PrM- and Cell-Binding Domains of the Dengue Virus E Protein

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Wang, S.
	Articles by Anderson, R.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Wang, S.
	Articles by Anderson, R.

Previous Article | Next Article

Journal of Virology, March 1999, p. 2547-2551, Vol. 73, No. 3
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

PrM- and Cell-Binding Domains of the Dengue Virus E Protein

Songli Wang, Runtao He, and Robert Anderson^*

Department of Microbiology and Immunology, Dalhousie University, Halifax, Nova Scotia B3H 4H7, Canada

Received 25 August 1998/Accepted 30 November 1998

	ABSTRACT

Top Abstract Text References

The E-prM proteins of flaviviruses are unusual complexes which play important roles in virus assembly and fusion modulationand in potential immunity-inducing vaccines. Despite their importance,little is known about the biogenesis and structural organizationof E-prM complexes. Pulse-chase radiolabeling of dengue virus-infectedVero cells demonstrated a rapid interassociation of E and prMproteins, and sucrose gradient sedimentation analysis suggestedthat E-prM complexes progressed from simple heteromers to moredensely sedimenting structures indicating increased multimerization.E-prM heteromers of even higher complexity were observed in virusparticles, suggesting an intracellular assembly process whichresults in the networking of E-prM subunits into a lattice-likestructure found in virus particles. Trypsin cleavage of E-prM-containingvirus particles resulted in the release of a soluble 45-kDa fragmentof the E protein which retained cell-binding activity. The resultssuggest that E-prM interactions in dengue virus particles arelargely mediated by domains in the carboxy-terminal anchoringdomain of E, while cell-binding activity is retained in a trypsin-releasableectodomain of the Eprotein.

	TEXT

Top Abstract Text References

The flavivirus E protein is a multifunctional protein which is involved in cell receptor binding (3, 6, 10) and virusentry via fusion with a host cell membrane (26). An unusualfeature of the flavivirus E protein is that some of its functionalactivities, notably membrane fusion, are regulated by interactionwith a second viral protein, prM. It is believed that the associationof prM with E stabilizes certain pH-sensitive epitopes on theE protein, thereby preventing the conformational changes whichnormally occur at acidic pH and which activate the fusogenic activityof the E protein (1, 9, 13). In addition to its normalrole in flavivirus assembly, the prM protein has also been includedin novel recombinant formulations in which it is generally coexpressedwith the E protein; the resultant E-prM complexes have been shownto be immunogenic and protective in vaccines against challengewith several flaviviruses, including Japanese encephalitis virus(20), yellow fever virus (22), dengue virus (8), and tick-borneencephalitis virus (11). Despite the importance of the E-prMcomplex in flavivirus biology and vaccinology, its structure andbiosynthesis remain incompletely understood, particularly in relationshipto dengue virus infection. The purposes of the present study wereto investigate the biogenesis of the E-prM complex in dengue virus-infectedcells and to partially localize the biologically important functionalactivities of prM binding and cell binding in the mature Eprotein.

Predominance of prM and E proteins in extracellular particles produced by dengue virus-infected Vero cells. In tick-borne encephalitis virus, the majority of extracellular virus is largely free of prM protein, due to a late intracellularprocessing event which generates a carboxy-terminal fragment designatedM; this fragment and the E and C proteins are believed to constitutethe protein components of the mature virus particle (13). Incontrast, dengue virus particles purified from cell culture containa mixture of prM and M proteins (4, 10, 23, 24) in whichprM often predominates (4, 10, 23). The preponderance ofprM (over M) in extracellular virus particles cannot be explainedsolely by enhanced radiolabeling (11 methionines in prM versus5 in M), since dengue virus virions containing prM (and very littleM) have also been observed by protein staining (23). Sucrosegradient fractionation of culture fluids from radiolabeled, denguevirus-infected cells clearly shows cosedimentation of infectivityand E-prM-containing particles (Fig. 1). The results indicatea predominance of prM-containing virus particles produced by virus-infectedVero cells, likely as a consequence of relatively inefficientcleavage of prM to M during the late stages of virus maturation.Nevertheless, dengue virus infectivity does not appear to dependon quantitative cleavage of prM to M, as dengue virus particlescontaining prM but no M (obtained from virus-infected cells culturedin the presence of ammonium chloride, which blocks prM-to-M cleavage)still retain one-eighth to one-sixth the specific infectivityof normal virus particles (24). We have shown previously thatvirus particles containing E and prM bind to permissive cellsand that binding can be blocked with E-specific antibody (10,29). Virus particles containing mainly E and prM also show antibody-enhancedbinding to Fc receptor-bearing K562 cells as well as to platelets(29). Thus, in addition to being requisite precursors to maturevirus particles, virus particles containing prM possess many propertiesassociated with mature virus particles. The preponderance of prM-containingvirus particles produced by dengue virus-infected Vero cells wasexploited in the present study in order to trace the interactionsbetween E and prM which occur during virus particle biogenesis.

