Temperature-dependent folding allows stable dimerization of secretory and virus-associated E proteins of Dengue and Zika viruses in mammalian cells

Slon-Campos, J; Marchese, S.; Rana, Jyoti; Mossenta, Monica; Poggianella, Monica; Bestagno, Marco; Burrone, Óscar R.

doi:10.1038/s41598-017-01097-5

Cited by 37 publications

(52 citation statements)

References 66 publications

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“…The tip of DII (Y' site), a conserved region among flavivirus genus such as West Nile virus, Japan encephalitis virus, Yellow fever virus, or Zika virus that immerses into the lipid bilayer of host endosomal membrane, has been suggested as the binding site for flavonoids, possibly interfering with the viral attachment and fusion [42,57,58]. In addition, the region between DI and DIII (X' and Y' sites), a promising target for vaccine development [59,60], was also used for drug discovery [50,54]. From an in vitro and in silico study [54], a flavanone derivative (5-hydroxy-7-methoxy-6-methylflavanone, FN5Y) has been shown to interrupt the progress of the disease at the early stage of infection, targeted at E protein at the four sites ( Figure 1).…”

Section: Introductionmentioning

confidence: 99%

Multiple Virtual Screening Strategies for the Discovery of Novel Compounds Active Against Dengue Virus: A Hit Identification Study

et al. 2019

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Dengue infection is caused by a mosquito-borne virus, particularly in children, which may even cause death. No effective prevention or therapeutic agents to cure this disease are available up to now. The dengue viral envelope (E) protein was discovered to be a promising target for inhibition in several steps of viral infection. Structure-based virtual screening has become an important technique to identify first hits in a drug screening process, as it is possible to reduce the number of compounds to be assayed, allowing to save resources. In the present study, pharmacophore models were generated using the common hits approach (CHA), starting from trajectories obtained from molecular dynamics (MD) simulations of the E protein complexed with the active inhibitor, flavanone (FN5Y). Subsequently, compounds presented in various drug databases were screened using the LigandScout 4.2 program. The obtained hits were analyzed in more detail by molecular docking, followed by extensive MD simulations of the complexes. The highest-ranked compound from this procedure was then synthesized and tested on its inhibitory efficiency by experimental assays.

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Section: Introductionmentioning

confidence: 99%

Multiple Virtual Screening Strategies for the Discovery of Novel Compounds Active Against Dengue Virus: A Hit Identification Study

et al. 2019

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“…Here, to investigate if ZIKV rE dimers are better subunit vaccine antigens than monomers, we expressed ZIKV rE variants (aa1-402) that are monomers (rE M ) or stable dimers (rE D ) under physiological conditions. We generated stable ZIKV rE D proteins as previously described for DENV E protein by introducing a disulfide bridge (A264C) in the E-domain II interactive region of the homodimer 9,10 ( Fig.1A ). The oligomeric state of the purified rE M and rE D proteins were confirmed by protein gel electrophoresis ( Fig.1B ).…”

Section: Resultsmentioning

confidence: 99%

Oligomeric state of the ZIKV E protein defines protective immune responses

Metz

Thomas

Brackbill

et al. 2019

Preprint

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8The current leading Zika vaccine candidates in clinical testing are based on live or killed virus 9 platforms, which have safety issues, especially in pregnant women. Zika subunit vaccines, 10 however, have shown poor performance in preclinical studies. We hypothesized that Zika 11Envelope (E) protein subunit vaccines have performed poorly because the antigens tested have 12been recombinant E monomers that do not display critical quaternary structure epitopes present 13on Zika E protein homodimers that cover the surface of the virus. To test this hypothesis, we 14 engineered and produced stable recombinant E protein homodimers. Unlike the E monomer, the 15 dimer was recognized by strongly neutralizing monoclonal antibodies isolated from Zika-immune 16 individuals. In a mouse model of vaccination, the dimeric antigen stimulated strongly neutralizing 17 antibodies that targeted epitopes that were similar to epitopes recognized by human antibodies 18 following natural Zika virus infection. In contrast, the monomer antigen stimulated lower levels of 19 neutralizing antibodies directed to simple epitopes on domain III of E protein. In a mouse model 20 of ZIKV challenge, only E dimer antigen stimulated protective antibodies, not the 21 monomer. These results highlight the importance of mimicking the highly structured flavivirus 22 surface when designing subunit vaccines. The flavivirus field has a long history of using E 23 monomers as vaccine antigens with limited success. These results are applicable to developing 24 second generation subunit vaccines against Zika as well as other medically important flaviviruses 25 such as dengue and yellow fever viruses. 26 130 Figure 3: ZIKV rE D stimulates antibodies that target complex epitopes on the virion. A) Method for 131 depleting EDIII binding antibodies from mouse immune sera. Recombinant ZIKV EDIII (His-tagged) was 132 coupled to nickel beads i then incubated with immune sera ii . Magnetic pull down removes nickel beads and 133 EDIII binding antibodies iii , leaving leavind sera depleted from EDIII binding antibodies iv . B) The level of 134 EDIII-binding antibodies in the serum of mice immunized with the indicated antigens is shown as a 135 percentage of the total level of ZIKV specific IgG, as measured by ELISA of EDIII-depleted and control-136 depleted serum. C) The neutralizing activity of EDIII-depleted and undepleted sera was determined and 137 expressed as the dilution at which 50% of the virus was neutralized (Neut50). D) A blockade of binding 138 (BOB) assay was used to evaluate if mice immunized with rE M or rE D developed antibodies that blocked 139 the binding of A9E, G9E and EDE C10 human mAbs. Data points represent individual mice. Statistical140differences were determined by one-way ANOVA followed by a Tukey's test (p<0.05).

