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Characterization, performance, and applications of a yeast surface display-based biocatalyst

机译:基于酵母表面展示的生物催化剂的表征,性能和应用

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摘要

This work demonstrates the efficacy and cost effectiveness of yeast surface display (YSD) as a method for producing and purifying enzyme catalysts. Lipase B from Candida antarctica ( CalB) and lipase from Photobacterium lipolyticum sp. M37 (M37L) were individually displayed on the surface of yeasts via fusion with alpha-agglutinin. The enzyme is produced, purified, and immobilized in a single step. The population expressing the enzyme was quantified by flow cytometry. After lyophilization, the hydrolytic activity of the biocatalyst was assayed with p-nitrophenyl butyrate and p-nitrophenyl palmitate substrates. Esterification reactions involving octanoic acid and either butanol or octanol were used to evaluate esterification activity. The lyophilized YSD biocatalyst hydrolytic activity matched or exceeded commercial lipase (Novozym 435) immobilized on acrylic resin at equal catalyst loading, and achieved esterification levels 10-50% that of Novozyme 435. Factoring in the cost of production, the YSD biocatalyst represents a considerable savings over traditionally prepared and purchased enzyme catalysts. This promises to significantly expand the catalytic applications of immobilized lipases, and immobilized enzymes more generally, in commercial processes.
机译:这项工作证明了酵母表面展示(YSD)作为生产和纯化酶催化剂的方法的功效和成本效益。来自南极假丝酵母(CalB)的脂肪酶B和来自解脂性细菌(Photobacter lipolyticum sp。)的脂肪酶。 M37(M37L)通过与α-凝集素融合而分别展示在酵母表面上。一步即可生产,纯化和固定酶。通过流式细胞术定量表达酶的群体。冻干后,用丁酸对硝基苯酯和棕榈酸对硝基苯酯底物测定生物催化剂的水解活性。涉及辛酸与丁醇或辛醇的酯化反应用于评估酯化活性。冻干的YSD生物催化剂的水解活性与固定在丙烯酸树脂上的商用脂肪酶(Novozym 435)在相同的催化剂负载量下达到或超过商业化的脂肪酶(Novozym 435),其酯化水平为Novozyme 435的10-50%。与传统制备和购买的酶催化剂相比节省了成本。这有望显着扩展固定化脂肪酶的催化应用,并且更广泛地将其固定化于商业化生产过程中。

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