Germany

Received 14 May 1998/Accepted 27 August 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

NS1, the major nonstructural protein of the parvovirus minute virus of mice, is a multifunctional phosphoprotein which isinvolved in cytotoxicity, transcriptional regulation, and initiationof viral DNA replication. For coordination of these various functionsduring virus propagation, NS1 has been proposed to be regulatedby posttranslational modifications, in particular phosphorylation.Recent in vitro studies (J. P. F. Nüesch, R. Corbau, P. Tattersall,and J. Rommelaere, J. Virol. 72:8002-8012, 1998) provided evidencethat distinct NS1 activities, notably the intrinsic helicase function,are modulated by the phosphorylation state of the protein. Inorder to study the dependence of the initiation of viral DNA replicationon NS1 phosphorylation and to identify the protein kinases involved,we established an in vitro replication system that is devoid ofendogenous protein kinases and is based on plasmid substratescontaining the minimal left-end origins of replication. Cellularcomponents necessary to drive NS1-dependent rolling-circle replication(RCR) were freed from endogenous serine/threonine protein kinasesby affinity chromatography, and the eukaryotic DNA polymeraseswere replaced by the bacteriophage T4 DNA polymerase. While nativeNS1 (NS1^P) supported RCR under these conditions, dephosphorylated NS1 (NS1^O) was impaired. Using fractionated HeLa cell extracts, we identifiedtwo essential protein components which are able to phosphorylateNS1^O, are enriched in protein kinase C (PKC), and, when present together,reactivate NS1^O for replication. One of these components, containing atypicalPKC, was sufficient to restore NS1^O helicase activity. The requirement of NS1^O reactivation for characteristic PKC cofactors such as Ca²⁺/phosphatidylserine or phorbol esters strongly suggests the involvementof this protein kinase family in regulation of NS1 replicativefunctions invitro.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Minute virus of mice (MVM) is the prototype of the genus Parvovirus. Members of this genus consist of nonenveloped sphericalparticles of about 20 to 24 nm in diameter, comprising a linearsingle-strand DNA genome of approximately 5.1 kb. Parvovirus DNAencodes the two structural (VP) and at least four nonstructural(NS) polypeptides, of which the 83-kDa nuclear phosphoproteinNS1 is the only viral product necessary for viral DNA replicationin all cell types (22, 54). Replication of the parvovirusgenome involves the formation of monomeric and concatemeric duplexDNA intermediates. These replicative forms are produced by anunidirectional, single-strand copy mechanism (for a review, seereference 16) which resembles the rolling-circle replication(RCR) mechanism described for single-stranded DNA plasmids, bacteriophages,and geminiviruses (for a review, see reference 35). After conversionof the single-strand genome into a monomeric duplex, which isexecuted solely by cellular components (3), replication initiatesat site-specific, single-strand nicks introduced by the viralNS1 protein into origin sequences located at either end of thegenome (14, 17, 18). This cleavage reaction leaves NS1 covalentlyattached to the 5' end at the nick site and generates a base-paired3' hydroxyl group which serves as a primer for DNA synthesis (8,13, 19, 59).

The minimal origin sequence at the left-end telomere has been mapped and consists of approximately 50 bp located within thestem of the Y-shaped terminal structure (13). This sequencecomprises binding sites for the cellular component PIF (parvovirusinitiation factor) (9) and for NS1 (21) and an NS1 nick site(13). The NS1 binding and nick sites are separated by an AT-richsequence, which most likely facilitates local unwinding duringthe nicking reaction. In the left-end hairpin structure of thegenome, between the binding sites for PIF and NS1, there is afunctionally important mismatched "bubble," with a 5'-GAA-3' tripleton one strand opposite a 5'-GA-3' doublet on the other strand.When replication through the hairpin unfolds and copies the palindrome,a double-strand intermediate is generated, in which these tri-and dinucleotide sequences are located on either side of the axisof symmetry. Although the origin sequences of both arms are nearlyidentical, only the arm containing the GA dinucleotide servesas an active origin for NS1-mediated RCR, while the trinucleotide-containingcounterpart remains silent (13).

Besides its key role as the initiator protein for viral DNA replication, NS1 is essential for several additional processesduring the viral life cycle. In particular, the NS1 protein isa strong trans activator of the parvovirus P38 promoter that controlscapsid gene expression (64). Furthermore, NS1 trans regulatesnonparvovirus promoters (27, 70), and it exerts cytotoxicand/or cytostatic effects for which oncogene-transformed cellsappear to be preferential targets (5, 7, 53). To accountfor the temporal coordination of these various functions duringvirus multiplication, NS1 has been proposed to be regulated byposttranslational modifications such as phosphorylation. NS1 wasindeed found to be phosphorylated in infected cells (2, 11,20, 51). Moreover, recent in vitro studies have shown thatHeLa cell-derived native NS1 differs from its dephosphorylatedcounterpart in its capacity for distinct biochemical activitiesinvolved in viral DNA replication (60).

In order to study the effect of phosphorylation on NS1-driven initiation of DNA replication, we used a previously describedRCR system, which is based on plasmid substrates containing theminimal left-end origins of replication (8, 13). This systemwas modified to deplete its protein components from endogenouskinases, allowing purified native NS1 (NS1^P) to be compared with dephosphorylated NS1 (NS1^O) with regard to their respective replication activities. In contrastto standard HeLa cell extracts, the kinase-free replication systemwas severely impaired in its ability to support RCR when suppliedwith NS1^O as compared with NS1^P. In reactivation experiments, the combination of two distinctprotein fractions from HeLa cell extracts proved to be able torestore at least in part the replication activity of NS1^O in the kinase-free system. This reactivation was dependent uponthe presence of either acid lipids and Ca²⁺ or the phorbol ester 12-O-tetradecanoylphorbol-13-acetate (TPA).This dependence on cofactors, together with the capacity of bothfractions to phosphorylate NS1^O in vitro, strongly suggests that members of the protein kinaseC (PKC) family are responsible for regulation of the NS1 replicativefunctions. Previous analyses of selected biochemical activitiesof native NS1^P versus NS1^O polypeptides have shown that the intrinsic helicase functionof the viral product is strikingly dependent upon phosphorylation(60). One of the protein components necessary to rescue thereplication activity of NS1^O in the kinase-free system, which was enriched in atypical PKC,was also found to reactivate the helicase function of NS1^O.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Viruses and cells. Recombinant vaccinia viruses were propagated in monolayer cultures of BSC-40 cells, collected, and purified over a sucrosecushion as described previously (41), except for the releaseof virus from infected cells, which was achieved by three cyclesof freezing and thawing instead of sonication. Recombinant vacciniaviruses were constructed as previously described (57). The 293cell line was adapted to suspension and grown in spinner bottleswith Joklik's medium supplemented with 10% fetal calf serum. HeLa-S3cells were grown in spinner bottles in the presence of 5% fetalcalfserum.

Production and purification of native and dephosphorylated NS1. Wild-type NS1 and mutant NS1 were produced from recombinant vaccinia viruses in suspension cultures of HeLa-S3 cells and harvestedat 18 h postinfection (57, 60). His-tagged NS1 present innuclear extracts was dephosphorylated, or not, with calf intestinealkaline phosphatase and purified immediately on Ni²⁺-NTA agarose columns (60). NS1 preparations were analyzed bydiscontinuous sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE), and proteins were detected by Coomassie blue staining.All NS1 preparations were tested for activities in various invitroassays.

Plasmids. Plasmid pTMHis is a derivative of pTM-1 (52), which allows the expression of N-terminal His₆-tagged proteins. The presenceof a unique NcoI site allows the in-frame cloning of the geneof interest starting from its initiation codon. pTMHis was constructedby insertion of the annealed oligonucleotide pair 5'-CATGCACCATCACCACCATCACGCCATGGAATTC-3'and 5'-GAATTCCATGGCGTGATGGTGGTGATGGTG-3' into the NcoI- and SmaI-cleavedpTM-1 vector. The plasmid used to obtain recombinant vacciniaviruses expressing His-tagged PKC $alpha$ was constructed by insertionof the full-length human PKC $alpha$ -coding sequence (30) into NcoI-and EcoRI-cleaved pTMHis. Plasmids used as templates for in vitroreplication assays were pL1-2TC and pL1-2GAA, containing the minimalactive left-end MVM origin and the corresponding inactive origin,respectively (13). The bacterial expression plasmid pYT202am,containing the MVM sequence from nucleotide (nt) 225 to 534, servedto produce peptides for rabbit immunization and generation ofNS-specific antisera (23). pQE-PKC $gamma$ was constructed by insertionof the BamHI-to-SmaI fragment (nt 1332 to 1956) of human PKC $gamma$ cDNA (37) into pQE-30 (Qiagen). pQE-PKC $zeta$ was produced by insertionof the HindII-to-BamHI fragment (nt 981 to 1403) of human PKC $zeta$ cDNA (34) into pQE-32(Qiagen).

Purification of peptides and production of antisera. Peptides from pYT202amNS, pQE-PKC $gamma$ , or pQE-PKC $zeta$ were expressed overnight in the presence of 1 mM IPTG (isopropyl- $beta$ -D-thiogalactopyranoside),extracted, and purified as described previously (23). Antiserawere produced by multiple injections into rabbits. For Westernblot analyses with anti-PKC $gamma$ ( $alpha$ PKC $gamma$ ) or $alpha$ PKC $zeta$ antibodies, IgGswere affinity purified on peptide columns by using the immunizingpeptides (31).

