Generation of Mutant Murine Cytomegalovirus Strains from Overlapping Cosmid and Plasmid Clones

doi:10.1128/JVI.74.19.8972-8979.2000

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Journal of Virology, October 2000, p. 8972-8979, Vol. 74, No. 19
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Generation of Mutant Murine Cytomegalovirus Strains from Overlapping Cosmid and Plasmid Clones

Mariam E. Ehsani, Tshge W. Abraha, Cecile Netherland-Snell,^§ Niklaus Mueller,^§ Meghan M. Taylor, and Barry Holwerda^*

Department of Veterinary Pathobiology, University of Missouri, Columbia, Missouri 65211

Received 11 January 2000/Accepted 26 June 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We have developed a cosmid and plasmid system to generate mutant strains of murine cytomegalovirus (MCMV). The system is basedon a series of seven overlapping cosmid clones that regenerateMCMV when cotransfected into mouse cells. The unaltered cosmidsproduce MCMV that is indistinguishable from wild-type MCMV basedon restriction enzyme digest patterns of virus DNA and growthrates both in vitro and in vivo. Analysis of viral DNA from plaque-purifiedrecombinant isolates taken from in vitro and in vivo stocks indicatedthat regeneration did not introduce novel mutations in the recombinantviral genomes. Isolation of specific genes and subsequent generationof specific mutant MCMVs was accomplished by replacement of cosmidswith overlapping plasmid subclones. A new vector, PmeSUB, featuringa multiple cloning site and a stringent origin of replication,was constructed to make large subclones for use with smaller subclonescontaining the gene of interest. The utility of this system wasdemonstrated by the generation of two different mutant MCMVs fromdifferent combinations of overlapping plasmid subclones of onecosmid. The advantages of this system are that (i) target genesare maintained as small clones making them amenable to standardin vitro mutagenesis manipulations and that (ii) no reporter orselection genes are necessary to identifymutants.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Murine cytomegalovirus (MCMV) is widely used as a model virus system for the study of human cytomegalovirus (HCMV) pathogenesis.MCMV and HCMV share an essentially collinear arrangement of genes(7, 31) and similar pathogenesis in their respective hosts(18). Our understanding of MCMV and HCMV biology has been greatlyfacilitated by the construction of recombinant viruses bearingspecific mutations in genes of interest. The most widely usedapproach to construct recombinant MCMV involves the introductionof viral DNA and a plasmid bearing the target gene adjacent toa selectable marker and/or reporter gene into permissive cells(reviewed in reference 28). Mutant viruses arise by homologousrecombination between the viral DNA and homologous sequences flankingthe target gene and are isolated by multiple rounds of plaquepurification. In addition, CMV genomes have been isolated as infectiousbacterial artificial chromosomes (BACs) and, from these, specificmutants were constructed (2, 4, 27). A recent versionof the MCMV BAC regenerates an intermediate virus that can deleteits BAC-specific sequences when passaged in vitro, yielding progenyvirus that replicates at wild-type levels in vivo (38). TheCMV BACs have proven to be useful in the identification of openreading frames (ORFs) necessary for MCMV replication (5). However,the construction of BAC mutants requires challenging genetic manipulationsto enable allelic exchange in Escherichia coli (30).

Alternatively, sets of overlapping cosmid and plasmid clones have been used in the construction and direct recovery of herpesvirusmutants that do not contain extra genetic material (10, 11,22, 32, 36, 37). The utility of cosmids and plasmids forthe rapid generation of mutant herpesviruses was demonstratedby the isolation of 17 different HCMV UL54 mutants (9). Herewe describe the isolation of an infectious set of cosmid clonesfor MCMV and its development into a system for generating specificMCMV mutants. The utility of this system was demonstrated by thegeneration of two mutant MCMV strains by replacement of one cosmidwith two different series of overlapping subclones. These combinationsof cosmids and plasmids generated mutant strains of MCMV withoutthe need for plaquepurification.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture and viruses. Murine fibroblasts (NIH 3T3; ATCC CRL-1658) were maintained on Dulbecco modified Eagle medium (DMEM) supplemented with 5%calf serum and 2 mM glutamine at 37°C in 6% CO₂ in a humidifiedincubator. MCMV (Smith strain, ATCC VR-1399) DNA was used forcosmid librariesconstructed.

Vector constructions. The cosmid vector, PmeCOS (pBH021; Fig. 1A), used to make libraries was derived from pJB8 (19). Complimentary oligonucleotides,5'-AATTCCGTTTAAACAG-3' and 5'-GATCCTGTTTAAACGG-3', were phosphorylatedusing T4 polynucleotide kinase (33) and allowed to anneal formingan adaptomer. This adaptomer featured a cut EcoRI site on oneend, with a PmeI site in the middle and a cut BamHI site on theother end. The adaptomer was ligated into EcoRI-cut pJB8 to yieldPmeCOS, which has the cloning site configuration of EcoRI-PmeI-BamHI-PmeI-EcoRI,as confirmed by DNA sequence analysis.

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FIG. 1. Cosmid and plasmid vectors for making infectious MCMV clone sets. (A) The PmeCOS cosmid vector was constructed by adding a pair of PmeI sites surrounding the BamHI cloning site of pJB8 (19) so that any cloned MCMV sequences can be removed intact. (B) The PmeSUB vector was derived from pACYC177 by replacement of the Kan^r gene with the MCS from pBluescript. The MCS was surrounded by PmeI sites to allow excision of MCMV sequences.

The plasmid vector PmeSUB (pBH060; Fig. 1B) was constructed for subcloning MCMV sequences from cosmid clones. The multiplecloning site (MCS) from pBluescript KS( $-$ ) (1, 34) was amplifiedby PCR using the primers 5'-ATTGACCACGTGTTTAAACGCCAGTGAATTGTAATACGAC-3'and 5'-ACTGCTCACGTGGTTTAAACACTAAAGGGAACAAAAGC-3'. The amplifiedproduct contained an MCS surrounded by PmeI restriction siteswith PmlI sites at its ends. The PCR fragment was blunt endedby digestion with PmlI, followed by ligation into the T4 DNA polymerase-bluntedHindIII and XhoI sites within the kanamycin resistance gene ofpACYC177 (6), yieldingPmeSUB.

MCMV DNA isolation. Viral DNA was isolated from purified virus as follows. Ten T-150 flasks of MCMV-infected cells, including media, were frozenat $-$ 80°C and thawed to lyse the cells. The lysate was clarifiedby two rounds of centrifugation (Beckman JA-14 rotor; 7,500 ×g, 20°C, 20 min), and the supernatant was further centrifuged(Beckman JA-14 rotor; 30,000 × g, 20°C, 3 h) to pellet the virus.The crude virus pellet was resuspended in 0.5 ml of 10 mM Tris-HClbuffer (pH 8.0) containing 10 mM MgCl₂. DNase (bovine pancreaticDNase I; Sigma) was added to a final concentration of 200 µg/ml,and the mixture incubated at 37°C for 1 h. EDTA was added to afinal concentration of 50 mM, and the viral suspension was centrifugedthrough a sucrose cushion (20% sucrose in 10 mM Tris-HCl buffer[pH 8.0], 150 mM NaCl, and 1 mM EDTA) in a Beckman SW28 rotor(113,000 × g, 20°C, 1 h). The resulting pellet was resuspendedin 200 µl of buffer (10 mM Tris-HCl buffer, pH 8.0; 10 mM EDTA)and incubated overnight at 37°C in the presence of sodium sarkosinate(1%), sodium dodecyl sulfate (SDS; 0.5%), and proteinase K (250µg/ml). The lysate was extracted twice with phenol-chloroform-isoamylalcohol, and purified MCMV DNA was recovered by precipitationwithethanol.

