DNA Immunization with Japanese Encephalitis Virus Nonstructural Protein NS1 Elicits Protective Immunity in Mice

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J Virol, January 1998, p. 191-200, Vol. 72, No. 1
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

DNA Immunization with Japanese Encephalitis Virus Nonstructural Protein NS1 Elicits Protective Immunity in Mice

Yi-Ling Lin,¹^,²^,^* Li-Kuang Chen,¹^,² Ching-Len Liao,¹^,² Chia-Tsui Yeh,¹ Shiou-Hwa Ma,¹ Jin-Ling Chen,² Yue-Ling Huang,¹ Shih-Shun Chen,² and Hsien-Yuan Chiang¹^,²

Institute of Preventive Medicine¹ and Department of Microbiology and Immunology,² National Defense Medical Center, Taipei, Taiwan, Republic of China

Received 17 June 1997/Accepted 1 October 1997

	ABSTRACT

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Japanese encephalitis virus (JEV), a mosquito-borne flavivirus, is a zoonotic pathogen that is prevalent in some SoutheastAsian countries and causes acute encephalitis in humans. To evaluatethe potential application of gene immunization to JEV infection,we characterized the immune responses from mice intramuscularlyinjected with plasmid DNA encoding JEV glycoproteins, includingthe precursor membrane (prM) plus envelope (E) proteins and thenonstructural protein NS1. When injected with the plasmid expressingprM plus E, 70% of the immunized mice survived after a lethalJEV challenge, whereas when immunized with the plasmid expressingNS1, 90% of the mice survived after a lethal challenge. As a control,the mice immunized with the DNA vector pcDNA3 showed a low level(40%) of protection, suggesting a nonspecific adjuvant effectof the plasmid DNA. Despite having no detectable neutralizingactivity, the NS1 immunization elicited a strong antibody responseexhibiting cytolytic activity against JEV-infected cells in acomplement-dependent manner. By contrast, immunization with aconstruct expressing a longer NS1 protein (NS1'), containing anextra 60-amino-acid portion from the N terminus of NS2A, failedto protect mice against a lethal challenge. Biochemical analysesrevealed that when individually expressed, NS1 but not NS1' couldbe readily secreted as a homodimer in large quantity and couldalso be efficiently expressed on the cell surface. Interestingly,when NS1 and NS1' coexisted in cells, the level of NS1 cell surfaceexpression was much lower than that in cells expressing NS1 alone.These data imply that the presence of partial NS2A might havea negative influence on an NS1-based DNA vaccine. The resultsherein clearly illustrate that immunization with DNA expressingNS1 alone is sufficient to protect mice against a lethal JEV challenge.

	INTRODUCTION

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Japanese encephalitis virus (JEV), a member of the family Flaviviridae, is transmitted to humans by infected mosquitoes andcauses acute encephalitis with fatality rates ranging from 20%to as high as 50% (3, 47). The JEV genome is a single-stranded,positive-sense RNA of approximately 11 kb which contains a singleopen reading frame encoding a polyprotein. In infected cells,this viral polyprotein is proteolytically cleaved into at least11 proteins. The virus structural proteins, including the capsid(C), membrane (M; precursor M [prM]), and envelope (E), are encodedby the 5' one-third of the open reading frame, and the nonstructural(NS) proteins, designated NS1 through NS5, are encoded in theremainder (reviewed in references 5 and 41). NS1 has a predictedmolecular mass of 40 kDa; because there are N-linked carbohydratechains at positions 130 and 207, the actual molecular mass ofNS1 detected in JEV-infected cells is approximately 46 kDa. Theproteolytic cleavage of E-NS1 ensues as a result of the translocationof NS1 into the lumen of the endoplasmic reticulum ER, and thecleavage of NS1-2A is thought to take place in the lumen of thevesicular compartments (5). An additional NS1-2A-related protein(named NS1'), with a molecular mass of 53 kDa, is often observedin JEV-infected cells (30) and is presumably generated by anunknown protease which recognizes an alternative cleavage sitewithin NS2A (5).

Three of the flavivirus proteins (prM, E, and NS1) are glycosylated and have been reported to be capable of inducing protectiveimmunity (reviewed in reference 34). The E protein, a majorstructural protein of flavivirus virions, appears to play a dominantrole in the generation of neutralizing antibodies and the inductionof a protective immune response (2, 20). The prM proteinis part of the immature virions, and at the late stages of infection,its proteolytic cleavage to M protein generates mature virions.However, in certain instances this prM cleavage may not be complete,thus allowing the prM protein to be an additional target on virionsfor neutralizing antibodies (1). In addition to the structuralproteins, the flavivirus NS1, which is expressed on the surfaceof and secreted extracellularly from infected cells (reviewedin reference 41), not only is able to elicit an immune responseduring the course of flavivirus infections but also confers protectionin experimental animals (reviewed in reference 34). This protectivephenomenon seems to be dependent on the Fc portion of antibodies,since such NS1-specific antibodies kill infected target cellsin a complement-dependent manner (44, 45). One proposed advantagefor employing flavivirus NS1 as a subunit vaccine (14) ratherthan conventional killed JEV vaccines is that NS1 is able to elicitprotective immunity in the host without adverse effects involvingantibody-dependent enhancement (17).

Effective vaccines to control JEV have been successfully developed by formalin inactivation of JEV cultured in mouse brains.Since the inception of vaccination programs for humans, casesof Japanese encephalitis in many areas such as Japan, Korea, andTaiwan have been greatly reduced (19, 36, 37). However,one of the major problems associated with the use of inactivatedJEV vaccines is the lack of long-term immunity (24). To obtaineffective protection, multiple boosts of inactivated JEV vaccineare routinely required, making the vaccination program costly;in addition, repeated immunizations with killed vaccines preparedfrom mouse brains may cause hypersensitivity reactions in vaccinees.Therefore the World Health Organization has recently designatedJEV vaccine a high-priority target for further research and development.