Preparation of L-threonine and protamine affinity columns. Affinity chromatography columns were prepared by coupling L-threonine or protamine sulfate with NIH-activated Hi-Trap columns(5 ml; Pharmacia) according to the manufacturer's instructions.L-Threonine (Sigma) or protamine chloride (Sigma) was dissolvedin coupling buffer (0.1 M NaCO₃ [pH 8.3], 0.5 M NaCl) at 10 mg/mland allowed to interact with the column material for 1 h at roomtemperature byrecirculation.

Protein extraction and fractionation by column chromatography. S100 extracts from 293S and HeLa cells were prepared and fractionated on phosphocellulose columns to obtain fractions P1,P2, and P3 as described previously (8, 68), except that P3was eluted at 1 M NaCl (see Fig. 2A). To remove endogenous serine/threoninekinases, P1 from a 10-liter suspension culture of 293 cells wasfurther purified on a 5-ml L-threonine affinity Hi-Trap columnin buffer A (25 mM Tris [pH 7.5], 1 mM EDTA, 1 mM dithiothreitol[DTT], 174 µg of phenylmethylsulfonyl fluoride [PMSF] per ml,10% glycerol) containing 150 mM NaCl. Individual flowthrough fractionswere dialyzed against buffer B (20 mM HEPES [pH 7.5], 5 mM MgCl₂,5 mM KCl, 0.1 mM DTT, 17.4 µg of PMSF per ml, 10% glycerol, 20%sucrose) overnight at 4°C and stored in aliquots at $-$ 80°C. Todetermine the extent of purification, all fractions were testedfor their ability to phosphorylate NS1^O in in vitro kinase assays. P2-pol was obtained by P2 fractionationon DE52 columns. P2 from a 10-liter HeLa cell culture was loadedon a DE52 column (5 ml of resin/liter of original culture) inbuffer A containing 50 mM NaCl. After thorough washing with thesame buffer, P2-pol was eluted with buffer A containing 1 M NaCl.The eluate was dialyzed against buffer B and frozen inaliquots.

Protein kinases present in the HeLa cell-derived P2 fraction were further purified by consecutive anion-exchange, protamineaffinity, and hydroxylapatite chromatographies (see Fig. 4). (i)P2 was adjusted to 200 mM NaCl and fractionated on a DE52 column(step 2). The flowthrough at 200 mM NaCl (DE-1) and the elutionfractions DE-2 (200 to 500 mM NaCl) and DE-3 (500 mM to 1 M NaCl)were collected. All fractions were dialyzed against buffer B,frozen, and stored at $-$ 80°C. The protein kinases necessary toachieve extensive reactivation of NS1^O in replication assays were found to be confined to fraction DE-1.(ii) PKC family members contained in DE-1 were further purifiedby protamine affinity chromatography (step 3), using a fast performanceliquid chromatography (FPLC) system (Pharmacia). DE-1 (correspondingto a 6-liter culture) was loaded on a 5-ml protamine Hi-Trap columnwith a constant flow rate of 0.5 ml/min. After collection of theflowthrough (PA-1), the column was washed with buffer C (20 mMHEPES [pH 7.5], 1 mM EDTA, 0.1 mM DTT, 10% glycerol) containing200 mM NaCl. The PKC-containing fraction PA-2 was then elutedwith buffer C containing 1 M NaCl and the protease inhibitorsPMSF (174 µg/ml), leupeptin (1 µg/ml), and aprotinin (1 µg/ml).PA-2 was dialyzed, adjusted to 50% glycerol, and stored in aliquotsat $-$ 80°C. (iii) PKC isoforms present in fraction PA-2 were separatedby FPLC on hydroxylapatite columns (step 4). PA-2 (correspondingto a 3-liter culture) was adjusted to 200 mM NaCl, loaded on a5-ml hydroxylapatite column (Merck) with constant flux (0.5 ml/min),and washed with 30 ml of buffer C containing 50 mM NaCl. Aftercollection of the flowthrough and wash, the HA-1 fraction waseluted from the column with buffer D (150 mM NaCl, 20 mM KPO₄[pH 7.5], 10% glycerol, and the protease inhibitors PMSF, leupeptin,and aprotinin). The protein peak was identified by UV monitoring(280 nm) and collected. HA-2 was then eluted with a linear gradientbetween buffer D and buffer E (150 mM NaCl, 0.5 M KPO₄ [pH 7.5],10% glycerol, and protease inhibitors) and consisted of pooledfractions recovered between 120 and 400 mM KPO₄. All fractionswere dialyzed against buffer B containing 50 mM NaCl overnightat 4°C, adjusted to 50% glycerol, and frozen in aliquots at $-$ 80°C.

Replication assays. Replication assays were carried out as described previously (13) in the presence of optimized amounts of the various cellfractions, using approximately 0.2 µg of His-tagged vaccinia virus-producedNS1 (determined by Coomassie blue staining after SDS-PAGE). Inthe modified replication system, 3 U of T4 DNA polymerase (BoehringerMannheim) was used instead of cellular polymerases. Each assaywas carried out in a 20-µl total volume of 20 mM HEPES-KOH (pH7.5)-5 mM MgCl₂-5 mM KCl-1 mM DTT-0.05 mM each deoxynucleosidetriphosphate-4 mM ATP-40 mM creatine phosphate-1 µg of phosphocreatinekinase-10 µCi of [ $alpha$ -³²P]dATP (3,000 mCi/mmol)-20 ng of the appropriate DNA template.After incubation at 37°C for 2 h, the reaction was stopped byadding 60 µl of 20 mM Tris (pH 7.5)-10 mM EDTA-0.2% SDS and incubatingthe mixture at 70°C for at least 30 min. In order to quantifythe extent of DNA replication, 3 µl of the terminated reactionmixture was spotted in duplicate on DE81 filters, washed extensivelywith 0.5 M Na₂HPO₄, and analyzed for incorporated radioactivityby scintillation counting. ³²P-labeled replication products were also linearized with restrictionendonuclease HindIII and analyzed by agarose gel electrophoresis,either directly after proteinase K digestion or after immunoprecipitationwith $alpha$ NS_N antiserum (13). This antiserum was raised againstthe common N terminus of MVM NS proteins (23).

In vitro kinase reactions. In vitro kinase reactions were performed as described previously (60), using various amounts of protein extracts, 100 ngof dephosphorylated NS1^O, and 10 µCi of [ $gamma$ -³²P]ATP (3,000 mCi/mmol) in 20 µl of 20 mM HEPES-KOH (pH 7.5)-7mM MgCl₂-5 mM KCl-1 mM DTT. After incubation for 30 min at 37°C,the reactions were stopped by adding the same volume of 20 mMTris (pH 7.5)-5 mM EDTA-0.2% SDS and heating for 30 min at 70°C.One-fifth of the reaction products were immunoprecipitated with $alpha$ NS_N antiserum, and in vitro-labeled NS1 was detected by 8% SDS-PAGEandautoradiography.

Helicase assays. Helicase assays were performed as described previously (59, 60) with M13-VAR as a template. Reaction mixtures with 10to 100 ng of purified NS1 were incubated for 40 min at 37°C. Forreactivation experiments, titrated amounts of protein extractswere added to the reaction mixtures together with one or moreof the following PKC cofactors: 2 mM Ca²⁺, 1 µg of L- $alpha$ -phosphatidyl-L-serine (PS) per µl, or 5 nM TPA.None of these PKC cofactors alone had any influence on the helicasefunction of native NS1^P, dephosphorylated NS1^O, or mutant NS1 proteins used as negativecontrols.

Western blot analyses. Protein extracts were fractionated by discontinuous 10% SDS-PAGE, blotted on nitrocellulose membranes, and revealed with rabbitantibodies directed against the most conserved domain of PKC ( $alpha$ PKC $gamma$ and $alpha$ PKC $zeta$ ), or with mouse antibodies specific for the atypicalPKC $iota$ (Transduction Laboratories). The $alpha$ PKC $gamma$ and $alpha$ PKC $zeta$ polyclonalantibodies were affinity purified on peptide columns, used at0.6 mg of IgG per ml, and revealed with ¹²⁵I-labeled protein A (ICN; 0.2 µCi/ml). Mouse $alpha$ PKC $iota$ antibodieswere used at a 1:2,500 dilution, and bound antibodies were revealedwith a 1:5,000 dilution of horseradish peroxidase-conjugated anti-mouseIgGs by using the ECL system(Amersham).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

NS1 phosphorylation is required for RCR. Previous investigations comparing biochemical activities of dephosphorylated NS1 (NS1^O) and native NS1 (NS1^P), both derived from HeLa cells, revealed modulation of site-specificbinding to the left-end origin, site-specific nicking, and helicaseand ATPase activities. In contrast, no significant differencebetween NS1^O and NS1^P could be observed in their respective capacities for dimer-bridgeresolution in an in vitro replication assay with HeLa cell extracts(60). It was suggested that NS1^O became phosphorylated by kinases present in cell extracts, leadingus to develop a kinase-free replication system, as presented inthisstudy.

Resolution of the left-end dimer-bridge junction is a complicated assay, probably requiring a number of so-far-unknown cellularcomponents. In addition, this assay is rather insensitive, becauseeach initiation event is associated with synthesis of only a shortstretch of labeled DNA. This prompted us to use a more simpleassay, which consists of the NS1-dependent initiation of RCR ofnonpalindromic substrates carrying the MVM origins of replication(13), to study the effect of phosphorylation on NS1 replicativefunctions. When performed with standard replication extract, wild-typeNS1, and a plasmid containing an active origin of replication,this assay leads to the synthesis of several kilobases of labeledDNA, which makes it far more sensitive than dimer-bridge resolution.In addition, in the absence of an active origin or without functionalNS1, only marginal replication due to repair synthesis is observed,which facilitates the analysis of the modulation of NS1 activity(13).

