Simian Virus 40 Vp1 DNA-Binding Domain Is Functionally Separable from the Overlapping Nuclear Localization Signal and Is Required for Effective Virion Formation and Full Viability

doi:10.1128/JVI.75.16.7321-7329.2001

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Journal of Virology, August 2001, p. 7321-7329, Vol. 75, No. 16
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.16.7321-7329.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Simian Virus 40 Vp1 DNA-Binding Domain Is Functionally Separable from the Overlapping Nuclear Localization Signal and Is Required for Effective Virion Formation and Full Viability

Peggy P. Li, Akira Nakanishi, Dorothy Shum, Peter C.-K. Sun, Adler M. Salazar, Cesar F. Fernandez, Sze-Wai Chan, and Harumi Kasamatsu^*

Department of Molecular, Cell and Developmental Biology and Molecular Biology Institute, University of California at Los Angeles, Los Angeles, California 90095

Received 19 January 2001/Accepted 17 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

A DNA-binding domain (DBD) was identified on simian virus 40 (SV40) major capsid protein Vp1, and the domain's function inthe SV40 life cycle was examined. The DBD was mapped by assayingvarious recombinant Vp1 proteins for DNA binding in vitro. Thecarboxy-terminal 58-residue truncated Vp1 $Delta$ C58 pentamer bound DNAwith a K_d of 1.8 × 10⁹ M in terms of the protein pentamer, while full-length Vp1 andcarboxy-terminal-17-truncated Vp1 $Delta$ C17 had comparable apparentK_ds of 5.3 × 10⁹ to 7.3 × 10⁹ M in terms of the protein monomers. Previously identified onVp1 was a nuclear localization signal (NLS) consisting of twoN-terminal basic clusters, NLS1 (4-KRK-6) and NLS2 (15-KKPK-18).Vp1 $Delta$ C58 pentamers harboring multiple-point mutations in NLS1 (NLSm1),NLS2 (NLSm2), or both basic clusters (NLSm1 · 2) had progressivelydecreased DNA-binding activity, down to 0.7% of the Vp1 $Delta$ C58 levelfor NLSm1 · 2 Vp1. These data, along with those of N-terminallytruncated proteins, placed the DBD in overlap with the bipartiteNLS. The role of the Vp1 DBD during infection was investigatedby taking advantage of NLS phenotypic complementation (N. Ishii,A. Nakanishi, M. Yamada, M. H. Macalalad, and H. Kasamatsu, J.Virol. 68:8209-8216, 1994), in which an NLS-defective Vp1 couldlocalize to the nucleus in the presence of wild-type minor capsidproteins Vp2 and Vp3. This approach made it possible to dissectthe role of the bifunctional Vp1 NLS-DBD in virion assembly inthe nucleus. Mutants of the viable nonoverlaping SV40 (NO-SV40)DNA NLSm1, NLSm2, and NLSm1 · 2 replicated normally followingtransfection into host cells and produced capsid proteins at normallevels. All mutant Vp1s were able to interact with Vp3 in vitro.The mutants NLSm1 and NLSm1 · 2 were nonviable, and the mutantVp1s unexpectedly failed to localize to the nucleus though Vp2and Vp3 did, suggesting that the mutated NLS1 acted as a dominantsignal for the cytoplasmic localization of Vp1. Mutant NLSm2,for which the mutant Vp1's nuclear localization defect was complementedby Vp2 and Vp3, displayed a 5,000-fold reduced viability. Analysisof NLSm2 DNA-transfected cell lysate revealed a 10-fold reductionin the level of DNase I-protected viral DNA, and yet virion-likeparticles were found among the DNase I-resistant material. Collectiveresults support a role for Vp1 NLS2-DBD2 in the assembly of virionparticles. The results also suggest that this determinant canfunction in the infection of newcells.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The virion particle of simian virus 40 (SV40), like those of other papovaviruses, packages the double-stranded circular viralDNA in an icosahedrally symmetric capsid. The SV40 capsid is composedof 72 pentamers of the major capsid protein Vp1, and the pentamericunits are tied together by the carboxy-terminal arms which extendinto neighboring pentamers (20, 27). The amino-terminal 15amino acids of Vp1 are not visible in the crystal structure dueto disorder but probably extend into the virion core to interactwith the viral minichromosome (20), which consists of the viralDNA and the four cellular core histones. A lower-resolution viewof murine polyomavirus virions identifies molecules of the minorcapsid proteins Vp2 and Vp3 (Vp2/3) as prongs that extend fromthe minichromosome core into the axial cavities of Vp1 pentamers(10). Though much is known about the structure of the virion,how virions are assembled in the cell nucleus during productiveinfection is still not well defined. Presumed to be importantfor the assembly is the interaction of the capsid proteins withDNA and with histones. Since all capsid proteins of SV40 bindDNA (4, 26), but only Vp1 of polyomavirus does (2, 22),the interactions involved in the assembly process can be differenteven among members of the papovavirus family. Defining a functionalDNA-binding domain (DBD) for the interaction of each capsid proteinwith viral DNA may unravel the unique process for the assemblyof individualviruses.

SV40 assembly is thought to consist of two phases. In the "subvirion" assembly phase, pentamerized Vp1 associates with Vp2/3in the cytoplasm soon after the proteins' synthesis, and theyare transported to the nucleus as such subvirion complexes (9,21). All of the SV40 Vp1, Vp2, and Vp3 harbor nuclear localizationsignals (NLSs) (3, 13). Consistent with the capsid proteins'interaction prior to nuclear transport, wild-type Vp2/3 couldrescue the nuclear localization of an NLS-defective Vp1 and viceversa (13). This phenotypic complementation would prove usefulin our functional dissection of the Vp1 DBD (see below). The secondphase of "virion" assembly begins once the capsid proteins enterthe nucleus, the site of viral DNA replication and packaging.In a stepwise model for virion formation, the capsid proteinsare sequentially added to and arranged on the viral minichromosome,resulting in the condensation and packaging of the viral DNA andthe formation of the capsid (1, 5, 15). All three SV40capsid proteins can bind DNA nonspecifically (4, 26). Thecooperative binding of Vp3 and the transcription factor Sp1 toses, the encapsidation signal of SV40 DNA, has been proposed toprovide packaging specificity by nucleating the capsid proteins'addition to the viral minichromosome (6, 11, 23). The DNA-bindingand protein-interactive functions of individual capsid proteinsmay collectively contribute to the packaging or virion assemblyprocess. In this study, we mapped the DBD of SV40 Vp1 and foundthat it overlaps with the previously identified, amino-terminalbipartite NLS (14), which comprises two clusters of basic residues,4-lysine-arginine-lysine-6 and 15-lysine-lysine-proline-lysine-18.We also examined whether this DBD is important for the formationof infectious virions in the viral life cycle. Despite the overlapof the DBD with the NLS, the application of phenotypic complementationhas allowed us to identify at least the second basic cluster,represented by mutant NLSm2, as a determinant for nuclear virionassembly. Our results are consistent with an important role ofthe Vp1 DNA-binding activity in the proper packaging ofvirions.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of plasmids. Subcloning was performed using standard techniques (25). All mutagenized nucleotides were confirmed by double-stranded DNAsequencing, as were the absence of unwanted mutations within theVp1 gene. In the DNA sequences below, mutated SV40 nucleotidesare given in lowercase letters, and relevant restriction sitesare underlined. Vp1 amino acids are numbered from the alanineof the secondcodon.

