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Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System

ZFN technology is a powerful research tool and has been used for genome editing in cells lines, animals and plants. The generation of functional ZFNs for particular targets in mammalian genome is still challenging for an average research group. The modular-assembly method is relatively fast, easy-to...

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Autores principales: Zhang, Weifeng, Guo, Yuanxu, Zhang, Chen, Ji, Haiyan, Meng, Wenpeng, Wang, Dongyang, Li, Xing, Mao, Qinwen, Xia, Haibin
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2012
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3445457/
https://www.ncbi.nlm.nih.gov/pubmed/23028823
http://dx.doi.org/10.1371/journal.pone.0045169
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author Zhang, Weifeng
Guo, Yuanxu
Zhang, Chen
Ji, Haiyan
Meng, Wenpeng
Wang, Dongyang
Li, Xing
Mao, Qinwen
Xia, Haibin
author_facet Zhang, Weifeng
Guo, Yuanxu
Zhang, Chen
Ji, Haiyan
Meng, Wenpeng
Wang, Dongyang
Li, Xing
Mao, Qinwen
Xia, Haibin
author_sort Zhang, Weifeng
collection PubMed
description ZFN technology is a powerful research tool and has been used for genome editing in cells lines, animals and plants. The generation of functional ZFNs for particular targets in mammalian genome is still challenging for an average research group. The modular-assembly method is relatively fast, easy-to-practice but has a high failure rate. Some recent studies suggested that a ZFP with low binding activity might be able to form a working ZFN pair with another binding active half-ZFP. In order to unveil the potential ZFP candidates among those with low binding activities, this paper established a highly sensitive mammalian cell-based transcriptional reporter system to assess the DNA binding activities of ZFPs by inserting multiple copies of ZFN target sequence fragment (TSF) of an interested gene (e. g., hPGRN or hVEGF). Our results showed that this system increased the screening sensitivity up to 50-fold and markedly amplified the differences in the binding activities between different ZFPs. We also found that the targeted chromosomal gene repair efficiency of each hPGRN or hVEGF ZFN pair was in proportion with the combination of the binding activities of the ZFL (Left zinc finger) and ZFR (Right zinc finger). A hPGRN ZFR with low binding ability was able to form a biological active ZFN if combined with a hPGRN ZFL with relatively high binding ability. Lastly, site-specific genome editing by hPGRN ZFNs generated by this system was confirmed by sequencing, and the PGRN knock-out cell line showed significantly decreased cell growth compared with the control. Our system will provide a valuable tool for further optimizing the nucleases with regard to specificity and cytotoxicity.
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spelling pubmed-34454572012-10-01 Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System Zhang, Weifeng Guo, Yuanxu Zhang, Chen Ji, Haiyan Meng, Wenpeng Wang, Dongyang Li, Xing Mao, Qinwen Xia, Haibin PLoS One Research Article ZFN technology is a powerful research tool and has been used for genome editing in cells lines, animals and plants. The generation of functional ZFNs for particular targets in mammalian genome is still challenging for an average research group. The modular-assembly method is relatively fast, easy-to-practice but has a high failure rate. Some recent studies suggested that a ZFP with low binding activity might be able to form a working ZFN pair with another binding active half-ZFP. In order to unveil the potential ZFP candidates among those with low binding activities, this paper established a highly sensitive mammalian cell-based transcriptional reporter system to assess the DNA binding activities of ZFPs by inserting multiple copies of ZFN target sequence fragment (TSF) of an interested gene (e. g., hPGRN or hVEGF). Our results showed that this system increased the screening sensitivity up to 50-fold and markedly amplified the differences in the binding activities between different ZFPs. We also found that the targeted chromosomal gene repair efficiency of each hPGRN or hVEGF ZFN pair was in proportion with the combination of the binding activities of the ZFL (Left zinc finger) and ZFR (Right zinc finger). A hPGRN ZFR with low binding ability was able to form a biological active ZFN if combined with a hPGRN ZFL with relatively high binding ability. Lastly, site-specific genome editing by hPGRN ZFNs generated by this system was confirmed by sequencing, and the PGRN knock-out cell line showed significantly decreased cell growth compared with the control. Our system will provide a valuable tool for further optimizing the nucleases with regard to specificity and cytotoxicity. Public Library of Science 2012-09-18 /pmc/articles/PMC3445457/ /pubmed/23028823 http://dx.doi.org/10.1371/journal.pone.0045169 Text en © 2012 Zhang 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
Zhang, Weifeng
Guo, Yuanxu
Zhang, Chen
Ji, Haiyan
Meng, Wenpeng
Wang, Dongyang
Li, Xing
Mao, Qinwen
Xia, Haibin
Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System
title Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System
title_full Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System
title_fullStr Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System
title_full_unstemmed Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System
title_short Rescue the Failed Half-ZFN by a Sensitive Mammalian Cell-Based Luciferase Reporter System
title_sort rescue the failed half-zfn by a sensitive mammalian cell-based luciferase reporter system
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3445457/
https://www.ncbi.nlm.nih.gov/pubmed/23028823
http://dx.doi.org/10.1371/journal.pone.0045169
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