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Detection of vector- and selectable marker-free transgenic maize with a linear GFP cassette transformation via the pollen-tube pathway

机译:通过花粉管途径通过线性GFP盒转化检测无载体和无选择标记的转基因玉米

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The pollen-tube pathway is feasible to transform vector- and selectable marker-free linear gene cassettes into plants to address the biosafety issues. However, its transformation frequency is low and the screening of selectable marker-free transformants by PCR analysis is time-consuming and expensive. In this study, a linear GFP cassette (Ubi-GFP-nos) flanked by 25bp T-DNA borders was transformed into maize via the pollen-tube pathway. The forepart of each maize ear was divided into five segments (segments I-V) at an interval of two rows of kernels. The segments that were most likely to contain transgenic kernels were identified by monitoring GFP expression in the immature embryos. A total of 21 ears were transformed with the linear GFP cassette. Seven out of 19 ears exhibited positive GFP expression in the immature embryos. Transgenic kernels were primarily identified in segments III and IV. A total of 121 plants derived from kernels located within segments III and IV of the remaining two ears were screened by PCR analysis. Six plants (4.96%) showed the presence of the GFP cassette. Southern blot analysis showed that the transgenic plants had simple integration patterns. The identification of transgenic kernels would facilitate PCR screening for marker-free transgenic plants.
机译:花粉管途径可将无载体​​和无选择标记的线性基因盒转化为植物,以解决生物安全问题。然而,其转化频率低,并且通过PCR分析筛选可选择的无标记转化体既费时又昂贵。在这项研究中,通过花粉管途径将侧翼为25bp T-DNA边界的线性GFP盒(Ubi-GFP-nos)转化为玉米。每个玉米穗的前部以两行谷粒的间隔分为五个部分(I-V段)。通过监测未成熟胚中的GFP表达,鉴定出最有可能含有转基因核的区段。用线性GFP盒转化总共21只耳朵。 19只耳朵中有7只在未成熟胚胎中显示GFP阳性表达。转基因玉米粒主要在片段III和IV中鉴定。通过PCR分析筛选了总共121株源自位于其余两只耳朵的第III和IV段内的仁的植物。六株植物(4.96%)显示了GFP盒的存在。 Southern印迹分析表明,转基因植物具有简单的整合模式。转基因谷粒的鉴定将有助于PCR筛选无标记的转基因植物。

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