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Optimised Production and Extraction of Astaxanthin from the Yeast Xanthophyllomyces dendrorhous

机译:酵母黄单胞菌中虾青素的优化生产与提取

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摘要

Currently, astaxanthin demand is fulfilled by chemical synthesis using petroleum-based feedstocks. As such, alternative pathways of natural astaxanthin production attracts much research interest. This study aimed at optimising bioreactor operation parameters for astaxanthin production and evaluating strategies for its subsequent extraction. The effect of pH and agitation was evident, as a significant reduction in both biomass and astaxanthin production was observed when the culture pH was not controlled and a low agitation speed was applied. At controlled pH conditions and a high agitation speed, a significant increase in biomass (16.4 g/L) and astaxanthin production (3.6 mg/L) was obtained. Enzymatic yeast cell lysis using two commercial enzymes (Accellerase 1500 and Glucanex) was optimised using the central composite design of experiment (DoE). Accellerase 1500 led to mild cell disruption and only 9% ( ) astaxanthin extraction. However, Glucanex treatment resulted in complete astaxanthin extractability, compared to standard extraction method (DMSO/acetone). When supercritical CO was employed as an extraction solvent in Accellerase-pre-treated cells, astaxanthin extraction increased 2.5-fold. Overall, the study showed that extraction conditions can be tailored towards targeted pigments present in complex mixtures, such as in microbial cells.
机译:当前,虾青素的需求通过使用石油基原料的化学合成来满足。因此,天然虾青素生产的替代途径吸引了许多研究兴趣。这项研究旨在优化生物反应器操作参数,以生产虾青素并评估其后续提取策略。 pH和搅动的影响是显而易见的,因为当不控制培养液的pH值并施加低搅动速度时,生物量和虾青素的产量均显着降低。在受控的pH条件和高搅拌速度下,生物量(16.4 g / L)和虾青素产量(3.6 mg / L)显着增加。使用实验的中央复合设计(DoE)优化了使用两种商业酶(Accellerase 1500和Glucanex)进行的酶促酵母细胞裂解。 Accellerase 1500导致轻度的细胞破坏,仅提取9%()的虾青素。但是,与标准提取方法(DMSO /丙酮)相比,葡聚糖处理可完全提取虾青素。当在Accellerase预处理的细胞中使用超临界CO作为提取溶剂时,虾青素的提取增加了2.5倍。总体而言,研究表明,提取条件可以针对复杂混合物(例如微生物细胞)中存在的目标色素进行调整。

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