High-Frequency Genetic Recombination and Reactivation of Orthopoxviruses from DNA Fragments Transfected into Leporipoxvirus-Infected Cells

Poxvirus DNA is not infectious because establishing an infectionrequires the activities of enzymes packaged in the virion. Thisbarrier can be overcome by transfecting virus DNA into cellspreviously infected with another poxvirus, since the residentvirus can provide the trans-acting systems needed to reactivatetransfected DNA. In this study we show that cells infected witha leporipoxvirus, Shope fibroma virus (SFV), can reactivatevaccinia virus DNA. Similar heterologous packaging systems whichused fowlpox-infected cells to reactivate vaccinia virus havebeen described, but SFV-infected cells promoted a far more efficientreaction that can produce virus titers exceeding 10⁶ PFU/µgof transfected DNA. SFV-promoted reactions also exploit thehyperrecombinogenic systems previously characterized in SFV-infectedcells, and these coupled recombination and reactivation reactionscould be used to delete nonessential regions of the vacciniavirus genome and to reconstruct vaccinia virus from overlappingDNA fragments. SFV-catalyzed recombination reactions need onlytwo 18- to 20-bp homologies to target PCR amplicons to restrictionenzyme-cut vaccinia virus vectors, and this reaction featurewas used to rapidly clone and express a gene encoding fluorescentgreen protein without the need for plaque purification or selectablemarkers. The ability of SFV-infected cells to reactivate fragmentsof vaccinia virus was ultimately limited by the number of recombinationalexchanges required and one cannot reconstruct vaccinia virusfrom multiple PCR fragments spanning essential portions of thegenome. These observations suggest that recombination is anintegral part of poxvirus reactivation reactions and providea useful new technique for altering the structure of poxvirusgenomes.

INTRODUCTION

Top

Introduction

Poxviruses are very large DNA viruses that replicate in thecytoplasm of infected cells. Because of interest in the poxvirusvariola virus as the causative agent of smallpox, poxvirus researchhas a long history, dating back the beginnings of modern virology.Some of the earliest experiments described a process called"nongenetic reactivation," wherein cells infected by one poxviruscan promote the recovery of a second virus rendered noninfectiouson its own by heat, UV light, or other treatment (8, 15). Acharacteristic feature of this reaction is that the two virusesneed not be genetically identical; for example, vaccinia viruswill reactivate variola virus, and myxoma virus will reactivaterabbit fibroma virus. Although the process of nongenetic reactivationhas never been characterized in molecular detail, it is generallyassumed that the helper virus provides the enzymatic machinerynecessary to uncoat, transcribe, repair, and perhaps replicatethe inactivated virus, complementing in trans other virion componentsinactivated by heat or other treatments.

Subsequent experiments have shown that replicating poxvirusescan also reactivate poxviruses from transfected virus DNA, andseveral applications of the process which facilitate the productionof recombinant viruses have been described. Sam and Dumbelloriginally demonstrated that one orthopoxvirus could be usedto reactivate the DNA of a second virus in a "homologous" packagingreaction (15). Scheiflinger et al. subsequently showed thatcells infected with fowlpox virus could reactivate transfectedvaccinia virus DNA in a "heterologous" packaging scheme andexploited the narrow host range of fowlpox virus to simplifythe rescue and packaging of vaccinia virus recombinants preparedin vitro by DNA ligation (16). Although the method is elegantand has been used in other studies (2, 9, 10), this approachproduced recombinant chimeras at efficiencies of only 6 to 14%,and the added technical complexities associated with propagatingfowlpox virus have seemingly limited its widespread adoption.A recent publication suggests ways in which the efficiency canbe enhanced substantially through the use of a psoralen-inactivatedhelper virus (19), although this homologous packaging reactionrisks recombination between two vaccinia virus genomes, oneof which has been subjected to highly mutagenic treatment.

In most of these studies, some care seems to have been takento extract and restrict virus DNA in ways that minimize shearingof the 190-kbp vaccinia virus genome. Yet no matter how carefullythis is done, it is difficult to imagine poxvirus DNA survivingthe transfection process intact, and thus the reactivation processpresumably repairs transfected viral DNA with the recombinationsystems readily detected in poxvirus-infected cells. This raisesquestions concerning the role of recombination in poxvirus reactivationreactions.

In this communication, we show that replicating poxviruses canexploit viral recombination reactions to produce simple recombinantsfrom mixtures of cotransfected virus and PCR-amplified DNAsas well as more complex recombinants from multiple overlappingfragments of virus DNA. The reaction products can then be packagedinto infectious particles. Our observations suggest that withan efficient heterologous poxvirus reactivation reaction inconjunction with virus recombination reactions, one can geneticallymanipulate the structure of poxvirus genomes in ways not previouslyappreciated. This work also provides further insights into thehyperrecombinogenic intracellular environment created by replicatingleporipoxviruses.

MATERIALS AND METHODS

Top

Materials and Methods

Viruses and cell culture. Vaccinia virus strain WR, SFV strain Kasza, myxomavirus strainLausanne and rabbit SIRC cells were originally obtained fromthe American Type Culture Collection. Vaccinia virus strainCopenhagen was obtained from N. Scollard (Aventis-Pasteur Canada),vaccinia virus strain VTF7.5 was obtained from P. Traktman (MedicalCollege of Wisconsin), and modified vaccinia virus strain Ankarabearing a lacZ insertion [MVA LZ (18)] was obtained from J.Bramson (McMaster University). BSC-40 cells were obtained fromE. Niles (SUNY Buffalo), BGMK cells were obtained from G. McFadden(University of Western Ontario), and BHK-21 cells were obtainedfrom Bramson. All cells were propagated at 37°C in 5% CO₂in minimal essential medium supplemented with L-glutamine, nonessentialamino acids, antibiotics, antimycotics, and 5 to 10% fetal calfserum (Cansera). SFV and myxoma viruses were propagated on SIRCcells, and most vaccinia viruses were propagated on BSC-40 cells.MVA LZ was propagated on BHK-21 cells.