View larger version (33K):
[in this window]
[in a new window]

FIG. 1. Predominance of E and prM proteins in virus particles produced by dengue 2 (strain 16681) virus-infected Vero cells (multiplicity of infection = 1). Cells were pulse-labeled for 12 h with [³⁵S]methionine-cysteine (400 µCi/ml; ICN, Irvine, Calif.) at 40 h postinfection. Clarified culture fluid was overlaid on a 5 to 55% (wt/wt in phosphate-buffered saline) sucrose gradient and centrifuged for 16 h at 45,000 rpm in a Beckman SW60 rotor. The gradient was fractionated from the bottom, and aliquots were taken for immunoprecipitation with human dengue virus 2 immune serum (1:200 dilution) and for isolation by using protein A-bearing formalin-fixed cells of Staphylococcus aureus. Immunoprecipitates were washed with phosphate-buffered saline (no detergents) in order to recover virus particles as well as immunoreactive soluble proteins. The immunoprecipitates were resolved and revealed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and fluorography (A). The identities of E and prM proteins were confirmed by additional immunoprecipitations with E-specific MAbs 3H5 and 1B7 and prM-specific MAb 2H2 (14) (data not shown). Aliquots from the same sucrose gradient fractions were titrated for virus infectivity by plaque assay; the percentage of total PFU (= 3 × 10⁶ PFU) in each fraction is shown (B).

Time course of intracellular association of dengue virus E and prM proteins. To investigate intracellular protein interactions with newly synthesized E protein, we performed a pulse-chase [³⁵S]methionine-cysteine labeling study with dengue virus-infectedVero cells followed by immunoprecipitation of cytoplasmic extractswith E-specific monoclonal antibody (MAb) 1B7 (14). For thisstudy we found digitonin to give the best results in terms ofpreservation of E-prM complexes following cell solubilization.Digitonin is a mild cell lysis agent (19) and is known to preserveprotein-protein interactions which may be unstable in other detergents,such as Triton X-100 (16). Dengue virus prM protein was foundto be associated with newly synthesized E protein (i.e., withinthe 15-min pulse [Fig. 2A, lane 1]). The prM-E complex persistedin the infected cell for approximately 4 to 6 h, at which timethe level of intracellular prM-E complex was observed to decline.The timing of this decline was consistent with the export of E-prMinto extracellular progeny virus particles (Fig. 2C).

View larger version (47K):
[in this window]
[in a new window]

FIG. 2. Kinetics of intracellular association of dengue virus E and prM proteins. Dengue virus-infected Vero cells were pulse-labeled for 15 min with [³⁵S]methionine-cysteine at 40 h postinfection. Cells were washed and incubated for various times in 0.5 ml of chase medium containing excess methionine and cysteine. Cells were harvested after being washed in Tris-buffered saline and then solubilized in 100 µl of Tris-buffered saline containing digitonin (1 mg/ml). Extracts were microcentrifuged for 15 min at 4°C, and the supernatants were used for immunoprecipitation with E-specific MAb 1B7 (14) and formalin-fixed protein A-bearing cells of S. aureus. Immunoprecipitates were analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and fluorographed (A). (B) Mock immunoprecipitations of the same digitonin extracts with irrelevant antibody (MAb against mouse hepatitis virus N protein). (C) Immunoprecipitations (with MAb 1B7) from culture fluid supernatants from the pulse-chase-labeled cells for detection of the appearance of radiolabeled viral E protein and E protein complexes in the extracellular fluid.

Multimerization of prM-E complexes. Evidence from studies with immature virions of tick-borne encephalitis virus suggest that E may associate with prM as multimericcomplexes (1, 13, 25). To investigate the formation ofhigher-order E-prM complexes in dengue virus-infected cells, weanalyzed pulse-chase-radiolabeled cell extracts on sucrose gradients(Fig. 3). Complexes consisting of prM and E were clearly visibleas densely sedimenting structures by 2 h of chase, even in nonimmunoprecipitatedtotal cell extracts (Fig. 3A). Following immunoprecipitation withE-specific MAb 1B7 (14) and semiquantitation of E-prM complexesin all sucrose gradient fractions, the distribution of E-prM complexesthroughout each gradient was determined; results are shown inFig. 3B. In the pulse-labeled sample, the prM-E complex was foundto sediment near the top of the gradient (fractions 6 and 7),consistent with the complex being a simple heterodimer. In contrast,by 6 h of chase, the prM-E complex was also found in higher-densityfractions (fractions 4 and 5), indicating the formation of morecomplex, multimeric structures. Similar, densely sedimenting E-prMcomplexes were also found in dengue virus particles (Fig. 3B,bottom panel), suggesting that the intracellular multimeric E-prMstructures may represent preassembly complexes required for incorporationinto virus particles. The results imply the existence of an intracellularscaffolding process which occurs within a few hours of E-prM proteinsynthesis and which leads to the formation of multimeric E-prMcomplexes. To our knowledge, this is the first evidence for time-dependentexpansion of intracellular flavivirus E-prM complexes which likelyrepresent intermediate structures involved in the assembly ofheterogeneous, multimeric E-prM structures of the kind reportedfor immature virions of tick-borne encephalitis virus (13).

View larger version (23K):
[in this window]
[in a new window]

FIG. 3. Multimerization of dengue virus E and prM proteins. Digitonin extracts from infected cells pulse-chase labeled with [³⁵S]methionine-cysteine were overlaid on 10 to 50% (wt/wt) in phosphate-buffered saline) sucrose gradients and centrifuged for 16 h at 45,000 rpm in a Beckman SW60 rotor. Gradient tubes were pierced from the bottom and drained by gravity into seven microcentrifuge tubes. Aliquots of sucrose gradient fractions (without immunoprecipitation [A] or immunoprecipitated with MAb 1B7 [B]) were analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and fluorography. With increases in chase time, the E-prM complexes were observed to sediment progressively lower in the gradient, below the bulk of cell proteins which are mainly found near the top (fraction 6) of the gradient (A). The fluorogram was deliberately overexposed to show the densely sedimenting E-prM complexes appearing in fractions 4 and 5 by 2 and 6 h of chase. (B) Relative distribution of radiolabel in each sucrose gradient fraction, as determined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and fluorography of E-prM complexes immunoprecipitated by MAb 1B7. In the 15-min-pulse sample, predominantly light complexes (presumably heterodimers) of prM-E were found near the top of the gradient (in fractions 6 and 7). With increases of chase time, progressively heavier E-prM complexes (likely representing multimers) were observed, as indicated by a skewing of the distribution of E-prM complexes towards lower fractions in the gradient. Also shown is the distribution of digitonin-released E-prM complexes from purified virus particles, harvested from culture fluids after 12 h of chase. For reference, intact virus particles sedimented in fraction 1, while yeast alcohol dehydrogenase (molecular weight, 150,000) and catalase (molecular weight, 250,000) banded in fraction 6 and fractions 4 and 5, respectively, in these 10 to 50% sucrose gradients.

