Moving the Glycoprotein Gene of Vesicular Stomatitis Virus to Promoter-Proximal Positions Accelerates and Enhances the Protective Immune Response

doi:10.1128/JVI.74.17.7895-7902.2000

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Journal of Virology, September 2000, p. 7895-7902, Vol. 74, No. 17
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Moving the Glycoprotein Gene of Vesicular Stomatitis Virus to Promoter-Proximal Positions Accelerates and Enhances the Protective Immune Response

E. Brian Flanagan, L. Andrew Ball, and Gail W. Wertz^*

Department of Microbiology, The Medical School, University of Alabama at Birmingham, Birmingham, Alabama 35294

Received 30 March 2000/Accepted 8 June 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Vesicular stomatitis virus (VSV) is the prototype of the Rhabdoviridae and contains nonsegmented negative-sense RNA as itsgenome. The 11-kb genome encodes five genes in the order 3'-N-P-M-G-L-5',and transcription is obligatorily sequential from the single 3'promoter. As a result, genes at promoter-proximal positions aretranscribed at higher levels than those at promoter-distal positions.Previous work demonstrated that moving the gene encoding the nucleocapsidprotein N to successively more promoter-distal positions resultedin stepwise attenuation of replication and lethality for mice.In the present study we investigated whether moving the gene forthe attachment glycoprotein G, which encodes the major neutralizingepitopes, from its fourth position up to first in the gene orderwould increase G protein expression in cells and alter the immuneresponse in inoculated animals. In addition to moving the G genealone, we also constructed viruses having both the G and N genesrearranged. This produced three variant viruses having the orders3'-G-N-P-M-L-5' (G1N2), 3'-P-M-G-N-L-5' (G3N4), and 3'-G-P-M-N-L-5'(G1N4), respectively. These viruses differed from one anotherand from wild-type virus in their levels of gene expression andreplication in cell culture. The viruses also differed in theirpathogenesis, immunogenicity, and level of protection of miceagainst challenge with wild-type VSV. Translocation of the G genealtered the kinetics and level of the antibody response in mice,and simultaneous reduction of N protein expression reduced replicationand lethality for animals. These studies demonstrate that generearrangement can be exploited to design nonsegmented negative-senseRNA viruses that have characteristics desirable in candidatesfor live attenuatedvaccines.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The order Mononegavirales is composed of four families, Rhabdoviridae, Paramyxoviridae, Filoviridae, and Bornaviridae. Theviruses in these families contain a single strand of nonsegmentednegative-sense RNA and are responsible for a wide range of significantdiseases in fish, plants, and animals (31). Viral gene expressionis controlled at the level of transcription by the order of thegenes on the genome relative to the single 3' promoter. Gene orderthroughout the Mononegavirales is highly conserved; genes encodingproducts required in stoichiometric amounts for replication arealways at or near the 3' end of the genome, while those whoseproducts are needed in catalytic amounts are more promoterdistal.

Vesicular stomatitis virus (VSV) is the prototypic virus of the Rhabdoviridae. Its 11-kb genome has five genes which encodethe five structural proteins of the virus: the nucleocapsid protein,N, which is required in stoichiometric amounts for encapsidationof the replicated RNA; the phosphoprotein, P, which is a cofactorof the RNA-dependent RNA polymerase, L; the matrix protein, M;and the attachment glycoprotein, G. The order of genes in thegenome is 3'-N-P-M-G-L-5', and previous work has shown that expressionis obligatorily sequential from a single 3' promoter (1, 3).Due to attenuation at each gene junction (15), the 3'-most genesare transcribed more abundantly than those which are more promoterdistal (15, 41). In nature, VSV infects a wide range of animals,of which horses, cattle, and domestic swine are the most economicallyimportant. Infection results in the appearance of lesions aroundthe mouth, hooves, and udder teats; while seldom fatal, it leadsto a loss in meat and milk production along with the expense ofquarantine and vaccination (13). There are two main VSV serotypes,Indiana and New Jersey; while these viruses are endemic in Centraland South American countries, outbreaks also occur within theUnited States. The most recent outbreak in the United States occurredin 1997 in horses (40) and was of the Indiana serotype, whileprevious cases identified in 1995 (6) and 1982 to 1983 (43)were of the New Jersey serotype. The ease with which these virusesare transmitted, and the similarity of their symptoms to thosecaused by foot-and-mouth disease virus in cattle and domesticswine, makes VSV a pathogen of concern to sections of the agricultureindustry.

In recent work we rearranged the three internal genes of VSV, P, M, and G, to all combinations and recovered viruses havingthe six possible gene orders (4). In every case, the relativelevels of protein expression in cells were in concordance withthe distance of the corresponding genes from the 3' promoter.These studies demonstrated that viruses with rearranged geneswere viable and that expression of a gene could be modulated ina predictable manner according to its positioning relative tothe 3'promoter.

VSV genome RNA replication is proportional to the amount of N protein synthesized (2, 27), and so in a second study weexamined the effects of moving the N gene from its promoter-proximalsite to successively promoter-distal positions. N transcriptionwas reduced in a systematic manner (45), and this resulted incorrespondingly reduced N protein synthesis, a stepwise reductionin the ability of these viruses to replicate in cell culture,and an attenuation of their lethality for mice. Mice that survivedinoculation with the rearranged variants were protected from challengewith a lethal dose of wild-type (wt) virus. Therefore, despiteattenuation of replication in cell culture and lethality in vivo,these viruses stimulated a protective immune response. These findingsshow that despite the highly conserved gene order of VSV, generearrangement was not lethal to the virus and could be used togenerate viruses with predictable degrees of attenuation. Translocationof an essential gene of a nonsegmented negative-strand virus providesa new approach for engineering viruses with different degreesof replication ability by design rather than traditional empiricalmethods.

