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Generating Novel Allelic Variation Through Activator Insertional Mutagenesis in Maize

机译:通过活化剂插入诱变在玉米中产生新的等位基因变异。

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摘要

The maize transposable element Activator (Ac) has been exploited as an insertional mutagen to disrupt, clone, and characterize genes in a number of plant species. To develop an Ac-based mutagenesis platform for maize, a large-scale mutagenesis was conducted targeting the pink scutellum1 locus. We selected 1092 Ac transposition events from a closely linked donor Ac, resulting in the recovery of 17 novel ps1 alleles. Multiple phenotypic classes were identified corresponding to Ac insertions in the 5′-UTR and coding region of the predicted Ps1 gene. To generate a stable allelic series, we employed genetic screens and identified 83 germinally heritable ps1 excision alleles. Molecular characterization of these excision alleles revealed a position-dependent bias in excision allele frequencies and the predominance of 7- and 8-bp footprint products. In total, 19 unique ps1 excision alleles were generated in this study, including several that resulted in weak mutant phenotypes. The analysis of footprint alleles suggests a model of Ac excision in maize that is consistent with recent in vitro studies of hAT element excision. Importantly, the genetic and molecular methods developed in this study can be extended to generate novel allelic variation at any Ac-tagged gene in the genome.
机译:玉米转座因子激活剂(Ac)已被用作插入诱变剂,以破坏,克隆和表征许多植物物种中的基因。为了开发针对玉米的基于Ac的诱变平台,针对粉红色scutellum1基因座进行了大规模诱变。我们从一个紧密相连的供体Ac中选择了1092个Ac换位事件,从而恢复了17个新颖的ps1等位基因。识别出多个表型类别,对应于在预测的Ps1基因的5'-UTR和编码区中的Ac插入。为了生成稳定的等位基因系列,我们采用了遗传筛选并鉴定了83个可生遗传的ps1切除等位基因。这些切除等位基因的分子表征揭示了切除等位基因频率中的位置依赖性偏差以及占优势的7和8 bp足迹产物。在这项研究中,总共产生了19个独特的ps1切除等位基因,包括几个导致弱突变表型的基因。足迹等位基因的分析表明玉米中Ac切除的模型与最近hAT元素切除的体外研究一致。重要的是,可以扩展本研究中开发的遗传和分子方法,以在基因组中任何带有Ac标签的基因上产生新的等位基因变异。

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