Infected-cell DNA was isolated as follows: MCMV-infected cells were scraped from tissue culture flasks (100% cytopathic effect)and washed twice with phosphate-buffered saline (PBS). The cellswere resuspended in 0.5 ml of 10 mM Tris-HCl buffer (pH 8.0) containing100 mM NaCl, 0.6% SDS, and 0.1 mg of proteinase K per ml and incubatedat 37°C overnight. This mixture was extracted twice with phenol-chloroform-isoamylalcohol, and the DNA was recovered by precipitation withethanol.

Library construction. Cosmid libraries were constructed from both purified virus DNA and MCMV-infected-cell DNA according to methods developed forlibrary construction in pJB8 (19). DNA from either purifiedvirions or virus-infected cells was partially digested with restrictionendonuclease Sau3AI to an average length of 40 to 45 kb. Purifiedviral DNA digested with Sau3AI was dephosphorylated with shrimpalkaline phosphatase (Boehringer Mannheim), followed by ligationwith BamHI-digested PmeCOS arms. In contrast, infected-cell MCMVDNA digested with Sau3AI was size fractionated by sucrose densitygradient centrifugation (33), but it was not dephosphorylatedprior to ligation. The left cosmid arm was the 5.4-kb HindIII-BamHIfragment of PmeCOS with the HindIII end dephosphorylated priorto cutting with BamHI, whereas the right arm was the 2.4-kb BamHI-SalIfragment with the SalI end dephosphorylated. Ligation reactions,containing Sau3AI-digested MCMV DNA and a molar excess of PmeCOSarms, were catalyzed by T4 DNA ligase at 16°C for 16 h. The ligationproducts were packaged into bacteriophage lambda using commerciallyavailable packaging mixes (Gigapack III XL and Gigapack III Plus;Stratagene). Escherichia coli DH10B (recA1) grown in the presenceof 10 mM MgCl₂ (33) was transduced with the packaged librariesfollowed by plating and growth on Luria-Bertani (LB) agar mediaplates containing 100 µg of ampicillin perml.

Selection of overlapping cosmid clones. Cosmid DNA from randomly picked colonies was digested with EcoRI to map cloned inserts, whereas DNA sequencing precisely identifiedthe boundaries of selected clones. Colony hybridization with radioactiveDNA probes against replicate filters (33) was used to find clonescovering (i) MCMV nucleotides (nt) 83,000 to 85,000 and (ii) thefused genome ends formed during viral replication (20, 21).Clones overlapping the 83,000-nt region were identified with a1.1-kb EcoRI fragment covering MCMV nt 83861 to 84978, whereasreplicative intermediate clones were found using a 1.8-kb EcoRI-HindIIIfragment from MCMV nt 888 to2718.

Cosmid subclones. The M78 ORF (31) was isolated from cosmid pBH551 on a 6.2-kb KpnI fragment in pUC18 (40), yielding pBH042. The remainderof the cosmid was isolated as a 5.8-kb PmlI fragment in pUC18,pBH045; a 13.4-kb NheI fragment in PmeSUB, pBH067; and a 22-kbPmeI-HindIII fragment in PmeSUB, pBH065. pBH042 was digested withNsiI, and the NsiI-ends were blunted with T4 DNA polymerase plusdeoxynucleoside triphosphates, followed by intramolecular ligationyieldingpBH057.

The M80 ORF was isolated as pBH058 by ligating the 3.3-kb XhoI fragment from pBH027 and the 3.5-kb XhoI-HindIII fragment ofpBH045 into HindIII-plus-SalI-cut pUC18. pBH027 was derived frompJML28 (25) through ablation of the SspI site at MCMV nt 113,356by oligonucleotide-directed mutagenesis (41, 42) using theoligonucleotide 5'-CGTGATGTGTAAGATTAGATGATTG-3' and a commerciallyavailable kit (GeneEditor; Promega). pBH064 was constructed byligating the 13-kb PmlI fragment from pBH551 into the SmaI siteofPmeSUB.

Cotransfection. Individual colonies from each cosmid set member or plasmid subclone were isolated on solid medium and used to inoculate 100-mlliquid cultures (LB medium containing 100 µg of ampicillin perml) for DNA purification using the Qiagen Plasmid Midi Kit (Qiagen).Occasionally, some cosmid clones were unstable and converted intosmall, undefined plasmids when grown under these conditions. Forthese, a 1- to 2-ml liquid culture grown overnight at 37°C wasused to inoculate 500-ml liquid cultures that were grown at 37°Cto middle logarithmic phase (0.4 to 0.6 optical density at 600nm) before isolation of cosmid DNA using the Qiagen Plasmid MidiKit. The integrity of each cosmid DNA preparation was checkedby digestion with EcoRI, followed by agarose gel electrophoresis.The MCMV sequences were released from the cosmid and plasmid vectorsby digestion with either PmeI or the appropriate restriction enzymes,followed by a single phenol-chloroform-isoamyl alcohol extractionand precipitation and washing with ethanol. The dried DNA pelletwas redissolved in sterile water in preparation forcotransfection.

PmeI-digested cosmids or cosmids plus plasmids were used to cotransfect mouse cells pretreated with DEAE-dextran (23, 29)in T-25 flasks using the calcium phosphate coprecipitation method(16), followed by glycerol shock at 6 h after cotransfection(15). At 36 to 48 h following cotransfection, the medium wasreplaced with fresh medium containing penicillin and streptomycin.A cytopathic effect was visible 5 to 7 days after cotransfectionand was allowed to progress until 100% cytopathic effect, at whichpoint the flasks were frozen at $-$ 80°C. A portion of the thawedlysate was used to infect cells in T-150 flasks to establish virusstocks for furtherstudy.

In vitro growth of cosmid-derived MCMV. Multistep growth curves were determined for wild-type (Smith strain) and cosmid-derived virus in NIH 3T3 cells. Cells wereinfected at an MOI of 0.01 for 1.5 h at 37°C, washed once withmedium, and incubated for various times in a six-well plate. Ateach time point cells, including media, were frozen at $-$ 80°C untiltiters were determined by standard plaque assay on NIH 3T3cells.

Analysis of DNA from plaque-purified virus isolates. Plaque-purified strains ("isolates") were established by four sequential rounds of plaque isolation using medium containing0.5% agarose as an overlay. DNA was isolated from purified virusand further refined using GeneClean (Bio 101) prior to restrictionenzyme digestion or amplification by PCR. DNA was exhaustivelydigested with HinP1I, followed by radioactive end labeling usingT4 polynucleotide kinase and [³³P]ATP (33). The fragments were resolved by polyacrylamide gelelectrophoresis on a gel composed of 10% acrylamide-0.11% bisacrylamideover a 1×-to-5× TAE buffer gradient (1× TAE is 40 mM Tris-acetatebuffer [pH 8.0] containing 1 mM EDTA) using a standard sequencinggel apparatus with the dried gel used to make an autoradiogram.Selected regions of the viral genome were amplified using PCRwith three different pairs of primers as follows: (i) 5'-GACCTAAACCTCCACCAAGACGand 5'-CGGAACTAGTCCCAAATCCATAC to amplify MCMV nt 6936 to 8827,(ii) 5'-AAACACAGGCTGACGAAGGT and 5'-CACGGAGTTTTCGCAAAGATA to amplifyMCMV nt 46119 to 47529, and (iii) 5'-AGCATACTGCACGGCGGTCT and5'-TGGCAGGGATTGAAAGCGAA to amplify MCMV nt 83321 to 84466. ThesePCR products were cloned into pCR2.1 TOPO (Invitrogen), followedby DNA sequence analysis of theinserts.

