Plant‐made E2 glycoprotein single‐dose vaccine protects pigs against classical swine fever

Laughlin, Richard; Madera, Rachel; Peres, Yair; Berquist, Brian R.; Wang, Lihua; Buist, Sterling; Burakova, Yulia; Palle, Sreenath; Chung, Chungwon J.; Rasmussen, Max V.; Martel, Erica; Brake, David A.; Neilan, John G.; Lawhon, Sara D.; Adams, L. Garry; Shi, Jishu; Marcel, Sylvain

doi:10.1111/pbi.12986

Cited by 31 publications

(38 citation statements)

References 43 publications

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“…The expected size of the E2 recombinant protein is 64 kD; therefore, the strong band appeared to be larger than expected. We assume that this is due to N-glycosylation since E2 protein has putative 7 N-glycosylation sites (Laughlin et al 2019). Consistent with this, previous studies reported that CBD-fused E2 recombinant proteins have several N-glycosylation sites and are larger than expected when expressed in plants (Park et al 2019;Sohn et al 2018).…”

Section: Generation Of the Pme2:pfc2 Fusion Construct And Protein Expsupporting

confidence: 82%

“…In addition, Arabidopsis thaliana-derived E2 antibodies in a mouse can recognize the native E2 protein suggesting that structure of plant-produced E2 is comparable to native E2 protein (Sohn et al 2018). In addition, transient expression of recombinant E2 protein from the leaves of Nicotiana benthamiana or from the leaves of transgenic N. benthamiana lines generates antibodies that can neutralize CSFV in pigs and protect them against subsequent challenge with CSFV (Laughlin et al 2019;Park et al 2019).…”

Section: Introductionmentioning

confidence: 99%

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A classical swine fever virus E2 fusion protein produced in plants elicits a neutralizing humoral immune response in mice and pigs

et al. 2020

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Classical swine fever (CSF) is one of the most important viral diseases of swine worldwide. Although live or attenuated virus vaccines have been used to control CSFV, it is difficult to distinguish vaccinated pigs from infected pigs; this leads to restrictions on import and export. Subunit vaccines based on the CSFV E2 glycoprotein have been developed using baculovirus or insect cell systems, but some weaknesses remain. Here, we describe production of an E2 recombinant protein using a Nicotiana benthamiana plant expression system. To do this, we took advantage of the ability of the swine Fc domain to increase solubility and stability of the fusion protein and to strengthen immune responses in target animals. N. benthamiana expressed high amounts of pFc2-fused E2 proteins, which were isolated and purified by affinity chromatography to yield a high pure recombinant protein in a cost-effective manner. Native-polyacrylamide gel electrophoresis and size exclusion chromatography confirmed that the pmE2:pFc2 fusion exists as a multimer rather than as a dimer. Injection of recombinant pmE2 protein into mice or piglets generated anti-pmE2 antibodies with efficient neutralizing activity against CSFV. These results suggest that a purified recombinant E2 protein produced in N. benthamiana generates high titers of neutralizing antibodies in vivo; as such, the protein could be developed as a subunit vaccine against CSFV. Keywords Nicotiana benthamiana Á Classical swine fever virus Á DIVA concept Á Subunit vaccine Á Molecular farming Á Fc-fusion protein Abbreviations CSFV Classical swine fever virus DIVA Differentiating infected from vaccinated animals ER Endoplasmic reticulum CBD Cellulose-binding domain BSA Bovine serum albumin MLV Modified live vaccines PCR Polymerase chain reaction Electronic supplementary material The online version of this article (

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Section: Generation Of the Pme2:pfc2 Fusion Construct And Protein Expsupporting

confidence: 82%

Section: Introductionmentioning

confidence: 99%

A classical swine fever virus E2 fusion protein produced in plants elicits a neutralizing humoral immune response in mice and pigs

et al. 2020

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“…The authors suggested that as cELISA proved to be nearly as sensitive and specific as the VNT while being simpler and more rapid, it would be an adequate screening test for CDV or PDV cases [23]. The glycoprotein E2 exposed on the outer surface of CSFV is the major immuno-protective antigen of C-strain vaccine that is responsible for inducing neutralizing antibodies and eliciting protective immunity against CSFV [13][14][15][16][17][18][19][20]. Thus, it is not surprising that E2 protein has been successfully used to develop ELISAs to measure anti-CSFV antibody response in pigs after vaccination [13][14][15][16].…”

Section: Discussionmentioning

confidence: 99%

“…Virus neutralization test (VNT) is considered as the gold standard for serological monitoring and efficacy evaluation of CSF vaccines. However, it has several limitations including time-consuming, requirement of cell culture, the need for live virus manipulation, and relatively expensive [2,[18][19][20][21]. Here, we described a competitive ELISA (cELISA) developed with a neutralizing anti-E2 monoclonal antibody.…”

Section: Introductionmentioning

confidence: 99%

A neutralizing monoclonal antibody-based competitive ELISA for classical swine fever C-strain post–vaccination monitoring