In a first step, NS1^P was compared with NS1^O in regard to the ability to support RCR from a parvovirus origin in standard HeLacell extracts. Purified NS1^P and NS1^O were prepared as reported previously (60). Plasmids carryingthe active (TC) or inactive (GAA) left-end origin of MVM DNA replicationwere used as substrates. The mutant NS1 derivative Y210F, whichis impaired in site-specific nicking due to an amino acid substitutionfor the active-site tyrosine but which is proficient in helicaseactivity (59), served as a negative control for NS1 replicativefunction. As shown in Fig. 1A, NS1^O was able to support RCR in crude HeLa cell extracts almost asefficiently as NS1^P, confirming previously reported findings with cloned dimer-bridgeas a substrate (60). Indeed, the replication activities of bothwild-type NS1 and the replication-competent NS1 mutant dlC67 werereduced to only a small extent by dephosphorylation; i.e., NS1^O sustained approximately 60% of the level of [³²P]dATP incorporation into newly synthesized DNA as did NS1^P (data not shown). To verify dephosphorylation, we also testedNS1^O for its biochemical activities in absence of any additional proteins.The most striking difference between native and dephosphorylatedNS1 has been described for the helicase function (60). As illustratedin Fig. 1B, NS1^O helicase activity was indeed reduced more than 10-fold comparedto that of the native polypeptide, in contrast to the significantactivity of NS1^O in replication assays. The helicase-deficient NS1 mutant K405Rserved as a negative control in these experiments.

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FIG. 1. Comparison of replicative functions of native NS1^P and dephosphorylated NS1^O. NS1 was expressed from recombinant vaccinia viruses in HeLa-S3 cells and harvested at 18 h postinfection by preparing nuclear extracts. Dephosphorylated NS1^O was obtained by treatment with calf intestine alkaline phosphatase. His-tagged native NS1^P and phosphatase-treated NS1^O were purified from nuclear extracts by Ni²⁺-NTA affinity chromatography. (A) NS1^P and NS1^O were compared for their capacities to support RCR in standard HeLa cell replication extracts, using plasmids containing the left-end active (T) or inactive (G) origin as substrates, in the presence of [³²P]dATP. The reaction products were linearized with HindIII and analyzed by 0.8% agarose gel electrophoresis. The linkage tyrosine mutant Y210F (59) served as a negative control. The dlC67 mutant is replication competent (60) and was also analyzed in its native (P) and dephosphorylated (O) forms. (B) NS1^P (100, 30, and 10 ng [lanes 4 to 6, respectively]) and NS1^O(100 ng [lane 7]) were compared for their intrinsic helicase activities, using M13-VAR template, for 40 min at 37°C in the presence of 2 mM ATP. The ATP-binding site mutant K405R (57) served as a negative control. Reaction products were analyzed by native 7% PAGE in the presence of 0.1% SDS. Lanes 1 and 2, native (NAT) and denatured (DEN) input DNA, respectively.

One possible explanation for the replication competence of NS1^O, despite the lack of helicase function, might be the presenceof protein kinases within the cell extracts used in the formerbut not in the latter assay, which would lead to NS1^O rephosphorylation and consequent reactivation. To test this possibility,and eventually to establish RCR in absence of endogenous proteinkinases, we first determined the presence of NS1^O-phosphorylating protein kinases after fractionation of replicationextracts on phosphocellulose columns, taking advantage of recentdevelopments in the identification of host cell determinants ofthis reaction. As indicated in Fig. 2A, it has been shown thatphosphocellulose fractions P1 and P2 derived from 293 cells aresufficient to support RCR of plasmids containing the left-endorigin in the presence of wild-type NS1 (8). When HeLa cellextracts were fractionated in the same way, protein kinases phosphorylatingNS1 were found to be confined to fractions 2 and 3, with no detectableactivity in the P1 flowthrough (Fig. 2B). Yet, HeLa cell P1 failedto support significant replication in the presence of P2 and nativeNS1^P (data not shown) and hence could not be used in subsequent experiments.Therefore, we prepared P1 from 293 cells as previously described(8), in order to obtain sufficient replication factors thereinto drive RCR. In contrast to HeLa cell P1, 293 cell P1 significantlyphosphorylated NS1^O, although the bulk of kinase activity was still found in fractionsP2 and P3 (Fig. 2B). To remove the residual endogenous serine/threoninekinases from 293 cell P1, this fraction was purified over an L-threonineaffinity column, resulting in P1-Thr, which was essentially freeof NS1^O-phosphorylating activity in comparison with the original P1 material(Fig. 2B). This kinase-free P1-Thr from 293 cells was then combinedwith fraction P2 obtained from HeLa cells in order to supply thecellular components allowing NS1-mediated RCR. As seen in Fig.2C, NS1^P was able to trigger RCR from the active (TC) origin in the presenceof P1-Thr and P2 fractions. This reaction was specific, sinceit occurred to only a small extent when the inactive (GAA) originwas used as a substrate. Furthermore, as seen previously withstandard HeLa extracts, NS1^O was also able to support RCR under these conditions, i.e., inthe presence of the sole protein kinases present in HeLa cellP2. Under these conditions, NS1^O achieved close to 50% of the RCR activity of NS1^P (Fig. 2C). The inactivity of the replication-deficient NS1 mutantY210F, used as a negative control, and the immunoprecipitationof labeled DNA products with NS1 antiserum confirmed the specificityof the RCR reaction (Fig. 2C). Together, these results indicatethat the phosphocellulose P3 fraction, as well as the proteinkinases therein, are dispensable for RCR initiated by NS1 at theleft-end origin.

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FIG. 2. Fractionation of cell extracts by phosphocellulose chromatography. S100 replication extracts were prepared from 293-S or HeLa-S3 cells and fractionated on phosphocellulose columns as described by Tsurimoto and Stillman (68). (A) Scheme of replication extract fractionation into P1, P2, and P3, with the expected distribution of known replication factors (8, 55, 68). The NaCl concentrations used for elution are indicated. F/T, flowthrough; PCNA, proliferating cell nuclear antigen; RPA, replicator protein A (also designated RF-A or human single-stranded-DNA-binding protein); PIF, parvovirus initiation factor; Pols, eukaryotic DNA polymerases; RFC: replication factor C; Topos, eukaryotic topoisomerases. As indicated, P1 plus P2 have been shown to contain all cellular components necessary to support NS1-dependent RCR from the active left-end (3') origin (ori) (8). (B) Detection of NS1^O-phosphorylating protein kinases in the distinct phosphocellulose fractions. NS1^O was incubated with the indicated fractions in the presence of [ $gamma$ -³²P]ATP for 30 min at 37°C and analyzed by SDS-PAGE after immunoprecipitation with $alpha$ NS_N (23). The migration of NS1 is indicated. P1-Thr corresponds to the P1 fraction from 293-S cells after purification on L-threonine affinity columns. (C) Comparison of NS1^P and NS1^O in RCR assays with P1-Thr derived from 293 cells plus P2-pol derived from HeLa cells, with plasmid templates containing the minimal active (T) or inactive (G) left-end origin. Since NS1^O has been shown to be activated for helicase activity by members of the PKC family (60), the reactions were carried out in the presence of the PKC cofactors Ca²⁺ and PS. The replication-deficient NS1 mutant Y210F was used as a negative control. Linearized, labeled reaction products (L) were analyzed by 0.8% agarose gel electrophoresis, either directly after proteinase K treatment (left panel) or after immunoprecipitation with $alpha$ NS_N (right panel).

Fraction P2 is thought to provide the DNA polymerases necessary for NS1-dependent RCR at the left-end origin (8, 55,68). In order to reconstitute a kinase-free system and supplyDNA polymerases in absence of protein kinases, we decided to replacethe whole fraction P2 by purified bacterial or bacteriophage polymerases.With native NS1^P, no replication products were obtained when either P1 or P2 wasomitted from the reaction (Fig. 3, lanes 1 and 2). On the otherhand, DNA synthesis took place when the P1-Thr fraction was supplementedwith Escherichia coli DNA polymerase I or the Klenow fragmentthereof (data not shown) or with DNA polymerase from bacteriophageT7 or T4 (Fig. 3). In the presence of standard replication extracts,the active origin from pL1-2TC is recognized by NS1, allowingthe establishment of a unidirectional single-strand replicationfork which progresses around the circular plasmid (13). Initiationof replication is achieved by site- and strand-specific nickingperformed by the NS1 protein, which remains covalently attachedto the 5' end of the nicked strand. In contrast to the activeorigin, the inactive origin in pL1-2GAA is not a substrate fornicking (8), and therefore no NS1-dependent replication occurs.We further analyzed the specificity of the RCR reactions takingplace in the reconstituted, kinase-free system by using pL1-2GAAas an inactive substrate and the mutant Y210F as replication-deficientNS1 control. In addition, replication products were analyzed afterimmunoprecipitation with $alpha$ NS antiserum. When E. coli Klenow fragment,DNA polymerase I (data not shown), or bacteriophage T7 polymerase(Fig. 3, lanes 8 to 12) was substituted for the eukaryotic polymerases,replication was found to occur irrespective of whether the templatescontained an active (T) or inactive (G) origin. The lack of NS1-dependentinitiation of the replication reactions driven by E. coli andphage T7 polymerases was also apparent from the failure of the $alpha$ NS1 serum to immunoprecipitate labeled DNA products (Fig. 3,lower panel) and the significant DNA synthesis detected with theNS1 mutant Y210F (Fig. 3, lane 8). In contrast, as reported previouslyfor simian virus 40 (SV40) DNA replication in vitro (69), T4DNA polymerase could successfully substitute for the cellularDNA polymerases contained in P2 to give rise to a specific RCRreaction with plasmids containing the active left-end (TC) originin the presence of P1 and NS1^P (Fig. 3, lane 4). Indeed, only limited repair synthesis occurredwith the substrate containing the inactive origin (Fig. 3, lane5), while initiation was NS1 dependent, as apparent from the formationof $alpha$ NS1-immunoprecipitatable replication products in the presenceof wild-type NS1^P but not Y210F (Fig. 3, lanes 3 and 4).