Recombinant virus construction. Vaccinia virus strain XY-I-SceIVV was constructed by standardmethods. Briefly, pTM3 (3, 11) was digested with NcoI and XhoI,and the excised polylinker was replaced with a 44-bp oligonucleotideadaptor encoding the I-SceI site (underlined) (5'-CATGGTAGGGATAACAGGGTAATGTGCACCATCACCACCACCAC-3'and 5'-TCGAGTGGTGGTGGTGATGGTGCACATTACCCTGTTATCCCTAC-3'). Theresulting plasmid (pXY-I-SceI) was purified and partially sequencedto confirm the insert structure, and calcium phosphate was usedto transfect the DNA into vaccinia virus-infected BSC-40 cells.Recombinant gpt⁺ viruses were passaged three times and plaquepurified twice with mycophenolic acid selection. Southern blotswere used to confirm the structure of the selected recombinantvirus and to confirm that the introduced site could be cut byI-SceI.

Virus reactivation assays and DNA transfection methods. BGMK cells were grown to near confluency in 60-mm dishes andthen infected with SFV at a multiplicity of infection of 1 to2 for 1 h at room temperature in 0.5 ml of phosphate-bufferedsaline. The buffer was replaced with 3 ml of warmed growth medium,and the cells were returned to the incubator for another hour.Lipofectamine complexes were prepared by mixing 2 to 5 µgof vaccinia virus DNA in 0.5 ml of Optimem medium with dilutedLipofectamine LF2000 reagent (6 to 15 µl of Lipofectamineplus 0.5 ml of Optimem medium). The mixture was incubated for20 min at room temperature, and then 1 ml was added to eachdish of cells and incubated for another 4 h at 37°C in aCO₂ incubator. The transfection solution was replaced with 5ml of fresh growth medium, and the cells were cultured another3 to 4 days at 37°C. Virus particles were recovered by scrapingthe cells into the culture medium and subjecting the mix tothree cycles of freezing and thawing. This crude extract wasdiluted 10¹- to 10⁵-fold in phosphate-buffered saline and platedon BSC-40 cells to recover vaccinia virus. Plaques were stainedwith a solution containing either 5-bromo-4-chloro-3-indolyl-ß-D-galactopyranoside(X-Gal), to detect recombinant ß-galactosidase activity,or with Giemsa or crystal violet stain, to titrate total virus.

Other DNAs. Vaccinia virus particles were purified by sedimentation throughsucrose gradients, and then the DNA was recovered and purifiedby proteinase K digestion, phenol extraction, and ethanol precipitation.A commercial pulsed-field gel electrophoresis system and 1%agarose gels were used as directed by the manufacturer (Bio-Rad)to size fractionate vaccinia virus DNAs. Gene targeting experimentsused a number of different ß-galactosidase gene cassettesprepared with the PCR and several different primer pairs. Ahigh-fidelity DNA polymerase (Expand high-fidelity PCR system;Roche) was used as directed by the manufacturer. The templatewas plasmid pTKZ-1, which encodes the Escherichia coli ß-galactosidasegene regulated by a vaccinia virus 7.5S promoter (17).

DNAs designed to target the endogenous NotI site in wild-typevaccinia virus were prepared with the two 37-mer primers pTKZ1-LacZNotI18-A(5'-ACACCGACGATGGCGGCCCTTAAAAATGGATGTTGTG-3') and pTKZ1-LacZNotI18-B(5'-TTCGTGTCTGTGGCGGCCCCTCAAAATACATAAACGG-3'). This createda targeting cassette sharing two repeats of 18 bp of flankinghomology with NotI-cut virus. To prepare inserts targeting theI-SceI site in virus XY-I-SceIVV, we PCR amplified the insertwith the 37-mer primers pTKZ1-LacZ-A (5'-GATAATACCATGGTAGGGCTTAAAAATGGATGTTGTG-3')and pTKZ1-LacZ-B (5'-ATGGTGCACATTACCCTGCCTCAAAATACATAAACGG-3')or the 69-mer primers pTKZ1-LacZ-A50 (5'-CCACGGGGACGTGGTTTTCCTTTGAAAAACACGATAATACCATGGTAGGGCTTAAAAATGGATGTTGTG-3')and pTKZ1-LacZ-B50 (5'-TAATTAATTAGGCCTCTCGAGTGGTGGTGGTGATGGTGCACATTACCCTGCCTCAAAATACATAAACGG-3').This created DNA cassettes sharing two 18-bp (7.5KZ18) or two50-bp (7.5KZ50) repeats of flanking homology with SceI-cut XY-I-SceIVV,respectively. A similar approach was used to target an openreading frame encoding enhanced green fluorescent protein (GFP)to the same I-SceI locus. In this case the gene was PCR amplifiedwith the primers GFP-SceI20A (5'-ACGATAATACCATGGTAGGGATGGTGAGCAAGGGCGAGGA-3')and GFP-SceI20B (5'-TGATGGTGCACATTACCCTGTTACTTGTACAGCTCGTCCA-3')and a pEGFP-N1 template (Clontech).

In addition to these substrates, a series of long overlappingPCR fragments spanning nearly all of the vaccinia virus genomewere prepared with the primer pairs summarized in Table 1. Anumber of different thermoresistant DNA polymerases were testedfor use in this application. The Roche Expand long templatePCR kits was eventually found to most reliably amplify longPCR fragments. The DNA sequence of vaccinia virus strain Copenhagen(GenBank entry M35027) and a draft sequence of vaccinia virusstrain WR (kindly provided by B. Moss, National Institutes ofHealth) were used in primer design work. These and other PCR-amplifiedDNAs were gel purified and electroeluted before use. Spectrophotometrywas used to calculate all of the DNA concentrations prior totransfection.

