生长素与营养胁迫耦合的百脉根体细胞胚胎发生
Auxin and nutritional stress coupled somatic embryogenesis in L.
作者信息
Krishnan S R Saranya, Siril E A
机构信息
Department of Botany, University of Kerala, Kariavattom, Thiruvananthapuram, 695 581 India.
出版信息
Physiol Mol Biol Plants. 2017 Apr;23(2):471-475. doi: 10.1007/s12298-017-0425-z. Epub 2017 Mar 14.
Somatic embryos were induced from internodal segment derived callus of L., in MS medium supplemented with different concentrations of 2,4-Dichlorophenoxy acetic acid (2,4-D). Initially calli were developed from internodes of microshoots inoculated in 2.5 µM NAA supplemented medium. Then calli were transferred to 2,4-D added medium for somatic embryogenesis. Nutritional stress coupled with higher concentration of 2,4-D triggered somatic embryogenesis. Nutritional stress was induced by culturing callus in a fixed amount of medium for a period up to 20 weeks without any external supply of nutrients. Addition of 2.5 µM 2,4-D gave 100% embryogenesis within 16 weeks of incubation. Callus mass bearing somatic embryos were transferred to germination medium facilitated production of in vitro plantlets. MS medium supplemented with 2.5 µM benzyl adenine and 0.5 µM α-naphthalene acetic acid produced 15.33 plants per culture within 4 weeks of culture. Somatic embryo germinated plants were then hardened and transferred to green house.
从L.的节间切段诱导出体细胞胚,培养于添加不同浓度2,4 - 二氯苯氧乙酸(2,4 - D)的MS培养基中。最初,愈伤组织从接种在添加2.5 μM萘乙酸(NAA)的培养基中的微茎节间发育而来。然后将愈伤组织转移到添加2,4 - D的培养基中进行体细胞胚胎发生。营养胁迫与较高浓度的2,4 - D共同触发了体细胞胚胎发生。营养胁迫是通过将愈伤组织培养在固定量的培养基中长达20周且不提供任何外部营养来诱导的。添加2.5 μM 2,4 - D在培养16周内产生了100%的胚胎发生。带有体细胞胚的愈伤组织团被转移到萌发培养基中,促进了离体小植株的产生。添加2.5 μM苄基腺嘌呤和0.5 μM α - 萘乙酸的MS培养基在培养4周内每个培养物产生了15.33株植株。体细胞胚萌发的植株随后进行炼苗并转移到温室中。
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