Production and Isolation of Azaspiracid-1 and-2 from Azadinium spinosum Culture in Pilot Scale Photobioreactors

被引:24
作者
Jauffrais, Thierry [1 ]
Kilcoyne, Jane [6 ]
Sechet, Veronique [1 ]
Herrenknecht, Christine [2 ]
Truquet, Philippe [1 ]
Herve, Fabienne [1 ]
Berard, Jean Baptiste [3 ]
Nulty, Ciara [6 ]
Taylor, Sarah [1 ]
Tillmann, Urban [4 ]
Miles, Christopher O. [5 ]
Hess, Philipp [1 ]
机构
[1] IFREMER, EMP PHYC Lab, F-44311 Nantes, France
[2] Nantes Atlantic Univ, MMS EA2160, F-44035 Nantes, France
[3] IFREMER, BRM PBA Lab, F-44311 Nantes, France
[4] Alfred Wegener Inst, D-27570 Bremerhaven, Germany
[5] Norwegian Vet Inst, N-0106 Oslo, Norway
[6] Inst Marine, Oranmore, Co Galway, Ireland
来源
MARINE DRUGS | 2012年 / 10卷 / 06期
关键词
solid phase extraction; photobioreactor; chemostat; dinoflagellate; micro-algae; LC-MS/MS; tangential flow filtration; azaspiracid; HP-20; DINOFLAGELLATE GENUS AZADINIUM; OKADAIC ACID; STRUCTURAL ELUCIDATION; DINOPHYSIS-ACUTA; MYTILUS-EDULIS; SHELLFISH; TOXIN; ANALOGS; MUSSELS; GROWTH;
D O I
10.3390/md10061360
中图分类号
R914 [药物化学];
学科分类号
100701 ;
摘要
Azaspiracid (AZA) poisoning has been reported following consumption of contaminated shellfish, and is of human health concern. Hence, it is important to have sustainable amounts of the causative toxins available for toxicological studies and for instrument calibration in monitoring programs, without having to rely on natural toxin events. Continuous pilot scale culturing was carried out to evaluate the feasibility of AZA production using Azadinium spinosum cultures. Algae were harvested using tangential flow filtration or continuous centrifugation. AZAs were extracted using solid phase extraction (SPE) procedures, and subsequently purified. When coupling two stirred photobioreactors in series, cell concentrations reached 190,000 and 210,000 cell.mL(-1) at steady state in bioreactors 1 and 2, respectively. The AZA cell quota decreased as the dilution rate increased from 0.15 to 0.3 day (1), with optimum toxin production at 0.25 day (1). After optimization, SPE procedures allowed for the recovery of 79 +/- 9% of AZAs. The preparative isolation procedure previously developed for shellfish was optimized for algal extracts, such that only four steps were necessary to obtain purified AZA1 and -2. A purification efficiency of more than 70% was achieved, and isolation from 1200 L of culture yielded 9.3 mg of AZA1 and 2.2 mg of AZA2 of >95% purity. This work demonstrated the feasibility of sustainably producing AZA1 and -2 from A. spinosum cultures.
引用
收藏
页码:1360 / 1382
页数:23
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