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首页> 外文期刊>Tree Physiology >Genetic transformation of European chestnut somatic embryos with a native thaumatin-like protein (CsTL1) gene isolated from Castanea sativa seeds
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Genetic transformation of European chestnut somatic embryos with a native thaumatin-like protein (CsTL1) gene isolated from Castanea sativa seeds

机译:欧洲栗板栗体细胞胚的遗传转化(从栗树种子中分离出一种类似天然甜蛋白类似蛋白(CsTL1)的基因)

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摘要

The availability of a system for direct transfer of antifungal candidate genes into European chestnut (Castanea sativa Mill.) would offer an alternative approach to conventional breeding for production of chestnut trees tolerant to ink disease caused by Phytophthora spp. For the first time, a chestnut thaumatin-like protein gene (CsTL1), isolated from chestnut cotyledons, has been overexpressed in three chestnut somatic embryogenic lines. Transformation experiments have been performed using an Agrobacterium tumefaciens Smith and Townsend vector harboring the neomycin phosphotransferase (NPTII) selectable and the green fluorescent protein (EGFP) reporter genes. The transformation efficiency, determined on the basis of the fluorescence of surviving explants, was clearly genotype dependent and ranged from 32.5% in the CI-9 line to 7.1% in the CI-3 line. A total of 126 independent transformed lines were obtained. The presence and integration of chestnut CsTL1 in genomic DNA was confirmed by polymerase chain reaction (PCR) and Southern blot analyses. Quantitative real-time PCR revealed that CsTL1 expression was up to 13.5-fold higher in a transgenic line compared with its corresponding untransformed line. In only one of the 11 transformed lines tested, expression of the CsTL1 was lower than the control. The remaining 115 transformed lines were successfully subjected to cryopreservation. Embryo proliferation was achieved in all of the transgenic lines regenerated and the transformed lines showed a higher mean number of cotyledonary stage embryos and total number of embryos per embryo clump than their corresponding untransformed lines. Transgenic plants were regenerated after maturation and germination of transformed somatic embryos. Furthermore, due to the low plantlet conversion achieved, axillary shoot proliferation cultures were established from partially germinated embryos (only shoot development), which were multiplied and rooted according to procedures already established. Transgenic plants were acclimatized and grown in a greenhouse. No phenotypic differences were found with control plants, suggesting no potential cytotoxic effects of the green fluorescent protein. The results reported in the present work could be considered as a first step toward the production of fungal-disease tolerant cisgenic chestnut plants.
机译:将抗真菌候选基因直接转移到欧洲板栗中的系统(Castanea sativa Mill。)的可用性将提供常规育种的替代方法,以生产耐受由疫霉属植物引起的墨病的板栗树。首次从栗子叶中分离出的栗子thaumatin样蛋白基因(CsTL1)在三种栗子体细胞胚发生系中过表达。已经使用携带可选择的新霉素磷酸转移酶(NPTII)和绿色荧光蛋白(EGFP)报道基因的根癌农杆菌Smith和Townsend载体进行了转化实验。根据存活的外植体的荧光确定的转化效率显然是基因型依赖性的,范围从CI-9系的32.5%到CI-3系的7.1%。总共获得了126条独立的转化株。通过聚合酶链反应(PCR)和Southern印迹分析证实了栗子CsTL1在基因组DNA中的存在和整合。实时定量PCR分析显示,与相应的未转化株系相比,转基因株系中CsTL1的表达高13.5倍。在测试的11个转化株中,只有1个的CsTL1的表达低于对照。其余的115个转化品系成功进行了低温保存。在所有再生的转基因品系中都实现了胚胎增殖,并且与相应的未转化品系相比,转化的品系显示出更高的平均子叶期胚数和每个胚块的胚总数。在转化的体细胞胚成熟和萌发之后,再生转基因植物。此外,由于实现的低植株转化,从部分发芽的胚胎中建立了腋生芽增殖培养物(仅芽发育),并根据已经建立的程序对其进行了繁殖和生根。使转基因植物适应环境并在温室中生长。对照植物未发现表型差异,表明绿色荧光蛋白没有潜在的细胞毒性作用。本工作中报道的结果可被视为迈向抗真菌病顺生板栗植物生产的第一步。

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