In Vitro and In Vivo Characterization of a Murine Cytomegalovirus with a Transposon Insertional Mutation at Open Reading Frame M43

doi:10.1128/JVI.74.20.9488-9497.2000

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Journal of Virology, October 2000, p. 9488-9497, Vol. 74, No. 20
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

In Vitro and In Vivo Characterization of a Murine Cytomegalovirus with a Transposon Insertional Mutation at Open Reading Frame M43

Jianqiao Xiao, Tuong Tong, Xiaoyan Zhan, Erik Haghjoo, and Fenyong Liu^*

Program in Infectious Diseases and Immunity, School of Public Health, University of California, Berkeley, California 94720

Received 7 June 2000/Accepted 25 July 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We have recently generated a pool of murine cytomegalovirus (MCMV) mutants by using a Tn3-based transposon mutagenesis approach.In this study, one of the MCMV mutants, RvM43, which containedthe transposon inserted in open reading frame M43, was characterized.Our results provide the first direct evidence to suggest thatM43 is not essential for viral replication in vitro in NIH 3T3cells. Moreover, RvM43 exhibited a titer similar to that of thewild-type virus in the lungs, livers, spleens, and kidneys ofboth BALB/c and SCID mice and was as virulent as the wild-typevirus in killing SCID mice that had been intraperitoneally infectedwith the viruses. In contrast, titers of the mutant virus in thesalivary glands of the infected animals at 21 days postinfectionwere significantly (100 to 1,000-fold) lower than those of thewild-type virus and a rescued virus that restored the M43 regionand its expression. Thus, M43 appears to be not essential forviral growth in vivo in the lungs, livers, spleens, and kidneysof infected animals and is also dispensable for virulence in killingSCID mice. Moreover, our results suggest that M43 is an MCMV determinantfor growth in the salivary glands. Studies of viral genes requiredfor replication in the salivary glands are important in understandingthe mechanism of viral tropism for the salivary glands and sheddingin saliva, which is believed to be one of the major routes ofCMV transmission among healthy humanpopulations.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Human cytomegalovirus (HCMV) is a serious opportunistic pathogen for both newborn and immunocompromised individuals (2,26). It is the leading viral cause of birth defects, affectingabout 7,000 infants yearly in the United States alone (13).Moreover, nearly 10% of the deaths of AIDS patients in 1992 wereattributed to HCMV diseases (38, 39). Meanwhile, HCMV infectioncontinues to be a major cause of morbidity and mortality in bonemarrow and solid organ transplant recipients (2, 26). Understandingthe mechanism of HCMV pathogenesis and the function of viral genesin HCMV-related diseases is necessary for developing new drugsand novel strategies for the treatment and prevention of HCMVinfections.

HCMV is a betaherpesvirus with a genome of about 230 kb and a coding capacity of more than 220 open reading frames (6,26). HCMV propagates only in human cells and grows slowly dueto a long lytic replication cycle. Strict species specificityhas prevented the study of HCMV in any animal model. Related viruses,such as murine CMV (MCMV), must be used to provide insight intothe tissue tropism, virulence, and latency ofHCMV.

MCMV provides an excellent model for studying the biology of CMV infection. MCMV offers several advantages, including rapidgrowth, the availability of a reliable animal model, and the factthat it has sequence homology with HCMV (2, 17, 19, 26).Infection of mice by MCMV resembles in many ways its human counterpartwith respect to transmission, pathogenesis during acute infection,establishment of latency, and reactivation after immunosuppression,transfusion, or transplantation (2, 17, 19, 26). Forexample, tropism for the salivary glands is believed to be importantin the infection of both HCMV and MCMV (2, 26). Persistentand recurrent shedding of viral particles from the salivary glandsappears to be the principal means by which these viruses spreadin the population. The MCMV genome is also 230 kb long and ispredicted to encode more than 170 open reading frames, 78 of whichhave extensive homology to those of HCMV (6, 34). A completeunderstanding of the biology of MCMV and the function of its genesmay provide insight into the pathogenesis ofHCMV.

One of the most powerful approaches for studying the function of virus-encoded genes is to introduce mutations into the viralgenome and to screen viral mutants in both tissue culture andanimals for possible growth defects in vitro and in vivo. Theconstruction of herpesvirus mutants by using site-directed homologousrecombination and transposon-mediated insertional mutagenesishas been reported (18, 27, 28, 33, 36, 47), as havemethods using overlapping cosmid DNA fragments to generate mutantsof HCMV and other herpesviruses (8, 9, 20, 43, 44).More recently, the MCMV genome as well as the genomes of otherherpesviruses have been cloned into a bacterial artificial chromosome(BAC), and viral mutants were successfully generated from theBAC-based viral genome by a bacterial mutagenesis procedure (3,12, 25, 37, 40-42, 46). It has been shown that the BACsequence in a BAC-based pseudorabies virus does not affect viralpathogenesis in vivo in animals (40, 41). Moreover, two differentapproaches to excise the BAC sequence from the viral genome havebeen described (41, 46). These studies have greatly facilitatedthe identification of the functions of viral genes in tissue cultureand inanimals.

Many of the CMV genes have been found to be dispensable for growth in cultured cells. Their presence in the viral genome indicatesthat they are likely needed to perform functions involved onlyin modulating the interactions between the virus and its humanor animal hosts. For example, HCMV US11, a nonessential protein,functions to downregulate the expression and presentation of majorhistocompatibility complex class I molecules (48). Meanwhile,MCMV open reading frame m133, which is also called salivary glandgene 1 (sgg1) and is dispensable for viral replication, is a determinantfor MCMV replication in salivary glands in vivo (21, 24).Thus, studies of viral mutants carrying mutations in genes foundto be dispensable in tissue culture are valuable for an understandingof gene function in viral pathogenesis and virus-host interactions,including tissue tropism andvirulence.

We have previously generated a pool of MCMV mutants using a Tn3 transposon-mediated shuttle mutagenesis system (49, 50).In this approach, the transposon is randomly inserted into theMCMV genomic DNA fragments in a plasmid library in Escherichiacoli. Regions bearing an insertion mutation are then transferredto the MCMV genome by cotransfecting the plasmid library and purifiedMCMV genomic DNA into NIH 3T3 cells. Characterization of one ofthe viral mutants (e.g., Rvm09) in NIH 3T3 cells and in both BALB/cand SCID mice indicated that the presence of the transposon sequenceper se in the viral genome does not significantly affect viralreplication and growth in vitro and in vivo (50). In the presentstudy, we have characterized an MCMV mutant, RvM43, which containsa transposon insertion in open reading frame M43. The functionof M43 in viral replication and pathogenesis is unknown. Indeed,this open reading frame has not been extensively characterizedtranscriptionally or translationally. Our results provide thefirst direct evidence to suggest that M43 is not essential forviral replication in vitro in tissue culture. Moreover, RvM43replicated as well as the wild-type virus in the lungs, livers,spleens, and kidneys of both the BALB/c and SCID mice and wasas virulent as the wild-type virus in killing SCID mice that hadbeen intraperitoneally infected with the viruses. In contrast,at 21 days postinfection, titers of the mutant virus were at least100- and 1,000-fold lower than those of the wild-type virus inthe salivary glands of BALB/c and SCID mice, respectively. Theseresults suggest that M43 functions as a viral determinant forreplication in the salivaryglands.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and viruses. Mouse NIH 3T3 cells and STO cells and the wild-type Smith strain of MCMV were obtained from the American Type Culture Collection,Manassas, Va. Cells were maintained in complete growth mediumconsisting of Dulbecco's modified Eagle medium (DMEM) supplementedwith 10% NuSerum (Becton Dickenson, Mountain View, Calif.), aminoacids, and antibiotics (each from a stock solution purchased fromLife Technologies Inc. [Gibco BRL, Grand Island, N.Y.]) (49).The wild-type Smith strain, mutant RvM43, and the rescued virusRqM43 were propagated in NIH 3T3 cells as described previously(49).