Southern hybridization. DNA (total infected cell, 1 µg; viral DNA, 0.25 µg) was digested overnight with restriction endonuclease before fractionationby agarose gel electrophoresis and blotting to a nitrocellulosemembrane using standard methods (33). DNA probes were labeledwith [³²P]dCTP using the random priming method (14) with a commerciallyavailable kit (Boehringer Mannheim) and hybridized overnight in6× SSPE (1× SSPE is 0.18 M NaCl, 10 mM NaH₂PO₄, and 1 mM EDTA[pH 7.7])-1× Denhardt's solution-0.1% SDS at 65°C. Following hybridization,the membrane was washed three times for 20 min in 0.1× SSPE plus0.1% SDS at 68°C before exposure to X-rayfilm.

In vivo growth of cosmid-derived MCMV. BALB/c mice were infected intraperitoneally with 5.0 × 10⁵ PFU of tissue culture-grown wild-type (Smith strain) or regeneratedMCMV. At 10 days postinfection, the animals were euthanized andthe salivary glands were removed and homogenized in DMEM containing5% calf serum, penicillin (100 IU/ml), streptomycin (100 µg/ml),and gentamicin sulfate (50 µg/ml). Virus titers for each animalwere determined by standard plaque assay on NIH 3T3cells.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

These results describe the construction of a set of infectious cosmid clones and its development into a system of cosmidsand plasmids that generate site-specific MCMVmutants.

Cosmid libraries were constructed using a new cosmid vector, PmeCOS, which was derived from the cosmid vector, pJB8 (19),by surrounding the BamHI cloning site with PmeI restriction sites(Fig. 1A). PmeI sites are not found in the genome of MCMV (31),and therefore any cloned MCMV sequence could be removed by digestionwith this enzyme. PmeCOS is 5.4 kb and will accept cloned insertsof up to 45kb.

Establishing an infectious set of cosmid clones required isolating recombinants containing inserts that covered the entireMCMV sequence, including the fused ends of the replicative intermediategenome (20, 21). Our initial selection of cosmid clones wasdeficient in those that covered the region around nt 83,000 andthe replicative intermediate. These were isolated from infected-cellDNA-derived libraries using hybridization probes specific to therespective regions of the genome (see Materials and Methods).The genome locations of the cosmid set are illustrated diagrammaticallyin Fig. 2 with the precise insert coordinates given in Table 1.The inserts ranged from 35 to 46 kb, with sequence overlaps rangingfrom 884 nt between pBH400 and pBH551 to 28,644 nt between pBH343and pBH325 (Table 1). Although these latter cosmid clones overlapby approximately 30 kb, they were included in the cosmid set analyzedhere since our immediate goal was to cover the entire genome andthen demonstrate the feasibility of using these clones to regenerateMCMV. We have mapped approximately 200 other cosmid clones fromwhich others having different regions and extents of overlap maybe selected to isolate different genes of interest. The restrictiondigests shown in Fig. 3 demonstrate the utility of using EcoRIto identify the approximate genomic location of each cosmid clone.EcoRI has 34 recognition sites in the Smith strain sequence (31)and, as a consequence, produces readily interpretable restrictionpatterns when used to digest the cosmid clones (see references13 and 26). As expected, digestion of the cosmid clones withPmeI releases the high-molecular-weight MCMV sequences from the5.4-kb PmeCOS vector (Fig. 3).

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FIG. 2. Genome coordinates of the cosmid set that regenerates MCMV. The gray bars indicate the extent and location of each cosmid insert. The MCMV genome nucleotide coordinates are indicated at the top in kilobases. The alphabetic designations for the larger EcoRI fragments of Smith strain (13, 26) are indicated below the genome coordinates. The vertical lines indicate the location of EcoRI sites.

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TABLE 1. MCMV genome coordinates of infectious cosmid and plasmid inserts

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FIG. 3. Restriction digests of the infectious cosmid set. The complete set of infectious cosmids for reconstituting MCMV was digested with either EcoRI or PmeI, fractionated by agarose gel electrophoresis and stained with ethidium bromide. The released MCMV sequences and cosmid vector, PmeCOS, are indicated on the right. The molecular size standards (std) are BstEII-digested $lambda$ DNA.

The set of cosmid clones was digested exhaustively with PmeI, mixed in equal proportions, and used to cotransfect mouse fibroblasts.After 5 to 6 days of incubation, the monolayer showed areas ofcytopathic effect that were similar in appearance to those inMCMV-infected cells (not shown). This result was achieved usinga range of from 1 to 3 µg of each cosmid, with the larger amountscausing more advanced infection at somewhat earlier times aftercotransfection (not shown). Three cosmid-derived MCMV lines, cM4,cM5, and cM6 ("cM" derived from cosmid MCMV) were establishedfrom cotransfections of 1, 2, or 3 µg of each cosmid, respectively,and these were analyzed as describedbelow.

Virus DNA prepared from stocks of Smith and regenerated lines of MCMV and was compared by visual examination of restrictionenzyme digests separated on electrophoretic gels (Fig. 4A). TheEcoRI and KpnI digests of cosmid-derived virus DNAs were indistinguishablefrom Smith MCMV DNA, indicating that large genomic rearrangementsdid not take place when the virus was regenerated. The in vitrogrowth characteristics of the regenerated lines were also indistinguishablefrom wild-type MCMV, as evidenced by the equivalence of viralyields at each time postinfection (Fig. 4B). Our long-term interestin developing a recombinant virus generation system was to eventuallyconstruct MCMV mutants for pathogenesis studies. Thus, it wasnecessary to show that cosmid-derived MCMVs demonstrated unalteredgrowth in vivo. Mice were infected with tissue culture-grown stocksof either Smith strain or cosmid-derived MCMVs, and salivary glandtiters were determined at 10 days postinfection (Fig. 4C). Theorgan titers developed by each recombinant strain resembled thosefrom the wild-type Smith strain, indicating that cosmid-derivedMCMVs are unaltered in their ability to replicate in vivo. Thus,comparison of in vitro and in vivo growth indicates that cosmid-derivedMCMVs are similar to wild-type MCMV.

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FIG. 4. Analysis of regenerated MCMV. (A) Analysis of viral DNA from cosmid-generated MCMVs. DNA from purified virions of three independent cosmid-generated MCMV strains (cM4, cM5, and cM6) was digested with EcoRI (E) or KpnI (K), separated on a 0.8% agarose electrophoretic gel, and stained with ethidium bromide. The wild-type MCMV DNA (wt) is the Smith strain, and the size standards (std) are $lambda$ DNA digested with BstEII. (B) In vitro multistep growth of cosmid-generated MCMV. Three independently generated strains of MCMV, cM4, cM5, and cM6, were used to infect NIH 3T3 cells at an MOI of 0.01. Virus was harvested at the times indicated postinfection, and titers were measured by a standard plaque assay. (C) In vivo growth of cosmid-generated MCMV. BALB/c mice were infected with 5.0 × 10⁵ PFU of the indicated strain of tissue culture-grown MCMV. At 10 days postinfection salivary glands were removed, and the titers for the individual mice were determined. The results are the means of three to five mice, with error bars showing the standard deviation for each group.