View this table:
[in this window]
[in a new window]
TABLE 1. PCR primers used to amplify overlapping fragments of the vaccinia virus genome^a

Confocal microscopy. The production of GFP by recombinant viruses was detected witha Leica TCS SP2 confocal microscope. BSC-40 cells were culturedon glass slides, coinfected with a mixture of reactivated recombinantvaccinia virus and a vaccinia virus expressing T7 RNA polymerase(VTF7.5), and imaged 24 h postinfection. The expression of GFPwas detected by epifluorescence, while cells were imaged withdifferential interference contrast optics.

RESULTS

Top

Results

Reactivation of vaccinia virus by Shope (rabbit) fibroma virus. The leporipoxvirus Shope fibroma virus (SFV) and the orthopoxvirusvaccinia virus offer several attractive biological featuresthat simplify the experimental approach that follows. In particular,SFV has a very narrow host range, replicating only in rabbitcells and a few selected monkey cells (BGMK). It also growsslowly to modest titers ( ${approx}$ 10⁷ PFU/ml), and the minute ( ${approx}$ 1-mm)plaques look much like transformed foci. In contrast, vacciniavirus has a much broader host range than SFV, grows rapidlyto high titers ( ${approx}$ 10⁹ PFU/ml), and produces large and distinctivecytolytic plaques. As with previously described vaccinia virus-fowlpoxsystems, these phenotypic properties greatly facilitate theseparation and differentiation of mixtures of SFV and vacciniaviruses.

We infected BGMK cells with SFV, and 2 hours later we transfectedthese cells with 2 to 5 µg of DNA extracted from sucrosegradient-purified particles of vaccinia virus strain XY-I-SceIVV.Three days posttransfection, all of the infectious particleswere recovered by cell lysis and replated on the BSC-40 cellline, which supports the growth only of vaccinia virus. Theresulting stained dishes are shown in Fig. 1. Large amountsof virus were recovered with this strategy (yields ranged upto 10⁷ PFU/dish of transfected cells), and the plaques visuallyresembled those produced by the parent strain of vaccinia virus.

View larger version (37K):
[in this window]
[in a new window]
FIG. 1. Reactivation of vaccinia virus DNA in SFV-infected cells. BGMK cells were infected with SFV for 1 h at a multiplicity of infection of 2, and 1 h later they were transfected with 5 µg of purified vaccinia virus XY-I-SceIVV DNA in Lipofectamine LF2000. The cells were cultured for 3 days at 37°C, any resulting virus particles were recovered by freeze-thawing, and different virus dilutions were plated on a BSC-40 cell line to select for growth of vaccinia virus. Some of the viruses were also plated in the presence of mycophenolic acid to select for the gpt⁺ selectable marker encoded by strain XY-I-SceIVV. The plates of BSC-40 cells shown here were stained with Giemsa dye 3 days postinfection and exhibited a characteristic pattern of cytolytic plaques typical of vaccinia virus. No vaccinia viruses were recovered from mock-infected and transfected cells or from cells infected only with SFV.

Strain XY-I-SceIVV encodes a gpt selectable marker, and thereactivated viruses also plated efficiently in the presenceof mycophenolic acid (74% of the plaques recovered in the absenceof selection). The limit of sensitivity was <20 PFU/ml; withinthis experimental constraint, no plaques were detected whenvaccinia virus DNA was transfected into uninfected cells, norwere any cytolytic plaque-forming particles recovered from cellsinfected only with SFV. Microscopic inspection of the controldishes also failed to detect any plaques resembling the fociformed by SFV, although we could not preclude the possibilitythat SFV establishes an abortive infection in BSC-40 cells.To prove that the method produces bona fide vaccinia viruses,we plaque purified several independent virus isolates, extractedvirus DNA, and used Southern blots to compare the HindIII fingerprintof each isolate with that of the parent vaccinia virus strain,XY-I-SceIVV, and its precursor strain, vaccinia virus WR. Figure2 illustrates one such Southern blot; all of the rescued virusesappeared identical to the parent strain at this level of resolution.

View larger version (78K):
[in this window]
[in a new window]
FIG. 2. Southern blot analysis of vaccinia virus genomes reactivated with a heterologous SFV helper virus. DNA was extracted from six different reactivated viruses, digested with HindIII, size fractionated by electrophoresis, and Southern blotted with a ³²P-labeled probe composed of purified vaccinia virus genomic DNA. All of the reactivated viruses that were recovered from cells transfected with XY-I-SceIVV DNA (lanes 2 to 7) displayed a restriction fragment pattern characteristic of the parent strain XY-I-SceIVV (lane 8). There was no evidence of deletions, fusions, or other rearrangements of the reactivated genomes. Lane 9 was loaded with HindIII-digested SFV DNA to show that SFV and vaccinia virus do not share a significant proportion of cross-hybridizing DNA fragments.

Reciprocal reactivation of leporipoxviruses. We also tested whether the reciprocal experiment would work,that is, can an orthopoxvirus reactivate a leporipoxvirus? Wetook advantage of the narrow host range of modified vacciniavirus strain Ankara to test whether MVA could reactivate myxomavirus. (Myxoma virus was used in these experiments because itproduces more easily visualized and accurately titered plaquesthan does SFV.) Preliminary tests showed that both viruses replicatedefficiently on hamster BHK-21 and monkey BGMK cells, but onlymyxoma virus produced plaques on rabbit SIRC cells. We infectedBGMK cells with a lacZ⁺ derivative of MVA [MVA LZ (18)] andthen transfected the cells with wild-type myxoma virus DNA.Four days later the resulting viruses were recovered and platedon SIRC cells. Viruses were recovered with yields of ${approx}$ 300 PFU/µgof transfected DNA, and none of these plaques stained positivelyfor the lacZ marker characteristic of MVA LZ or lacZ⁺ intertypicrecombinants. Thus, it would seem that although the reactionis less efficient, if one uses the appropriate selection strategyan orthopoxvirus can reactivate a leporipoxvirus.