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FIG. 3. NS1-dependent RCR in a kinase-free in vitro system. Plasmids containing the active (T) or inactive (G) left-end origin were used as substrates to measure the capacity of NS1^P and NS1^O to support RCR in absence of endogenous protein kinases, in a system based on P1-Thr and bacteriophage DNA polymerases. T4 and T7, bacteriophage T4 and T7 DNA polymerases, respectively. The replication-deficient NS1 mutant Y210F was used as a negative control. Linearized ³²P-labeled replication products were analyzed on 0.8% agarose gels, either directly after proteinase K digestion (top panel) or after immunoprecipitations with $alpha$ NS_N (bottom panel). The positions of the linearized plasmid (a) and slower-migrating products (b and c) are indicated.

Since we were able to obtain a specific RCR reaction by using a kinase-free P1-Thr and T4 DNA polymerase in the presence ofnative NS1^P, we further investigated the requirements of this reaction forNS1 phosphorylation. As illustrated in Fig. 3, the patterns oflabeled DNA products generated in the presence of NS1^O and NS1^P could be distinguished in three respects. (i) The overall levelof DNA synthesis was much reduced when NS1 was dephosphorylated,which strongly suggests that phosphorylation modulates the capacityof NS1 for initiation and/or promoting RCR. (ii) Major productsof the RCR reaction taking place in the presence of NS1^P migrated more slowly than linearized plasmid DNA and can be ascribedto multiple rounds of plasmid template DNA copying, yielding circularmolecules with single-stranded tails of various lengths (13).These intermediates, marked c in Fig. 3, were not formed efficientlyin the presence of NS1^O, although labeled DNA was detected in the plasmid length region,which argues for a role of NS1 phosphorylation in the strand displacementsynthesis during RCR (and parvovirus DNA replication). This conclusionis in agreement with the previously reported main deficiency ofNS1^O in the helicase activity, which is thought to facilitate unwindingof the double-stranded template to allow the replication forkto proceed (Fig. 1B) (60). (iii) The predominantly labeled DNAproduct obtained with NS1^O (marked b in Fig. 3) was slightly upshifted compared with thelinearized plasmid (marked a). This mobility shift is expectedfor DNA molecules which underwent nicking and replication initiation,resulting in a short stretch of newly synthesized DNA in the absenceof extensive strand displacement synthesis. This species b wasnot detected when replication-competent NS1^P was used, suggesting that the lack of NS1 phosphorylation isassociated with an impairment of growing-strand elongation inalready initiated DNA molecules. It should also be stated thatbesides this modulation of the elongation step, the initiationof parvovirus DNA replication also appears to be stimulated byNS1 phosphorylation. Indeed, recently reported in vitro assayshave shown that although it is proficient in site-specific nicking,NS1^O is less efficient than NS1^P for this function (60).

Reactivation of NS1^O for RCR by members of the PKC family. Since NS1^O was able to support RCR in the presence of cell extracts containing endogenous protein kinases but distinguisheditself from NS1^P in its low capacity to achieve this reaction in the kinase-freein vitro replication system, we further attempted to reactiveNS1^O for RCR by providing exogenous cellular components. Previousinvestigations using commercially available PKC preparations indicatedthe involvement of this protein kinase family in regulation ofNS1 helicase activity (60). Therefore, we performed the followingreactivation experiments in the presence of Ca²⁺ and PS, which are known cofactors for PKC (44, 61). Indeed,under these conditions, NS1^O replication activity could be stimulated to a significant extentby supplying the reaction mixture with limited amounts of wholeHeLa cell replication extracts (data not shown). This result encouragedus to fractionate HeLa cell extracts in order to characterizethe NS1^O-activating components, and in particular to determine whetherthe rescue of NS1^O replication activity cosegregated with NS1 phosphorylation byspecific protein kinases aspostulated.

Figure 4 gives the purification scheme for HeLa cell extracts used for these reactivation experiments. Individual fractionswere tested for their ability to phosphorylate NS1^O. In parallel, various protein concentrations were used to determinethe capacity of individual or combined HeLa cell fractions forreactivating the RCR function of the underphosphorylated polypeptide.Native wild-type NS1^P and the replication-deficient mutant Y210F served as positiveand negative controls in these assays, respectively. The specificityof the reactions was also ascertained by using active (pL1-2TC)versus inactive (pL1-2GAA) origin-containing substrates and byimmunoprecipitating NS1-bound replication products with $alpha$ NS_N antiserum.Chromatography steps 1 and 2 were designed to achieve a firstbulk segregation of the multiple protein kinases which are ableto phosphorylate NS1^O. As illustrated in Fig. 2B and C, more than 50% of the NS1-targetedkinase activity segregated in phosphocellulose fraction P3 (step1) and proved to be nonessential, since NS1^O was almost as efficient as NS1^P for RCR in the sole presence of proteins contained in P1-Thrand P2. Furthermore, neither the whole P3 fraction nor subfractionsthereof were able to activate NS1^O in the kinase-free replication system (data not shown). Thisresult indicated that specific rather than random phosphorylationof NS1 was necessary for the replicative functions of the viralproduct. After further purification of P2 on anion-exchange columns(step 2), NS1^O-stimulating activity was recovered in the low-affinity DE-1 fraction,eluting between 50 and 200 mM NaCl (Fig. 5, lanes 4 and 7). Noadditional stimulation resulted from the supply of kinases presentin fractions eluting at higher salt concentrations, despite theirability to phosphorylate NS1^O to a significant extent in vitro (data not shown).

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FIG. 4. Purification scheme used to identify NS1^O-activating protein kinases. HeLa cell replication extracts were analyzed for protein kinases which are able to phosphorylate and activate NS1^O for RCR in a kinase-free system. Chromatography steps 1 (phosphocellulose) and 2 (anion exchange) allow the bulk separation of protein kinases. Steps 3 (protamine) and 4 (hydroxylapatite) are performed to further purify members of the PKC family. Selective elution of the fractions under investigation from rows 1, 2, and 3 was achieved with the indicated NaCl concentrations, while the hydroxylapatite-bound components (row 4) were eluted in phosphate buffer. PK: $-$ and PK: +++, undetectable and strong protein kinase activities, respectively, assayed in vitro with NS1^O as a substrate. F/T, flowthrough.

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FIG. 5. Activation of NS1^O for RCR by fractionated HeLa cell extracts. NS1-dependent RCR of plasmids containing the left-end active (T) or inactive (G) origin was determined in a kinase-free in vitro system based on P1-Thr and T4 DNA polymerase. Activation of NS1^O (lanes 4 to 14) was achieved by using the indicated protein components (see Fig. 4) in the presence or absence of protein kinase C cofactors. Only some of the protein-cofactor combinations that have been tested are illustrated, as most representative. Lanes 4 to 8 show the dependency of NS1^O activation on PKC cofactors. PS, Ca²⁺ plus PS. Lanes 9 to 14 show the segregation of protein components allowing the reactivation of dephosphorylated NS1. The illustrated reactions were carried out in presence of the PKC activators Ca²⁺ and PS (HA-1) or TPA (HA-2 and HA-1 plus HA-2). It should be mentioned that TPA-stimulated HA-1 or Ca²⁺+PS-stimulated HA-2 also failed to activate NS1^O (data not shown), while the combined protein components (HA-1 plus HA-2) were able to rescue NS1^O in the presence of Ca²⁺+PS instead of TPA. The NS1 mutant Y210F served as a negative control (lane 1). Native NS1^P was used as a phosphorylated, replication-competent standard (lanes 2 and 3). L, migration of the linearized plasmid. The lower panel presents reaction products after immunoprecipitation with $alpha$ NS_N.