A series of pQE-Vp1 plasmids were used to express Vp1 as carboxy-terminally (histidine)₆ (H6)-tagged proteins (see Fig. 1Efor diagrams). First, pQE-XbaMCS was made from pQE60 (Qiagen)by knocking out the XbaI site and inserting a linker through NcoIand BgIII sites to introduce XbaI and BamHI sites in the multicloningregion. To express the first 344 Vp1 residues (Vp1 $Delta$ C17), pQE-Vp1- $Delta$ C17was constructed by subcloning the 1,040-bp XbaI-to-BamHI fragmentsof pSV-Vp1 (13) into pQE-XbaMCS. To express the first 303 Vp1residues (Vp1 $Delta$ C58) of which cysteines 104 and 254 are changedinto alanines (to minimize possible oxidative cross-linking ofVp1 during protein isolation), pQE-Vp1-2CA- $Delta$ C58 was constructedby inserting the 953-bp XbaI-to-BamHI fragment of pBS-Vp1-2CA- $Delta$ C58into pQE-XbaMCS. pBS-Vp1-2CA- $Delta$ C58 was made by inserting into pBS-Vp1- $Delta$ C58(19) the 495-bp XbaI-to-PstI fragment from pBS-Vp1-C104A (19)and the 458-bp PstI-to-BamHI fragment from pBS-Vp1-C254A (19).To express the N-terminal mutant counterparts of $Delta$ C17 or $Delta$ C58Vp1s, pQE-Vp1- $Delta$ C17 or pQE-Vp1-2CA- $Delta$ C58 was inserted with the 206-bpor smaller XbaI-to-AflII fragments from pSV-Vp1 -p567, -p81 (14),-p25 (14), -d20, and -d50 to yield the N-terminal mutant counterpartsNLSm1, NLSm2, NLSm1 · 2 (see Table 1), $Delta$ N(2-21), and $Delta$ N(2-51)(see Fig. 1E). pSV-Vp1 -p567, -d20, and -d50 were made from pSV-Vp1by site-directed mutagenesis using the SacI antisense primer (5'-CAAGAATTCGAGCTCGCCCAACTTG-3')and either the p567-XbaI sense primer (5'-CAGGTCCATGGTCTAGA ATGAAGATGGCCCCAACAAAcgGAAAcGGAAGTTGTCCAGGGGCAGCTCCCAA-3'), the d20-XbaI sense primer (5'-CAGGTCCATGGTCTAGAATGAAGATGGCCCAAGTGCCAAAGCTCGTCAT-3'),or the d50-XbaI sense primer (5'-CAGGTCCATGGTCTAGAATGAAGATGGCCAATCCTCAAATGGGCAATCC-3').

pSG5-Vp1 $Delta$ C58-GFP was used for the transient mammalian cell expression of fluorescently tagged Vp1 fusion proteins. The proteinsconsist of the first 303 Vp1 amino acids connected to the red-shiftedgreen fluorescsent protein (GFP) by a flexible linker, which ismade up of three repeats of (glycine)₄-serine [(G₄S)₃]. First,pSG5-XNAB was made from pSG5 (Stratagene) by knocking out theXbaI site and inserting into EcoRI and BamHI sites a linker thatintroduces unique XbaI, NotI, AgeI, and BsrGI sites. pSG5-Vp1 $Delta$ C58-GFPwas then constructed by inserting three fragments into pSG5-XNAB:the 925-bp XbaI-to-NotI Vp1 fragment from pBS-Vp1- $Delta$ C58, the 85-bpNotI-to-AgeI (G₄S)₃ fragment from pETC-64M5-NotAge, and the 722-bpAgeI-to-BsrGI GFP fragment from pEGFP-1 (Clontech). pETC-64M5-NotAgewas made from pETC-64M5LH15His (17) by inserting a NotI linkerthrough KpnI and NheI sites and inserting an AgeI linker throughEcoRI and SacIsites.

The NLSm1, NLSm2, or NLSm1 · 2 derivatives of pBS-Vp1 (19), of pSG5-Vp1 $Delta$ C58-GFP, and of the viral plasmid NO-pSV40 (13)were obtained by substituting the 206-bp XbaI-to-AflII fragmentsfrom pSV-Vp1 -p567, -p567, -p81, or -p25, respectively. NO-SV40DNAs were prepared from respective NO-pSV40 plasmids by BamHIdigestion and ligation as previously described (13). pBS-Vp1plasmids were used for the in vitro synthesis of Vp1 proteinsfrom T7 promoter-driven codingsequences.

Preparation of recombinant proteins. GST (glutathione S-transferase)-Vp1 was expressed from pGEX-Vp1, purified, and cleaved with factor X_a as described previously(7).