Wang

Madera

et al. 2020

BMC Vet Res

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Background: Virus neutralization test (VNT) is widely used for serological survey of classical swine fever (CSF) and efficacy evaluation of CSF vaccines. However, VNT is a time consuming procedure that requires cell culture and live virus manipulation. C-strain CSF vaccine is the most frequently used vaccine for CSF control and prevention. In this study, we presented a neutralizing monoclonal antibody (mAb) based competitive enzyme-linked immunosorbent assay (cELISA) with the emphasis on the replacement of VNT for C-strain post-vaccination monitoring. Results: One monoclonal antibody (6B211) which has potent neutralizing activity against C-strain was generated. A novel cELISA was established and optimized based on the strategy that 6B211 can compete with C-strain induced neutralizing antibodies in pig serum to bind capture antigen C-strain E2. By testing C-strain VNT negative pig sera (n = 445) and C-strain VNT positive pig sera (n = 70), the 6B211 based cELISA showed 100% sensitivity (95% confidence interval: 94.87 to 100%) and 100% specificity (95% confidence interval: 100 to 100%). The C-strain antibody can be tested in pigs as early as 7 days post vaccination with the cELISA. By testing pig sera (n = 139) in parallel, the cELISA showed excellent agreement (Kappa = 0.957) with VNT. The inhibition rate of serum samples in the cELISA is highly correlated with their titers in VNT (r 2 = 0.903, p < 0.001). In addition, intra-and inter-assays of the cELISA exhibited acceptable repeatability with low coefficient of variations (CVs). Conclusions: This novel cELISA demonstrated excellent agreement and high level correlation with VNT. It is a reliable tool for sero-monitoring of C-strain vaccination campaign because it is a rapid, simple, safe and cost effective assay that can be used to monitor vaccination-induced immune response at the population level.

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“…In this study, we developed a neutralizing mAb based cELISA with the emphasis on the replacement of and specific as the VNT while being simpler and more rapid, it would be an adequate screening test for CDV or PDV cases [23]. The glycoprotein E2 exposed on the outer surface of CSFV is the major immuno-protective antigen of C-strain vaccine that is responsible for inducing neutralizing antibodies and eliciting protective immunity against CSFV [13][14][15][16][17][18][19][20]. Thus, it is not surprising that E2 protein has been successfully used to develop ELISAs to measure anti-CSFV antibody response in pigs after vaccination [13][14][15][16].…”

Section: Discussionmentioning

confidence: 99%

A neutralizing monoclonal antibody-based competitive ELISA for classical swine fever C-strain post–vaccination monitoring

Wang

Madera

et al. 2020

Preprint

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Background: Virus neutralization test (VNT) is widely used for serological survey of classical swine fever (CSF) and efficacy evaluation of CSF vaccines. However, VNT is a time consuming procedure that requires cell culture and live virus manipulation. C-strain CSF vaccine is the most frequently used vaccine for CSF control and prevention. In this study, we presented a neutralizing monoclonal antibody (mAb) based competitive enzyme-linked immunosorbent assay (cELISA) with the emphasis on the replacement of VNT for C-strain post–vaccination monitoring. Results: One monoclonal antibody (6B211) which has potent neutralizing activity against C-strain was generated. A novel cELISA was established and optimized based on the strategy that 6B211 can compete with C-strain induced neutralizing antibodies in pig serum to bind capture antigen C-strain E2. By testing C-strain VNT negative pig sera (n=445) and C-strain VNT positive pig sera (n=70), the 6B211 based cELSIA showed 100% sensitivity (95% confidence interval: 94.87 to 100%) and 100% specificity (95% confidence interval: 100 to 100%). The C-strain antibody can be detected in pigs as early as 7 days post vaccination with the cELISA. By testing pig sera (n=139) in parallel, the cELISA showed excellent agreement (Kappa=0.957) with VNT. The inhibition rate of serum samples in the cELISA is highly correlated with their titers in VNT (r 2 =0.903, p<0.001). In addition, intra- and inter-assays of the cELISA exhibited acceptable repeatability with low coefficient of variations (CVs). Conclusions: This novel cELISA demonstrated excellent agreement and high level correlation with VNT. It is a reliable tool for sero-monitoring of C-strain vaccination campaign because it is a rapid, simple, safe and cost effective assay that can be used to monitor vaccination-induced immune response at the population level.

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Plant‐made E2 glycoprotein single‐dose vaccine protects pigs against classical swine fever

Cited by 31 publications

References 43 publications

A classical swine fever virus E2 fusion protein produced in plants elicits a neutralizing humoral immune response in mice and pigs

A classical swine fever virus E2 fusion protein produced in plants elicits a neutralizing humoral immune response in mice and pigs

A neutralizing monoclonal antibody-based competitive ELISA for classical swine fever C-strain post–vaccination monitoring

A neutralizing monoclonal antibody-based competitive ELISA for classical swine fever C-strain post–vaccination monitoring

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