Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein

Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein

Porcine reproductive and respiratory syndrome virus (PRRSV) is still one of the most important infectious diseases threatening the swine industry. To construct North American type II PRRSV infectious clone containing green fluorescent protein (GFP) gene, we amplify gfp gene, flanked by PRRSV Nsp2 ge...

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Main Authors: Liyue Wang, Kao Zhang, Hongyu Lin, Wenyan Li, Jiexia Wen, Jianlou Zhang, Yonghong Zhang, Xiujin Li, Fei Zhong
Format: Article
Language:English
Published: Hindawi Limited 2014-01-01
Series:BioMed Research International
Online Access:http://dx.doi.org/10.1155/2014/368581
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spelling doaj-e2ae225a63734fb6914cd2bbe3bfb6be2020-11-24T22:18:56ZengHindawi LimitedBioMed Research International2314-61332314-61412014-01-01201410.1155/2014/368581368581Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent ProteinLiyue Wang0Kao Zhang1Hongyu Lin2Wenyan Li3Jiexia Wen4Jianlou Zhang5Yonghong Zhang6Xiujin Li7Fei Zhong8Laboratory of Molecular Virology and Immunology, College of Veterinary Medicine, Agricultural University of Hebei, Hebei Engineering and Technology Research Center of Veterinary Biotechnology, Baoding 071001, ChinaLaboratory of Molecular Virology and Immunology, College of Veterinary Medicine, Agricultural University of Hebei, Hebei Engineering and Technology Research Center of Veterinary Biotechnology, Baoding 071001, ChinaDepartment of Biotechnology, College of Environmental and Chemical Engineering, Yanshan University, Qinhuangdao 066004, ChinaLaboratory of Molecular Virology and Immunology, College of Veterinary Medicine, Agricultural University of Hebei, Hebei Engineering and Technology Research Center of Veterinary Biotechnology, Baoding 071001, ChinaLaboratory of Molecular Virology and Immunology, College of Veterinary Medicine, Agricultural University of Hebei, Hebei Engineering and Technology Research Center of Veterinary Biotechnology, Baoding 071001, ChinaLaboratory of Molecular Virology and Immunology, College of Veterinary Medicine, Agricultural University of Hebei, Hebei Engineering and Technology Research Center of Veterinary Biotechnology, Baoding 071001, ChinaLaboratory of Molecular Virology and Immunology, College of Veterinary Medicine, Agricultural University of Hebei, Hebei Engineering and Technology Research Center of Veterinary Biotechnology, Baoding 071001, ChinaDepartment of Biotechnology, College of Environmental and Chemical Engineering, Yanshan University, Qinhuangdao 066004, ChinaLaboratory of Molecular Virology and Immunology, College of Veterinary Medicine, Agricultural University of Hebei, Hebei Engineering and Technology Research Center of Veterinary Biotechnology, Baoding 071001, ChinaPorcine reproductive and respiratory syndrome virus (PRRSV) is still one of the most important infectious diseases threatening the swine industry. To construct North American type II PRRSV infectious clone containing green fluorescent protein (GFP) gene, we amplify gfp gene, flanked by PRRSV Nsp2 gene fragments upstream and downstream, using overlap PCR method from pcDNA-EF1-GFP plasmid and FL12 plasmid containing PRRSV infectious genome as the templates. The Nsp2 fragment-flanked gfp gene was inserted into Nsp2 gene of the FL12 plasmid by Spe I and Xho I sites to generate PRRSV infectious recombinant plasmid (FL12-GFP) containing gfp gene. The recombinant PRRSV expressing GFP (PRRSV-GFP) was rescued in baby hamster kidney-21 (BHK-21) cells by transfecting PRRSV mRNA synthesized in vitro and amplified in Marc-145 cells. The PRRSV-GFP infectivity and replication capacity were identified. Results showed that, by adopting overlap PCR strategy, the gfp gene was successfully inserted into and fused with PRRSV Nsp2 gene in the PRRSV infectious clone plasmid FL-12 to generate FL12-GFP plasmid. The recombinant PRRSV-GFP was generated through transfecting PRRSV mRNA in BHK-2 cells. Like its parental virus, the recombinant PRRSV-GFP maintains its infectivity to Marc-145 cells and porcine alveolar macrophages (PAMs). This study provides essential conditions for further investigation on PRRSV.http://dx.doi.org/10.1155/2014/368581
collection DOAJ
language English
format Article
sources DOAJ
author Liyue Wang
Kao Zhang
Hongyu Lin
Wenyan Li
Jiexia Wen
Jianlou Zhang
Yonghong Zhang
Xiujin Li
Fei Zhong
spellingShingle Liyue Wang
Kao Zhang
Hongyu Lin
Wenyan Li
Jiexia Wen
Jianlou Zhang
Yonghong Zhang
Xiujin Li
Fei Zhong
Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein
BioMed Research International
author_facet Liyue Wang
Kao Zhang
Hongyu Lin
Wenyan Li
Jiexia Wen
Jianlou Zhang
Yonghong Zhang
Xiujin Li
Fei Zhong
author_sort Liyue Wang
title Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein
title_short Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein
title_full Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein
title_fullStr Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein
title_full_unstemmed Preparation of North American Type II PRRSV Infectious Clone Expressing Green Fluorescent Protein
title_sort preparation of north american type ii prrsv infectious clone expressing green fluorescent protein
publisher Hindawi Limited
series BioMed Research International
issn 2314-6133
2314-6141
publishDate 2014-01-01
description Porcine reproductive and respiratory syndrome virus (PRRSV) is still one of the most important infectious diseases threatening the swine industry. To construct North American type II PRRSV infectious clone containing green fluorescent protein (GFP) gene, we amplify gfp gene, flanked by PRRSV Nsp2 gene fragments upstream and downstream, using overlap PCR method from pcDNA-EF1-GFP plasmid and FL12 plasmid containing PRRSV infectious genome as the templates. The Nsp2 fragment-flanked gfp gene was inserted into Nsp2 gene of the FL12 plasmid by Spe I and Xho I sites to generate PRRSV infectious recombinant plasmid (FL12-GFP) containing gfp gene. The recombinant PRRSV expressing GFP (PRRSV-GFP) was rescued in baby hamster kidney-21 (BHK-21) cells by transfecting PRRSV mRNA synthesized in vitro and amplified in Marc-145 cells. The PRRSV-GFP infectivity and replication capacity were identified. Results showed that, by adopting overlap PCR strategy, the gfp gene was successfully inserted into and fused with PRRSV Nsp2 gene in the PRRSV infectious clone plasmid FL-12 to generate FL12-GFP plasmid. The recombinant PRRSV-GFP was generated through transfecting PRRSV mRNA in BHK-2 cells. Like its parental virus, the recombinant PRRSV-GFP maintains its infectivity to Marc-145 cells and porcine alveolar macrophages (PAMs). This study provides essential conditions for further investigation on PRRSV.
url http://dx.doi.org/10.1155/2014/368581
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