DNA-based vaccines have recently been shown to induce protective immune responses against several viral agents, such as humanimmunodeficiency virus (49, 50), bovine and human herpesviruses(9, 32), hepatitis B virus (10), influenza virus (13,40, 42, 46), rabies virus (51), hepatitis C virus (25,28), measles virus (4), St. Louis encephalitis virus (38),and murine cytomegalovirus (15). Endogenous expression of antigenfrom DNA introduced into host cells leads to the production ofstructurally and conformationally relevant molecules of the antigenthat are able to be presented by major histocompatibility complexclasses I and II to activate specific immunity. This cellularprocess of antigen presentation, in some aspects, resembles thenatural course of viral infection. Indeed, in immunized hostswith expressible virus DNA, a broad spectrum of immune responseshave been observed, including antibodies, cytotoxic T cells, andhelper T cells, as well as protections against challenge withvarious viruses. The possession of such capacity by the vaccinesappears to be particularly crucial for developing DNA vaccinesto control viral diseases.

To assess the feasibility of DNA vaccination for JEV infection, in this study we characterized the immunogenicity and theprotective capability of plasmid DNA expressing either prM plusE, NS1, or NS1' with mice as an animal model. Our results revealedthat the plasmid expressing NS1, but not its longer derivativeNS1', could induce protective immunity as effectively as couldthe construct expressing prM plus E. However, our data suggeststhat the protective mechanisms involved in the NS1 and prME constructsappear to be different. In addition, as a result of comparisonof the biochemical properties between recombinant NS1 and NS1'expressed in cultured cells, we suggest that the ability of JEVglycoproteins to be readily secreted from and effectively expressedon the surface of cells appears to be a pivotal determinant fortheir ability to act as effective and potent immunogens. The possiblerole of NS2A in down-regulating the efficacy of an NS1-based genevaccine is also discussed. The present results not only suggestthat DNA immunization can be a potential vaccine approach butalso illustrate that gene immunization with JEV NS1 alone is adequateto protect mice against JEV infection.

	MATERIALS AND METHODS

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Viruses and cell lines. The Taiwanese local JEV strain NT109 (7), isolated from infected Culex tritaeniorhynchus mosquitoes in 1985, and strainNT113, isolated from infected Culex annulus mosquitoes in 1985,were used for the cloning of JEV genes. A neurovirulent JEV strain,RP-9 (7), was used in the challenge experiments. Virus propagationwas carried out with BHK-21 cells in RPMI 1640 medium containing2% fetal calf serum (GIBCO). Virus titers were determined by aplaque-forming assay on BHK-21 cells.

Construction of plasmids expressing JEV proteins. For the expression of JEV prM and E proteins, a cDNA fragment of 2,058 bp was amplified from strain NT113 by reverse transcription-PCR(6) with the primer set 5'-GCGGATCCAGAAGGCTCAATCATGTGGCT-3'(positive sense) and 5'-GACGCAAGCTTGCTAAGCATGCACATTGGTCG-3' (negativesense), which hybridize to nucleotides (nt) 420 to 439 and 2461to 2477, respectively. This fragment comprised the coding regionsfor both prM and E, as well as the region encoding a 15-amino-acidsignal peptide derived from the C terminus of C protein. The cDNAfragment was cloned into a PCR cloning vector, pCRII (Invitrogen),and then the EcoRI insert fragment was excised and subcloned intoa eucaryotic expression vector, pcDNA3 (Invitrogen), in whichprME is under the control of the enhancer-promoter sequences ofthe immediately-early gene of human cytomegalovirus. The resultingplasmid construct was named pJME (Fig. 1).

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FIG. 1. Schematic diagram of plasmid constructs expressing various JEV glycoproteins in the mammalian expression vector. The numbers with straight or bent arrows are the nucleotide positions on the JEV genome.

JEV NS1 and NS1' cDNA fragments were generated by reverse transcription-PCR amplification of the genomic RNA of strain NT109.Two different 3' primers were used for the NS1 or NS1' constructionsin the first-strand cDNA synthesis step: 5'-GCGGATCCTAAGCATCAACCTGTGA-3',complementary to nt 3519 to 3533 in the NS1 region, and 5'-CGCTATAGCACCACATACC-3',complementary to nt 3700 to 3713 in the NS1' region. The same5' primer was used for both constructions during the PCR step:5'-GCACCATGGGCGTCAACGCA-3', hybridizing to nt 2388 to 2402. TheNS1 cDNA fragment was first cloned to a ddT-tailed, EcoRV-digestedpBluescript (Stratagene) generated by a published method (29),and the correct insert was then subcloned to an expression vectorpcDNA3 (Invitrogen). The NS1' cDNA fragment was directly clonedinto an expression vector, pCR3 (Invitrogen), by the TA cloningmethod. The resulting constructs were named pJNS1 and pJNS1' (Fig.1); they both encode a so-called signal peptide of 30 amino acidsderived from the C terminus of E protein. Plasmid pJNS1' is almostidentical to pJNS1, except that the coding sequence of the formerwas extended into the NS2A region with 60 amino acids.