For H6-tagged Vp1s, XL1-Blue Escherichia coli cells harboring individual pQE-Vp1 plasmids were induced at the early log phasewith 0.2 to 0.5 mM IPTG for 6 h at 30°C or for 24 h at 20°C. H6proteins were purified using the Talon metal affinity resin (Clontech)according to the supplier's protocols as follows. Vp1 $Delta$ C17 andN-terminal-mutant $Delta$ C17 proteins were purified according to thedenaturing-buffer protocol, and the eluted protein in 20 mM Tris-Cl(pH 8.0)-100 mM NaCl-8 M urea-100 mM imidazole was dialyzed againstchanges of 20 mM Tris-Cl (pH 8.0)-10 mM NaCl-0.1 mM $beta$ -mercaptoethanolin which the concentration of urea was decreased from 8 M to none.The dialysate was removed of insoluble materials by a 15-min centrifugationat 15,000 × g and concentrated using a Microcon-30 concentrator(Amicon). Except for $Delta$ N(2-51)- $Delta$ C58, which failed to express touseful quantities in bacteria, Vp1 $Delta$ C58 and N-terminal-mutant $Delta$ C58proteins were prepared as follows. Each protein was purified fromlysozyme- and DNase I-treated, sonicated bacterial lysate accordingto the native-buffer protocol, and the pentamer fraction was isolatedby sedimenting 150 to 300 µg of the eluted protein, in 20 mM Tris-Cl(pH 8.0)-100 mM NaCl-100 mM imidazole, through a 10.5-ml, 5 to20% continuous sucrose gradient in the same buffer without imidazolefor 23 h at 35,000 rpm at 4°C in an SW41 rotor. Fifteen fractionswere collected from the bottom of the gradient, and two to threepeak pentamer fractions (see Fig. 1C), containing 50 to 75% ofthe total input protein, were pooled foruse.

All protein preparations were quantitated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and Coomassieblue staining and were stored in aliquots at 0.1 to 1 mg/ml at $-$ 70°C.

DNA-binding assays. Southwestern blots were performed as previously described (without dithiothreitol in the blotting buffer) (4) using nick-translated,³²P-labeled SV40 DNA (4) and 0.4 to 2.0 µg of cleaved GST-Vp1or $Delta$ C17 Vp1s. Filter-binding assays (4) were performed usingnick-translated, ³²P-labeled SV40 or pBR322 DNA for cleaved GST-Vp1 and $Delta$ C17 Vp1s,or using a 326-bp, ³²P-labeled PCR fragment of SV40 DNA (see below) for $Delta$ C58 pentamers.Each binding experiment used at least seven protein concentrations,and an apparent K_d was determined from the binding curve as theprotein monomer or pentamer concentration at which 50% of theDNA probe was retained on the filter. An average K_d value fromthree experiments was tabulated along with the standarddeviation.

The 326-bp labeled fragment, corresponding to SV40 nucleotides 1670 to 1996, was amplified by PCR in a 20-µl reaction containing1 ng of NO-pSV40 as template; 10 pmol each of sense and antisenseprimers; SV40 nucleotides 1670 to 1689 and 1996 to 1976; 120 µCiof [ $alpha$ -³²P]dATP (ICN; specific activity, 3,000 Ci/mmol); 150 nM each ofdCTP, dGTP, and dTTP; 37 nM cold dATP; and 5 U of Taq DNA polymerase(Gibco-BRL) in 1× Mg²⁺-free PCR buffer (Gibco-BRL) supplemented with 2 mM MgCl₂. Thereaction was brought to 94°C for 1 min and cycled 35 times through94°C for 45 s, 60°C for 45 s, and 72°C for 2 min, and the approximately1 µg of PCR product was purified using the Qiaquick PCR PurificationKit(Qiagen).

Immunofluorescence and plaque assays. TC7 cells were nuclearly microinjected with NO-SV40 DNAs and analyzed for the localization of virally encoded Vp1 and Vp2/3by indirect immunofluorescence microscopy (3, 7) or analyzedfor plaque formation (29) with the modification that a totalof five agar overlays were performed, and cells were visualizedon day 25. Plaque assays were also performed by transfecting CV-1cells with NO-SV40 DNAs and infecting the harvested cell lysatesonto new cells as described previously (19). To examine thelocalization of wild-type or mutant Vp1s expressed alone, cellswere transfected as before (19) with pSG5-Vp1 $Delta$ C58-GFP DNAs,fixed at 24 h posttransfection with 3.7% formaldehyde in phosphate-bufferedsaline, and processed for anti-Vp1 immunofluorescence as before(3, 7). The autofluorescence of GFP was alsorecorded.

Analyses for viral DNA replication, capsid protein production, and viral DNA packaging. To examine viral DNA replication, CV-1 cells on 60-mm dishes were transfected with NO-SV40 DNAs as described above and harvestedat various hours posttransfection for the extraction of totalviral DNAs by the Hirt method (12). One-tenth of each DNA preparationwas analyzed by Southern slot blot using radiolabeled SV40 DNAas a probe. Individual slots were excised from the membrane andquantitated for radioactivity in a liquid scintilationcounter.

To examine the steady-state levels of virally encoded capsid proteins, CV-1 cells on a 60-mm dish were transfected with a4:1 molar mixture of each NO-SV40 DNA and pmiwZ (28), whichexpresses $beta$ -galactosidase under the control of a complex of Roussarcoma virus and $beta$ -actin promoter-enhancers. The cells were harvestedat 72 h posttransfection, and aliquots of cells containing equal $beta$ -galactosidase activities as determined from the $beta$ -GalactosidaseAssay Kit (Stratagene) were analyzed by anti-Vp1 and anti-Vp3Western blots using polyclonal rabbit anti-Vp1 and anti-Vp3 sera(16) and the Enhanced Chemiluminescence Western Blotting System(Amersham-Pharmacia).

To examine viral DNA packaging, NO-SV40 DNAs-transfected CV-1 cells were harvested at 72 h posttransfection and analyzed asdescribed previously (19). Briefly, cells from each 150-mm dishwere lysed by sonication in 0.5 ml of hypotonic buffer, and thetotal viral DNA and DNase I-resistant viral DNA were extractedfrom aliquots of the cell lysate. After the extracted viral DNAswere linearized with KpnI, and the proportion of DNase I-resistantto total viral DNA was determined by Southern blot and phosphorimaging.A value of 65 to 80% was obtained for wild-type NO-SV40 transfectedlysate. To examine the presence of virions or virion-like particles,DNase I-treated lysates were sedimented through 5 to 32% sucrosegradient, and the resulting fractions were analyzed for totalviral DNA by Southern blot as before (19), as well as analyzedfor Vp1 by Western blot using polyclonal rabbit anti-Vp1 serumand ¹²⁵I-labeled protein A detection as described elsewhere (21). Notethat the amount of DNase I used in the above assays was severaltimes higher than was needed to completely degrade free viralDNA and yet did not noticeably affect the integrity of wild-typevirion particles (19).