In the present study we examined whether we could increase the expression of a promoter-distal gene, the gene that encodesthe attachment glycoprotein G, by moving it to a promoter-proximalsite. The attachment glycoprotein contains the neutralizing site(17, 21, 35, 36), along with helper T-cell (7) andcytotoxic T-cell epitopes (19, 37), of the virus. It has beenshown that stimulation of neutralizing antibodies is an importantfeature in the protection of mice (12, 20) and the naturalhost against infection with VSV (22). To determine if an increasein the production of G protein in cells during infection couldelicit a greater protective immune response, we engineered changesinto an infectious cDNA clone of the VSV genome and recoveredtwo novel viruses in which the glycoprotein gene was moved fromits normal fourth position to the first position in the gene order.One virus, referred to as G1N2, had the gene order 3'-G-N-P-M-L-5';the gene order of the second, G1N4, was 3'-G-P-M-N-L-5'. The invitro and in vivo characteristics of these viruses were assessedand compared to those of viruses having the gene orders 3'-P-M-G-N-L-5'(G3N4) and 3'-N-P-M-G-L-5' (N1G4), the latter being the wt geneorder. Differences were observed in the replication of these virusesin cell culture, their lethality in mice, the kinetics and levelsof antibody production after inoculation, and their ability toprotect mice against challenge with a lethal dose of wtVSV.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Viruses and cells. The San Juan isolate of the Indiana serotype of VSV provided the template for all of the cDNA clone of the VSV genome exceptthe G protein gene, which was derived from the Orsay isolate ofVSV-Indiana (46). All viruses were recovered from cDNAs in babyhamster kidney (BHK-21) cells. BHK-21 cells were also used forsingle-step growth assays and radioisotopic labeling of viralRNAs and proteins. Plaque assays were performed on the Africangreen monkey kidney cell line Vero-76.

Plasmid construction and recovery of infectious virus. The construction of a full-length cDNA clone of the VSV genome and its use for the recovery of infectious virus have beendescribed elsewhere (46). This infectious clone was manipulatedusing methods which allowed the genome to be assembled with thegenes in different orders (4). No other changes were made inthe genome except for a single nucleotide in the intergenic regiondownstream of the P gene. This change, from 3'-CA-5' to 3'-GA-5',has little effect on transcription (5).

To recover infectious viruses from the rearranged cDNA clones, BHK-21 cells were infected with a recombinant vaccinia virusexpressing the T7 RNA polymerase (vTF7-3) (11). One hour later,the cells were transfected with the rearranged VSV cDNA alongwith three plasmids, which expressed the N, P, and L proteinsrequired for encapsidation and replication of the antigenomicRNA (4, 45, 46). Infectious viruses were harvested fromthe supernatant medium and amplified in BHK-21 cells at a lowmultiplicity of infection (MOI) to avoid formation of defectiveinterfering particles and in the presence of cytosine arabinoside(25 µg/ml) to suppress the replication of vaccinia virus. Supernatantmedium was filtered through 0.2-µm-pore-size filters, and thevirus was banded on 15 to 45% sucrose velocity gradients to separateit from any remaining vTF7-3. The gene orders of the recoveredviruses were confirmed by amplifying the rearranged portions ofthe genomes using reverse transcription and PCR followed by restrictionenzymeanalysis.

Analysis of viral protein synthesis. Viral protein synthesis directed by each of the variant viruses was measured in BHK-21 cells infected at an MOI of 50, withactinomycin D (5 µg/ml) added at 3 h postinfection. At 5 h postinfection,the cells were washed and incubated in methionine-free mediumfor 30 min. Cells were exposed to [³⁵S]methionine (30 µCi/ml; specific activity, 10.2 mCi/ml) for 1h. Cell monolayers were harvested directly into gel loading buffer;after normalizing for equal counts per minute, the viral proteinswere separated on 10% polyacrylamide gels using a low bisacrylamide-to-acrylamideratio to separate the P and N proteins. Viral proteins were quantitatedusing a phosphorimager, and their molar ratios werecalculated.

Analysis of virion proteins. To assess the quantity of each of the proteins in the mature virions, BHK-21 cells were infected at an MOI of 5. After 2 h,the cells were washed and incubated in methionine-free mediumfor 30 min. Cells were labeled with [³⁵S]methionine (50 µCi/ml; specific activity, 10.2 mCi/ml) overnight,with unlabeled methionine added to 10% of normal medium level.Supernatant fluid was collected, cell debris was removed by centrifugation,and virus was collected by centrifugation through 10% sucrose.After normalizing the counts per minute, the viral pellet wasresuspended in gel loading buffer and virion proteins were separatedon a 10% polyacrylamide gel. Virion proteins were quantitatedusing a phosphorimager, and the molar ratios weredetermined.

Single-cycle virus replication. BHK-21 cells were infected at an MOI of 3. After 1 h of adsorption, the inoculum was removed and the monolayer was washedtwice. Fresh medium was added, and the cells were incubated at37°C. Supernatant fluids were harvested at indicated intervalsover a 30-h period, and viral yields were determined by plaqueassay on Vero-76cells.

Lethality in mice. Male Swiss Webster mice, 3 to 4 weeks old, were purchased from Taconic Farms, Germantown, N.Y., and housed under BL2 containmentconditions. Groups of six mice were lightly anesthetized withketamine-xylazine and inoculated intranasally with 10-µl aliquotsof serial 10-fold viral dilutions of the individual viruses inDulbecco's modified Eagle medium. Control animals were given asimilar volume of DMEM. Animals were observed, and each groupwas weighed daily. The 50% lethal dose (LD₅₀) for each virus wascalculated by the method of Reed and Muench (33).

Determination of serum antibody levels and neutralization titers. After virus inoculation, blood was collected at weekly intervals from groups of two to four animals. Serum samples were pooledand heated to 57°C for 40 min to inactivate complement. Cell monolayersinfected with wt VSV (N1G4) and uninfected BHK-21 cells were lysedin detergent buffer (1% NP-40, 0.4% sodium deoxycholate, 66 mMEDTA, 10 mM Tris-HCl [pH 7.4]) and used as antigen in a directenzyme-linked immunosorbent assay (ELISA). Samples were seriallydiluted and detected using goat anti-mouse immunoglobulin conjugatedto horseradish peroxidase. The optical density (OD) was read at450 nm, and the antibody titers were calculated by linear regressionanalysis of a plot of OD versus serum dilution. The endpoint titers(log₁₀) were deduced at an OD 1.5 times that of the preimmunesamples. Serum neutralizing antibody titers on day of challengewere determined by a standard plaque reduction assay on Vero-76cells, and the titer was expressed as the reciprocal of the dilutiongiving 50%neutralization.

