首页> 美国卫生研究院文献>Scientifica >An Improved Micropropagation Protocol by Ex Vitro Rooting of Passiflora edulis Sims. f. flavicarpa Deg. through Nodal Segment Culture
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An Improved Micropropagation Protocol by Ex Vitro Rooting of Passiflora edulis Sims. f. flavicarpa Deg. through Nodal Segment Culture

机译:一种改进的西番莲离体生根的微繁协议。 F。黄皮果通过节段文化

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摘要

A procedure for rapid clonal propagation of Passiflora edulis Sims. f. flavicarpa Deg. (Passifloraceae) has been developed in this study. Nodal explants were sterilized with 0.1% HgCl2 and inoculated on Murashige and Skoog (MS) basal medium. The addition of 2.0 mgL−1 6-benzylaminopurine (BAP) to MS medium caused an extensive proliferation of multiple shoots (8.21 ± 1.13) primordial from the nodal meristems. Subculturing of these multiple shoots on the MS medium augmented with 1.0 mgL−1 of each BAP and Kinetin (Kin) was successful for the multiplication of the shoots in vitro with maximum numbers of shoots (25.73 ± 0.06) within four weeks of incubation. Shoots were rooted best (7.13 ± 0.56 roots/shoots) on half strength MS medium supplemented with 2.0 mgL−1 indole-3 butyric acid (IBA). All in vitro regenerated shoots were rooted by ex vitro method, and this has achieved 6-7 roots per shoot by pulsing of cut ends of the shoots using 200 as well as 300 mgL−1 IBA. The plantlets were hardened in the greenhouse for 4-5 weeks. The hardened plantlets were shifted to manure containing nursery polybags after five weeks and then transferred to a sand bed for another four weeks for acclimatization before field planting with 88% survival rate.
机译:一种西番莲快速克隆繁殖的程序。 F。黄皮果(西番莲科)已在这项研究中开发。将结节外植体用0.1%HgCl2灭菌,并接种在Murashige和Skoog(MS)基础培养基上。向MS培养基中添加2.0 mgL −1 6-苄氨基嘌呤(BAP)会导致结分生组织的原始芽大量繁殖(8.21±1.13)。将这些多枝芽在每个BAP和Kinetin(Kin)均增高1.0 mgL -1 的MS培养基上进行亚培养成功地繁殖了芽,并获得了最大芽数(25.73±0.06)孵育四个星期内。枝条最好在半强度MS培养基上(2.03 mgL -1 吲哚-3丁酸(IBA))生根(7.13±0.56根/芽)。所有离体再生芽都通过离体方法生根,通过使用200以及300 mgL -1 IBA对芽的切割末端进行脉冲处理,每根芽可获得6-7个根。将小植株在温室中硬化4-5周。在五周后,将已硬化的小苗转移到装有苗圃塑料袋的肥料中,然后再转移到沙床中再适应四周,以便在田间种植之前达到88%的成活率。

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