Construction of an MCMV DNA subclone pool, transposon shuttle mutagenesis, and generation of MCMV recombinant mutants. Isolation of viral genomic DNA, construction of an MCMV genomic subclone pool, and transposon-based shuttle mutagenesis togenerate a pool of MCMV DNA fragments containing a transposoninsertion were performed as described by Zhan et al. (49). Togenerate a pool of MCMV mutants that contained the transposonsequence, intact MCMV genomic DNAs and plasmid DNAs containingthe Tn3-guanine phosphorlbosyltransferase gene (gpt)-MCMV fragmentswere cotransfected into NIH 3T3 cells using a calcium phosphateprecipitation protocol (Gibco BRL). The recombinant MCMV mutantswere selected in the presence of mycophenolic acid (25 µg/ml;Gibco BRL) and xanthine (50 µg/ml; Sigma, St. Louis, Mo.) andthen plaque purified six times as described previously (49).To confirm the integration of the transposon in the viral genomeand to identify the genes that were disrupted by the transposoninsertion, viral DNA was purified and directly sequenced usingthe primer FL110PRIM (5'-GCAGGATCCTATCCATATGAC-3') and an fmolcycle sequencing kit (Promega, Inc., Madison, Wis.).

To construct the rescued virus RqM43, the full-length genomic DNA of RvM43 was isolated from infected cells as described previously(49). The DNA sequence that contained the coding sequence ofM43 was generated by PCR using the viral genomic DNA as the template,the 5' primer M43-sense (5'-CATGCCTGGCGGACTGGAAA-3'), and the3' primer M43-antisense (5'-TCATAGTTCCGGTTCGGATG-3'). The PCRproduct that contained the M43 coding sequence (1 to 3 µg) andthe full-length intact RvM43 viral genomic DNA (8 to 12 µg) weresubsequently cotransfected into mouse STO cells using a calciumphosphate precipitation protocol (Gibco BRL). The recombinantvirus was selected in STO cells in the presence of 6-thioguanine(25 µg/ml; Sigma) and purified by six rounds of amplificationand plaque purification as described previously (14). For eachcotransfection, several viral plaques were picked and expanded.Viral stocks were prepared by growing the viruses in T-150 flasksof NIH 3T3cells.

Southern and Northern analyses of recombinant viruses. Viral genomic DNA was purified from NIH 3T3 cells infected with the viruses as described previously (45, 49). Briefly,cells that exhibited 100% cytopathic effect were washed with phosphate-bufferedsaline and then subjected to proteolysis with a solution containingsodium dodecyl sulfate and proteinase K. The genomic DNA was purifiedby extraction with phenol-chloroform followed by precipitationwith 2-propanol. The DNA was then digested with HindIII or NotI,separated on agarose gels (0.8%), transferred to Zeta-Probe nylonmembranes (Bio-Rad, Hercules, Ca), and hybridized with ³²P-labeled DNA probes specific for both the transposon and theMCMV sequences. A STORM 840 PhosphorImager was used to analyzetheblots.

For Northern blot analysis, cells were infected with viruses at a multiplicity of infection (MOI) of 5 and harvested at differenttime points postinfection. In the experiments to assay the expressionof immediate-early (IE) transcripts, cells were pretreated withcycloheximide (100 µg/ml; Sigma), then infected with viruses,and harvested at 6 h postinfection. Total cytoplasmic RNA wasisolated from NIH 3T3 cells infected with the viruses as describedpreviously (22). Viral RNAs were separated in a 1% agarose gelthat contained formaldehyde, transferred to a nitrocellulose membrane,hybridized with the ³²P-radiolabeled DNA probes that contained specific MCMV sequences,and finally analyzed with a STORM 840 PhosphorImager. The DNAprobes used for Northern analyses were generated by PCR usingviral DNA as the template and radiolabeled with a random primersynthesis kit in the presence of [³²P]dCTP (Boehringer Mannheim, Indianapolis, Ind.). The 5' and 3'PCR primers used for construction of the DNA probe for Northernanalysis were M43/1 (5'-TACACGTTGGCTGTTACCGCTAGGT-3') and M43/2(5'-TCACCGTCGGTTCGACGTTCTCGTA-3'),respectively.

Analysis of growth of the viruses in vitro. The growth kinetics of the viruses was determined as described previously (50). Briefly, NIH 3T3 cells grown to 50 to 60%confluence were inoculated with virus at an MOI of either 0.5or 5. At 0, 1, 2, 4, and 7 days postinfection, the infected cellstogether with medium were harvested, and an equal volume of 10%skim milk was added before sonication. Virus titer was determinedby plaque assays in NIH 3T3 cells. Viral titers reported wereaverages from triplicateexperiments.

Analysis of growth of the viruses in animals. Four-week-old male BALB/c-Byj mice (Jackson Laboratory, Bar Harbor, Maine) or 6-week-old CB17 SCID mice (National Cancer Institute,Bethesda, Md.) were infected intraperitoneally with 10⁴ PFU of each virus. The animals were sacrificed at 1, 3, 7, 10,14, and 21 days postinoculation. For each time point, at leastthree animals were used as a group and infected with the samevirus. The salivary glands, lungs, spleens, livers, and kidneyswere harvested and sonicated as a 10% (wt/vol) suspension in a1:1 mixture of DMEM and skim milk. The sonicates were stored at $-$ 80°C until plaque assays wereperformed.

Viruses harvested from the mice were titered on NIH 3T3 cells in six-well tissue culture plates (Corning Inc., Corning, N.Y.).Briefly, cells were first infected with the viruses at 10-foldserial dilutions. After 2 h of incubation with the homogenatesdiluted in 1 ml of complete medium at 37°C with 5% CO₂, the cellswere overlaid with fresh complete medium containing 1% agaroseand cultured for 3 to 4 days before the plaques were counted underan inverted microscope. Viral titers were recorded as PFU permilliliter of organ homogenates. Each sample was titered in triplicate.The limit of virus detection in the organ homogenates was 10 PFU/mlof the sonicated mixture. Those samples that were negative ata 10¹ dilution were assigned a titer of 10 (10¹) PFU/ml.

Virulence assays. Virulence of the viruses was studied by determining the mortality of the animals infected with the Smith strain, RvM43, orRqM43. The CB17 SCID mice (five animals per group) were infectedintraperitoneally with 10⁴ PFU of each virus. The animals were observed twice daily; mortalityof the infected animals was monitored for at least 28 days postinfection,and the survival rates weredetermined.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Isolation of an MCMV mutant containing the transposon insertion at open reading frame M43. We have constructed a pool of MCMV mutants using an E. coli Tn3-based transposon mutagenesis system (49). Figure 1A showsthe structure of the transposon used to generate MCMV mutants.The transposon contains the gpt expression cassette (which includesthe gpt coding sequence driven by a promoter and a transcriptiontermination signal) and an additional transcription terminationsite to allow selection of mutant MCMV in mammalian cells andtranscription truncation of the disrupted gene (49). Since thegpt expression cassette and the additional poly(A) signal in thetransposon are in opposite orientations, the expression of nearbygenes that may share a common poly(A) signal with the target genewould not be disrupted (Fig. 1A). In our mutagenesis procedure,an MCMV genomic library containing a randomly inserted transposonin each viral DNA fragment was first generated using a shuttlemutagenesis method as described previously (49). Such a poolof MCMV genomic fragments containing randomly inserted Tn3-gptsequence was then cotransfected with the full-length genomic DNAof the wild-type virus (Smith strain) into mouse NIH 3T3 cellsin which homologous recombination occurred. Cells that harboredthe progeny viruses expressing the gpt gene were selected forgrowth in the presence of mycophenolic acid and xanthine (14,30, 45). After multiple rounds of selection and plaque purification,we isolated individual recombinant viruses and determined thelocation of the inserted transposon by directly sequencing thegenomic DNA of the recombinants. One of the recombinant viruseswas further characterized and is reported here. This viral mutant,designated RvM43, contains the transposon sequence inserted withinopen reading frame M43 (Fig. 1B). Sequencing analyses of the junctionbetween the transposon and the viral sequence revealed that thetransposon in RvM43 is located at nucleotide position 56204 (thecodon for amino acid 313 of M43), with reference to the genomesequence of the wild-type Smith strain (34) (Fig. 1B and datanot shown).

