Micropropagación del lirio amazónico (Eucharis grandiflora Planch. & Linden) mediante organogénesis directa

F. A. Guerrero-Valencia, M. D. J. Juárez-Hernández, J. Ayala-Arreola, G. Ramírez-González
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引用次数: 1

Abstract

R ESUMEN : El lirio amazónico ( Eucharis grandiflora Planch. & Linden) es una planta geófita de uso ornamental y se propaga a través de la división de brotes adventicios. No obstante, este método es limitado, debido a que un bulbo produce solo dos o tres hijuelos después de un año de cultivo, por lo que el objetivo de esta investigación fue elaborar una metodología que permita la micropropagación de esta especie mediante organogénesis directa, y de este modo incrementar el número de plántulas nuevas en sistemas comerciales. Durante el establecimiento in vitro , se usaron explantes de 0.5 X 1.0 cm conformados por una porción del catáfilo y del disco basal y se cultivaron en el medio de Murashige & Skoog (MS) suplementado con 2.0 ml·L -1 de Plant Preservative Mixture (PPM™). Para la inducción y multiplicación de brotes adventicios se evaluó el efecto de la 6-bencil-aminopurina (BAP) en concentraciones de 0.0, 0.1, 0.3, 1.0 medium (MS) supplemented with 2.0 ml·L -1 of Plant Preservative Mixture (PPM™). For the induction and multiplication of adventitious shoots, the effect of 6-benzyl-aminopurine (BAP) was evaluated in concentrations of 0.0, 0.1, 0.3, 1.0 and 3.0 mg·L -1 and the number of new shoots every week was determined. The shoots obtained were subcultured in a medium without regulators to promote their development, and the sucrose content was evaluated in concentrations of 30 to 70 g·L -1 . For rooting, indol-3-acetic acid (AIA), indol-3-butyric acid (AIB), and α-naphthaleneacetic acid (ANA) were used, in concentrations of 0.3 and 1.0 mg·L -1 . Incubation conditions were a photoperiod of 16 light hours and 8 dark hours, at a temperature of 25 ± 2 ºC and a light intensity of 50 µmol·m -2 ·s -1 . The rooted shoots were acclimatized in pots with peat moss and were kept in a glass greenhouse with 50% shade. In the establishment, contamination of 30% was obtained. During multiplication, the use of 3.0 mg·L -1 BAP produced a maximum of 3.8 shoots per explant 35 days after culture. The best development of shoots was obtained with 50 g·L -1 of sucrose. In rooting, AIA, and AIB (0.3 mg·L -1 ) produced a greater root length. During acclimatization, 100% survival was obtained 50 days after transplanting and acclimatization.
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直接器官发生法繁殖亚马逊百合
R esumen:亚马逊百合(Eucharis grandiflora Planch&Linden)是一种观赏性的地理植物,通过不定芽的分裂传播。然而,这种方法是有限的,因为一个鳞茎在培养一年后只产生两三个幼崽,因此这项研究的目的是制定一种方法,允许通过直接器官发生进行该物种的微繁殖,从而增加商业系统中的新幼苗数量。在体外建立过程中,使用由Cataphil和基盘的一部分组成的0.5 x 1.0厘米的外植体,在Murashige&Skoog(MS)培养基中培养,并添加2.0 ml·L-1植物保护剂混合物(PPM)™). 在0.0、0.1、0.3、1.0培养基(MS)中添加2.0 ml·L-1植物保护剂混合物(PPM),评估了6-苄基氨基嘌呤(BAP)对不定芽诱导和繁殖的影响™). 对于不定芽的诱导和繁殖,在0.0、0.1、0.3、1.0和3.0 mg·L-1的浓度下评估了6-苄基氨基嘌呤(BAP)的影响,并确定了每周的新芽数量。所获得的快照在没有监管机构促进其发育的介质中进行了亚培养,并在30至70 g·L-1的浓度下对这些玫瑰的含量进行了评估。生根用吲哚-3-乙酸(AIA)、吲哚-3-丁酸(AIB)和α-萘乙酸(ANA),浓度分别为0.3和1.0 mg·L-1。培养条件为光周期为16小时和8小时,温度为25±2ºC,光强度为50µmol·m-2·s-1。根芽在装有泥炭藓的罐子里被驯化,并保存在一个有50%遮阳篷的玻璃温室里。在该机构中,获得了30%的污染。在繁殖过程中,培养35天后,使用3.0 mg·L-1 BAP每外植体最多可产生3.8个芽。射门的最佳发展是用50 g·L-1蔗糖获得的。在生根过程中,AIA和AIB(0.3 mg·L-1)产生了更大的根长。在适应期间,在移植和适应50天后获得了100%的存活率。
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