In vitro culture initiation and regeneration of two highly productive clones of poplar

Q4 Agricultural and Biological Sciences
Yuliia Khoma, L. Khudolieieva, N. Rashydov, N. Kutsokon
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引用次数: 1

Abstract

In vitro shoot regeneration is a fast and reliable method for propagation of valuable tree genotypes and important step in genetic manipulations. This study aimed to establish an optimal in vitro culture initiation and regeneration protocol for highly productive poplar clones ‘Novoberlinska-3’ (Populus pyramidalis × P. laurifolia) and ‘Volosystoplidna’ (P. trichocarpa). In vitro culture was initiated either on MS (IM-MS) or WPM (IM-WPM) medium both containing BAP (0.2 mg.L-1) and IBA (0.1 mg.L-1). Results demonstrated that the best initiation medium for the clone ‘Volosystoplidna’ was IM-WPM on which 93.3 % of explants survived, while explants from ‘Novoberlinska-3’ better survived on IM-MS. After establishing both genotypes into aseptic culture, regeneration experiments were started using two types of explants, leaf and petioles, planted on callus induction medium containing 2iP (1.02 mg.L-1) and NAA (1.86 mg.L-1). Furthermore, microshoots were placed on shoot induction medium supplemented with 0.04 mg.L-1 thidiazuron, and then transferred on shoot elongation medium with 0.2 mg.L-1 BAP. Regeneration protocol showed better performance of poplar ‘Novoberlinska-3’, but it was also efficient for ‘Volosystoplidna’. Plant regeneration from leaf explants in the clone ‘Novoberlinska-3’ showed the highest regeneration percentage (92.3 %) and the number of shoots per explant (3.1), which significantly exceeded other explants. Our results showed a significant difference between the survivability of two clones during culture initiation. The differences in regeneration rates between the clones as well as leaf and petiole explants were also determined. Obtained aseptic cultures of highly productive poplar hybrids will be used in our further studies, especially for genetic transformation.
两个杨树高产无性系的离体培养启动与再生
离体茎再生是一种快速、可靠的有价值树种基因型繁殖方法,是遗传操作的重要步骤。本研究旨在建立杨树高产无性系“Novoberlinska-3”(Populus pyramidalis × P. laurifolia)和“volosystopplidna”(P. trichocarpa)的最佳离体培养启动和再生方案。在含有BAP (0.2 mg.L-1)和IBA (0.1 mg.L-1)的MS (IM-MS)或WPM (IM-WPM)培养基上进行离体培养。结果表明,‘volosystopplidna’克隆的最佳起始培养基为IM-WPM,其外植体成活率为93.3%,而‘Novoberlinska-3’的外植体在IM-MS上成活率更高。将两种基因型均建立为无菌培养后,将两种外植体叶片和叶柄分别置于含2iP (1.02 mg.L-1)和NAA (1.86 mg.L-1)的愈伤组织诱导培养基上进行再生实验。将微芽置于添加0.04 mg的诱导培养基上。L-1噻脲,然后以0.2 mg转移到芽伸长培养基上。l - 1软面包卷。再生方案对‘Novoberlinska-3’的再生效果较好,对‘volosystopplidna’的再生效果也较好。以叶片外植体再生植株的再生率最高(92.3%),每外植体再生芽数最高(3.1),显著高于其他外植体。结果表明,两个无性系在培养起始阶段的存活率存在显著差异。还测定了无性系之间以及叶片和叶柄外植体之间再生率的差异。获得的高产杨树杂种无菌培养物将用于我们进一步的研究,特别是遗传转化。
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来源期刊
Nova Biotechnologica et Chimica
Nova Biotechnologica et Chimica Agricultural and Biological Sciences-Food Science
CiteScore
0.60
自引率
0.00%
发文量
47
审稿时长
24 weeks
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