Release of a non-prM-associated E protein ectodomain by trypsin cleavage of virus particles. The observation of densely sedimenting, apparently multimeric E-prM complexes in virus particles (Fig. 3) suggests the existenceof multiple E-prM interactions, similar to those postulated fromstudies with immature particles of tick-borne encephalitis virus(1, 13, 25). In order to gain further insight into theintermolecular associations between E and prM within dengue virusparticles, radiolabeled virus particles (purified as for Fig.1) were treated with trypsin to release surface-exposed, trypsin-cleavableproteins. The virus trypsinate was immunoprecipitated with E-specificMAbs 3H5 and 1B7 (14). In addition to immunoprecipitating full-lengthE protein (as well as prM complexed to E), both antibodies wereable to immunoprecipitate an E protein fragment of about 45 kDa,designated $Delta$ E (Fig. 4A). Immunoprecipitation with MAb 1B7 wasmore effective than with MAb 3H5, perhaps due to the proximityof the MAb 3H5 binding site to the suspected trypsin cleavagesite (see below).

View larger version (46K):
[in this window]
[in a new window]

FIG. 4. (A) Cleavage of dengue virus E protein by trypsin. Dengue virus-infected Vero cells were labeled with [³⁵S]methionine-cysteine for 12 h, from 36 to 48 h postinfection. Radiolabeled virus was purified by sucrose gradient centrifugation (as for Fig. 1) and treated with trypsin (at final concentrations of 100, 20, and 4 µg/ml) on ice for 1 h. Reactions were terminated by adding a stop buffer containing bovine serum albumin (30 mg/ml) and 5 mM N- $alpha$ -tosyl-L-lysyl-chloromethyl ketone (TLCK). Samples were immunoprecipitated (IP) with MAbs 3H5 and 1B7 in the absence of detergents. (B) Release of $Delta$ E from dengue virus particles by trypsin. Radiolabeled dengue virus was treated with trypsin (20 µg/ml) for 1 h at 4°C, overlaid onto a 10 to 50% (wt/wt) sucrose gradient in phosphate-buffered saline, and centrifuged for 16 h at 45,000 rpm in a Beckman SW60 rotor. Samples were collected in seven fractions (from bottom to top) and immunoprecipitated with E-specific MAb 1B7. Aliquots of each sample were analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and fluorography.

In order to determine whether the trypsin-cleaved 45-kDa $Delta$ E fragment was virus associated, trypsin-treated dengue virus wascentrifuged through a 15 to 50% (wt/wt) sucrose gradient. Fractionsof the sucrose gradients were collected and immunoprecipitatedwith anti-dengue virus E-specific MAb 1B7 (Fig. 4B). In contrastto uncleaved virus, which sedimented near the bottom of the gradient(fractions 1 to 3), the trypsin-generated 45-kDa $Delta$ E fragment wasmainly found as a soluble protein near the top of the gradient(fraction 6). There was no detectable prM in this fraction, norwas there any $Delta$ E found in virus particles, suggesting that themajor prM binding sites are located in the membrane-anchoringcarboxy terminus of the E protein. The results suggest furtherthat the major intermolecular associations which stabilize theE-prM network within the virus particle do not appear to involvethe E ectodomain but rather are located in the carboxy-terminalportion of E. These results may be analogous to observations madewith tick-borne encephalitis virus in which full-length E proteinwas shown to form more stable complexes with prM than was anchor-freeE protein (2). It is also conceivable that $Delta$ E is derived solelyfrom a subset of E protein molecules which are not associatedwith prM. This possibility requires furtherinvestigation.

