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一种用于从海枣(Phoenix dactylifera L.,品种:Deglet Nour)胚性悬浮培养物中进行植株再生的优化方案。

An optimised protocol for plant regeneration from embryogenic suspension cultures of date palm, Phoenix dactylifera L., cv. Deglet Nour.

作者信息

Fki L, Masmoudi R, Drira N, Rival A

机构信息

Laboratoire des Biotechnologies Végétales, Faculté des Sciences de Sfax 802, 3018 Sfax, Tunisia.

出版信息

Plant Cell Rep. 2003 Feb;21(6):517-24. doi: 10.1007/s00299-002-0558-5. Epub 2003 Jan 10.

Abstract

An improved protocol is described for the large-scale micropropagation of an elite date palm ( Phoenix dactylifera L.) cultivar, Deglet Nour. Clonal plants were regenerated from somatic embryos derived from highly proliferating suspension cultures. Friable embryogenic calli were initiated from both leaf and inflorescence explants. Suspension cultures consisting of pro-embryonic masses were established from calli showing a high competency for somatic embryogenesis. The subculture of suspensions in liquid medium enriched with low amounts of plant growth regulators (1 mg l(-1) 2,4-dichlorophenoxyacetic acid with 300 mg l(-1) charcoal) resulted in the differentiation of large numbers of somatic embryos. The productivity of the cultures increased 20-fold (from 10 to 200 embryos per month per 100 mg fresh weight of embryogenic callus) when embryogenic suspensions were used instead of standard cultures on solid media. The overall production of somatic embryos reached 10,000 units per litre per month. Partial desiccation of the mature somatic embryos, corresponding to a decrease in water content from 90% to 75%, significantly improved germination rates (from 25% to 80%). The cutting back of the cotyledonary leaf was also found to stimulate embryo germination. Flow cytometric analysis showed that the micropropagation protocol followed here did not affect the ploidy level of somatic embryo-derived plantlets.

摘要

本文描述了一种改良方案,用于优良海枣(Phoenix dactylifera L.)品种Deglet Nour的大规模微繁殖。克隆植株从高度增殖的悬浮培养物衍生的体细胞胚再生而来。从叶片和花序外植体诱导出易碎的胚性愈伤组织。从显示出高体细胞胚胎发生能力的愈伤组织建立了由原胚团组成的悬浮培养物。在富含少量植物生长调节剂(1 mg l(-1) 2,4-二氯苯氧乙酸加300 mg l(-1) 活性炭)的液体培养基中对悬浮培养物进行继代培养,导致大量体细胞胚分化。当使用胚性悬浮培养物而非固体培养基上的标准培养物时,培养物的生产力提高了20倍(从每100 mg鲜重胚性愈伤组织每月10个胚胎增加到200个胚胎)。体细胞胚的总产量达到每月每升10,000个单位。成熟体细胞胚的部分干燥,对应于含水量从90% 降至75%,显著提高了发芽率(从25% 提高到80%)。还发现切除子叶叶可刺激胚发芽。流式细胞术分析表明,这里采用的微繁殖方案不影响体细胞胚衍生植株的倍性水平。

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