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Potential of Somatic Embryogenesis in Elimination of East Africa Cassava Mosaic Virus from Infected Cassava Cultivars in Kenya

机译:从肯尼亚受感染的木薯品种中去除东非木薯花叶病毒后体细胞胚发生的潜力

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Cassava mosaic disease (CMD) is an economically important disease limiting production of cassava ( Manihot esculenta Crantz) in sub-Saharan Africa. Use of virus-free planting material is among the strategies for management of CMD. However, obtaining clean planting material for farmer-preferred varieties is often difficult. This study evaluated the efficacy of somatic embryogenesis to produce disease-free cassava planting materials from CMD-infected cultivars TME 14, Ex-Mariakani, Sagalato, Kibandameno and TMS 60444. Axillary buds of East Africa cassava mosaic virus (EACMV)-infected cassava nodal cuttings were cultured on MS salts with vitamins supplemented with 12 mg/l picloram for generation of primary somatic embryos (SE) which were subcultured onto the same fresh medium for generation of secondary SE. Primary and secondary SE were cultured separately onto MS supplemented with 1 mg/l naphthaleneacetic acid (NAA) for induction of cotyledons and subsequent regeneration of plants on MS supplemented with 0.4 mg/l 6-benzylaminopurine (BAP). Polymerase chain reaction (PCR) was used to discern the presence of EACMV in regenerated plants. Plants regenerated from primary and secondary somatic embryos were 87.6% and 93.5% virus free, respectively, with the PCR technique of viral particle detection. The virus-free plants acclimatized in the glasshouse showed absence of viral symptoms morphologically. These findings demonstrated the effectiveness of somatic embryogenesis in elimination of EACMV from infected cassava plants to produce clean planting materials.
机译:木薯花叶病(CMD)是限制撒哈拉以南非洲木薯(Manihot esculenta Crantz)生产的经济上重要的疾病。使用无病毒的种植材料是CMD管理的策略之一。但是,通常很难获得农民偏爱的品种的清洁种植材料。这项研究评估了体细胞胚发生从CMD感染的品种TME 14,Ex-Mariakani,Sagalato,Kibandameno和TMS 60444生产无病的木薯种植材料的功效。东非木薯花叶病毒(EACMV)感染的木薯结的腋芽将插条在MS盐上添加了12 mg / l吡咯仑的维生素进行培养,以生成原代体细胞胚(SE),然后将其继代培养到相同的新鲜培养基上,以生成次生SE。将初级和次级SE分别培养在补充有1 mg / l萘乙酸(NAA)的MS上,以诱导子叶,随后在补充有0.4 mg / l 6-苄基氨基嘌呤(BAP)的MS上再生植物。聚合酶链反应(PCR)用于识别再生植物中EACMV的存在。使用病毒颗粒检测的PCR技术,从初级和次级体细胞胚再生的植物分别不含病毒,分别为87.6%和93.5%。在温室中适应的无病毒植物在形态上没有病毒症状。这些发现证明了体细胞胚发生在消除受感染的木薯植物中的EAMCV以产生清洁的种植材料方面的有效性。

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