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An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants

Transgenic technology can transfer favorable traits regardless of reproductive isolation and is an important method in plant synthetic biology and genetic improvement. Complex metabolic pathway modification and pyramiding breeding strategies often require the introduction of multiple genes at once,...

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Autores principales: Qin, Guannan, Wu, Suting, Zhang, Liying, Li, Yanyao, Liu, Chunmei, Yu, Jianghui, Deng, Lihua, Xiao, Guoying, Zhang, Zhiguo
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2022
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8879548/
https://www.ncbi.nlm.nih.gov/pubmed/35214820
http://dx.doi.org/10.3390/plants11040488
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author Qin, Guannan
Wu, Suting
Zhang, Liying
Li, Yanyao
Liu, Chunmei
Yu, Jianghui
Deng, Lihua
Xiao, Guoying
Zhang, Zhiguo
author_facet Qin, Guannan
Wu, Suting
Zhang, Liying
Li, Yanyao
Liu, Chunmei
Yu, Jianghui
Deng, Lihua
Xiao, Guoying
Zhang, Zhiguo
author_sort Qin, Guannan
collection PubMed
description Transgenic technology can transfer favorable traits regardless of reproductive isolation and is an important method in plant synthetic biology and genetic improvement. Complex metabolic pathway modification and pyramiding breeding strategies often require the introduction of multiple genes at once, but the current vector assembly systems for constructing multigene expression cassettes are not completely satisfactory. In this study, a new in vitro gene stacking system, GuanNan Stacking (GNS), was developed. Through the introduction of Type IIS restriction enzyme-mediated Golden Gate cloning, GNS allows the modular, standardized assembly of target gene expression cassettes. Because of the introduction of Gateway recombination, GNS facilitates the cloning of superlarge transgene expression cassettes, allows multiple expression cassettes to be efficiently assembled in a binary vector simultaneously, and is compatible with the Cre enzyme-mediated marker deletion mechanism. The linked dual positive-negative marker selection strategy ensures the efficient acquisition of target recombinant plasmids without prokaryotic selection markers in the T-DNA region. The host-independent negative selection marker combined with the TAC backbone ensures the cloning and transfer of large T-DNAs (>100 kb). Using the GNS system, we constructed a binary vector containing five foreign gene expression cassettes and obtained transgenic rice carrying the target traits, proving that the method developed in this research is a powerful tool for plant metabolic engineering and compound trait transgenic breeding.
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spelling pubmed-88795482022-02-26 An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants Qin, Guannan Wu, Suting Zhang, Liying Li, Yanyao Liu, Chunmei Yu, Jianghui Deng, Lihua Xiao, Guoying Zhang, Zhiguo Plants (Basel) Article Transgenic technology can transfer favorable traits regardless of reproductive isolation and is an important method in plant synthetic biology and genetic improvement. Complex metabolic pathway modification and pyramiding breeding strategies often require the introduction of multiple genes at once, but the current vector assembly systems for constructing multigene expression cassettes are not completely satisfactory. In this study, a new in vitro gene stacking system, GuanNan Stacking (GNS), was developed. Through the introduction of Type IIS restriction enzyme-mediated Golden Gate cloning, GNS allows the modular, standardized assembly of target gene expression cassettes. Because of the introduction of Gateway recombination, GNS facilitates the cloning of superlarge transgene expression cassettes, allows multiple expression cassettes to be efficiently assembled in a binary vector simultaneously, and is compatible with the Cre enzyme-mediated marker deletion mechanism. The linked dual positive-negative marker selection strategy ensures the efficient acquisition of target recombinant plasmids without prokaryotic selection markers in the T-DNA region. The host-independent negative selection marker combined with the TAC backbone ensures the cloning and transfer of large T-DNAs (>100 kb). Using the GNS system, we constructed a binary vector containing five foreign gene expression cassettes and obtained transgenic rice carrying the target traits, proving that the method developed in this research is a powerful tool for plant metabolic engineering and compound trait transgenic breeding. MDPI 2022-02-11 /pmc/articles/PMC8879548/ /pubmed/35214820 http://dx.doi.org/10.3390/plants11040488 Text en © 2022 by the authors. https://creativecommons.org/licenses/by/4.0/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 (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Qin, Guannan
Wu, Suting
Zhang, Liying
Li, Yanyao
Liu, Chunmei
Yu, Jianghui
Deng, Lihua
Xiao, Guoying
Zhang, Zhiguo
An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants
title An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants
title_full An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants
title_fullStr An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants
title_full_unstemmed An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants
title_short An Efficient Modular Gateway Recombinase-Based Gene Stacking System for Generating Multi-Trait Transgenic Plants
title_sort efficient modular gateway recombinase-based gene stacking system for generating multi-trait transgenic plants
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8879548/
https://www.ncbi.nlm.nih.gov/pubmed/35214820
http://dx.doi.org/10.3390/plants11040488
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