Vp3 interaction assay. The GST-Vp3 fusion protein and its preparation from the soluble fraction of the bacterial lysate by binding to glutathioneaffinity resin have been described (4). ³⁵S-labeled Vp1 proteins were synthesized by in vitro transcriptionand translation of pBS-Vp1 plasmids as described previously (19).For the interaction assay, 5 µl of a slurry of glutathione resinbound with 10 pmol of GST-Vp3 was extensively washed and thenreacted for 30 min at room temperature with 50 fmol of ³⁵S-labeled wild-type or NLS-mutant Vp1 in 400 µl of a buffer (20mM HEPES [pH 7.5], 150 mM NaCl, 1 mM EDTA, 0.5% Triton X-100,0.1% sodium deoxycholate, 0.1% SDS, 1 mM phenylmethylsulfonylfluoride, and 10 µg of aprotinin, 10 µg of leupeptin, 10 µg ofpepstatin, and 50 ng of ethidium bromide per ml). The resin wascollected and extensively washed with the same buffer withoutethidium bromide, and the bound proteins were analyzed by SDS-PAGEand fluorography using the Amplify reagent (Amersham-Pharmacia).In control assays, the same amount of resin-bound GST, expressedfrom pGEX-3X (Amersham-Pharmacia)-transformed bacteria, was usedinstead of resin-bound GST-Vp3.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

DNA binding by recombinant SV40 Vp1 proteins. We used two types of in vitro assays to examine the DNA-binding abilities of E. coli-expressed recombinant Vp1s. In the Southwesternassay, proteins resolved by SDS-PAGE were transferred to nitrocelluloseand renatured on the membrane before probing with labeled DNA.GST-Vp1 was inactive in DNA binding (Fig. 1A, GST-Vp1 band inlanes 1 and 3) unless the Vp1 moiety (Fig. 1A, Vp1* band in lanes1 and 3) was freed by proteolytic cleavage at its amino-terminaljunction with GST. Vp1 $Delta$ C17, with a natural N terminus and a C-terminalpolyhistidine tag, was active in Southwestern assay (lanes 2 and4). To estimate the DNA binding affinities of GST-Vp1-derivedVp1 and Vp1 $Delta$ C17, a solution-phase filter-binding assay was used.Both proteins had dissociation constants (K_ds) in the range of5.3 × 10⁹ to 7.3 × 10⁹ M for interacting with either SV40 or pBR322 DNA (Fig. 1E). Therecombinant Vp1's apparent lack of DNA-sequence specificity (Fig.1E) is in agreement with a previous report (26).

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FIG. 1. DNA binding by recombinant Vp1 proteins. (A and B) Southwestern blots. Protein samples were resolved on SDS-10% polyacrylamide gels and either stained with Coomassie blue (A, lanes 1 and 2; B, lanes 1 to 5) or electrotransferred to nitrocellulose and probed with nick-translated ³²P-labeled SV40 DNA (10 to 12 ng/ml) (A, lanes 3 and 4; B, lanes 6 to 10). In panel A, 0.5 µg of Vp1 (Vp1*, lanes 1 and 3) as a cleavage product of GST-Vp1, or 0.5 µg of Vp1 $Delta$ C17 (lanes 2 and 4), were used. Intact GST-Vp1 (GST-Vp1) and the GST moiety (GST*) were also present in the samples of lanes 1 and 3. In panel B, 2 µg of Vp1 $Delta$ C17 (lanes 1 and 6) or of the following N-terminal mutant $Delta$ C17 proteins were used: NLSm2 (lanes 2 and 7), NLSm1 · 2 (lanes 3 and 8), $Delta$ N(2-21) (lanes 4 and 9), and $Delta$ N(2-51) (lanes 5 and 10). Four bars to the left of each Coomassie gel mark the positions (from top to bottom) for molecular mass standards of 110, 74, 45, and 26 kilodaltons. (C) Isolation of pentameric Vp1 $Delta$ C58 and $Delta$ N(2-21)- $Delta$ C58. Sedimentation through sucrose gradients was performed as described in Materials and Methods, and an aliquot from each of the 15 fractions was analyzed by SDS-PAGE and Coomassie blue staining. In the profiles shown, twice as much protein was sedimented for $Delta$ N(2-21)- $Delta$ C58 (lower panel) than for Vp1 $Delta$ C58 (upper panel). Six bars to the left of each gel mark the positions for six molecular mass standards of 100, 71, 44, 28, 19, and 14 kilodaltons. Pentamers were found in fractions 8 and 9 for Vp1 $Delta$ C58 and in fractions 8 through 10 for $Delta$ N(2-21)- $Delta$ C58. NLSm1 $Delta$ C58, NLSm2 $Delta$ C58, and NLSm1 · 2 $Delta$ C58 gave sedimentation profiles similar to that of Vp1 $Delta$ C58. (D) Solution-phase DNA binding. Filter-binding assays were performed by incubating various concentrations of each protein with ³²P-labeled DNA, and the percentages of the input radiolabel that was retained on nitrocellulose membrane upon filtration were determined. Average values from three experiments are shown with error bars for the binding of a 326-bp PCR-derived SV40 fragment by pentameric Vp1 $Delta$ C58 or its N-terminal mutant derivatives. Values from one experiment are shown for the binding of nick-translated SV40 DNA by $Delta$ N(2-51)- $Delta$ C17 whose monomeric concentrations are given in parentheses. Dissociation constants (K_ds) were determined as molar protein concentrations at 50% DNA retention. (E) Summary of DNA-binding activities for recombinant Vp1s. For GST-Vp1-derived Vp1 and for Vp1 $Delta$ C17, the apparent K_d was given in protein monomer concentration for the binding of nick-translated SV40 (SV) or pBR322 (pBR) DNA. For $Delta$ C58 proteins, an average K_d along with the standard deviation was given in the protein pentamer concentration for the binding of a 326-bp SV40 fragment. The relative activity is the reciprocal of K_d made relative to that of the Vp1 $Delta$ C58 K_d, which was taken to be 100%. An "X" on the schematic protein diagram represents the mutation of an N-terminal basic cluster; a dot beneath residues 104 and 254 indicates their mutation from cysteines into alanines, n.d., not done.