To further analyze regenerated virus, we prepared plaque-purified isolates from one of the regenerated lines, cM4, and comparedthese to plaque-purified isolates from Smith MCMV. Specifically,16 isolates were prepared and included 4 isolates from the cM4in vitro-passaged stock, 4 isolates from cM4 in vivo-passaged(salivary gland) stock, 4 isolates from in vitro-passaged Smithstock, and 4 isolates from in vivo-passaged (salivary gland) Smithstock. Virus DNA from each isolate was purified and digested withHinP1I, and the resulting fragments were radioactively end labeledbefore separation by gel electrophoresis and autoradiography (Fig.5). HinP1I has 1,826 recognition sites in the MCMV genome sequence(31), and thus digestion with this restriction enzyme mightreveal more-subtle differences between the strains. Our electrophoresissystem allowed us to resolve more than 200 distinct fragmentsfor each isolate, and the majority of these were identical betweenall the isolates. However, there were a small number of differencesbetween the isolates. In one case, an additional fragment at approximately510 bp (Fig. 5, indicated as "[ii]") was found in two of the Smithin vitro and in vivo isolates, all four of the cM4 in vitro isolates,and two of the cM4 in vivo isolates. Additionally, one of theSmith in vitro isolates possessed a unique fragment shift (Fig.5, [i]), whereas another of the Smith in vivo isolates was missinga fragment (Fig. 5, [iii]). Lastly, an additional ~400-bp fragment(Fig. 5, [iv]) was found in three of the Smith in vitro isolatesand two of Smith in vivo isolates but was not found in any ofthe cM4 in vitro or in vivo isolates. A HinP1I digest of DNA froma non-plaque-purified stock of Smith MCMV was included in thisanalysis (Fig. 5, lane L). This sample possessed the additionalfragments [ii] and [iv], but not the variations [i] or [iii] describedabove.

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FIG. 5. Analysis of plaque-purified isolates of MCMV. Radioactively labeled HinP1I restriction fragments separated by gel electrophoresis were used to produce the autoradiogram sections illustrated. Plaque-purified isolates, designated A through D at the top of the lanes, were derived from stocks of in vitro- and in vivo-propagated Smith stocks (wild-type) and in vitro- and in vivo-propagated cM4 stocks. DNA from non-plaque-purified Smith stock, designated L, was included for comparison. Only portions of the autoradiogram showing differences between the isolates are shown, with the location of size standards (MspI-digested pUC19 fragments) indicated on the left. Fragment variations, [i] through [iv], are indicated where they occur by symbols ( $black-triangle-right$ , $right-triangle$ , and $right-arrow$ ).

One of the cM4 isolates, in vitro isolate B (see Fig. 5) was further examined by DNA sequence analysis through three regions,where its component cosmids overlap. Specifically, the overlapregions between cosmids pBH504 and pBH303 (MCMV nt 6936 to 8827),pBH303 and pBH400 (MCMV nt 467119 to 47529), and pBH400 and pBH551(MCMV nt 83321 to 84466) were amplified by PCR, cloned, and sequenced.As a control, the same regions of viral DNA from a non-plaque-purifiedSmith stock were also amplified, cloned, and sequenced. The DNAsequence from each region of the cM4 in vitro isolate B was identicalto the Smith MCMV sequence (data not shown and reference 33).This result indicates that regeneration with cosmids did not introduceany of the cosmid vector sequences in the recombinant viral genome.In contrast, one PCR product from Smith MCMV DNA possessed a T-to-Cpoint mutation at MCMV nt 46272. We cannot rule out the possibilitythat this mutation was an artifact of PCR amplification, but ifit exists in the MCMV genome it would result in a Ser-to-Pro mutationin the M25 gene product (31). Most importantly, the HinP1I restrictionpatterns and DNA sequence analysis of plaque-purified regeneratedvirus isolates, propagated either in vitro and in vivo, indicatesthat they do not possess any novel or excessive numbers of mutationswhen compared to wild-typeMCMV.

The development of the infectious cosmids into a system for producing MCMV mutants required an approach to alter specificgenes since cosmids are generally too large for routine moleculargenetic manipulations. The route taken was to isolate the targetgene on a smaller plasmid clone and include this in a series ofoverlapping subclones to replace one of the infectious cosmids.This approach was taken to demonstrate the generation of two strainsof MCMV with mutations in the M78 and M80 ORFs,respectively.

The M78 gene encodes a putative G-protein coupled receptor homologue (31) and is likely involved in pathogenesis (3,8, 12). Hence, a mutation in this gene was not likely tocause serious impairment of in vitro replication, thus allowingus to use this as an uncomplicated test of our mutagenesis system.The M78 ORF is contained on cosmid pBH551 and was subcloned asa 6.2-kb KpnI fragment in pUC18, yielding pBH042 (Fig. 6). A mutationwas introduced into the M78 gene so that it could be identifiedin the recombinant virus. Specifically, an NsiI restriction sitewithin the translated region was removed yielding pBH057 (Fig.6). Another subclone, pBH045, consisting of a 5.8-kb PmlI fragmentfrom pBH551 maintained in pUC18, was constructed to overlap withpBH042 and the adjacent cosmid pBH343 (Fig. 6). To facilitatesubcloning, the remainder of the cosmid a new vector, PmeSUB,was constructed (Fig. 1B). PmeSUB was derived from pACYC177 bythe addition of an MCS surrounded by PmeI sites. The significantfeatures of this vector are that it can maintain large clonedinserts because of its stringent origin of replication (6)and that any cloned MCMV sequence can be released by digestionwith PmeI. PmeSUB was used to maintain a 13.4-kb NheI fragment,pBH067, and a 22-kb PmeI-HindIII fragment, pBH065, to completethe overlapping series of subclones from cosmid pBH551 (Fig. 6).

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FIG. 6. MCMV genome coordinates of plasmids replacing cosmid pBH551. Two series of overlapping plasmid clones were constructed to isolate the M78 and M80 ORFs on smaller replicons. Restriction sites: B, BamHI; H, HindIII; K, KpnI; N, NheI; Nsi, NsiI; P, PmlI; Pst, PstI; S and Ssp, SspI; X, XhoI. Nsi (crossed out) in pBH057 and Ssp (crossed out) in pBH058 indicate the location of mutations ablating the respective restriction sites.

Two recombinant MCMVs were generated by cotransfection of NIH 3T3 cells using cosmids (pBH303, -400, -343, -325, -341, and-504, excluding pBH551) and plasmids (pBH045, -067, and -065)plus either the wild-type M78 gene on pBH042 or the mutated M78gene on pBH057, yielding strains cM10 and cM11, respectively.Strain cM10 was constructed from nonmutated plasmids and shouldresemble wild-type MCMV. In contrast, strain cM11 was expectedto have a mutation (NsiI site ablation) since it was generatedby using the mutated M78 ORF from plasmid pBH057. Both cotransfectionsresulted in a cytopathic effect in the cells following 5 to 6days of incubation, and stocks of cM10 and cM11 were establishedwithout complementation on NIH 3T3 cells. Viral DNA from cM10and cM11 and wild-type MCMV was digested with NsiI and separatedby gel electrophoresis, followed by blotting to a nitrocellulosemembrane for hybridization with a probe for the M78 ORF (Fig.7A). Ablation of the NsiI site in cM11 DNA yielded a new 28.6-kbNsiI fragment derived from the 15.9- and 12.7-kb fragments foundin wild-type and cM10 MCMV DNA (Fig. 7A). A radioactive M78-specificprobe, pBH042, hybridized only to the aforementioned DNA fragments,confirming that the NsiI mutation was incorporated into the M78ORF of cM11 and not cM10 as expected (Fig. 7A). The recovery ofthese particular NsiI fragments in the respective strains indicatesthat regeneration of MCMV from a mixture of cosmids and plasmidsproduced only the desired viruses.

