In vitro culture of Zingeria biebersteiniana (Claus) P. Smirn. as a method for conservation and restoration of genetic diversity

M. O. Twardovska, V. Kunakh
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Abstract

Aim. The aim of the work was to determine the conditions for development of in vitro culture, induction of callus formation, and long-term tissue culture of Zingeria biebersteiniana (Claus) P. Smirn. Methods. In vitro clonal propagation, tissue culture techniques. Results. The seed germination rate was found to increase significantly after long-term cold stratification. The protocol for seed sterilization was developed, which yielded 57.3% of aseptic plants. Collections of in vitro and pot cultured plants were created. Experiments on the adaptation of in vitro propagated plants to pot culture conditions revealed a high level of their survival. The optimal medium for in vitro clonal propagation was MS, supplemented with 0.1 mg/L NAA; while the most effective media for induction of callus formation and for long-term tissue culture was B5 supplemented with 2 mg/L 2,4-D and 0.1 mg/L BAP. Conclusions. The protocols and conditions for seed germination, in vitro clonal propagation, induction of callus formation, as well as long-term tissue culture of Z. biebersteiniana have been developed. The developed techniques of in vitro culture can be used for conservation and restoration of genetic diversity of the species, as well as to obtain sufficient plant material for further studies.
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浙姜的离体培养。作为一种保护和恢复遗传多样性的方法
的目标。本研究的目的是确定扁姜(Zingeria bibersteiniana, Claus) P. Smirn的离体培养、愈伤组织诱导和长期组织培养的条件。方法。体外克隆繁殖,组织培养技术。结果。经长期冷分层处理,种子发芽率显著提高。制定了种子灭菌方案,无菌植株率达57.3%。建立了离体和盆栽植物的集合。离体繁殖植株对盆栽条件的适应实验表明,其成活率较高。体外克隆繁殖的最佳培养基为MS,添加0.1 mg/L NAA;诱导愈伤组织形成和长期组织培养最有效的培养基为B5 + 2 mg/L 2,4- d + 0.1 mg/L BAP。结论。研究了紫茎草种子萌发、离体无性系繁殖、愈伤组织诱导和长期组织培养的方法和条件。开发的离体培养技术可用于保护和恢复该物种的遗传多样性,并为进一步的研究获取充足的植物材料。
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