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Establishment of the Regeneration System for Vicia faba L.

机译:建立蚕豆蚕豆再生系统

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摘要

A reliable regeneration system for faba bean has been difficult to establish and therefore, the genetic improvement of Vicia faba L. was delayed. The paper describes a method of somatic embryo induction in callus of V. faba . Two Egyptian faba bean cultivars u27Giza 2u27 and u2724 Hytou27 were used. Callus was induced from epicotyls and shoot tips cultured on MS or Gamborg medium supplemented with 3% sucrose and 0.025% (w/v) for each of ascorbic and citric acid, 0.8% agar and different concentrations of 10 mg/l BAP, 0.5 mg/l of each NAA and 2,4-dichlorophenoxyacetic acid (M1) and 1 mg/l BAP and 0.5 mg/l NAA (M2) . The media with BAP, NAA and 2,4-D were optimal for embryogenic callus induction. Somatic embryos developed after transfer of the callus to 1/2 B5 medium with no plant growth regulators. There were various stages of somatic embryo development present including globular, heart-shaped, torpedo, and cotyledonary stages. Embryos developed into plantlets and plants were regenerated. RAPD analyses were performed to investigate the genetic stability of the regenerated plants obtained from different treatments and different explants. The cultivar Giza 2 exhibited more genetic stability than cultivar 24 Hyto. In conclusion, a regeneration system was established suitable for both gene transformation and the isolation of somaclonal mutants. The regeneration system will be used in order to improve the nutritional value of faba bean.
机译:难以建立可靠的蚕豆再生系统,因此,蚕豆的遗传改良被延迟。本文介绍了一种在蚕豆愈伤组织中诱导体细胞胚的方法。使用了两个埃及蚕豆栽培种 u27Giza 2 u27和 u2724 Hyto u27。由上胚轴和茎尖诱导愈伤组织,茎尖在MS或Gamborg培养基上培养,培养基中分别添加3%蔗糖和0.025%(w / v)的抗坏血酸和柠檬酸,0.8%琼脂和不同浓度的10 mg / l BAP,0.5 mg每升NAA和2,4-二氯苯氧基乙酸(M1)和每升BAP 1 mg / l和每升NAA 0.5 mg / l(M2)的每升。具有BAP,NAA和2,4-D的培养基最适合诱导胚性愈伤组织。愈伤组织转移至没有植物生长调节剂的1/2 B5培养基后,体细胞胚发育。存在着体细胞胚发育的各个阶段,包括球形,心形,鱼雷和子叶阶段。胚胎发育成小植株,并再生了植物。进行了RAPD分析,以研究通过不同处理和外植体获得的再生植物的遗传稳定性。吉萨2品种比24 Hyto品种表现出更高的遗传稳定性。总之,建立了一个既适合基因转化又适合体细胞克隆突变体分离的再生系统。将使用再生系统以提高蚕豆的营养价值。

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