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首页> 外文期刊>In Vitro Cellular and Development Biology. Plant: Journal of the Tissue Culture Association >Cryoconservation and regeneration of axillary shoot meristems of Indigofera tinctoria (L.) by encapsulation-dehydration technique
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Cryoconservation and regeneration of axillary shoot meristems of Indigofera tinctoria (L.) by encapsulation-dehydration technique

机译:包埋脱水技术对蓝靛蓝腋生分生组织的低温保存和再生

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摘要

In vitro axillary shoot proliferation was achieved from single-node explants of Indigofera tinctoria on a well-defined medium, Murashige and Skoog (MS) medium supplemented with 1.0 mg l(-1) N (6)-benzyl adenine (BA) and 0.1 mg l(-1) indole-3-acetic acid. Axillary shoot meristems from cultures derived from up to three subcultures were used in the encapsulation-dehydration technique. Preconditioned, calcium alginate-encapsulated, and precultured axillary shoot meristems were subjected to different lengths of desiccation in a laminar flow cabinet. Maximum survival and regeneration rates of 56.7% and 62.2%, respectively, were obtained in half-strength (half the macro- and micronutrients and full-strength vitamins) MS medium supplemented with 0.5 mg l(-1) gibberellic acid and 0.2 mg l(-1) BA after 4 h of desiccation, during which the moisture content was reduced to 16.0%. According to the analysis of six random amplified polymorphic DNA markers, plantlets derived from cultures initiated with cryopreserved plant material were genetically identical to those derived from nonfrozen (control) tissues.
机译:体外腋芽增殖是通过在明确定义的培养基,Murashige和Skoog(MS)培养基上添加1.0 mg l(-1)N(6)-苄基腺嘌呤(BA)和0.1的明确培养基上的Indigofera tinctoria单节外植体实现的mg l(-1)吲哚-3-乙酸。包囊-脱水技术中使用了来自最多三个继代培养物的腋生芽分生组织。在层流柜中对经过预处理,藻酸钙包囊和预培养的腋生枝条分生组织进行不同长度的干燥。在补充0.5 mg l(-1)赤霉素和0.2 mg l的半强度(一半,大量营养素和微量营养素和全强度维生素)MS培养基中,最大存活率和再生率分别为56.7%和62.2%。 (-1)干燥4小时后的BA,其期间水分含量降低至16.0%。根据对六个随机扩增的多态性DNA标记的分析,从以低温保存的植物材料开始的培养物中获得的小植株与从非冷冻(对照)组织获得的植株在遗传上相同。

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