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“…E-homodimer stability was proved several times to be affected by temperature: dimerization is favoured at 28˚C and reduced at 37°C, hence physiological temperature is another element that contributes to impair dimers exposure to the immune system (39). But 28˚C is also a crucial temperature for expression and secretion of E protein, both in the soluble form but also as part of VLPs (28). Since this temperature is not compatible with genetic vaccination approaches, in which DNA or RNA encoding the antigen is administered and the antigen is then produced by the host cells at physiological temperature, the full potential of our antigens as candidate vaccines was evaluated in a protein-based vaccination approach.…”

Section: Discussionmentioning

confidence: 99%

“…In order to further characterise the types of antibodies elicited by our cvD antigens, we used a recently developed cytofluorimetry assay of cells displaying dimers of ZIKV sE protein (paper in submission). In this assay, the C-terminus of sE is fused to the transmembrane and cytosolic tail of the type-I trans-membrane protein MHC-Iα for plasma membrane display of the protein, as previously reported (28). This assay has the potential to discriminate antibodies binding exclusively to dimeric E on the basis of the pH-dependent mobility of E protein: at pH7, that resembles the neutral extracellular environment, the protein is in a dimeric conformation but at pH6, mimicking the conformational changes that occur in the acidic endosome vesicles during infection, it moves to a pre-fusion monomeric conformation.…”

Section: Design Expression and Purification Of E Covalent Dimer-basementioning

confidence: 99%

Zika virus-like particles bearing covalent dimer of envelope protein protect mice from lethal challenge

Lorenzo

Tandavanitj

Doig

et al. 2020

Preprint

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Zika virus (ZIKV) envelope (E) protein is the major target of neutralizing antibodies in infected host, and thus represents a candidate of interest for vaccine design. However, a major concern in the development of vaccines against ZIKV and the related dengue virus is the induction of cross-reactive poorly neutralizing antibodies that can cause antibody-dependent enhancement (ADE) of infection. This risk necessitates particular care in vaccine design. Specifically, the engineered immunogens should have their cross-reactive epitopes masked, and they should be optimized for eliciting virus-specific strongly neutralizing antibodies upon vaccination. Here, we developed ZIKV subunit- and virus-like particle (VLP)-based vaccines displaying E in its wild type form, or E locked in a covalently linked dimeric (cvD) conformation to enhance the exposure of E dimers to the immune system. Compared with their wild-type derivatives, cvD immunogens elicited antibody with higher capacity of neutralizing virus infection of cultured cells. More importantly, these immunogens protected animals from lethal challenge with both the African and Asian lineages of ZIKV, impairing virus dissemination to brain and sexual organs. Moreover, the locked conformation of E reduced the exposure of epitopes recognized by cross-reactive antibodies and therefore showed a lower potential to induce ADE in vitro. Our data demonstrated a higher efficacy of the VLPs in comparison with the soluble dimer and support VLP-cvD as a promising ZIKV vaccine.

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Temperature-dependent folding allows stable dimerization of secretory and virus-associated E proteins of Dengue and Zika viruses in mammalian cells

Cited by 37 publications

References 66 publications

Multiple Virtual Screening Strategies for the Discovery of Novel Compounds Active Against Dengue Virus: A Hit Identification Study

Multiple Virtual Screening Strategies for the Discovery of Novel Compounds Active Against Dengue Virus: A Hit Identification Study

Oligomeric state of the ZIKV E protein defines protective immune responses

Zika virus-like particles bearing covalent dimer of envelope protein protect mice from lethal challenge

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