The subsequent purification steps (steps 3 and 4) were applied to concentrate PKCs and to separate distinct isoforms of thisprotein kinase family. Protamine affinity columns are commonlyused to purify PKC from bulk proteins, due to the high affinityof these kinases for basic protein substrates (61). On the otherhand, at least some of the structurally related PKC isoforms canbe separated on hydroxylapatite columns, based on their variousrequirements for Ca²⁺ ions and affinities to phosphate groups (32, 62). As expected,NS1^O-activating components were retained on the protamine column andrecovered in fraction PA-2 after high-salt elution (data not shown).A further concentration of these components was achieved by hydroxylapatitechromatography, yielding an inactive flowthrough and two boundfractions of low (HA-1) and high (HA-2) affinity (eluting at 20and 120 to 400 mM KPO₄, respectively). Though inactive on theirown, the HA-1 and HA-2 fractions were able to reactivate NS1^O when supplied in combination in RCR assays (Fig. 5, lanes 9 to14; Table 1). The reaction stimulated by HA-1 and -2 was a specificNS1-dependent RCR process. Indeed, no significant DNA synthesiswas observed when the inactive GAA origin was used as a substrate(Fig. 5, lane 14), and the reaction products obtained with theactive (TC) origin were covalently attached to NS1 as shown byimmunoprecipitation (Fig. 5, bottom panel, lane 13). To furtherevaluate the active components within fractions HA-1 and HA-2,we performed the reactivation experiments in the presence or absenceof characteristic cofactors for PKCs (44, 61). As summarizedin Table 1 and illustrated in Fig. 5 and 6, reactivation of NS1^O in replication assays was strictly dependent upon addition ofPS, Ca²⁺+PS, TPA, or PS + TPA. This strongly argues for the involvementof members of the PKC family in modulation of NS1 replicativefunctions in vitro.

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TABLE 1. Dependence of the reactivation of NS1^O replicative function on PKC cofactors

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FIG. 6. Effect of PKC cofactors on activation of the NS1^O replicative functions in an entirely eukaryotic replication system. NS1^P and NS1^O were compared for RCR of plasmids containing the left-end active (T) or inactive (G) origin of replication by using P1-Thr plus P2-pol (containing endogenous DNA polymerases). NS1^O activity was tested in either the absence or presence (+ PS) of 1.5 µg of PS. All reaction were performed in the presence of 2 mM CaCl₂.

The reactivation experiments described above were carried out with a rather artificial replication system based on bacteriophageT4 DNA polymerase. To substantiate these data in the presenceof eukaryotic polymerases, we took advantage of the requirementof NS1^O activation for PKC cofactors. Unlike standard HeLa cell replicationextracts, fractions P1-Thr (purified on phosphocellulose and L-Thraffinity columns) and P2-pol (purified on phosphocellulose andDE52 columns) are depleted of residual membrane structures whichcan serve as PKC activators (61). Assuming that the resultsobtained with the kinase-free reconstituted system can be extrapolatedto mammalian DNA polymerases, these fractions should be supplementedwith PKC activators in order to render NS1^O competent for RCR. This prediction was tested by comparing NS1^P and NS1^O for RCR with P1-Thr plus P2-pol in the presence or absence ofPKC cofactors. As shown in Fig. 6, the ability of NS1^O (but not NS1^P) to support RCR of pL1-2TC templates under these conditions wasdependent upon addition of the PKC cofactors Ca²⁺ and PS, despite the fact that P2-pol contains, besides DNA polymerases,multiple protein kinases which do not require additional cofactorsfor activation. This experiment clearly demonstrates that dephosphorylatedNS1^O is not irreversibly inactivated with regard to its replicationfunction, and it extends the above-mentioned results to suggestthat phosphorylation by distinct protein kinases is required forNS1 activity in a purely eukaryotic DNA replicationsystem.

The purification profile and the cofactor requirements of the NS1^O-reactivating components in replication assays strongly suggestedPKC to be an essential kinase(s) for NS1 activation in vitro.In order to ascertain the presence of active PKC within the reactivatingHeLa cell fractions, we produced polyclonal antibodies againstthe most-conserved regions of PKC, which are between amino acids416 and 569 in PKC $gamma$ and between amino acids 310 and 444 in PKC $zeta$ ,and performed Western blotting with these immune affinity-purifiedantisera. As illustrated in Fig. 7A, multiple proteins with thesizes of known PKC isoforms were indeed immunodetected withinfractions HA-1 and HA-2, in addition to a major product of lowermolecular weight corresponding to PKCm, the proteolytically cleavedcatalytic domain of PKC. Moreover, as seen in Fig. 7B, both fractionsHA-1 and HA-2 were enriched in PKC activity compared with crudeHeLa cell extract or the negative controls P1-Thr (which doesnot contain significant protein kinase activity), and P3-DE3 (forwhich NS1^O constitutes a target for in vitro phosphorylation but not replicationreactivation [data not shown]), as determined with a commerciallyavailable PKC detection system (Amersham). Furthermore, by performingin vitro kinase assays in the presence of [ $gamma$ -³²P]ATP under conditions used in replication assays, NS1^O was found to serve as a substrate for semipurified protein kinasescontained in HA-1 and/or HA-2 (Fig. 7C). Surprisingly, overallNS1 phosphorylation was only slightly stimulated upon additionof PKC cofactors (data not shown). This may be because eitheradditional kinases were still present within the HA-1 and -2 fractionsor the cofactors target PKC on a specific phosphorylation site(s)within the NS1 polypeptide. Together, these results clearly demonstratedthat cellular factors able to reactivate the replicative functionsof NS1^O copurified with highly active PKCs contained within both fractionsHA-1 and HA-2. Furthermore, the requirement of HA-1 and -2-inducedRCR reactivation for specific PKC cofactors substantiated therole of one or more PKC isoforms from HA-1 and/or HA-2 in theupmodulation of NS1 replicative functions.

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FIG. 7. Detection of PKC within fractions HA-1 and HA-2 from HeLa cell extracts. (A) Western blot analysis of HA-1 or HA-2 after 10% SDS-PAGE, using peptide affinity-purified polyclonal antisera that were raised against the most-conserved regions of classical PKCs (PKC $gamma$ , amino acids 416 to 569; PKC $zeta$ , amino acids 310 to 444) and revealed the various PKC isoforms by cross-reaction. The expected migration positions of known PKC isoforms are given on the left: cPKC, classical PKC $alpha$ , - $beta$ , and - $gamma$ (approximately 80 kDa); a/nPKC, atypical PKC $iota$ / $lambda$ and - $zeta$ (70 to 72 kDa) and novel PKC $delta$ , - $eta$ , and - $theta$ (72 to 78 kDa). PKC $varepsilon$ (90 kDa) and PKCµ (115 kDa), higher-molecular-mass novel PKCs; PKCm (approximately 45 kDa), PKC catalytic domains produced by proteolytic cleavage. (B) PKC activity assays (Amersham) of fractions used for reactivation of NS1^O in replication reactions. Buffer, negative control in the absence of added protein components; PKC $alpha$ , 10 ng of His tag-purified recombinant PKC $alpha$ produced by recombinant vaccinia virus expression in HeLa cells; P1-Thr, fraction containing no NS1^O-targeted protein kinase activity (see Fig. 2B); P3-DE3: fraction which proved able to phosphorylate but failed to reactivate NS1^O (see Fig. 4); HeLa, standard HeLa cell replication extract; HA-1 and HA-2, NS1^O-activating fractions in RCR assays (see Fig. 5). The values are expressed as transferred ³²P-labeled substrate per 10 ng (recombinant PKC $alpha$ ) or 10 µg (HeLa cell fractions) of total effector proteins. (C) In vitro phosphorylation of 1 µg of NS1^O with protein fractions HA-1 and HA-2, used individually or in combination in the presence of PKC cofactors. The reactions were performed in the presence of [ $gamma$ -³²P]ATP for 30 min at 37°C, and radiolabeled NS1 was revealed by autoradiography after SDS-PAGE. In lane 4, the NS1^O substrate was omitted. The migration of NS1 is indicated.

Stimulation of NS1^O helicase activity by members of the PKC family. The above-mentioned analyses of NS1-driven RCR in the kinase-free in vitro replication system indicated that a major NS1 phosphorylation-dependentstep consisted of processive strand displacement synthesis (Fig.3). This step of RCR (and also parvovirus DNA replication) isthought to involve the unwinding function of NS1. Consistently,NS1^O was found to be heavily impaired for this biochemical activityin standard helicase assays (Fig. 1B) (60). In order to investigatewhether the intrinsic helicase function of NS1 might be regulatedby the same components as those identified with the in vitro RCRsystem, the HA- fractions were also tested for their ability torescue NS1^O in helicase assays. As illustrated in Fig. 8A, one of these fractions,HA-1, was able to stimulate the helicase function of NS1^O to a significant extent, whereas HA-2 or the flowthrough (HA-0)had no detectable effect. None of the hydroxylapatite fractionsexerted helicase activity by itself, even when tested in a 100-foldexcess over the amount used to stimulate the NS1^O helicase function (Fig. 8A, lanes 4 to 6), indicating that thisstimulation resulted from the activation of NS1^O rather than supply of a cellular helicase(s).

