Preparation and Identification of a Monoclonal Antibody against the Pseudorabies Virus gE Glycoprotein through a Novel Strategy

Zhenyang Guo; Siyu Zhang; Hu Xu; Wansheng Li; Chao Li; Jing Zhao; Bangjun Gong; Qi Sun; Lirun Xiang; Hongyuan Zhao; Qian Wang; Guohui Zhou; Yandong Tang; Tongqing An; Xuehui Cai; Zhijun Tian; Hongliang Zhang; Jinmei Peng

doi:10.3390/vetsci10020133

Preparation and Identification of a Monoclonal Antibody against the Pseudorabies Virus gE Glycoprotein through a Novel Strategy

Zhenyang Guo, Siyu Zhang, Hu Xu, Wansheng Li, Chao Li, Jing Zhao, Bangjun Gong, Qi Sun, Lirun Xiang, Hongyuan Zhao, Qian Wang, Guohui Zhou, Yandong Tang, Tongqing An, Xuehui Cai, Zhijun Tian, Hongliang Zhang, Jinmei Peng

Research output: Contribution to journal › Article › peer-review

4 Scopus citations

Abstract

Since 2011, pseudorabies virus (PRV) has recurred in several vaccinated pig farms in China. PRV variants with high virulence were found to be the main cause of the outbreaks. In the face of the PRV epidemic, detection of the wild strain is as important as vaccine immunization, so we hoped to achieve differential diagnosis of PRV by obtaining a monoclonal antibody (mAB) that could be used to identify the wild strain. In this study, we used a novel immunization and screening strategy to prepare an mAB and obtained mAB 1H5 against the gE glycoprotein. An immunofluorescence assay (IFA) revealed that this mAB was specific to both classic and variant strains of PRV. Subsequently, we further identified the linear epitopes of B cells recognized using the mAB. The mAB 1H5 bound at ⁶⁷RRAG⁷⁰, which is a novel epitope and is conserved in almost all PRV strains. These findings provide novel insight into the structure and function of PRV proteins, the analysis of antigenic epitope characteristics, and the establishment of antigen or antibody detection methods.

Original language	English
Article number	133
Journal	Veterinary Sciences
Volume	10
Issue number	2
DOIs	https://doi.org/10.3390/vetsci10020133
State	Published - Feb 2023
Externally published	Yes

Keywords

PRV
epitopes
gE
monoclonal antibody

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10.3390/vetsci10020133

Cite this

Guo, Z., Zhang, S., Xu, H., Li, W., Li, C., Zhao, J., Gong, B., Sun, Q., Xiang, L., Zhao, H., Wang, Q., Zhou, G., Tang, Y., An, T., Cai, X., Tian, Z., Zhang, H., & Peng, J. (2023). Preparation and Identification of a Monoclonal Antibody against the Pseudorabies Virus gE Glycoprotein through a Novel Strategy. Veterinary Sciences, 10(2), Article 133. https://doi.org/10.3390/vetsci10020133

@article{ef56096dafcd4b35b0696abfac8cb982,

title = "Preparation and Identification of a Monoclonal Antibody against the Pseudorabies Virus gE Glycoprotein through a Novel Strategy",

abstract = "Since 2011, pseudorabies virus (PRV) has recurred in several vaccinated pig farms in China. PRV variants with high virulence were found to be the main cause of the outbreaks. In the face of the PRV epidemic, detection of the wild strain is as important as vaccine immunization, so we hoped to achieve differential diagnosis of PRV by obtaining a monoclonal antibody (mAB) that could be used to identify the wild strain. In this study, we used a novel immunization and screening strategy to prepare an mAB and obtained mAB 1H5 against the gE glycoprotein. An immunofluorescence assay (IFA) revealed that this mAB was specific to both classic and variant strains of PRV. Subsequently, we further identified the linear epitopes of B cells recognized using the mAB. The mAB 1H5 bound at 67RRAG70, which is a novel epitope and is conserved in almost all PRV strains. These findings provide novel insight into the structure and function of PRV proteins, the analysis of antigenic epitope characteristics, and the establishment of antigen or antibody detection methods.",