Since Vp1 $Delta$ C17 was found mostly in inclusion bodies in bacteria, its purification required urea denaturation and subsequentrenaturation steps. We sought to improve recombinant Vp1 designand preparation in the following ways. First, recombinant SV40Vp1s can be expected to exist as pentamers or their complexes,similar to bacterially purified polyomavirus Vp1 (24). Deletingup to about 58 amino acids from the C terminus should eliminatethe assembly of SV40 Vp1 pentamers into higher complexes withoutaffecting pentamerization. Second, urea-denatured proteins maynot regain proper folding and tend to aggregate upon the denaturant'sremoval. It would be preferable to use native buffer conditionsthroughout purification. Third, Vp1 pentamers may also aggregatethrough disulfide linkages, such as those between cysteines 104observed in virion crystal structure (27) or perhaps artifactualones involving cysteine 254. Eliminating these cysteines shouldminimize such cross-links. Hence, we expressed the C-terminal-58truncated Vp1 $Delta$ C58 in which cysteines 104 and 254 are replacedby alanines, purified it under native buffer conditions, and isolatedthe pentamer fraction in a sucrose gradient (Fig. 1C). To derivea K_d that is more likely to reflect the one-to-one stoichiometricinteraction between the pentamer and DNA, the filter-binding assaywas performed using 326-bp, PCR-generated SV40 DNA probe ratherthan nick-translated DNA, which may consist of fragments thatare longer or heterogeneous in length. Under these conditionsthe K_d measured for Vp1 $Delta$ C58 was 1.8 (±0.2) × 10⁹ M in terms of the protein pentamer (Fig. 1D and E). Thus, theDNA-binding ability of Vp1 as a homogeneous, C-terminal-58 truncatedpentamer was comparable to those of full-length Vp1 and Vp1 $Delta$ C17.These results indicated that the Vp1 C terminus does not mediateDNA binding and led us to investigate whether the Vp1 DBD liesin the Nterminus.

The Vp1 DBD overlaps with the bipartite Vp1 NLS. The N terminus of Vp1 is likely to harbor a DBD because of its proximity to the core of the virion (20) and by analogy tothe mapped polyomavirus Vp1 DBD (22). It is also the locationfor the previously identified bipartite NLS (14), which consistsof two clusters of basic residues. We will refer to the firstcluster, 4-lysine-arginine-lysine-6, as NLS1 and to the secondcluster, 15-lysine-lysine-proline-lysine-18, as NLS2 (Table 1).To test whether these basic clusters also mediate Vp1 DNA binding,sets of multiple-point mutations (NLSm1, NLSm2, and NLSm1 · 2)and N-terminal truncations [ $Delta$ N(2-21) and $Delta$ N(2-51)] were introducedinto Vp1 $Delta$ C17 and Vp1 $Delta$ C58, and DNA-binding assays were performed.In NLSm1, NLS1 is mutated into asparagine-glycine-asparagine;in NLSm2, NLS2 is changed to asparagine-asparagine-proline-asparagine;and in NLSm1 · 2, both clusters are correspondingly changed (Table1). In $Delta$ N(2-21) or $Delta$ N(2-51), residues 2 to 21 or residues 2 to51, respectively, were deleted. Among the mutant $Delta$ C17 proteins,NLSm2 had partial activity in the Southwestern blot, while NLSm1· 2 and both N-terminal deleion mutants were inactive (Fig. 1B),suggesting that the basic clusters were necessary for the DNAbinding. For the N-terminal mutant $Delta$ C58 proteins, the K_ds weredetermined with purified pentamers as before. The multiple-pointmutant $Delta$ C58 proteins sedimented in the sucrose gradients witha similar profile as Vp1 $Delta$ C58 (data not shown), while the N(2-21)- $Delta$ C58pentamer sedimented somewhat slower than Vp1 $Delta$ C58, an expectedresult for the additional deletion (Fig. 1C). We found that mutantsNLSm1, NLSm2, $Delta$ N(2-21), and NLSm1 · 2 bound DNA with progressivelydecreased affinities; their K_ds in terms of the protein pentamer,4.4 (±0.6) × 10⁹, 1.3 (±0.2) × 10⁸, 4.8 (±0.9) × 10⁸, and 2.6 (±0.4) × 10⁷, respectively, correspond to 41, 14, 4, and 0.7% of the Vp1 $Delta$ C58activity, respectively (Fig. 1D and E). A K_d was not determinedfor $Delta$ N(2-51)-C58 because of difficulty with its bacterial expression,but its $Delta$ C17 counterpart, $Delta$ N(2-51)- $Delta$ C17, was found not to havesufficient DNA-binding affinity for K_d measurement (Fig. 1D andE). These results indicate that NLS1 and NLS2 $---$ that is, NLS1-DBD1and NLS2-DBD2 $---$ represent essential parts of the Vp1 DBD, with thelatter part contributing more to DNA binding than the former part.The N-terminal 22-to-51 region also appears to harbor a smallfraction of total binding activity.

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TABLE 1. Multiple-point mutants of the Vp1 N terminus

The NLS function of the N-terminal basic clusters was confirmed in cells transfected with pSG5-Vp1 $Delta$ C58-GFP, for which thefusion protein of Vp1 N-terminal 303 residues and GFP was expressedfrom the SV40 early promoter in the absence of Vp2/3 and the tumorantigens. Both the Vp1 immunofluorescence (Fig. 2) and the GFPautofluorescence (data not shown) indicated that, while wild-typeVp1 $Delta$ C58-GFP localized effectively to the nucleus (Fig. 2a), themutant counterpart NLSm1, NLSm2, and NLSm1 · 2 proteins largelyaccumulated in the cytoplasm (Fig. 2b, c, and d). A mostly cytoplasmiclocalization pattern was also observed for full-length mutantVp1s expressed from pSV-Vp1-p81 (NLSm2) and -p25 (NLSm1 · 2),in which the tumor antigen coding sequences are present, and frompSG5-Vp1-p25 (14). Therefore, the two basic clusters withinN-terminal 21 serve as the NLS of Vp1. The collective resultsindicate that the DBD of Vp1 overlaps with the NLS, sharing therequirement for at least the two basic amino acid clusters.

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FIG. 2. Subcellular localization of NLS-mutant Vp1 $Delta$ C58-GFP proteins. Cells transfected with wild-type (a), NLSm1 (b), NLSm2 (c), and NLSm1.2 mutant pSG5-Vp1 $Delta$ C58-GFP were fixed and stained with guinea pig anti-Vp1, followed by rhodamine-labeled anti-guinea pig antibody. Photographs of the rhodamine fluorescence are shown. The GFP autofluorescence in each case gave an essentially identical pattern, although the intensity was less than the corresponding Vp1 immunofluorescence.