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FIG. 1. (A) Schematic representation of the structure of the transposon construct used for mutagenesis. The gpt expression cassette includes the gpt coding sequence driven by a promoter and a transcription termination signal. TR, terminal repeat; Tet, tetracycline resistance gene; poly(A), transcription termination signal. (B) Location of the transposon insertion in the recombinant virus. The transposon sequence is shown as a filled bar; the coding sequence of open reading frame M43 is represented by an open arrow. The orientation of the arrow represents the direction of the translation and transcription predicted based on the nucleotide sequence (34). The numbers represent sizes (in kilobases) of the DNA fragments of the viruses that were generated by digestion with HindIII (H) or NotI (N). (C) Southern analyses of the recombinant viruses. The DNA fractions were isolated from cells infected with the wild-type virus (WT), RvM43, or RqM43. The DNA samples (20 µg) were digested with either HindIII (H) or NotI (N), separated on 0.8% agarose gels, transferred to a Zeta-Probe membrane, and hybridized to a DNA probe. The probe used for the analyses was the plasmid that contained the MCMV DNA fragment inserted with the transposon sequence.

Southern analyses of RvM43 and rescued virus RqM43. The genomic structure of RvM43 and the location of the transposon insertion in the viral genome were examined by Southernblot hybridization with a DNA probe containing both the transposonand the viral sequence (Fig. 1B and C). When the viral DNA sampleswere digested with HindIII and subjected to Southern analyses,a small fragment of 1.8 kb representing the gpt gene was detected,indicating the presence of the transposon sequence within theviral genome (Fig. 1C, lane 1). This finding was further supportedby the results of Southern analyses of the RvM43 DNA samples digestedwith another restriction enzyme, NotI (Fig. 1C, lanes 4). In theseexperiments, the genomic fragments containing the transposon werefound to be larger than those of the wild-type virus by 3.6 kb,which is the size of the transposon (Fig. 1B andC).

The Southern blots also showed that the stocks of the mutant virus were pure and free of the wild-type strain since the hybridizingDNA fragments from the mutant did not comigrate with those ofthe wild-type Smith strain (Fig. 1C, lanes 1, 3, 4, and 6). Forexample, the hybridization patterns of the RvM43 and Smith strainDNAs digested with HindIII gave rise to three (20, 8.2, and 1.8kb) and one (26.4 kb) DNA band(s), respectively (Fig. 1C, lanes1 and 3). Meanwhile, the hybridized species (12.8 kb) of the NotI-digestedRvM43 DNA migrated differently from that (9.2 kb) of the wild-typeviral DNA digested with the same enzyme (Fig. 1C, lanes 4 and6). The sizes of the hybridized DNA fragments (Fig. 1C) were consistentwith the predicted digestion patterns of the recombinant virus,based on the MCMV genomic sequence (34) and the location ofthe transposon insertion in the viral genome as determined bysequence analysis (Fig. 1B). The restriction enzyme digestionpatterns of the regions of the mutant genomic DNA other than thetransposon insertional site appeared to be identical to thoseof the parental Smith strain, as indicated by ethidium bromidestaining of the digested DNAs (data not shown). This observationsuggests that regions of the viral genome other than that containingthe transposon insertion remained intact in this MCMVmutant.

To restore the M43 open reading frame, a rescued virus, designated RqM43, was derived from RvM43, using a protocol similarto the procedure used for construction of the viral mutant. ADNA fragment that contained the M43 coding region was cotransfectedwith the full-length RvM43 genomic DNA into mouse STO cells toallow homologous recombination to occur. The cells that harboredthe progeny viruses were allowed to grow in the presence of 6-thioguanine,which selects against gpt expression (14, 30). The rescuedvirus, RqM43, which did not express the gpt protein and no longercontained the transposon, was isolated after multiple rounds ofselection and plaquepurification.

Southern hybridization analyses with DNA probes containing the transposon and the viral sequence were used to examine thegenomic structure of RqM43 and determine if the M43 region wasrestored (Fig. 1B and C). Analysis of the RqM43 DNA samples digestedwith HindIII and NotI showed that the hybridized DNA fragmentsfor RqM43 were the same size as the hybridized fragments for theSmith strain but not those for RvM43. These results indicatedthat RqM43 did not contain the transposon sequence and the M43region was restored (Fig. 1C, lanes 2 and 5). Moreover, the restrictionenzyme digestion patterns of the regions of the rescued RqM43genomic DNA samples other than the M43 region appeared to be identicalto those of the parental RvM43, as indicated by ethidium bromidestaining of the digested DNAs (data not shown). This observationsuggests that the regions of the RqM43 genome other than the M43region remained intact and were identical to those of RvM43. Thus,RqM43 may represent a rescued virus forRvM43.

Expression of the transcripts from the viral M43 region in tissue culture. Transcription from the target M43 region is expected to be disrupted due to the presence of the two transcription terminationsignals within the transposon (Fig. 1A). In particular, the regionof the M43 open reading frame downstream from the transposon insertionsite is not expected to be expressed. To determine whether thisis the case, cytoplasmic RNAs were isolated from cells infectedwith the mutant virus at different time points (e.g., 4, 12, and24 h) postinfection. Northern analysis was carried out to examinethe expression of the transcripts from the M43 open reading framedownstream from the transposon insertion site (Fig. 2). The probeused in the Northern analyses contained the DNA sequence complementaryto the M43 coding region about 50 nucleotides downstream fromthe site of the transposon insertion. An abundant RNA specieswas detected in RNA fractions isolated from cells that were infectedwith the wild-type Smith strain (Fig. 2, lane 3) but not in RNAfractions isolated from cells infected with RvM43 when the sameprobe was used (lane 2). Indeed, no truncated transcripts or bandswere detected from cells infected with RvM43 (Fig. 2 and datanot shown), indicating that the region downstream from the transposoninsertion site was not expressed. Meanwhile, expression of thetranscript was found in RNA fractions of cells infected with therescued virus RqM43 (Fig. 2, lane 4) and was at a level similarto that of the RNA fractions from cells infected with the Smithstrain (compare lanes 3 and 4). The level of MCMV M25 transcript(10, 49) was used as the internal control for the expressionof the M43 transcript. As shown in Fig. 2 (lanes 5 to 8), thelevels of the M25 transcript detected in cells that were infectedwith RvM43 and RqM43 were found to be similar to that of M25 transcriptin cells infected with the Smith strain. Thus, the transposoninsertion in RvM43 truncated or disrupted the transcript expressedfrom the M43 open reading frame, whereas expression of the transcriptwas restored in RqM43.

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FIG. 2. Northern analyses of RNA fractions isolated from cells that were mock infected (lanes 1 and 5) or infected with the wild-type virus (WT; lanes 3 and 7), RvM43 (lanes 2 and 6), and RqM43 (lanes 4 and 8); 10⁷ NIH 3T3 cells were infected with each virus at an MOI of 5 PFU per cell, and cells were harvested at 24 h postinfection. Equal amounts of RNA samples (30 µg) were separated on agarose gels that contained formaldehyde, transferred to a nitrocellulose membrane, and hybridized to a ³²P-radiolabeled probe that contained the sequence of M43 (lanes 1 to 4) or M25 (lanes 5 to 8).

