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生姜(姜科姜属植物)离体培养芽的冷冻保存。

Cryopreservation of in vitro grown shoots of ginger (Zingiber officinale Rosc.).

作者信息

Yamuna G, Sumathi V, Geetha S P, Praveen K, Swapna N, Babu K Nirmal

机构信息

Division of Crop Improvement and Biotechnology, Indian Institute of Spices Research, Kerala, India.

出版信息

Cryo Letters. 2007 Jul-Aug;28(4):241-52.

Abstract

An efficient cryopreservation technique for in vitro grown shoots of ginger (Zingiber officinale Rosc) was developed based on encapsulation dehydration, encapsulation vitrification and vitrification procedures. Pregrowth and serial preculture were needed to obtain the best regrowth for all techniques. The vitrification procedure resulted in higher regrowth (80%) when compared to encapsulation vitrification (66%) and encapsulation dehydration (41%). In the vitrification procedure shoots were: precultured in liquid Murashige-Skoog medium containing 0.3 M sucrose for 3 days; cryoprotected with a mixture of 5% DMSO and 5% glycerol for 20 min at room temperature; osmoprotected with a mixture of 2 M glycerol and 0.4 m sucrose for 20 min at 25 degrees C; before being dehydrated with a highly concentrated vitrification solution (PVS2) for 40 min at 25 degrees C. The dehydrated shoots were transferred to 2 ml cryotubes, suspended in 1 ml PVS2 and plunged directly into liquid nitrogen. In all the three cryopreservation procedures tested, shoots grew from cryopreserved shoot tips without intermediary callus formation. The genetic stability of cryopreserved ginger shoot buds were confirmed using ISSR and RAPD profiling.

摘要

基于包埋脱水、包埋玻璃化和玻璃化法,开发了一种高效的生姜(姜科姜属)离体生长芽的冷冻保存技术。所有技术都需要进行预生长和连续预培养以获得最佳的再生效果。与包埋玻璃化法(66%)和包埋脱水法(41%)相比,玻璃化法的再生率更高(80%)。在玻璃化法中,芽的处理步骤如下:在含有0.3M蔗糖的液体Murashige-Skoog培养基中预培养3天;在室温下用5%DMSO和5%甘油的混合物进行20分钟的冷冻保护;在25℃下用2M甘油和0.4M蔗糖的混合物进行20分钟的渗透保护;然后在25℃下用高浓度玻璃化溶液(PVS2)脱水40分钟。脱水后的芽转移到2ml冷冻管中,悬浮在1ml PVS2中,直接投入液氮。在测试的所有三种冷冻保存程序中,冷冻保存的茎尖都能长出芽,且无中间愈伤组织形成。使用ISSR和RAPD分析证实了冷冻保存的生姜芽的遗传稳定性。

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