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Establishment of cell suspension cultures and plant regeneration in halophytic Leymus chinensis (Trin.)

机译:盐生羊草的细胞悬浮培养和植株再生的建立。

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The establishment of cell suspension culture from the callus of the halophytic Leymus chinensis (Trin.) LcWT07 line and plant regeneration from suspension-derived callus are described in this study for the first time. Solid medium containing Murashige and Shoog (MS) basic salt, 2,4-dichlorophenoxyacetic acid (2,4-D, 2.0 mg l−1), and L-glumatic acid (5.0 mg l−1) induced the highest rate of cell division among various solid media with various concentrations of 2,4-D, with good distribution of different mature seeds derived-callus types. Liquid medium with the same hormone distribution was therefore, used for cell suspension culture of L. chinensis. A slight increase in relative water contents was observed in suspension-derived callus than Type 1 callus, but not Type 2 to 4 calli. Over a 30 d-suspension culture, high growth rates were observed, and great amounts of biomass were accumulated, with 71.07% average daily increment and 22.32-fold total fresh weight increment. The potential of plant regeneration was induced on solid medium containing MS basic salt, 0.2 mg l−1 α-naphthalene acetic acid (NAA), 2.0 mg l−1 kinetin (Kn), and 2.0 g l−1 casamino acid, with faster somatic embryogenesis than that using Type 1 callus. Rooting of all regenerated shoots was successfully performed on half-strength MS medium. This procedure provide basis for morphological, biochemical and molecular studies of the nature of somatic embryogenesis from single cell to whole plant, and shorten the process of somatic embryogenesis.
机译:本研究首次描述了盐生羊草(Trin。)LcWT07系愈伤组织的细胞悬浮培养的建立和悬浮来源愈伤组织的植物再生。包含Murashige和Shoog(MS)碱性盐,2,4-二氯苯氧基乙酸(2,4-D,2.0 mg l -1 )和L-谷氨酸(5.0 mg lsup)的固体培养基> -1 )在具有不同浓度的2,4-D的各种固体培养基中诱导了最高的细胞分裂速率,并且不同成熟种子衍生的愈伤组织类型均具有良好的分布。因此,具有相同激素分布的液体培养基被用于中华乳杆菌的细胞悬浮培养。在悬浮液衍生的愈伤组织中观察到相对水含量比1型愈伤组织略有增加,但没有观察到2至4型愈伤组织。在30 d的悬浮培养中,观察到高生长速率,并积累了大量生物量,平均日增重为71.07%,总鲜重增重为22.32倍。在含有MS碱性盐,0.2 mg l -1 α-萘乙酸(NAA),2.0 mg l -1 动蛋白的固体培养基上诱导植物再生的潜力( Kn)和2.0 gl -1 酪蛋白氨基酸,与使用1型愈伤组织相比,具有更快的体细胞胚发生能力。所有再生芽的生根均在半强度MS培养基上成功进行。该程序为从单细胞到整个植物的体细胞胚发生的性质的形态学,生化和分子研究提供了基础,并缩短了体细胞胚发生的过程。

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