Replication of RvM43 and RqM43 in vitro in tissue culture. Growth rates of the recombinant viruses in NIH 3T3 cells were studied in order to determine whether these viruses had anygrowth defects in vitro. Cells were infected with the virusesat both low and high MOIs, and their growth rates were assayedby triplicate experiments. No significant difference was foundin growth rates among RvM43, RqM43, and the Smith strain. Forexample, the peak titers of RvM43 and RqM43 were similar to thoseof the Smith strain after both high- and low-MOI infections (Fig.3). Combined with the results from the Southern and Northern analyses,these observations indicate that M43 is not essential for viralgrowth in vitro.

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FIG. 3. In vitro growth of MCMV mutants in tissue culture. Mouse NIH 3T3 cells were infected with each virus at an MOI of either 0.5 (A) or 5 (B) PFU per cell. At 0, 1, 2, 4, and 7 days postinfection, cells and culture media were harvested and sonicated. The viral titers were determined by plaque assays on NIH 3T3 cells. The virus titers represent averages from triplicate experiments. Standard deviations are indicated by error bars. WT, wild type.

Growth of recombinant viruses RvM43 and RqM43 in immunocompetent animals. To determine whether disruption of M43 significantly affects viral replication in vivo, BALB/c-Byj mice were injected intraperitoneallywith 10⁴ PFU of RvM43, RqM43, or the wild-type Smith strain. At 1, 3,7, 10, 14, and 21 days postinfection, salivary glands, lungs,spleens, livers, and kidneys were harvested and virus titers inthese five organs were determined on NIH 3T3 cells; titers inthe salivary glands at 28 and 35 days postinfection were alsodetermined. These organs are among the major targets for MCMVinfection (2, 17, 19, 26). RvM43 exhibited similar titersas the Smith strain and RqM43 in the lungs, spleens, livers, andkidneys of the infected animals (Fig. 4B to E). These resultssuggest that open reading frame M43 is dispensable for MCMV replicationin these organs in vivo. However, the titers of mutant RvM43 inthe salivary glands at 14 and 21 days postinfection were foundto be at least 100-fold less than those of the Smith strain andRqM43 (Fig. 4). Previous studies have shown that the presenceof the transposon sequence per se within the viral genome doesnot significantly affect viral growth in mice in vivo (50).Thus, these results suggest that the attenuated growth of RvM43in the salivary glands is due to the disruption of M43 and thatopen reading frame M43 is important for viral growth in the salivaryglands in vivo.

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FIG. 4. Titers of MCMV mutants in the salivary glands (A), lungs (B), spleens (C), livers (D), and kidneys (E) of infected BALB/c mice. BALB/c-Byj mice were infected intraperitoneally with 10⁴ PFU of each virus. At 1, 3, 7, 10, 14, and 21 days postinfection, the animals (three mice per group) were sacrificed. The salivary glands, lungs, spleens, livers, and kidneys were collected and sonicated; salivary glands were also collected from animals at 28 and 35 days postinfection. Viral titers in the tissue homogenates were determined by standard plaque assays in NIH 3T3 cells. The limit of detection was 10 PFU/ml of the tissue homogenate. The virus titers represent averages from triplicate experiments. Error bars indicate standard deviations; error bars that are not evident indicate that the standard deviation was less than or equal to the height of the symbols. WT, wild type.

Virulence and growth of viral mutants in SCID mice. It has been shown that immunodeficient animals are extremely susceptible to MCMV infection (15, 31, 32, 35). For example,the CB17 SCID mice, which lack functional T and B lymphocytes,are extremely sensitive to viral infection (as few as 10 PFU ofMCMV cause serious infection) (31, 32). Analysis of viralreplication in these mice therefore serves as an excellent meansfor determining the virulence of different MCMV strains and mutantsand for studying the mechanism whereby they cause opportunisticinfections in immunocompromised hosts. To determine whether theM43 open reading frame plays a significant role in CMV virulence,we compared the survival rates of animals infected with RvM43and those of mice infected with RqM43 and the wild-type Smithstrain. For each virus, five SCID mice were injected intraperitoneallywith 10⁴ PFU of RvM43, RqM43, or the Smith strain. We found that 50% ofthe infected mice died within 24 to 26 days postinfection, indicatingthat disruption of the M43 open reading frame does not significantlyaffect viral virulence (Fig. 5). Moreover, these results are consistentwith our previous observations that the presence of the transposonsequence per se in the viral genome does not significantly affectthe virulence of MCMV in SCID mice (50).

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FIG. 5. Mortality of SCID mice infected with the Smith strain (wild type [WT]), RvM43, and RqM43. CB17 SCID mice (five animals per group) were infected intraperitoneally with 10⁴ PFU of each virus. Mortality of mice was monitored for at least 28 days postinfection, and survival rates were determined.

To further study the pathogenesis of the mutant virus in these immunodeficient animals, the replication of RvM43 in differentorgans of the animals was studied during a 21-day infection periodbefore the mortality of the infected animals became apparent.In these experiments, SCID mice were injected intraperitoneallywith 10⁴ PFU of each virus (RvM43, RqM43, or the wild-type Smith strain).At 1, 3, 7, 10, 14, and 21 days postinfection, three mice fromeach virus group were sacrificed and the salivary glands, lungs,spleens, livers, and kidneys were harvested. The viral titersin these five organs were determined. The titers of RvM43 in thelungs, spleens, livers, and kidneys were similar to those of theSmith strain and the rescued RqM43 (Fig. 6), indicating that disruptionof M43 does not significantly affect MCMV growth in these fourorgans. In contrast, titers of the mutant virus in the salivaryglands at 21 days postinfection were at least 1,000-fold lowerthan those of the wild-type virus and RqM43 (Fig. 6). Thus, RvM43is attenuated in growth in the salivary glands. These resultssuggest that open reading frame M43 may be essential for efficientreplication of MCMV in the salivary glands.

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FIG. 6. Titers of MCMV mutants in the salivary glands (A), lungs (B), spleens (C), livers (D), and kidneys (E) of infected SCID mice. CB17 SCID mice were infected intraperitoneally with 10⁴ PFU of each virus. At 1, 3, 7, 10, 14, and 21 days postinfection, the animals (three mice per group) were sacrificed. The salivary glands, lungs, spleens, livers, and kidneys were collected and sonicated. Viral titers in the tissue homogenates were determined by standard plaque assays in NIH 3T3 cells. The limit of detection was 10 PFU/ml of the tissue homogenate. The virus titers represent averages obtained from triplicate experiments. Error bars indicate standard deviations; error bars that are not evident indicate that the standard deviation was less than or equal to the height of the symbols. WT, wild type.

The transposon insertion at the M43 open reading frame is stable in the viral genome. Our previous studies indicated that a transposon sequence inserted at several regions (e.g., m09 and M83) of the MCMV genomeis stable during viral replication in NIH 3T3 cells and in bothBALB/c and SCID mice (50). However, it has been reported thatviral mutants with an additional inserted sequence were not stableand generated spontaneous mutations during replication in vitroand in vivo (1, 24). It is possible that the transposon sequencein RvM43 is not stable during viral replication in vivo and thatintroduction of the second mutation may be responsible for theobserved phenotypes of the virus in animals. To address this issue,viruses were recovered from the lungs and salivary glands of theBALB/c and SCID mice at 21 days postinfection and subsequentlyused to infect NIH 3T3 cells. Viral DNAs were purified from theinfected cells, and their restriction digestion patterns wereanalyzed in agarose gels. Figure 7 shows a Southern analysis ofthe RvM43 viral DNAs with a DNA probe that contained the transposonand the M43 sequence. These results indicated that no change inthe hybridization patterns of RvM43 occurred as a result of viralgrowth in animals for 21 days (lanes 1 to 4). Moreover, the overallHindIII digestion patterns of RvM43 DNA isolated from either infectedcultured cells or animals were identical to those of the originalrecombinant virus RvM43, as visualized by ethidium bromide stainingof the viral DNAs (data not shown). Thus, the transposon insertionin RvM43 appeared to be stable and the genome of RvM43 remainedintact during replication in both BALB/c and SCID mice.

