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The genetic intractability of Symbiodinium microadriaticum to standard algal transformation methods

机译:Symbiodinium microiaticum对标准藻类转化方法的遗传难以

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摘要

Modern transformation and genome editing techniques have shown great success across a broad variety of organisms. However, no study of successfully applied genome editing has been reported in a dinoflagellate despite the first genetic transformation of Symbiodinium being published about 20 years ago. Using an array of different available transformation techniques, we attempted to transform Symbiodinium microadriaticum (CCMP2467), a dinoflagellate symbiont of reef-building corals, with the view to performing subsequent CRISPR-Cas9 mediated genome editing. Plasmid vectors designed for nuclear transformation containing the chloramphenicol resistance gene under the control of the CaMV p35S promoter as well as several putative endogenous promoters were used to test a variety of transformation techniques including biolistics, electroporation and agitation with silicon carbide whiskers. Chloroplast-targeted transformation was attempted using an engineered Symbiodinium chloroplast minicircle encoding a modified PsbA protein expected to confer atrazine resistance. We report that we have been unable to confer chloramphenicol or atrazine resistance on Symbiodinium microadriaticum strain CCMP2467.
机译:现代转型与基因组编辑技术已经显示在广泛的各种生物的巨大成功。但是,没有成功地应用于基因组编辑的研究已在鞭毛藻共生,尽管的第一个遗传转化的问世大约20年前的报道。使用的不同的可用的转化技术的阵列,我们试图变换共生microadriaticum(CCMP2467),造礁珊瑚的甲藻共生体,以期执行后续CRISPR-Cas9介导的基因组编辑。设计用于含有CaMV启动子P35S以及几种推定的内源启动子的控制下的氯霉素抗性基因核转化质粒载体被用来测试各种转化技术,包括基因枪,电穿孔和用搅动碳化硅晶须。叶绿体靶向转化用编码预期赋予莠去津抗性的修饰的蛋白的psbA的工程改造的共生叶绿体小环尝试。我们报告,我们已经无法赋予氯霉素或阿特拉津抗性上共生microadriaticum株CCMP2467。

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