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Micropropagation Shortens the Time to Blooming of Begonia montaniformis x Begonia ningmingensis var. bella F1 Progeny

机译:微扑通缩短了秋山蒙内叶X秋海棠宁明森var的时间。 贝拉F1后代

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Begonia montaniformis x Begonia ningmingensis var. bella hybrids have high ornamental potential. Hence, the aim of this study was to determine the optimal conditions for the micropropagation of a Begonia montaniformis x Begonia ningmingensis var. bella F-1 progeny by using various concentrations of plant growth regulators (PGRs) and varying light spectra in half-strength Murashige and Skoog (1/2 MS) medium. The results showed that the explant regeneration was optimal when the lamina was incubated in a medium supplemented with 2.0 mu M N-6-benzylaminopurine and 0.8 mu M alpha-naphthaleneacetic acid (NAA). Under such conditions, 98% of the explants regenerated adventitious shoots after 8 weeks, and 41 buds were produced per explant on average. The mean shoot length was 9.6 mm, and on average, 4.5 shoots per explant were more than 2 mm long. Subsequently, the induced adventitious shoots were transferred into rooting medium consisting of 1/2 MS and various NAA concentrations. After 4 weeks, the shoots subcultured in this medium showed approximate to 93% root induction and an average of 3.5 adventitious roots per explant. Furthermore, the applied light spectrum significantly influenced shoot regeneration, and optimal results were achieved under an equal distribution of blue, red, and infrared light. The histological sections of shoots regenerated from direct organogenesis were observed through scanning electron microscopy (SEM). Afterward, the rooting adventitious shoots were subcultured in PGR-free medium for 8 weeks. The seedlings were successfully acclimated 4 weeks after being transferred to soil and bloomed after 11 months in a greenhouse. Thus, the PGR composition in micropropagation efficiently shortened the time to blooming from 25 to 16 months.
机译:Begonia montaniformis x秋海棠宁明斯var。贝拉杂交种装饰潜力很高。因此,本研究的目的是确定秋海棠蒙癌虫X秋天丁明森毒素的微扑相的最佳条件。 Bella F-1通过使用各种浓度的植物生长调节剂(PGR)和半强度Murashige和Skoog(1/2 ms)培养基的不同光谱。结果表明,当薄膜在补充有2.0μmn-6-苄基氨基嘧啶和0.8μmα-萘酸(Naa)的培养基中孵育薄膜时,将进行外植体再生。在此类条件下,8周后,98%的外植体再生出不定芽,平均每次探测蛋白产生41个芽。平均枝条长度为9.6毫米,平均,每次外植体的4.5次枝条长度超过2毫米。随后,将诱导的不定量芽转移到由1/2mS和各种NAA浓度组成的生根培养基中。 4周后,在该培养基中转移的芽显示近似为93%的根诱导和平均每次外植体的3.5个不定根。此外,所施加的光谱显着影响抗血液再生,并且在蓝色,红色和红外光的平等分布下实现了最佳结果。通过扫描电子显微镜(SEM)观察从直接器官发生中再生的芽的组织学部分。之后,将生根不定量芽转移到无遗传培养基中8周。在温室转移到土壤后4周,幼苗成功地适应4周,并在温室11个月后绽放。因此,微扑通中的PGR组合物有效地缩短了25至16个月的时间。

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