首页> 外文期刊>African Journal of Biotechnology >Nucellar embryogenesis and plantlet regeneration in monoembryonic and polyembryonic mango (Mangifera indica L.) cultivars
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Nucellar embryogenesis and plantlet regeneration in monoembryonic and polyembryonic mango (Mangifera indica L.) cultivars

机译:单胚和多胚芒果(Mangifera indica L.)品种的细胞胚胚发生和幼苗再生

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Biotic and abiotic stress particularly fungal diseases and salinity are major challenges facing mango cultivations in Oman. Micropropagation technique for multiplying disease resistant and salinity tolerant elite cultivars could be utilized to replace dead and infected plants in mango orchards but standardize in-vitro regeneration protocol via somatic embryogenesis is prerequisite. Nucellar tissues from immature mango fruits of monoembryonic cultivars Alphonso, Amrapali, Dashehari and Zafran, and polyembryonic cultivars Carabao and Turpentine were used as explants to induce somatic embryogenesis plantlets. Gamborg’s B5 macronutrients, Murashige and Skoog micronutrients, iron source, vitamins and organics were used as standard basal media for all types of media used at each stage of somatic embryo development and regeneration. Induction medium 2 containing 2 mg/l 2,4-Dichlorophenoxyacetic acid and 0.5 mg/l 6-Benzylaminopurine were induced highest percentage of primary somatic embryos for Alphonso (22.08%) while induction medium 3 having 1 mg/l 2,4- Dichlorophenoxyacetic acid? with sucrose 60 gm/l and induction medium 1 containing 1 mg/l 2,4- Dichlorophenoxyacetic acid and 0.25 mg/l 6-Benzylaminopurine induced highest percentage of primary somatic embryos in Carabao (29.17%) and Turpentine (42.71%) respectively. Maximum somatic embryo germination were achieved in germination medium 2 containing 0.1 mg/l Indole-3-acetic acid and 0.5 mg/l Gibberellic acid for Alphonso (7.34%) and Turpentine (3.34%) while for Carabao (18.59%) in germination medium 1 which does not contain any plant growth regulators. Germinated plantlets are surviving well in ex-vitro conditions after 4 months of transfer to greenhouse and survival rate of 66.66% for Alphonso, 26.68% for Carabao and 49.16% for Turpentine was obtained.
机译:生物和非生物胁迫,特别是真菌疾病和盐碱化是阿曼芒果种植面临的主要挑战。微繁殖技术可用于繁殖抗病和耐盐碱的优良品种,以替代芒果园中已死和受感染的植物,但是通过体细胞胚发生标准化体外再生方案是前提。来自单胚变种Alphonso,Amrapali,Dashehari和Zafran的未成熟芒果果实的核细胞组织以及多胚变种Carabao和Turpentine被用作外植体来诱导体细胞胚发生小植株。 Gamborg的B5大量营养素,Murashige和Skoog微量营养素,铁源,维生素和有机物被用作体细胞胚胎发育和再生各个阶段使用的所有类型培养基的标准基础培养基。含有2 mg / l 2,4-二氯苯氧基乙酸和0.5 mg / l 6-苄基氨基嘌呤的诱导培养基2诱导了Alphonso初生体细胞胚的最高百分比(22.08%),而诱导培养基3含有1 mg / l 2,4-二氯苯氧基乙酸酸?用蔗糖60克/升和诱导培养基1分别在卡拉宝(29.17%)和松节油(42.71%)中诱导最高百分比的初级体细胞胚,所述诱导培养基1包含1毫克/升的2,4-二氯苯氧基乙酸和0.25毫克/升的6-苄基氨基嘌呤。在含有0.1 mg / l吲哚-3-乙酸和0.5 mg / l赤霉素的发芽培养基2中,阿方索(7.34%)和松节油(3.34%)达到最大的体细胞胚发芽,而卡拉宝(Carabao)(18.59%)在发芽培养基中达到了最大的胚芽发芽率。 1不包含任何植物生长调节剂。转入温室4个月后,发芽的小苗在离体条件下存活良好,阿方索,卡拉宝和松节油的成活率分别为66.66%,26.68%和49.16%。

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