The trypsin-released ectodomain of E retains cell-binding activity. We used the trypsin-cleaved soluble E fragment in a cell binding assay to determine whether this fragment possessed receptor-bindingactivity. In parallel, cell binding of intact dengue virus (asa positive control) and the NS1 dimer (as a negative control)was monitored. Cell binding was performed with three cell linescommonly used in dengue virus infection studies, i.e., monkeykidney Vero and LLCMK2 cells and human monocyte-like U937 cells.Unequivocal binding of intact virus was observed with Vero andLLCMK2 cells, while much lower binding was seen with U937 cells(Fig. 5A to C). In contrast to Vero and LLCMK2 cells, U937 cellsare Fc receptor-bearing monocyte-like cells which support antibody-dependentdengue virus infection but are relatively poorly infectible inthe absence of dengue virus-specific antibody (7, 17). Thecell binding results with intact virus further support the ideathat permissiveness to dengue virus infection is determined atleast in part by the degree of virus-cell binding (3), whichis a reflection of the relative abundance of virus receptors.As shown in Fig. 5A to C the trypsin-released dengue virus E ectodomain, $Delta$ E, retained partial cell-binding activity. This is the firstdirect demonstration that the cell receptor-binding portion ofany flavivirus E protein can be released in functional form bytrypsin cleavage of virus particles. It is noteworthy that $Delta$ Ebound to all three cell types apparently less efficiently thandid intact virus (Fig. 5A to C). However, this likely reflectsthe fact that cell binding of intact virus particles would bescored with greater sensitivity in our binding assay than wouldisolated E proteins. Each cell-bound virus particle contains manyE protein molecules (of the order of 90 E dimers as estimatedfor tick-borne encephalitis virus [27]), only a few of which(per virus particle) would be expected to actually participatein cell attachment. The results therefore indicate that $Delta$ E possessesmost if not all of the structural features required for cell binding.Specificity of cell binding for both virus particles and $Delta$ E wasshown by blocking studies with E-specific MAbs 3H5 and 1B7 (Fig.5D and E). For comparison, the virus neutralization activitiesfor each MAb were determined in parallel on the same preparationof radiolabeled virus. Both MAbs blocked binding of virus particlesand $Delta$ E to Vero cells (Fig. 5D and E). Blocking of virus particlebinding correlated more closely to virus neutralization for MAb3H5 than for MAb 1B7. This may suggest that MAb 3H5 neutralizesdengue virus predominantly by blocking virus-cell attachment,while MAb 1B7 neutralizes dengue virus largely by a postattachmentmechanism.

View larger version (23K):
[in this window]
[in a new window]

FIG. 5. Cell-binding activities of trypsin-released $Delta$ E and purified dengue virus. (A to C) Equal amounts of radiolabeled purified dengue virus ( $open circle$ ), trypsin-released E ectodomain () (purified by sucrose gradient fractionation as shown in Fig. 4B), and purified NS1 dimer (

) (obtained by sucrose gradient fractionation of culture fluid supernatant from virus-infected Vero cells as for Fig. 1) were incubated with equal numbers (10⁵) of Vero (A), LLC-MK2 (B), and U937 (C) cells for 90 min at 4°C. Cells were washed four times with phosphate-buffered saline, and the amount of cell-bound radiolabel was determined by liquid scintillation counting. (D and E) Blocking of cell binding of purified dengue virus ( $open circle$ ) and $Delta$ E () was performed as described above, except that virus and $Delta$ E were preincubated with either MAb 3H5 (D) or 1B7 (E) for 60 min at room temperature prior to cell binding. Samples treated with irrelevant MAb showed no significant inhibition of binding (data not shown). For reference, the neutralization activity for each MAb was determined on the same sample of radiolabeled dengue virus (

). Data points and error bars represent the means ± standard deviations for triplicate determinations.

The precise location of the trypsin cleavage site on the dengue virus E protein remains uncertain. The E protein of tick-borneencephalitis virus is also cleaved by trypsin, at a site betweenresidues 395 and 408, probably at Lys-408 (12, 25). The correspondingregion in the dengue virus E protein similarly contains severalbasic amino acid residues representing potential trypsin sites.MAb binding sites provide some help in localizing the trypsincleavage site of the dengue virus E protein. In the present study,both MAbs 3H5 and 1B7 were shown to immunoprecipitate the trypsin-releasedE protein ectodomain. The MAb 3H5 binding site on the dengue virusE protein has been partly characterized (15, 21, 28) andprobably encompasses, at a minimum, residues 383 to 385 (15).This places the trypsin cleavage site on the carboxy side of aminoacid 385. Further studies, such as studies involving C-terminalsequencing, will help to define the trypsin cleavage site of thedengue virus Eprotein.

Elucidation of the precise sites within $Delta$ E which are involved in cell receptor binding is important to understanding celltropism of dengue virus as well as to designing possible inhibitorsof infection. Potential glycosaminoglycan-binding motifs havebeen identified on the dengue virus E protein at two sites, thebest characterized of which appears to be comprised of amino acids188, 284 to 295, and 305 to 310 and which may also play a rolein virus-cell attachment (5). There exists considerable homologyamong flaviviral E proteins, raising the possibility that differentflaviviruses may have similar receptor-binding motifs. For example,many mosquito-borne flaviviruses contain an RGD sequence (e.g.,residues 388 to 390 of the Murray Valley encephalitis virus Eprotein) which has been implicated in virulence (18) and potentialreceptor binding, by analogy with integrin-binding motifs (25).Further analyses of cell-binding activities and potential receptor-bindingactivities of proteolytic or recombinantly produced fragmentsof flaviviral E protein may help to define the sites involvedin recognition between flaviviruses and cell surfacemacromolecules.

	ACKNOWLEDGMENTS

This work was supported by the Natural Sciences and Engineering Research Council of Canada. R.A. is an associate of the DalhousieMedical ResearchFoundation.

We are grateful to Alan King, Walter Reed Army Institute of Research, for generously providing MAbs used in thisstudy.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, Dalhousie University, Halifax, Nova ScotiaB3H 4H7, Canada. Phone: (902) 494-1063. Fax: (902) 494-5125. E-mail:Anderson{at}Tupdean1.med.dal.ca.

Present address: Laboratory of Ocular Therapeutics, National Eye Institute, National Institutes of Health, Bethesda, MD20892.

REFERENCES

Top
Abstract
Text
References

1. Allison, S. L., J. Schalich, K. Stiasny, C. W. Mandl, C. Kunz, and F. X. Heinz. 1995. Oligomeric rearrangement of tick-borne encephalitis virus envelope proteins induced by an acidic pH. J. Virol. 69:695-700[Abstract].

