Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer

Multiple genetic modifications in pigs can essentially benefit research on agriculture, human disease and xenotransplantation. Most multi-transgenic pigs have been produced by complex and time-consuming breeding programs using multiple single-transgenic pigs. This study explored the feasibility of p...

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Autores principales: Deng, Wei, Yang, Dongshan, Zhao, Bentian, Ouyang, Zhen, Song, Jun, Fan, Nana, Liu, Zhaoming, Zhao, Yu, Wu, Qinghong, Nashun, Bayaer, Tang, Jiangjing, Wu, Zhenfang, Gu, Weiwang, Lai, Liangxue
Formato: Texto
Lenguaje:English
Publicado: Public Library of Science 2011
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3094386/
https://www.ncbi.nlm.nih.gov/pubmed/21603633
http://dx.doi.org/10.1371/journal.pone.0019986
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author Deng, Wei
Yang, Dongshan
Zhao, Bentian
Ouyang, Zhen
Song, Jun
Fan, Nana
Liu, Zhaoming
Zhao, Yu
Wu, Qinghong
Nashun, Bayaer
Tang, Jiangjing
Wu, Zhenfang
Gu, Weiwang
Lai, Liangxue
author_facet Deng, Wei
Yang, Dongshan
Zhao, Bentian
Ouyang, Zhen
Song, Jun
Fan, Nana
Liu, Zhaoming
Zhao, Yu
Wu, Qinghong
Nashun, Bayaer
Tang, Jiangjing
Wu, Zhenfang
Gu, Weiwang
Lai, Liangxue
author_sort Deng, Wei
collection PubMed
description Multiple genetic modifications in pigs can essentially benefit research on agriculture, human disease and xenotransplantation. Most multi-transgenic pigs have been produced by complex and time-consuming breeding programs using multiple single-transgenic pigs. This study explored the feasibility of producing multi-transgenic pigs using the viral 2A peptide in the light of previous research indicating that it can be utilized for multi-gene transfer in gene therapy and somatic cell reprogramming. A 2A peptide-based double-promoter expression vector that mediated the expression of four fluorescent proteins was constructed and transfected into primary porcine fetal fibroblasts. Cell colonies (54.3%) formed under G418 selection co-expressed the four fluorescent proteins at uniformly high levels. The reconstructed embryos, which were obtained by somatic cell nuclear transfer and confirmed to express the four fluorescent proteins evenly, were transplanted into seven recipient gilts. Eleven piglets were delivered by two gilts, and seven of them co-expressed the four fluorescent proteins at equivalently high levels in various tissues. The fluorescence intensities were directly observed at the nose, hoof and tongue using goggles. The results suggest that the strategy of combining the 2A peptide and double promoters efficiently mediates the co-expression of the four fluorescent proteins in pigs and is hence a promising methodology to generate multi-transgenic pigs by a single nuclear transfer.
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spelling pubmed-30943862011-05-19 Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer Deng, Wei Yang, Dongshan Zhao, Bentian Ouyang, Zhen Song, Jun Fan, Nana Liu, Zhaoming Zhao, Yu Wu, Qinghong Nashun, Bayaer Tang, Jiangjing Wu, Zhenfang Gu, Weiwang Lai, Liangxue PLoS One Research Article Multiple genetic modifications in pigs can essentially benefit research on agriculture, human disease and xenotransplantation. Most multi-transgenic pigs have been produced by complex and time-consuming breeding programs using multiple single-transgenic pigs. This study explored the feasibility of producing multi-transgenic pigs using the viral 2A peptide in the light of previous research indicating that it can be utilized for multi-gene transfer in gene therapy and somatic cell reprogramming. A 2A peptide-based double-promoter expression vector that mediated the expression of four fluorescent proteins was constructed and transfected into primary porcine fetal fibroblasts. Cell colonies (54.3%) formed under G418 selection co-expressed the four fluorescent proteins at uniformly high levels. The reconstructed embryos, which were obtained by somatic cell nuclear transfer and confirmed to express the four fluorescent proteins evenly, were transplanted into seven recipient gilts. Eleven piglets were delivered by two gilts, and seven of them co-expressed the four fluorescent proteins at equivalently high levels in various tissues. The fluorescence intensities were directly observed at the nose, hoof and tongue using goggles. The results suggest that the strategy of combining the 2A peptide and double promoters efficiently mediates the co-expression of the four fluorescent proteins in pigs and is hence a promising methodology to generate multi-transgenic pigs by a single nuclear transfer. Public Library of Science 2011-05-13 /pmc/articles/PMC3094386/ /pubmed/21603633 http://dx.doi.org/10.1371/journal.pone.0019986 Text en Deng et al. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Deng, Wei
Yang, Dongshan
Zhao, Bentian
Ouyang, Zhen
Song, Jun
Fan, Nana
Liu, Zhaoming
Zhao, Yu
Wu, Qinghong
Nashun, Bayaer
Tang, Jiangjing
Wu, Zhenfang
Gu, Weiwang
Lai, Liangxue
Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer
title Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer
title_full Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer
title_fullStr Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer
title_full_unstemmed Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer
title_short Use of the 2A Peptide for Generation of Multi-Transgenic Pigs through a Single Round of Nuclear Transfer
title_sort use of the 2a peptide for generation of multi-transgenic pigs through a single round of nuclear transfer
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3094386/
https://www.ncbi.nlm.nih.gov/pubmed/21603633
http://dx.doi.org/10.1371/journal.pone.0019986
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