keywords = "PRV, epitopes, gE, monoclonal antibody",

author = "Zhenyang Guo and Siyu Zhang and Hu Xu and Wansheng Li and Chao Li and Jing Zhao and Bangjun Gong and Qi Sun and Lirun Xiang and Hongyuan Zhao and Qian Wang and Guohui Zhou and Yandong Tang and Tongqing An and Xuehui Cai and Zhijun Tian and Hongliang Zhang and Jinmei Peng",

note = "Publisher Copyright: {\textcopyright} 2023 by the authors.",

year = "2023",

month = feb,

doi = "10.3390/vetsci10020133",

language = "English",

volume = "10",

journal = "Veterinary Sciences",

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Guo, Z, Zhang, S, Xu, H, Li, W, Li, C, Zhao, J, Gong, B, Sun, Q, Xiang, L, Zhao, H, Wang, Q, Zhou, G, Tang, Y, An, T, Cai, X, Tian, Z, Zhang, H & Peng, J 2023, 'Preparation and Identification of a Monoclonal Antibody against the Pseudorabies Virus gE Glycoprotein through a Novel Strategy', Veterinary Sciences, vol. 10, no. 2, 133. https://doi.org/10.3390/vetsci10020133

TY - JOUR

T1 - Preparation and Identification of a Monoclonal Antibody against the Pseudorabies Virus gE Glycoprotein through a Novel Strategy

AU - Guo, Zhenyang

AU - Zhang, Siyu

AU - Xu, Hu

AU - Li, Wansheng

AU - Li, Chao

AU - Zhao, Jing

AU - Gong, Bangjun

AU - Sun, Qi

AU - Xiang, Lirun

AU - Zhao, Hongyuan

AU - Wang, Qian

AU - Zhou, Guohui

AU - Tang, Yandong

AU - An, Tongqing

AU - Cai, Xuehui

AU - Tian, Zhijun

AU - Zhang, Hongliang

AU - Peng, Jinmei

PY - 2023/2

Y1 - 2023/2

N2 - Since 2011, pseudorabies virus (PRV) has recurred in several vaccinated pig farms in China. PRV variants with high virulence were found to be the main cause of the outbreaks. In the face of the PRV epidemic, detection of the wild strain is as important as vaccine immunization, so we hoped to achieve differential diagnosis of PRV by obtaining a monoclonal antibody (mAB) that could be used to identify the wild strain. In this study, we used a novel immunization and screening strategy to prepare an mAB and obtained mAB 1H5 against the gE glycoprotein. An immunofluorescence assay (IFA) revealed that this mAB was specific to both classic and variant strains of PRV. Subsequently, we further identified the linear epitopes of B cells recognized using the mAB. The mAB 1H5 bound at 67RRAG70, which is a novel epitope and is conserved in almost all PRV strains. These findings provide novel insight into the structure and function of PRV proteins, the analysis of antigenic epitope characteristics, and the establishment of antigen or antibody detection methods.

AB - Since 2011, pseudorabies virus (PRV) has recurred in several vaccinated pig farms in China. PRV variants with high virulence were found to be the main cause of the outbreaks. In the face of the PRV epidemic, detection of the wild strain is as important as vaccine immunization, so we hoped to achieve differential diagnosis of PRV by obtaining a monoclonal antibody (mAB) that could be used to identify the wild strain. In this study, we used a novel immunization and screening strategy to prepare an mAB and obtained mAB 1H5 against the gE glycoprotein. An immunofluorescence assay (IFA) revealed that this mAB was specific to both classic and variant strains of PRV. Subsequently, we further identified the linear epitopes of B cells recognized using the mAB. The mAB 1H5 bound at 67RRAG70, which is a novel epitope and is conserved in almost all PRV strains. These findings provide novel insight into the structure and function of PRV proteins, the analysis of antigenic epitope characteristics, and the establishment of antigen or antibody detection methods.

KW - PRV

KW - epitopes

KW - gE

KW - monoclonal antibody

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U2 - 10.3390/vetsci10020133

DO - 10.3390/vetsci10020133

M3 - Article

AN - SCOPUS:85149232520

SN - 2306-7381

VL - 10

JO - Veterinary Sciences

JF - Veterinary Sciences

IS - 2

M1 - 133

ER -

Preparation and Identification of a Monoclonal Antibody against the Pseudorabies Virus gE Glycoprotein through a Novel Strategy

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Keywords

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