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首页> 外文期刊>Molecular biotechnology >Improved FLP recombinase, FLPe, efficiently removes marker gene from transgene locus developed by Cre-lox mediated site-specific gene integration in Rice
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Improved FLP recombinase, FLPe, efficiently removes marker gene from transgene locus developed by Cre-lox mediated site-specific gene integration in Rice

机译:改良的FLP重组酶FLPe可有效地从Cre-lox介导的水稻定点基因整合开发的转基因基因座中去除标记基因

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摘要

Site-specific recombination systems, such as FLP-FRT and Cre-lox, carry out precise recombination reactions on their respective targets in plant cells. This has led to the development of two important applications in plant biotechnology: marker-gene deletion and site-specific gene integration. To draw benefits of both applications, it is necessary to implement them in a single transformation process. In order to develop this new process, the present study evaluated the efficiency of FLP-FRT system for excising marker gene from the transgene locus developed by Cre-lox mediated site-specific integration in rice. Two different FLP recombinases, the wild-type FLP (FLPwt) and its thermostable derivative, FLPe, were used for the excision of marker gene flanked by FLP recombination targets (FRT). While marker excision mediated by FLPwt was undetectable, use of FLPe resulted in efficient marker excision in a number of transgenic lines, with the relative efficiency reaching up to ~100%. Thus, thermo-stability of FLP recombinase in rice cells is critical for efficient site-specific recombination, and use of FLPe offers practical solutions to FLP-FRT-based biotechnology applications in plants.
机译:特定于位点的重组系统(例如FLP-FRT和Cre-lox)对植物细胞中各自的靶标进行精确的重组反应。这导致了植物生物技术中两个重要应用的发展:标记基因缺失和位点特异性基因整合。为了从两个应用程序中受益,有必要在单个转换过程中实现它们。为了开发这种新方法,本研究评估了FLP-FRT系统从Cre-lox介导的水稻位点特异性整合开发的转基因基因座中切除标记基因的效率。两种不同的FLP重组酶,即野生型FLP(FLPwt)和其热稳定衍生物FLPe,用于切除侧翼为FLP重组靶标(FRT)的标记基因。尽管无法检测到由FLPwt介导的标记切除,但FLPe的使用导致了许多转基因品系的有效标记切除,相对效率高达〜100%。因此,FLP重组酶在水稻细胞中的热稳定性对于有效的位点特异性重组至关重要,并且FLPe的使用为植物中基于FLP-FRT的生物技术应用提供了实用的解决方案。

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