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A protocol for efficiently retrieving and characterizing flanking sequence tags (FSTs) in Brachypodium distachyon T-DNA insertional mutants

机译:一种有效检索和表征曲霉蛙T-DNA插入突变体中侧翼序列标签(FST)的协议

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Brachypodium distachyon is emerging as a new model system for bridging research into temperate cereal crops, such as wheat andbarley, and for promoting research in novel biomass grasses. Here, we provide an adapter ligation PCR protocol that allows the large-scale characterization of T-DNA insertions into the genome of Brachypodium. The procedure enables the retrieval and mappingof the regions flanking the right and left borders (RB and LB) of the T-DNA inserts and consists of five steps: extraction andrestriction digest of genomic DNA; ligation of an adapter to the genomic DNA; PCR amplification of the regions flanking the T-DNA insert(s) using primers specific to the adapter and the T-DNA; sequencing of the PCR products; and identification of the flanking sequence tags (FSTs) characterizing the T-DNA inserts. Analyzing the regions flanking both the LB and RB of the T-DNA insertssignificantly improves FST retrieval and the frequency of mutant lines for which at least one FST can be identified. It takes approximately 16 or 10 d for a single person to analyze 96 T-DNA lines using individual or batch procedures, respectively.
机译:短枝曲霉(Brachypodium distachyon)成为一种新的模型系统,可将研究与温带谷物作物(例如小麦和大麦)衔接起来,并促进新型生物质草的研究。在这里,我们提供了一个衔接子连接PCR协议,该协议允许大规模表征T-DNA插入腕足动物基因组中。该程序能够检索和定位T-DNA插入片段左右边界(RB和LB)两侧的区域,并包括五个步骤:基因组DNA的提取和限制酶切;衔接子与基因组DNA的连接;使用对衔接子和T-DNA有特异性的引物,PCR扩增T-DNA插入片段侧翼的区域; PCR产物的测序;并鉴定了表征T-DNA插入片段的侧翼序列标签(FST)。分析T-DNA插入片段的LB和RB两侧的区域显着改善了FST检索和突变株的频率,可以鉴定出至少一个FST。一个人分别使用单独或批处理过程分析96条T-DNA系大约需要16或10 d。

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