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Micropropagation of Scaevola —Australian native of ornamental horticulture

机译:Scaevola的微繁殖-观赏园艺的澳大利亚原住民

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Summary. A number of commercially available cultivars of Scaevola aemula, S. albida, S. phlebopetala, S. striata and material collected from the wild of S. glandulifera, S. hookeri and S. ramonissima were successfully propagated by tissue culture. Shoot segments 3–4 cm in length were multiplied in Murashige and Skoog medium without hormones. Addition of 25–150 µmol kinetin/L in the micropropagation medium of S. aemula and S. phlebopetala resulted in the formation of deformed shoots. Tissue cultured shoots rooted in hormone-free medium in 4–6 weeks. Indole-3-butyric acid (10–20 µmol/L) had an effect on rate of root initiation of S. phlebopetala but not on percentage of rooting. A high survival percentage (>95%) was obtained when plants were transferred to soil under glasshouse conditions indicating that micropropagation of Scaevola is feasible.
机译:摘要。通过组织培养成功地繁殖了许多Scaevola aemula,S。albida,S。phlebopetala,S。striata和从野生S. glandulifera,S。hookeri和S. ramonissima收集的材料。在没有激素的Murashige和Skoog培养基中将长度为3-4 cm的芽段繁殖。在沙蒿和竹假单胞菌的微繁培养基中添加25–150 µmol激动素/ L,导致畸形芽形成。组织培养的芽在4-6周内根植于无激素的培养基中。吲哚-3-丁酸(10–20 µmol / L)对竹假单胞菌的根起始速率有影响,但对生根百分比没有影响。当植物在温室条件下转移到土壤中时,可获得很高的成活率(> 95%),这表明Scaevola的微繁是可行的。

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