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Isolation and purification of ent-pimara-8(14),15-diene from engineered Aspergillus nidulans by accelerated solvent extraction combined with HPLC

机译:加速溶剂萃取与HPLC结合从工程化构巢曲霉中分离和纯化ent-pimara-8(14),15-二烯

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We recently engineered Aspergillus nidulans to produce a pimarane-type diterpene, ent-pimara-8(14),15-diene. Here, we describe methods for its isolation and purification from the engineered A. nidulans production strain and extend these findings with structural confirmation for the diterpene from this fungal source. The extraction protocol was optimized using accelerated solvent extraction (ASE) with three varying parameters: solvent composition, pressure, and temperature. This ASE method using 100% ethyl acetate at 90 °C with 12.07 MPa was more efficient and faster compared to ultrasonic-assisted extraction. Using both analytical and preparative C18 columns at isocratic elution of acetonitrile developed an HPLC separation; and, the diterpene was well separated within 28 min and 35 min, respectively. Also, TLC of the fungal culture extracts was performed with visualization using rhodamine. The reproduction and efficiency of the purification methods were evaluated by GC-MS; and, the structure of the compound was verified by NMR. The method enabled the isolation of this very lipophilic diterpene in pure form, allowing its testing in a number of bioactivity assays. Notably, we demonstrate for the first time the antioxidant activity for ent-pimara-8(14),15-diene using the 2,2-diphenyl-1-picrylhydrazyl (DPPH) assay...
机译:最近,我们设计了构巢曲霉,以生产一个pimarane型双萜,ent-pimara-8(14),15-diene。在这里,我们描述了从构巢曲霉生产菌株中分离纯化的方法,并通过对这种真菌来源的二萜进行结构确认来扩展这些发现。使用具有三个不同参数的加速溶剂萃取(ASE)对萃取方案进行了优化:溶剂组成,压力和温度。与超声辅助萃取相比,这种ASE方法在90°C和12.07 MPa下使用100%乙酸乙酯,效率更高,速度更快。在乙腈等度洗脱中同时使用分析性C18和制备型C18色谱柱进行了HPLC分离。并且,二萜分别在28分钟和35分钟内分离良好。另外,真菌培养物提取物的TLC使用罗丹明进行可视化。通过GC-MS评估纯化方法的重现性和效率。并且,通过NMR验证了化合物的结构。该方法能够分离纯形式的这种亲脂性二萜,从而可以在许多生物活性测定中进行测试。值得注意的是,我们首次使用2,2-二苯基-1-吡啶并肼基(DPPH)测定法证明了对pimara-8(14),15-二烯的抗氧化活性...

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