Use of Aqueous Two-Phase and Three-Phase Partitioning Systems for Purification of Lipase Obtained in Solid-State Fermentation by Rhizopus arrhizus

V. Dobreva, B. Zhekova, G. Dobrev
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引用次数: 11

Abstract

Purification of enzymes by conventional methods such as precipitation and chromatographic techniques is a costly and time-consuming procedure and may lead to low yields of enzyme activity. Alternative liquid-liquid extraction methods such as Aqueous Two-Phase Systems (ATPS) and Three Phase Partitioning (TPP) are characterized by the high enzyme yields and purification degree. The objective of this study was the application of partitioning systems ATPS and TPP for purification of lipase produced in solid-state fermentation by Rhizopus arrhizus. ATPS and TPP were used for purification of lipase, obtained by solid state cultivation of Rhizopus arrhizus. Lipase was isolated with PEG4000/potassium sodium tartrate ATPS and the effect of the system composition, including PEG 4000 and potassium sodium tartrate concentrations on lipase partitioning was studied. When using 30% PEG4000/21% potassium sodium tartrate, lipase was distributed in the top phase, and the highest recovery yield of 217% and purification fold of 6.1 were achieved. It was found that at PEG4000 concentration of or higher than 15%, the enzyme was present in the top polymer-rich phase with a partitioning yield of over 90%. Upon application of TPP for lipase isolation, the effect of t-butanol concentration, ammonium sulfate concentration and pH on enzyme partitioning was investigated. The highest lipase recovery yield of 71% and 19.1-fold purification were achieved in the interfacial phase in the presence of 30% ammonium sulfate saturation with 1.0:0.5 crude extract/t-butanol ratio at pH 7 in a single step. The sodium dodecyl sulfate-polyacrylamide gel electrophoresis and zymographic analysis showed significant purification of lipase by TPP and the presence of two multiple forms of the enzyme. ATPS (PEG4000/ Potassium sodium tartrate) and TPP (1.0:0.5 crude extract/t-butanol ratio, 30% ammonium sulfate saturation, pH 7) proved to be rapid methods for the isolation and purification of lipase and they can be used in downstream processing for industrial preparation of the enzyme.
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利用水两相和三相分配系统纯化根霉固态发酵所得脂肪酶
用沉淀法和色谱法等传统方法纯化酶是一个昂贵且耗时的过程,并且可能导致酶活性的低产量。水两相萃取(ATPS)和三相萃取(TPP)等液液萃取方法具有产酶率高、纯化程度高的特点。本研究的目的是应用分离体系ATPS和TPP对阿根霉固态发酵脂肪酶进行纯化。利用ATPS和TPP对固态培养的阿根霉脂肪酶进行纯化。采用PEG4000/酒石酸钾钠ATPS分离脂肪酶,研究了体系组成(PEG4000和酒石酸钾钠浓度)对脂肪酶分配的影响。当使用30% PEG4000/21%酒石酸钾钠时,脂肪酶分布在顶相,最高回收率为217%,纯化倍数为6.1倍。结果表明,当PEG4000浓度大于或等于15%时,酶存在于顶层富聚相,分配率达90%以上。应用TPP分离脂肪酶,考察了丁醇浓度、硫酸铵浓度和pH对酶分配的影响。在硫酸铵饱和度为30%、粗提液/丁醇比为1.0:0.5、pH为7的条件下,界面相脂肪酶回收率最高,为71%,纯化倍数为19.1倍。十二烷基硫酸钠-聚丙烯酰胺凝胶电泳和酶谱分析表明,TPP对脂肪酶有明显的纯化作用,并且存在两种多种形式的脂肪酶。ATPS (PEG4000/酒石酸钾钠)和TPP(1.0:0.5粗提物/丁醇比,硫酸铵饱和度30%,pH 7)是脂肪酶的快速分离纯化方法,可用于脂肪酶的下游工业制备。
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