以混合营养方式将细胞密集接种体发育成盐杜氏藻种子群培养单位的营养培养基

Suman Keerthi, U. Koduru, N. Sarma
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引用次数: 3

摘要

盐渍杜氏藻在天然池塘中广泛栽培,或在人工池塘中集约栽培,用于生产β-胡萝卜素。用在实验室条件下或在中试植物中培养的接种物播种。由于其生长对光的要求很高,盐藻培养物的细胞稀释程度很高。因此,需要大量的培养接种物来播种大众培养单位。用一株印度菌株- I3研究了以混合营养方式培养盐芽孢杆菌获得细胞密集接种物的可行性。矿物培养基的成分及其浓度首先在生长试验中标准化。在优化后的培养基中添加有机碳源(甘油、乙酸钠和麦芽浸膏)和有机氮源(酵母浸膏和蛋白胨),考察混合营养培养的最佳效果。在海水中添加100 mg L-1硝酸钾或尿素、0.35 mg L-1磷酸钾、1 ml L-1微量元素混合物(Walne培养基)(不含硼酸盐)和12.5% NaCl的矿物培养基效果最佳。在优化的矿物质培养基中,以1:3 g L-1比例的麦芽和酵母提取物可产生细胞致密培养。混合营养培养的接种体在优化的矿物质培养基中光自养生长,生物量增加,胡萝卜素含量高于光自养培养。与自养培养相比,生产周期缩短了11天
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A nutrient medium for development of cell dense inoculum in mixotrophic mode to seed mass culture units of Dunaliella salina
Dunaliella salina is cultivated extensively in natural ponds or intensively in race way ponds for β-carotene production. The ponds are seeded with culture inoculum developed in laboratory conditions or in pilot plant. Because of its high light requirement for growth, D. salina cultures are very cell dilute. Therefore, a large volume of culture inoculum is required to seed mass culture units. The feasibility of culture of D. salina in mixotrophic mode to obtain cell dense inoculum was investigated with an Indian isolate – I3. The constituents of the mineral medium and their concentration were first standardized in growth assays. The optimized mineral medium was supplemented with organic carbon sources – glycerol, sodium acetate and malt extract and organic nitrogen sources – yeast extract and peptone to test for the best results of mixotrophic culture. A mineral medium with 100 mg L–1 potassium nitrate or urea, 0.35 mg L–1 potassium phosphate, 1 ml L–1 trace elements mix (Walne's medium) without borate and 12.5 % NaCl in sea water was found optimal. Malt and yeast extracts in the proportion of 1:3 g L–1 in optimized mineral medium was found to result in cell dense cultures. Mixotrophically cultured inoculum grown photoautotrophically in optimized mineral medium resulted in increased biomass production with higher carotene content than when photoautotrophically cultured. The production cycle decreased by 11 days compared to autotrophic cultures
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