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首页> 外文期刊>Journal of Medicinal Plants Research >Evaluation of genetic fidelity of in vitro propagated shampoo ginger (Zingiber zerumbet (L.) Smith) using DNA based markers
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Evaluation of genetic fidelity of in vitro propagated shampoo ginger (Zingiber zerumbet (L.) Smith) using DNA based markers

机译:使用基于DNA的标记评估体外繁殖的洗发姜(Zingiber zerumbet(L.)Smith)的遗传保真度

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Drug yielding potential of shampoo ginger (Zingiber zerumbet?(L.) Smith) is due to the presence of important phytoconstituent such as Zerumbone, which is currently being explored for its effects on cancer and HIV. Slow multiplication rate, high susceptibility to rhizome rot and leaf spot disease restricted the availability of the wild gingers. Thus, a protocol has been developed for?in vitro?propagation of Z.?zerumbet?using sprouted bud explants from rhizome. The explants in MS media with 4 mg/L benzyl adenine, 1 mg/L indole-3-acetic acid showed highest percentage of response, that is, 93.8%. The aseptic shoots of?Z.?zerumbet?were formed with 5 multiple shoots on MS media with 3 mg/L?benzyl adenine and 1 mg/L?indole-3-acetic acid and 100 mg/L?adenine sulfate.?In vitro?grown plantlets of?Z. zerumbet?could be conserved in MS media containing 0.5 mg dm-3?of benzyladenine and 60 mg/L?of sucrose subcultured at an interval of eight months. Survival of?in vitro?conserved plants on multiplication media was 85%. Genetic stability of micropropagated clones were periodically evaluated at an interval of 6 months up to 30 months in culture using random amplified polymorphic DNA (RAPD) and inter simple sequence repeat (ISSR) analysis and genetic uniformity in all regenerants was confirmed.
机译:香波姜(Zingiber zerumbet?(L.)Smith)的产药潜力是由于存在重要的植物成分,例如Zerumbone,目前正在研究其对癌症和HIV的作用。繁殖速度慢,对根茎腐烂和叶斑病的敏感性高,限制了野生生姜的供应。因此,已经开发了一种使用来自根茎的发芽的外植体在体外进行Z.zumbetbet的繁殖的方案。 MS培养基中含有4 mg / L苄基腺嘌呤,1 mg / L吲哚-3-乙酸的外植体显示出最高的响应百分比,即93.8%。在含有3 mg / L苄基腺嘌呤和1 mg / L吲哚-3-乙酸和100 mg / L硫酸腺嘌呤的MS培养基上,通过5次多次芽形成Z.Zerumbet的无菌芽。 Z的离体生长小植株。 zerumbet™可以在含有0.5 mg dm-3?苄基腺嘌呤和60 mg / L?蔗糖的MS培养基中保存,间隔八个月。体外保存的植物在繁殖培养基上的存活率为85%。使用随机扩增多态性DNA(RAPD)和简单序列重复(ISSR)分析,在培养中的6个月至30个月的间隔中定期评估微繁殖克隆的遗传稳定性,并确认所有再生子的遗传均一性。

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