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FIG. 7. Analysis of recombinant MCMV bearing directed mutations. (A) Analysis of strains cM10 and cM11. DNA from purified virions was digested with NsiI and separated by agarose gel electrophoresis (left panel), followed by blotting to a nitrocellulose membrane. The membrane was hybridized to a radioactively labeled DNA probe, pBH042 (right panel). The closed arrowhead indicates the location of the 28.6-kb NsiI fragment unique to cM11, and the open arrowheads indicate the 15.9- and 12.7-kb NsiI fragments unique to wild-type (Smith strain) and cM10. (B) Analysis of strain cM9. Infected cell DNA was digested with BamHI plus SspI and separated by agarose gel electrophoresis, followed by blotting to a nitrocellulose membrane. The membrane was hybridized to a radioactively labeled DNA probe, pJML28 (see Fig. 6).

As a different example, the cosmid pBH551 was replaced with overlapping subclones so that mutations could be introduced intothe M80 gene. The M80 gene, which encodes the protease and assemblyprotein (24, 39), was isolated from cosmid pBH551 on a 6.8-kbfragment subcloned into pUC18, yielding pBH058 (see Materialsand Methods). This construct overlaps another plasmid, pBH064,and the cosmid pBH343 (Fig. 6). Additionally, pBH058 carries anablated SspI site mutation located 57 nt proximal to the initiationcodon of M80 and in the adjacent M79 ORF (25, 31). The SspImutation was introduced to distinguish the regenerated virus,but it did not change the amino acid sequence of the predictedM79 gene product. The remainder of cosmid pBH551 was isolatedin PmeSUB as a 22-kb PmeI-HindIII fragment, pBH065, and a 13-kbPmlI fragment, pBH064 (Fig. 6). Cotransfection of the three pBH551subclones (pBH058, -064, and -065) and the remainder of the cosmids(pBH303, -400, -343, -325, -341, and -504, excluding pBH551) intomouse cells resulted in a cytopathic effect at 5 to 6 days posttransfection.This recombinant MCMV was designated cM9. Hybridization analysisof infected-cell DNA showed that cM9 MCMV DNA lacked the SspIsite originally ablated in pBH058 (Fig. 7B). Specifically, theM80 probe, pJML28 (25; Fig. 6) hybridized to 1.95- and 1.3-kbfragments in Smith strain DNA in contrast to a single 3.25-kbfragment in cM9 DNA. The probe did not hybridize to 1.95- and1.3-kb fragments in cM9 DNA even upon extended exposure, indicatingthat this was the only product of regeneration (data not shown).The probe also hybridized to short sequences outside the BamHIsites of pJML28, yielding weak signals at 6.6 and 0.7 kb for bothSmith and cM9 DNA (Fig. 7B). Overall, the results of manipulatingthe M78 and M80 ORFs demonstrate that a combination of cosmidsand plasmids could be used to generate different desired mutantstrains ofMCMV.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The aim of this work was to develop a facile system for constructing specific mutant strains of MCMV. Our results demonstratethat an appropriately designed set of cosmid and plasmid clonescan be used to accomplish this goal. In one example, a recombinantvirus, cM11, bearing a restriction site mutation in the M78 ORFwas generated using an overlapping set of six cosmids and fourplasmid clones. The mutation was introduced into one plasmid,pBH057, which was used to replace the nonmutated plasmid, pBH042,yielding the desired mutant virus. Use of the nonmutated cosmidand plasmid set produced a "wild-type" recombinant, cM10, whichserved as a control for regeneration efficiency. In a differentexample, we produced another recombinant virus, cM9, with a restrictionsite mutation in the M79 ORF using a set of six cosmids and threeplasmids. Again, the mutation was engineered into one of the plasmids,pBH058, using standard molecular geneticmethods.

These results suggest that it is feasible to generate specific mutant viruses for any gene provided the mutation does notincapacitate basic replication functions. However, it should bepossible to generate viruses bearing lethal mutations by cotransfectioninto appropriately constructed complementing cell lines. We haveconstructed the mutants described here using a set of seven cosmidclones, but we have approximately 200 other partially characterizedcosmid clones available. It is reasonable to assume that differentcosmids can be used to generate mutants specific to genes locatedin the overlap regions of the cosmid set used here. The abilityto vary the composition of the cosmids and plasmids immediatelysuggests that more than one mutation might be simultaneously introducedinto a single recombinant virus. MCMVs carrying multiple specificlesions may become useful tools to gain a better understandingof viral replication andpathogenesis.

Cosmid and plasmid combinations have been used to regenerate specific mutants in other herpesviruses, including herpes simplexvirus type 1 (11, 32), pseudorabies virus (37), varicella-zostervirus (10), Epstein-Barr virus (36), and HCMV (9, 22).In all cases, the regeneration of virus depended upon using aset of clones covering the entire sequence of the virus with sufficientoverlap across adjacent clones to allow homologous recombinationof the viral DNA sequences. MCMV regeneration from cosmids furthershows that this method does not result in the production of unwantedmutations or rearrangements in the viral genome (see Fig. 5).The development of these systems followed the seminal observationby Graham et al. (17) showing that herpesvirus DNA is infectious.In addition to isolating infectious cosmids for MCMV, we havedeveloped a general system for producing MCMV mutants by includingthe subcloning vector, PmeSUB. This vector was designed to makesets of overlapping plasmid subclones for the replacement of cosmids.Although most MCMV genes are small enough to be stably maintainedin high-copy-number vectors such as pUC18, the subcloning of theremaining cosmid sequences is hindered by their large size. PmeSUBwas derived from pACYC177 (6) in order to take advantage ofits stringent origin of replication which can maintain large clonedinserts. The MCMV genome was originally restriction mapped usinga series of clones maintained in pACYC177 (13, 26), thus provingthe value of thisreplicon.

Most commonly, the construction of mutant MCMVs involved the introduction of viral DNA and a plasmid bearing the target geneplus an extraneous selection and/or reporter gene into permissivecells. Mutants arose by homologous recombination and were isolatedfrom an excess of wild-type virus by multiple cycles of plaquepurification. The successes from using this approach are underscoredby the many different mutants it has produced (reviewed in reference28). In some instances, however, the insertion of extraneousselection or reporter genes in the recombinant virus may interferewith the expression of adjacent genes preventing recovery of thedesired mutant. The development of the MCMV cosmid and plasmidsystem was prompted because of this problem. The constructionof specific mutants in the M80 gene is encumbered by the arrangementof adjacent genes. Specifically, the initiation codon of the M80ORF overlaps with the initiation codon of the upstream adjacentM79 ORF, whereas the poly(A) signals of M80 overlap with thoseof the downstream M82 ORF (31). Although we placed a $beta$ -galactosidaseexpression cassette between duplicated poly(A) signals for M80and M82, we were still unable to recover a legitimate recombinantvirus (unpublishedobservations).

