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Evidence for stable transformation of wheat by floral dip in Agrobacterium tumefaciens

机译:根癌农杆菌中浸花稳定转化小麦的证据

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Hexaploid wheat, one of the world’s most important staple crops, remains a challenge for genetic transformation. We are developing a floral transformation protocol for wheat that does not require tissue culture. This paper presents three transformants in the hard red germplasm line Crocus that have been characterized thoroughly at the molecular level over three to six generations. Wheat spikes at the early boot stage, i.e. the early, mid or late uninucleate microspore stages, were immersed in an infiltration medium of strain C58C1 harboring pDs(Hyg)35S, or strain AGL1 harboring pBECKSred. pDs(Hyg)35S contains the NPTII and hph selectable markers, and transformants were detected using paromomycin spray at the whole plant level, NPTII ELISAs, or selection on medium with hygromycin. Strain AGL1, harboring pBECKSred, which contains the maize anthocyanin regulators, Lc and C1, and the NPTII gene, was also used to produce a Crocus transformant. T1 and T2 seeds with red embryos were selected; T1 and T2 plants were screened by sequential tests for paromomycin resistance and NPTII ELISAs. The transformants were low copy number and showed Mendelian segregation in the T2. Stable transmission of the transgenes over several generations has been demonstrated using Southern analysis. Gene expression in advanced progeny was shown using Reverse Transcriptase-PCR and ELISA assays for NPTII protein expression. This protocol has the potential to reduce the time and expense required for wheat transformation.
机译:六倍体小麦是世界上最重要的主粮之一,仍然是遗传转化的挑战。我们正在为不需要组织培养的小麦开发花卉转化方案。本文介绍了硬红种质番红花系番红花中的三个转化体,这些转化体已在三到六代的分子水平上得到了充分表征。将处于启动阶段早期,即早期,中期或晚期单核小孢子阶段的小麦穗浸入带有pDs(Hyg)35S的菌株C58C1或带有pBECKSred的菌株AGL1的浸润培养基中。 pDs(Hyg)35S含有NPTII和hph选择标记,转化株的检测采用全植物水平的巴龙霉素喷雾剂,NPTII ELISA或在潮霉素培养基上进行选择。含有pBECKSred的AGL1菌株也用于生产番红花转化体,该菌株包含玉米花色苷调节剂Lc和C1以及NPTII基因。选择具有红色胚胎的T1和T2种子;通过序贯试验对巴龙霉素抗性和NPTII ELISA筛选了T1和T2植物。转化体的拷贝数低,并且在T2中显示孟德尔偏析。使用Southern分析已经证明了转基因在几代中的稳定传播。使用逆转录酶-PCR和ELISA测定法显示了NPTII蛋白表达在高级子代中的基因表达。该协议有可能减少小麦转化所需的时间和费用。

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