Flavivirus nonstructural protein 1 (NS1) is a unique secreted nonstructural glycoprotein. Although it is absent from the flavivirus virion, intracellular and extracellular forms of NS1 have essential roles in viral replication and the pathogenesis of infection. The fate of NS1 in insect cells has been more controversial, with some reports suggesting it is exclusively cell associated. In this study, we confirm NS1 secretion from cells of insect origin and characterize its physical, biochemical, and functional properties in the context of dengue virus (DENV) infection. Unlike mammalian cell–derived NS1, which displays both high mannose and complex type N-linked glycans, soluble NS1 secreted from DENV-infected insect cells contains only high mannose glycans. Insect cell–derived secreted NS1 also has different physical properties, including smaller and more heterogeneous sizes and the formation of less stable NS1 hexamers. Both mammalian and insect cell–derived NS1 bind to complement proteins C1s, C4, and C4-binding protein, as well as to a novel partner, mannose-binding lectin. Binding of NS1 to MBL protects DENV against mannose-binding lectin–mediated neutralization by the lectin pathway of complement activation. As we detected secreted NS1 and DENV together in the saliva of infected Aedes aegypti mosquitoes, these findings suggest a mechanism of viral immune evasion at the very earliest phase of infection.

Dengue fever, dengue hemorrhagic fever, and dengue shock syndrome have increased markedly due to the global spread of dengue virus (DENV) and the expansion of its mosquito vectors, Aedes aegypti and Aedes albopictus. DENV is now the most important viral illness transmitted by insects (1), with an estimated 390 million infections per year (2). DENV belongs to the genus Flavivirus of the Flaviviridae family. It is a positive sense single-stranded enveloped RNA virus with an ∼11-kb genome encoding three structural proteins (capsid [C], premembrane/membrane [prM/M], and envelope [E]) and seven nonstructural (NS) proteins (NS1, NS2a, NS2b, NS3, NS4a, NS4b, and NS5) that are absent from the virion, but function in viral replication and immune evasion within an infected cell. Among the NS proteins, only NS1 is displayed on cell surfaces and secreted from infected cells. DENV NS1 is a 46-kDa glycoprotein with two N-linked glycans and originally was described as a soluble complement-fixing Ag (3). DENV NS1 also functions intracellularly as a cofactor for viral replication by interacting with other structural and NS proteins, although the mechanistic basis for this activity remains poorly understood (4, 5).

NS1 is postulated to contribute to the pathogenicity of dengue diseases. High plasma levels of NS1 and terminal complement complexes C5b-9 observed in DENV-infected patients correlate with the development of severe dengue disease (6). Soluble NS1 enhances infection in hepatocyte cell lines (7), elicits autoantibodies that cross-react with platelets and extracellular matrix proteins, and promotes endothelial cell damage via Ab-dependent complement-mediated cytolysis (810). Moreover, soluble NS1 facilitates immune complex formation and complement activation, which can trigger microvesicle shedding from erythrocytes (6, 11). Soluble hexameric NS1 associates with lipids and forms lipoprotein particles that can impact vascular endothelial function and integrity (12, 13). Binding of soluble NS1 to endothelial cells triggers TLR-2, TLR-4, and TLR-6 activation, resulting in proinflammatory cytokine generation and loss of endothelial cell junction integrity (1315). Soluble NS1 also binds back to the plasma membrane of cells through an interaction with specific sulfated glycosaminoglycans (GAGs) (16), which could contribute to tissue-specific vascular leakage that occurs during a severe secondary DENV infection (6, 17). Moreover, NS1 has a separate immune evasion activity as it antagonizes complement activation, which limits inhibitory effects on flavivirus infection (1820).

Previous studies have reported that flavivirus-infected mammalian but not insect cells secrete NS1 into the extracellular milieu (4, 18, 19). However, using a more sensitive assay for NS1 detection, we and others have detected NS1 in the culture supernatants of DENV-infected insect cells, including Spodoptera frugiperda cells (20) and A. albopictus mosquito-derived C6/36 cells (21). The presence of NS1 in the culture medium of insect cells was not due to lysis, but rather an active process requiring N-linked glycosylation and the protein secretory pathway. In this study, we investigated the physical and functional properties of NS1 secreted from DENV-infected insect cells. We showed that soluble NS1 from DENV-infected insect cells, analogous to mammalian cell–derived NS1, formed hexamers and bound to human complement components C1s, C4, and C4b-binding protein to restrict classical pathway–dependent complement activation. We also observed a novel complement evasion function of NS1 via an interaction with mannose-binding lectin (MBL) to protect DENV from MBL-mediated neutralization. Finally, along with DENV, NS1 was detected in the saliva of infected mosquitoes, suggesting a potential role for limiting complement recognition and activation at the site of the mosquito bite.

All transformed cell lines were obtained from the American Type Culture Collection. Three insect cell lines, the C6/36 clone of A. albopictus cells, the AP-61 cell line from Aedes pseudoscutellaris, and the TRA-284 cell line from Toxorhynchites amboinensis, were grown in L-15 medium (Life Technologies) supplemented with 10% tryptose phosphate broth (Sigma-Aldrich) and 10% FBS (Hyclone) at 28°C. The swine fibroblast cell line (PscloneD) was grown in L-15 medium supplemented with 10% tryptose phosphate broth and 10% FBS at 37°C. Baby hamster kidney fibroblast (BHK) and Vero cell lines were cultured in DMEM supplemented with 10% FBS, 50 mM HEPES, 4 mM l-glutamine, 100 U/ml penicillin G, and 100 μg/ml streptomycin sulfate and complete MEM at 37°C. BHK cells that stably propagate a DENV-2 subgenomic replicon (BHK DENV-2 Rep cells) (22) were grown in DMEM containing 10% FBS and 3 μg/ml puromycin (Sigma-Aldrich).

DENV serotype 2 strain 16681 was propagated in C6/36 cells (17). DENV titer was determined by focus-forming assay (FFA) on Vero cells, as previously described (8).

Sources of insect cell–derived NS1 were from culture supernatants of the following: 1) DENV-infected C6/36 cells; 2) DENV-infected AP-61 cells; 3) DENV-infected TRA-284 cells; and 4) DENV NS1–transfected Drosophila S2 cells. Mammalian cell–derived DENV NS1 was prepared from culture supernatants of serum-free DENV-infected PscloneD or Vero cells and BHK DENV-2 Rep cells. For the PscloneD and Vero cells, cells were infected with DENV-2 at a multiplicity of infection (MOI) of 0.1 and cultured in serum-free L-15 medium. At 3 d postinfection, clarified supernatants were collected, aliquoted, and stored at −70°C until use. In some experiments, supernatants were concentrated by ultrafiltration with a 30-kDa cutoff membrane (Millipore). Levels of NS1 in culture supernatants were determined by quantitative NS1-ELISA (6).

Drosophila S2 cells stably expressing recombinant NS1 of DENV-2 (S2-NS1 cells) were generated following cotransfection of plasmids pMT/DV2NS1 (gene encoding NS1 protein of dengue serotype 2 cloned into an expression vector, pMT/BiP/V5-His) and pCoHygro after hygromycin drug selection. The resulting S2/DV2NS1 stable cells were induced by CuSO4 for 5–7 d to produce and secrete S2-NS1 into serum-free culture supernatant. S2-NS1 was purified subsequently by immunoaffinity chromatography using anti-NS1 mAb 2G6-coupled beads and eluted with 20 mM diethylamine in PBS (pH 11.3), as modified from a previously described protocol (6). Purified S2-NS1 possessed similar physical characteristics to that of naturally produced viral NS1, including a heat-sensitive dimeric form in SDS-PAGE and Western blot analysis and a hexameric form in solution, as judged by size exclusion chromatography (C. Puttikhunt and T. Prommool, unpublished observations).

Soluble NS1 from DENV-infected C6/36 or Vero supernatants was purified by affinity chromatography. Briefly, 1 L DENV-infected C6/36 or Vero supernatants was centrifuged at 13,000 × g for 10 min at 4°C before purification by anti-NS1 mAbs (clone 2E11) conjugated to cyanogen bromide beads (6). Purified NS1 protein was dialyzed against PBS and stored at −70°C until use.

C6/36 or PscloneD cells were infected with DENV at MOIs of 0.01, 0.1, and 1.0. After viral adsorption for 2 h at 37°C, cell monolayers were washed once with culture medium and incubated for 2 d. Levels of NS1 and DENV in culture supernatants were determined by NS1-ELISA (6) and FFA, as described above. To determine cell viability, cells were collected using a cell scraper and washed twice with RPMI 1640 (Life Technologies) containing 1% FBS, and then 106 cells were added to 300 μl RPMI 1640 containing 1% FBS and 0.1 μg propidium iodide (Invitrogen) and analyzed by flow cytometry (BD Biosciences). To determine viral Ag expression, cells were fixed and permeabilized with 3.7% formaldehyde in PBS and 1% Triton X-100 in PBS prior to incubation with mAbs specific for NS1 (clone 2G6) or E (clone 3H5) proteins. After three washes, the cells were incubated with a rabbit anti-mouse Ig conjugated to FITC (1:50; Dako) before analysis by flow cytometry.