2. Allison, S. L., K. Stadler, C. W. Mandl, C. Kunz, and F. X. Heinz. 1995. Synthesis and secretion of recombinant tick-borne encephalitis virus protein E in soluble and particulate form. J. Virol. 69:5816-5820[Abstract].

3. Anderson, R., A. D. King, and B. L. Innis. 1992. Correlation of E protein binding with cell susceptibility to dengue 4 virus infection. J. Gen. Virol. 73:2155-2159[Abstract/Free Full Text].

4. Anderson, R., S. Wang, C. Osiowy, and A. C. Issekutz. 1997. Activation of endothelial cells via antibody-enhanced dengue virus infection of peripheral blood monocytes. J. Virol. 71:4226-4232[Abstract].

5. Chen, Y., T. Maguire, R. E. Hileman, J. R. Fromm, J. D. Esko, R. J. Linhardt, and R. M. Marks. 1997. Dengue virus infectivity depends on envelope protein binding to target cell heparan sulfate. Nat. Med. 3:866-871[Medline].

6. Chen, Y., T. Maguire, and R. M. Marks. 1996. Demonstration of binding of dengue virus envelope protein to target cells. J. Virol. 70:8765-8772[Abstract].

7. Daughaday, C. C., W. E. Brandt, J. M. McCown, and P. K. Russell. 1981. Evidence for two mechanisms of dengue virus infection of adherent human monocytes: trypsin-sensitive virus receptors and trypsin-resistant immune complex receptors. Infect. Immun. 32:469-473[Abstract/Free Full Text].

8. Fonseca, B. A. L., S. Pincus, R. E. Shope, E. Paoletti, and P. W. Mason. 1994. Recombinant vaccinia viruses co-expressing dengue-1 glycoproteins prM and E induce neutralizing antibodies in mice. Vaccine 12:279-285[Medline].

9. Guirakhoo, F., R. A. Bolin, and J. T. Roehrig. 1992. The Murray Valley encephalitis virus prM protein confers acid resistance to virus particles and alters the expression of epitopes within the R2 domain of E glycoprotein. Virology 191:921-931[Medline].

10. He, R. T., B. L. Innis, A. Nisalak, W. Usawattanakul, S. Wang, S. Kalayanarooj, and R. Anderson. 1995. Antibodies that block virus attachment to Vero cells are a major component of the human neutralizing antibody response against dengue virus type 2. J. Med. Virol. 45:451-461[Medline].

11. Heinz, F. X., S. L. Allison, K. Stiasny, J. Schalich, H. Holzmann, C. W. Mandl, and C. Kunz. 1995. Recombinant and virion-derived soluble and particulate immunogens for vaccination against tick-borne encephalitis. Vaccine 13:1636-1642[Medline].

12. Heinz, F. X., C. W. Mandl, H. Holzmann, C. Kunz, B. A. Harris, F. Rey, and S. C. Harrison. 1991. The flavivirus envelope protein E: isolation of a soluble form from tick-borne encephalitis virus and its crystallization. J. Virol. 65:5579-5583[Abstract/Free Full Text].

13. Heinz, F. X., K. Stiasny, G. Puschner-Auer, H. Holzmann, S. L. Allison, C. W. Mandl, and C. Kunz. 1994. Structural changes and functional control of the tick-borne encephalitis virus glycoprotein E by the heterodimeric association with protein prM. Virology 198:109-117[Medline].

14. Henchal, E. A., J. M. McCown, D. S. Burke, M. C. Seguin, and W. E. Brandt. 1985. Epitopic analysis of antigenic determinants on the surface of dengue 2 virions using monoclonal antibodies. Am. J. Trop. Med. Hyg. 34:162-169.

15. Hiramatsu, K., M. Tadano, R. Men, and C.-J. Lai. 1996. Mutational analysis of a neutralization epitope on the dengue type 2 virus (DEN2) envelope protein: monoclonal antibody resistant DEN2/DEN4 chimeras exhibit reduced mouse neurovirulence. Virology 224:437-445[Medline].

16. Hochstenbach, F., V. David, S. Watkins, and M. B. Brenner. 1992. Endoplasmic reticulum resident protein of 90 kilodaltons associates with the T- and B-cell antigen receptors and major histocompatibility complex antigens during their assembly. Proc. Natl. Acad. Sci. USA 89:4734-4738[Abstract/Free Full Text].

17. Kliks, S. C., A. Nisalak, W. E. Brandt, L. Wahl, and D. S. Burke. 1989. Antibody-dependent enhancement of dengue virus growth in human monocytes as a risk factor for dengue hemorrhagic fever. Am. J. Trop. Med. Hyg. 40:444-451.

18. Lobigs, M., R. Usha, A. Nestorowicz, I. D. Marshall, R. C. Weir, and L. Dalgarno. 1990. Host cell selection of Murray Valley encephalitis virus variants altered at an RGD sequence in the envelope protein and in mouse virulence. Virology 176:587-595[Medline].

19. Mackall, J., M. Meredith, and M. D. Lane. 1979. A mild procedure for the rapid release of cytoplasmic enzymes from cultured animal cells. Anal. Biochem. 95:270-274[Medline].

20. Mason, P. W., S. Pincus, M. J. Fournier, T. L. Mason, R. E. Shope, and E. Paoletti. 1991. Japanese encephalitis virus-vaccinia recombinants produce particulate forms of the structural membrane proteins and induce high levels of protection against lethal JEV infection. Virology 180:294-305[Medline].

