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首页> 外文期刊>Physiology and Molecular Biology of Plants >Co-culturing on dry filter paper significantly increased the efficiency of Agrobacterium-mediated transformations of maize immature embryos
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Co-culturing on dry filter paper significantly increased the efficiency of Agrobacterium-mediated transformations of maize immature embryos

机译:在干滤纸上共同培养显着提高了农杆菌介导的玉米未成熟胚的效率

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摘要

In the Agrobacterium tumefaciens-mediaied transformations of maize immature embryos (IEs), the common co-culturing media used are MS or N6-based (MC). Here, we used a novel co-culturing method in which maize 'Qi319' IEs inoculated with Agrobacterium-har-boring target vector were placed on dry filter paper (DC) in a petri dish. To compare the effects of the DC and MC co-culturing methods on transformation efficiency, we designed three experiments: (1) A. tumefaciens strain AGL1 independently carryingtwo plasmids, pXQD12 and pXQD70; (2) two A. tumefaciens strains, AGL1 and EHA105, carrying pXQD12; and (3) strains AGL1 and EHA105 each independently inoculated with pXQD12 and pXQD70 for different infiltration periods, 5, 10, 15, 20 and 25 min. We usedA. tumefaciens to inoculate IEs derived from maize ears 9-15 d after pollination, and then IEs were placed in petri dishes for co-culturing. The DC treatment significantly increased the percentage of IEs expressing green fluorescence protein (%GFP), indicating positive transformants. DC-treated IEs had ~ 3 to 4 times the %GFP compared with MC-treated IEs at 8 d after inoculation (3 d co-culture and 5 d restoration). The average regeneration frequency (%GFP positive regenerated calliof infected IEs) and stable transformation frequency (%GFP positive T0 plants of infected IEs) significantly increased with the DC treatment. Thus, the DC method may be used to develop a more efficient Agrobacterium-mediated transformation method for maize IEs.
机译:在玉米未成熟胚胎(IES)的肿瘤瘤瘤瘤瘤瘤转化中,所使用的常见共培养介质是MS或N6基(MC)。在此,我们使用了一种新的共培养方法,其中将用农杆菌 - 钻杆靶向载体接种的玉米'QI319'IE在培养皿中的干滤纸(DC)上。为了比较DC和MC共同培养方法对转化效率的影响,我们设计了三个实验:(1)A.Tumefaciens菌株AGL1独立携带Two质粒,PXQD12和PXQD70; (2)两种A. Tumefaciens菌株,AgL1和EHA105,携带PXQD12; (3)菌株AGL1和EHA105各自独立地接种PXQD12和PXQD70,用于不同的渗透周期,5,10,15,20和25分钟。我们使用过。在授粉之后,Tumefaciens接种来自玉米耳9-15d的IES,然后将IES放入培养皿中进行共同培养。 DC治疗显着增加了表达绿色荧光蛋白(%GFP)的IE的百分比,表明阳性转化体。在接种后,DC处理的IES在8d(3d共培养和5 d恢复)中,在8 d处与MC处理的IES相比具有约3至4倍。随着DC治疗,平均再生频率(IS%的GFP阳性再生Caliafated IES)和稳定的转化频率(受感染IES的GFP阳性T0植物%)显着增加。因此,DC方法可用于开发更有效的农杆菌介导的玉米IE的转化方法。

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