胡萝卜悬浮培养高频体细胞胚发生同步:模式系统及其在植物发育中的应用。

K Osuga, H Masuda, A Komamine
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引用次数: 21

摘要

本文介绍了以胡萝卜悬浮培养为高等植物培养模式的高等植物细胞高频诱导同步体细胞胚胎发生的材料和方法。本文报道了在本实验室建立的四种同步体细胞胚胎发生系统:(1)单细胞体细胞胚胎发生。a)在含有2,4- d、玉米素和甘甘醇的悬浮培养中,通过筛选、Percoll溶液中的密度梯度离心和人工挑选获得的小球形单细胞,形成胚性细胞团,当胚性细胞团转移到缺乏2,4- d的培养基中时,胚性细胞团以高频率分化为胚胎。b)体胚再生植株经2,4- d处理后,下胚轴外植体培养12-24 h,然后转移到不含2,4- d的新鲜培养基中。单细胞从下胚轴外植体中释放并分化为胚胎的频率很高。在该系统中,可以收集到大量的单细胞和胚性细胞。(2)胚性细胞簇的体细胞胚胎发生,是由悬浮培养物经过筛分、密度梯度离心(Ficoll溶液)、低速离心获得的,在高频率下同步分化为球形胚胎。植株由球形胚形成。(3)根据(2)中描述的程序获得的胚胎性细胞团以2 × 10(3)个细胞团ml(-1)的细胞密度培养。当培养密度低于150个球形胚ml(-1)时,球形胚分化为鱼雷形胚,随后在高频率下分化为植株。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Synchronization of somatic embryogenesis at high frequency using carrot suspension cultures: model systems and application in plant development.

Materials and methods for the high frequency induction and synchronous somatic embryogenesis from cultured cells of higher plants are described, using carrot suspension cultures as a model system of higher plants. The following four synchronous systems of somatic embryogenesis, which were established in our laboratories, are reported: (1) Somatic embryogenesis from single cells. a) Small spherical single cells, obtained from suspension cultures in the presence of 2,4-D, zeatin and mannitol by sieving, density gradient centrifugation in Percoll solutions and manual picking up, form embryogenic cell clusters, which differentiate to embryos at high frequency, when embryogenic cell clusters are transferred to a medium lacking 2,4-D. b) Explants of hypocotyls of regenerated plantlets from somatic embryos were cultured after treatment with 2,4-D for 12-24 h, and then transferred into a fresh medium lacking 2,4-D. Single cells are released from hypocotyl explants and differentiated into embryos at high frequency. In this system, a large number of single cells and embryogenic cells can be collected. (2) Somatic embryogenesis from embryogenic cell clusters, which are obtained from suspension cultures by sieving, density gradient centrifugation in Ficoll solutions, and subsequent centrifugation at a low speed, differentiate synchronously to globular embryos at high frequency. Plantlets are formed from globular embryos. (3) Embryogenic cell clusters obtained according to the procedure described in (2) are cultured at cell densities of 2x10(3) cell clusters ml(-1). Globular embryos differentiate to torpedo-shaped embryos and subsequently to plantlets at high frequency when they are cultured at densities below 150 globular embryos ml(-1).

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