21. Megret, F., J. P. Hugnot, A. Falconar, M. K. Gentry, D. M. Morens, J. M. Murray, J. J. Schlesinger, P. J. Wright, P. Young, M. H. V. Van Regenmortel, and V. Deubel. 1992. Use of recombinant fusion proteins and monoclonal antibodies to define linear and discontinuous antigenic sites on the dengue virus envelope glycoprotein. Virology 187:480-491[Medline].

22. Pincus, S., P. W. Mason, E. Konishi, B. A. L. Fonseca, R. E. Shope, C. M. Rice, and E. Paoletti. 1992. Recombinant vaccinia virus producing the prM and E proteins of yellow fever virus protects mice from lethal yellow fever encephalitis. Virology 187:290-297[Medline].

23. Putnak, R., D. A. Barvir, J. M. Burrous, D. R. Dubois, V. M. D'Andrea, C. H. Hoke, J. C. Sadoff, and K. H. Eckels. 1996. Development of a purified, inactivated, dengue-2 virus vaccine prototype in Vero cells: immunogenicity and protection in mice and rhesus monkeys. J. Infect. Dis. 174:1176-1184[Medline].

24. Randolph, V. B., G. Winkler, and V. Stollar. 1990. Acidotropic amines inhibit proteolytic processing of flavivirus prM protein. Virology 174:450-458[Medline].

25. Rey, F. A., F. X. Heinz, C. Mandl, C. Kunz, and S. C. Harrison. 1995. The envelope glycoprotein from tick-borne encephalitis virus at 2A resolution. Nature 375:291-298[Medline].

26. Rice, C. M. 1996. Flaviviridae: the viruses and their replication, p. 931-959. In B. N. Fields, D. M. Knipe, P. M. Howley, et al. (ed.), Fields virology. Lippincott-Raven, Philadelphia, Pa.

27. Schalich, J., S. L. Allison, K. Stiasny, C. W. Mandl, C. Kunz, and F. X. Heinz. 1996. Recombinant subviral particles from tick-borne encephalitis virus are fusogenic and provide a model system for studying flavivirus envelope glycoprotein functions. J. Virol. 70:4549-4557[Abstract].

28. Trirawatanapong, T., B. Chandran, R. Putnak, and R. Padmanabhan. 1992. Mapping of a region of dengue virus type-2 glycoprotein required for binding by a neutralizing monoclonal antibody. Gene 116:139-150[Medline].

29. Wang, S., R. He, J. Patarapotikul, B. L. Innis, and R. Anderson. 1995. Antibody-enhanced binding of dengue-2 virus to human platelets. Virology 213:254-257[Medline].

This article has been cited by other articles:

Zybert, I. A., van der Ende-Metselaar, H., Wilschut, J., Smit, J. M. (2008). Functional importance of dengue virus maturation: infectious properties of immature virions. J. Gen. Virol. 89: 3047-3051 [Abstract] [Full Text]
Junjhon, J., Lausumpao, M., Supasa, S., Noisakran, S., Songjaeng, A., Saraithong, P., Chaichoun, K., Utaipat, U., Keelapang, P., Kanjanahaluethai, A., Puttikhunt, C., Kasinrerk, W., Malasit, P., Sittisombut, N. (2008). Differential Modulation of prM Cleavage, Extracellular Particle Distribution, and Virus Infectivity by Conserved Residues at Nonfurin Consensus Positions of the Dengue Virus pr-M Junction. J. Virol. 82: 10776-10791 [Abstract] [Full Text]
Etemad, B., Batra, G., Raut, R., Dahiya, S., Khanam, S., Swaminathan, S., Khanna, N. (2008). An Envelope Domain III-based Chimeric Antigen Produced in Pichia pastoris Elicits Neutralizing Antibodies Against All Four Dengue Virus Serotypes. Am J Trop Med Hyg 79: 353-363 [Abstract] [Full Text]
Kim, J.-M., Yun, S.-I., Song, B.-H., Hahn, Y.-S., Lee, C.-H., Oh, H.-W., Lee, Y.-M. (2008). A Single N-Linked Glycosylation Site in the Japanese Encephalitis Virus prM Protein Is Critical for Cell Type-Specific prM Protein Biogenesis, Virus Particle Release, and Pathogenicity in Mice. J. Virol. 82: 7846-7862 [Abstract] [Full Text]
van der Schaar, H. M., Rust, M. J., Waarts, B.-L., van der Ende-Metselaar, H., Kuhn, R. J., Wilschut, J., Zhuang, X., Smit, J. M. (2007). Characterization of the Early Events in Dengue Virus Cell Entry by Biochemical Assays and Single-Virus Tracking. J. Virol. 81: 12019-12028 [Abstract] [Full Text]
Brown, M. G., King, C. A., Sherren, C., Marshall, J. S., Anderson, R. (2006). A dominant role for Fc{gamma}RII in antibody-enhanced dengue virus infection of human mast cells and associated CCL5 release. J. Leukoc. Biol. 80: 1242-1250 [Abstract] [Full Text]
Dinglasan, R. R., Jacobs-Lorena, M. (2005). Insight into a Conserved Lifestyle: Protein-Carbohydrate Adhesion Strategies of Vector-Borne Pathogens. Infect. Immun. 73: 7797-7807 [Full Text]
Lin, Y.-J., Wu, S.-C. (2005). Histidine at Residue 99 and the Transmembrane Region of the Precursor Membrane prM Protein Are Important for the prM-E Heterodimeric Complex Formation of Japanese Encephalitis Virus. J. Virol. 79: 8535-8544 [Abstract] [Full Text]
Pryor, M. J., Azzola, L., Wright, P. J., Davidson, A. D. (2004). Histidine 39 in the dengue virus type 2 M protein has an important role in virus assembly. J. Gen. Virol. 85: 3627-3636 [Abstract] [Full Text]
Keelapang, P., Sriburi, R., Supasa, S., Panyadee, N., Songjaeng, A., Jairungsri, A., Puttikhunt, C., Kasinrerk, W., Malasit, P., Sittisombut, N. (2004). Alterations of pr-M Cleavage and Virus Export in pr-M Junction Chimeric Dengue Viruses. J. Virol. 78: 2367-2381 [Abstract] [Full Text]
Allison, S. L., Tao, Y. J., O'Riordain, G., Mandl, C. W., Harrison, S. C., Heinz, F. X. (2003). Two Distinct Size Classes of Immature and Mature Subviral Particles from Tick-Borne Encephalitis Virus. J. Virol. 77: 11357-11366 [Abstract] [Full Text]
Gritsun, T. S., Frolova, T. V., Zhankov, A. I., Armesto, M., Turner, S. L., Frolova, M. P., Pogodina, V. V., Lashkevich, V. A., Gould, E. A. (2002). Characterization of a Siberian Virus Isolated from a Patient with Progressive Chronic Tick-Borne Encephalitis. J. Virol. 77: 25-36 [Abstract] [Full Text]
Twiddy, S. S., Woelk, C. H., Holmes, E. C. (2002). Phylogenetic evidence for adaptive evolution of dengue viruses in nature. J. Gen. Virol. 83: 1679-1689 [Abstract] [Full Text]
Lorenz, I. C., Allison, S. L., Heinz, F. X., Helenius, A. (2002). Folding and Dimerization of Tick-Borne Encephalitis Virus Envelope Proteins prM and E in the Endoplasmic Reticulum. J. Virol. 76: 5480-5491 [Abstract] [Full Text]
Mackenzie, J. M., Westaway, E. G. (2001). Assembly and Maturation of the Flavivirus Kunjin Virus Appear To Occur in the Rough Endoplasmic Reticulum and along the Secretory Pathway, Respectively. J. Virol. 75: 10787-10799 [Abstract] [Full Text]
Courageot, M.-P., Frenkiel, M.-P., Duarte Dos Santos, C., Deubel, V., Desprès, P. (2000). alpha -Glucosidase Inhibitors Reduce Dengue Virus Production by Affecting the Initial Steps of Virion Morphogenesis in the Endoplasmic Reticulum. J. Virol. 74: 564-572 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Wang, S.
	Articles by Anderson, R.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Wang, S.
	Articles by Anderson, R.