NS1 in the culture supernatants of DENV-infected C6/36, AP-61, and TRA-284 cells was concentrated by ultrafiltration, as described above, and analyzed by Western blotting with a mAb specific for NS1, clone 1F11, and HRP-conjugated anti-goat IgG (GE Healthcare).

Fifty-fold concentrated supernatants from DENV-infected C6/36 or PscloneD cells were mixed with nonreducing sample buffer (40% glycerol, 0.02% bromophenol blue in 0.2 M Tris-HCl, pH 6.8) without boiling. After separation in a 4–12% gradient native PAGE, as previously described (23), Western blotting analysis was performed with anti-DENV NS1 mAb, as described above.

Two hundred microliters of 50-fold concentrated DENV-2–infected C6/36 or PscloneD culture supernatants was loaded onto a Superdex 200 column (Pharmacia) at a rate of 0.4 ml/min. Thirty fractions (0.5 ml each) were collected, and the NS1 concentration in each fraction was determined by NS1-ELISA (6). The reference protein size markers (0.5 mg/ml, 200 μl), including thyroglobulin (Sigma-Aldrich), RNase A (Pharmacia), BSA (Sigma-Aldrich), and human Ig (Alpha Therapeutic), were separated in parallel.

Fifty-fold concentrated DENV-infected C6/36 or PscloneD supernatant was loaded on top of a 5–55% sucrose gradient (1 ml at each concentration with a 5% decrease in concentration at each step) and centrifuged at 35,000 × g for 20 h at 4°C using an SW-40ti rotor (Beckman). One-milliliter fractions were collected from top to bottom. The presence of NS1 in each fraction was detected by Western blotting with anti-NS1 mAb (clone 1F11).

Fifty-fold concentrated culture supernatants from DENV-infected C6/36 or PscloneD cells were subjected to digestion with endoglycosidase H (Endo H) or peptide N-glycosidase F (PNGase F) (New England Biolabs), according to the manufacturer’s protocol. NS1 bands were determined by Western blotting assay, as described above.

The binding of NS1 to complement proteins, including C1s proenzyme (proC1s), C4, C4BP, factor H, and MBL, was determined by ELISA, as previously described (24). Briefly, microtiter plates were coated with BSA or purified human complement proC1s, C4, C4BP, factor H, and MBL (15 μg/ml in PBS). Nonspecific binding sites in each well were blocked with 2% BSA in PBS before incubation with equal concentrations (determined by NS1-ELISA) of NS1 in the culture supernatants from DENV-infected C6/36 or PscloneD cells, S2-NS1 cells, or purified soluble NS1 from DENV-infected C6/36 or Vero cells. The plates were incubated with 10 μg/ml DENV NS1–specific polyclonal Abs, followed by biotinylated goat anti-mouse IgG (10 μg/ml; Sigma-Aldrich) and HRP-conjugated streptavidin (2 μg/ml). The signal was developed with ortho-phenylene diaminedihydrochloride (Sigma-Aldrich), and the reaction was terminated by the addition of 4 M H2SO4 before evaluation on a 96-well plate reader at an OD of 492 nm. Five washes with 0.05% Tween 20 in PBS were performed between each step. Mock-infected supernatants from each cell type were used as negative controls.

One milliliter NS1-containing supernatants was incubated with purified human MBL (0.75 μg; Enzon) at 4°C overnight and then immunoprecipitated with anti-NS1 mAb (2G6)–Sepharose at 4°C overnight. After five washes, the samples were added to SDS sample buffer and separated by 10% SDS-PAGE (reducing or nonreducing conditions). Western blotting was performed using 0.2 μg/ml mouse anti-human MBL mAb (Quidel), followed by HRP-conjugated anti-mouse IgG (GE Healthcare).

Binding of NS1 to cell surfaces was determined, as previously described (16). Briefly, the human keratinocyte cell line HaCat and BHK cells were removed from tissue culture plates after incubation with an EDTA solution (4 mM EDTA plus 10% FBS in PBS). Cells (5 × 105) in suspension were incubated on ice for 1 h with 100 μl 2-fold serially diluted NS1-containing culture supernatants from DENV-infected C6/36 and PscloneD or DENV NS1–transfected S2 cells. After washing once with 3 ml medium, 50 μl DENV-2 NS1–specific mAb 2G6 (10 μg/ml) was added to the cells and incubated on ice for 45 min. After subsequent washing, bound primary mAbs were detected after a 30-min incubation with a 1:500 dilution of Alexa Fluor 647–conjugated anti-mouse IgG (Invitrogen). In some experiments, 10 μg/ml heparin was added to inhibit NS1 binding. Propidium iodide (0.2 μg/ml) was added immediately before analysis by flow cytometry to exclude dead cells.

The experiments were performed, as previously described (25). Adherent BHK or HaCat cells were detached by an EDTA solution, as described above. Concentrated serum-free supernatants from S2-NS1 cells (containing 32 μg/ml NS1, as judged by NS1-ELISA) or BSA (2.5 μg/ml) were mixed with C4BP (2.5 μg/ml), and the BSA-C4BP or NS1-C4BP mixture was added to cells (1 × 106). After a 1-h incubation on ice, the cells were washed three times with cold DMEM. Surface-bound C4BP and NS1 were detected after adding mouse anti-DENV NS1 2G6 mAb (26) or mouse anti-human C4BP MK 104 mAb (27), followed by a 1:500 dilution of Alexa Fluor 647–conjugated goat anti-mouse IgG (Invitrogen) and 0.2 μg/ml propidium iodide to exclude dead cells and analyzed by flow cytometry. BHK cells were incubated with BSA, supernatants containing NS1, or C4BP alone.

Recruitment of C4BP by NS1 to the cell surface, followed by measurement of the cofactor activity of C4BP, was performed according to a previous study (25). Briefly, serum-free supernatants (200 μl) containing 12 μg/ml NS1 from DENV-infected C6/36, DENV-infected PscloneD cells, or S2-NS1 cells were incubated with C4BP (2.5 μg/ml, 50 μl) for 1 h on ice. Adherent BHK cells (1 × 106) were detached by PBS supplemented with 8 mM EDTA. Subsequently, 10% FBS was added to the C4BP solution (with or without NS1) and incubated for 1 h on ice. After three washes with 1 ml DMEM at 4°C, cells were washed with 1 ml dextrose veronal-buffered saline (2.5 mM veronal buffer [pH 7.35], 25 mM NaCl, and 240 mM glucose) at 4°C. C4b (400 ng) and factor I (200 ng) diluted in dextrose veronal-buffered saline were added to cell pellets in a total volume of 50 μl. After a 15-min incubation at 37°C, cells were pelleted and supernatants were mixed with SDS sample buffer supplemented with 2-ME (5% v/v) and subjected to 12% SDS-PAGE. C4b fragmentation was analyzed by Western blotting using a 1:2000 dilution of anti-C4d mAb (Quidel), followed by a 1:5000 dilution of HRP-conjugated anti-mouse IgG.

The binding of MBL to DENV was determined by a MBL-DENV capture ELISA, as previously described (28). Briefly, microtiter plates were adsorbed with an anti-DENV prM protein-specific mAb 2H2 (10 μg/ml in PBS) (29) at 4°C overnight. DENV-2 stocks were diluted in DMEM to 5 × 105 PFU/ml in 50 μl and added to the wells. After five washes, MBL (3 μg/ml) was diluted in binding buffer (20 mM Tris-HCl [pH 7.4], 0.05% Tween 20, 0.1% [w/v] BSA, 1 M NaCl, and 10 mM CaCl2) together with 2-fold increasing concentrations (0–50 ng/ml) of recombinant NS1 from S2 cell culture supernatants. After five washes, DENV-bound MBL was detected with biotin-conjugated mouse anti-human MBL mAb (1 μg/ml; Cedarlane), followed by HRP-conjugated streptavidin (2 μg/ml). After six final washes with PBS, the signal was detected, as described above. For a negative control, purified human MBL was diluted in 20 mM Tris-HCl (pH 7.4) and 150 mM NaCl supplemented with 40 mM EDTA. In some experiments, NS1 was depleted by preincubation of culture supernatants with anti-NS1 mAb (2E11)–Sepharose (100 μl supernatants per 30 μl packed beads) at 4°C for 24 h. Anti-E mAb (4G2)–Sepharose was used as a negative control for NS1 depletion condition.

