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Southern-by-Sequencing: A Robust Screening Approach for Molecular Characterization of Genetically Modified Crops

机译:测序南方:一种健壮的筛选方法,用于转基因作物的分子表征

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Molecular characterization of events is an integral part of the advancement process during genetically modified (GM) crop product development. Assessment of these events is traditionally accomplished by polymerase chain reaction (PCR) and Southern blot analyses. Southern blot analysis can be time-consuming and comparatively expensive and does not provide sequence-level detail. We have developed a sequence-based application, Southern-by-Sequencing (SbS), utilizing sequence capture coupled with next-generation sequencing (NGS) technology to replace Southern blot analysis for event selection in a high-throughput molecular characterization environment. SbS is accomplished by hybridizing indexed and pooled whole-genome DNA libraries from GM plants to biotinylated probes designed to target the sequence of transformation plasmids used to generate events within the pool. This sequence capture process enriches the sequence data obtained for targeted regions of interest (transformation plasmid DNA). Taking advantage of the DNA adjacent to the targeted bases (referred to as next-to-target sequence) that accompanies the targeted transformation plasmid sequence, the data analysis detects plasmid-to-genome and plasmid-to-plasmid junctions introduced during insertion into the plant genome. Analysis of these junction sequences provides sequence-level information as to the following: the number of insertion loci including detection of unlinked, independently segregating, small DNA fragments; copy number; rearrangements, truncations, or deletions of the intended insertion DNA; and the presence of transformation plasmid backbone sequences. This molecular evidence from SbS analysis is used to characterize and select GM plants meeting optimal molecular characterization criteria. SbS technology has proven to be a robust event screening tool for use in a high-throughput molecular characterization environment.
机译:事件的分子表征是基因改造(GM)作物产品开发过程中不可或缺的一部分。传统上,这些事件的评估是通过聚合酶链反应(PCR)和Southern blot分析来完成的。 Southern印迹分析可能是耗时且相对昂贵的,并且不提供序列水平的细节。我们已经开发了一种基于序列的应用程序,即按序列测序的南部测序(SbS),它利用序列捕获与下一代测序(NGS)技术相结合,代替了用于高通量分子表征环境中事件选择的Southern blot分析。 SbS是通过将转基因植物的索引和合并全基因组DNA文库与生物素化探针杂交而设计的,该探针设计用于靶向用于在水池中产生事件的转化质粒的序列。该序列捕获过程丰富了从目标感兴趣区域(转化质粒DNA)获得的序列数据。利用与目标转化质粒序列相伴的与目标碱基相邻的DNA(称为下一个目标序列)的优势,数据分析可检测插入质粒中的质粒与基因组和质粒与质粒的连接。植物基因组。这些连接序列的分析提供了有关以下方面的序列水平信息:插入基因座的数量,包括未连接的,独立分离的小DNA片段的检测;副本编号;预期的插入DNA的重排,截短或缺失;以及转化质粒主链序列的存在。来自SbS分析的分子证据用于表征和选择符合最佳分子表征标准的转基因植物。 SbS技术已被证明是用于高通量分子表征环境的强大事件筛选工具。

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