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FIG. 7. The stability of the transposon mutation of RvM43 in BALB/c and SCID mice. Viral DNAs were isolated either from cells that were infected with RvM43 (MOI, <0.01) and allowed to grow in culture for 5 days (P0; lane 4) or from cells that were infected with the virus collected from the salivary glands (SG; lanes 2 and 3) and lungs (Lu; lane 1) of either BALB/c (lane 3) or SCID (lanes 1 and 2) mice 21 days after intraperitoneal inoculation with 10⁴ PFU of RvM43. Southern analyses of the viral DNA fractions digested with HindIII are shown. The DNA of the wild-type virus (WT) is shown in lane 5. The ³²P-radiolabeled probe was derived from the same plasmid as was used for Southern analyses of RvM43 in Fig. 1 and contained the transposon and the M43 open reading frame sequence.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study, a recombinant virus that contained the insertional mutation at open reading frame M43 was characterized. Ourresults provide the first direct evidence to suggest that M43is not essential for viral replication in NIH 3T3 cells in vitro.Moreover, M43 appears to function as a viral determinant for MCMVgrowth in the salivaryglands.

While it is possible that the functional protein product is synthesized from the transposon-disrupted region, several linesof evidence strongly suggest that this is not the case. First,the transposon sequence was inserted into the coding sequenceof the M43 open reading frame (Fig. 1B). Second, transcriptionfrom the region downstream from the transposon insertion sitewas not detected in cells infected with the mutant virus (Fig.2). Thus, the region of the target open reading frame downstreamfrom the transposon insertion site was not expressed, and thetranscript expressed from the disrupted open reading frame wastruncated.

The function of M43 is unknown. Indeed, to our knowledge, neither the transcript nor the protein product coded by this openreading frame has been reported. Our results indicate that a transcriptof about 5,000 nucleotides is expressed from the M43 open readingframe. The growth rate of RvM43 in NIH 3T3 cells was not significantlydifferent from that of the Smith strain. Since the transposoninsertion in RvM43 is within the M43 coding region and the codingsequence 3' from the insertion site was not transcribed, it islikely that no functional M43 protein was expressed from the viralmutant. Thus, our results suggest that M43 is not essential forviral replication in NIH 3T3cells.

Our results indicate that RvM43 replicated as well as the wild-type Smith strain in the lungs, livers, spleens, and kidneysof both BALB/c and SCID mice that were infected intraperitoneallywith these viruses. These results suggest that RvM43 is not essentialfor viral growth in these organs in vivo. Moreover, RvM43 wasas virulent as the Smith strain in killing the SCID mice, suggestingthat the M43 open reading frame does not play a significant rolein viral virulence in SCID mice. In contrast, RvM43 was attenuatedin replication in the salivary glands of the infected animals.The titers of RvM43 in the salivary glands of SCID mice at 21days postinfection were at least 1,000-fold lower than those ofthe wild-type virus, whereas the rescued virus RqM43 exhibitedsimilar titers as the Smith strain. These results strongly suggestthat M43 is a viral determinant for replication in the salivaryglands. Furthermore, our data suggest that viral replication inthe salivary glands does not significantly contribute to MCMVvirulence in killing the SCIDmice.

It is possible that the observed change in the levels of replication of the mutant is due to other adventitious mutationsaccumulated during the construction and growth of the recombinantvirus in cultured cells or in animals. However, several linesof evidence strongly suggest that this is unlikely. First, rescuedvirus RqM43 replicated as well as the wild-type virus in the salivaryglands (Fig. 4 and 6). The genomic sequence of M43 and its expressionin the rescued virus were restored (Fig. 1 and 2). These observationssuggest that the transposon insertion, rather than a second mutation,is responsible for the observed attenuation of RvM43 replicationin the salivary glands. Second, our previous studies indicatedthat a virus with a transposon insertion at the m09 open readingframe replicated as well as the wild-type virus in the salivaryglands, indicating that the transposon sequence per se in theviral genome does not significantly affect viral replication inthe organs (50). Third, the transposon insertion was stableduring replication in animals. There was no change in the hybridizationpatterns of the DNAs from the mutant virus recovered from thesalivary glands and lungs of the infected animals at 21 days postinfection(Fig. 7). Moreover, the HindIII digestion patterns of the RvM43mutant DNAs, other than the region with the inserted transposon,appeared to be identical to those of the wild-type virus DNA (datanot shown). Thus, the observed change in the RvM43 titer in thesalivary glands is probably due to the insertional mutation atM43 introduced by thetransposon.

Our results suggest that M43 functions as a viral determinant for growth in salivary glands and that the lack of expressionof the functional full-length M43 product is responsible for theobserved low level of growth of RvM43 in the salivary glands.However, it is possible that expression of the N-terminal truncatedportion of the M43 open reading frame rather than the lack ofexpression of the full-length M43 product may be responsible forthe observed phenotype of the mutant in vivo. This is becausethe truncated protein, which is possibly expressed under the controlof the wild-type viral M43 promoter and translation initiationsite, may interfere with viral growth in the salivary glands.To address this issue, another viral mutant with a transposoninsertion at M43 (at the codon for amino acid 116) was isolatedindependently from RvM43. The titers of this second mutant inthe salivary glands of the infected animals were similar to thoseof RvM43 and lower than those of the Smith strain and RqM43 (J.Xiao, X. Zhan, E. Haghjoo, and F. Liu, unpublished results). Thus,it is unlikely that expression of the truncated N-terminal productrather the lack of expression of the full-length M43 product isresponsible for the low level of growth of the viral mutant inthe salivary glands, although we cannot completely rule out thispossibility.

Open reading frame M43 and its HCMV counterpart, UL43, belong to the MCMV M23 and HCMV US22 gene families, respectively (6,34). The MCMV M23 gene family, consisting of 12 open readingframes, includes M23, M24, M36, M43, m25.1, m25.2, m128 (ie2),m139, m140, 141, m142, and m143. The HCMV US22 gene family includesUL23, UL24, UL28, UL29, UL36, UL43, US22, US23, US24, US26, IRS1,and TRS1. A spontaneous deletion at the UL42 and UL43 region duringHCMV growth in vitro has been observed, and UL43 appeared to bedispensable for HCMV replication in vitro (11, 29). Previousstudies have also shown that several members of the MCMV M23 genefamily (e.g., m128 [ie2] and m140) are dispensable for MCMV replication(4, 5, 16, 23). Indeed, the replication of a virus witha deletion in m139, m140, and m141 was significantly attenuatedin growth in animals (5, 16), while a virus carrying a deletionin m128 (ie2) appeared to replicate as well as the wild-type virus(4, 23). Moreover, some members (e.g., m140 and m141) ofthe M23 gene family have been implicated as important for celland tissue tropism of MCMV infection (5, 16). Our resultssuggest that M43 plays a significant role in MCMV infection inthe salivary glands. It will be interesting to determine whetherUL43 is also a viral determinant for HCMV replication in the sameorgan.