Experiments showing the effect of NS1 on MBL-mediated neutralization of DENV were modified from a previous paper (28). Briefly, 3 μg/ml purified recombinant human MBL was preincubated with 10-fold increasing concentrations (0–150 ng/ml in gelatin veronal buffer supplemented with Mg2+ and Ca2+ [GVB2+; Complement Technology]) of recombinant NS1 from S2 cells at 4°C for 2 h. DENV (102 focus-forming unit) was incubated with a MBL-NS1 mixture for 1 h at 37°C. Infectious DENV was quantified subsequently by FFA (8) or plaque-forming assay (28). In some experiments, NS1 in culture supernatants was depleted, as described above, and MBL (3 μg/ml) premixed with purified hexameric NS1 (24) (4, 21, and 43 μg/ml), thyroglobulin (10, 50, and 100 μg/ml), or BSA (1, 5, and 10 μg/ml) with molar ratios of 1:1, 1:5, and 1:10 (MBL:protein). Soluble mannan (100 μg/ml) was used as a MBL inhibitor. To confirm this effect of NS1 derived from DENV-infected insect cells, purified soluble NS1 from DENV-infected C6/36 was used. Briefly, MBL (2 μg/ml) was premixed with purified soluble NS1 from DENV-infected C6/36 supernatant (0, 1, 2, 4, 8, and 16 μg/ml). An equal concentration of BSA was used as a negative control.

The virus attachment assay was based on a published protocol (30) with some modifications. DENV (105 focus-forming unit/ml) was incubated with or without 80 μg/ml MBL (diluted with GVB2+) together with purified NS1 (50 μg/ml) from NS1-transfected S2 cells or DENV-infected Vero cells at 37°C for 1 h. The mixture was then added to a BHK cell suspension (4 × 103, MOI = 25), followed by a 2-h incubation on ice. Cells were washed five times with GVB2+ prior to RNA extraction using a conventional TRIzol-chloroform method. DENV genome copies per cell were determined by real-time RT-PCR with capsid-specific primers using SYBR Green detection technique (6). The penultimate wash buffers were collected and subjected to RNA extraction and virus quantitation as negative controls.

Laboratory-reared female A. aegypti mosquitoes were used in this experiment. Mosquitoes were reared at 27°C ± 2°C at 80% relative humidity under a photo regimen of 12:12 h (light:dark). Larvae were fed with fish food (C.P. Hi Pro) on a regular basis. Adults were provided with 10% sucrose solutions as an energy source. A. aegypti females (4–6 d old) were starved for 6 h prior to the experiments.

Infectious blood meal comprising human blood mixed with DENV was used. Mosquitoes were infected using a membrane-feeding technique for 30 min. Glass feeders containing infectious blood meal were maintained at 37°C during feeding using a water circulator system. After feeding, mosquitoes were anesthetized using a chill table. The fully engorged females were sorted and placed in new containers. Mosquitoes were incubated at 27°C ± 2 at 80% relative humidity for 12 d and provided with sucrose-soaked cotton balls until use. After 12 d, mosquitoes were fed with fresh blood using a membrane-feeding technique for 30 min. After feeding, the remaining blood was collected, and NS1 and DENV viral RNA were determined by Western blotting, NS1-ELISA, and seminested RT-PCR, as previously described (6, 31). Mosquitoes were anesthetized using a chill table. Approximately 50 mosquito salivary glands were dissected, smeared, and fixed on glass slides to determine NS1 expression using an immunofluorescent staining assay, as previously described (6). Another 50 dissected salivary glands were lysed with 0.5% SDS sample buffer for 15 min prior to 12% SDS-PAGE (heated and reduced conditions). Western blotting was performed using anti-DENV NS1 mAb, as described above.

Data sets were statistically analyzed using Prism software (GraphPad). The Kolmogorov Smirnov test was used to test for normality. Comparisons between each group were done by t test when the distribution of the variables was comparable to a normal parametric distribution; otherwise, the Mann–Whitney U test was used. The p value ≤0.05 was considered to be statistically significant. All analyzed p values were two sided. All data were analyzed from three to four independent experiments.

Based on immunoprecipitation and Western blot analyses, it was believed previously that NS1 was secreted only from flavivirus-infected mammalian, but not insect cells (18, 19). However, consistent with more recent studies (20, 21), our sensitive NS1 capture ELISA (6) detected soluble NS1 in the culture supernatants of DENV-infected C6/36 A. albopictus cells at 2 d postinfection, albeit at lower levels than those from DENV-infected mammalian cells, including PscloneD (a pig fibroblast) and BHK (a baby hamster kidney fibroblast) cells (Fig. 1A). Increasing the inoculum of DENV virions per cell (MOI) did not affect cell viability at the time evaluated (Fig. 1B), but did increase the percentage of cells infected as determined by intracellular staining with anti-NS1 (Fig. 1C) and anti-E (Fig. 1D) Abs, virus production (Fig. 1E), and NS1 accumulation in the supernatants (Fig. 1A). Although marginal differences in the percentage of infected cells and virion production were observed between DENV-infected insect and mammalian cells (Fig. 1E), NS1 levels were higher (∼2-fold, p = 0.012) in the supernatants of infected mammalian cells (Fig. 1A). These data imply that infected insect cells secrete NS1 less efficiently than infected mammalian cells. Notably, there was a direct correlation between the levels of NS1 in the supernatant and titers of infectious virus produced in all three cell types (Fig. 1F–H).

FIGURE 1.

Detection of extracellular NS1 derived from DENV-infected insect cells. C6/36 (black bars), PscloneD (white bars), and BHK (gray bars) cells were infected with DENV at a MOI of 0.01, 0.1, or 1.0 for 2 d. The levels of secreted NS1 (A), cell viability (B), percentage of NS1 (C)- and E (D)-expressing cells, and DENV production (E) were determined by NS1-ELISA, flow cytometry analysis using propidium iodide exclusion, anti-NS1 mAb (clone 1F11), and anti-E mAb (clone 4G2) and FFA, respectively. The data are shown as mean ± SD of three to four independent experiments. Asterisks denote levels of NS1 detected in supernatants that are statistically different (*p < 0.05). The correlation coefficients between secreted NS1 and DENV production in DENV-infected C6/36 (F), DENV-infected PscloneD (G), and DENV-infected BHK (H) were analyzed by linear regression. NS1 in 50-fold concentrated supernatants of DENV-infected C6/36, AP-61, and TRA-284 cells was analyzed by Western blotting using anti-DENV NS1 mAb clone 1F11 (I).

FIGURE 1.

Detection of extracellular NS1 derived from DENV-infected insect cells. C6/36 (black bars), PscloneD (white bars), and BHK (gray bars) cells were infected with DENV at a MOI of 0.01, 0.1, or 1.0 for 2 d. The levels of secreted NS1 (A), cell viability (B), percentage of NS1 (C)- and E (D)-expressing cells, and DENV production (E) were determined by NS1-ELISA, flow cytometry analysis using propidium iodide exclusion, anti-NS1 mAb (clone 1F11), and anti-E mAb (clone 4G2) and FFA, respectively. The data are shown as mean ± SD of three to four independent experiments. Asterisks denote levels of NS1 detected in supernatants that are statistically different (*p < 0.05). The correlation coefficients between secreted NS1 and DENV production in DENV-infected C6/36 (F), DENV-infected PscloneD (G), and DENV-infected BHK (H) were analyzed by linear regression. NS1 in 50-fold concentrated supernatants of DENV-infected C6/36, AP-61, and TRA-284 cells was analyzed by Western blotting using anti-DENV NS1 mAb clone 1F11 (I).

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To determine whether NS1 secretion by mosquito cells was specific to A. albopictus cells, we extended our study to cells of other mosquito species, including AP-61 and TRA-284, which are derived from A. pseudoscutellaris and T. amboinensis, respectively. These two cell lines have been shown to efficiently generate DENV progeny and are used to isolate DENV from clinical specimens (32). Indeed, NS1 was detectable in the supernatants of all types of DENV-infected mosquito cells (Fig. 1I).

N-linked glycosylation on NS1 is essential for its folding, surface expression, secretion, and hexamer stabilization in mammalian cells (33, 34). To confirm that NS1 in the supernatants of infected insect cells (Fig. 1A) was not caused by cell lysis, DENV-infected C6/36 cells (at 24 h postinfection) were washed extensively to remove NS1-containing culture medium and treated with fresh medium containing tunicamycin, an inhibitor of N-linked glycosylation (35, 36) (Fig. 2). NS1 accumulation in the supernatant of infected C6/36 cells was reduced 10-fold over a period of 6 h with tunicamycin treatment (10 μg/ml), compared with cells treated with the vehicle control, DMSO (p = 0.02; Fig. 2A). Under these conditions, virtually no differences in the percentages of DENV-infected cells were observed (Fig. 2B, 2C), and, importantly, the intracellular expression levels of NS1 as indicated by mean fluorescence intensity between tunicamycin-treated and untreated cells were equivalent (black bars, Fig. 2B). These data suggest that inhibition of N-linked glycosylation by tunicamycin interfered only with extracellular NS1 secretion, but not intracellular NS1 or DENV infection. The decrease of NS1 secretion into the culture supernatants was not due to cell death or cell cycle arrest as there was no difference in cell viability and total cell number between tunicamycin-treated and DMSO-treated control cells (Fig. 2D, 2E). Similar to NS1 secretion, and as reported previously (37, 38), levels of DENV released into the supernatant also were reduced after tunicamycin treatment, suggesting that N-linked glycosylation is necessary for the egress of DENV from infected C6/36 cells (Fig. 2F). Overall, our data indicate that DENV-infected insect cells can secrete NS1 into the extracellular milieu and that this process requires N-linked glycosylation on the NS1 molecule.

