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A multi-landing pad DNA integration platform for mammalian cell engineering

Engineering mammalian cell lines that stably express many transgenes requires the precise insertion of large amounts of heterologous DNA into well-characterized genomic loci, but current methods are limited. To facilitate reliable large-scale engineering of CHO cells, we identified 21 novel genomic...

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Autores principales: Gaidukov, Leonid, Wroblewska, Liliana, Teague, Brian, Nelson, Tom, Zhang, Xin, Liu, Yan, Jagtap, Kalpana, Mamo, Selamawit, Tseng, Wen Allen, Lowe, Alexis, Das, Jishnu, Bandara, Kalpanie, Baijuraj, Swetha, Summers, Nevin M, Lu, Timothy K, Zhang, Lin, Weiss, Ron
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Oxford University Press 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5934685/
https://www.ncbi.nlm.nih.gov/pubmed/29617873
http://dx.doi.org/10.1093/nar/gky216
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author Gaidukov, Leonid
Wroblewska, Liliana
Teague, Brian
Nelson, Tom
Zhang, Xin
Liu, Yan
Jagtap, Kalpana
Mamo, Selamawit
Tseng, Wen Allen
Lowe, Alexis
Das, Jishnu
Bandara, Kalpanie
Baijuraj, Swetha
Summers, Nevin M
Lu, Timothy K
Zhang, Lin
Weiss, Ron
author_facet Gaidukov, Leonid
Wroblewska, Liliana
Teague, Brian
Nelson, Tom
Zhang, Xin
Liu, Yan
Jagtap, Kalpana
Mamo, Selamawit
Tseng, Wen Allen
Lowe, Alexis
Das, Jishnu
Bandara, Kalpanie
Baijuraj, Swetha
Summers, Nevin M
Lu, Timothy K
Zhang, Lin
Weiss, Ron
author_sort Gaidukov, Leonid
collection PubMed
description Engineering mammalian cell lines that stably express many transgenes requires the precise insertion of large amounts of heterologous DNA into well-characterized genomic loci, but current methods are limited. To facilitate reliable large-scale engineering of CHO cells, we identified 21 novel genomic sites that supported stable long-term expression of transgenes, and then constructed cell lines containing one, two or three ‘landing pad’ recombination sites at selected loci. By using a highly efficient BxB1 recombinase along with different selection markers at each site, we directed recombinase-mediated insertion of heterologous DNA to selected sites, including targeting all three with a single transfection. We used this method to controllably integrate up to nine copies of a monoclonal antibody, representing about 100 kb of heterologous DNA in 21 transcriptional units. Because the integration was targeted to pre-validated loci, recombinant protein expression remained stable for weeks and additional copies of the antibody cassette in the integrated payload resulted in a linear increase in antibody expression. Overall, this multi-copy site-specific integration platform allows for controllable and reproducible insertion of large amounts of DNA into stable genomic sites, which has broad applications for mammalian synthetic biology, recombinant protein production and biomanufacturing.
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spelling pubmed-59346852018-05-09 A multi-landing pad DNA integration platform for mammalian cell engineering Gaidukov, Leonid Wroblewska, Liliana Teague, Brian Nelson, Tom Zhang, Xin Liu, Yan Jagtap, Kalpana Mamo, Selamawit Tseng, Wen Allen Lowe, Alexis Das, Jishnu Bandara, Kalpanie Baijuraj, Swetha Summers, Nevin M Lu, Timothy K Zhang, Lin Weiss, Ron Nucleic Acids Res Molecular Biology Engineering mammalian cell lines that stably express many transgenes requires the precise insertion of large amounts of heterologous DNA into well-characterized genomic loci, but current methods are limited. To facilitate reliable large-scale engineering of CHO cells, we identified 21 novel genomic sites that supported stable long-term expression of transgenes, and then constructed cell lines containing one, two or three ‘landing pad’ recombination sites at selected loci. By using a highly efficient BxB1 recombinase along with different selection markers at each site, we directed recombinase-mediated insertion of heterologous DNA to selected sites, including targeting all three with a single transfection. We used this method to controllably integrate up to nine copies of a monoclonal antibody, representing about 100 kb of heterologous DNA in 21 transcriptional units. Because the integration was targeted to pre-validated loci, recombinant protein expression remained stable for weeks and additional copies of the antibody cassette in the integrated payload resulted in a linear increase in antibody expression. Overall, this multi-copy site-specific integration platform allows for controllable and reproducible insertion of large amounts of DNA into stable genomic sites, which has broad applications for mammalian synthetic biology, recombinant protein production and biomanufacturing. Oxford University Press 2018-05-04 2018-04-02 /pmc/articles/PMC5934685/ /pubmed/29617873 http://dx.doi.org/10.1093/nar/gky216 Text en © The Author(s) 2018. Published by Oxford University Press on behalf of Nucleic Acids Research. http://creativecommons.org/licenses/by-nc/4.0/ This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/4.0/), which permits non-commercial re-use, distribution, and reproduction in any medium, provided the original work is properly cited. For commercial re-use, please contact journals.permissions@oup.com
spellingShingle Molecular Biology
Gaidukov, Leonid
Wroblewska, Liliana
Teague, Brian
Nelson, Tom
Zhang, Xin
Liu, Yan
Jagtap, Kalpana
Mamo, Selamawit
Tseng, Wen Allen
Lowe, Alexis
Das, Jishnu
Bandara, Kalpanie
Baijuraj, Swetha
Summers, Nevin M
Lu, Timothy K
Zhang, Lin
Weiss, Ron
A multi-landing pad DNA integration platform for mammalian cell engineering
title A multi-landing pad DNA integration platform for mammalian cell engineering
title_full A multi-landing pad DNA integration platform for mammalian cell engineering
title_fullStr A multi-landing pad DNA integration platform for mammalian cell engineering
title_full_unstemmed A multi-landing pad DNA integration platform for mammalian cell engineering
title_short A multi-landing pad DNA integration platform for mammalian cell engineering
title_sort multi-landing pad dna integration platform for mammalian cell engineering
topic Molecular Biology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5934685/
https://www.ncbi.nlm.nih.gov/pubmed/29617873
http://dx.doi.org/10.1093/nar/gky216
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