Importance of Vp1 NLS-DBD for viability. To test the role of the overlapping Vp1 DBD and NLS in the viral life cycle, we examined the viability of nonoverlapping SV40(NO-SV40) genomes into which NLSm1, NLSm2, and NLSm1 · 2 mutationshad been introduced. NO-SV40 is a viable SV40 DNA containing allof the regulatory sequences, the early genes, and spatially separatedVp2/3 and Vp1 coding sequences (13). Two types of viabilityassays were performed, one by microinjection of the viral DNAand the other by infection of the viral DNA-transfected cell lysate.Mutants NLSm1 and NLSm1 · 2 failed to produce plaques in the microinjectionassay, and the infection assay confirmed NLSm1 to be incapableof producing infectious particles (Table 2). Compared with wild-typeNO-SV40, mutant NLSm2 formed smaller plaques in the microinjectionassay and formed plaques that were 5,000 times fewer, as wellas smaller, in the infection assay (Table 2).

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TABLE 2. Plaque-forming abilities of NO-SV40 Vp1 NLS-DBD mutants

To determine which stages of the viral life cycle were affected by the Vp1 NLS mutations, we examined the state of variousviral processes, beginning with viral DNA replication and capsidprotein production. The amount of intracellular viral DNA, quantitatedby Southern slot blot, increased steadily with increasing timesposttransfection for the wild type and the three Vp1 NLS-mutantDNAs (Fig. 3A). Comparable amounts of Vp1, Vp2, or Vp3 were detectedby Western blot in cell lysates from transfection with eitherwild-type or the three mutant viral DNAs (Fig. 3B). Thus, defectsother than those in viral DNA replication or capsid protein productionwere responsible for the abolished or greatly reduced viabilitiesof the Vp1 NLS-DBD mutants.

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FIG. 3. DNA replication and capsid protein production by N-terminal Vp1 mutants. (A) Time course of viral DNA replication. Cells transfected with each NO-SV40 DNA were harvested at the indicated time points, and the total intracellular viral DNA was extracted and probed with nick-translated SV40 DNA in a Southern slot blot. The radioactivities of the individual slots were counted and plotted against time. (B) Levels of capsid proteins. Cells transfected with individual NO-SV40 DNAs were analyzed by immunoblotting with anti-Vp1 (upper panel) or anti-Vp3 (lower panel) antibodies. The amount of cells analyzed was adjusted for transfection efficiency as measured by the activity of $beta$ -galactosidase expressed from pmiwZ, which was cotransfected with each NO-SV40 DNA. Bands corresponding to Vp1, Vp2, and Vp3 are indicated at the right.

Nuclear localization defect of mutant Vp1s expressed by NO-SV40-NLSm1 and-NLSm1 · 2. We next examined the NO-SV40 mutants for the subcellular distribution of the capsid proteins. Since mutations in either orboth of NLS1 and NLS2 impaired the nuclear localization of a Vp1fusion protein (Fig. 2), at least two different scenarios arepossible when the mutant Vp1s were present along with Vp2/3 incells introduced with the mutant viral DNAs. One is that the intactNLSs of wild-type Vp2/3 can complement the defective NLS of Vp1,as observed for NO-SV40-Vp1 $Delta$ N5 (13), and the mutant Vp1 is piggybackedto the nucleus by Vp2/3. This phenotype was seen for mutant NLSm2.Both the mutant Vp1 and the Vp2/3 were nuclearly localized (Fig.4e and f), as were the capsid proteins expressed by wild-typeNO-SV40 (Fig. 4a and b). The second scenario is that NLS complementationfails to occur, for example, because cytoplasmic Vp1-Vp2/3 interactionis somehow blocked; as a result, Vp2/3, but not the mutant Vp1,enters the nucleus. This phenotype was observed for mutants NLSm1and NLSm1 · 2, whose mutant Vp1s remained in the cytoplasm despitethe nuclear localization of Vp2/3 (Fig. 4c, d, g, and h). Thus,the major defect of nonviable mutants NLSm1 and NLSm1 · 2 appearsto lie in the inability of the mutant Vp1s produced to localizeto the nucleus. This defect could arise from the mutant Vp1s'lack of intrinsic Vp2/3-interactive ability or from the mutantVp1s' inability to reach a cytoplasmic site necessary for theVp1-Vp2/3 interaction. The former possibility is examined below.

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FIG. 4. Subcellular localization of capsid proteins expressed from Vp1 N-terminal-mutant NO-SV40 DNAs. Cells were nuclearly microinjected with individual NO-SV40 DNAs, cultured for 24 h, fixed, and doubly stained with guinea pig anti-Vp1 (a, c, e, and g) and rabbit anti-Vp3 (b, d, f, and h), followed by rhodamine-labeled (a, c, e, and g) or fluorescein-labeled (b, d, f, and h) secondary antibodies. The same cells are shown in panels a and b, c and d, e and f, and g and h.

In vitro interaction of mutant Vp1s with Vp3. To determine if the N-terminal mutant Vp1 proteins had the intrinsic ability to associate with Vp3, an in vitro interactionassay was performed. In vitro-transcribed and-translated, ³⁵S-labeled NLSm1, NLSm2, and NLSm1 · 2 mutant Vp1s bound resin-immobilizedGST-Vp3, as did wild-type Vp1, whereas little of the Vp1s boundto GST alone (Fig. 5). Thus, the intrinsic interaction betweenVp1 and Vp2/3 was not affected by the Vp1 N-terminal mutations.

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FIG. 5. Interaction of N-terminal-mutant Vp1s with Vp3. In vitro-transcribed and -translated, ³⁵S-labeled Vp1 from each pBS-Vp1 DNA was mixed with the resin to which either GST-Vp3 (first panel) or GST (second panel) had been immobilized. The resin-bound proteins were analyzed by SDS-PAGE and fluorography. The amounts of input ³⁵S-labeled Vp1s used for the pull-down experiments are also shown (third panel).

Nuclear virion assembly defect of NO-SV40-NLSm2. Since all capsid proteins of mutant NLSm2 were produced in normal quantities and could localize to the nucleus, and the mutantDNA replicated normally, we tested whether the mutant could formvirion-like particles. When viral DNA-transfected cell lysateswere treated with DNase I, only 6.9% of the total mutant DNA remained,compared with 71% of the total wild-type DNA. Thus, mutant NLSm2either packaged only 1/10 the amount of viral DNA as wild-typeNO-SV40 or packaged the viral DNA mostly in a manner that leftthe DNA susceptible to DNase Idigestion.