FIGURE 2.

Tunicamycin treatment inhibits NS1 and virion release from DENV-infected insect cells. At 24 h after DENV infection, C6/36 cells were extensively washed to remove NS1-containing culture medium and treated with fresh medium containing either 0.1% DMSO or 10 μg/ml tunicamycin in 0.1% DMSO for 6 h. Levels of NS1 in supernatants (A), percentage and mean fluorescent intensity (MFI) of NS1-positive cells (B), and percentages of E-positive cells (C), percentage of living cells (D), total cell number (E), and intracellular and extracellular DENV genome copies (F) were analyzed, as described in 2Materials and Methods. The data are shown as mean ± SD from three independent experiments. Asterisks denote the means that are statistically different among indicated groups (*p < 0.05).

FIGURE 2.

Tunicamycin treatment inhibits NS1 and virion release from DENV-infected insect cells. At 24 h after DENV infection, C6/36 cells were extensively washed to remove NS1-containing culture medium and treated with fresh medium containing either 0.1% DMSO or 10 μg/ml tunicamycin in 0.1% DMSO for 6 h. Levels of NS1 in supernatants (A), percentage and mean fluorescent intensity (MFI) of NS1-positive cells (B), and percentages of E-positive cells (C), percentage of living cells (D), total cell number (E), and intracellular and extracellular DENV genome copies (F) were analyzed, as described in 2Materials and Methods. The data are shown as mean ± SD from three independent experiments. Asterisks denote the means that are statistically different among indicated groups (*p < 0.05).

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Despite the heterogeneous sizing profile of secreted flavivirus NS1 obtained from culture supernatants of mammalian cells that stably propagate DENV or West Nile virus (WNV) subgenomic replicons (16, 32), the main species of soluble NS1 is hexameric, which is similar to the soluble NS1 generated by flavivirus-infected mammalian cells (18). The size of mosquito cell–derived soluble NS1 was investigated by native gel electrophoresis, size exclusion chromatography, and sucrose density gradient centrifugation (Fig. 3). In native-PAGE analysis, secreted NS1 from DENV-infected C6/36 cells displayed three major bands, similar to NS1 secreted from DENV-infected Vero cells (molecular mass ranged between >200 and 660 kDa), but were slightly smaller in size and migrated faster in the gel (upper panel, lane 1 [C6/36-NS1] versus lane 3 [Vero-NS1], Fig. 3A). The size of extracellular NS1 released from Vero cells was slightly larger, most likely due to the addition of complex type N-linked glycans at position Asn130 of the NS1 molecule in the Golgi apparatus, which only occurs in mammalian cells (39) (lower panel, lane 3 versus lanes 1, 2, and 4, Fig. 3A). In contrast, intracellular NS1 derived from both DENV-infected mammalian and insect cells appeared more heterogeneous, showing broadly smeared bands on the native PAGE (upper panel, lanes 2 and 4; Fig. 3A), whereas, in a regular SDS-PAGE under heat and reducing conditions, both secreted and cell-associated NS1 from insect and mammalian cells migrated at 45–50 kDa (lower panel, Fig. 3A).

FIGURE 3.

Oligomeric assembly, glycosylation pattern, and stability of NS1 secreted from DENV-infected insect cells. Fifty-fold concentrated supernatants (lanes 1 and 3) and cell lysates (lanes 2 and 4) from DENV-infected C6/36 cells (lanes 1 and 2) and Vero cells (lanes 3 and 4) were separated by native PAGE [(A), upper panel] and reducing 10% SDS-PAGE [(A), lower panel] and Western blotted with 1F11 DENV NS1–specific mAb. (B) Fifty-fold concentrated DENV-2–infected C6/36 (dashed line) and PscloneD (solid line) supernatants were passed over a Superdex 200 column, and fractions were collected and quantitated for NS1 concentration by NS1-ELISA. Molecular weights of reference protein standards fractionated in parallel are depicted. (C) Fifty-fold concentrated DENV-infected C6/36 or PscloneD supernatant was loaded on a 5–55% sucrose gradient. NS1 in each fraction was detected by Western blotting with 1F11 anti-NS1 mAb. Arrowheads indicate molecular mass of protein standards. (D) Endoglycosidase (Endo H or PNGase F) treatment of extracellular NS1 derived from C6/36 (lanes 1, 2, 5, and 6) and PscloneD (lanes 3, 4, 7, and 8) cells prior to Western blot analysis with 1F11 anti-NS1 mAb. (E and F) NS1 stability test. Supernatants from DENV-infected C6/36 and Vero cells were incubated in the presence of a protease inhibitor (10 mM PMSF) at 4°C or 37°C for 3 d. Amounts of NS1 at each time point of C6/36 cell derived or Vero cell derived at 4°C and 37°C were determined by ELISA and calculated by normalizing the zero time point of each condition to 100% (E) and by Western blotting with 1F11 anti-NS1 mAb (F). Error bars indicate SD corresponding to three independent experiments. Values that are significantly different from the value for zero time point are indicated by asterisks, as follows: *p < 0.05, **p < 0.01, ***p < 0.001.

FIGURE 3.

Oligomeric assembly, glycosylation pattern, and stability of NS1 secreted from DENV-infected insect cells. Fifty-fold concentrated supernatants (lanes 1 and 3) and cell lysates (lanes 2 and 4) from DENV-infected C6/36 cells (lanes 1 and 2) and Vero cells (lanes 3 and 4) were separated by native PAGE [(A), upper panel] and reducing 10% SDS-PAGE [(A), lower panel] and Western blotted with 1F11 DENV NS1–specific mAb. (B) Fifty-fold concentrated DENV-2–infected C6/36 (dashed line) and PscloneD (solid line) supernatants were passed over a Superdex 200 column, and fractions were collected and quantitated for NS1 concentration by NS1-ELISA. Molecular weights of reference protein standards fractionated in parallel are depicted. (C) Fifty-fold concentrated DENV-infected C6/36 or PscloneD supernatant was loaded on a 5–55% sucrose gradient. NS1 in each fraction was detected by Western blotting with 1F11 anti-NS1 mAb. Arrowheads indicate molecular mass of protein standards. (D) Endoglycosidase (Endo H or PNGase F) treatment of extracellular NS1 derived from C6/36 (lanes 1, 2, 5, and 6) and PscloneD (lanes 3, 4, 7, and 8) cells prior to Western blot analysis with 1F11 anti-NS1 mAb. (E and F) NS1 stability test. Supernatants from DENV-infected C6/36 and Vero cells were incubated in the presence of a protease inhibitor (10 mM PMSF) at 4°C or 37°C for 3 d. Amounts of NS1 at each time point of C6/36 cell derived or Vero cell derived at 4°C and 37°C were determined by ELISA and calculated by normalizing the zero time point of each condition to 100% (E) and by Western blotting with 1F11 anti-NS1 mAb (F). Error bars indicate SD corresponding to three independent experiments. Values that are significantly different from the value for zero time point are indicated by asterisks, as follows: *p < 0.05, **p < 0.01, ***p < 0.001.

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To analyze the oligomeric states of NS1 secreted from infected insect cells in more detail, culture supernatants were subjected to size exclusion chromatography and sucrose density gradient centrifugation in parallel with those from infected mammalian cells (Fig. 3B, 3C). Consistent with secreted mammalian cell–derived NS1, the form of NS1 released from DENV-infected C6/36 cells ranged from monomer to oligomer. However, insect cell–derived NS1 exhibited a more heterogeneous profile with two separate peaks of monomer and higher-order oligomer, whereas the sizing profile of NS1 from infected mammalian cells appeared as a broad single peak at ∼44–660 kDa (Fig. 3B, 3C). Sucrose density gradient centrifugation analysis revealed a high molecular mass, and possibly aggregated, form of insect cell–derived NS1, which was not observed in the supernatants of mammalian cells (fraction 1, Fig. 3C). As we previously reported that the complex-type N-linked glycosylation at Asn130 is required for the stability of hexameric NS1 (34), and insect cells lack glycosyltransferase enzymes that synthesize hybrid and complex-type N-linked glycans (40), we reasoned that the aggregated form of insect cell–derived NS1 was most likely due to the lack of complex-type glycans.

