Mutation analysis of the cross-reactive epitopes of Japanese encephalitis virus envelope glycoprotein

Chiou, Shyan Song; Fan, Yao-Chung; Crill, Wayne D.; Chang, Ruey Yi; Chang, Gwong Jen J.

doi:10.1099/vir.0.040238-0

Cited by 37 publications

(39 citation statements)

References 38 publications

(71 reference statements)

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“…or of the different forms of virus (mature, immature, or partially mature) being delivered. Nevertheless, VLPs produced by our flavivirus and DENV plasmids in tissue culture do contain prM and vaccination with these plasmids can produce antibody recognizing prM (Chang et al, 2003; Chiou et al, 2012). CRR substitutions introduced into these plasmids do not alter the prM processing or change the relative ratios of VLP prM and E or their induced antibody populations in comparison to WT (Chiou et al, 2012).…”

Section: Discussionmentioning

confidence: 99%

“…Nevertheless, VLPs produced by our flavivirus and DENV plasmids in tissue culture do contain prM and vaccination with these plasmids can produce antibody recognizing prM (Chang et al, 2003; Chiou et al, 2012). CRR substitutions introduced into these plasmids do not alter the prM processing or change the relative ratios of VLP prM and E or their induced antibody populations in comparison to WT (Chiou et al, 2012). Thus, prM antibodies may be of concern in human vaccination and they could explain the residual enhancement observed in CRR vaccinated AG129 mice (Henchal et al, 1985; Roehrig et al, 1998), but they are unlikely to account for the differences in pathology and mortality between pVD1-CRR and -WT immunized mice in this study.…”

Section: Discussionmentioning

confidence: 99%

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Sculpting humoral immunity through dengue vaccination to enhance protective immunity

Crill¹,

Hughes²,

Trainor³

et al. 2012

Front. Immun.

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Dengue viruses (DENV) are the most important mosquito transmitted viral pathogens infecting humans. DENV infection produces a spectrum of disease, most commonly causing a self-limiting flu-like illness known as dengue fever; yet with increased frequency, manifesting as life-threatening dengue hemorrhagic fever (DHF). Waning cross-protective immunity from any of the four dengue serotypes may enhance subsequent infection with another heterologous serotype to increase the probability of DHF. Decades of effort to develop dengue vaccines are reaching the finishing line with multiple candidates in clinical trials. Nevertheless, concerns remain that imbalanced immunity, due to the prolonged prime-boost schedules currently used in clinical trials, could leave some vaccinees temporarily unprotected or with increased susceptibility to enhanced disease. Here we develop a DENV serotype 1 (DENV-1) DNA vaccine with the immunodominant cross-reactive B cell epitopes associated with immune enhancement removed. We compare wild-type (WT) with this cross-reactivity reduced (CRR) vaccine and demonstrate that both vaccines are equally protective against lethal homologous DENV-1 challenge. Under conditions mimicking natural exposure prior to acquiring protective immunity, WT vaccinated mice enhanced a normally sub-lethal heterologous DENV-2 infection resulting in DHF-like disease and 95% mortality in AG129 mice. However, CRR vaccinated mice exhibited redirected serotype-specific and protective immunity, and significantly reduced morbidity and mortality not differing from naїve mice. Thus, we demonstrate in an in vivo DENV disease model, that non-protective vaccine-induced immunity can prime vaccinees for enhanced DHF-like disease and that CRR DNA immunization significantly reduces this potential vaccine safety concern. The sculpting of immune memory by the modified vaccine and resulting redirection of humoral immunity provide insight into DENV vaccine-induced immune responses.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Sculpting humoral immunity through dengue vaccination to enhance protective immunity

Crill¹,

Hughes²,

Trainor³

et al. 2012

Front. Immun.

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“…Most of the antibodies elicited by JEV infection or immunization are conformation-dependent and, for the most part, recognize the viral E protein and are able to help prevent virus infection [15,53]. Formalin inactivation of several human vaccines has been shown to result in antigenic alteration to the viral particles, which can be measured by the binding activity of specific MAbs [38,40], but the effect of formalin inactivation on commercially available JEV vaccines has not been evaluated.…”

Section: Mab Binding Activity Of Ficvmentioning

confidence: 99%

“…Formalin inactivation of several human vaccines has been shown to result in antigenic alteration to the viral particles, which can be measured by the binding activity of specific MAbs [38,40], but the effect of formalin inactivation on commercially available JEV vaccines has not been evaluated. Previously, an established Ag-ELISA protocol was successfully used to determine the antigenic structure of JEV using a panel of anti-E protein MAbs [49,53].…”