Genetic recombination is associated with virus reactivation. The vaccinia virus genome spans 196 kbp, and no special effortswere made to avoid shearing viral DNA during the process ofDNA extraction. Pulsed-field gels showed that the double-strandedDNA used in these experiments contained the expected distributionof broken molecules ranging in size from <10 kbp to nearfull length (Fig. 3, lane 2). We have shown previously (21)that poxvirus-infected cells catalyze high-frequency recombinationof transfected DNAs with a single-strand annealing mechanism,and we presumed that SFV-infected cells catalyze recombinationalrepair of this sheared vaccinia virus DNA in much the same wayin reactivation reactions.

View larger version (62K):
[in this window]
[in a new window]
FIG. 3. Pulsed-field gel analysis of untreated and restriction enzyme-digested vaccinia virus DNA. DNA was extracted from vaccinia virus virions, size fractionated by pulsed-field agarose gel electrophoresis, and visualized by staining with ethidium bromide. Lanes 1 and 11, molecular size markers; lane 2, purified vaccinia virus DNA (strain WR); lanes 3 to 8, vaccinia virus DNA cut with the indicated restriction enzymes; lane 9, uncut vaccinia virus DNA (strain XY-I-SceIVV); lane 10, XY-I-SceIVV DNA cut with I-SceI.

To examine this question in more detail, we separately digestedpurified wild-type vaccinia virus DNA with BssHII and SacIIand examined the ability of SFV-infected cells to reconstructintact genomes and live viruses from these linearized fragments.Pulsed-field gels showed that these enzymes cut vaccinia virusstrain WR DNA to completion (Fig. 3), and the restriction fragments,with some strain-specific exceptions, closely matched thosepredicted by computational methods (Fig. 4). When these DNAswere transfected separately into SFV-infected BGMK cells, theyproduced no recombinant vaccinia viruses detectable by platingon BSC-40 cells (<20 PFU/dish). However, cotransfecting amixture of SacII- and BssHII-cut DNAs into SFV-infected cellspermitted the production of infectious vaccinia virus particlesat levels essentially identical to the control, uncut, reactionefficiency (2.5 x 10⁵ versus 2.6 x 10⁵ PFU/dish). Similarly,cotransfecting SFV-infected cells with an equimolar mixtureof two large gel-purified BglI-A and StuI-A restriction fragments(Fig. 4) also permitted the recovery of recombinant viruses(2 x 10³ PFU/dish). Nevertheless, there are limits to thesereactions. Attempts to reconstruct vaccinia virus from a mixtureof HindIII- and XhoI-cut molecules were unsuccessful, suggestingthat such enzymes probably cut too frequently or too close toeach other to preclude the reassembly of intact vaccinia virusgenomes by SFV-infected cells.

View larger version (24K):
[in this window]
[in a new window]
FIG. 4. Reactivation of vaccinia virus from transfected mixtures of overlapping DNA fragments. The upper portion of the figure shows a map of the restriction sites predicted and/or known to be present in vaccinia virus strain WR. It should be noted that our ATCC-derived stock of vaccinia virus strain WR lacks a SacII site found at position 36041 in other stocks of strain WR as well as encoding a novel BssHII site at position ${approx}$ 41800. Arrows mark the terminal inverted repeats. Vaccinia virus DNA was digested with the indicated enzymes, and the three different pairwise combinations of fragments shown in the lower panels were transfected into SFV-infected cells. Vaccinia virus was recovered from cells transfected with a mixture of BssHII- and SacII-digested DNA but not from cells transfected with XhoI and HindIII fragments. The former reaction requires at least four recombination events to reassemble a complete vaccinia virus genome (x), and the latter requires at least 12 recombination events. Recombinant vaccinia viruses were also recovered from cells transfected with a mixture of BglI-A and StuI-A fragments. In this case, the two largest restriction fragments were first purified of the remaining portions of the vaccinia virus genome by pulsed-field gel electrophoresis and recovered by electroelution.

Production of recombinant viruses by targeted double-strand break repair. Targeted double-strand break repair can be exploited to simplifythe construction and recovery of recombinant vaccinia viruseswithout plasmid cloning or DNA ligation reactions. Vacciniavirus was modified by standard molecular biological and plasmid-by-virusrecombination methods to incorporate an I-SceI site and Escherichiacoli gpt selectable marker into the thymidine kinase gene locus(strain XY-I-SceI; Fig. 5). Virus DNA was then isolated frompurified XY-I-SceI particles, digested with I-SceI, and cotransfectedalong with a 20-fold molar excess of a PCR-amplified ß-galactosidasegene cassette into SFV-infected cells (Fig. 5). In this case,the ß-galactosidase gene was placed under the regulationof a 7.5S promoter, and the PCR amplicon incorporated two 18-bpend sequences identical to sequences flanking the recombinantI-SceI site.

View larger version (43K):
[in this window]
[in a new window]
FIG. 5. Double-stranded break repair in SFV-infected cells. A recombinant vaccinia virus DNA was digested to completion with I-SceI (Fig. 3) and purified by phenol extraction and ethanol precipitation. This DNA was transfected into SFV-infected cells along with a PCR-amplified DNA fragment encoding the E. coli lacZ gene and a vaccinia virus P7.5S promoter (17). The PCR primers used to amplify the lacZ cassette added two 18-bp terminal sequences identical to sequences surrounding the I-SceI site (gray termini). Reactivated vaccinia viruses were plated on BSC-40 cells, and X-Gal was added to the medium to identify recombinants. DNA was extracted from lacZ⁺ viruses and digested with AvrII and StuI, and a Southern blot was performed to examine the DNA structure. Panel A shows the targeting strategy. Panel B shows a Southern blot probed with a DNA encompassing sequences upstream of and including the I-SceI cleavage site. All of the lacZ⁺ recombinant virus encoded a new 3.8-kbp restriction fragment (lanes 1 to 10). This fragment would be expected to form if recombinational repair reactions used DNA encoding the lacZ gene to repair I-SceI-cut DNA.