RIP. Briefly, for radioimmunoprecipitation (RIP), BHK-21 cells were infected with virus at a multiplicity of infection (MOI) of5. At 24 h postinfection, the medium was removed, replaced withwarm methionine (Met)- and cystein (Cys)-free RPMI 1640 mediumcontaining 100 µCi of [³⁵S]Pro-mix (Amersham) per ml plus 2% dialyzed fetal bovine serum(GIBCO), and incubated for 2 h at 37°C. The culture fluids wereremoved, and the cell layers were rinsed with ice-cold phosphate-bufferedsaline (PBS) and harvested in lysis buffer (1% Nonidet P-40, 150mM NaCl, 50 mM Tris-HCl [pH 7.5], 1 mM EDTA) containing a cocktailof protease inhibitors (20 µg of phenylmethylsulfonyl fluorideper ml, 2 µg of leupeptin per ml, 2 µg of aprotinin per ml). Aspositive controls, ascitic fluids containing monoclonal antibody(MAb) specific for the JEV NS1 proteins (6) were used in RIP.The tested serum samples were first incubated with a mixture ofprotein A-Sepharose and protein G-Sepharose (Pharmacia) at roomtemperature for 1 h; the ³⁵S-labeled cell lysates were then added and incubated at room temperaturefor another 1 h. The resulting immune complexes were washed threetimes with RIPA buffer (10 mM Tris-HCl [pH 7.5], 150 mM NaCl,5 mM EDTA, 0.1% sodium dodecyl sulfate [SDS], 1% Triton X-100,1% sodium deoxycholate), analyzed by SDS-polyacrylamide gel electrophoresis(PAGE), and fluorographed at $-$ 70°C.

Western immunoblot analysis. Cell lysates were mixed with an equal volume of sample buffer without 2-mercaptoethanol, treated by boiling or left untreated,separated by SDS-PAGE, and transferred to a nitrocellulose membrane(Hybond-C Super; Amersham). The nonspecific antibody-binding siteswere blocked with 5% skim milk in PBS, and the membranes werereacted with anti-JEV MAb (6). The resulting blot was treatedwith horseradish peroxidase-conjugated goat anti-mouse immunoglobulin(Cappel) and developed either with enhanced chemiluminescencereagent (Amersham) or by alkaline phosphatase-conjugated secondaryantibody treatment with nitroblue tetrazolium (NBT) and 5-bromo-4-chloro-3-indolylphosphate(BCIP).

Viral proteins expressed by recombinant plasmids. To verify the viral protein expressed by pJME, the plasmid DNA was transfected into COS-7 cells by the calcium phosphate-DNAcoprecipitation method (16). At 44 h postinfection, cytoplasmicextracts were prepared as previously described (8). The sampleswere analyzed by SDS-PAGE (10% polyacrylamide) under denaturingconditions, transferred to a nitrocellulose membrane, and blottedwith MAbs specific for JEV E protein as described above. The specificbinding of recombinant E protein to MAbs was revealed by an alkalinephosphatase-conjugated secondary antibody with the enzyme substratesNBT and BCIP. To check for NS1 expression, a transient-expressionsystem involving recombinant vaccinia virus expressing T7 polymerase(vTF7-3) was used. BHK-21 cells were infected with vTF7-3 at MOI5, and at 1 h postinfection the infected cells were transfectedwith Lipofectamine (Bethesda Research Laboratories) mixed witheither pJNS1 or pJNS1', both comprising a T7 promoter in frontof the genes to be expressed (see Fig. 1A). After overnight incubation,the resulting cells were labeled with [³⁵S]Pro-mix (Amersham), and the cell lysates were isolated and immunoprecipitatedas described above. For endoglycosidase F (endo-F) digestion,the immunoprecipitated proteins were boiled in endo-F boilingbuffer (50 mM sodium phosphate [pH 7.5], 0.5% SDS, 1% 2-mercaptoethanol)and the resulting proteins were incubated overnight at 37°C witha equal volume of the endo-F incubation buffer (50 mM sodium phosphate[pH 7.5], 2% Nonidet P-40, 0.2% SDS, 1% 2-mercaptoethanol, 25mM EDTA) with or without endo-F (Boehringer Mannheim).

Indirect immunofluorescence staining of NS1-expressing cells. For intracellular staining, the cells were fixed in acetone-methanol (1:1) solution for 3 min and then reacted with MAb againstJEV NS1 (6). For cell surface staining, the unfixed cells werealso reacted with MAb against JEV NS1 at 4°C for 1 h. After beingwashed with PBS, the cells were further treated with goat anti-mousefluorescein-conjugated secondary antibody (Cappel), and the resultingcells were examined under a Leitz fluorescent microscope.

Immunization and challenge in mice. Plasmid DNA was prepared by the Midiprep procedure (Qiagen) as specified by the manufacturer. Groups of 3- to 4-week-old femaleICR mice were immunized with 80 µg of recombinant pJME, pJNS1,pJNS1', or pcDNA3 DNA as a control. DNA in PBS or PBS alone wasintramuscularly (i.m.) injected into the thighs of the mice; themice were subsequently given booster doses by the same methodtwice at 2-week intervals. At 2 weeks after the final boosterdose, each mouse was intraperitoneally (i.p.) challenged with2 × 10⁷ PFU of a neurovirulent JEV strain RP-9 (about 10 50% lethal dosesfor 10-week-old ICR mice) in 300 µl of PBS and simultaneouslyinjected intracerebrally (i.c.) with 30 µl of PBS alone into theright hemisphere of the brain (i.p. + i.c. route) (26). To ensurethe depth of each i.c. injection, we used 27-gauge one-stop needles(Top Injection Needle, Tokyo, Japan). Mouse mortality was monitoreddaily for 3 weeks.

