Cloning and expression of Aujeszky's disease virus glycoprotein E (gE) in a baculovirus system
Aujeszky' s disease (AD) is an infectious disease causing important economic losses to the swine industry worldwide. The disease is caused by an alpha-herpesvirus, Aujeszky' s disease virus (ADV), an enveloped virus with a double stranded linear DNA genome. The ADV genome encodes 11 glycop...
Main Authors: | Dambros, Régia Maria Feltrin, Ribeiro, Bergman Moraes, Aguiar, Raimundo Wagner de Souza, Schaefer, Rejane, Esteves, Paulo Augusto, Perecmanis, Simone, Simon, Neide Lisiane, Silva, Nayara Cavalcante, Coldebella, Michele, Ciacci-Zanella, Janice Reis |
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Format: | Artigo |
Language: | English |
Published: |
Sociedade Brasileira de Microbiologia
2017
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Subjects: | |
Online Access: |
http://repositorio.unb.br/handle/10482/27099 |
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Summary: |
Aujeszky' s disease (AD) is an infectious disease causing important economic losses to the swine industry worldwide. The disease is caused by an alpha-herpesvirus, Aujeszky' s disease virus (ADV), an enveloped virus with a double stranded linear DNA genome. The ADV genome encodes 11 glycoproteins, which are major targets for the immune system of the host in response to the infection. The glycoprotein E (gE) is a non-essential protein and deletion of the gE gene has been used for the production of marker vaccines. Aiming to develop molecular reagents for the production of a gE specific ELISA test, the gE gene was amplified by PCR, cloned and expressed into a baculovirus expression system. The recombinant DNA vector pFastBac-gE-ADV was used for site-specific transposition into the recombinant baculovirus (bacmid). Colonies with recombinant bacmid-pFastBac-gE-ADV were selected by antibiotic and color selection and the presence of the gE gene was confirmed by PCR. The recombinant bacmid-pFastBac-gE-ADV was cotransfected in insect Trichoplusia ni and the presence of the recombinant DNA and gE protein were detected by PCR, SDS-PAGE and Western blotting, respectively. |
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