To determine if the protected mutant DNA was packaged in a particle form, the DNase I-resistant materials from wild-type andNLSm2 DNA-transfected lysates were examined by sedimentation throughsucrose gradients. To adjust for the 10-fold-reduced amount ofthe nuclease-resistant mutant viral DNA, 10 times as much nuclease-treatedNLSm2 sample as the corresponding wild-type sample was sedimented,and equal aliquots of wild-type and NLSm2 sucrose fractions wereanalyzed for viral DNA by Southern blot (Fig. 6). Since Vp1, whetherwild type or mutant, would quantitatively remain after the nucleasetreatment, it would be much more abundant in the 10-times-largerNLSm2 sample than in the wild-type sample. Accordingly, one-fifthas much of the NLSm2 fractions than the wild-type fractions wasanalyzed by anti-Vp1 Western blot (Fig. 6). The distribution profilesshowed that wild-type viral DNA and Vp1 were present mostly infractions 1 through 9 as well as 17 (Fig. 6A and C). About 42%of the wild-type DNA resided in fractions 3 through 5, which correspondedto the sedimentation location of purified virions (Fig. 6C). Thedistributions of NLSm2 DNA and the mutant Vp1 were somewhat broaderthan their wild-type counterparts, with comparatively more ofboth mutant DNA and Vp1 present in fractions 7 through 9 (Fig.6B and C). Nonetheless, about 30% of the mutant viral DNA waspresent in the expected particle fractions 3 through 5 (Fig. 6C).These results indicated that mutant NLSm2 could form virion-likeparticles, though at a reduced level. Taken together, these resultspoint to a reduced level of viral DNA packaging by mutant NLSm2and hence a role for NLS2-DBD2 in the virion assembly process.

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FIG. 6. Virion particle formation by NO-SV40-NLSm2. (A and B) Sonicated lysate prepared from wild-type (Wt, A) or mutant NLSm2 (NLSm2, B) NO-SV40 DNA transfected cells was treated with DNase I, and aliquots containing equivalent amounts of DNase I-resistant viral DNAs (60 µl for wild-type raised to 600 µl with buffer and 600 µl for NLSm2) were sedimented through 5 to 32% sucrose gradients and fractionated from the bottom into 17 fractions. Five-sixths of each fraction was analyzed for viral DNA by Southern blot (upper panels). One-sixth of each wild-type fraction or one-thirtieth of each NLSm2 fraction was also analyzed for Vp1 by Western blot (lower panels). An arrowhead points to fraction 4, the peak fraction for viral DNA and Vp1 from purified virions sedimented in a parallel gradient. (C) Distribution of post-DNase I viral DNA and Vp1 in sucrose fractions. Wild-type (upper plot) and NLSm2 (lower plot). For each Southern or Western profile, the radioactivity per lane of the DNase I-resistant viral DNA or Vp1, obtained by phosphorimager quantitation of the observed band(s), was made relative to the total radioactivity of the DNA or Vp1 for all 17 fractions, which was taken to be 100%. The percentages were plotted against the fraction number.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study, we mapped within the N-terminal 21 amino acids of SV40 Vp1, a DBD that accounted for most (96 to 99%) of thein vitro-measured Vp1 DNA-binding activity. This DBD overlapsthe two basic clusters, NLS1-DBD1 and NLS2-DBD2, of the bipartiteVp1 NLS (14). Both basic clusters are required for full DNA-bindingactivity, though the second cluster (15-lysine-lysine-proline-lysine-18)is more important for the binding than the first cluster (4-lysine-arginine-lysine-6).The biological functions of the overlapping DBD and NLS were thendissected in vivo using mutant NO-SV40 viral genomes with theapplication of the NLS phenotypic complementation we have previouslyestablished (13). Nonviable multiple-point mutants NLSm1 andNLSm1 · 2 were exceptional in that their mutant Vp1s were unableto enter the nucleus despite the presence of Vp2/3, though themutant Vp1s' ability to interact with Vp3 in vitro was not affected.For a multiple-point mutant of NLS2-DBD2, NLSm2, a greatly decreasedviability was correlated with a decreased level of virion packagingbut not with any defects in viral DNA replication or capsid proteinproduction, interaction, or nuclear localization. Our resultsdemonstrated, for the first time, that NLS2-DBD2 is importantfor the formation of infectious particles and that the Vp1 DNA-bindingfunction is likely to have an essential role in this process.The N-terminal location of the DBD is consistent with the crystallographicstructure of the virion in which the Vp1 N terminus is orientedtoward the minichromosomal core and is disordered (20).

To obtain a K_d for homogeneous Vp1 pentamers and to favor a one-to-one molar pentamer-DNA interaction, we used the purifiedVp1 $Delta$ C58 pentamer, mutated in cysteines 104 and 254 to minimizeartifactual pentamer-pentamer aggregation, and a short (326-bp)DNA probe. A K_d of 1.8 × 10⁹ M in terms of the protein pentamer was obtained. Two other recombinantVp1s, cleaved GST-Vp1 and Vp1 $Delta$ C17, had apparent K_ds 5.3 × 10⁹ to 7.3 × 10⁹ M in terms of the protein monomers, which are roughly comparableto the Vp1 $Delta$ C58 pentamer value and reinforce the reliability ofour assays. Whereas the DBD of SV40 Vp1 comprises NLS1 and NLS2,that of the related polyomavirus Vp1 consists of a single basiccluster, 1-alanine-proline-lysine-arginine-lysine-5 (2, 22),with a sequence resemblance to that of NLS1-DBD1. For SV40, itis NLS2-DBD2 (represented by mutant NLSm2) that was attributedwith a larger share of DNA-binding activity and a role in in vivovirion packaging. Whether mutating the polyomavirus Vp1 DBD impairspolyomavirus particle packaging would make an interesting comparison.The reported apparent K_d for DNA binding by polyomavirus Vp1 is1-2 × 10¹¹ M in term of the protein monomer (22). The difference betweenthis value and the values for SV40 Vp1 may reflect either a comparativelyhigher DNA-binding affinity of polyomavirus Vp1 or differencesin the assay methodsemployed.