Specific tropism for host tissues, particularly the salivary glands, is an important determinant of CMV biology. Tropism forthe salivary glands and persistent and recurrent viral sheddingfrom this organ are believed to be among the main routes for HCMVtransmission in normally healthy individuals (2). Previousstudies have suggested that open reading frame m133 (sgg1) isa viral determinant for MCMV replication in the salivary glands(21, 24). A viral mutant with a deletion in sgg1 was defectivein growth in the salivary glands of BALB/c mice (24). Meanwhile,this mutant did not exhibit any growth defects in other organsexamined and was as virulent as the wild-type virus in killingBALB/c mice (21, 24). Although there is little sequence homologybetween M43 and sgg1, it is conceivable that the function of theM43 gene is related to that of sgg1. There are other examplesin the herpesvirus family that some viral genes are necessaryfor viral replication in specific tissues or organs. For example,herpes simplex virus type 1 $gamma$ 1-34.5, which is dispensable forviral replication in cultured cells, is essential for viral replicationin neuronal cells and has been suggested to play a significantrole in viral neuronal tropism and neuroinvasiveness (7). Itis intriguing that more than one gene is needed for MCMV tissuetropism in a specific organ. It would be interesting to determinehow these determinants function in concert with the replicationcycle of MCMV in vivo. These studies will further provide insightinto the biology of CMVs and functions of the viral genes in CMVpathogenesis.

	ACKNOWLEDGMENTS

We thank Edward Mocarski, Stanford University, for insightful advice and Michael Snyder, Yale University, for providing theTn3 constructs and the E. coli strains for transposon shuttlemutagenesis. Gratitude also goes to Gerry Abenes and Manfred Leefor sharing unpublished results and helpful discussions and toIlse Von Reis and John Kim for technicalassistance.

F.L. is a Pew Scholar in Biomedical Sciences and a recipient of a Hellman Family Faculty Award, a Basil O'Connor Starter ScholarResearch Award (March of Dimes National Birth Defects Foundation),and a Regents Junior Faculty Fellowship (University of California).This research was supported in part by a Chancellor's SpecialInitiative Grant Award (UC-Berkeley) and a grant from the Stateof California AIDS researchprogram.

	FOOTNOTES

^* Corresponding author. Mailing address: Program in Infectious Diseases and Immunity, School of Public Health, 140 Warren Hall,University of California, Berkeley, CA 94720. Phone: (510) 643-2436.Fax: (510) 642-6350. E-mail: liu_fy{at}uclink4.berkeley.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Boname, J. M., and J. K. Chantler. 1992. Characterization of a strain of murine cytomegalovirus which fails to grow in the salivary glands of mice. J. Gen. Virol. 73:2021-2029[Abstract/Free Full Text].

2. Britt, W. J., and C. A. Alford. 1996. Cytomegalovirus, p. 2493-2523. In B. N. Fields, D. M. Knipe, et al. (ed.), Virology, 3rd ed. Raven Press, New York, N.Y.

3. 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].

4. Cardin, R. D., G. B. Abenes, C. A. Stoddart, and E. S. Mocarski. 1995. Murine cytomegalovirus IE2, an activator of gene expression, is dispensable for growth and latency in mice. Virology 209:236-241[CrossRef][Medline].

5. Cavanaugh, V. J., R. M. Stenberg, T. L. Staley, H. W. Virgin III, M. R. MacDonald, S. Paetzold, H. E. Farrell, W. D. Rawlinson, and A. E. Campbell. 1996. Murine cytomegalovirus with a deletion of genes spanning HindIII-J and -I displays altered cell and tissue tropism. J. Virol. 70:1365-1374[Abstract].

6. Chee, M. S., A. T. Bankier, S. Beck, R. Bohni, C. M. Brown, R. Cerny, T. Horsnell, C. A. Hutchison, T. Kouzarides, and J. A. Martignetti. 1990. Analysis of the protein-coding content of the sequence of human cytomegalovirus strain AD169. Curr. Top. Microbiol. Immunol. 154:125-169[Medline].

7. Chou, J., E. R. Kern, R. J. Whitley, and B. Roizman. 1990. Mapping of herpes simplex virus-1 neurovirulence to gamma 134.5, a gene nonessential for growth in culture. Science 250:1262-1266[Abstract/Free Full Text].

8. 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].

9. 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].

10. Dallas, P. B., P. A. Lyons, J. B. Hudson, A. A. Scalzo, and G. R. Shellam. 1994. Identification and characterization of a murine cytomegalovirus gene with homology to the UL25 open reading frame of human cytomegalovirus. Virology 200:643-650[CrossRef][Medline].

11. Dargan, D. J., F. E. Jamieson, J. MacLean, A. Dolan, C. Addison, and D. J. McGeoch. 1997. The published DNA sequence of human cytomegalovirus strain AD169 lacks 929 base pairs affecting genes UL42 and UL43. J. Virol. 71:9833-9836[Abstract].

12. Delecluse, H. J., T. Hilsendegen, D. Pich, R. Zeidler, and W. Hammerschmidt. 1998. Propagation and recovery of intact, infectious Epstein-Barr virus from prokaryotic to human cells. Proc. Natl. Acad. Sci. USA 95:8245-8250[Abstract/Free Full Text].

13. Fowler, K. B., S. Stagno, R. F. Pass, W. J. Britt, T. J. Boll, and C. A. Alford. 1992. The outcome of congenital cytomegalovirus infection in relation to maternal antibody status. N. Engl. J. Med. 326:663-667[Abstract].

14. Greaves, R. F., J. M. Brown, J. Vieira, and E. S. Mocarski. 1995. Selectable insertion and deletion mutagenesis of the human cytomegalovirus genome using the Escherichia coli guanosine phosphoribosyl transferase (gpt) gene. J. Gen. Virol. 76:2151-2160[Abstract/Free Full Text].

15. Grundy, J. E., and C. J. Melief. 1982. Effect of Nu/Nu gene on genetically determined resistance to murine cytomegalovirus. J. Gen. Virol. 61:133-136[Abstract/Free Full Text].

16. Hanson, L. K., J. S. Slater, Z. Karabekian, H. W. Virgin III, C. A. Biron, M. C. Ruzek, N. van Rooijen, R. P. Ciavarra, R. M. Stenberg, and A. E. Campbell. 1999. Replication of murine cytomegalovirus in differentiated macrophages as a determinant of viral pathogenesis. J. Virol. 73:5970-5980[Abstract/Free Full Text].

17. Hudson, J. B. 1979. The murine cytomegalovirus as a model for the study of viral pathogenesis and persistent infections. Arch. Virol. 62:1-29[CrossRef][Medline].

18. Jenkins, F. J., M. J. Casadaban, and B. Roizman. 1985. Application of the mini-Mu-phage for target-sequence-specific insertional mutagenesis of the herpes simplex virus genome. Proc. Natl. Acad. Sci. USA 82:4773-4777[Abstract/Free Full Text].

19. Jordan, M. C. 1983. Latent infection and the elusive cytomegalovirus. Rev. Infect. Dis. 5:205-215[Medline].

20. 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].

21. Lagenaur, L. A., W. C. Manning, J. Vieira, C. L. Martens, and E. S. Mocarski. 1994. Structure and function of the murine cytomegalovirus sgg1 gene: a determinant of viral growth in salivary gland acinar cells. J. Virol. 68:7717-7727[Abstract/Free Full Text].

22. Liu, F., 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].

23. Manning, W. C., and E. S. Mocarski. 1988. Insertional mutagenesis of the murine cytomegalovirus genome: one prominent alpha gene (ie2) is dispensable for growth. Virology 167:477-484[Medline].

24. Manning, W. C., C. A. Stoddart, L. A. Lagenaur, G. B. Abenes, and E. S. Mocarski. 1992. Cytomegalovirus determinant of replication in salivary glands. J. Virol. 66:3794-3802[Abstract/Free Full Text].

25. 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].

26. Mocarski, E. S. 1996. Cytomegaloviruses and their replication, p. 2447-2492. In B. N. Fields, D. M. Knipe, et al. (ed.), Virology, 3rd ed. Raven Press, New York, N.Y.