Antibody-dependent complement-mediated cytolytic assay. A modified complement-mediated cytolysis assay was performed to determine the ability of pooled mouse sera to lyse JEV-infectedcells. Briefly, target BHK-21 cells grown in 96-well microtiterplates (Corning) were infected with JEV (RP-9) at an MOI of 5overnight. Pooled sera obtained from the immunized mice were preheatedat 56°C for 30 min to inactivate complement, serially diluted,and then incubated with various dilutions of guinea pig complement(Cappel) at 37°C for 60 min before being added to the target cells.After a 4-h incubation, cytolysis was measured by the releaseof lactate dehydrogenase (LDH), a cytoplasmic enzyme, with a commercialkit (cytotoxicity detection kit; Boehringer Mannheim) as specifiedby the manufacturer. Briefly, the culture supernatants were clarifiedby centrifugation, incubated with the reaction mixture (diaphorase/NAD⁺ and tetrazolium salt INT-sodium lactate) at room temperaturefor about 30 min, and then read by an enzyme-linked immunosorbentassay reader at 490 nm (microplate reader; Molecular Devices).RPMI 1640 without phenol red (GIBCO) was used throughout thisexperiment to decrease the background adsorbance. The maximumLDH release was determined from the wells (three wells for eachexperiment) containing the target cells lysed with 1% Triton X-100;spontaneous LDH release was determined from the wells containingthe target cells and medium only. The percent specific lysis wascalculated as follows: 100 × (experimental LDH release $-$ spontaneousLDH release)/(maximum LDH release $-$ spontaneous LDH release).

Flow cytometry. For cell surface staining, the cells were harvested from the culture plates with suspension buffer (PBS containing 0.5 mMEDTA [pH 8.0]) and the cell suspensions were blocked with fluorescence-activatedcell sorter (FACS) buffer (1% bovine serum albumin and 0.02% sodiumazide in PBS) at 4°C for 30 min. JEV NS1-specific MAb (1:1,000dilution) (6), a primary antibody, and fluorescein isothiocyanate-conjugatedgoat anti-mouse immunoglobulin (1:1,000 dilution) (Cappel), asecondary antibody, were added consecutively to the cell suspensions,which were then incubated at 4°C for 30 min. Cell staining wasanalyzed with a FACS Calibur (Becton Dickinson) and CELLQuestsoftware.

	RESULTS

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Construction of plasmids expressing JEV proteins. By using recombinant vaccinia viruses that specified the synthesis of JEV glycoproteins, the coexpression of prM and E haspreviously been shown to protect mice from a lethal challengewith JEV (21, 52). In addition to a possible role in elicitingneutralizing antibodies, prM has been implicated in the stabilizationof E protein by prevention of its low-pH-induced rearrangementduring transport through the acidic compartments of the trans-Golginetwork (18). Therefore, to investigate whether the structuralglycoproteins of JEV (prM and E) could be used in gene immunization,we constructed a pcDNA3-based plasmid expressing prM plus E underthe control of the cytomegalovirus promoter. To obtain propermodifications in the ER-Golgi apparatus complex, a sequence containinga 15-amino-acid signal peptide derived from the C terminus ofJEV C protein was added in front of prM plus E, and the resultingconstruct was named pJME (Fig. 1). To verify the viral proteinexpression from pJME, the plasmid DNA was transfected into COS-7cells and cell extracts from transfectants were immunoblottedwith a MAb against JEV E protein (6). As shown in Fig. 2A,a single band with a molecular mass of 56 kDa was detected inthe pJME-transfected (lane 2) but not in the mock-transfected(lane 1) cell lysate, which correlated with the expected molecularmass of JEV E protein. Moreover, as analyzed by endo-F cleavage,the E protein expressed by pJME appeared to be properly glycosylated,as evidenced by its comigration with the authentic viral E protein(data not shown). The absence of the full-length prME proteinin Fig. 2A was probably because the cleavage of prME was bothrapid and complete in the ER. These data indicate that pJME couldexpress E glycoprotein indistinguishable from the one expressedby JEV-infected cells. However, it remains unclear why, althoughabundant E proteins could be found in the lysate of pJME-transfectedcells, only small amounts of secreted E proteins were detectedin the culture supernatant (data not shown).

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FIG. 2. JEV glycoproteins expressed from recombinant plasmids in cell cultures. (A) JEV E protein expressed by pJME. Cell lysates from pJME-transfected (lane 2) or mock-transfected (lane 1) COS-7 were immunoblotted with MAb against JEV E protein as described in Materials and Methods. The position of the E protein is indicated by the arrow. Numbers on the left figure are the molecular mass standards in kilodaltons. (B) JEV NS1 proteins expressed by pJNS1 and pJNS1' were immunoprecipitated with anti-NS1 MAb and analyzed by SDS-PAGE. Cell lysates were isolated from BHK-21 cells transfected with pJNS1 (lanes 2, 6, and 10), pJNS1' (lanes 3, 7, and 11), or vector pcDNA3 (lanes 4, 8, and 12); as a control, lysates purified from JEV-infected BHK-21 cells (lanes 1, 5, and 9) were also included. The expression profiles of viral proteins analyzed by RIP are shown in lanes 1 to 4. For endo-F analysis, cell extracts either from JEV-infected cells or from transfected cells were digested with endo-F (lanes 5 to 8), or treated with buffer alone (lane 9 to 12) at 37°C overnight. Lane M contains the molecular weight standards (given in kilodaltons on the left). The positions of the glycosylated NS1 and NS1' proteins are indicated by the arrows on the right. The asterisks denote the endo-F-sensitive species of NS1 glycoproteins.