The construction of mutant herpesviruses has also been facilitated by the isolation of the respective genomes as infectiousBACs (2, 4, 27, 35). A limitation of the first-describedBAC MCMVs was their inability to replicate in vivo, but a laterversion deletes incorporated BAC sequences upon repeated passagein vitro, yielding virus that replicates normally in vivo (38).The BAC CMVs promise to be a great utility in the identificationof genes necessary for virus replication (for example, see reference5). However, construction of specific mutants requires themanipulation of E. coli recombination genetics to recover thedesired product of allelic exchange between the wild-type BACand a plasmid bearing the mutant gene of interest (30). Althoughelegant in design, manipulation of BACs is not readily masteredin most virologylaboratories.

In comparison to other methods of constructing specific MCMV mutants, the cosmid and plasmid system has the major advantagethat only the desired recombinant virus is produced. This allowsthe rapid isolation of different mutant strains using standardmolecular techniques once a target gene is isolated and appropriatelyconfigured in a cosmid and plasmid set. This system is designedto complement existing methods of mutant virus construction andwill be of use in ongoing studies of MCMV replication andpathogenesis.

	ACKNOWLEDGMENTS

We are grateful to our colleagues Greg Chinchar, Carol Wu, Paul Hippenmeyer, and Ed Mocarski for critical reading of themanuscript.

This work was supported by Monsanto grant MON-99-018, University of Missouri Research Board grant RB-98-144, and the Universityof Missouri College of Veterinary Medicine, Committee on Researchgrant COR FY 98/99.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, University of Mississippi Medical Center, 2500 N. StateSt., Jackson, MS 39216-4505. Phone: (601) 984-1705. Fax: (601)984-1708. E-mail: bholwerda{at}microbio.umsmed.edu.

Present address: Eli Lilly & Co., Indianapolis, IN46285.

Veterinary Biomedical Sciences, College of Veterinary Medicine, University of Missouri, Columbia, MO65211.

^§ Present address: Department of Microbiology, University of Mississippi Medical Center, Jackson, MS39216.

St. Louis University Health Sciences Center, St. Louis MO63104.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Alting-Mees, M. A., and J. M. Short. 1989. pBluescript II: gene mapping vectors. Nucleic Acids Res. 17:9494[Free Full Text].

2. Angulo, A., M. Messerle, U. H. Koszinowski, and P. Ghazal. 1998. Enhancer requirement for murine cytomegalovirus growth and genetic complementation by the human cytomegalovirus enhancer. J. Virol. 72:8502-8509[Abstract/Free Full Text].

3. Billstrom, M. A., G. L. Johnson, N. J. Avdi, and G. S. Worthen. 1998. Intracellular signaling by the chemokine receptor US28 during human cytomegalovirus infection. J. Virol. 72:5535-5544[Abstract/Free Full Text].

4. Borst, E. M., G. Hahn, U. H. Koszinowski, and M. Messerle. 1999. Cloning of the human cytomegalovirus (HCMV) genome as an infectious bacterial artificial chromosome in Escherichia coli: a new approach for construction of HCMV mutants. J. Virol. 73:8320-8329[Abstract/Free Full Text].

5. Brune, W., C. Menard, U. Hobom, S. Odenbreit, M. Messerle, and U. H. Koszinowski. 1999. Rapid identification of essential and nonessential herpesvirus genes by direct transposon mutagenesis. Nat. Biotechnol. 17:360-364[CrossRef][Medline].

6. Chang, A. C., and S. N. Cohen. 1978. Construction and characterization of amplifiable multicopy DNA cloning vehicles derived from the P15A cryptic miniplasmid. J. Bacteriol. 134:1141-1156[Abstract/Free Full Text].

7. Chee, M. S., A. T. Bankier, S. Beck, R. Bohni, C. M. Brown, R. Cerny, T. Horsnell, C. A. Hutchinson III, T. Kouzarides, J. A. Matignetti, E. Preddie, S. C. Satchwell, P. Tomlinson, K. M. Weston, and B. G. Barrel. 1990. Analysis of the protein-coding content of the sequence of human cytomegalovirus strain AD169. Curr. Top. Microbiol. Immunol. 154:125-169[Medline].

8. Chee, M. S., S. C. Satchwell, E. Preddie, K. M. Weston, and B. G. Barrell. 1990. Human cytomegalovirus encodes three G protein-coupled receptor homologues. Nature 344:774-777[CrossRef][Medline].

9. Cihlar, T., M. D. Fuller, and J. M. Cherrington. 1998. Characterization of drug resistance-associated mutations in the human cytomegalovirus DNA polymerase gene by using recombinant mutant viruses generated from overlapping DNA fragments. J. Virol. 72:5927-5936[Abstract/Free Full Text].

10. Cohen, J. I., and K. E. Seidel. 1993. Generation of varicella-zoster virus (VZV) and viral mutants from cosmid DNAs: VZV thymidylate synthetase is not essential for replication in vitro. Proc. Natl. Acad. Sci. USA 90:7376-7380[Abstract/Free Full Text].

11. Cunningham, C., and A. J. Davison. 1993. A cosmid-based system for constructing mutants of herpes simplex virus type 1. Virology 197:116-124[CrossRef][Medline].

12. Davis-Poynter, N. J., D. M. Lynch, H. Vally, G. R. Shellam, W. D. Rawlinson, B. G. Barrell, and H. E. Farrell. 1997. Identification and characterization of a G protein-coupled receptor homolog encoded by murine cytomegalovirus. J. Virol. 71:1521-1529[Abstract].

13. Ebeling, A., G. M. Keil, E. Knust, and U. H. Koszinowski. 1983. Molecular cloning and physical mapping of murine cytomegalovirus DNA. J. Virol. 47:421-433[Abstract/Free Full Text].

14. Feinberg, A. P., and B. Vogelstein. 1983. A technique for radiolabeling DNA restriction endonuclease fragments to high specific activity. Anal. Biochem. 132:6-13[CrossRef][Medline].

15. Frost, E., and J. Williams. 1978. Mapping temperature-sensitive and host-range mutations of adenovirus type 5 by marker rescue. Virology 91:39-50[CrossRef][Medline].

16. Graham, F. L., and A. J. Van der Eb. 1973. Transformation of rat cells by DNA of human adenovirus 5. Virology 54:536-539[CrossRef][Medline].

17. Graham, F. L., G. Veldhuisen, and N. M. Wilkie. 1973. Infectious herpesvirus DNA. Nat. New Biol. 245:265-266[Medline].

18. Ho, M. 1991. Cytomegalovirus: biology and infection. Plenum Medical Book Company, New York, N.Y.

19. Ish-Horowicz, D., and J. F. Burke. 1981. Rapid and efficient cosmid cloning. Nucleic Acids Res. 9:2989-2998[Abstract/Free Full Text].

20. Jacob, R. J., L. S. Morse, and B. Roizman. 1979. Anatomy of herpes simplex virus DNA. XII. Accumulation of head-to-tail concatemers in nuclei of infected cells and their role in the generation of the four isomeric arrangements of viral DNA. J. Virol. 29:448-457[Abstract/Free Full Text].

21. Jacob, R. J., and B. Roizman. 1977. Anatomy of herpes simplex virus DNA VIII. Properties of the replicating DNA. J. Virol. 23:394-411[Abstract/Free Full Text].

22. Kemble, G., G. Duke, R. Winter, and R. Spaete. 1996. Defined large-scale alterations of the human cytomegalovirus genome constructed by cotransfection of overlapping cosmids. J. Virol. 70:2044-2048[Abstract].

23. Laithier, M., and P. Sheldrick. 1975. Influence of DEAE-dextran treatment and cellular "age" on infection by herpes simplex virus DNA, p. 85-90. In P. Buccalossi, U. Veronesi, and N. Coscinelli (ed.), Chemical and viral carcinogenesis 2. IARC Scientific Publications, Amsterdam, The Netherlands.

