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ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome

Programmable nucleases have allowed the rapid development of gene editing and transgenics, but the technology still suffers from the lack of predefined genetic loci for reliable transgene expression and maintenance. To address this issue, we used ФC31 integrase to navigate the porcine genome and ide...

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Autores principales: Bi, Yanzhen, Hua, Zaidong, Ren, Hongyan, Zhang, Liping, Xiao, Hongwei, Liu, Ximei, Hua, Wenjun, Mei, Shuqi, Molenaar, Adrian, Laible, Götz, Zheng, Xinmin
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5796098/
https://www.ncbi.nlm.nih.gov/pubmed/29300364
http://dx.doi.org/10.3390/ijms19010149
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author Bi, Yanzhen
Hua, Zaidong
Ren, Hongyan
Zhang, Liping
Xiao, Hongwei
Liu, Ximei
Hua, Wenjun
Mei, Shuqi
Molenaar, Adrian
Laible, Götz
Zheng, Xinmin
author_facet Bi, Yanzhen
Hua, Zaidong
Ren, Hongyan
Zhang, Liping
Xiao, Hongwei
Liu, Ximei
Hua, Wenjun
Mei, Shuqi
Molenaar, Adrian
Laible, Götz
Zheng, Xinmin
author_sort Bi, Yanzhen
collection PubMed
description Programmable nucleases have allowed the rapid development of gene editing and transgenics, but the technology still suffers from the lack of predefined genetic loci for reliable transgene expression and maintenance. To address this issue, we used ФC31 integrase to navigate the porcine genome and identify the pseudo attP sites suitable as safe harbors for sustained transgene expression. The combined ФC31 integrase mRNA and an enhanced green fluorescence protein (EGFP) reporter donor were microinjected into one-cell zygotes for transgene integration. Among the resulting seven EGFP-positive piglets, two had transgene integrations at pseudo attP sites, located in an intergenic region of chromosome 1 (chr1-attP) and the 6th intron of the TRABD2A gene on chromosome 3 (chr3-attP), respectively. The integration structure was determined by TAIL-PCR and Southern blotting. Primary fibroblast cells were isolated from the two piglets and examined using fluorescence-activated cell sorting (FACS) and enzyme-linked immunosorbent assay (ELISA), which demonstrated that the chr1-attP site was more potent than chr3-attP site in supporting the EGFP expression. Both piglets had green feet under the emission of UV light, and pelleted primary fibroblast cells were green-colored under natural light, corroborating that the two pseudo attP sites are beneficial to transgene expression. The discovery of these two novel safe harbors for robust and durable transgene expression will greatly facilitate the use of transgenic pigs for basic, biomedical and agricultural studies and applications.
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spelling pubmed-57960982018-02-09 ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome Bi, Yanzhen Hua, Zaidong Ren, Hongyan Zhang, Liping Xiao, Hongwei Liu, Ximei Hua, Wenjun Mei, Shuqi Molenaar, Adrian Laible, Götz Zheng, Xinmin Int J Mol Sci Article Programmable nucleases have allowed the rapid development of gene editing and transgenics, but the technology still suffers from the lack of predefined genetic loci for reliable transgene expression and maintenance. To address this issue, we used ФC31 integrase to navigate the porcine genome and identify the pseudo attP sites suitable as safe harbors for sustained transgene expression. The combined ФC31 integrase mRNA and an enhanced green fluorescence protein (EGFP) reporter donor were microinjected into one-cell zygotes for transgene integration. Among the resulting seven EGFP-positive piglets, two had transgene integrations at pseudo attP sites, located in an intergenic region of chromosome 1 (chr1-attP) and the 6th intron of the TRABD2A gene on chromosome 3 (chr3-attP), respectively. The integration structure was determined by TAIL-PCR and Southern blotting. Primary fibroblast cells were isolated from the two piglets and examined using fluorescence-activated cell sorting (FACS) and enzyme-linked immunosorbent assay (ELISA), which demonstrated that the chr1-attP site was more potent than chr3-attP site in supporting the EGFP expression. Both piglets had green feet under the emission of UV light, and pelleted primary fibroblast cells were green-colored under natural light, corroborating that the two pseudo attP sites are beneficial to transgene expression. The discovery of these two novel safe harbors for robust and durable transgene expression will greatly facilitate the use of transgenic pigs for basic, biomedical and agricultural studies and applications. MDPI 2018-01-04 /pmc/articles/PMC5796098/ /pubmed/29300364 http://dx.doi.org/10.3390/ijms19010149 Text en © 2018 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Bi, Yanzhen
Hua, Zaidong
Ren, Hongyan
Zhang, Liping
Xiao, Hongwei
Liu, Ximei
Hua, Wenjun
Mei, Shuqi
Molenaar, Adrian
Laible, Götz
Zheng, Xinmin
ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome
title ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome
title_full ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome
title_fullStr ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome
title_full_unstemmed ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome
title_short ФC31 Integrase-Mediated Isolation and Characterization of Novel Safe Harbors for Transgene Expression in the Pig Genome
title_sort фc31 integrase-mediated isolation and characterization of novel safe harbors for transgene expression in the pig genome
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5796098/
https://www.ncbi.nlm.nih.gov/pubmed/29300364
http://dx.doi.org/10.3390/ijms19010149
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