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首页> 外文期刊>Plant Cell, Tissue and Organ Culture: An International Journal on in Vitro Culture of Higher Plants >High-quality embryo production and plant regeneration using a two-step culture system in isolated microspore cultures of hot pepper (Capsicum annuum L.)
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High-quality embryo production and plant regeneration using a two-step culture system in isolated microspore cultures of hot pepper (Capsicum annuum L.)

机译:在辣椒(Capsicum annuum L.)的分离小孢子培养中,使用两步培养系统进行高质量的胚胎生产和植物再生

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摘要

We developed an efficient culture system for producing cotyledonary embryos from isolated microspores of hot pepper (Capsicum annuum L.) and analyzed the ploidy levels of regenerated plants. Three culture protocols were studied: liquid, double-layer, and two-step culture. In the double-layer culture, cotyledonary embryos were produced more efficiently when the same medium composition was used for the liquid upper-layer and the solid under-layer. The two-step culture system, in which microspores were first incubated on liquid medium and then subcultured on double-layer medium, was most effective for producing cotyledonary embryos. Cotyledonary embryos were produced more efficiently when the isolated microspores were cultured in liquid medium for 1 week in 60 x 15-mm plates at a density of 8-10 x 10(4)/mL and microspore suspensions from two liquid culture plates were combined into a single 100 x 20-mm plate containing solid medium, and the culture was continued for an additional 3 weeks. When cotyledonary embryos obtained from this two-step culture were transplanted into regeneration medium, more than 95 % developed into plants. Only 31 of the 190 analyzed plants (16.3 %) generated by this method were spontaneous doubled haploids. This two-step culture system outperforms all previously reported culture protocols for isolated microspores of hot pepper, and appears to be a promising tool for the production of haploid plants for hot pepper breeding.
机译:我们开发了一种有效的培养系统,用于从辣椒(辣椒)的小孢子产生子叶胚,并分析了再生植株的倍性水平。研究了三种培养方案:液体培养,双层培养和两步培养。在双层培养中,当液体上层和固体下层使用相同的培养基组成时,子叶胚的产生效率更高。首先在液体培养基上培养小孢子,然后在双层培养基上继代培养的两步培养系统对产生子叶胚最有效。当分离的小孢子在液体培养基中于60 x 15-mm平板中以8-10 x 10(4)/ mL的密度培养1周,并将来自两个液体培养平板的小孢子悬浮液合并为子孢子时,子叶胚的生产效率更高。一张装有固体培养基的100 x 20 mm平板,再继续培养3周。当将从这种两步培养获得的子叶胚移植到再生培养基中时,超过95%的胚发育成了植物。通过这种方法产生的190种分析植物中,只有31种(16.3%)是自发的双倍单倍体。该两步培养系统的性能优于以前报道的所有分离辣椒小孢子的培养方案,并且似乎是生产用于辣椒育种的单倍体植物的有前途的工具。

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