Protection of mice from wt challenge. Mice were immunized intranasally with doses of each virus ranging from 1 to 10,000 PFU in DMEM. Twenty-one days postinoculation,groups of mice that received nonlethal doses of each of the variantviruses were challenged intranasally with 5.4 × 10⁶ PFU of N1G4 (wt) virus. Challenged animals and controls weremonitored for a further 21 days. At weekly intervals, blood wascollected by tail bleeds for serum antibodytitrations.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Generation and recovery of rearranged viruses. In previous work we generated a full-length cDNA clone of the genome of VSV from which infectious virus was recovered (46).We subsequently developed a way to rearrange the order of thegenes at the cDNA level without introducing other changes intothe genome by using remote cutting restriction enzymes to cleavewithin the conserved sequences at the 3' and 5' ends of each gene(4). This strategy allowed us to recover viruses from rearrangedcDNAs in which the N gene had been moved to successively promoter-distalpositions in order to downregulate its expression (45). In thepresent work, we used this approach to generate cDNA clones inwhich the G gene was moved from its normal position of fourthin the gene order to the first, most promoter-proximal positionto determine if doing so would increase its expression. Two newgene rearrangements were generated: one in which the G gene wasmoved to first in the gene order and the remaining four geneswere left undisturbed to generate the order 3'-G-N-P-M-L-5' (G1N2),and the second in which the positions of the G and N genes wereexchanged to generate the order 3'-G-P-M-N-L-5' (G1N4) (Fig. 1).These cDNAs were transfected into cells as described previously(45), and virus was recovered in both cases. The recovered viruseswere designated G1N2 and G1N4, respectively, according to thepositions of the N and G genes in the rearranged gene order. Theproperties of these viruses were examined in comparison to a virusderived from a cDNA clone created using the same gene rearrangementprocess to regenerate the wt gene order (N1G4) and a virus withthe gene order 3'-P-M-G-N-L-5' (G3N4) (45).

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FIG. 1. Gene orders of N1G4 (wt), G1N2, G3N4, and G1N4. Le, leader; Tr, trailer.

Effect of gene rearrangement on viral protein expression. BHK-21 cells were infected with viruses with rearranged genomes, and the relative levels of viral protein synthesis were examinedby labeling for 1 h with [³⁵S]methionine at 5 h postinfection. Total cellular proteins wereresolved by sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE) and visualized by autoradiography. A typical gel isshown in Fig. 2A. Infection with wt VSV and the rearranged variantsresulted in rapid inhibition of host protein synthesis which allowedthe viral N, P, M, G, and L proteins to be detected directly.Synthesis of G protein was significantly increased relative tothe other viral proteins in cells infected with G1N2 and G1N4viruses (Fig. 2A, lanes 2 and 4) compared to wt (N1G4)-infectedcells (Fig. 2A, lane 1).

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FIG. 2. Synthesis of viral proteins in BHK-21 cells infected with the variant viruses. (A) BHK-21 cells were infected at an MOI of 50 and incubated at 37°C for 5 h in the presence of actinomycin D (5 µg/ml) for the final 2 h. Infected cells were then starved for methionine for 30 min and exposed to medium containing [³⁵S]methionine (30 µCi/ml) for 1 h. Total infected cell proteins were analyzed by SDS-PAGE. (B) Virions were isolated from supernatant fluids of BHK-21 cells infected at an MOI of 5 and exposed to [³⁵S]methionine (50 µCi/ml) from 2.5 to 12 h postinfection. Virus particles were purified by centrifugation through 10% sucrose, and their protein contents were determined by SDS-PAGE. Viral proteins shown in panels A and B were quantitated by phosphorimaging and expressed as molar percentages of each viral protein in infected BHK-21 cells (C) or purified virions (D). Data shown are averages from two independent experiments. Lanes: 1, N1G4 (wt); 2, G1N2; 3, G3N4; 4, G1N4; 5, uninfected cells.

Proteins were quantitated by phosphorimaging. The molar percentage of G protein synthesized during a 1-h labeling period was2.3-fold higher in G1N2-infected cells and 1.7-fold higher inG1N4-infected cells than in cells infected with wt virus. Similarly,translocation of the N gene from its promoter-proximal positionto a more distal position in viruses G1N2, G3N4, and G1N4 decreasedthe rate of N protein synthesis (Fig. 2C).

The protein contents of purified virus particles were also examined to determine if changes in protein synthesis in cellsaffected protein assembly into virions. BHK-21 cells were infectedwith each of the viruses and labeled with [³⁵S]methionine overnight, and virions were harvested from supernatantfluids and separated from cell debris by centrifugation through10% sucrose. Analysis of the virion proteins by SDS-PAGE (Fig.2B) showed no gross differences in the relative protein contents.Phosphorimager quantitation confirmed that despite the alteredrelative levels of protein synthesis in infected cells, the amountsof proteins in virions were similar to that of wild-type virusexcept for virus G1N2, in which the level of G was 1.6-fold higherthan in the wt virus or other rearranged viruses (Fig. 2D). Thisobservation is being investigatedfurther.