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FIG. 8. Reactivation of dephosphorylated NS1^O for helicase activity. Helicase assays were performed as described for Fig. 1B, using M13-VAR as a template. (A) Hydroxylapatite column fractions HA-0, HA-1, and HA-2 were tested for their intrinsic helicase activities (lanes 4 to 6) and for activation of the NS1^O helicase function in the presence of the PKC cofactor Ca²⁺+PS (lanes 8 to 10). Lane 7 shows the helicase activity of unstimulated NS1^O. The NS1 mutant K405R served as a negative control (lane 3). The reaction products were analyzed by native 7% PAGE in the presence of 0.1% SDS. Lanes 1 and 2, native (NAT) and denatured (DEN) input DNA, respectively. (B and C) Characterization of PKC isoforms present within the HA-1 fraction, which is able to reactivate NS1^O for helicase activity. (B) Dependence of HA-1-induced reactivation of NS1^O helicase function on defined PKC cofactors. Atypical PKCs ( $iota$ / $lambda$ and $zeta$ ) are stimulated by acid lipids (PS) but are insensitive to phorbol esters such as TPA, whereas novel and classical PKCs are only slightly activated by PS alone but respond strongly to TPA. Dephosphorylated NS1^O was assayed for helicase activity either alone (lane 5) or in the presence of HA-1 with or without the indicated PKC cofactors (lanes 7 to 9). The NS1 mutant K405R (lane 3) and native NS1^P (lane 4) served as negative and positive controls, respectively. The effect of HA-1 in the absence of NS1 is shown in lane 6. Lanes 1 and 2, native and denatured input DNA, respectively. (C) Immunodetection of atypical PKC in hydroxylapatite fractions. Equal protein amounts of HA-1 and HA-2 were analyzed by Western blotting with $alpha$ PKC $iota$ antibodies (Transduction Laboratories). A HeLa cell replication extract served as a positive control. Size markers and expected migrations of different PKC isoforms are indicated on the right (for abbreviations, see the legend to Fig. 7A). The estimated migrations of PKC $lambda$ / $iota$ and PKCm, which are recognized by $alpha$ PKC $iota$ , are indicated on the left.

These assays were performed in the presence of Ca²⁺+PS, i.e., under conditions which activate all members of the PKC familyin vitro. PKCs have been subdivided into three subgroups accordingto their cofactor requirements. Classical ( $alpha$ , $beta$ , and $gamma$ ) and novel( $delta$ , $varepsilon$ , $theta$ , $eta$ , and µ) PKC isoforms are stimulated through bindingof phorbol esters (such as TPA) and only to a minor extent bybinding of acid lipids (such as PS). Full activation of classicalPKC is also achieved by Ca²⁺ in addition to PS, while novel PKCs do not contain a Ca²⁺-binding site. Members of the last group, designated atypicalPKC isoforms ( $iota$ / $lambda$ and $zeta$ ), lack a calcium-binding domain and donot respond to TPA either, but they are stimulated by acid lipids.Finally, PKCm, the catalytic domain of PKC which derives fromproteolytic cleavage, is constitutively active; i.e., its kinaseactivity is independent of cofactors (44, 61). In order tocharacterize the activating kinase(s) present in fraction HA-1,we further tested NS1^O reactivation for helicase function in the presence of HA-1 togetherwith selected PKC cofactors. As seen in Fig. 8B, the HA-1 fractionhad a moderate, constitutive stimulatory effect in absence ofcofactors (lane 7), which may be ascribed to PKCm and/or othercofactor-independent components. Interestingly, this activationwas significantly enhanced upon supply of PS (lane 8), while TPAfailed to increase the capacity of HA-1 to stimulate the helicasefunction of NS1^O (lane 9). As summarized in Table 1, this PS responsiveness andTPA insensitivity of the HA-1-induced rescue of NS1^O point to an atypical PKC(s) as the effector(s) mediating thedependence of NS1 helicase activity on phosphorylation. This conclusionwas substantiated by Western blot analysis of fractions HA-1 andHA-2 with specific antibodies recognizing the atypical PKC $iota$ . Asshown in Fig. 8C, the atypical PKC $iota$ segregated mainly to fractionHA-1 during the purification procedure, while HA-2, which wasunable to activate NS1^O in helicase assays, did not contain substantial amounts of thisPKC isoform. The PS responsiveness of the NS1 helicase-stimulatingfactor(s) and its cosegregation with PKC $iota$ into HA-1 strongly suggestedthat atypical PKCs are involved in the upmodulation of the NS1DNA-unwindingfunction.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

NS1, the major nonstructural protein of MVM, is involved in multiple functions necessary for progeny virus production, rangingfrom DNA replication to promoter regulation and toxic action onthe host cell (15). Such a variety of tasks is unlikely to beachievable by a single polypeptide and usually requires the multifunctionalprotein to interact with heterologous proteins (42), to self-assembleinto higher-order oligomers (4), to associate with cofactors(61), and/or to become posttranslationally modified. The lastpossibility can provide an original polypeptide with functionalheterogeneity through the addition of various molecule groups,catalyzed with high efficiency by enzymes present in rather smallamounts, targeted on a large protein pool. All of the above-mentionedmodes of regulation have been assigned to NS1, including interactionswith cellular partner proteins (24, 36), oligomerization (58),and phosphorylation (20). Interestingly, NS1 oligomerizationhas been implicated in the control of NS1 replicative functions,in particular helicase activity (63). It is worth noting thatNS1 self-assembly to produce higher-order oligomers is dependenton an intact nucleoside triphosphate-binding domain (58) andmight thus be regulated by association with this cofactor. Furthermore,the ATP-bound form of NS1 was found to be most competent for site-specificDNA binding (21). Indeed, ATP binding and/or hydrolysis seemsto be crucial for many NS1 functions, as apparent from the factthat mutagenesis of the ATP-binding domain abolishes all NS1 activitiesdescribed so far (10, 21, 38, 39, 57-59). In turn, theNS1-associated ATP turnover was recently found to be controlledby phosphorylation, at least under in vitro conditions (60).Thus, the regulation of an activity which plays a pivotal rolein NS1 functions may be traced back to the modification of NS1through phosphorylation. NS1 dephosphorylation correlates witha reduction of NS1 ATPase activity in vitro, which is associatedwith an increase in the affinity of the viral product for itsDNA recognition motif and with a decrease of helicase and site-specificnickase functions (60). This regulation might be physiologicallyrelevant, since NS1 has been shown to be phosphorylated in vivo(2, 11, 20). The present work was carried out to furthercharacterize the cellular protein kinases involved in the upmodulationof NS1 replicativefunctions.

In this study, using an in vitro replication system devoid of endogenous protein kinases, we obtained evidence that a centralNS1 function necessary for progeny virus production, namely, replicationinitiated at the left-end origin, is upmodulated by phosphorylationof NS1 and that members of the PKC family participate in thisstimulation. The phosphorylation dependence of NS1 is reminiscentof the regulation of large T antigen (LT), the initiator proteinfor SV40 DNA replication (71). LT, which is expressed in nondividingcells and is able to drive quiescent cells into S phase, becomesactivated for replication by phosphorylation at T124 through cyclin-dependentkinases. This regulation results in a coordination between SV40and host cell DNA replication (1, 47). As in the case ofSV40, parvovirus DNA replication has been shown to be dependenton the S phase of host cells (15), hence the restriction ofparvovirus multiplication in vivo to proliferating tissues (43).Yet, in contrast to the case for LT, NS1 production is limitedduring G₀/G₁ (25, 66), and parvoviruses fail to drive quiescentcells into S phase (15). Moreover, extracts derived from cellsarrested in G₀ are able to activate the replicative functionsof dephosphorylated NS1 in vitro (56). Therefore, posttranslationalmodifications of NS1 do not account for the S phase dependencyof parvovirus DNA replication. Another feature of parvovirusesis their striking oncotropism (65). This tropism could be mimickedin various cell culture systems, where the restrictions to parvovirusreplication detected in normal parental cell lines were foundto be at least partly overcome upon neoplastic transformation(12). In this context, it is interesting that PKC activators,such as phorbol esters, also exert strong effects on cell proliferation,differentiation, and, most intriguingly, tumor promotion (44,61). Moreover, it has been reported that overexpression of PKC $varepsilon$ ,a novel PKC isoform which is activated by phorbol esters and hasbeen detected in A9 cells (a natural host cell line permissivefor MVMp [26]), leads to cell transformation in vitro (6,49). These correlations of oncogenic transformation with changesin both PKC activity and cell permissiveness to parvovirus replication,together with the present evidence of a role of PKC in the regulationof the pivotal viral replicator protein NS1, raise the possibilitythat this regulation may contribute to the oncotropism ofparvoviruses.

Native NS1^P was able to initiate RCR, leading to extensive strand displacement synthesis in the absence of protein kinases.In contrast, NS1^O had a restricted phenotype that was characterized by the formationof a distinct NS1-bound replication intermediate. This intermediatemigrated in agarose gels as a molecule in which DNA synthesiswas initiated but became arrested prior to strand displacementsynthesis, suggesting that besides its role in the site-specificinitiation of DNA replication, NS1 is also essential to drivethe subsequent strand displacement reaction in a phosphorylation-dependentway. This is in agreement with previously reported findings thatdephosphorylated NS1^O is deficient in helicase activity (60), which would accountfor its inability to allow the replication fork to proceed duringDNA synthesis. Therefore, regulation of the DNA-unwinding activityof NS1 might be of crucial importance to turn on replication.It should be stated, however, that the helicase deficiency ofNS1^O could be corrected by supplementing solely the HA-1 fraction,while RCR reactivation of NS1^O required both protein fractions HA-1 and HA-2. Thus, more thanone protein kinase seem to be necessary to switch NS1^O on for DNA replication. The additional replicative functionsof NS1 which are regulated by phosphorylation, besides helicaseactivity, are as yet undefined. One candidate is the nicking reaction,which is achieved by NS1^O to a detectable, albeit reduced level compared to NS1^P, both in the RCR assay and in an in vitro nicking assay performedin the absence of additional cellular components (60). However,this reduction could also be a consequence of the defect of NS1^O in DNA unwinding, since the latter is thought to facilitate single-strandnicking (35, 67). Other potential phosphorylation-dependentNS1 replicative functions might be considered by analogy withSV40 LT. LT binds to the origin of replication in the absenceof phosphorylation (45, 46, 50) and is able to interactwith components of the basic replication machinery such as replicatorprotein A (48) or polymerase $alpha$ primase (28, 29) to establishthe replication complex by protein-protein interactions. It istempting to speculate that NS1 may act in a similar way, sinceit is known that LT- and NS1-driven in vitro replications sharespecific requirements for eukaryotic DNA polymerases or the relatedT4 DNA polymerase (69) and for template DNA unwinding by thehelicase activities of the respective viral proteins (71). Whilebinding to target (ACCA) motifs on the viral DNA, NS1 fulfillsfunctions involved not only in DNA replication but also in promoterregulation, raising the possibility that distinct NS1 phosphorylationevents may regulate the interaction of the viral polypeptide withproteins from the basal replication and/or transcription machinery.NS1 was indeed demonstrated to interact specifically with generaltranscription factors (36, 40).