To determine whether the JEV nonstructural protein NS1 could be used for DNA immunization, we constructed plasmids expressingeither NS1 or NS1'. Similar to pJME, a sequence consisting ofa 30-amino-acid signal peptide derived from the C terminus ofJEV E was also situated immediately in front of both NS1 and NS1'constructs, as shown in Fig. 1, and the resulting plasmids werecalled pJNS1 and pJNS1', respectively. Plasmid pJNS1' is identicalto pJNS1, except that the coding sequence of the former was extendedfrom the NS1 region into the NS2A region (Fig. 1). The NS1 expressionpatterns of both constructs were examined by a transient-expressionsystem in BHK-21 cells with recombinant vaccinia virus expressingT7 polymerase to drive the gene tested. From the results shownin Fig. 2B, obtained by immunoprecipitation with the MAb againstJEV NS1 (6), protein bands, comigrating with either the authenticNS1 or NS1' (lane 1) from infected cell lysates, were detectedin both the pJNS1-transfected (lane 2) and pJNS1'-transfected(lane 3) cell lysates. No corresponding precipitates could beobserved in cells transfected with vector pcDNA3 alone (Fig. 2B,lane 4). pJNS1' appeared to be able to express only NS1' but notNS1 (lane 3), implying that NS1' expressed by this construct wasnot the precursor of NS1. Alternatively, since the exact C terminusof JEV NS1' protein is unknown, the cleavage requirements forconverting NS1' to NS1 might not be completely included in thisarbitrary pJNS1' construct.

Both NS1 and NS1' proteins contain two predicted N-linked glycosylation sites at amino acid positions 130 and 207. We nextdetermined whether recombinant NS1 and NS1' had undergone properglycosylation during biosynthesis. After complete digestion byendo-F, the sizes of both NS1 and NS1', expressed either by JEVinfection or by recombinant-plasmid transfection, decreased byapproximately 4 to 6 kDa (Fig. 2B, compare lane 1 with lane 5,lane 2 with lane 6, and lane 3 with lane 7). As a negative control,no size alteration could be seen when the samples were treatedwith just buffer only (lanes 9 to 12). These data confirm theprevious finding (12) that NS1 can be targeted to the ER compartment,where it is properly glycosylated in the absence of other viralproteins. Together, these results illustrate that the recombinantNS1 constructs were able to express glycosylated NS1 proteinswhich were indistinguishable from the ones derived from naturalJEV infection.

DNA immunization and JEV challenge in the outbred-mouse model. To assess the efficacy of DNA immunization against JEV infection, groups of 3- to 4-week-old female outbred ICR mice wereimmunized with either recombinant constructs, control vector DNA,or PBS buffer alone. Two weeks after the second immunizing boost,the mice were challenged with a neurovirulent JEV strain, RP-9(26). The mice were checked daily for survival, and the resultsare shown in Fig. 3. The survival rates for the different experimentalgroups at 21 days postchallenge and the results of the statisticalanalysis are summarized in Table 1. The greatest survival wasobserved in the group of mice immunized with pJNS1, in which 9of the 10 tested mice survived the lethal JEV challenge (P < 0.001).The second best survival rate was observed in the pJME-immunizedgroup, whose survival rate was 70% (P < 0.01) (Fig. 3; Table 1).In contrast, pJNS1', which expressed a longer form of NS1, failedto confer a comparable level of protection on the immunized miceto that conferred by its counterpart pJNS1; instead, pJNS1', likeits parental vector pcDNA3, demonstrated only a 40% survival rate(P < 0.25) (Fig. 3; Table 1). The low level of protective capabilityobserved with pcDNA3, compared to the 17% survival rate of thegroup of mice which received only PBS buffer, was most probablydue to the nonspecific immunostimulatory effect resulting fromthe bacterial DNA with CpG motifs (23). These results clearlyillustrate that immunization with the genes encoding either JEVstructural or nonstructural proteins could protect mice from alethal challenge.

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FIG. 3. Survival of DNA-immunized mice after lethal JEV challenge. Groups of 3- to 4-week-old female ICR mice were immunized with the indicated plasmids or buffer alone and later lethally challenged with JEV as described in Materials and Methods. The JEV-infected mice were monitored daily for survival up to 21 days postchallenge.

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TABLE 1. Survival rate of ICR mice immunized with plasmid DNA expressing JEV glycoproteins after a lethal challenge^a

Characterization of JEV-specific antibody response in immunized mice. To study the JEV-specific antibody responses elicited by DNA immunization described above, pooled sera from groups of immunizedmice were collected and tested by immunoprecipitation with ³⁵S-labeled JEV-infected cell lysates as the antigen. As shown inFig. 4, in sera from the mice injected with pJNS1, antibodiesreadily precipitated both NS1 and NS1' after only one boost (lanes1 to 3) whereas antisera from the pJNS1'-immunized mice appearedto only weakly precipitate NS1 and NS1' even after a second boost(lanes 4 to 6). No NS1-specific antibody responses could be detectedin the negative controls immunized with either pcDNA3 or PBS bufferonly (lanes 7 and 8). The extent of the antibody responses stimulatedby pJNS1 and pJNS1' appeared to correlate well with their protectivecapabilities, as shown in Table 1 and Fig. 3; that is, pJNS1,rather than pJNS1', not only elicited a good humoral immunitybut also conferred on immunized mice sufficient protection froma subsequent lethal challenge. However, as expected, pJNS1-mediatedprotection did not appear to be the result of direct neutralizationof JEV, since only a basal level of activity (less than a 20-foldserum dilution) could be detected in the sera examined by the70% plaque reduction neutralization test (data not shown). InpJME-injected mice, we failed to detect any JEV-specific antibodyresponse by immunoprecipitation (data not shown). However, a lowtiter (40-fold serum dilution) in the plaque reduction neutralizationtest could be detected (data not shown). Whether this low levelof neutralization was responsible for the protection observedin the pJME-immunized group or whether other immune system mechanisms,such as cellular immunity, contributed to this protection remainsunclear. The discrepancy between the pJME immunization resultsand the previously published ones (21, 22, 31) was probablydue to different secretion capabilities of the engineered E proteinsproduced by different recombinant constructs.