1.	Allison, S. L., J. Schalich, K. Stiasny, C. W. Mandl, C. Kunz, and F. X. Heinz. 1995. Oligomeric rearrangement of tick-borne encephalitis virus envelope proteins induced by an acidic pH. J. Virol. 69:695-700[Abstract].
2.	Allison, S. L., K. Stadler, C. W. Mandl, C. Kunz, and F. X. Heinz. 1995. Synthesis and secretion of recombinant tick-borne encephalitis virus protein E in soluble and particulate form. J. Virol. 69:5816-5820[Abstract].
3.	Anderson, R., A. D. King, and B. L. Innis. 1992. Correlation of E protein binding with cell susceptibility to dengue 4 virus infection. J. Gen. Virol. 73:2155-2159[Abstract/Free Full Text].
4.	Anderson, R., S. Wang, C. Osiowy, and A. C. Issekutz. 1997. Activation of endothelial cells via antibody-enhanced dengue virus infection of peripheral blood monocytes. J. Virol. 71:4226-4232[Abstract].
5.	Chen, Y., T. Maguire, R. E. Hileman, J. R. Fromm, J. D. Esko, R. J. Linhardt, and R. M. Marks. 1997. Dengue virus infectivity depends on envelope protein binding to target cell heparan sulfate. Nat. Med. 3:866-871[Medline].
6.	Chen, Y., T. Maguire, and R. M. Marks. 1996. Demonstration of binding of dengue virus envelope protein to target cells. J. Virol. 70:8765-8772[Abstract].
7.	Daughaday, C. C., W. E. Brandt, J. M. McCown, and P. K. Russell. 1981. Evidence for two mechanisms of dengue virus infection of adherent human monocytes: trypsin-sensitive virus receptors and trypsin-resistant immune complex receptors. Infect. Immun. 32:469-473[Abstract/Free Full Text].
8.	Fonseca, B. A. L., S. Pincus, R. E. Shope, E. Paoletti, and P. W. Mason. 1994. Recombinant vaccinia viruses co-expressing dengue-1 glycoproteins prM and E induce neutralizing antibodies in mice. Vaccine 12:279-285[Medline].
9.	Guirakhoo, F., R. A. Bolin, and J. T. Roehrig. 1992. The Murray Valley encephalitis virus prM protein confers acid resistance to virus particles and alters the expression of epitopes within the R2 domain of E glycoprotein. Virology 191:921-931[Medline].
10.	He, R. T., B. L. Innis, A. Nisalak, W. Usawattanakul, S. Wang, S. Kalayanarooj, and R. Anderson. 1995. Antibodies that block virus attachment to Vero cells are a major component of the human neutralizing antibody response against dengue virus type 2. J. Med. Virol. 45:451-461[Medline].
11.	Heinz, F. X., S. L. Allison, K. Stiasny, J. Schalich, H. Holzmann, C. W. Mandl, and C. Kunz. 1995. Recombinant and virion-derived soluble and particulate immunogens for vaccination against tick-borne encephalitis. Vaccine 13:1636-1642[Medline].
12.	Heinz, F. X., C. W. Mandl, H. Holzmann, C. Kunz, B. A. Harris, F. Rey, and S. C. Harrison. 1991. The flavivirus envelope protein E: isolation of a soluble form from tick-borne encephalitis virus and its crystallization. J. Virol. 65:5579-5583[Abstract/Free Full Text].
13.	Heinz, F. X., K. Stiasny, G. Puschner-Auer, H. Holzmann, S. L. Allison, C. W. Mandl, and C. Kunz. 1994. Structural changes and functional control of the tick-borne encephalitis virus glycoprotein E by the heterodimeric association with protein prM. Virology 198:109-117[Medline].
14.	Henchal, E. A., J. M. McCown, D. S. Burke, M. C. Seguin, and W. E. Brandt. 1985. Epitopic analysis of antigenic determinants on the surface of dengue 2 virions using monoclonal antibodies. Am. J. Trop. Med. Hyg. 34:162-169.
15.	Hiramatsu, K., M. Tadano, R. Men, and C.-J. Lai. 1996. Mutational analysis of a neutralization epitope on the dengue type 2 virus (DEN2) envelope protein: monoclonal antibody resistant DEN2/DEN4 chimeras exhibit reduced mouse neurovirulence. Virology 224:437-445[Medline].