The glycosylation state of DENV NS1 secreted from infected mosquito cells was further analyzed by digestion with two glycosidase enzymes, as follows: Endo H, which removes high mannose-content sugars (41), and PNGase F, which cleaves all types of N-linked glycans (42, 43). As expected, after digestion with either Endo H or PNGase F, NS1 secreted from DENV-infected C6/36 cells had similar sizes in SDS-PAGE (lanes 2 and 6, Fig. 3D), whereas Endo H–digested DENV-infected mammalian cell–derived NS1 had a band that was higher in molecular mass compared with PNGase F digestion (lanes 4 versus 8, Fig. 3D). The presence of uncleaved NS1 after PNGase F treatment was most likely from inefficient digestion (upper bands, lanes 6 and 8, Fig. 3D). These data confirm that secreted NS1 from DENV-infected C6/36 cells had high mannose-type glycosylation, whereas mammalian cell–derived NS1 displayed both Endo H–sensitive high mannose and Endo H–resistant complex-type glycans.

Data from our previous study demonstrated that N-linked glycans regulate NS1 transport through the secretory pathway and affect protein stability (34). We therefore tested the stability of soluble NS1 protein derived from DENV-infected C6/36 and Vero cells by incubating the supernatants in the presence of a protease inhibitor (10 mM PMSF) at either 4 or 37°C. The supernatants were collected daily for 3 d for NS1 quantification by ELISA (Fig. 3E) and Western blotting assay (Fig. 3F). As expected, NS1 derived from DENV-infected C6/36 cells, which lacks complex-type N-linked glycans, was degraded more rapidly, especially at 37°C, compared with NS1 derived from DENV-infected Vero cells (Fig. 3E, 3F).

Soluble NS1 from DENV-infected mammalian cells has immune evasion properties, as it directly antagonizes complement activation (24, 25); binding of DENV NS1 to C4 and C1s/C1s proenzyme resulted in C4 degradation and decreased complement activation (24). Additionally, DENV NS1 binds to C4BP, the major inhibitor of the classical/lectin pathway of complement activation in plasma, to control the activation of these pathways on cell surfaces (25). We hypothesize that insect cell–derived NS1 also has complement-inhibitory functions. In the skin, at the site of the mosquito bite in which both DENV and potentially soluble NS1 are simultaneously inoculated, complement antagonism might prevent the recognition and immediate complement-dependent neutralization of DENV and thus facilitate infection and spread.

To assess whether insect cell–derived NS1 could antagonize complement functions, we initially determined its capacity to bind human complement proteins (Fig 4A). Using comparable levels of NS1, as measured by ELISA (Fig. 4B), we observed that NS1 secreted from two different cells of insect origin (DENV-infected C6/36 cells and Drosophila S2-transfected cells) bound human complement proteins, including proC1s, C4, and C4BP, to the same extent as mammalian cell–derived NS1 (Fig. 4A). As previously observed, and in contrast to WNV NS1 (18), DENV NS1 did not bind to factor H, the major complement-regulatory protein of the alternative pathway (Fig. 4A).

FIGURE 4.

Functional properties of extracellular NS1 derived from DENV-infected insect cells. (A) Insect cell–derived NS1 binds human complement. Microtiter plates were coated with BSA, factor H, ProC1s, C4, and C4BP (5 μg/ml) and incubated with culture supernatants of DENV-infected C6/36, PscloneD, and S2-NS1 cells. Bound NS1 was detected with specific mAbs. Values (OD at 492 nm) of NS1 binding to each complement component were subtracted from those of BSA control. Error bars indicate SD corresponding to three independent experiments. Asterisks denote NS1 binding that is statistically different from corresponding mock controls (**p < 0.01, ***p < 0.001). Levels of NS1 in the supernatants were determined by NS1-ELISA (B). (C and D) Insect cell–derived NS1 binds to cell surfaces via GAGs. Serum-free supernatants of DENV-infected PscloneD (C and D), C6/36 (C and D), and S2-NS1 (D) cells containing indicated concentrations of NS1 were incubated with BHK (C) and HaCat (D) cells, and NS1 binding was detected by 2G6 anti-DENV NS1 mAb. Binding also was performed in the presence of 10 mM heparin (C). Error bars indicate SD of the mean corresponding to three independent experiments. Asterisks denote the means that are statistically different from 0 μg/ml NS1 (*p < 0.05, **p < 0.01, ***p < 0.001). (E) NS1 secreted from insect cells recruits C4BP to the cell surface. C4BP or BSA (2.5 μg/ml) was incubated with serum-free supernatants of S2-NS1 cells and 106 BHK cells. Binding of NS1 and C4BP to the cell surface was assessed by mAbs to DENV NS1 or C4BP and analyzed by flow cytometry. Examples of contour plots from three independent experiments are depicted. The y-axis indicates the levels of cell surface–associated C4BP or NS1, and the x-axis shows the forward scatter of the cell population. Percentages of cells positive for surface NS1 or C4BP staining are shown in the right upper quadrant. (F) Extracellular NS1 derived from insect cells recruits C4BP to degrade C4b on the cell surface. Serum-free supernatants (containing 12 μg/ml NS1) from DENV-infected PscloneD (lane 2), DENV-infected C6/36 (lanes 3 and 6), or S2-NS1 (lane 4) cells were preincubated with 2.5 μg/ml C4BP, and the NS1-C4BP solution was added to BHK cells. After three washes, the cells were incubated with C4b and factor I for 15 min. Cofactor activity was determined in the supernatants by the appearance of C4b cleavage products, a 70-kDa α3-C4d and a 45-kDa C4d after 12% SDS-PAGE under reducing condition, followed by Western blot with anti-C4d mAb. (G) Diagram of factor I (FI)–mediated cleavage of C4b in the presence of a cofactor C4BP. FI cleaves the α′ chain of C4b at two sites [designated as (A) and (B)]. Cleavage at either one of the two sites generates two partial cleavage fragments, C4d-α4 (59 kDa) and α3-C4d (70 kDa). Further cleavage by FI yields the final product C4d (45 kDa).

FIGURE 4.

Functional properties of extracellular NS1 derived from DENV-infected insect cells. (A) Insect cell–derived NS1 binds human complement. Microtiter plates were coated with BSA, factor H, ProC1s, C4, and C4BP (5 μg/ml) and incubated with culture supernatants of DENV-infected C6/36, PscloneD, and S2-NS1 cells. Bound NS1 was detected with specific mAbs. Values (OD at 492 nm) of NS1 binding to each complement component were subtracted from those of BSA control. Error bars indicate SD corresponding to three independent experiments. Asterisks denote NS1 binding that is statistically different from corresponding mock controls (**p < 0.01, ***p < 0.001). Levels of NS1 in the supernatants were determined by NS1-ELISA (B). (C and D) Insect cell–derived NS1 binds to cell surfaces via GAGs. Serum-free supernatants of DENV-infected PscloneD (C and D), C6/36 (C and D), and S2-NS1 (D) cells containing indicated concentrations of NS1 were incubated with BHK (C) and HaCat (D) cells, and NS1 binding was detected by 2G6 anti-DENV NS1 mAb. Binding also was performed in the presence of 10 mM heparin (C). Error bars indicate SD of the mean corresponding to three independent experiments. Asterisks denote the means that are statistically different from 0 μg/ml NS1 (*p < 0.05, **p < 0.01, ***p < 0.001). (E) NS1 secreted from insect cells recruits C4BP to the cell surface. C4BP or BSA (2.5 μg/ml) was incubated with serum-free supernatants of S2-NS1 cells and 106 BHK cells. Binding of NS1 and C4BP to the cell surface was assessed by mAbs to DENV NS1 or C4BP and analyzed by flow cytometry. Examples of contour plots from three independent experiments are depicted. The y-axis indicates the levels of cell surface–associated C4BP or NS1, and the x-axis shows the forward scatter of the cell population. Percentages of cells positive for surface NS1 or C4BP staining are shown in the right upper quadrant. (F) Extracellular NS1 derived from insect cells recruits C4BP to degrade C4b on the cell surface. Serum-free supernatants (containing 12 μg/ml NS1) from DENV-infected PscloneD (lane 2), DENV-infected C6/36 (lanes 3 and 6), or S2-NS1 (lane 4) cells were preincubated with 2.5 μg/ml C4BP, and the NS1-C4BP solution was added to BHK cells. After three washes, the cells were incubated with C4b and factor I for 15 min. Cofactor activity was determined in the supernatants by the appearance of C4b cleavage products, a 70-kDa α3-C4d and a 45-kDa C4d after 12% SDS-PAGE under reducing condition, followed by Western blot with anti-C4d mAb. (G) Diagram of factor I (FI)–mediated cleavage of C4b in the presence of a cofactor C4BP. FI cleaves the α′ chain of C4b at two sites [designated as (A) and (B)]. Cleavage at either one of the two sites generates two partial cleavage fragments, C4d-α4 (59 kDa) and α3-C4d (70 kDa). Further cleavage by FI yields the final product C4d (45 kDa).