NS1 has been shown to be a target for phosphorylation by many protein kinases in vitro (2, 60). Indeed, most HeLa cellfractions tested in this study were found to exhibit NS1 phosphorylationactivity. In contrast, only selected fractions of the originalHeLa cell replication extract were able to activate NS1^O for replication activity, pointing to the involvement of specifickinases and phosphorylation events in NS1 regulation. Based onthe cofactor requirements for NS1^O reactivation and the purification properties of effector kinases,we were able to assign, at least in part, the capacity for NS1phosphorylation and reactivation in vitro to members of the PKCfamily. In particular, the NS1 unwinding function might be modulatedby atypical PKCs, given its responsiveness to acid lipids butnot to phorbol esters. As stated above, regulation of the NS1replicative functions appears to be complex and to involve morethan one protein kinase, as indicated by the fact that rescueof NS1^O for RCR required at least two protein components that could beseparated by hydroxylapatite chromatography. When combined, theactive HA- fractions were able to rescue the RCR functions ofNS1^O to a significant extent in the presence of the phorbol esterTPA. Since TPA was unable to activate the PKC responsible forstimulating the helicase function of NS1, our results suggestthat at least two PKCs may be involved in NS1 regulation. Oneof these kinases appears to be one of the classical or novel PKCisoforms (which respond to TPA) and controls an as-yet-undefinedNS1 replicative function, while the other is a TPA-insensitiveatypical PKC isoform that regulates the DNA-unwinding activityof NS1. The latter PKC may be activated by the former, therebyaccounting for the sole requirement of TPA as a cofactor to rescuethe RCR capacity of NS1^O, in agreement with the fact that PKCs are themselves regulatedby phosphorylation (33). Mapping of the NS1 phosphorylationsites involved in the modulation of replicative functions, aswell as further characterization of the cellular protein kinasesresponsible for these modifications, should contribute to understandingthe posttranslational regulation of NS1activities.

	ACKNOWLEDGMENTS

We are indebted to Bernard Moss (National Institutes of Health) for making pTM-1 plasmid and the vTF7-3 virus available andto Hubert Hug (Deutsches Krebsforschungzentrum) for providingfull-length PKC $alpha$ , PKC $gamma$ , and PKC $zeta$ cDNA clones. We are most gratefulto Peter Tattersall and Susan Cotmore for sharing constructs usedin our assays, stimulating discussions, and critical comments.We also thank Claudia Plotzky for technical assistance and RainerSchmidt, Michael Gschwendt, and Jesper Christensen for helpfulcomments concerning fractionation of replication extracts andcharacterization ofPKC.

This work was supported by the Commission of the European Communities and the German-Israeli Foundation for Scientific Researchand Development. R.C. was supported in part by a fellowship fromLa Ligue Nationale Contre leCancer.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Applied Tumor Virology, Abt. F0100, and INSERM U375, Deutsches Krebsforschungszentrum,Im Neuenheimer Feld 242, D-69120 Heidelberg, Germany. Phone: (49)6221 424963. Fax: (49) 6221 424962. E-mail: jpf.nuesch{at}dkfz-heidelberg.de.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Adamczewsky, J. P., J. V. Gannon, and T. Hunt. 1993. Simian virus 40 large T antigen associates with cyclin A and p33-cdk2. J. Virol. 67:6551-6557[Abstract/Free Full Text].

2. Astell, C. R., Q. Liu, C. E. Harris, J. Brunstein, H. K. Jindal, and P. Tam. 1996. Minute virus of mice cis-acting sequences required for genome replication and the role of the trans-acting viral protein, NS1. Prog. Nucleic Acid Res. Mol. Biol. 55:245-285[Medline].

3. Baldauf, A., K. Willwand, E. Mumtsidu, J. P. F. Nüesch, and J. Rommelaere. 1997. Formation of circular replicative form (RF) from single-stranded virion DNA and initiation of DNA replication at the RF 5' telomere induced by the minute virus of mice nonstructural protein NS1. J. Virol. 71:971-980[Abstract].

4. Bradley, M. K., J. D. Griffin, and D. M. Livingston. 1982. Relationship of oligomerization to enzymatic and DNA-binding properties of the SV40 large T antigen. Cell 28:125-134[Medline].

5. Brandenburger, A., D. Legendre, B. Avalosse, and J. Rommelaere. 1990. NS1 and NS2 proteins may act synergistically in the cytopathogenicity of parvovirus MVMp. Virology 174:576-584[Medline].

6. Cacace, A. M., S. N. Guadagno, R. S. Krauss, D. Fabbro, and I. B. Weinstein. 1993. The epsilon isoform of protein kinase C is an oncogene when overexpressed in rat fibroblasts. Oncogene 8:2095-2104[Medline].

7. Caillet Fauquet, P., M. Perros, A. Brandenburger, P. Spegelaere, and J. Rommelaere. 1990. Programmed killing of human cells by means of an inducible clone of parvoviral genes encoding non-structural proteins. EMBO J. 9:2989-2995[Medline].

8. Christensen, J., S. F. Cotmore, and P. Tattersall. 1997. A novel cellular site-specific DNA-binding protein cooperates with the viral NS1 polypeptide to initiate parvovirus DNA replication. J. Virol. 71:1405-1416[Abstract].

9. Christensen, J., S. F. Cotmore, and P. Tattersall. 1997. Parvovirus initiation factor (PIF): a novel human DNA binding factor which coordinately recognizes two ACGT motifs. J. Virol. 71:5733-5741[Abstract].

10. Christensen, J., M. Pederson, B. Aasted, and S. Alexandersen. 1995. Purification and characterization of the major nonstructural protein (NS1) of Aleutian mink disease parvovirus. J. Virol. 69:1802-1809[Abstract].

11. Corbau, R., J. P. F. Nüesch, N. Salome, and J. Rommelaere. 1997. Phosphorylation study of minute virus of mice NS1 protein, P20. VIIth International Parvovirus Workshop, Heidelberg, Germany .

12. Cornelis, J. J., P. Becquart, N. Duponchel, N. Salome, B. L. Avalosse, M. Namba, and J. Rommelaere. 1988. Transformation of human fibroblasts by ionizing radiation, a chemical carcinogen, or simian virus 40 correlates with an increase in susceptibility to the autonomous parvovirus H-1 and minute virus of mice. J. Virol. 62:1679-1686[Abstract/Free Full Text].

13. Cotmore, S. F., and P. Tattersall. 1994. An asymmetric nucleotide in the parvoviral 3' hairpin directs segregation of a single active origin of DNA replication. EMBO J. 13:4145-4152[Medline].

14. Cotmore, S. F., J. P. Nüesch, and P. Tattersall. 1993. Asymmetric resolution of a parvovirus palindrome in vitro. J. Virol. 67:1579-1589[Abstract/Free Full Text].

15. Cotmore, S. F., and P. Tattersall. 1987. The autonomously replicating parvoviruses of vertebrates. Adv. Virus Res. 33:91-174[Medline].

16. Cotmore, S. F., and P. Tattersall. 1995. DNA replication in the autonomous parvoviruses. Semin. Virol. 6:271-281.

17. Cotmore, S. F., J. P. Nüesch, and P. Tattersall. 1992. In vitro excision and replication of 5' telomeres of minute virus of mice DNA from cloned palindromic concatemer junctions. Virology 190:365-377[Medline].

18. Cotmore, S. F., and P. Tattersall. 1992. In vivo resolution of circular plasmids containing concatemer junction fragments from minute virus of mice DNA and their subsequent replication as linear molecules. J. Virol. 66:420-431[Abstract/Free Full Text].

19. Cotmore, S. F., and P. Tattersall. 1988. The NS1 polypeptide of minute virus of mice is covalently attached to the 5' termini of duplex replicative-form DNA and progeny single strands. J. Virol. 62:851-860[Abstract/Free Full Text].

20. Cotmore, S. F., and P. Tattersall. 1986. The NS1 polypeptide of the autonomous parvovirus MVM is a nuclear phosphoprotein. Virus Res. 4:243-250[Medline].

21. Cotmore, S. F., J. Christensen, J. P. Nüesch, and P. Tattersall. 1995. The NS1 polypeptide of the murine parvovirus minute virus of mice binds to DNA sequences containing the motif [ACCA]2-3. J. Virol. 69:1652-1660[Abstract].

22. Cotmore, S. F., A. M. D'Abramo, L. F. Carbonell, J. Bratton, and P. Tattersall. 1997. The NS2 polypeptide of parvovirus MVM is required for capsid assembly in murine cells. Virology 231:267-289[Medline].

23. Cotmore, S. F., and P. Tattersall. 1986. Organization of nonstructural genes of the autonomous parvovirus minute virus of mice. J. Virol. 58:724-732[Abstract/Free Full Text].