Virus replication in cell culture. Replication of the rearranged viruses under single-step growth conditions was examined in cultured BHK-21 cells infected atan MOI of 3 followed by incubation at 37°C. Supernatant fluidswere harvested at various times, and the virus yields were measuredby plaque assay. As described previously (45), translocationof the N gene away from the promoter-proximal position resultedin stepwise reduction of replication as the gene was moved furtherfrom the first position. Movement of N to the second position(G1N2) decreased replication 3-fold, whereas moving N to the fourthposition (G3N4) reduced replication as much as 1,000-fold (Fig.3). However, the two viruses with N in the fourth position (G3N4and G1N4) replicated to different levels under single-step growthconditions. We attribute this to the fact that the molar ratioof N to P, which is critical for optimal replication, was lessperturbed in G1N4 than G3N4. Measurement of the intracellularrates of protein synthesis 5 h after infection showed molar ratiosof N to P of 1:1.6 in cells infected with G1N4 and 1:1.8 in G3N4-infectedcells (Fig. 2C). An N:P molar ratio of between 1:0.5 and 1:1 isoptimal for replication (14, 29, 45), as shown by the N:Pratios of 1:0.7 in wt-infected cells and 1:0.8 for cells infectedwith G1N2. Both the wt virus and G1N2 have N directly followedby P in the gene order (Fig. 1). Too much or too little P relativeto N decreases replication significantly (14, 26, 28, 29);thus, in cells infected with G3N4, not only is N limiting, butalso the molar ratio of N:P is more than twice the optimal value.The kinetics of replication of G3N4 and G1N4 were delayed in comparisonto wt and G1N2. Single-step growth of G3N4 and G1N4 was not completeuntil 24 h postinfection, compared to 12 h for N1G4 and G1N2.It is unlikely that the overabundance of G in the infected cellwas responsible for this delay in replication since G1N2 showedno delay in replication relative to wild-type virus.

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FIG. 3. Single-step growth analysis. Viruses were assayed for the ability to replicate by single-step growth in BHK-21 cells at 37°C. Cells were infected at an MOI of 3, and samples of the supernatant medium were harvested at the indicated time points. Samples were titrated in duplicate by plaque assay on Vero-76 cells. Average virus yields per cell were determined at 24 h postinfection (inset).

Lethality in mice. Young mice provide a sensitive animal model for the study of neuropathology caused by VSV and its mutants, (24, 38, 42),and inoculation of mice with wt VSV via the intranasal route resultsin fatal encephalitis. We compared the pathogenesis of the rearrangedvariant viruses to that of wt (N1G4) virus after intranasal inoculationin 3 to 4 week-old Swiss-Webster mice. The doses that constitutedLD₅₀s were 100, 50, >100,000, and 19,000 PFU of N1G4, G1N2, G3N4,and G1N4,respectively.

All of the viruses were lethal for mice if given in sufficiently high doses, although the doses of G3N4 administered in theseexperiments did not reach the LD₅₀ seen previously (45). Ingeneral, the position of the N gene, the N:P ratio, and the resultinglevel of virus replication were major determinants of lethality.Viruses in which the N gene was moved away from the promoter requiredgreatly increased doses to constitute an LD₅₀. These results confirmedour previous observations with viruses N1 to N4 in which the Ngene was moved sequentially (45). However, the results presentedhere show that for viruses with N in the fourth position (G3N4and G1N4), both the replication ability and the LD₅₀ also wereaffected by the position of the Ggene.

The LD₅₀s reported here are expressed in terms of the viral titers on Vero-76 cells. These titers are about 10-fold higherthan titers on BSC-40 cells, as reported in our previous publications(4, 45). We changed cell lines because we discovered thatrearranging the gene order of VSV could affect the interactionsof the variant viruses with the interferon system (reference 23and unpublished results). BSC-40 cells are competent to produceinterferon after infection, while Vero cells are not (10). Therefore,changing to Vero cells circumvented possible differences in interferoninduction or sensitivity. Studies of the interactions of the rearrangedviruses with the interferon system are inprogress.

The first symptoms of sickness (a haunched posture and hind-limb paralysis) appeared 5 days after inoculation with both N1G4and G1N2 viruses, although the first deaths occurred earlier inanimals inoculated with N1G4 (Fig. 4). The viruses with N in thefourth position induced symptoms more slowly; at a dose of 1,000PFU per mouse, G3N4 caused neither morbidity nor mortality, asobserved before (45). In an attempt to detect subclinical signsof sickness, the groups of mice were weighed daily throughoutthe study period (Fig. 5). However, whereas the mice that showedsymptoms invariably lost weight and died, those that showed nosymptoms showed no weight differences from uninoculated controlanimals (Fig. 5). Similar results were observed after challengeof the inoculated mice with wt virus; all animals that developedsymptoms subsequently died, and those that did not develop symptomsalso showed no weight loss.

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FIG. 4. Pathogenesis in mice. The viruses shown were administered intranasally to groups of six mice at a dose of 1,000 PFU per mouse, and the animals were monitored daily for signs of morbidity and mortality. No further changes occurred after day 12.

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FIG. 5. Average weights of mice inoculated with the rearranged viruses. Groups of six mice were inoculated intranasally with serial 10-fold dilutions of N1G4 (wt), G1N2, G3N4, or G1N4 ranging from 10,000 to 1 PFU/animal. Control mice received inoculation medium alone. The vertical dotted line indicates day of challenge with 5.4 × 10⁶ PFU of wt virus per mouse. For each group, all living animals were weighed together and the average weight was determined. $black-lozenge$ , 10,000 PFU;

, 1,000 PFU; $black-triangle$ , 100 PFU;

, 10 PFU; *, 1 PFU; +, medium.

Serum antibody. To assess the effect of inoculation of viruses with rearranged G genes on the humoral immune response, mice were inoculatedintranasally with serial 10-fold dilutions of each of the variantviruses. Blood was collected at weekly intervals by tail bleed,and the level of serum antibody was determined by ELISA. Sincesurvival of the inoculation was a prerequisite for this experiment,only doses at or below the LD₅₀ were used. Translocation of theG gene changed the kinetics and magnitude of the antibody response(Fig. 6). Mice inoculated with wt virus made barely detectablelevels of antibody within 21 days, whereas animals that received100 PFU of G1N2 and G1N4, respectively, had significant antibodytiters by 14 and 7 days postinoculation. This accelerated andenhanced response can be seen most clearly by comparing the micethat received 100 PFU (Fig. 6). The results demonstrate that translocationof the G gene from the fourth to the first position enhanced thehumoral immune response to VSV. Mice given G1N4 synthesized antibodyearlier and at higher levels than those given G3N4. This furtherconfirmed the observation that putting the G gene first in thegene order increased the immunogenicity of VSV.