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We next tested whether NS1 secreted from DENV-infected insect cells bound to the surface of cells. Again, analogous to mammalian cell–derived NS1 (16), NS1 secreted from DENV-infected and transfected insect cells bound to the surface of BHK cells in a dose-dependent manner (Fig. 4C). This binding required GAGs on the BHK cell surface, as the soluble GAGs (e.g., heparin) competitively inhibited NS1 attachment to the cells (Fig. 4C). A dose-dependent binding of soluble NS1 from three different sources (DENV-infected mammalian PscloneD cells, DENV-infected insect C6/36 cells, and S2-NS1 cells) also bound equivalently to the human skin keratinocyte cell line, HaCat (Fig. 4D). Keratinocytes are one of the major target cells for flavivirus infection in the skin, and the cells also have immunomodulatory functions during virus inoculation by infected mosquitoes (4447). Importantly, the interaction of insect cell–derived NS1 with the complement-regulatory protein C4BP in solution led to the attachment of C4BP to the plasma membrane via the cell-binding property of NS1 (Fig. 4E). C4BP on cell surfaces that was recruited by insect and mammalian cell–derived NS1 acted as a cofactor for factor I to cleave the α′ chain of C4b to inactive forms, the 70-kDa partial-cleavage fragment α3-C4d, and the final end product C4d (Fig. 4F, lanes 3 and 4; Fig. 4G). Of note, the 70-kDa partial-cleavage product α3-C4d also was detected without NS1 (Fig. 4F, lane 5), suggesting a small background interaction of C4BP with cells (Fig. 4E, upper panel). However, C4d was not observed when NS1 or factor I was absent (Fig. 4F, lanes 1, 5, and 6). Collectively, these experiments establish that NS1 secreted from insect cells behaves similarly to mammalian cell–derived NS1 as it binds to cell surface GAGs, specific human complement proteins, and recruits C4BP through its cofactor activity to degrade C4b on the surface of cells.

Using a complement protein-binding ELISA, we observed that soluble NS1 derived from both mammalian and insect cells bound in a dose-dependent manner to MBL, a pattern recognition molecule that initiates the lectin pathway of complement activation (Fig. 5A–C). The interaction of secreted DENV NS1 and MBL was confirmed by coimmunoprecipitation experiments (Fig. 5D). Because we previously demonstrated that direct binding of MBL to DENV neutralized infection through both complement activation-dependent and -independent mechanisms (28, 30), we reasoned that direct binding of soluble NS1 to MBL might interfere with its recognition and neutralization of DENV, independent of complement activation. To test this, purified human MBL was preincubated with culture supernatants containing increasing concentrations of insect cell–derived NS1 prior to addition to microtiter wells containing immobilized virions (Fig. 5E). As expected, NS1 competitively bound MBL in solution, which resulted in decreased MBL binding to captured DENV (Fig. 5E). Removal of NS1 from the culture supernatants using NS1-specific mAb 2E11 (26)–coupled Sepharose beads, but not anti-E mAb (4G2)–Sepharose, prior to incubating with purified MBL, restored the MBL recognition of captured DENV (Fig. 5F). Of note, abrogation of Ca2+-dependent MBL binding to DENV in the presence of EDTA served as negative controls for these experiments (Fig. 5E, 5F).

FIGURE 5.

NS1 protects DENV from MBL-mediated neutralization. (AC) NS1 binds directly to MBL. Purified human MBL was coated on a microtiter plate and incubated with NS1-containing supernatants from DENV-infected C6/36, DENV-infected PscloneD, and S2-NS1 cells (A), or with increasing concentrations of NS1 in culture supernatants of DENV-infected PscloneD and S2-NS1 cells (B), or with increasing concentrations of purified (p.) soluble NS1 from culture supernatants of DENV-infected C6/36 or Vero cells (C). Bound NS1 was detected with an anti-NS1–specific mAb. Error bars indicate SD for three independent experiments. (D) Coimmunoprecipitation experiments. Serum-free supernatants from BHK-DENV2-Rep or control BHK cells were incubated with purified human MBL (0.75 μg), and Western blots were performed after immunoprecipitation with anti-DENV NS1 2G6 mAb–Sepharose. Immunoprecipitates were probed with a mouse anti-human MBL mAb after nonreduced (upper panel) or reduced (lower panel) SDS-PAGE. (E and F) NS1 reduces MBL binding to DENV. DENV virions were captured on a microtiter plate using an anti-DENV prM protein-specific mAb and incubated with purified human MBL (3 μg/ml) with or without increasing concentrations of NS1-containing supernatants from S2-NS1 cells (E). MBL binding to captured DENV was detected with an anti-MBL–specific mAb and inhibited by the presence of 20 mM EDTA. (F) Culture supernatants from S2-NS1 cells (containing 12.5 μg/ml NS1) were incubated with anti-NS1 mAb (2E11)–Sepharose, anti-E mAb (4G2)–Sepharose, or without Sepharose (no beads) prior to addition of purified human MBL and subjected to ELISA, as described in (E). MBL binding to DENV captured on a microtiter plate in GVB2+ buffer (without NS1) or in buffer containing 20 mM EDTA was used as positive and negative controls, respectively. (GJ) NS1 inhibits MBL-mediated neutralization of DENV. DENV virions were incubated with purified human MBL without or with indicated concentrations of NS1 in supernatants from S2-NS1 cells or with NS1 supernatants alone. The mixtures were then added to a BHK monolayer, and, after carboxymethylcellulose overlay, cells were cultured for 3 d. After fixation and staining with anti-DENV E mAb, infected foci were counted (G). (H) DENV virions were incubated with purified MBL in GVB2+ buffer without or with NS1-containing supernatants (12 μg/ml) from S2-NS1 cells that were preincubated with anti-NS1 mAb (2E11)– or anti-E mAb (4G2)–Sepharose. The samples were added to a BHK monolayer, and DENV-infected foci were determined, as described in (G). MBL-mediated neutralization of DENV was abolished by 20 mM EDTA. (I) DENV virions were incubated with purified human MBL with or without indicated concentrations of purified soluble NS1 from DENV-infected C6/36 cells or with BSA control protein prior to the addition to a BHK monolayer to assess viral infectivity, as described in (G). (J) DENV virions were incubated with MBL premixed with purified hexameric NS1 derived from BHK-DENV2-Rep, thyroglobulin, or BSA at molar ratios of 1:1, 1:5, and 1:10 (MBL:protein). The samples were added to BHK monolayers, and, after agarose overlay, cultured for 5 d. After fixation and staining of wells, plaques were counted. Soluble mannan (100 μg/ml) was used as a MBL inhibitor. (K) Soluble NS1 facilitates DENV attachment to cells in the presence of human MBL. DENV was incubated with 80 μg/ml MBL (diluted with GVB2+ buffer) alone or with MBL plus BSA or purified NS1 (50 μg/ml) derived from S2-NS1 cells or DENV-infected Vero cells. The mixture was then added to BHK cell suspensions for 2 h on ice. Cell-bound DENV was determined by real-time RT-PCR. Error bars indicate SD corresponding to three independent experiments. Asterisks denote the means that are statistically different among indicated groups (*p < 0.05, **p < 0.01, ***p < 0.001).

FIGURE 5.

