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高效制备海洋假交替单胞菌 QD1-2 的伪交替单胞菌素 A 通过响应面法和高速逆流色谱法的结合:与高效液相色谱法的比较。

Efficient preparation of pseudoalteromone A from marine Pseudoalteromonas rubra QD1-2 by combination of response surface methodology and high-speed counter-current chromatography: a comparison with high-performance liquid chromatography.

机构信息

Key Laboratory of Applied Marine Biotechnology of Ministry of Education, Ningbo University, Ningbo, 315211, China.

出版信息

Appl Microbiol Biotechnol. 2014 May;98(10):4369-77. doi: 10.1007/s00253-014-5530-0. Epub 2014 Jan 31.

DOI:10.1007/s00253-014-5530-0
PMID:24477384
Abstract

Pseudoalteromone A (PA) is a cytotoxic and anti-inflammatory ubiquinone discovered recently from a marine bacterium Pseudoalteromonas sp. CGH2XX. In order to meet its sample supply for further in vivo pharmacological investigation, an efficient method was developed for the preparation of PA by combination of response surface methodology (RSM) and high-speed counter-current chromatography (HSCCC) from marine bacterium P. rubra QD1-2. First, optimization of culture conditions was studied by the RSM to enhance PA production. The results indicated that the optimal cultivation condition was peptone (2.21 g/l), yeast extract (3.125 g/l), glucose (0.125 g/l), KBr (0.02 g/l), inoculum size (6.5 %), medium volume (595 ml), initial pH value (7.0), temperature (28 °C). Under the optimized fermentation condition, PA production was 1.04 mg/l with 14.8-fold increase comparing to 0.07 mg/l under original standard fermentation condition. The PA production was further investigated using a 14-l jar fermenter. Compared to the flask culture, P. rubra QD1-2 offered 45 % increase of PA production at 1.51 mg/l. Then, a rapid and efficient method for the separation and purification of PA from crude culture extract was developed using HSCCC. The two-phase solvent system used for HSCCC separation was composed of n-hexane-ethyl acetate-methanol-water (5:5:9:5, v/v/v/v). The isolation was accomplished within 100 min, and the purity of PA was over 95 %. The recovery of the process was 93 %.

摘要

假性交替单胞菌 A(PA)是一种从海洋细菌假交替单胞菌 CGH2XX 中发现的具有细胞毒性和抗炎作用的泛醌。为满足其用于进一步体内药理学研究的样品供应,从海洋细菌红球菌 QD1-2 中结合响应面法(RSM)和高速逆流色谱(HSCCC)开发了一种制备 PA 的有效方法。首先,通过 RSM 研究了培养条件的优化,以提高 PA 的产量。结果表明,最佳培养条件为蛋白胨(2.21 g/l)、酵母提取物(3.125 g/l)、葡萄糖(0.125 g/l)、KBr(0.02 g/l)、接种量(6.5%)、培养基体积(595 ml)、初始 pH 值(7.0)、温度(28°C)。在优化的发酵条件下,PA 的产量为 1.04 mg/l,比原始标准发酵条件下的 0.07 mg/l 提高了 14.8 倍。在 14 升罐式发酵罐中进一步研究了 PA 的生产。与摇瓶培养相比,红球菌 QD1-2 的 PA 产量在 1.51 mg/l 时提高了 45%。然后,使用 HSCCC 从粗培养提取物中分离和纯化 PA 开发了一种快速有效的方法。HSCCC 分离所用的两相溶剂系统由正己烷-乙酸乙酯-甲醇-水(5:5:9:5,v/v/v/v)组成。分离在 100 min 内完成,PA 的纯度超过 95%。该过程的回收率为 93%。

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