X-Gal staining showed that this approach produced about 30%recombinant viruses, and Southern blots confirmed that all ofthe putative recombinants tested (10 of 10) arose through theexpected targeted recombination between the ß-galactosidasegene and the I-SceI cleavage site (Fig. 5). Subsequent experimentsshowed that the frequency of recombinant production was enhancedby increasing the ratio of insert to virus vector and by increasingthe length of terminal homology. Cells cotransfected with I-SceI-cutvaccinia virus DNA and a 40-fold excess of PCR-amplified DNAproduced 100% lacZ⁺ recombinant viruses when the homology wasincreased to two 50-bp sequences (Fig. 6). We also confirmedthat these results were not specific just for I-SceI-cut vacciniavirus DNA. NotI cuts vaccinia virus strain WR only once in nonessentialsequences (10). Similar yields of recombinant virus (4 x 10⁴PFU/µg, 22% recombinants) were obtained when lacZ-encodingPCR amplicons prepared with primers that added two 18-nucleotidesequence homologous to that flanking the NotI site were cotransfectedinto SFV-infected cells along with NotI-cut vaccinia virus DNA.

View larger version (22K):
[in this window]
[in a new window]
FIG. 6. Effect of DNA concentration and homology length on efficiency of recombinant virus production. SFV-infected cells were transfected with a mixture of DNAs comprising a fixed quantity of I-SceI-cut vaccinia virus DNA and various amounts of PCR-amplified DNA encoding a P7.5S-lacZ expression cassette. Two different pairs of PCR primers were used to amplify the lacZ-encoding DNA, which added either two 18-bp or two 50-bp terminal sequences homologous to sequences flanking the I-SceI-cut site (see Fig. 5). Reactivated viruses were subsequently diluted and plated, and the plaques were stained to detect ß-galactosidase activity. A 30- to 40-fold molar excess of insert to vector molecules produced the greatest yield of recombinant virus with either substrate. Incorporating two 50-bp homologies permitted yields of ${approx}$ 100% recombinant viruses.

The production of lacZ⁺ viruses need not have involved homology,since nonhomologous end-joining reactions could serve the samepurpose and Southern blots would not be capable of discriminatingbetween these two types of reactions. We tested the requirementfor homology with a combination of I-SceI-cut virus and thePCR amplicon originally designed to recombine with NotI-cutviral DNA. Such a combination of virus and DNA shows no endsequence homology beyond a few chance nucleotides. Cotransfectingthis mixture of I-SceI-cut vaccinia virus and PCR-amplifiedDNAs into SFV-infected cells yielded significant numbers ofvirus (5 x 10⁵ PFU/µg), possibly by direct ligation, butonly 0.08% were lacZ⁺ recombinants. This low frequency of nonhomologousrecombination is thus very similar to that observed previouslyin vaccinia virus-infected cells with transfected fragmentsof luciferase-encoding DNA (21).

Because the I-SceI site is preceded by a T7 promoter and internalribosome entry site derived from plasmid pTM3 (3, 11), the virusvector used in these reactions can also be used for the directcloning and expression of recombinant proteins. DNA was extractedfrom vaccinia virus strain XY-I-SceI, digested with I-SceI,and cotransfected into SFV-infected cells along with a 760-bppromoterless DNA fragment encoding a GFP open reading frame.Two 20-nucleotide regions of homology permitted a recombinationreaction that was expected to place the GFP gene under the regulationof the T7 promoter (Fig. 7A). Three days posttransfection, theresulting mixture of recombinant and nonrecombinant viruseswas recovered and subsequently cocultivated for another 24 hon glass coverslips along with a helper virus expressing T7RNA polymerase (5). Fluorescence microscopy was used to identifywhich infected cells produced recombinant green fluorescentprotein. A significant portion (perhaps one-third) of the infectedcells expressed GFP under these conditions (Fig. 7B).

View larger version (59K):
[in this window]
[in a new window]
FIG. 7. Single-step construction of recombinant vaccinia viruses expressing green fluorescent protein. (A) SFV-infected cells were transfected with a mixture of DNAs consisting of I-SceI-cut vaccinia virus DNA and PCR-amplified DNA encoding a GFP open reading frame. The PCR primers added two 20-bp terminal sequences homologous to sequences flanking the I-SceI-cut site and created an in-frame fusion between the GFP open reading frame (capital letters) and a vector-encoded start codon (lowercase letters). (B) The resulting mixture of parental and recombinant viruses was recovered and titered and subsequently used to coinfect BSC-40 cells along with a helper virus expressing T7 RNA polymerase. Confocal fluorescence microscopy was used to detect GFP expression 24 h postinfection. These experiments used about 0.6 PFU of the reactivated virus mixture and about 6 PFU of VTF7.5 helper virus per cell.

Targeted deletion of a vaccinia virus restriction fragment. The efficiency of SFV-catalyzed reactivation methods suggestedthat the approach might also be used to assemble other modifiedforms of vaccinia virus genomes. To test this hypothesis, weinvestigated whether an 11.5-kbp fragment of the vaccinia virusgenome could be deleted in a single step with a specially designedPCR amplicon. The experiment involved first digesting vacciniavirus DNA with BglI and then recovering the three largest DNAfragments from an agarose gel. The 11.5-kbp BglI-D fragmentdiscarded at this stage has been shown previously to lack anygenes essential for replication in culture (13). Four PCR primers,a vaccinia virus DNA template, two ordinary PCRs, and a subsequentPCR fragment fusion reaction were then used to prepare a 3.6-kbplinker DNA sharing end sequence homology with the two fragmentsflanking the missing BglI-D fragment but omitting nucleotides21943 to 33500 (Fig. 8). This linker DNA (PCR1 ${Delta}$ ) was then transfectedinto SFV-infected cells along with the other three BglI restrictionfragments and a large PCR-amplified splice fragment (PCR5).PCR5 DNA was added to direct the recombinational repair of thedouble-stranded break separating the BglI-A and BglI-B fragments(Fig. 8). Reactivated viruses were then recovered, plaque purified,and characterized by PCR and Southern blotting (data not shown).In these experiments, the yield of reactivated virus was 3.8x 10³ PFU/µg, and 100% of the viruses (10 of 10) encodeda deletion of the expected number of bases. This yield of viruswas very similar to that obtained by transfecting the threeBglI restriction fragments into SFV-infected cells along withfragment PCR5 and a PCR fragment (PCR1) encoding all of thesequences deleted in PCR1 ${Delta}$ .