The DBD and the bipartite NLS of SV40 Vp1 overlap within the N-terminal 21 residues. A number of other proteins, includingpolyomavirus Vp1, influenza virus matrix protein M1, and proteinswith bHLH/bZIP, zinc finger, and homeobox domains, are also knownto harbor a DNA- or RNA-binding domain in overlap with an NLS(18). This overlapping or bifunctional domain arrangement isnot surprising, since clustered basic residues typify many knownNLSs and nucleic acid-binding domains (8, 18). Nevertheless,we were able to distinguish the two functions in our analysis(see below). Our data, however, do not rule out a possibilitythat Vp1 amino acids other than the first 21 residues also makean additional contribution to DNA binding. Such residues wouldconceivably be at the base of the Vp1 pentamer. This questionis not addressed in thisstudy.

The functional duality of the Vp1 N-terminal domain can potentially complicate the determination of how an individual domainfunction contributes to viral viability. Yet by applying NLS phenotypiccomplementation, we found that the phenotype of viral mutant NLSm2was consistent with a role for the Vp1 DBD in nuclear virion assembly.This mutant was viable but had a 5,000-fold-lowered infectioustiter and notably smaller plaque sizes. The pattern of capsidprotein nuclear localization is consistent with the reported functionalcomplementation of NLSs, in which an NLS-defective Vp1 (e.g.,Vp1 $Delta$ N5) accumulated in the nucleus in the presence of wild-typeVp2/3 as a result of the capsid proteins' association in the cytoplasmprior to nuclear entry (13). Given this effective complementationof NLSm2 Vp1 nuclear localization, the normal levels of viralDNA replication and capsid protein production, and the normalability of the mutant Vp1 to interact with Vp3 in vitro, the mutant'sreduced viability is likely the result of the mutant Vp1's impairedDNA-binding ability. There are at least two major ways a compromisedVp1 DNA-binding function can lead to a lower viral infectivity.First, impaired Vp1 DNA binding could affect the efficiency ofDNA packaging in the nucleus and reduce number of particles produced.Second, the mutant virion-like particles assembled may be lessstable or less effective at cell entry or nuclear targeting stepsin a new round of infection. Our NLSm2 results reflect defectspossibly at both stages of the viral life cycle. The observed10-fold reduction in the packaging of the viral DNA (Fig. 6) wouldcertainly lower the yield of potentially infectious particles.In view of the 5,000-fold-lowered overall viability, it is alsolikely that the particles that did form were less infectious thanwild-type particles in the next infection cycle. Further experimentswould be needed to address the defect of mutant NLSm2 particlesduringreinfection.

Distinctly different from the apparent defect of mutant NLSm2 is the intriguing phenotype of mutants NLSm1 and NLSm1 · 2,which harbor mutations in the first basic cluster, NLS1. In contrastto NO-SV40-NLSm2 (above) and -Vp1 $Delta$ N5 (13), these two nonviablemutants produced cytoplasmically localized mutant Vp1s despitethe nuclear localization of Vp2/3, indicating that the defectiveNLSs of the mutant Vp1s were not complemented by the presenceof wild-type Vp2/3 NLS. This phenotype also indicates that Vp2/3could enter the nucleus independently of the mutant Vp1s. Twolines of evidence support the hypothesis that the mutated NLS1acts as a dominant signal for the cytoplasmic retention of NLSm1and NLSm1 · 2 Vp1s. First, since all mutant Vp1 proteins weremade in the mutant DNAs-transfected cells (Fig. 3B) and couldinteract with Vp3 in vitro (Fig. 5), the lack of complementationsuggests that mutant Vp1s were prevented from interacting withVp2/3 in vivo. Second, deleting NLS1 as in the case of NO-SV40-Vp1 $Delta$ N5actually restored NLS complementation (13). Thus, the evidencepoints to the presence of an unidentified function, aside fromthose of nuclear localization and DNA binding, in NLS1-DBD1. Thatis, NLS1 may define a process in the cytoplasmic Vp1 biosyntheticpathway that precedes the association and the nuclear import ofVp1 and Vp2/3. We observed that Vp1 bearing single arginine 5-to-glycinepoint mutation (also part of the NLSm1 mutations) exhibited acytoskeleton-like localization pattern when expressed from a pSG5-basedplasmid (N. Ishii and N. Minami, unpublished results) but showeda diffuse cytoplasmic staining when expressed from pSV-Vp1-p1(14), from which the tumor antigens were also expressed. Thesuggestive role of cytoskeletal elements in Vp1's nuclear transportand association with Vp2/3 remains to bedetermined.

In summary, our study has mapped a DBD on SV40 Vp1 and has found that the DNA-binding contribution from NLS2-DBD2 plays arole during virion assembly. This Vp1 region may also functionduring next-cycle infection. DBDs have now been defined for allthree SV40 capsid proteins. These domains are expected to functionin conjunction with other known and as-yet-unknown interactivedomains during the packaging of viralDNA.

	ACKNOWLEDGMENTS

P.P.L. and A.N. contributed equally to thiswork.

We thank Hiroshi Morioka of Hokkaido University, Sapporo, Japan, for supplying the pETC-64M5LH15His plasmid DNA. We also thankMary A. Tran for assistance in constructing pQE-Vp1-2CA- $Delta$ C58.

This work was supported by Public Health Service grant CA50574 from the National Institutes of Health (NIH) and by a grantfrom the UCLA Academic Senate. P.P.L. was supported by a predoctoralfellowship from USPHS National Research Service Award GM07185.A.M.S. and C.F.F. were supported in part by undergraduate fellowshipsfrom, respectively, NIH Minority Scientist Development programGM55052, and NIH Minority Access to Research Careers programGM08563.

	FOOTNOTES

^* Corresponding author. Mailing address: Molecular Biology Institute, 456 Boyer Hall, University of California at Los Angeles,611 E. Charles E. Young Dr., Box 951570, Los Angeles, CA 90095-1570.Phone: (310) 825-3048. Fax: (310) 206-7286. E-mail: harumi_K{at}mbi.ucla.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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Nakanishi, A., Shum, D., Morioka, H., Otsuka, E., Kasamatsu, H. (2002). Interaction of the Vp3 Nuclear Localization Signal with the Importin {alpha}2/{beta} Heterodimer Directs Nuclear Entry of Infecting Simian Virus 40. J. Virol. 76: 9368-9377 [Abstract] [Full Text]
Gordon-Shaag, A., Ben-Nun-Shaul, O., Roitman, V., Yosef, Y., Oppenheim, A. (2002). Cellular Transcription Factor Sp1 Recruits Simian Virus 40 Capsid Proteins to the Viral Packaging Signal, ses. J. Virol. 76: 5915-5924 [Abstract] [Full Text]

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