16.	Hochstenbach, F., V. David, S. Watkins, and M. B. Brenner. 1992. Endoplasmic reticulum resident protein of 90 kilodaltons associates with the T- and B-cell antigen receptors and major histocompatibility complex antigens during their assembly. Proc. Natl. Acad. Sci. USA 89:4734-4738[Abstract/Free Full Text].
17.	Kliks, S. C., A. Nisalak, W. E. Brandt, L. Wahl, and D. S. Burke. 1989. Antibody-dependent enhancement of dengue virus growth in human monocytes as a risk factor for dengue hemorrhagic fever. Am. J. Trop. Med. Hyg. 40:444-451.
18.	Lobigs, M., R. Usha, A. Nestorowicz, I. D. Marshall, R. C. Weir, and L. Dalgarno. 1990. Host cell selection of Murray Valley encephalitis virus variants altered at an RGD sequence in the envelope protein and in mouse virulence. Virology 176:587-595[Medline].
19.	Mackall, J., M. Meredith, and M. D. Lane. 1979. A mild procedure for the rapid release of cytoplasmic enzymes from cultured animal cells. Anal. Biochem. 95:270-274[Medline].
20.	Mason, P. W., S. Pincus, M. J. Fournier, T. L. Mason, R. E. Shope, and E. Paoletti. 1991. Japanese encephalitis virus-vaccinia recombinants produce particulate forms of the structural membrane proteins and induce high levels of protection against lethal JEV infection. Virology 180:294-305[Medline].
21.	Megret, F., J. P. Hugnot, A. Falconar, M. K. Gentry, D. M. Morens, J. M. Murray, J. J. Schlesinger, P. J. Wright, P. Young, M. H. V. Van Regenmortel, and V. Deubel. 1992. Use of recombinant fusion proteins and monoclonal antibodies to define linear and discontinuous antigenic sites on the dengue virus envelope glycoprotein. Virology 187:480-491[Medline].
22.	Pincus, S., P. W. Mason, E. Konishi, B. A. L. Fonseca, R. E. Shope, C. M. Rice, and E. Paoletti. 1992. Recombinant vaccinia virus producing the prM and E proteins of yellow fever virus protects mice from lethal yellow fever encephalitis. Virology 187:290-297[Medline].
23.	Putnak, R., D. A. Barvir, J. M. Burrous, D. R. Dubois, V. M. D'Andrea, C. H. Hoke, J. C. Sadoff, and K. H. Eckels. 1996. Development of a purified, inactivated, dengue-2 virus vaccine prototype in Vero cells: immunogenicity and protection in mice and rhesus monkeys. J. Infect. Dis. 174:1176-1184[Medline].
24.	Randolph, V. B., G. Winkler, and V. Stollar. 1990. Acidotropic amines inhibit proteolytic processing of flavivirus prM protein. Virology 174:450-458[Medline].
25.	Rey, F. A., F. X. Heinz, C. Mandl, C. Kunz, and S. C. Harrison. 1995. The envelope glycoprotein from tick-borne encephalitis virus at 2A resolution. Nature 375:291-298[Medline].
26.	Rice, C. M. 1996. Flaviviridae: the viruses and their replication, p. 931-959. In B. N. Fields, D. M. Knipe, P. M. Howley, et al. (ed.), Fields virology. Lippincott-Raven, Philadelphia, Pa.
27.	Schalich, J., S. L. Allison, K. Stiasny, C. W. Mandl, C. Kunz, and F. X. Heinz. 1996. Recombinant subviral particles from tick-borne encephalitis virus are fusogenic and provide a model system for studying flavivirus envelope glycoprotein functions. J. Virol. 70:4549-4557[Abstract].
28.	Trirawatanapong, T., B. Chandran, R. Putnak, and R. Padmanabhan. 1992. Mapping of a region of dengue virus type-2 glycoprotein required for binding by a neutralizing monoclonal antibody. Gene 116:139-150[Medline].
29.	Wang, S., R. He, J. Patarapotikul, B. L. Innis, and R. Anderson. 1995. Antibody-enhanced binding of dengue-2 virus to human platelets. Virology 213:254-257[Medline].