View larger version (20K):
[in this window]
[in a new window]
FIG. 8. Method used to construct a vaccinia virus deletion virus. Vaccinia virus DNA was digested with BglI, and the three largest fragments were separated from the smallest BglI-D fragment by pulsed-field gel electrophoresis. The three large fragments were recovered by electroelution and transfected into SFV-infected cells along with the PCR-amplified fragments indicated (PCR1 plus PCR5 or PCR1 ${Delta}$ plus PCR5). The ends of fragment PCR1 ${Delta}$ are identical to the ends of fragment PCR1, but an in vitro fusion reaction was used to join intermediate fragments PCR1 ${Delta}$ -left to PCR1 ${Delta}$ -right and thus eliminate most of the sequences that comprise the nonessential BglI-D fragment (boxed inset). Fragment PCR5 served to bridge the cut separating the BglI-A and BglI-B fragments.

It should be noted that the viruses reactivated in the controlreactions from mixtures of three BglI restriction fragmentsplus PCR1 and PCR5 DNA fragments are indistinguishable fromthe parental virus (vaccinia virus strain WR) because all ofthe DNAs were prepared with vaccinia virus WR reagents. To confirmthat the genetic information incorporated between nucleotides21943 and 33500 actually derived from PCR1 and not from a contaminatingBglI-D fragment, we also prepared a PCR1 fragment with vacciniavirus strain Copenhagen DNA as the template. All of the virusreactivated from cells transfected with this PCR1_COP DNA plusWR-derived BglI and PCR5 fragments bore an XbaI polymorphismindicative of the presence of BglI-D sequences originating invaccinia virus strain Copenhagen (eight of eight viruses tested;data not shown). Besides demonstrating the purity of the mixtureof strain WR-derived BglI-A, BglI-B, and BglI-C fragments, thisresult illustrates how the method can be used to more preciselycontrol the assembly of recombinant viruses from different viralstrains.

In these experiments, we should also note that the PCR1 ${Delta}$ linkerfragment was assembled from two separate DNAs, each encodingone of the two sequences homologous to those found flankingthe BglI-D fragment. The assembly was accomplished with additionalhomologous sequences incorporated into the two central primers,and an in vitro PCR fusion reaction, to combine the 3.3-kbp(PCR1 ${Delta}$ -left) and 0.4-kbp (PCR1 ${Delta}$ -right) fragments into a single3.6-kbp linker (PCR1 ${Delta}$ , Fig. 8). This step proved to be unnecessary,because deletion virus could also be recovered from SFV-infectedcells that had been transfected with PCR1 ${Delta}$ -left, PCR1 ${Delta}$ -right,three BglI restriction fragments, and PCR5. However, requiringthe additional recombinational exchange between DNAs sharing30 nucleotide of sequence homology may have been responsiblefor reducing the yield of reactivated virus about fivefold (from4 x 10³ to 8 x 10² PFU/µg).

Recombinational substitution of essential portions of the vaccinia virus genome with large PCR amplicons. The studies described above showed that one can delete the BglI-Dfragment and rescue the deficiency in reactivated viruses witha large PCR-amplified homolog. However, this is not a very rigoroustest of the method because we used only a single fragment ofDNA and BglI-D encodes no genes essential for virus replication.As a more demanding test of the approach, we examined whetherportions of the virus encoding genes essential for growth inculture could also be PCR amplified and rescued into viablevirus.

The first study examined whether a nearly complete set of overlappingPCR products could be assembled into a reactivated virus. Weused Expand long-range PCRs to amplify a series of 12- to 22-kbpoverlapping fragments spanning most of the vaccinia virus genome(Fig. 9). These fragments included the PCR1 and PCR5 fragmentsused previously. The lengths of the overlaps between differentPCR fragments ranged from 0.3 to 9.3 kbp and were randomly determinedby the manner in which a primer design program (Oligo 6) identifiedsuitable primers. We did not try to amplify DNA located at theimmediate ends of the genome because of anticipated difficultieswith using PCR to reproduce such telomeric features as hairpinsand mismatched bases. Instead, vaccinia virus genomic DNA wasdigested with XhoI, and the resulting ${approx}$ 5-kbp restriction fragmentswere isolated from agarose gels. All of these DNA fragmentswere combined in the appropriate molar ratios and cotransfectedinto SFV-infected BGMK cells, and any resulting virus was rescuedby replating on BSC-40 cells. Despite repeated attempts, theseexperiments failed to generate reactivated virus.

View larger version (34K):
[in this window]
[in a new window]
FIG. 9. Reactivation of vaccinia virus from cotransfected mixtures of PCR-amplified DNAs and vaccinia virus restriction fragments. The two top panels show the PCR fragments amplified for this study and their locations relative to a restriction map of vaccinia virus strain WR. The lower panels show the different combinations of PCR and restriction fragments tested as substrates in SFV-promoted reactivation reactions. No essential genes are encoded by fragment PCR1 (13). To create a sufficiently large overlap between PCR-amplified and SacII-digested DNAs, the 18.6-kbp PCR4 fragment (top panel) was replaced with a larger 21.3-kbp PCR4L fragment (Table 1). Genetic analysis and gene ablation studies have shown that PCR4L encodes numerous essential genes. These include but are not limited to a portion of I3L (14), I8R (6), G2R (7), G4L (20), and G8R (22).

