首页> 外文期刊>Plant Cell, Tissue and Organ Culture: An International Journal on in Vitro Culture of Higher Plants >Agrobacterium-mediated transformation of Hyacinthus orientalis with thaumatin II gene to control fungal diseases
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Agrobacterium-mediated transformation of Hyacinthus orientalis with thaumatin II gene to control fungal diseases

机译:农杆菌介导的thaumatin II基因介导的风信子转化控制真菌病

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Transgenic plants of hyacinth (Hyacinthus orientalis L.) cvs. Edisson and Chine Pink have been obtained by Agrobacterium-mediated transformation. Leaf explants of the both hyacinth cultivars regenerated shoots on MS medium containing 2.2 mu M BAP and 0.3 mu M NAA at a frequency of 95%. A. tumefaciens strain CBE21 carrying binary vector pBIThau35 was used for transformation. Plasmid pBIThau35 has been produced by cloning preprothaumatin II cDNA into pBI121 instead of uidA gene. Inoculated leaf explants formed calli and shoots at high frequency on selective medium with 100 mg l(-1) kanamycin. Four hyacinth transgenic lines of cv. Chine Pink and one line of cv. Edisson have been selected on medium containing 200 mg l(-1) kanamycin. The insertion of thaumatin II gene into hyacinth genome has been confirmed by PCR-analysis. All transgenic plants expressed substantial amounts of thaumatin II (between 0.06 and 0.28% of the total soluble protein). Hyacinth transgenic lines were assayed for resistance to the pathogenic fungi Fusarium culmorum and Botrytis cinerea. There were no significant differences between nontransformed control and transgenic leaves of both cultivars. At the same time the bulbs of the transgenic line H7401 cv. Chine Pink showed the higher level of resistance to B. cinerea, the bulbs of the transgenic line Y7404 were more resistant to F. culmorum. In both cases the signs of the fungal disease were developed more slowly. The resistance of the bulbs cv. Edisson line to these fungi was not changed. All transgenic hyacinth plant were successfully transferred to soil for further evaluation.
机译:风信子(Hyacinthus Orientalis L.)cvs的转基因植物。 Edisson和Chine Pink已通过农杆菌介导的转化获得。两个风信子品种的叶片外植体均在含有2.2μMBAP和0.3μMNAA的MS培养基上以95%的频率再生芽。携带二元载体pBIThau35的根癌农杆菌CBE21用于转化。质粒pBIThau35是通过将前原蛋白II cDNA而非uidA基因克隆到pBI121中而产生的。接种的叶外植体在含有100 mg l(-1)卡那霉素的选择性培养基上形成愈伤组织和芽,频率很高。简历的四个风信子转基因品系。 Chine Pink和一线简历。已在含有200 mg l(-1)卡那霉素的培养基上选择了Edisson。通过PCR分析已证实将thaumatin II基因插入风信子基因组中。所有转基因植物均表达大量的奇异果甜蛋白II(占可溶性蛋白总量的0.06-0.28%)。测定风信子转基因品系对病原真菌镰刀镰刀菌和灰葡萄孢的抗性。两个品种的非转化对照和转基因叶片之间没有显着差异。同时,转基因系H7401 cv的鳞茎。 Chine Pink表现出对灰葡萄孢的较高抗性,转基因品系Y7404的鳞茎对小球藻的抗性更高。在这两种情况下,真菌病的体征发展都比较缓慢。灯泡的电阻cv。埃迪森线对这些真菌没有改变。所有的转基因风信子植物都成功转移到土壤中进行进一步评估。

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