NS1 protects DENV from MBL-mediated neutralization. (AC) NS1 binds directly to MBL. Purified human MBL was coated on a microtiter plate and incubated with NS1-containing supernatants from DENV-infected C6/36, DENV-infected PscloneD, and S2-NS1 cells (A), or with increasing concentrations of NS1 in culture supernatants of DENV-infected PscloneD and S2-NS1 cells (B), or with increasing concentrations of purified (p.) soluble NS1 from culture supernatants of DENV-infected C6/36 or Vero cells (C). Bound NS1 was detected with an anti-NS1–specific mAb. Error bars indicate SD for three independent experiments. (D) Coimmunoprecipitation experiments. Serum-free supernatants from BHK-DENV2-Rep or control BHK cells were incubated with purified human MBL (0.75 μg), and Western blots were performed after immunoprecipitation with anti-DENV NS1 2G6 mAb–Sepharose. Immunoprecipitates were probed with a mouse anti-human MBL mAb after nonreduced (upper panel) or reduced (lower panel) SDS-PAGE. (E and F) NS1 reduces MBL binding to DENV. DENV virions were captured on a microtiter plate using an anti-DENV prM protein-specific mAb and incubated with purified human MBL (3 μg/ml) with or without increasing concentrations of NS1-containing supernatants from S2-NS1 cells (E). MBL binding to captured DENV was detected with an anti-MBL–specific mAb and inhibited by the presence of 20 mM EDTA. (F) Culture supernatants from S2-NS1 cells (containing 12.5 μg/ml NS1) were incubated with anti-NS1 mAb (2E11)–Sepharose, anti-E mAb (4G2)–Sepharose, or without Sepharose (no beads) prior to addition of purified human MBL and subjected to ELISA, as described in (E). MBL binding to DENV captured on a microtiter plate in GVB2+ buffer (without NS1) or in buffer containing 20 mM EDTA was used as positive and negative controls, respectively. (GJ) NS1 inhibits MBL-mediated neutralization of DENV. DENV virions were incubated with purified human MBL without or with indicated concentrations of NS1 in supernatants from S2-NS1 cells or with NS1 supernatants alone. The mixtures were then added to a BHK monolayer, and, after carboxymethylcellulose overlay, cells were cultured for 3 d. After fixation and staining with anti-DENV E mAb, infected foci were counted (G). (H) DENV virions were incubated with purified MBL in GVB2+ buffer without or with NS1-containing supernatants (12 μg/ml) from S2-NS1 cells that were preincubated with anti-NS1 mAb (2E11)– or anti-E mAb (4G2)–Sepharose. The samples were added to a BHK monolayer, and DENV-infected foci were determined, as described in (G). MBL-mediated neutralization of DENV was abolished by 20 mM EDTA. (I) DENV virions were incubated with purified human MBL with or without indicated concentrations of purified soluble NS1 from DENV-infected C6/36 cells or with BSA control protein prior to the addition to a BHK monolayer to assess viral infectivity, as described in (G). (J) DENV virions were incubated with MBL premixed with purified hexameric NS1 derived from BHK-DENV2-Rep, thyroglobulin, or BSA at molar ratios of 1:1, 1:5, and 1:10 (MBL:protein). The samples were added to BHK monolayers, and, after agarose overlay, cultured for 5 d. After fixation and staining of wells, plaques were counted. Soluble mannan (100 μg/ml) was used as a MBL inhibitor. (K) Soluble NS1 facilitates DENV attachment to cells in the presence of human MBL. DENV was incubated with 80 μg/ml MBL (diluted with GVB2+ buffer) alone or with MBL plus BSA or purified NS1 (50 μg/ml) derived from S2-NS1 cells or DENV-infected Vero cells. The mixture was then added to BHK cell suspensions for 2 h on ice. Cell-bound DENV was determined by real-time RT-PCR. Error bars indicate SD corresponding to three independent experiments. Asterisks denote the means that are statistically different among indicated groups (*p < 0.05, **p < 0.01, ***p < 0.001).

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Preincubation of MBL with increasing concentrations of soluble NS1 derived from insect cells (NS1 in supernatants from S2-NS1 cells) also resulted in more DENV-infected foci (Fig. 5G). Conversely, neutralization of DENV by MBL was restored when MBL was preincubated with NS1-containing supernatants that had been precleared with anti-NS1 (2E11), but not anti-E (4G2) Sepharose beads (Fig. 5H). The dose-dependent activity of insect cell–derived NS1 to inhibit DENV neutralization by human MBL was further demonstrated using NS1 purified from culture supernatants of DENV-infected C6/36 cells (Fig. 5I). Consistent with these results, complement activation-independent neutralization of DENV by MBL was also inhibited by mammalian cell–derived NS1 (Fig. 5J). Preincubation of MBL with increasing concentrations of hexameric NS1 purified from the supernatants of BHK cells that propagate DENV-2 subgenomic replicons (22, 34), but not with the control proteins, abrogated MBL-mediated neutralization of DENV (Fig. 5J).

We next investigated the mechanism by which NS1 inhibited MBL-mediated neutralization of DENV. We speculated that MBL binding to DENV prevented the attachment of viruses to cells, and, in the presence of NS1, the protein competitively bound MBL and thus allowed DENV to bind and enter target cells. To test this hypothesis, we incubated BHK cells with DENV in the presence or absence of purified human MBL. After a 2-h incubation at 4°C, cell-bound DENV was measured by real-time RT-PCR for viral genome copies. As expected, MBL efficiently inhibited DENV attachment to BHK cells. However, preincubation of MBL with either purified mammalian or insect cell–derived NS1, but not with the control protein BSA, increased the binding of DENV to BHK cells (Fig. 5K). Overall, these experiments establish that MBL inhibits DENV infection at the step of virus attachment and that NS1 competitively binds MBL, which facilitates DENV binding and entry to initiate infection.

Our data showed that mosquito cell–derived NS1 retained its biological functions, despite being secreted at a lower level than mammalian cell–derived NS1. We reasoned that during blood feeding when DENV is inoculated into the skin of a susceptible host, the presence of NS1 in the saliva of infected mosquitoes could protect DENV from immune recognition, and thus facilitate its spread from the site of inoculation. To demonstrate the relevance of our in vitro findings, we evaluated whether NS1 is present in the saliva of DENV-infected mosquitoes. A total of 1500 female A. aegypti mosquitoes was challenged orally with DENV via an infectious blood meal, as previously described (48). Successfully fed mosquitoes (∼1200) with a blood-filled midgut were sorted and subsequently incubated for 14 d until a second noninfectious blood meal was offered. The blood that remained in a container after mosquito feeding was subjected to both viral RNA and NS1 analysis. In addition, salivary glands from 50 mosquitoes were harvested and processed for immunofluorescence staining and Western blotting for DENV NS1. As expected, NS1 was detected in the salivary glands of ∼30–50% of blood-fed mosquitoes (Fig. 6A, 6B, and data not shown). Along with the DENV genome (Fig. 6C), NS1 was detected in the residual blood after mosquito feeding (Fig. 6D, 6E), indicating that both DENV and soluble NS1 were present in the saliva of infected mosquitoes and were released during blood feeding (Fig. 7).

FIGURE 6.

Both DENV and soluble NS1 are released during blood feeding from infected mosquitoes. (A) Representative bright field and immunofluorescence images of the salivary glands of mock- and DENV-infected mosquitoes. A. aegypti female mosquitoes were challenged orally with DENV by feeding them with an infectious blood meal and incubated for 14 d. Salivary glands of mosquitoes were harvested, smeared, and fixed on glass slides. NS1 was detected using a mouse anti-DENV NS1 mAb 1F11 (1 μg/ml), followed by Cy3-conjugated goat anti-mouse IgG. Nuclei were stained with Hoechst, a DNA-specific dye. Salivary glands harvested from uninfected mosquitoes served as a negative control. Analysis was performed by confocal microscopy. (B) Expression of NS1 in the salivary glands of DENV-infected mosquitoes was analyzed by Western blotting. Fifty-fold concentrated supernatants from DENV-infected C6/36 cells (DENV sup) and the salivary glands harvested from uninfected mosquitoes (Mock) served as positive and negative controls, respectively. (C and D) At 14 d after initial challenge with DENV, a total of 600–1200 mosquitoes was fed with a second noninfectious blood meal, the presence of DENV and NS1 in the remaining blood was determined by RT-PCR (C), and Western blotting was performed with DENV NS1–specific mAb 1F11 (D) and NS1-ELISA (E), respectively. Error bars indicate SD corresponding to three independent experiments. Asterisks denote the means that are statistically different among indicated groups (***p < 0.001).

FIGURE 6.

Both DENV and soluble NS1 are released during blood feeding from infected mosquitoes. (A) Representative bright field and immunofluorescence images of the salivary glands of mock- and DENV-infected mosquitoes. A. aegypti female mosquitoes were challenged orally with DENV by feeding them with an infectious blood meal and incubated for 14 d. Salivary glands of mosquitoes were harvested, smeared, and fixed on glass slides. NS1 was detected using a mouse anti-DENV NS1 mAb 1F11 (1 μg/ml), followed by Cy3-conjugated goat anti-mouse IgG. Nuclei were stained with Hoechst, a DNA-specific dye. Salivary glands harvested from uninfected mosquitoes served as a negative control. Analysis was performed by confocal microscopy. (B) Expression of NS1 in the salivary glands of DENV-infected mosquitoes was analyzed by Western blotting. Fifty-fold concentrated supernatants from DENV-infected C6/36 cells (DENV sup) and the salivary glands harvested from uninfected mosquitoes (Mock) served as positive and negative controls, respectively. (C and D) At 14 d after initial challenge with DENV, a total of 600–1200 mosquitoes was fed with a second noninfectious blood meal, the presence of DENV and NS1 in the remaining blood was determined by RT-PCR (C), and Western blotting was performed with DENV NS1–specific mAb 1F11 (D) and NS1-ELISA (E), respectively. Error bars indicate SD corresponding to three independent experiments. Asterisks denote the means that are statistically different among indicated groups (***p < 0.001).

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FIGURE 7.

Model of complement antagonism by DENV NS1. Together with DENV virions, soluble NS1 is released from DENV-infected insect or mammalian cells. Attenuation of the classical and lectin pathways of complement activation in tissue is promoted by three mechanisms, as follows: 1) NS1 binds proC1s and C4, forming a tripartite complex promoting the cleavage of C4 to C4b, which is rapidly inactivated by hydrolysis in the fluid phase (C4 degradation), thereby limiting the supply of native C4 (24). 2) NS1 binds and recruits C4BP to the cell surface to restrict the classical and lectin pathway C3 and C5 convertases via the cofactor activity of C4BP on cells (25). 3) NS1 competitively binds MBL and prevents the recognition of DENV by MBL, thereby protecting the virus from MBL-mediated neutralization. Overall, NS1 possesses complement evasion functions and protects DENV and DENV-infected cells from complement activation and inhibition.