24. Cziepluch, C., E. Kordes, R. Poirey, A. Grewenig, J. Rommelaere, and J.-C. Jauniaux. 1998. Identification of a novel cellular TPR-containing protein, SGT, that interacts with the nonstructural protein NS1 of parvovirus H-1. J. Virol. 72:4149-4156[Abstract/Free Full Text].

25. Deleu, L., F. Fuks, D. Spitkovsky, R. Horlein, S. Faisst, and J. Rommelaere. 1998. Opposite transcriptional effects of cyclic AMP-responsive elements on confluent or p27-kip-expressing cells versus serum-starved or growing cells. Mol. Cell. Biol. 18:409-419[Abstract/Free Full Text].

26. Dettwiler, S. Unpublished observations.

27. Doerig, C., B. Hirt, J. P. Antonietti, and P. Beard. 1990. Nonstructural proteins of parvovirus B19 and minute virus of mice control transcription. J. Virol. 64:387-396[Abstract/Free Full Text].

28. Dornreiter, I., L. F. Erdile, I. U. Gilbert, W. D. von Winkler, T. J. Kelly, and E. Fanning. 1992. Interaction of DNA polymerase alpha-primase with cellular replication protein A and SV40 T antigen. EMBO J. 11:769-779[Medline].

29. Dornreiter, I., A. Hoss, A. K. Arthur, and E. Fanning. 1990. SV40 T antigen binds directly to the catalytic subunit of DNA polymerase a. EMBO J. 9:3329-3336[Medline].

30. Finkenzeller, G., D. Marme, and H. Hug. 1990. Sequence of human protein kinase C a. Nucleic Acids Res. 18:2183[Free Full Text].

31. Harlow, E., and D. Lane. 1988. Antibodies: a laboratory manual. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

32. Huang, K.-P., and F. L. Huang. 1991. Purification and analysis of protein kinase C isozymes, p. 241-252. In T. Hunter, and B. M. Sefton (ed.), Protein phosphorylation, part A, vol. 200. Academic Press, Inc., San Diego, Calif.

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1.	Adamczewsky, J. P., J. V. Gannon, and T. Hunt. 1993. Simian virus 40 large T antigen associates with cyclin A and p33-cdk2. J. Virol. 67:6551-6557[Abstract/Free Full Text].
2.	Astell, C. R., Q. Liu, C. E. Harris, J. Brunstein, H. K. Jindal, and P. Tam. 1996. Minute virus of mice cis-acting sequences required for genome replication and the role of the trans-acting viral protein, NS1. Prog. Nucleic Acid Res. Mol. Biol. 55:245-285[Medline].
3.	Baldauf, A., K. Willwand, E. Mumtsidu, J. P. F. Nüesch, and J. Rommelaere. 1997. Formation of circular replicative form (RF) from single-stranded virion DNA and initiation of DNA replication at the RF 5' telomere induced by the minute virus of mice nonstructural protein NS1. J. Virol. 71:971-980[Abstract].
4.	Bradley, M. K., J. D. Griffin, and D. M. Livingston. 1982. Relationship of oligomerization to enzymatic and DNA-binding properties of the SV40 large T antigen. Cell 28:125-134[Medline].
5.	Brandenburger, A., D. Legendre, B. Avalosse, and J. Rommelaere. 1990. NS1 and NS2 proteins may act synergistically in the cytopathogenicity of parvovirus MVMp. Virology 174:576-584[Medline].
6.	Cacace, A. M., S. N. Guadagno, R. S. Krauss, D. Fabbro, and I. B. Weinstein. 1993. The epsilon isoform of protein kinase C is an oncogene when overexpressed in rat fibroblasts. Oncogene 8:2095-2104[Medline].
7.	Caillet Fauquet, P., M. Perros, A. Brandenburger, P. Spegelaere, and J. Rommelaere. 1990. Programmed killing of human cells by means of an inducible clone of parvoviral genes encoding non-structural proteins. EMBO J. 9:2989-2995[Medline].
8.	Christensen, J., S. F. Cotmore, and P. Tattersall. 1997. A novel cellular site-specific DNA-binding protein cooperates with the viral NS1 polypeptide to initiate parvovirus DNA replication. J. Virol. 71:1405-1416[Abstract].
9.	Christensen, J., S. F. Cotmore, and P. Tattersall. 1997. Parvovirus initiation factor (PIF): a novel human DNA binding factor which coordinately recognizes two ACGT motifs. J. Virol. 71:5733-5741[Abstract].
10.	Christensen, J., M. Pederson, B. Aasted, and S. Alexandersen. 1995. Purification and characterization of the major nonstructural protein (NS1) of Aleutian mink disease parvovirus. J. Virol. 69:1802-1809[Abstract].
11.	Corbau, R., J. P. F. Nüesch, N. Salome, and J. Rommelaere. 1997. Phosphorylation study of minute virus of mice NS1 protein, P20. VIIth International Parvovirus Workshop, Heidelberg, Germany .
12.	Cornelis, J. J., P. Becquart, N. Duponchel, N. Salome, B. L. Avalosse, M. Namba, and J. Rommelaere. 1988. Transformation of human fibroblasts by ionizing radiation, a chemical carcinogen, or simian virus 40 correlates with an increase in susceptibility to the autonomous parvovirus H-1 and minute virus of mice. J. Virol. 62:1679-1686[Abstract/Free Full Text].
13.	Cotmore, S. F., and P. Tattersall. 1994. An asymmetric nucleotide in the parvoviral 3' hairpin directs segregation of a single active origin of DNA replication. EMBO J. 13:4145-4152[Medline].
14.	Cotmore, S. F., J. P. Nüesch, and P. Tattersall. 1993. Asymmetric resolution of a parvovirus palindrome in vitro. J. Virol. 67:1579-1589[Abstract/Free Full Text].
15.	Cotmore, S. F., and P. Tattersall. 1987. The autonomously replicating parvoviruses of vertebrates. Adv. Virus Res. 33:91-174[Medline].
16.	Cotmore, S. F., and P. Tattersall. 1995. DNA replication in the autonomous parvoviruses. Semin. Virol. 6:271-281.
17.	Cotmore, S. F., J. P. Nüesch, and P. Tattersall. 1992. In vitro excision and replication of 5' telomeres of minute virus of mice DNA from cloned palindromic concatemer junctions. Virology 190:365-377[Medline].
18.	Cotmore, S. F., and P. Tattersall. 1992. In vivo resolution of circular plasmids containing concatemer junction fragments from minute virus of mice DNA and their subsequent replication as linear molecules. J. Virol. 66:420-431[Abstract/Free Full Text].
19.	Cotmore, S. F., and P. Tattersall. 1988. The NS1 polypeptide of minute virus of mice is covalently attached to the 5' termini of duplex replicative-form DNA and progeny single strands. J. Virol. 62:851-860[Abstract/Free Full Text].
20.	Cotmore, S. F., and P. Tattersall. 1986. The NS1 polypeptide of the autonomous parvovirus MVM is a nuclear phosphoprotein. Virus Res. 4:243-250[Medline].
21.	Cotmore, S. F., J. Christensen, J. P. Nüesch, and P. Tattersall. 1995. The NS1 polypeptide of the murine parvovirus minute virus of mice binds to DNA sequences containing the motif [ACCA]2-3. J. Virol. 69:1652-1660[Abstract].
22.	Cotmore, S. F., A. M. D'Abramo, L. F. Carbonell, J. Bratton, and P. Tattersall. 1997. The NS2 polypeptide of parvovirus MVM is required for capsid assembly in murine cells. Virology 231:267-289[Medline].
23.	Cotmore, S. F., and P. Tattersall. 1986. Organization of nonstructural genes of the autonomous parvovirus minute virus of mice. J. Virol. 58:724-732[Abstract/Free Full Text].
24.	Cziepluch, C., E. Kordes, R. Poirey, A. Grewenig, J. Rommelaere, and J.-C. Jauniaux. 1998. Identification of a novel cellular TPR-containing protein, SGT, that interacts with the nonstructural protein NS1 of parvovirus H-1. J. Virol. 72:4149-4156[Abstract/Free Full Text].
25.	Deleu, L., F. Fuks, D. Spitkovsky, R. Horlein, S. Faisst, and J. Rommelaere. 1998. Opposite transcriptional effects of cyclic AMP-responsive elements on confluent or p27-kip-expressing cells versus serum-starved or growing cells. Mol. Cell. Biol. 18:409-419[Abstract/Free Full Text].
26.	Dettwiler, S. Unpublished observations.
27.	Doerig, C., B. Hirt, J. P. Antonietti, and P. Beard. 1990. Nonstructural proteins of parvovirus B19 and minute virus of mice control transcription. J. Virol. 64:387-396[Abstract/Free Full Text].
28.	Dornreiter, I., L. F. Erdile, I. U. Gilbert, W. D. von Winkler, T. J. Kelly, and E. Fanning. 1992. Interaction of DNA polymerase alpha-primase with cellular replication protein A and SV40 T antigen. EMBO J. 11:769-779[Medline].
29.	Dornreiter, I., A. Hoss, A. K. Arthur, and E. Fanning. 1990. SV40 T antigen binds directly to the catalytic subunit of DNA polymerase a. EMBO J. 9:3329-3336[Medline].
30.	Finkenzeller, G., D. Marme, and H. Hug. 1990. Sequence of human protein kinase C a. Nucleic Acids Res. 18:2183[Free Full Text].
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