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大麦中多代高频Ds转座促进了大基因组谷物中的基因标记。

High-frequency Ds remobilization over multiple generations in barley facilitates gene tagging in large genome cereals.

作者信息

Singh Jaswinder, Zhang Shibo, Chen Calvin, Cooper Laurel, Bregitzer Phil, Sturbaum Anne, Hayes Patrick M, Lemaux Peggy G

机构信息

Department of Plant and Microbial Biology, University of California, Berkeley, CA 94720, USA.

出版信息

Plant Mol Biol. 2006 Dec;62(6):937-50. doi: 10.1007/s11103-006-9067-1. Epub 2006 Sep 27.

Abstract

Transposable elements have certain advantages over other approaches for identifying and determining gene function in large genome cereals. Different strategies have been used to exploit the maize Activator/dissociation (Ac/Ds) transposon system for functional genomics in heterologous species. Either large numbers of independent Ds insertion lines or transposants (TNPs) are generated and screened phenotypically, or smaller numbers of TNPs are produced, Ds locations mapped and remobilized for localized gene targeting. It is imperative to characterize key features of the system in order to utilize the latter strategy, which is more feasible in large genome cereals like barley and wheat. In barley, we generated greater than 100 single-copy Ds TNPs and determined remobilization frequencies of primary, secondary, and tertiary TNPs with intact terminal inverted repeats (TIRs); frequencies ranged from 11.8 to 17.1%. In 16% of TNPs that had damaged TIRs no transposition was detected among progeny of crosses using those TNPs as parental lines. In half of the greater than 100 TNP lines, the nature of flanking sequences and status of the 11 bp TIRs and 8-bp direct repeats were determined. BLAST searches using a gene prediction program revealed that 86% of TNP flanking sequences matched either known or putative genes, indicating preferential Ds insertion into genic regions, critical in large genome species. Observed remobilization frequencies of primary, secondary, tertiary, and quaternary TNPs, coupled with the tendency for localized Ds transposition, validates a saturation mutagenesis approach using Ds to tag and characterize genes linked to Ds in large genome cereals like barley and wheat.

摘要

在大型基因组谷类作物中,转座元件在识别和确定基因功能方面比其他方法具有某些优势。人们已采用不同策略利用玉米激活子/解离子(Ac/Ds)转座子系统进行异源物种的功能基因组学研究。要么生成大量独立的Ds插入系或转座体(TNPs)并进行表型筛选,要么产生较少数量的TNPs,对Ds位置进行定位并使其重新激活以进行局部基因靶向。为了利用后一种策略(在大麦和小麦等大型基因组谷类作物中更可行),必须对该系统的关键特征进行表征。在大麦中,我们生成了100多个单拷贝Ds TNPs,并确定了具有完整末端反向重复序列(TIRs)的一级、二级和三级TNPs的重新激活频率;频率范围为11.8%至17.1%。在16%的TIRs受损的TNPs中,在以这些TNPs作为亲本系的杂交后代中未检测到转座。在100多个TNP系中的一半中,确定了侧翼序列的性质以及11 bp TIRs和8 bp直接重复序列的状态。使用基因预测程序进行的BLAST搜索显示,86%的TNP侧翼序列与已知或推定基因匹配,这表明Ds优先插入基因区域,这在大型基因组物种中至关重要。观察到的一级、二级、三级和四级TNPs的重新激活频率,再加上Ds局部转座的趋势,验证了一种使用Ds标记和表征与大麦和小麦等大型基因组谷类作物中Ds相关基因的饱和诱变方法。

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