木兰花愈伤组织的培养</i>研究。:获得,培养条件选择,体细胞胚胎诱导

Q3 Pharmacology, Toxicology and Pharmaceutics
D. A. Nekrasova, M. N. Povydysh, N. S. Pivovarova, K. O. Sidorov
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引用次数: 0

摘要

介绍。细胞培养广泛应用于生物学、生物技术和农业的各个领域。木香是一种多年生草本植物,已被列入俄罗斯联邦红皮书。以紫檀属植物为原料的药品。具有有价值的药理活性类型,在东方医学中被广泛应用。恢复自然种群的一个严重障碍是植物种子存在形态生理休眠期,这需要一个长时间的分层过程。自然地理范围的限制和对人类有用的生物活动的结合使其成为一种稀有的植物。体外引入的前瞻性对象。的目标。本研究的目的是获得芫荽的活细胞培养。,体细胞胚胎发生条件的研究。材料和方法。以俄罗斯科学院科马罗夫植物学研究所产的木香完整植株叶片为初代外植体。将叶片片在2%苯扎氯铵溶液中灭菌5分钟,在Murasige - Skoog培养基上诱导初代骨痂形成。为选择适合愈伤组织长期培养的营养培养基,发现了不同成分的培养基。在生长素含量高的营养培养基上诱导体细胞胚胎发生。用HPTLC PRO系统(CAMAG AG,瑞士)检测完整植株和愈伤组织培养物的乙醇提取物。结果和讨论。培养2周后,外植体表面形成初生愈伤组织。减少蔗糖量(20 g/l)的Linsmaier - Skoog培养基被认为是最适合培养物长期维持的培养基。目前,我们正在继续收集这一过程的分析数据。定性分析表明,愈伤组织积累了三萜苷,其组成与完整植株接近。结论。木耳愈伤组织培养的一株活菌。,建立了一种长期培养愈伤组织的营养培养基。体细胞胚胎已经获得,目前正在监测它们的进一步发育。初步的植物化学研究表明,愈伤组织的化学成分与完整植物的化学成分接近。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Callus Culture of <i>Aralia cordata</i> Thunb.: Obtaining, Selection of Cultivating Conditions, Somatic Embryogenesis Induction
Introduction. Cell cultures spreads widely in different areas of biology, biotechnology and agriculture. Aralia cordata is a perennial herbaceous plant, which has been listed in Red book of the Russian Federation. Pharmaceuticals which are based on raw materials of Aralia ssp. have valuable types of pharmacological activity and are widely used in oriental medicine. A serious obstacle for resumption of the natural populations is the presence of the period of morphophysiological dormancy in the seeds of the plants, which requires a long-time stratification process. Limitation of the natural geographic range and the combination of biological activities useful for humans make Aralia cordata Thunb. prospective object for in vitro introduction. Aim. The aim of the study is obtaining of the viable cell culture of Aralia cordata Thunb., investigation of the somatic embryogenesis conditions. Materials and methods. Pieces of the leaves of Aralia cordata intact plant from Komarov Botanical Institute of the Russian Academy of Sciences were used as a primary explants. Pieces of leaves were sterilized in a 2 % benzalkonium chloride solution for 5 minutes, induction of primary callogenesis was carried out on Murasige – Skoog medium. Nutrient media with different constituents were discovered for choosing one for long-time cultivation of calli. Induction of somatic embryogenesis was carried out on the nutrient media with high auxins content. Ethanol extracts from the intact plant and calli cultures were assayed with HPTLC PRO SYSTEM (CAMAG AG, Switzerland). Results and discussion. After two weeks of cultivation, the formation of primary callus was observed on the surface of the explants. The Linsmaier – Skoog medium with a reduced amount of sucrose (20 g/l) was recognized as the most suitable medium for long-term maintenance of cultures. Embryoid structures of Aralia cordata have been obtained, now we are continuing to collect analytics data about this process. Qualitative analysis of the extracts showed that callus cultures accumulate triterpene glycosides, their composition is close to that of the intact plant. Conclusion. A viable strain of callus culture of Aralia cordata Thunb. was obtained, a nutrient medium for long-term cultivation of calli was established. Somatic embryoids have been obtained, and their further development is currently being monitored. A preliminary phytochemical study showed that the composition of the chemical components of calli is close to that of an intact plant.
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来源期刊
Drug Development and Registration
Drug Development and Registration Pharmacology, Toxicology and Pharmaceutics-Pharmaceutical Science
CiteScore
1.20
自引率
0.00%
发文量
61
审稿时长
8 weeks
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