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FIG. 6. Kinetics of antibody production in response to inoculation with the rearranged and wt viruses. Groups of six mice were inoculated intranasally with serial 10-fold dilutions of N1G4 (wt), G1N2, G3N4, or G1N4 ranging from 10,000 to 1 PFU/animal. Control mice received inoculation medium only. The vertical dotted line indicates the day of challenge with 5.4 × 10⁶ PFU of wt virus per mouse. Serum was collected by tail bleeds from two to four animals at weekly intervals, the serum samples were pooled, and the level of antibody raised against VSV was determined by titration on detergent-lysed VSV-infected cell antigen in an ELISA. Antibody levels are expressed as log₁₀ titers. $black-lozenge$ , 10,000 PFU;

, 1,000 PFU; $black-triangle$ , 100 PFU;

, 10 PFU; *, 1 PFU.

Twenty-one days postinoculation, the mice were challenged with 5.4 × 10⁶ PFU of wt VSV. A rapid increase in antibody titer was observedin animals given either N1G4 or G1N2, although there was no furtherrise in the already high titers that had been achieved prior tochallenge in mice inoculated with G3N4 orG1N4.

Neutralizing antibody titer after inoculation. The level of neutralizing antibody in the serum at the time of challenge was measured. In mice and cattle, neutralizing antibodiesare an important element in protection against VSV infection (12,20, 22). On the day of challenge, mice were bled and serumsamples were assayed for the ability to neutralize wt VSV in astandard plaque reduction assay on Vero-76 cells. The reciprocalof the highest dilution that gave a 50% reduction of plaque numberswas calculated to determine the neutralizing titers of thesera.

All of the viruses with rearranged genomes elicited serum neutralizing antibody in mice (Fig. 7A). Neutralizing antibody wasnot detected at a dose of 1 or 10 PFU/mouse of either N1G4 orG1N2, but both viruses elicited detectable titers at doses of100 PFU, the response to G1N2 being 10-fold higher than that towt virus. Thus, for N1G4 and G1N2, the level of neutralizing antibodydid not correlate with virus replication in cell culture, wherethe wt virus replicated two- to threefold more abundantly thanG1N2 (Fig. 3). This conclusion was reinforced by the responseto G3N4 and G1N4, which elicited approximately 10-fold-highertiters than the wt virus despite greatly reduced replication potential.

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FIG. 7. Groups of six mice were inoculated intranasally with serial 10-fold dilutions of N1G4 (wt), G1N2, G3N4, or G1N4 ranging from 10,000 to 1 PFU/animal. Control mice received inoculation medium only. (A) Neutralizing antibody levels as measured in serum samples on the day of challenge by plaque reduction assay. Neutralizing antibody levels are expressed as the reciprocal of the highest dilution giving a 50% reduction in wt virus plaques on Vero-76 cells. Asterisks denote that sera from animals given 1 or 10 PFU of N1G4 or G1N2 virus had background levels of neutralizing antibody. (B) Ability to survive intranasal challenge by 5.4 × 10⁶ PFU of N1G4 virus. The dotted line shows the lethality of this dose (83%) in unvaccinated, age-matched, control animals 21 days after challenge.

In summary, viruses which overexpressed G and underexpressed N in infected cells yielded increased levels of neutralizingantibody compared to wt virus (N1G4) following intranasal inoculation.The combination of overexpressing G and underexpressing N combinedthis enhanced immunogenicity with virus attenuation, which allowedthe administration of higher doses that elicited correspondinglyhigher titers of neutralizing antibodies. Moreover, because ofthe lower lethality of these viruses, 100 times more virus couldbe administered without detriment, and under these conditionsthey elicited up to 100-fold more neutralizing antibody than couldbe attained in response to wtvirus.

Protection of mice from challenge. These results establish that nonpathogenic doses of the viruses that overexpressed G protein could elicit significant humoralimmune responses in mice. To see whether immunization with therearranged viruses could confer protection against VSV disease,animals that survived inoculation with each of the rearrangedviruses were challenged after 21 days with 5.4 × 10⁶ PFU of wt virus. This dose was sufficient to kill 83% of theuninoculated, age-matched, control group ofanimals.

All of the viruses with rearranged genomes conferred protection, the level of which varied with the dose of inoculum (Fig.7B). The levels of protection elicited by N1G4 and G1N2 were alike,reflecting the comparable levels of replication and lethalityof these viruses described previously (Fig. 3; see also "Lethalityin mice," above). Similarly, the protection conferred by G1N4resembled that of G3N4. By 21 days postinoculation, both viruseselicited solid immunity at doses of 1,000 PFU per mouse. Importantly,these fully protective doses were 20- to 100-fold less than thecorresponding LD₅₀s. This emphasizes the conclusion that generearrangement is an effective method to systematically changethe phenotype of VSV to optimize the properties required of alive attenuatedvaccine.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The recovery of infectious viruses from cDNA clones of the Mononegavirales permits experimental manipulation of the viralgenome (8, 9). Gene expression in these viruses is controlledat the transcriptional level by the order of the genes relativeto the single promoter at the 3' end of the viral genome (15,41). We developed a method to rearrange the order of the geneswithout introducing other changes into the genome (4, 45).Gene rearrangement altered the relative levels of synthesis ofthe viral proteins, as expected, and produced infectious viruseshaving a variety of different phenotypes. In previous work weshowed that moving the N gene from its promoter-proximal positionto more distal positions resulted in a stepwise decrease in Nprotein synthesis, viral RNA replication, infectious virus production,and lethality of the variant viruses for mice (45). The presentstudies examined the consequences of moving the G protein gene,which encodes the major neutralizing epitopes of the virus, fromits promoter-distal position to first in the gene order. As predictedby our previous work, expression of G protein in infected cellswas significantly increased when its gene was moved from the fourthto the first position. However, the protein content of the purifiedvirus particles was largely unaffected by changes in the viralgene order. Any differences that may exist were at the limitsof the quantitation methods used in this study and will requirethe application of more precisetechniques.

The overexpression of G protein by these viruses allowed us to explore whether they elicited an altered humoral immune responsein animals. The data in Fig. 6 show that at an inoculum dose of100 PFU, antibody was produced more quickly and at higher levelsin animals infected with the viruses with G moved to a promoter-proximalposition compared to the wt virus. Doses higher than 100 PFU couldnot be assayed with the N1G4 (wt) and G1N2 viruses because oftheir lethality. At the dose of 100 PFU, viruses G1N2, G3N4, andG1N4 all elicited higher antibody titers more rapidly than N1G4.The reduced lethality of the G1N4 and G3N4 viruses allowed higherdoses to be administered, and in these cases antibody levels increasedmore rapidly than at lowerdoses.