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FIG. 4. Seroconversion of mice immunized with pJNS1 or pJNS1'. The antibody responses specific to JEV NS1 in immunized mice were examined by RIP analysis with ³⁵S-labeled, JEV-infected cell lysates. The pooled sera were collected 2 weeks after the primary (lanes 1 and 4), secondary (lanes 2 and 5), and third (lanes 3 and 6 to 8) DNA injections. The serum samples were from mice immunized with pJNS1 (lanes 1 to 3), pJNS1' (lanes 4 to 6), vector control pcDNA3 (lane 7), or PBS buffer alone (lane 8). A MAb specific for JEV NS1 ( $alpha$ NS1) was used as a positive control (lane 9). The positions of NS1 and NS1' are indicated by the arrows on the right. Numbers on the left are the molecular mass standards in kilodaltons.

Anti-NS1 antibodies could induce a complement-mediated cytotoxicity in JEV-infected cells. To determine whether NS1-specific antisera can cause cytolysis of JEV-infected cells in the presence of complement, a modifiedcomplement-mediated cytotoxicity assay was performed. By measuringthe release of a cytoplasmic enzyme, LDH, pooled sera from DNA-or JEV-immunized mice were analyzed for their abilities to lyseJEV-infected BHK-21 cells in the presence of complement. As theresults in Fig. 5 indicate, antiserum from pJNS1-immunized micewas able to lyse target JEV-infected cells (Fig. 5C); in contrast,no apparent specific cytolytic could be detected with sera frompJME-immunized (Fig. 5B) and pJNS1'-immunized (data not shown)mice. As controls, sera from JEV-immunized mice displayed a highlevel of cytolytic activity when complement was included (Fig.5D) whereas sera from pcDNA3-immunized mice showed no specificactivity (Fig. 5A). These results are consistent with previousobservations in which flavivirus NS1-induced protective immunitymight have resulted from antibody-dependent complement-mediatedcytolysis of infected cells (11, 43).

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FIG. 5. The pJNS1-immunized sera exhibited antibody-dependent complement-mediated cytolysis of JEV-infected cells. The sera obtained 2 weeks after the second injections were pooled from ICR mice immunized with pcDNA3 (A), pJME (B), or pJNS1 (C). As a control, sera were also collected from mice that had been infected with JEV (D). In the presence of complement (C') at different dilutions (none, 1:10, 1:20, or 1:40), the pooled sera were analyzed for their ability to lyse JEV-infected BHK-21 cells at various serum dilutions (no antibody, 1:20, 1:40, or 1:80). The percent specific lysis was determined as described in Materials and Methods.

Biochemical analysis of the differences between JEV NS1 and NS1' in cultured cells. In contrast to other flaviviruses, both NS1 and NS1' are often detected in lysates of JEV-infected cells (30). However,the biological significance of and the biochemical differencebetween these two NS1 proteins remain uncharacterized. BecauseJEV NS1' contains all the genetic information of NS1, it is intriguingto suggest that NS1 and NS1' from JEV might possess differentimmune stimulation capabilities. One possible mechanism involvedis that NS1 differs from NS1' in its ability to be secreted fromand expressed on JEV-infected cells, a characteristic believedto be important for eliciting an adequate immune response. Totest this hypothesis, we further biochemically analyzed the twoproteins expressed in cultured cells by a transient- or permanent-expressionsystem. JEV NS1 proteins are secreted from infected cells as dimerswhich are highly sensitive to heat treatment, as shown by analyzedby Western blotting (12). To assess the amount of secreted NS1proteins in dimeric form, we prepared the protein samples in thenext two experiments without heat treatment before subjectingthem to SDS-PAGE. In the JEV-infected cell lysate (Fig. 6A, lane5), which served as a positive control, three NS1-related bands,corresponding to homodimers of NS1 and NS1' and a heterodimerbetween NS1 and NS1', were detected; however, in the culture supernatant,only two major NS1-related bands could be detected (lane 1), indicatingthat one of the NS1-related dimers, presumably the NS1' homodimer,might not be secreted from the cells as efficiently as the othertwo. When transiently expressed by recombinant vaccinia virusproducing T7 polymerase, NS1 derived from pJNS1 construct appearednot only to form dimers intracellularly (lane 6) but also to besecreted as dimers extracellularly (lane 2). The secreted formsof NS1 proteins migrated more slowly than did their counterpartsin cell lysates, probably due to the different glycosylation patterns(compare lane 2 with lane 6 and lane 1 with lane 5), as previouslydescribed elsewhere (30). In marked contrast, NS1' expressedby the pJNS1' construct could form dimers only intracellularly(lane 7) but failed to be secreted in the culture supernatant(lane 3).

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FIG. 6. Intracellular and extracellular protein patterns of JEV NS1 and NS1' expressed in cell culture. (A) Viral proteins expressed from plasmids by a transient system involving recombinant vaccinia virus vTF7-3. By immunoblotting with MAb against JEV NS1, the culture media (lanes 1 to 4) and their corresponding cell lysates (lanes 5 to 8) were prepared to detect the presence of JEV NS1. Lanes: 1 and 5, samples derived from JEV-infected cells (positive control); 2 and 6, samples from pJNS1-transfected, vTF7-3-infected cells; 3 and 7, samples from pJNS1'-transfected, vTF7-3-infected cells; 4 and 8, samples from pcDNA3-transfected, vTF7-3-infected cells (negative control). Putative homo- and heterodimers of JEV NS1s are marked by arrows. (B) Viral proteins expressed by cell clones containing different plasmids as indicated. JEV NS1s in the culture media (lanes 1 to 4) and in cell lysates (lanes 5 to 8) were analyzed by immunoblotting. Samples to be examined were prepared from cell clones containing pJNS1 (lanes 2 and 6), pJNS1' (lanes 3 and 7), and no plasmid (lane 4 and 8). Lanes 1 and 5 contain control samples derived from JEV-infected cells.

