Iantcheva Anelia, Chabaud Mireille, Cosson Viviane, Barascud Marielle, Schutz Bernadette, Primard-Brisset Catherine, Durand Patricia, Barker David G, Vlahova Mariana, Ratet Pascal
AgroBioInstitute, bul. Dragan Tzankov 8, 1164 Sofia, Bulgaria.
Plant Cell Rep. 2009 Oct;28(10):1563-72. doi: 10.1007/s00299-009-0755-6. Epub 2009 Aug 18.
Insertion mutant collections are powerful tools for genetic studies in plants. Although large-scale insertional mutagenesis using T-DNA is not feasible in legumes, the Tnt1 tobacco retrotransposon can be used as a very efficient mutagen in the Medicago truncatula R108 genotype. In this article, we show that Tnt1 can also be exploited to create insertional mutants via transformation and/or regeneration in the reference cultivar Jemalong. Tnt1 insertional mutagenesis in Jemalong following Agrobacterium tumefaciens-mediated transformation was found to be very efficient, with an average of greater than 15 insertions/line. In contrast, regeneration using low-copy transgenic starter lines resulted in a highly variable rate of new Tnt1 insertions. With the goal of increasing the number of additional Tnt1 insertions during regeneration of starter lines, we have compared the insertion frequencies for a number of different regeneration protocols. In addition, we have been able to show that sucrose-mediated osmotic shock preceding regeneration significantly increases the transposition frequency. Under optimal conditions, 95% of the regenerated Jemalong plants possess new insertions.
插入突变体库是植物遗传学研究的有力工具。虽然利用T-DNA进行大规模插入诱变在豆科植物中不可行,但Tnt1烟草反转录转座子可作为蒺藜苜蓿R108基因型中一种非常有效的诱变剂。在本文中,我们表明Tnt1也可用于通过在参考品种Jemalong中转化和/或再生来创建插入突变体。发现在根癌农杆菌介导的转化后,Jemalong中的Tnt1插入诱变非常有效,平均每个株系有超过15个插入。相比之下,使用低拷贝转基因起始株系进行再生导致新Tnt1插入的频率高度可变。为了增加起始株系再生过程中额外Tnt1插入的数量,我们比较了多种不同再生方案的插入频率。此外,我们已经能够证明再生前蔗糖介导的渗透休克显著提高了转座频率。在最佳条件下,95%的再生Jemalong植株具有新的插入。
