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首页> 外文期刊>Industrial Crops and Products >Pathogenic fungal elicitors enhance ginsenoside biosynthesis of adventitious roots in Panax quinquefolius during bioreactor culture
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Pathogenic fungal elicitors enhance ginsenoside biosynthesis of adventitious roots in Panax quinquefolius during bioreactor culture

机译:在生物反应器培养过程中,致病性真菌激发子增强西洋参不定根的人参皂苷生物合成

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摘要

Fungi have been widely used as biotic elicitors to promote metabolite production of plant cell, tissue, and organ cultures. Alternaria panax Whetz. and Cylindrocarpon destructans (Zinss) Scholten are the main pathogenic fungi in ginseng cultivation. The present study used extracts of A. panax and C destructans as elicitors to simulate adventitious roots (ARs) of Panax quinquefolius L for improvement of ginsenoside accumulation during AR bioreactor culture. To select a suitable elicitation method, the effects of treatment duration and concentration of both fungal extracts were investigated. After 30 d of AR bioreactor culture, the addition of A. panax and C. destructans extracts for 8 d to the culture medium produced higher ginsenoside content and productivity than the other treatment periods. During the elicitation of both fungal extracts, the peak contents of nitric oxide (NO), putrescine (Put), and ginsenoside were observed at 2, 4, and 8 d, respectively. Therefore, NO and Put-could be upstream signals to regulate ginsenoside synthesis. The optimal elicitor concentration varied between extracts of A. panax and C. destructans. The maximum total ginsenoside content and productivity were observed with 4 mg/L and 20 mg/L of the A. panax and C. destructans extracts, respectively. The ginsenoside monomers with the most increase were Rg3, Rh2, and Re for the A. panax extract and Rg3, Rh2, and Rf for the C. destructans extract. In addition, the AR biomass was more inhibited by the C. destructans (20 mg/L) extract, although its ginsenoside content (34.1 mg/g DW) was higher than that with the A. panax (4 mg/L) extract. The maximum ginsenoside production (276.0 mg/L) was achieved with the A. panax (4 mg/L) extract. Therefore, the A. panax extract was more suitable as an elicitor for ginsenoside production during AR bioreactor culture. The present study confirmed that treating 30-d-old P. quinquefolius ARs with 4 mg/L A. panax extract for 8 d during bioreactor culture is the optimal elicitation method; these ARs can be applied to the commercial production of P. quinquefolius products. (C) 2016 Elsevier B.V. All rights reserved.
机译:真菌已被广泛用作生物引发剂,以促进植物细胞,组织和器官培养物中代谢产物的产生。交链孢霉人参栽培中主要的致病真菌是Cylindrocarpon destructans(Zinss)。本研究使用人参和提取物的提取物作为引诱物来模拟西洋参的不定根(ARs),以改善AR生物反应器培养过程中人参皂苷的积累。为了选择合适的诱导方法,研究了处理时间和两种真菌提取物浓度的影响。在AR生物反应器培养30 d后,向培养基中添加人参和提取物的提取物8 d产生的人参皂苷含量和生产率均高于其他处理时期。在两种真菌提取物的诱导过程中,分别在第2、4和8 d观察到一氧化氮(NO),腐胺(Put)和人参皂苷的峰值含量。因此,NO和Put-可能是调控人参皂甙合成的上游信号。最佳激发子浓度在人参和C. destructans的提取物之间变化。分别以4 mg / L和20 mg / L的A. panax和C. destructans提取物观察到最大的总人参皂苷含量和生产率。人参皂苷单体中人参皂苷单体的增加量最大,分别为Rg3,Rh2和Re,而C.destructans提取物的人参皂苷单体为Rg3,Rh2和Rf。此外,尽管其人参皂甙含量(34.1 mg / g DW)比人参(4 mg / L)提取物高,但其生物量却受到解构梭菌(20 mg / L)提取物的抑制。人参提取物(4 mg / L)达到了最大的人参皂甙产量(276.0 mg / L)。因此,人参提取物更适合作为AR生物反应器培养过程中人参皂甙生产的引发剂。本研究证实,在生物反应器培养过程中,用4 mg / L人参提取物处理30 d的西洋参假单胞菌8 d是最佳诱导方法。这些AR可用于商业化的P. quinquefolius产品。 (C)2016 Elsevier B.V.保留所有权利。

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