The observation that all three viruses which had G moved closer to the promoter elicited an enhanced humoral immune responsein mice has implications for our understanding of protective immunityin this system. Although we do not know the relative levels ofreplication of the variant inocula in the cells that are mostrelevant for induction of the immune response, it seems likelythat they mirrored, at least qualitatively, the relative levelsof replication seen in cell culture. If this is the case, G1N2,G3N4, and G1N4 expressed higher levels of G protein per inoculatedmouse only during the first round of replication. After that,the more robust replication of the wt virus should have more thancompensated for its weaker G protein synthesis. Yet at the sameinoculated dose of 100 PFU per mouse, the variant viruses elicitedan enhanced and accelerated humoral immune response compared tothe wt-inoculatedanimals.

The results suggest that the kinetics and magnitude of the humoral immune response become established very early in infection.Either there is a short temporal window during which the scaleof the immune response becomes established irrevocably or theimmune response to VSV infection is somehow determined by thelevel of G protein synthesis per infected cell rather than bythe aggregate immunogenic load. A similar conclusion is suggestedby the efficacy of vaccines using recombinant canarypox vectorsunder conditions where they are unable to replicate (25). Robustsynthesis of antigen by a highly attenuated vector appears tobe an effective vaccine strategy that warrants furtherexploration.

Studies outside the scope of this report are under way to investigate the types and subtypes of antibodies produced by thevariant viruses and to investigate T-cell responses and localizationof the viruses following infection. It is difficult to compareour present work with that of others on the pathogenesis of VSVin mice and the complexities of the immune response because ofsignificant differences in the ages and strains of the experimentalanimals as well as in the routes of inoculation and challenge(12, 20, 36). In the work presented here, we used the Swiss-Webstermouse model of VSV established by Sabin and Olitsky (38) andWagner (42), and all experiments were controlled relative tothe action of the wtvirus.

In agreement with previous findings, we observed that the position of the N gene and the level of N protein expression correlatedwith efficiency of replication because the N protein is requiredin stoichiometric amounts for genomic RNA replication. The wtvirus N1G4 replicated to the highest titers, followed by G1N2virus and finally G1N4 and G3N4, which replicated least well.G1N4, however, replicated significantly better than G3N4, althoughthey both had the N gene in the fourth position. Both of theseviruses showed delayed replication kinetics, as might be expectedif the formation of progeny virus was limited by the supply ofNprotein.

It is known that the relative levels of N and P proteins, in addition to the absolute amount of N protein, are critical forefficient replication (14, 29). One function of P proteinis to maintain N in a soluble state such that it is able to supportencapsidation of newly replicated RNA (14, 44). Consistentwith this, G1N2 virus, while having reduced N protein expression(Fig. 2A and C), had the N and P genes in the same relative orderas the N1G4 (wt) (Fig. 1). Accordingly, G1N2 expressed the N andP proteins at about the same relative rates as wt virus, 1:0.8and 1:0.7, respectively. In agreement with this, G1N2 replicatedonly slightly less than N1G4. Further to this point, althoughG1N4 and G3N4 both had N in the fourth position, G1N4 replicatedsubstantially better than G3N4 (Fig. 3). The ratio between therates of synthesis of N and P proteins was disparate from thewt value in both of these viruses. However, G3N4, which had Pin the first position, had an N:P ratio in infected cells of 1:1.8,whereas the N:P ratio in cells infected with G1N4, where P wasin the second position, was 1:1.6, closer to that of wt virus.There was also a difference between these two viruses in the ratesof G protein expression, and it is possible that increased levelsof G protein provided an advantage for replication ofG1N4.

The reduced lethality of the viruses with gene rearrangements was also consistent with our previous work showing that attenuationof lethality in mice correlated with reduced replication capacity.Reduced replication, in turn, was related to the overall expressionlevels of N protein and the N:P ratio as discussed above. Obviouslyany gene rearrangement which brings the G gene to the first positionwill displace the N gene from its wt position and therefore decreaseN protein expression. It will also alter the molar ratios of proteinswhose gene positions relative to one another are changed by therearrangement in question. Both types of change would be expectedto alter replication efficiency and lethality. As noted in Results,the viruses which replicated best, wt and G1N2, required only50 to 100 PFU to constitute an LD₅₀, whereas 200 and 1,000 timesmore G1N4 and G3N4, respectively, were required for an LD₅₀. Thedata presented here show that rearrangement of genes allowed themanipulation of two important aspects of the viral phenotype,lethality and the stimulation of neutralizing antibody. By reducingN protein expression and altering the N:P ratio, it was possibleto decrease replication potential and lethality for animals; byincreasing G protein expression, it was possible to alter thekinetics and level of antibodysynthesis.

These results expand on our earlier demonstration that gene rearrangement can be used to generate viruses with novel, beneficialphenotypes. This approach provides the ability to alter the phenotypein a stepwise manner to achieve a desired level of attenuationor to alter the expression of a particular gene. It allows thelevel of attenuation and immunogenicity to be modulated independentlyand systematically, exactly what is needed to generate and manipulatelive attenuated vaccine candidates. This approach should be applicableto other members of the Mononegavirales, all of which have a commonmechanism for the control of gene expression via obligatorilysequential transcription originating from a single 3' promoter.Furthermore, viruses of the Mononegavirales have not been foundto undergo homologous recombination; therefore, changes made tothe gene order should be irreversible by natural processes (30,32). Several foreign genes have been expressed from VSV (16,18, 34, 39), and in one study mice were protected againstthe corresponding pathogen (34). These properties make thisvirus an excellent candidate in which to generate future vaccinesdirected against VSV itself or against other pathogens. Studiesdesigned to evaluate the pathogenesis and immunogenicity of theG1N2, G3N4, and G1N4 viruses in a natural host are underway.

