Ling Huang, Yuting Zhang, Can Zhou, Fangwei Zhu, Zhuo Lv, Shuguang Wang
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MS medium containing 3 mg L<sup>−1</sup> BA, 0.5 mg L<sup>−1</sup> KT, 0.10 mg L<sup>−1</sup> NAA and 25 g L<sup>−1</sup> sucrose showed the highest multiplication rates, and those supplemented with 5 mg L<sup>−1</sup> BA, 0.5 mg L<sup>−1</sup> KT, 1.0 mg L<sup>−1</sup> NAA and 25 g L<sup>−1</sup> sucrose were the best for shoot proliferation. 1/2 MS medium supplemented with the hormone combination of 0.1 mg L<sup>−1</sup> IBA, and 1.0 mg L<sup>−1</sup> NAA was optimal for root induction. For plantlets regeneration from the single nodal buds of multiple shoots, the optimal medium was MS + BA 2.0 mg L<sup>−1</sup> + NAA 0.5 mg L<sup>−1</sup> for shoot multiplication and 1/2MS + BA 0.1 mg L<sup>−1</sup> + NAA 2.0 mg L<sup>−1</sup> for root induction. The optimal acclimatization medium was vermiculite + perlite (1:1). This study firstly and systematically established the micropropagation system of D. brandisii by using the seeds and nodal buds of the multiple shoots as explants. 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引用次数: 0
摘要
作为一种著名的、广泛种植的笋用竹种,很少有人关注烙竹的微繁殖研究。本研究通过种子和多梢节芽的离体截取,建立了一种高效的白竹微繁殖系统。采用正交试验筛选出诱导多芽、体外增殖和体外诱导生根的最佳消毒时间和激素组合。结果表明,最佳消毒时间为 10 分钟。含有 3 mg L-1 BA、0.5 mg L-1 KT、0.10 mg L-1 NAA 和 25 g L-1 蔗糖的 MS 培养基繁殖率最高,而添加 5 mg L-1 BA、0.5 mg L-1 KT、1.0 mg L-1 NAA 和 25 g L-1 蔗糖的 MS 培养基芽增殖效果最好。添加了 0.1 mg L-1 IBA 和 1.0 mg L-1 NAA 激素组合的 1/2 MS 培养基对根系诱导效果最佳。对于多芽单节芽的小植株再生,最佳培养基是 MS + BA 2.0 mg L-1 + NAA 0.5 mg L-1 用于芽增殖,1/2MS + BA 0.1 mg L-1 + NAA 2.0 mg L-1 用于根诱导。最佳适应性培养基为蛭石+珍珠岩(1:1)。本研究首次系统地建立了白兰地的微繁殖系统,以种子和多生芽的节芽为外植体。由多肉芽的节芽诱导出的多肉芽可进一步提高微繁殖效率。
Establishment of micropropagation system of Dendrocalamus brandisii
As a famous and widely planted shoot-use bamboo species, few researches have been focused on the micropropagation of Dendrocalamus brandisii. This study established an efficient micropropagation system of D. brandisii through seeds and cutoff nodal buds from the multiple shoots in vitro. The orthogonal tests were employed to screen out the optimal disinfection time and hormone combination for multiple shoot induction, proliferation in vitro and root induction in vitro. The results showed that the optimal disinfection time was 10 min. MS medium containing 3 mg L−1 BA, 0.5 mg L−1 KT, 0.10 mg L−1 NAA and 25 g L−1 sucrose showed the highest multiplication rates, and those supplemented with 5 mg L−1 BA, 0.5 mg L−1 KT, 1.0 mg L−1 NAA and 25 g L−1 sucrose were the best for shoot proliferation. 1/2 MS medium supplemented with the hormone combination of 0.1 mg L−1 IBA, and 1.0 mg L−1 NAA was optimal for root induction. For plantlets regeneration from the single nodal buds of multiple shoots, the optimal medium was MS + BA 2.0 mg L−1 + NAA 0.5 mg L−1 for shoot multiplication and 1/2MS + BA 0.1 mg L−1 + NAA 2.0 mg L−1 for root induction. The optimal acclimatization medium was vermiculite + perlite (1:1). This study firstly and systematically established the micropropagation system of D. brandisii by using the seeds and nodal buds of the multiple shoots as explants. Multiple shoots induced from the cutoff nodal buds of the multiple shoots could further expand the micropropagation efficiency.
期刊介绍:
The Brazilian Journal of Botany is an international journal devoted to publishing a wide-range of research in plant sciences: biogeography, cytogenetics, ecology, economic botany, physiology and biochemistry, morphology and anatomy, molecular biology and diversity phycology, mycology, palynology, and systematics and phylogeny.
The journal considers for publications original articles, short communications, reviews, and letters to the editor.
Manuscripts describing new taxa based on morphological data only are suitable for submission; however information from multiple sources, such as ultrastructure, phytochemistry and molecular evidence are desirable.
Floristic inventories and checklists should include new and relevant information on other aspects, such as conservation strategies and biogeographic patterns.
The journal does not consider for publication submissions dealing exclusively with methods and protocols (including micropropagation) and biological activity of extracts with no detailed chemical analysis.