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H2O2-Based Method for Rapid Detection of Transgene-Free Rice Plants from Segregating CRISPR/Cas9 Genome-Edited Progenies

机译:基于H2O2的从CRISPR / Cas9基因组编辑后代分离中快速检测无转基因水稻的方法

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摘要

Genome-editing techniques such as CRISPR/Cas9 have been widely used in crop functional genomics and improvement. To efficiently deliver the guide RNA and Cas9, most studies still rely on Agrobacterium-mediated transformation, which involves a selection marker gene. However, several limiting factors may impede the efficiency of screening transgene-free genome-edited plants, including the time needed to produce each life cycle, the response to selection reagents, and the labor costs of PCR-based genotyping. To overcome these disadvantages, we developed a simple and high-throughput method based on visual detection of antibiotics-derived H2O2 to verify transgene-free genome-edited plants. In transgenic rice containing hygromycin phosphotransferase (HPT), H2O2 content did not change in the presence of hygromycin B (HyB). In contrast, in transgenic-free rice plants with 10-h HyB treatment, levels of H2O2 and malondialdehyde, indicators of oxidative stress, were elevated. Detection of H2O2 by 3,3′-diaminobenzidine (DAB) staining suggested that H2O2 could be a marker to efficiently distinguish transgenic and non-transgenic plants. Analysis of 24 segregating progenies of an HPT-containing rice plant by RT-PCR and DAB staining verified that DAB staining is a feasible method for detecting transformants and non-transformants. Transgene-free genome-edited plants were faithfully validated by both PCR and the H2O2-based method. Moreover, HyB induced overproduction of H2O2 in leaves of Arabidopsis, maize, tobacco, and tomato, which suggests the potential application of the DAB method for detecting transgenic events containing HPT in a wide range of plant species. Thus, visual detection of DAB provides a simple, cheap, and reliable way to efficiently identify transgene-free genome-edited and HPT-containing transgenic rice.
机译:CRISPR / Cas9等基因组编辑技术已广泛用于作物功能基因组学和改良中。为了有效地递送指导RNA和Cas9,大多数研究仍依赖于农杆菌介导的转化,该转化涉及选择标记基因。但是,一些限制因素可能会阻碍筛选无转基因的基因组编辑植物的效率,包括产生每个生命周期所需的时间,对选择试剂的反应以及基于PCR的基因分型的人工成本。为了克服这些缺点,我们开发了一种基于视觉检测抗生素衍生的H2O2的简单且高通量的方法,以验证无转基因的基因组编辑的植物。在含有潮霉素磷酸转移酶(HPT)的转基因水稻中,潮霉素B(HyB)的存在下H2O2含量没有变化。相反,在经过10小时HyB处理的无转基因水稻植株中,H2O2和丙二醛(氧化应激指标)的水平升高。通过3,3'-二氨基联苯胺(DAB)染色检测H2O2表明,H2O2可以作为有效区分转基因植物和非转基因植物的标记。通过RT-PCR和DAB染色分析了含有HPT的水稻植物的24个分离后代,证明DAB染色是检测转化体和非转化体的可行方法。通过PCR和基于H2O2的方法均忠实地验证了无转基因基因组编辑的植物。此外,HyB诱导了拟南芥,玉米,烟草和番茄叶片中H2O2的过量生产,这表明DAB方法在检测多种植物中含有HPT的转基因事件中的潜在应用。因此,DAB的视觉检测提供了一种简单,便宜和可靠的方法,可以有效地鉴定无转基因的基因组编辑的和含有HPT的转基因水稻。

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