27. Mocarski, E. S., G. W. Kemble, J. M. Lyle, and R. F. Greaves. 1996. A deletion mutant in the human cytomegalovirus gene encoding IE1(491aa) is replication defective due to a failure in autoregulation. Proc. Natl. Acad. Sci. USA 93:11321-11326[Abstract/Free Full Text].

28. 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 22:243-255[CrossRef][Medline].

29. Mocarski, E. S., M. N. Prichard, C. S. Tan, and J. M. Brown. 1997. Reassessing the organization of the UL42-UL43 region of the human cytomegalovirus strain AD169 genome. Virology 239:169-175[CrossRef][Medline].

30. Mulligan, R. C., and P. Berg. 1981. Selection for animal cells that express the Escherichia coli gene coding for xanthine-guanine phosphoribosyltransferase. Proc. Natl. Acad. Sci. USA 78:2072-2076[Abstract/Free Full Text].

31. Okada, M., and Y. Minamishima. 1987. The efficacy of biological response modifiers against murine cytomegalovirus infection in normal and immunodeficient mice. Microbiol. Immunol. 31:45-57[Medline].

32. Pollock, J. L., and H. W. Virgin, III. 1995. Latency, without persistence, of murine cytomegalovirus in the spleen and kidney. J. Virol. 69:1762-1768[Abstract].

33. Post, L. E., and B. Roizman. 1981. A generalized technique for deletion of specific genes in large genomes: alpha gene 22 of herpes simplex virus 1 is not essential for growth. Cell 25:227-232[CrossRef][Medline].

34. 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].

35. Reynolds, R. P., R. J. Rahija, D. I. Schenkman, and C. B. Richter. 1993. Experimental murine cytomegalovirus infection in severe combined immunodeficient mice. Lab. Anim. Sci. 43:291-295[Medline].

36. Roizman, B., and F. J. Jenkins. 1985. Genetic engineering of novel genomes of large DNA viruses. Science 229:1208-1214[Abstract/Free Full Text].

37. Saeki, Y., T. Ichikawa, A. Saeki, E. A. Chiocca, K. Tobler, M. Ackermann, X. O. Breakefield, and C. Fraefel. 1998. Herpes simplex virus type 1 DNA amplified as bacterial artificial chromosome in Escherichia coli: rescue of replication-competent virus progeny and packaging of amplicon vectors. Hum. Gene Ther. 9:2787-2794[Medline].

38. Selik, R. M., S. Y. Chu, and J. W. Ward. 1995. Trends in infectious diseases and cancers among persons dying of HIV infection in the United States from 1987 to 1992. Ann. Intern. Med. 123:933-936[Abstract/Free Full Text].

39. Selik, R. M., J. M. Karon, and J. W. Ward. 1997. Effect of the human immunodeficiency virus epidemic on mortality from opportunistic infections in the United States in 1993. J. Infect. Dis. 176:632-636[Medline].

40. 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].

41. Smith, G. A., and L. W. Enquist. 2000. A self-recombining bacterial artificial chromosome and its application for analysis of herpesvirus pathogenesis. Proc. Natl. Acad. Sci. USA 97:4873-4878[Abstract/Free Full Text].

42. Stavropoulos, T. A., and C. A. Strathdee. 1998. An enhanced packaging system for helper-dependent herpes simplex virus vectors. J. Virol. 72:7137-7143[Abstract/Free Full Text].

43. 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].

44. 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].

45. Vieira, J., H. E. Farrell, W. D. Rawlinson, and E. S. Mocarski. 1994. Genes in the HindIII J fragment of the murine cytomegalovirus genome are dispensable for growth in cultured cells: insertion mutagenesis with a lacZ/gpt cassette. J. Virol. 68:4837-4846[Abstract/Free Full Text].

46. 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].

47. Weber, P. C., M. Levine, and J. C. Glorioso. 1987. Rapid identification of nonessential genes of herpes simplex virus type 1 by Tn5 mutagenesis. Science 236:576-579[Abstract/Free Full Text].

48. Wiertz, E. J., T. R. Jones, L. Sun, M. Bogyo, H. J. Geuze, and H. L. Ploegh. 1996. The human cytomegalovirus US11 gene product dislocates MHC class I heavy chains from the endoplasmic reticulum to the cytosol. Cell 84:769-779[CrossRef][Medline].

49. Zhan, X., G. Abenes, M. Lee, I. VonReis, C. Kittinunvorakoon, P. Ross-Macdonald, M. Snyder, and F. Liu. 2000. Mutagenesis of murine cytomegalovirus using a Tn3-based transposon. Virology 266:264-274[CrossRef][Medline].

50. Zhan, X., M. Lee, J. Xiao, and F. Liu. 2000. Construction and characterization of murine cytomegaloviruses that contain a transposon insertion at open reading frames m09 and M83. J. Virol. 74:7411-7421[Abstract/Free Full Text].

