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用于大麦功能基因组学的定位Ds/T-DNA插入位点

Mapped Ds/T-DNA launch pads for functional genomics in barley.

作者信息

Zhao Tiehan, Palotta Margaret, Langridge Peter, Prasad Manoj, Graner Andreas, Schulze-Lefert Paul, Koprek Thomas

机构信息

Department of Plant-Microbe Interactions, Max Planck Institute for Plant Breeding Research, Carl-von-Linné Weg 10, 50829 Cologne, Germany.

出版信息

Plant J. 2006 Sep;47(5):811-26. doi: 10.1111/j.1365-313X.2006.02831.x. Epub 2006 Aug 2.

DOI:10.1111/j.1365-313X.2006.02831.x
PMID:16889649
Abstract

A system for targeted gene tagging and local saturation mutagenesis based on maize transposable elements (Ac/Ds) was developed in barley (Hordeum vulgare L.). We generated large numbers of transgenic barley lines carrying a single copy of the non-autonomous maize Ds element at defined positions in the genome. Independent Ds lines were either generated by activating Ds elements in existing single-copy lines after crossing with AcTPase-expressing plants or by Agrobacterium-mediated transformation. Genomic DNA flanking Ds and T-DNA insertion sites from over 200 independent lines was isolated and sequenced, and was used for a sequence based mapping strategy in a barley reference population. More than 100 independent Ds insertion sites were mapped and can be used as launch pads for future targeted tagging of genes in the vicinity of the insertion sites. Sequence analysis of Ds and T-DNA flanking regions revealed a sevenfold preference of both mutagens for insertion into non-redundant, gene-containing regions of the barley genome. However, whilst transposed Ds elements preferentially inserted adjacent to regions with a high number of predicted and experimentally validated matrix attachment regions (nuclear MARs), this was not the case for T-DNA integration sites. These findings and an observed high transposition frequency from mapped launch pads demonstrate the future potential of gene tagging for functional genomics and gene discovery in barley.

摘要

在大麦(Hordeum vulgare L.)中开发了一种基于玉米转座元件(Ac/Ds)的靶向基因标记和局部饱和诱变系统。我们生成了大量转基因大麦品系,这些品系在基因组的特定位置携带单个拷贝的非自主玉米Ds元件。独立的Ds品系要么通过与表达AcTPase的植物杂交后激活现有单拷贝品系中的Ds元件来产生,要么通过农杆菌介导的转化来产生。从200多个独立品系中分离并测序了Ds和T-DNA插入位点两侧的基因组DNA,并将其用于大麦参考群体中的基于序列的定位策略。绘制了100多个独立的Ds插入位点,可将其用作未来对插入位点附近基因进行靶向标记的起始点。对Ds和T-DNA侧翼区域的序列分析表明,两种诱变剂在插入大麦基因组的非冗余、含基因区域方面都有七倍的偏好。然而,虽然转座的Ds元件优先插入到预测和实验验证的大量基质附着区域(核MARs)附近的区域,但T-DNA整合位点并非如此。这些发现以及从绘制的起始点观察到的高转座频率证明了基因标记在大麦功能基因组学和基因发现方面的未来潜力。

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