24. Liu, F. Y., and B. Roizman. 1991. The herpes simplex virus 1 gene encoding a protease also contains within its coding domain the gene encoding the more abundant substrate. J. Virol. 65:5149-5156[Abstract/Free Full Text].

25. Loutsch, J. M., N. J. Galvin, M. L. Bryant, and B. C. Holwerda. 1994. Cloning and sequence analysis of murine cytomegalovirus protease and capsid assembly protein genes. Biochem. Biophys. Res. Commun. 203:472-478[CrossRef][Medline].

26. Mercer, J. A., J. R. Marks, and D. H. Spector. 1983. Molecular cloning and restriction endonuclease mapping of the murine cytomegalovirus genome (Smith strain). Virology 129:94-106[CrossRef][Medline].

27. Messerle, M., I. Crnkovic, W. Hammerschmidt, H. Ziegler, and U. H. Koszinowski. 1997. Cloning and mutagenesis of a herpesvirus genome as an infectious bacterial artificial chromosome. Proc. Natl. Acad. Sci. USA 94:14759-14763[Abstract/Free Full Text].

28. Mocarski, E. S., Jr., and G. W. Kemble. 1996. Recombinant cytomegaloviruses for study of replication and pathogenesis. Intervirology 39:320-30[Medline].

29. Mocarski, E. S., L. E. Post, and B. Roizman. 1980. Molecular engineering of the herpes simplex virus genome: insertion of a second L-S junction into the genome causes additional genome inversions. Cell 22:243-55[CrossRef][Medline].

30. O'Connor, M., M. Peifer, and W. Bender. 1989. Construction of large DNA segments in Escherichia coli. Science 244:1307-1312[Abstract/Free Full Text].

31. Rawlinson, W. D., H. E. Farrell, and B. G. Barrell. 1996. Analysis of the complete DNA sequence of murine cytomegalovirus. J. Virol. 70:8833-8849[Abstract].

32. Register, R. B., and J. A. Shafer. 1996. A facile system for construction of HSV-1 variants: site-directed mutation of the UL26 protease gene in HSV-1. J. Virol. Methods 57:181-193[CrossRef][Medline].

33. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Press, Cold Spring Harbor, N.Y.

34. Short, J. M., J. M. Fernandez, J. A. Sorge, and W. D. Huse. 1988. Lambda ZAP: a bacteriophage lambda expression vector with in vivo excision properties. Nucleic Acids Res. 16:7583-7600[Abstract/Free Full Text].

35. Smith, G. A., and L. W. Enquist. 1999. Construction and transposon mutagenesis in Escherichia coli of a full-length infectious clone of pseudorabies virus, an alphaherpesvirus. J. Virol. 73:6405-6414[Abstract/Free Full Text].

36. Tomkinson, B., E. Robertson, R. Yalamanchili, R. Longnecker, and E. Kieff. 1993. Epstein-Barr virus recombinants from overlapping cosmid fragments. J. Virol. 67:7298-7306[Abstract/Free Full Text].

37. Van Zijl, M., W. Quint, J. Briaire, T. de Rover, A. Gielkens, and A. Berns. 1988. Regeneration of herpesviruses from molecularly cloned subgenomic fragments. J. Virol. 62:2191-2195[Abstract/Free Full Text].

38. Wagner, M., S. Jonjic, U. H. Koszinowski, and M. Messerle. 1999. Systematic excision of vector sequences from the BAC-cloned herpesvirus genome during virus reconstitution. J. Virol. 73:7056-7060[Abstract/Free Full Text].

39. Welch, A. R., A. S. Woods, L. M. McNally, R. J. Cotter, and W. Gibson. 1991. A herpesvirus maturational proteinase, assemblin: identification of its gene, putative active site domain, and cleavage site. Proc. Natl. Acad. Sci. USA 88:10792-10796[Abstract/Free Full Text].

40. Yanisch-Perron, C., J. Vieira, and J. Messing. 1985. Improved M13 phage cloning vectors and host strains: nucleotide sequences of the M13mp18 and pUC19 vectors. Gene 33:103-119[CrossRef][Medline].

41. Zoller, M. J., and M. Smith. 1983. Oligonucleotide-directed mutagenesis of DNA fragments cloned into M13 vectors. Methods Enzymol. 100:468-500[Medline].

42. Zoller, M. J., and M. Smith. 1982. Oligonucleotide-directed mutagenesis using M13-derived vectors: an efficient and general procedure for the production of point mutations in any fragment of DNA. Nucleic Acids Res. 10:6487-6500[Abstract/Free Full Text].