FIGURE 7.

Model of complement antagonism by DENV NS1. Together with DENV virions, soluble NS1 is released from DENV-infected insect or mammalian cells. Attenuation of the classical and lectin pathways of complement activation in tissue is promoted by three mechanisms, as follows: 1) NS1 binds proC1s and C4, forming a tripartite complex promoting the cleavage of C4 to C4b, which is rapidly inactivated by hydrolysis in the fluid phase (C4 degradation), thereby limiting the supply of native C4 (24). 2) NS1 binds and recruits C4BP to the cell surface to restrict the classical and lectin pathway C3 and C5 convertases via the cofactor activity of C4BP on cells (25). 3) NS1 competitively binds MBL and prevents the recognition of DENV by MBL, thereby protecting the virus from MBL-mediated neutralization. Overall, NS1 possesses complement evasion functions and protects DENV and DENV-infected cells from complement activation and inhibition.

Close modal

It has been reported previously that NS1 is secreted from DENV-infected mammalian cells, but not from cells of insect origin (4, 18). The claim of detectable soluble NS1 in the culture medium of DENV-infected mosquito cells has been controversial, as it could reflect the liberation of intracellular NS1 from dying cells as opposed to an active cellular secretory process (21). Our data provide the following supportive evidence that NS1 is secreted from infected insect cells: 1) tunicamycin treatment affected extracellular NS1 and virion release, but not levels of NS1 protein expression within infected insect cells; 2) extracellular NS1 derived from infected insect cells appeared to form higher order oligomers, most likely hexameric in nature, unlike cell-associated NS1, which exhibits different characteristics under native conditions (12); and 3) soluble insect cell–derived NS1 possessed functional characteristics similar to mammalian cell-derived NS1, as it bound to GAGs on cell surfaces and inhibited complement activation. We also observed a novel complement antagonism function of NS1 secreted from both mammalian and insect cells as it targets MBL, the major recognition receptor of the lectin pathway of complement activation. Importantly, we showed that soluble NS1 was released together with DENV virions in the context of mosquito blood feeding.

Although NS1 was released from DENV-infected insect cells, concentrations of soluble NS1 in culture media were lower (up to a 10-fold difference) than those observed in infected mammalian cell cultures. The disparity between the two cell types could be attributed to different glycosylation machinery, which affects NS1 processing and secretion efficiency (34). Insect cells lack glycosyltransferases that are needed for synthesis of hybrid and complex-type glycans (40); DENV NS1 produced in insect cells had polymannose-type glycans at both N130 and N207 positions, whereas N-linked glycosylation at N130 is further processed to complex-type glycans in mammalian cells (39, 49). In support of the lower levels of NS1 in the supernatants from insect cells, loss of complex-type glycans at N130 results in a decrease in secretion of soluble NS1 (18, 50). Additionally, low levels of NS1 detected in the culture medium of infected insect cells could result from instability of NS1 hexamers, resulting in protein aggregation, which we observed when NS1 was subjected to density gradient fractionation and a protein stability test. These results are consistent with a study in which mutation of Asn130 resulted in a loss of hexameric NS1 and an increase in the formation of higher order NS1 oligomers (34). Indeed, our data agree with recent studies showing that NS1 secreted from DENV-infected C6/36 cells is hexameric in nature (51).

Compared with mammalian cell–derived NS1, soluble NS1 derived from insect cells bound comparably to the plasma membrane via interactions with sulfated GAGs such as heparan sulfate, despite lacking a complex-type glycan at position Asn130 (16). This is consistent with our previous observation that the N-linked glycan at position Asn207, but not at Asn130, was required for cell surface attachment of NS1 (34). NS1 binding back to the cell surface could have an important role in immune evasion through interaction with the plasma complement regulator C4BP (25). Analogous to mammalian cell–derived NS1, recruitment of C4BP to the cell surface by insect cell–derived soluble NS1 attenuated classical and lectin pathway activation through C4BP’s cofactor activity, which resulted in C4b degradation by factor I. Insect cell–derived NS1 also interacted with other complement components, including C4 and C1s/ProC1s. This could facilitate C4 degradation and protect DENV from C4-mediated neutralization in solution similar to what has been previously described for soluble NS1 from mammalian cells (24).

It has been suggested that the complement system has dual roles in pathogenesis and protection against DENV infection depending on the type of immune response (primary versus secondary infection), disease period (early versus critical phase), and host genetic factors (6, 17, 25). The lectin pathway of complement activation as triggered by the direct interaction of DENV and MBL has been shown to neutralize all four DENV serotypes and thus may control the spread of DENV within a host, especially during a primary infection (28). We described a novel interaction between soluble DENV NS1 and human MBL. NS1 competitively bound to MBL, which decreased DENV recognition by MBL and protected the virus from MBL-mediated neutralization. Mechanistically, without a requirement for further complement activation, MBL directly bound DENV and prevented DENV attachment to target cells. Soluble NS1 competitively inhibited MBL binding, and thus allowed the virus to bind, enter, and replicate within susceptible host cells. Consistent with this, binding of MBL to surface glycoproteins of influenza A virus (52), hepatitis C virus (53), and HIV (54) blocked virus attachment to target cells in a complement activation–independent manner. In WNV infection, however, MBL-mediated neutralization occurs by blocking viral fusion, not cellular attachment (30). Nevertheless, independent interference of MBL with DENV fusion could not be ruled out.

The finding that DENV-infected insect cells could secrete soluble hexameric NS1 that retains complement-inhibitory activity prompted us to explore its biological relevance. Detection of soluble NS1 and DENV in a blood meal of DENV-infected A. aegypti mosquitoes implies that the mosquito saliva most likely contains both soluble NS1 and infectious DENV virions, which could be released simultaneously into the skin and possibly blood during feeding. Complement antagonism functions of soluble NS1 (both insect cell and mammalian cell derived) could protect DENV from complement-mediated neutralization, thereby facilitating viral spread either at the earliest stages of infection (during mosquito feeding) or during subsequent replication cycles of DENV in a human host (Fig. 7). First, soluble NS1 forms a tripartite complex with C4 and C1s/C1s proenzyme, which results in C4 degradation and decreases complement activation (24) (pathway 1, Fig. 7). Second, DENV NS1 binds to C4BP, the major inhibitor of the classical/lectin pathway of complement activation in plasma, to control the activation of the classical and lectin pathways on cell surfaces (25) (pathway 2, Fig. 7). Third, a novel interaction between DENV NS1 and human MBL described in this study results in the protection of DENV from MBL-mediated neutralization (pathway 3, Fig. 7). However, further studies are required to define sites on the NS1 molecule that interact with complement components and to determine which interactions play more significant roles for DENV evasion in vivo.

NS1 immunization has been demonstrated to have a protective effect against a DENV challenge in animals (reviewed in Ref. 5). Mechanisms of protection by nonneutralizing anti-NS1 Abs have been suggested to involve complement-mediated lysis of infected cells (55, 56). It is also possible that NS1-specific Abs blocking the interaction of NS1 with complement components such as C1s, C4BP, and MBL could afford protection. Epitopes on NS1 that confer protection could serve as a basis for future NS1-based vaccine development that circumvents the undesired risk of enhancing Abs against the prM and E structural proteins.

We thank all staff members at the Department of Entomology, Armed Forces Research Institute of Medical Sciences, for advice on the mosquito experiments. We thank Kasima Wasuworawong for help with SDS-PAGE analyses. We also thank Dr. Wichit Suthammarak at the Department of Biochemistry, Faculty of Medicine Siriraj Hospital, Mahidol University, for providing materials and advice on native-PAGE analysis and Lee Greenberger (Enzon) for providing the purified human MBL protein.

This work was supported by Faculty of Medicine Siriraj Hospital, Mahidol University Grant R015633003, Thailand Research Fund RSA 5680049 (to P.A.), and National Institutes of Health Grant R01 AI077955 (to M.S.D.). P.A. has been supported by a Siriraj Chalermprakiat Grant and a Research Lecturer Grant from the Faculty of Medicine, Siriraj Hospital, Mahidol University. S.T. is a Ph.D. scholar in the Royal Golden Jubilee Ph.D. Program (PHD/0101/2554).

Abbreviations used in this article:

BHK

baby hamster kidney fibroblast

DENV

dengue virus

Endo H

endoglycosidase H

FFA

focus-forming assay

GAG

glycosaminoglycan

GVB2+

gelatin veronal buffer supplemented with Mg2+ and Ca2+

MBL

mannose-binding lectin

MOI

multiplicity of infection

NS

nonstructural

PNGase F

peptide N-glycosidase F

proC1s

C1s proenzyme

WNV

West Nile virus.

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The authors have no financial conflicts of interest.