To exclude any possible effects of vaccinia virus infection, we established permanent cell lines expressing NS1 by transfectingBHK-21 cells with either pJNS1 or pJNS1'. After selection by geneticin(G418 sulfate [GIBCO]) and screening by an indirect immunofluorescenceassay (IFA) with MAb against JEV NS1, several cell clones constitutivelyexpressing NS1 or NS1' were established. A similar experimentto that in Fig. 6A was performed, and representative data obtainedfrom two such cell clones are shown in Fig. 6B. Similar to theresult in Fig. 6A, NS1 dimers were readily detected in the celllysates from both NS1- and NS1'-expressing cell clones (Fig. 6B,lanes 6 and 7). However, only the recombinant NS1 made by theNS1-expressing clone could be released as homodimers extracellularly(lane 2) whereas the secreted form of NS1' was never detectedin the culture medium from NS1'-expressing cells (lane 3). Together,these results clearly indicate that NS1 differs from NS1' in itsability to be secreted from genetically engineered cells.

By using IFA with MAb against JEV NS1, the NS1 distribution in NS1- and NS1'-expressing cell clones was also studied. Althoughcytoplasmic staining of NS1 was observed in both cell clones,the distribution patterns differed; in NS1-expressing cells, someof the recombinant NS1 appeared to aggregate in granules scatteredaround the cytoplasm (Fig. 7C), while a relatively homogeneouscytoplasmic staining of the engineered NS1' was observed in NS1'-expressingcells (Fig. 7E). The cytoplasmic pattern of NS1 in JEV-infectedcells (Fig. 7A) was also somewhat homogeneous compared to thatin NS1-expressing cells (Fig. 7C). The biological significanceof this difference remains to be further elucidated. One possiblefunction of NS1 granules seen in the cytoplasm is to act as transportvehicles participating in the secretory process of JEV NS1. Finally,we characterized the surface expression of NS1s on unfixed cellsby IFA, and the results demonstrated positive surface stainingon the exterior of NS1-expressing cells (Fig. 7D) as well as onJEV-infected cells (Fig. 7B). By contrast, no detectable surfacestaining could be seen on NS1'-expressing cells (Fig. 7F). Thesephenomena were further substantiated by FACS analysis, as shownin Fig. 8. The level of NS1 surface expression from cells containingpJNS1 (Fig. 8A) was much higher than that from cells expressingpJNS1' (Fig. 8B) (97.74 and 13.20%, respectively). Interestingly,only a moderate level (49.56%) of NS1 surface staining could bedetected when NS1 and NS1' coexisted (data not shown) in cellsconstitutively expressing JEV NS1 and full-length NS2A (Fig. 8C).Taken together, these data strongly suggest that NS1, rather thanits counterpart NS1', could be efficiently expressed on and secretedfrom pJNS1-transfected cells, and this biochemical discrepancymay contribute to the difference in the efficacy of DNA immunizationwith pJNS1 and pJNS1'.

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FIG. 7. NS1 protein localization in NS1- or NS1'-expressing cell clones. By using indirect immunofluorescence staining of cells with MAb against JEV NS1, the NS1 expression patterns from cell clones containing pJNS1 (C and D) or pJNS1' (E and F) were investigated. The NS1 pattern from JEV-infected BHK-21 cells (A and B) was included as a control. The intracellular distribution of NS1 was analyzed from cells fixed with acetone-methanol (1:1) (A, C, and E); on the other hand, cell surface expression of NS1 was analyzed from unfixed cells (B, D, and F) (see Materials and Methods).

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FIG. 8. Flow cytometry of NS1 surface expression from three permanent cell clones. NS1 antigen expressed on the surface of cell clones containing pJNS1 (A), pJNS1' (B), or pJNS1-2A (C) was analyzed with a FACS Caliber (Becton Dickinson) and CELLQuest software. Cells were stained for surface antigen with a MAb against JEV NS1 followed by fluorescein isothiocyanate-conjugated goat anti-mouse immunoglobulin (shaded areas). The open area was derived from the staining of parental BHK-21 cells. The numbers above the shaded areas in each panel indicate the percentage of positive staining from tested cells compared to that from parental BHK-21 cells.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

By passive immunization with MAbs against NS1 and by active immunization with NS1 proteins, flavivirus NS1 has been demonstratedto contain epitopes that are able to stimulate protective immunity(reviewed in references 14, 34, and 48). In the presentstudy, we further demonstrate that DNA immunization with NS1 (aswell as with prME) can also confer protection against a lethalJEV challenge in an outbred mouse model. The success of gene vaccination,as shown by our results, clearly indicates the applicability ofthis approach in the development of a subunit vaccine againstflavivirus infection. One obvious advantage of immunizing withDNA over immunizing with purified viral antigens is that JEV glycoproteinsexpressed on the cell surface from DNA constructs can be correctlypresented to the immune system in a native state. Additionally,DNA vaccination can circumvent the detrimental alterations ofantigenic integrity during the purification procedure for thepreparation of conventional viral antigens. Thus, immunizationwith genes encoding viral glycoproteins, such as the JEV proteins,can in theory elicit a whole range of immune responses, closelyresembling the process of natural virus infection (reviewed inreference 35). It would be of interest to know whether geneimmunization with the NS1 gene can also block JEV replicationin other viremic amplifying hosts such as birds and pigs.