It was of some concern that all of the DNAs used in these experimentshad been purified from agarose gels, because this method canintroduce contaminants into DNA substrates. To show that noinhibitory contaminants were present, we added XhoI-cut vacciniavirus DNA to the mixture and cotransfected this pool of substratesinto SFV-infected cells. This mix of natural and synthetic DNAfragments permitted recovery of virus with a yield of ${approx}$ 2 x 10³PFU/µg.

To gain some understanding as to what other factor(s) mighthave prevented these experiments from working, we examined whetherprogressively less complex mixtures of natural and PCR-amplifiedvaccinia virus DNAs could be recombined and reactivated in SFV-infectedcells. Noting that a mixture of PCR1 and PCR5 fragments alongwith BglI-A, -B, and -C restriction fragments permitted recoveryof reactivated virus, we tested whether virus could also berescued from a combination of just the BglI-A and BglI-C restrictionfragments plus PCR fragments 1 to 5 (Fig. 9). Again, no reactivatedviruses were recovered with this strategy. Finally, we furthersimplified the experiment so that only a single large and yetessential PCR fragment had to be rescued into the vaccinia virusgenome. Several different regions of the vaccinia virus genomewere examined, and we were able to reproducibly recover recombinantand reactivated virus with at least one particular combinationof natural and PCR-amplified DNA.

These studies used the three largest vaccinia virus SacII restrictionfragments and PCR fragments 4L and 8 (Fig. 9). PCR4L (a slightlylarger derivative of PCR4) shared 3.3 and 2.5 kbp of flankingsequence homology with the adjacent SacII fragments and spannedthe genetic interval encompassing genes I3L to L4R. It thusencoded many genes known to be essential for viral growth andassembly (6, 7, 14, 20, 22). PCR8 served only as a recombinationalbridge between the SacII-B and SacII-C fragments (Fig. 9). WhenSFV-infected BGMK cells were transfected with this DNA mixture,we obtained yields of recombinant virus that were essentiallyidentical to those obtained when a control PmeI-B restrictionfragment was used instead of PCR4L (8.5 x 10⁵ versus 8.2 x 10⁵PFU/µg, respectively).

Southern blots were later used to confirm that all (10 of 10)of the viruses recovered and tested were genetic hybrids. Toshow this, we assembled a recombinant virus with a heterologouscombination of WR SacII restriction fragments and Copenhagen"templated" PCR4L_COP DNA and used restriction fragment polymorphismsto identify the origins of different parts of the resultingvirus. A probe targeting SacII-D sequences detected a HincIIsite polymorphism in the reactivated viruses characteristicof strain Copenhagen, while a probe targeting the BglI-D region(Fig. 9) detected an XbaI site polymorphism characteristic ofstrain WR (data not shown). We concluded that one can rearrangeessential portions of the vaccinia virus genome with these methods,but probably only a single amplicon at a time.

DISCUSSION

Top

Discussion

These experiments show that SFV, like fowlpox virus, can beused to rescue and reactivate vaccinia virus in cells transfectedwith vaccinia virus DNA. However, an important difference isthat this seems to be by far the most efficient in vitro heterologouspoxvirus reactivation reaction described to date, and this contentionis supported by direct comparisons. These show that SFV-infectedcells yield ${approx}$ 100-fold more reactivated vaccinia virus than dofowlpox-infected cells (M. Merchlinsky, personal communication).This increase in efficiency offers significant experimentaladvantages, but the numbers still suggest that only a smallproportion of input genomes contribute to the pool of reactivatedviruses that one can eventually recover from SFV-infected cells.Perhaps this is not too surprising because, during the earlysteps in the process of virus rescue, a mixture of virus proteinswould be expected to arise that might well interfere with theactivity of multicomponent protein complexes or the assemblyof virus capsids.

Either mixed infections of orthopoxviruses, leporipoxviruses,and avipoxviruses are thus able to segregate orthologous proteinsinto properly distinct protein complexes, or the architectureof these complexes is sufficiently flexible to accommodate proteinstypically showing only 60 to 80% amino acid identity. The observationthat SFV seems to reactivate vaccinia virus much better thanfowlpox virus suggests that the latter process may operate underthese experimental conditions, since SFV proteins might be morecompatible with vaccinia virus proteins, given the closer evolutionaryrelationship. SFV-infected cells also catalyze very high levelsof nonspecific DNA replication (1) and recombination (4, 12),and these reactions may be another factor contributing to theefficiency of the overall process by more efficiently amplifyingand repairing transfected vaccinia virus genomes.

One advantage of using fowlpox helper viruses is that the geneticdistances which separate avipoxviruses from orthopoxvirusesminimize the risk that mixed infections will produce intertypicvirus recombinants. Leporipoxviruses and orthopoxviruses alsoappear to have been sufficiently isolated by evolutionary processesto prevent SFV from recombining with vaccinia virus. All ofthe viruses that we have rescued to date seem to grow normally,and although we have not pursued an exhaustive screen for intertypicrecombinants, no such viruses were detected with either Southernblots (vaccinia virus) or genetic methods (myxoma virus).

This failure to recover intertypic recombinants probably dependsupon two favorable factors. First, hybrid viruses would probablyexhibit growth deficiencies of various severities that wouldreduce their abundance in mixed populations of replicating viruses.Second, when one compares DNA sequences, about one-quarter ofthe bases differ between even the most closely related virusgenes (probably SFV S068R and vaccinia virus J6R), and one cannotdetect even this limited homology with Southern blots (Fig.2). This is probably insufficient sequence identity to permitefficient recombination, and collectively these two constraintswould compromise the recovery of intertypic recombinant viruses.We believe that, as a method of genetic isolation, the use ofhelper viruses like fowlpox and SFV to reactivate orthopoxvirusesis preferred to the use of homologous psoralen-inactivated orthopoxviruses(19). Heterologous helper viruses seem to be genetically inert,while chemically inactivated viruses could contribute heavilydamaged DNAs to a pool of molecules interacting in a highlyrecombinogenic environment.

