首页> 外文期刊>Plant Cell, Tissue and Organ Culture (PCTOC) >Stress treatments and in vitro culture conditions influence microspore embryogenesis and growth of callus from anther walls of sweet pepper (Capsicum annuum L.)
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Stress treatments and in vitro culture conditions influence microspore embryogenesis and growth of callus from anther walls of sweet pepper (Capsicum annuum L.)

机译:胁迫处理和体外培养条件影响甜椒(辣椒)花药壁的小孢子胚发生和愈伤组织的生长。

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摘要

Production of doubled haploids (DHs) is a convenient tool to obtain pure lines for breeding purposes. Until now, the easiest and most useful approach to obtain pepper DHs is via anther culture. However, this method has an associated possibility of producing calli from anther wall tissues that would be coexisting in the anther locule with embryos derived from microspores. Using two established protocols for anther culture, Dumas de Vaulx et al. (Agronomie 2:983–988, 1981) and Supena et al. (Sci Hort 107:226–232, 2006a; Plant Cell Rep 25:1–10, 2006b) callus and embryo development was assessed in four sweet pepper cultivars. For all genotypes tested, the protocol of Dumas de Vaulx et al. (Agronomie 2:983–988, 1981) promoted both embryo development and callus growth, whereas the protocol of Supena et al. (Sci Hort 107:226–232, 2006a; Plant Cell Rep 25:1–10, 2006b) produced no callus but only embryos. However, differences in embryo production were observed among these genotypes. In parallel, anthers were exposed to a 35 °C inductive heat shock for 4, 8, 12 and 16 days, prior to culture at 25 °C. The duration of the heat shock had significant effects in embryo production, but also in callus generation. Callus generation increased with prolonged exposures to 35 °C. Embryo and callus origin was analyzed by flow cytometry, light microscopy and molecular markers. Tests conducted demonstrated a gametophytic origin for all of the embryos tested, and a sporophytic origin for all of the calli. Together, our results reveal that culture conditions have a significant influence on the presence of calli derived from anther walls, which could be minimized by reducing heat shock exposure and/or using a shed-microspore approach.
机译:生产双倍单倍体(DHs)是获得用于育种目的的纯品系的便捷工具。迄今为止,获得花椒DHs的最简单,最有用的方法是通过花药培养。然而,该方法具有从花药壁组织中产生愈伤组织的可能性,所述花药壁组织与来自小孢子的胚共存于花药室中。使用两个已建立的花药培养方案,Dumas de Vaulx等。 (Agronomie 2:983–988,1981)和Supena等人。 (Sci Hort 107:226–232,2006a; Plant Cell Rep 25:1–10,2006b)在四个甜椒品种中评估了愈伤组织和胚胎的发育。对于所有测试的基因型,Dumas de Vaulx等人的方案。 (Agronomie 2:983–988,1981)促进了胚胎的发育和愈伤组织的生长,而Supena等人的方案却是。 (Sci Hort 107:226–232,2006a; Plant Cell Rep 25:1–10,2006b)未产生愈伤组织,仅产生了胚胎。但是,在这些基因型之间观察到胚胎产生的差异。平行地,在25°C培养之前,将花药暴露于35°C的感应热激下4、8、12和16天。热休克的持续时间不仅对胚胎产生有重要影响,而且对愈伤组织的产生也有重要影响。长时间暴露于35°C,愈伤组织的生成会增加。通过流式细胞术,光学显微镜和分子标记分析了胚和愈伤组织的起源。进行的测试表明,所有受试胚胎的配子体起源,以及所有愈伤组织的孢子体起源。总之,我们的结果表明,培养条件对源自花药壁的愈伤组织的存在具有重大影响,可以通过减少热激暴露和/或使用小孢子小孢子方法将其最小化。

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