2019
DOI: 10.3389/fpls.2019.00455
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Epitope Presentation of Dengue Viral Envelope Glycoprotein Domain III on Hepatitis B Core Protein Virus-Like Particles Produced in Nicotiana benthamiana

Abstract: Dengue fever is currently ranked as the top emerging tropical disease, driven by increased global travel, urbanization, and poor hygiene conditions as well as global warming effects which facilitate the spread of Aedes mosquitoes beyond their current distribution. Today, more than 100 countries are affected most of which are tropical Asian and Latin American nations with limited access to medical care. Hence, the development of a dengue vaccine that is dually cost-effective and able to c… Show more

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Cited by 25 publications
(21 citation statements)
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“…The chimeric particle diameter ranged from 28 to 38 nm, and the surface appeared to be rather “knobbly” ( Figure 5 , panel b). The “knobbly” surface morphology is expected for HBcAg core particles displaying a heterologous sequence on their surface [ 34 , 42 ]. This indicates that HEV ORF2 551–607 aa were presented on the surface of HBcAg spikes.…”
Section: Discussionmentioning
confidence: 99%
See 1 more Smart Citation
“…The chimeric particle diameter ranged from 28 to 38 nm, and the surface appeared to be rather “knobbly” ( Figure 5 , panel b). The “knobbly” surface morphology is expected for HBcAg core particles displaying a heterologous sequence on their surface [ 34 , 42 ]. This indicates that HEV ORF2 551–607 aa were presented on the surface of HBcAg spikes.…”
Section: Discussionmentioning
confidence: 99%
“…The hepatitis B capsid protein (HBcAg) has been shown to be capable of self-assembly into VLPs when expressed in a number of eukaryotic heterologous systems including mammalian cells [ 27 ], plants [ 28 , 29 , 30 ], yeast [ 31 ], insect cells [ 32 ], and Xenopus oocytes [ 33 ]. VLPs composed of HBcAg are safe and potent vaccine delivery systems [ 34 , 35 ]. HBcAg consists of 183 amino acids with an N-terminal assembly domain (1–149 aa) and a C-terminal arginine-rich domain (34 aa) required for the packaging of nucleic acid [ 36 ].…”
Section: Introductionmentioning
confidence: 99%
“…Therefore, we compared the performance of two expression systems, i.e., the -pEAQ vector based on genetic elements of the CPMV genome, which we were unable to replicate in plant cells, and PVX-based self-replicating pEff vector. Both systems have been successfully used for the expression of a number of recombinant proteins in plants [37][38][39][40][41]. The first two-four days post infiltration of the plant leaves with pEff vector showed an accumulation of higher level of the HEV ORF2 proteins compared with pEAQ-HT vector expression of the same proteins.…”
Section: Discussionmentioning
confidence: 99%
“… Pathogen Epitope(s) Expression system Site of epitope insertion Ref. Dengue virus cEDIII N. benthamiana MIR [ 68 ] H1N1 Influenza A virus matrix protein 2 E. coli MIR [ 188 ] H7N9 Influenza long alpha-helix (LAH) E. coli MIR [ 189 ] Mycobacterium Tuberculosis (Tuberculosis) Culture filtrate protein 10 (CFP 10) E. coli MIR [ 190 ] Hepatitis B Core Antigen E. coli MIR [ 86 ] Nicotiana benthamiana GGS sequence Influenza virus M2e E. coli MIR [ 191 ] Influenza virus M2e N. benthamiana N-terminal [ 192 ] Dengue virus EDIII-2 E. coli MIR [ 193 ] Dengue virus EDIII E. coli MIR [ …”
Section: Vlp-based Vaccinesmentioning
confidence: 99%
“…After the primary study by Clarke et al in 1987 [ 65 ], different epitopes and antigens have been introduced into HBc protein for vaccine development ( Table 6 ). The immunogenic epitope of the virus was fused to the N-terminus end of the HBc sequence [ [66] , [67] , [68] , [69] ]. This VLP has been used to produce HBV vaccine in yeast [ 70 , 71 ] and mammalian cells (CHO) [ 20 ].…”
Section: Engineering Vlps As a Vaccine Platformmentioning
confidence: 99%