	ACKNOWLEDGMENTS

This work was supported by Public Health Service grants R37 AI 12464 to G.W.W. and R37 AI 18270 to L.A.B.

We thank Claire Hankin for experimental assistance and the members of the Wertz and Ball laboratories for constructivecomments.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, The Medical School, University of Alabama at Birmingham,BBRB 17 Room 366, 845 19th St., South, Birmingham, AL 35294. Phone:(205) 934-0453. Fax: (205) 934-1636. E-mail: gail_wertz{at}microbio.uab.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Abraham, G., and A. K. Banerjee. 1976. Sequential transcription of the genes of vesicular stomatitis virus. Proc. Natl. Acad. Sci. USA 73:1504-1508[Abstract/Free Full Text].

2. Arnheiter, H., N. L. Davis, G. Wertz, M. Schubert, and R. A. Lazzarini. 1985. Role of the nucleocapsid protein in regulating vesicular stomatitis virus RNA synthesis. Cell 41:259-267[CrossRef][Medline].

3. Ball, L. A., and C. N. White. 1976. Order of transcription of genes of vesicular stomatitis virus. Proc. Natl. Acad. Sci. USA 73:442-446[Abstract/Free Full Text].

4. Ball, L. A., C. P. Pringle, B. Flanagan, V. P. Perepelitsa, and G. W. Wertz. 1999. Phenotypic consequences of rearranging the P, M, and G genes of vesicular stomatitis virus. J. Virol. 73:4705-4712[Abstract/Free Full Text].

5. Barr, J. N., S. P. J. Whelan, and G. W. Wertz. 1997. Role of the intergenic dinucleotide in vesicular stomatitis virus RNA transcription. J. Virol. 71:1794-1801[Abstract].

6. Bridges, V. E., B. J. McCluskey, M. D. Salman, H. S. Hurd, and J. Dick. 1997. Review of the 1995 vesicular stomatitis outbreak in the western United States. J. Am. Vet. Med. Assoc. 211:556-560[Medline].

7. Burkhart, C., G. Freer, R. Castro, L. Adorini, K.-H. Wiesmüller, R. M. Zinkernagel, and H. Hengartner. 1994. Characterization of T-helper epitopes of the glycoprotein of vesicular stomatitis virus. J. Virol. 68:1573-1580[Abstract/Free Full Text].

8. Conzelmann, K.-K. 1996. Genetic manipulation of non-segmented negative-strand RNA viruses. J. Gen. Virol. 77:381-389[Abstract/Free Full Text].

9. Conzelmann, K.-K. 1998. Nonsegmented negative-strand RNA viruses: genetics and manipulation of viral genomes. Annu. Rev. Genet. 32:123-162[CrossRef][Medline].

10. Desmyter, J., J. L. Melnick, and W. E. Rawls. 1968. Defectiveness of interferon production and of rubella virus interference in a line of African green monkey kidney cells (Vero). J. Virol. 2:955-961[Abstract/Free Full Text].

11. Fuerst, T. R., E. G. Niles, F. W. Studier, and B. Moss. 1986. Eukaryotic transient-expression system based on recombinant vaccinia virus that synthesizes bacteriophage T7 RNA polymerase. Proc. Natl. Acad. Sci. USA 83:8122-8126[Abstract/Free Full Text].

12. Gobet, R., A. Cerny, E. Rüedi, H. Hengartner, and R. M. Zinkernagel. 1988. The role of antibodies in natural and acquired resistance of mice to vesicular stomatitis virus. Exp. Cell Biol. 56:175-180[Medline].

13. Hayek, A. M., B. J. McCluskey, G. T. Chavez, and M. D. Salman. 1998. Financial impact of the 1995 outbreak of vesicular stomatitis on 16 beef ranches in Colorado. J. Am. Vet. Med. Assoc. 212:820-823[Medline].

14. Howard, M., and G. Wertz. 1989. Vesicular stomatitis virus RNA replication: a role for the NS protein. J. Gen. Virol. 70:2683-2694[Abstract/Free Full Text].

15. Iverson, L. E., and J. K. Rose. 1981. Localization attenuation and discontinuous synthesis during vesicular stomatitis virus transcription. Cell 23:477-484[CrossRef][Medline].

16. Kahn, J. S., M. J. Schnell, L. Buonocore, and J. K. Rose. 1999. Recombinant vesicular stomatitis virus expressing the respiratory syncytial virus (RSV) glycoproteins: RSV fusion protein can mediate infection and cell fusion. Virology 254:81-91[CrossRef][Medline].

17. Kelley, J. R., S. U. Emerson, and R. R. Wagner. 1972. The glycoprotein of vesicular stomatitis virus is the antigen that gives rise to and reacts with neutralizing antibody. J. Virol. 10:1231-1235[Abstract/Free Full Text].

18. Kretzschmur, E., L. Buonocore, M. J. Schnell, and J. K. Rose. 1997. High-efficiency incorporation of functional influenza virus glycoproteins into recombinant vesicular stomatitis viruses. J. Virol. 71:5982-5989[Abstract].

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20. Lefrancois, L. 1984. Protection against lethal viral infection by neutralizing and nonneutralizing monoclonal antibodies: distinct mechanisms of action in vivo. J. Virol. 51:208-214[Abstract/Free Full Text].

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22. Mackett, M., T. Yilma, J. K. Rose, and B. Moss. 1985. Vaccinia virus recombinants: expression of VSV genes and protective immunization of mice and cattle. Science 227:433-435[Abstract/Free Full Text].

23. Marcus, P. I., M. J. Sekellick, L. A. Ball, and G. W. Wertz. 1999. Phenotypic variation in the interferon-inducing capacity of vesicular stomatitis virus with rearranged genomes. J. Interferon Res. 19:S101.

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40. USDA Animal and Plant Health Inspection Service-Veterinary Services, Centers for Epidemiology and Animal Health. 1997. 1997 vesicular stomatitis virus (VSV) outbreak in the United States. DxMonitor Anim. Health Rep. Fall:1-2.