Several practical uses for the method have been identified inthis study which exploit the high-frequency recombination andnonspecific DNA replication systems we characterized previously.In particular, one can utilize fortuitously located restrictionsites and PCR-generated linker fragments to create targeteddeletions of nonessential portions of poxvirus genomes. Onecould presumably continue with this process in a stepwise mannerby taking further advantage of existing as well as newly introducedrestriction sites to create a succession of progressively smallerviruses. Appropriately modified viruses can also be used tofacilitate the conditional expression of recombinant proteins.The production of recombinants is most efficient when ratherlong patches of flanking homology are used to target the insertinto the double-stranded break (two 50-bp patches, Fig. 6),but even two 18-bp patches of homology can yield recombinantsat frequencies of up to 30%. In this regard, the effect of homologylength on reaction efficiency is qualitatively similar to thatwe characterized previously in vaccinia virus-infected cells(12, 21), although the different selection methods render absolutecomparisons difficult. SFV-promoted recombination and reactivationreactions are sufficiently efficient that one can directly detectthe expression of vaccinia virus-encoded recombinant green fluorescentprotein without further selection, propagation, or plaque purificationof the recombinant virus (Fig. 7).

Despite the high recombination frequencies detectible in SFV-and vaccinia virus-infected cells, it seems likely that a "numbersgame" ultimately places practical limits on the capacity ofthese systems to generate recombinant viruses. These limitsare of little concern where a simple double strand break repairreaction is used to insert one piece of DNA into a cut vectorwith reactions of the type illustrated in Fig. 5 and 7. However,as the number of exchanges increases, the overall yield of reactivatedvirus is expected to decrease in a manner that depends uponthe efficiency of each component recombination reaction. Thisis best illustrated by considering the impact of each additionalrecombination step occurring with an efficiency near 50% versusonly 20%. The overall yield of virus is crudely expected tofollow the relationship N = N_o x E^x, where N is the overallyield of virus (PFU per microgram), N_o is the maximal yieldpossible with intact transfected DNA, E is the average efficiencyof each component recombination event, and x is the number ofexchanges. With a typical maximal yield of approximately N_o= 10⁶ PFU/µg and the lowest practical yield N = 1 PFU/µg,solving for x suggests that virus should be recoverable if thenumber of exchanges ranges from 8 (E = 0.2) to 20 (E = 0.5).

These values do seem to be useful working limits for this system.For example, very high yields of virus were obtained with mixturesof BssHII- and SacII-cut vaccinia virus DNA (Fig. 4) in a reactionrequiring only four exchanges and involving extensive (i.e.,efficiently recombined) overlaps. Conversely, virus could notbe recovered from cells transfected with a mixture of XhoI-and HindIII-cut vaccinia virus DNA. In this situation, at least12 exchanges are required, and some of the short overlaps betweenfragments (as little as 0.2 kbp) might also be expected to reducethe average recombination efficiency.

A rather surprising feature of this process is that it can beused to reactivate vaccinia viruses from transfected mixturesof virus restriction fragments and large PCR-amplified portionsof the virus genome. It is surprising because it is expectedthat viruses produced by this method would encode multiple newmutations due to the poor fidelity of the DNA polymerases usedin the PCR. These error frequencies vary from 2.6 x 10^-5 (forTaq polymerase) to 8.5 x 10^-6 (Roche high-fidelity PCR system).Using the Roche long-template PCR systems, we are exhibitingan accuracy that probably falls somewhere between these twobounds. If one used 20 PCR cycles to create a pool of ${approx}$ 17-kbpPCR products, each DNA would then bear an average of 3 or 13mutations per molecule if these DNAs were amplified with high-fidelityand Taq polymerases, respectively. Only ${approx}$ 5% of the 17-kbp moleculesamplified with high-fidelity proofreading enzymes would be expectedto be free of errors, and essentially none of the DNAs amplifiedwith Taq polymerase would be error free. Most of these mutationswould be silent, and so these errors might not be enough toprevent the recovery of recombinant viruses with a single largePCR amplicon encoding numerous essential virus genes. However,it becomes more and more unlikely that one could reactivatea virus from mutation-free PCR amplicons as the number of suchfragments increases. This fact may explain why one cannot reactivatevirus from multiple pieces of PCR-amplified DNAs and suggeststhat even the most efficient poxvirus reactivation methods couldnot provide a facile route for reactivating orthopoxvirusesif the only available source of virus DNA was PCR-amplifiedor chemically synthesized materials.

In conclusion, we have shown that the DNA replication and recombinationsystems found in cells infected with replicating poxviruses(1, 12) probably also play an important role in catalyzing virusreactivation reactions. The unusually hyperrecombinogenic environmentcreated in SFV-infected cells can also be exploited to providea simple method for rearranging the structure of poxvirus genomesand might ultimately even provide a novel way of securely archivingorthopoxviruses in an inert form. One could envision purifyingthe virus DNA, cutting it with different restriction enzymes,and storing different digests in separate locations. This processwould address public concerns about the storage of variola virusby rendering the stocks noninfectious and difficult to reactivateunless one had access to both pools of DNA.

ACKNOWLEDGMENTS

We thank I. Damon for advice on long-fragment PCR, N. Scollardfor providing vaccinia virus strain Copenhagen, J. Bramson forproviding MVA LZ, and B. Moss for providing a draft sequenceof vaccinia virus strain WR.

This research was supported by an operating grant to D.H.E.from the Canadian Institutes for Health Research and NSERC equipmentgrants to D.H.E. and colleagues. X.-D.Y. is an NSERC PostdoctoralFellow.

FOOTNOTES

* Corresponding author. Present address: Department of Medical Microbiology and Immunology, University of Alberta, Edmonton, Alberta T6G 2H7, Canada. Phone: (780) 492-2308. Fax: (780) 492-7521. E-mail: devans{at}ualberta.ca.

REFERENCES

Top