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RNA Interference-Based Transgenic Maize Resistant to Maize Dwarf Mosaic Virus

机译:基于RNA干扰的转基因玉米对玉米矮花叶病毒具有抗性

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Maize dwarf mosaic virus (MDMV) is a widespread pathogenic virus that causes serious loss of yield in maize (Zea mays). RNA interference (RNAi) triggered by hairpin RNA (hpRNA) transcribed from a transgenic inverted-repeat sequence is an effective way to defend against viruses in plants. In this study, an hpRNA expression vector containing a sense arm and an antisense arm of 150 bp separated by an intron of the maize actin gene was constructed to target the P1 protein (protease) gene of MDMV and used to transform Agrobacterium tumefaciens strain EHA105. The transformed Agrobacterium strain was used to transform maize embryonic calli isolated from immature embryos by an improved culture technique. In all, 46 plants were regenerated after stringent hygromycin B selection, and 18 of them were certified to be positive by PCR amplification. Of these positive plants, 13 were grown to produce offspring, and nine were identified by Southern blotting to have the transgene integrated with one or two copies. The resistance of three T-2 lines was evaluated in a field trial of dual MDMV inoculation in two environments and was found to be improved compared with the non-transformed control. The disease indexes of the transgenic plant lines h2, 13, and h1 were not significantly different from the highly resistant control line H9-21. The viral titers of the inoculated plants were detected by double antibody sandwich enzyme-linked immunosorbent assay (DAS-ELISA), and the result was in accord with the resistance evaluated in the field trial. The addition of uniconazole S3307 (0.25 mg l(-1)) and ABT root-promoting powder (0.5 mg l(-1)) showed a significant improvement of hardening in regenerated plantlets, which were stronger and generated a better fibrous root system than the control. This improvement could facilitate the transgenic operation of maize.
机译:玉米矮花叶病毒(MDMV)是一种广泛的致病性病毒,会导致玉米(Zea mays)的单产严重下降。从转基因反向重复序列转录的发夹RNA(hpRNA)触发的RNA干扰(RNAi)是防御植物病毒的有效方法。在这项研究中,构建了一个由玉米肌动蛋白基因的内含子分隔的150 bp的有义臂和反义臂的hpRNA表达载体,以靶向MDMV的P1蛋白(蛋白酶)基因,并用于转化根癌农杆菌菌株EHA105。通过改良的培养技术,将转化的农杆菌菌株用于转化从未成熟胚中分离的玉米胚愈伤组织。严格选择潮霉素B后,总共再生了46株植物,其中18株通过PCR扩增证明为阳性。在这些阳性植物中,有13个生长产生后代,通过Southern杂交鉴定了9个,使转基因整合了一个或两个拷贝。在两种环境中双重MDMV接种的田间试验中评估了3条T-2株系的抗性,发现与未转化的对照相比,该抗性得到了改善。转基因植物品系h2、13和h1的病害指数与高抗性对照品系H9-21没有显着差异。通过双抗体夹心酶联免疫吸附试验(DAS-ELISA)检测接种植物的病毒滴度,结果与田间试验的抗性相符。加入烯康唑S3307(0.25 mg l(-1))和ABT根系促进剂粉末(0.5 mg l(-1))可以显着改善再生小植株的硬化程度,其强度和产生的纤维根系均优于控制。这种改善可以促进玉米的转基因操作。

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