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1.	Boname, J. M., and J. K. Chantler. 1992. Characterization of a strain of murine cytomegalovirus which fails to grow in the salivary glands of mice. J. Gen. Virol. 73:2021-2029[Abstract/Free Full Text].
2.	Britt, W. J., and C. A. Alford. 1996. Cytomegalovirus, p. 2493-2523. In B. N. Fields, D. M. Knipe, et al. (ed.), Virology, 3rd ed. Raven Press, New York, N.Y.
3.	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].
4.	Cardin, R. D., G. B. Abenes, C. A. Stoddart, and E. S. Mocarski. 1995. Murine cytomegalovirus IE2, an activator of gene expression, is dispensable for growth and latency in mice. Virology 209:236-241[CrossRef][Medline].
5.	Cavanaugh, V. J., R. M. Stenberg, T. L. Staley, H. W. Virgin III, M. R. MacDonald, S. Paetzold, H. E. Farrell, W. D. Rawlinson, and A. E. Campbell. 1996. Murine cytomegalovirus with a deletion of genes spanning HindIII-J and -I displays altered cell and tissue tropism. J. Virol. 70:1365-1374[Abstract].
6.	Chee, M. S., A. T. Bankier, S. Beck, R. Bohni, C. M. Brown, R. Cerny, T. Horsnell, C. A. Hutchison, T. Kouzarides, and J. A. Martignetti. 1990. Analysis of the protein-coding content of the sequence of human cytomegalovirus strain AD169. Curr. Top. Microbiol. Immunol. 154:125-169[Medline].
7.	Chou, J., E. R. Kern, R. J. Whitley, and B. Roizman. 1990. Mapping of herpes simplex virus-1 neurovirulence to gamma 134.5, a gene nonessential for growth in culture. Science 250:1262-1266[Abstract/Free Full Text].
8.	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].
9.	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].
10.	Dallas, P. B., P. A. Lyons, J. B. Hudson, A. A. Scalzo, and G. R. Shellam. 1994. Identification and characterization of a murine cytomegalovirus gene with homology to the UL25 open reading frame of human cytomegalovirus. Virology 200:643-650[CrossRef][Medline].
11.	Dargan, D. J., F. E. Jamieson, J. MacLean, A. Dolan, C. Addison, and D. J. McGeoch. 1997. The published DNA sequence of human cytomegalovirus strain AD169 lacks 929 base pairs affecting genes UL42 and UL43. J. Virol. 71:9833-9836[Abstract].
12.	Delecluse, H. J., T. Hilsendegen, D. Pich, R. Zeidler, and W. Hammerschmidt. 1998. Propagation and recovery of intact, infectious Epstein-Barr virus from prokaryotic to human cells. Proc. Natl. Acad. Sci. USA 95:8245-8250[Abstract/Free Full Text].
13.	Fowler, K. B., S. Stagno, R. F. Pass, W. J. Britt, T. J. Boll, and C. A. Alford. 1992. The outcome of congenital cytomegalovirus infection in relation to maternal antibody status. N. Engl. J. Med. 326:663-667[Abstract].
14.	Greaves, R. F., J. M. Brown, J. Vieira, and E. S. Mocarski. 1995. Selectable insertion and deletion mutagenesis of the human cytomegalovirus genome using the Escherichia coli guanosine phosphoribosyl transferase (gpt) gene. J. Gen. Virol. 76:2151-2160[Abstract/Free Full Text].
15.	Grundy, J. E., and C. J. Melief. 1982. Effect of Nu/Nu gene on genetically determined resistance to murine cytomegalovirus. J. Gen. Virol. 61:133-136[Abstract/Free Full Text].
16.	Hanson, L. K., J. S. Slater, Z. Karabekian, H. W. Virgin III, C. A. Biron, M. C. Ruzek, N. van Rooijen, R. P. Ciavarra, R. M. Stenberg, and A. E. Campbell. 1999. Replication of murine cytomegalovirus in differentiated macrophages as a determinant of viral pathogenesis. J. Virol. 73:5970-5980[Abstract/Free Full Text].
17.	Hudson, J. B. 1979. The murine cytomegalovirus as a model for the study of viral pathogenesis and persistent infections. Arch. Virol. 62:1-29[CrossRef][Medline].
18.	Jenkins, F. J., M. J. Casadaban, and B. Roizman. 1985. Application of the mini-Mu-phage for target-sequence-specific insertional mutagenesis of the herpes simplex virus genome. Proc. Natl. Acad. Sci. USA 82:4773-4777[Abstract/Free Full Text].
19.	Jordan, M. C. 1983. Latent infection and the elusive cytomegalovirus. Rev. Infect. Dis. 5:205-215[Medline].
20.	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].
21.	Lagenaur, L. A., W. C. Manning, J. Vieira, C. L. Martens, and E. S. Mocarski. 1994. Structure and function of the murine cytomegalovirus sgg1 gene: a determinant of viral growth in salivary gland acinar cells. J. Virol. 68:7717-7727[Abstract/Free Full Text].
22.	Liu, F., 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].
23.	Manning, W. C., and E. S. Mocarski. 1988. Insertional mutagenesis of the murine cytomegalovirus genome: one prominent alpha gene (ie2) is dispensable for growth. Virology 167:477-484[Medline].
24.	Manning, W. C., C. A. Stoddart, L. A. Lagenaur, G. B. Abenes, and E. S. Mocarski. 1992. Cytomegalovirus determinant of replication in salivary glands. J. Virol. 66:3794-3802[Abstract/Free Full Text].
25.	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].
26.	Mocarski, E. S. 1996. Cytomegaloviruses and their replication, p. 2447-2492. In B. N. Fields, D. M. Knipe, et al. (ed.), Virology, 3rd ed. Raven Press, New York, N.Y.
27.	Mocarski, E. S., G. W. Kemble, J. M. Lyle, and R. F. Greaves. 1996. A deletion mutant in the human cytomegalovirus gene encoding IE1(491aa) is replication defective due to a failure in autoregulation. Proc. Natl. Acad. Sci. USA 93:11321-11326[Abstract/Free Full Text].
28.	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 22:243-255[CrossRef][Medline].
29.	Mocarski, E. S., M. N. Prichard, C. S. Tan, and J. M. Brown. 1997. Reassessing the organization of the UL42-UL43 region of the human cytomegalovirus strain AD169 genome. Virology 239:169-175[CrossRef][Medline].
30.	Mulligan, R. C., and P. Berg. 1981. Selection for animal cells that express the Escherichia coli gene coding for xanthine-guanine phosphoribosyltransferase. Proc. Natl. Acad. Sci. USA 78:2072-2076[Abstract/Free Full Text].
31.	Okada, M., and Y. Minamishima. 1987. The efficacy of biological response modifiers against murine cytomegalovirus infection in normal and immunodeficient mice. Microbiol. Immunol. 31:45-57[Medline].
32.	Pollock, J. L., and H. W. Virgin, III. 1995. Latency, without persistence, of murine cytomegalovirus in the spleen and kidney. J. Virol. 69:1762-1768[Abstract].
33.	Post, L. E., and B. Roizman. 1981. A generalized technique for deletion of specific genes in large genomes: alpha gene 22 of herpes simplex virus 1 is not essential for growth. Cell 25:227-232[CrossRef][Medline].
34.	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].
35.	Reynolds, R. P., R. J. Rahija, D. I. Schenkman, and C. B. Richter. 1993. Experimental murine cytomegalovirus infection in severe combined immunodeficient mice. Lab. Anim. Sci. 43:291-295[Medline].
36.	Roizman, B., and F. J. Jenkins. 1985. Genetic engineering of novel genomes of large DNA viruses. Science 229:1208-1214[Abstract/Free Full Text].
37.	Saeki, Y., T. Ichikawa, A. Saeki, E. A. Chiocca, K. Tobler, M. Ackermann, X. O. Breakefield, and C. Fraefel. 1998. Herpes simplex virus type 1 DNA amplified as bacterial artificial chromosome in Escherichia coli: rescue of replication-competent virus progeny and packaging of amplicon vectors. Hum. Gene Ther. 9:2787-2794[Medline].
38.	Selik, R. M., S. Y. Chu, and J. W. Ward. 1995. Trends in infectious diseases and cancers among persons dying of HIV infection in the United States from 1987 to 1992. Ann. Intern. Med. 123:933-936[Abstract/Free Full Text].
39.	Selik, R. M., J. M. Karon, and J. W. Ward. 1997. Effect of the human immunodeficiency virus epidemic on mortality from opportunistic infections in the United States in 1993. J. Infect. Dis. 176:632-636[Medline].
40.	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].
41.	Smith, G. A., and L. W. Enquist. 2000. A self-recombining bacterial artificial chromosome and its application for analysis of herpesvirus pathogenesis. Proc. Natl. Acad. Sci. USA 97:4873-4878[Abstract/Free Full Text].
42.	Stavropoulos, T. A., and C. A. Strathdee. 1998. An enhanced packaging system for helper-dependent herpes simplex virus vectors. J. Virol. 72:7137-7143[Abstract/Free Full Text].
43.	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].
44.	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].
45.	Vieira, J., H. E. Farrell, W. D. Rawlinson, and E. S. Mocarski. 1994. Genes in the HindIII J fragment of the murine cytomegalovirus genome are dispensable for growth in cultured cells: insertion mutagenesis with a lacZ/gpt cassette. J. Virol. 68:4837-4846[Abstract/Free Full Text].
46.	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].
47.	Weber, P. C., M. Levine, and J. C. Glorioso. 1987. Rapid identification of nonessential genes of herpes simplex virus type 1 by Tn5 mutagenesis. Science 236:576-579[Abstract/Free Full Text].
48.	Wiertz, E. J., T. R. Jones, L. Sun, M. Bogyo, H. J. Geuze, and H. L. Ploegh. 1996. The human cytomegalovirus US11 gene product dislocates MHC class I heavy chains from the endoplasmic reticulum to the cytosol. Cell 84:769-779[CrossRef][Medline].
49.	Zhan, X., G. Abenes, M. Lee, I. VonReis, C. Kittinunvorakoon, P. Ross-Macdonald, M. Snyder, and F. Liu. 2000. Mutagenesis of murine cytomegalovirus using a Tn3-based transposon. Virology 266:264-274[CrossRef][Medline].
50.	Zhan, X., M. Lee, J. Xiao, and F. Liu. 2000. Construction and characterization of murine cytomegaloviruses that contain a transposon insertion at open reading frames m09 and M83. J. Virol. 74:7411-7421[Abstract/Free Full Text].