The present data appear to support the notion that flavivirus NS1 by itself is sufficient to elicit protective immunity, makingJEV NS1 a suitable candidate in addition to prME for a subunitvaccine. However, in contrast to the results presented here, severalearlier studies in which recombinant viruses were used as an expressionvector, including vaccinia virus (21), Sindbis virus (39),and baculovirus (33), have shown that JEV NS1 could induce onlylow levels of protection in the tested hosts. This discrepancymost probably results from different expression systems beingused (DNA immunization versus recombinant viruses) and differentcoding sequences being included in NS1 constructs. It is possiblethat JEV NS1 became a relatively weak immunogen when coimmunizedwith its immunodominant virus vectors, so that the infected hostfailed to properly recognize and respond to NS1. Alternatively,the possession of extra sequences from NS2A in some cases (21,39) probably also contributed to the inability of recombinantviruses expressing NS1 to elicit protective immunity. Similarconclusions can be drawn from immunization with pJNS1' DNA containingabout one-quarter of the NS2A sequence constructed in this study,which indeed conferred on the mice only partial protection againsta lethal JEV infection (Fig. 3). By contrast, pJNS1 DNA, withoutany NS2A sequence, was able to provide robust protection againstlethal JEV challenge. These data are also consistent with theresults of a previous study (11) in which mice immunized withrecombinant vaccinia virus expressing dengue virus NS1 alone,but not NS1 plus 15% of NS2A, were fully protected from a subsequentdengue virus challenge.

In JEV-infected cells, both NS1 and NS1' can be normally generated, yet little is known about their functions in JEV replicationand whether NS1' is the precursor to NS1. Biochemical analysesconducted in this study however, indicate that when these proteinsare individually expressed, NS1 differs primarily from its longerversion, NS1', in its ability to be secreted from and expressedon cells (Fig. 6 through 8). In fact, NS1' is identical to NS1,except that the former contains an extra portion of approximately60 amino acids from the N terminus of NS2A. JEV NS2A, a smallhydrophobic protein, is probably inserted into and spans the lipidbilayer of the ER lumen at least once during biosynthesis. Conceivably,after entry into the lumen of the ER, NS1' is likely to be retainedrather than proceed along the secretory pathway. On the otherhand, NS1, which does not seem to contain any recognizable membraneanchorage domains, appears to be proficient in both cell associationand secretion (Fig. 6 through 8). This biochemical property ofNS1 is particularly relevant because our results clearly demonstratedthat NS1 was far more immunogenic than NS1' with respect to humoralresponses (Fig. 4 and 5) and protective immunity (Fig. 3) inducedin the immunized hosts. Interestingly, when NS1 and NS1' coexistedin cells containing pJNS1-2A, the level of cell surface expressionof NS1 was significantly lower than that in cells constitutivelyexpressing NS1 alone (Fig. 8). These data seem to imply that thepresence of NS1' might have retarded the normal secretory processfor NS1, probably through forming a heterodimer between NS1 andNS1'. It is reasonable to hypothesize that partial NS2A may havea negative impact on NS1-based gene immunization when it is cosynthesizedde novo with NS1 in the cell. Exclusion of NS2A would thereforebe strategically beneficial for developing NS1 subunit vaccinesagainst JEV infection. However, the motif(s) that dictates thefate of NS1 proteins in cell association or secretion remainsto be further elucidated.

With regard to the expression of viral glycoproteins on the cell surface, JEV replication should be able to render infectedcells susceptible to antibody-dependent complement-mediated cytolysisand/or antibody-dependent cell-mediated cytotoxicity. Indeed,the fact that immunized sera raised against JEV NS1 caused cytolysisof the JEV-infected cells in a complement-dependent manner (Fig.5) strongly suggests the involvement of an Fc-mediated cell killingmechanism in the protection of mice from a lethal JEV challenge.Moreover, these data also imply that pJNS1 immunization couldstimulate antibody responses with not only the correct epitopespecificity but also the appropriate antibody isotype essentialfor governing the Fc receptor-dependent interactions. Such cytophilicbut not neutralizing NS1-specific antibodies could conceivablyempower leukocytes involved in the antibody-dependent cell-mediatedcytotoxicity reaction important for the elimination of JEV-infectedcells. However, the level of specific lysis in pJNS1-immunizedsera appeared to be much lower than that in JEV-immunized sera(Fig. 5), indicating that other mechanisms, such as cell-mediatedimmunity, might also contribute to this protection. Plausibly,NS1 expressed by plasmid DNA from the cells might also be ableto elicit specific cytotoxic T-cell responses, as previously suggestedby Lobigs et al. (27), whereby cytotoxic T-cell peptide determinantsof flavivirus were derived predominantly from viral nonstructuralproteins. This may be of interest in JEV vaccination, since flavivirusinfections are renowned for inducing MHC class I up-regulation,which leads to down-regulation of virus-specific cytotoxic T-cellmemory (reviewed in reference 27). The success of DNA immunizationagainst JEV infection with only portions of viral polyproteinsmay open avenues for exploring new epitopes that can confer onthe immunized host a long-lasting cytotoxic T-cell memory withoutcompromising protection capability.

	ACKNOWLEDGMENTS

JEV NT109 and NT113 were kindly provided by the National Institute of Preventive Medicine, Taiwan, Republic of China (ROC).

Y.-L.L. was supported by grant DOH87-TD-1002 from the Department of Health, ROC; grant NSC-87-2314-B-016-090 from the NationalScience Council (NSC), ROC; and grant (DD01-86IX-CR-501P) fromthe National Health Research Institute (NHRI) ROC. L.-K.C. wassupported by grant NSC 87-2314-B-016-037 M07 from NSC and grantDD01-86IX-CR-501P from NHRI. C.-L.L. was supported by grant NSC87-2314-B-016-088 from NSC and two grants (DOH87-HR-608 and DD01-86IX-CR-501P)from NHRI.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Preventive Medicine, National Defense Medical Center, P.O. Box 90048-700,18 Sih-Yuan St., Taipei 100, Taiwan, Republic of China. Phone:(886)-2-673-2230. Fax: (886)-2-930-8867. E-mail: yll{at}ms11.hinet.net.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
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