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1.	Alting-Mees, M. A., and J. M. Short. 1989. pBluescript II: gene mapping vectors. Nucleic Acids Res. 17:9494[Free Full Text].
2.	Angulo, A., M. Messerle, U. H. Koszinowski, and P. Ghazal. 1998. Enhancer requirement for murine cytomegalovirus growth and genetic complementation by the human cytomegalovirus enhancer. J. Virol. 72:8502-8509[Abstract/Free Full Text].
3.	Billstrom, M. A., G. L. Johnson, N. J. Avdi, and G. S. Worthen. 1998. Intracellular signaling by the chemokine receptor US28 during human cytomegalovirus infection. J. Virol. 72:5535-5544[Abstract/Free Full Text].
4.	Borst, E. M., G. Hahn, U. H. Koszinowski, and M. Messerle. 1999. Cloning of the human cytomegalovirus (HCMV) genome as an infectious bacterial artificial chromosome in Escherichia coli: a new approach for construction of HCMV mutants. J. Virol. 73:8320-8329[Abstract/Free Full Text].
5.	Brune, W., C. Menard, U. Hobom, S. Odenbreit, M. Messerle, and U. H. Koszinowski. 1999. Rapid identification of essential and nonessential herpesvirus genes by direct transposon mutagenesis. Nat. Biotechnol. 17:360-364[CrossRef][Medline].
6.	Chang, A. C., and S. N. Cohen. 1978. Construction and characterization of amplifiable multicopy DNA cloning vehicles derived from the P15A cryptic miniplasmid. J. Bacteriol. 134:1141-1156[Abstract/Free Full Text].
7.	Chee, M. S., A. T. Bankier, S. Beck, R. Bohni, C. M. Brown, R. Cerny, T. Horsnell, C. A. Hutchinson III, T. Kouzarides, J. A. Matignetti, E. Preddie, S. C. Satchwell, P. Tomlinson, K. M. Weston, and B. G. Barrel. 1990. Analysis of the protein-coding content of the sequence of human cytomegalovirus strain AD169. Curr. Top. Microbiol. Immunol. 154:125-169[Medline].
8.	Chee, M. S., S. C. Satchwell, E. Preddie, K. M. Weston, and B. G. Barrell. 1990. Human cytomegalovirus encodes three G protein-coupled receptor homologues. Nature 344:774-777[CrossRef][Medline].
9.	Cihlar, T., M. D. Fuller, and J. M. Cherrington. 1998. Characterization of drug resistance-associated mutations in the human cytomegalovirus DNA polymerase gene by using recombinant mutant viruses generated from overlapping DNA fragments. J. Virol. 72:5927-5936[Abstract/Free Full Text].
10.	Cohen, J. I., and K. E. Seidel. 1993. Generation of varicella-zoster virus (VZV) and viral mutants from cosmid DNAs: VZV thymidylate synthetase is not essential for replication in vitro. Proc. Natl. Acad. Sci. USA 90:7376-7380[Abstract/Free Full Text].
11.	Cunningham, C., and A. J. Davison. 1993. A cosmid-based system for constructing mutants of herpes simplex virus type 1. Virology 197:116-124[CrossRef][Medline].
12.	Davis-Poynter, N. J., D. M. Lynch, H. Vally, G. R. Shellam, W. D. Rawlinson, B. G. Barrell, and H. E. Farrell. 1997. Identification and characterization of a G protein-coupled receptor homolog encoded by murine cytomegalovirus. J. Virol. 71:1521-1529[Abstract].
13.	Ebeling, A., G. M. Keil, E. Knust, and U. H. Koszinowski. 1983. Molecular cloning and physical mapping of murine cytomegalovirus DNA. J. Virol. 47:421-433[Abstract/Free Full Text].
14.	Feinberg, A. P., and B. Vogelstein. 1983. A technique for radiolabeling DNA restriction endonuclease fragments to high specific activity. Anal. Biochem. 132:6-13[CrossRef][Medline].
15.	Frost, E., and J. Williams. 1978. Mapping temperature-sensitive and host-range mutations of adenovirus type 5 by marker rescue. Virology 91:39-50[CrossRef][Medline].
16.	Graham, F. L., and A. J. Van der Eb. 1973. Transformation of rat cells by DNA of human adenovirus 5. Virology 54:536-539[CrossRef][Medline].
17.	Graham, F. L., G. Veldhuisen, and N. M. Wilkie. 1973. Infectious herpesvirus DNA. Nat. New Biol. 245:265-266[Medline].
18.	Ho, M. 1991. Cytomegalovirus: biology and infection. Plenum Medical Book Company, New York, N.Y.
19.	Ish-Horowicz, D., and J. F. Burke. 1981. Rapid and efficient cosmid cloning. Nucleic Acids Res. 9:2989-2998[Abstract/Free Full Text].
20.	Jacob, R. J., L. S. Morse, and B. Roizman. 1979. Anatomy of herpes simplex virus DNA. XII. Accumulation of head-to-tail concatemers in nuclei of infected cells and their role in the generation of the four isomeric arrangements of viral DNA. J. Virol. 29:448-457[Abstract/Free Full Text].
21.	Jacob, R. J., and B. Roizman. 1977. Anatomy of herpes simplex virus DNA VIII. Properties of the replicating DNA. J. Virol. 23:394-411[Abstract/Free Full Text].
22.	Kemble, G., G. Duke, R. Winter, and R. Spaete. 1996. Defined large-scale alterations of the human cytomegalovirus genome constructed by cotransfection of overlapping cosmids. J. Virol. 70:2044-2048[Abstract].
23.	Laithier, M., and P. Sheldrick. 1975. Influence of DEAE-dextran treatment and cellular "age" on infection by herpes simplex virus DNA, p. 85-90. In P. Buccalossi, U. Veronesi, and N. Coscinelli (ed.), Chemical and viral carcinogenesis 2. IARC Scientific Publications, Amsterdam, The Netherlands.
24.	Liu, F. Y., and B. Roizman. 1991. The herpes simplex virus 1 gene encoding a protease also contains within its coding domain the gene encoding the more abundant substrate. J. Virol. 65:5149-5156[Abstract/Free Full Text].
25.	Loutsch, J. M., N. J. Galvin, M. L. Bryant, and B. C. Holwerda. 1994. Cloning and sequence analysis of murine cytomegalovirus protease and capsid assembly protein genes. Biochem. Biophys. Res. Commun. 203:472-478[CrossRef][Medline].
26.	Mercer, J. A., J. R. Marks, and D. H. Spector. 1983. Molecular cloning and restriction endonuclease mapping of the murine cytomegalovirus genome (Smith strain). Virology 129:94-106[CrossRef][Medline].
27.	Messerle, M., I. Crnkovic, W. Hammerschmidt, H. Ziegler, and U. H. Koszinowski. 1997. Cloning and mutagenesis of a herpesvirus genome as an infectious bacterial artificial chromosome. Proc. Natl. Acad. Sci. USA 94:14759-14763[Abstract/Free Full Text].
28.	Mocarski, E. S., Jr., and G. W. Kemble. 1996. Recombinant cytomegaloviruses for study of replication and pathogenesis. Intervirology 39:320-30[Medline].
29.	Mocarski, E. S., L. E. Post, and B. Roizman. 1980. Molecular engineering of the herpes simplex virus genome: insertion of a second L-S junction into the genome causes additional genome inversions. Cell 22:243-55[CrossRef][Medline].
30.	O'Connor, M., M. Peifer, and W. Bender. 1989. Construction of large DNA segments in Escherichia coli. Science 244:1307-1312[Abstract/Free Full Text].
31.	Rawlinson, W. D., H. E. Farrell, and B. G. Barrell. 1996. Analysis of the complete DNA sequence of murine cytomegalovirus. J. Virol. 70:8833-8849[Abstract].
32.	Register, R. B., and J. A. Shafer. 1996. A facile system for construction of HSV-1 variants: site-directed mutation of the UL26 protease gene in HSV-1. J. Virol. Methods 57:181-193[CrossRef][Medline].
33.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Press, Cold Spring Harbor, N.Y.
34.	Short, J. M., J. M. Fernandez, J. A. Sorge, and W. D. Huse. 1988. Lambda ZAP: a bacteriophage lambda expression vector with in vivo excision properties. Nucleic Acids Res. 16:7583-7600[Abstract/Free Full Text].
35.	Smith, G. A., and L. W. Enquist. 1999. Construction and transposon mutagenesis in Escherichia coli of a full-length infectious clone of pseudorabies virus, an alphaherpesvirus. J. Virol. 73:6405-6414[Abstract/Free Full Text].
36.	Tomkinson, B., E. Robertson, R. Yalamanchili, R. Longnecker, and E. Kieff. 1993. Epstein-Barr virus recombinants from overlapping cosmid fragments. J. Virol. 67:7298-7306[Abstract/Free Full Text].
37.	Van Zijl, M., W. Quint, J. Briaire, T. de Rover, A. Gielkens, and A. Berns. 1988. Regeneration of herpesviruses from molecularly cloned subgenomic fragments. J. Virol. 62:2191-2195[Abstract/Free Full Text].
38.	Wagner, M., S. Jonjic, U. H. Koszinowski, and M. Messerle. 1999. Systematic excision of vector sequences from the BAC-cloned herpesvirus genome during virus reconstitution. J. Virol. 73:7056-7060[Abstract/Free Full Text].
39.	Welch, A. R., A. S. Woods, L. M. McNally, R. J. Cotter, and W. Gibson. 1991. A herpesvirus maturational proteinase, assemblin: identification of its gene, putative active site domain, and cleavage site. Proc. Natl. Acad. Sci. USA 88:10792-10796[Abstract/Free Full Text].
40.	Yanisch-Perron, C., J. Vieira, and J. Messing. 1985. Improved M13 phage cloning vectors and host strains: nucleotide sequences of the M13mp18 and pUC19 vectors. Gene 33:103-119[CrossRef][Medline].
41.	Zoller, M. J., and M. Smith. 1983. Oligonucleotide-directed mutagenesis of DNA fragments cloned into M13 vectors. Methods Enzymol. 100:468-500[Medline].
42.	Zoller, M. J., and M. Smith. 1982. Oligonucleotide-directed mutagenesis using M13-derived vectors: an efficient and general procedure for the production of point mutations in any fragment of DNA. Nucleic Acids Res. 10:6487-6500[Abstract/Free Full Text].