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1.	Abraham, G., and A. K. Banerjee. 1976. Sequential transcription of the genes of vesicular stomatitis virus. Proc. Natl. Acad. Sci. USA 73:1504-1508[Abstract/Free Full Text].
2.	Arnheiter, H., N. L. Davis, G. Wertz, M. Schubert, and R. A. Lazzarini. 1985. Role of the nucleocapsid protein in regulating vesicular stomatitis virus RNA synthesis. Cell 41:259-267[CrossRef][Medline].
3.	Ball, L. A., and C. N. White. 1976. Order of transcription of genes of vesicular stomatitis virus. Proc. Natl. Acad. Sci. USA 73:442-446[Abstract/Free Full Text].
4.	Ball, L. A., C. P. Pringle, B. Flanagan, V. P. Perepelitsa, and G. W. Wertz. 1999. Phenotypic consequences of rearranging the P, M, and G genes of vesicular stomatitis virus. J. Virol. 73:4705-4712[Abstract/Free Full Text].
5.	Barr, J. N., S. P. J. Whelan, and G. W. Wertz. 1997. Role of the intergenic dinucleotide in vesicular stomatitis virus RNA transcription. J. Virol. 71:1794-1801[Abstract].
6.	Bridges, V. E., B. J. McCluskey, M. D. Salman, H. S. Hurd, and J. Dick. 1997. Review of the 1995 vesicular stomatitis outbreak in the western United States. J. Am. Vet. Med. Assoc. 211:556-560[Medline].
7.	Burkhart, C., G. Freer, R. Castro, L. Adorini, K.-H. Wiesmüller, R. M. Zinkernagel, and H. Hengartner. 1994. Characterization of T-helper epitopes of the glycoprotein of vesicular stomatitis virus. J. Virol. 68:1573-1580[Abstract/Free Full Text].
8.	Conzelmann, K.-K. 1996. Genetic manipulation of non-segmented negative-strand RNA viruses. J. Gen. Virol. 77:381-389[Abstract/Free Full Text].
9.	Conzelmann, K.-K. 1998. Nonsegmented negative-strand RNA viruses: genetics and manipulation of viral genomes. Annu. Rev. Genet. 32:123-162[CrossRef][Medline].
10.	Desmyter, J., J. L. Melnick, and W. E. Rawls. 1968. Defectiveness of interferon production and of rubella virus interference in a line of African green monkey kidney cells (Vero). J. Virol. 2:955-961[Abstract/Free Full Text].
11.	Fuerst, T. R., E. G. Niles, F. W. Studier, and B. Moss. 1986. Eukaryotic transient-expression system based on recombinant vaccinia virus that synthesizes bacteriophage T7 RNA polymerase. Proc. Natl. Acad. Sci. USA 83:8122-8126[Abstract/Free Full Text].
12.	Gobet, R., A. Cerny, E. Rüedi, H. Hengartner, and R. M. Zinkernagel. 1988. The role of antibodies in natural and acquired resistance of mice to vesicular stomatitis virus. Exp. Cell Biol. 56:175-180[Medline].
13.	Hayek, A. M., B. J. McCluskey, G. T. Chavez, and M. D. Salman. 1998. Financial impact of the 1995 outbreak of vesicular stomatitis on 16 beef ranches in Colorado. J. Am. Vet. Med. Assoc. 212:820-823[Medline].
14.	Howard, M., and G. Wertz. 1989. Vesicular stomatitis virus RNA replication: a role for the NS protein. J. Gen. Virol. 70:2683-2694[Abstract/Free Full Text].
15.	Iverson, L. E., and J. K. Rose. 1981. Localization attenuation and discontinuous synthesis during vesicular stomatitis virus transcription. Cell 23:477-484[CrossRef][Medline].
16.	Kahn, J. S., M. J. Schnell, L. Buonocore, and J. K. Rose. 1999. Recombinant vesicular stomatitis virus expressing the respiratory syncytial virus (RSV) glycoproteins: RSV fusion protein can mediate infection and cell fusion. Virology 254:81-91[CrossRef][Medline].
17.	Kelley, J. R., S. U. Emerson, and R. R. Wagner. 1972. The glycoprotein of vesicular stomatitis virus is the antigen that gives rise to and reacts with neutralizing antibody. J. Virol. 10:1231-1235[Abstract/Free Full Text].
18.	Kretzschmur, E., L. Buonocore, M. J. Schnell, and J. K. Rose. 1997. High-efficiency incorporation of functional influenza virus glycoproteins into recombinant vesicular stomatitis viruses. J. Virol. 71:5982-5989[Abstract].
19.	Kündig, T. M., I. Castelmur, M. F. Bachmann, D. Abraham, D. Binder, H. Hengartner, and R. M. Zinkernagel. 1993. Fewer protective cytotoxic T-cell epitopes than T-helper cell epitopes on vesicular stomatitis virus. J. Virol. 67:3680-3683[Abstract/Free Full Text].
20.	Lefrancois, L. 1984. Protection against lethal viral infection by neutralizing and nonneutralizing monoclonal antibodies: distinct mechanisms of action in vivo. J. Virol. 51:208-214[Abstract/Free Full Text].
21.	Lefrancois, L., and D. S. Lyles. 1982. The interaction of antibody with the major surface glycoprotein of vesicular stomatitis virus. I. Analysis of neutralizing epitopes with monoclonal antibodies. Virology 121:157-167[CrossRef][Medline].
22.	Mackett, M., T. Yilma, J. K. Rose, and B. Moss. 1985. Vaccinia virus recombinants: expression of VSV genes and protective immunization of mice and cattle. Science 227:433-435[Abstract/Free Full Text].
23.	Marcus, P. I., M. J. Sekellick, L. A. Ball, and G. W. Wertz. 1999. Phenotypic variation in the interferon-inducing capacity of vesicular stomatitis virus with rearranged genomes. J. Interferon Res. 19:S101.
24.	Miyoshi, K., D. H. Harter, and K. C. Hsu. 1971. Neuropathological and immunofluorescence studies of experimental vesicular stomatitis encephalitis in mice. J. Neuropathol. Exp. Neurol. 30:266-277[Medline].
25.	Paoletti, E. 1996. Applications of poxvirus vectors to vaccination: an update. Proc. Natl. Acad. Sci. USA 93:11349-11353[Abstract/Free Full Text].
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