Section: Mab Binding Activity Of Ficvmentioning

confidence: 99%

Formalin Inactivation of Japanese Encephalitis Virus Vaccine Alters the Antigenicity and Immunogenicity of a Neutralization Epitope in Envelope Protein Domain III

et al. 2015

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Formalin-inactivated Japanese encephalitis virus (JEV) vaccines are widely available, but the effects of formalin inactivation on the antigenic structure of JEV and the profile of antibodies elicited after vaccination are not well understood. We used a panel of monoclonal antibodies (MAbs) to map the antigenic structure of live JEV virus, untreated control virus (UCV), formalin-inactivated commercial vaccine (FICV), and formalin-inactivated virus (FIV). The binding activity of T16 MAb against Nakayama-derived FICV and several strains of FIV was significantly lower compared to live virus and UCV. T16 MAb, a weakly neutralizing JEV serocomplex antibody, was found to inhibit JEV infection at the post-attachment step. The T16 epitope was mapped to amino acids 329, 331, and 389 within domain III (EDIII) of the envelope (E) glycoprotein. When we explored the effect of formalin inactivation on the immunogenicity of JEV, we found that Nakayama-derived FICV, FIV, and UCV all exhibited similar immunogenicity in a mouse model, inducing anti-JEV and anti-EDII 101/106/107 epitope-specific antibodies. However, the EDIII 329/331/389 epitope-specific IgG antibody and neutralizing antibody titers were significantly lower for FICV-immunized and FIV-immunized mouse serum than for UCV-immunized. Formalin inactivation seems to alter the antigenic structure of the E protein, which may reduce the potency of commercially available JEV vaccines. Virus inactivation by H2O2, but not by UV or by short-duration and higher temperature formalin treatment, is able to maintain the antigenic structure of the JEV E protein. Thus, an alternative inactivation method, such as H2O2, which is able to maintain the integrity of the E protein may be essential to improving the potency of inactivated JEV vaccines.

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“…The antigenic drifts of an antigen permit it to calmly escape the human memory cells response. Similarly, allergenicity in vaccine development is also a calling obstacle (Chiou, Fan, Crill, Chang, & Chang, ). Because most of the vaccines, instead of provoking immunity against an antigen, they cause allergic reaction by the initiation of helper T and type 2 cells along with immunoglobulin E. Thus, we confirmed both the antigenic and allergenic nature of the proposed peptides, and at this point, it is claimed that these peptides are safe to be tested and will not cause any response that is unintentional.…”

Section: Discussionmentioning

confidence: 99%

Prediction and validation of potent peptides against herpes simplex virus type 1 via immunoinformatic and systems biology approach

2019

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The human herpes simplex virus type 1 (HSV‐1) is an extremely rampant human pathogen, and its infection could cause life‐long diseases, including the central nervous system disorders. The glycoproteins of HSV‐1 such as glycoprotein B, glycoprotein C, glycoprotein D, glycoprotein H, and glycoprotein L are highly involved in mediating the viral attachment and infection of the host cell. Therefore, immunoinformatic approaches followed by molecular dynamics simulation and systems biology has been used to analyze these glycoproteins in order to propose effective peptide‐based vaccine candidates against the HSV‐1 infection. The ElliPro and NetCTL.1.2 online tools were employed to forecast the B‐ and T‐lymphocyte (CTL) epitopes for gB, gC, gD, gH, and gL. The 3D coordinates of these epitopes were modeled and docked against the human major histocompatibility complex molecule‐1. The outcomes obtained from postdocking analysis along with TAP (Transporter associated with antigen processing), MHC binding, and C‐terminal cleavage score assisted in the selection of potential epitopes. These epitopes were further subjected to molecular dynamics simulation and systems biology approach which showed significant results. On the basis of these substantial outcomes, peptides are proposed that could be used to provoke immunity against the HSV‐1 infection.

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Mutation analysis of the cross-reactive epitopes of Japanese encephalitis virus envelope glycoprotein

Cited by 37 publications

References 38 publications

Sculpting humoral immunity through dengue vaccination to enhance protective immunity

Sculpting humoral immunity through dengue vaccination to enhance protective immunity

Formalin Inactivation of Japanese Encephalitis Virus Vaccine Alters the Antigenicity and Immunogenicity of a Neutralization Epitope in Envelope Protein Domain III

Prediction and validation of potent peptides against herpes simplex virus type 1 via immunoinformatic and systems biology approach

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