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Liquid–liquid extraction of lipase produced by psychrotrophic yeast Leucosporidium scottii L117 using aqueous two-phase systems

机译:液液萃取脂肪酶的脂肪酶,由两相体系水溶液苏格西L117产生

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摘要

Aqueous two-phase systems (ATPS) have been used in biomolecules separation and as an efficient alternative to traditional purification systems for lipases extraction. Here, we investigated the partitioning and recovery of lipase derived from Leucosporidium scottii L117 using ATPS and aqueous two-phase micellar systems (ATPMS). Thus, we evaluated three ATPS: (i) polyethylene glycol (PEG)/phosphate salts and (ii) PEG/polyacrylic acid (NaPA) in different molecular weights (1500, 4000 and 8000 g/mol). (iii) Triton X-114 (TX-114)/McIlvaine buffer pH 7.0 in different conditions (2.0% (w/w) of TX-114 at 25.0 and 28.0 degrees C). The PEG/phosphate and PEG/NaPA systems resulted in a great loss of enzymatic activity; thus these systems do not represent viable alternatives for these lipase extraction. The micellar systems yielded the best results for lipase extraction with enzyme activity balances ranging between 84.7% and 113.05%. After optimizing the micellar system by experimental design of the partition coefficient of lipase increased by 10.3-fold (0.75-7.76). Lipase preferentially partitioned into the micelle-rich phase with K-Lip = 7.76, % RECBot = 93.85% and PF = 1.2 at 25.03 degrees C, 5.1 pH and 10.38% TX-114 and K-Lip, = 4.77, % RECBot = 73.53% and PF = 1.97 at 28.00 degrees C, 4.5 pH and 8.0% TX-114, indicating that the ATPMS represents an alternative to purification/extraction of lipase L scottii L117. A crude lipase extract was also evaluated to define the optimum pH and temperature. Lipase reached optimal activity at 40 degrees C, and remained stable in pH values ranging from pH 3.0 to 8.0 and temperatures from 20.0 to 45.0 degrees C, with relative residual lipase activity above 80% after 30 min of incubation. (C) 2015 Elsevier B.V. All rights reserved.
机译:已经在生物分子分离中使用两相系统(ATP),并作为用于脂肪酶提取的传统净化系统的有效替代品。在此,我们研究了使用ATP和含水两相胶束系统(ATPMS)从白孢素狼Scottii L117衍生的脂肪酶的分区和回收。因此,我们在不同分子量(1500,4000和8000g / mol)中评估了三个ATP:(I)聚乙二醇(PEG)/磷酸盐(磷脂)和(ii)PEG /聚丙烯酸(NAPA)。 (iii)在不同条件下的TRITON X-114(TX-114)/ McIlVaine缓冲液pH 7.0(22.0和28.0℃的TX-114的2.0%(w / w))。 PEG /磷酸盐和PEG / NAPA系统导致酶活性很大;因此,这些系统不代表这些脂肪酶提取的可行替代品。胶束系统产生了脂肪酶提取的最佳效果,酶活性平衡范围为84.7%至113.05%。通过实验设计优化胶束系统后,脂肪酸分配系数增加10.3倍(0.75-7.76)。脂肪酶优先用K-Lip = 7.76分配到富含胶束的相中,%Recbot = 93.85%,PF = 1.2,5.03℃,5.1 pH和10.38%TX-114和K唇,= 4.77,%RECBOT = 73.53 %和PF = 1.97,在28.00℃,4.5 pH和8.0%TX-114,表明ATPMS表示纯化/提取脂肪酶L Scottii L117的替代方案。还评估了粗脂肪酶提取物以定义最佳pH和温度。脂肪酶在40℃下达到最佳活性,并在pH值范围内稳定,从pH 3.0至8.0和20.0至45.0℃的温度,在孵育30分钟后,相对残余脂肪酶活性高于80%。 (c)2015 Elsevier B.v.保留所有权利。

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