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首页> 外文期刊>Trees. Structure and Function >Analysis of re-integrated Ac element positions in the genome of Populus provides a basis for Ac/Ds-transposon activation tagging in trees
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Analysis of re-integrated Ac element positions in the genome of Populus provides a basis for Ac/Ds-transposon activation tagging in trees

机译:杨树基因组中重新整合的Ac元素位置的分析为树木中Ac / Ds-转座子激活标记提供了基础

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With a view to establish an efficient gene tagging system for forest tree species, we assessed the transposition behaviour of the maize transposable element Ac in poplar. In earlier work, we showed that new integration sites were often located within predicted or known coding sequences. However, somatic transposition behaviour of Ac with regard to conserved chromosome specificity or, more specifically, whether Ac transposition is restricted to the chromosome on which the primary insertion locus (donor) is located or whether it is able to pass chromosomal boundaries, remained unclear. To answer these questions, we took advantage of the publicly available Populus trichocarpa genome sequence (Phytozome v5.0; http://www.phytozome.net) and three 35S::Ac-rolC transgenic hybrid aspen lines to determine the flanking sequences of Ac re-integration sites for tissue sectors from which Ac had been excised. Only about one-third of the analysed re-integrations were positioned within the scaffold containing the primary Ac donor locus, and the majority of re-integrations were found scattered over many unlinked sites on other scaffolds confirming that Ac transposition in poplar does in fact cross chromosome boundaries. The majority of re-integration sites (57.1%) were found within or near coding regions demonstrating that Ac/Ds transposon tagging in poplar holds much promise for the efficient induction of mutants and functional genomics studies in forest tree species.
机译:为了建立一个有效的林木物种基因标签系统,我们评估了玉米转座因子Ac在杨树中的转座行为。在较早的工作中,我们表明新的整合位点通常位于预测或已知的编码序列内。然而,关于保守的染色体特异性,或者更确切地说,Ac的转座是否限于主要插入基因座(供体)所在的染色体,或者它是否能够通过染色体边界,Ac的体细胞转座行为仍不清楚。为了回答这些问题,我们利用了可公开获得的毛果杨基因组序列(Phytozome v5.0; http://www.phytozome.net)和三个35S :: Ac-rolC转基因杂种白杨品系来确定侧翼序列。从中切除了Ac的组织扇区的Ac重新整合位点。分析的重新整合中只有大约三分之一位于包含主要Ac供体基因座的支架内,并且发现大多数重新整合散布在其他支架上许多未连接的位点上,这确认了白杨中的Ac转运确实可以交叉染色体边界。在编码区内或编码区附近发现了大多数重新整合位点(57.1%),这表明杨树中的Ac / Ds转座子标签为在森林树种中有效诱导突变体和进行功能基因组学研究提供了广阔前景。

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