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A novel and simple method for the purification of extracellular levansucrase from Zymomonas mobilis

机译:一种从运动发酵单胞菌中纯化细胞外葡聚糖的新方法

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A new and simple method for the purification of extracellular levansucrase from Zymomonas mobilis from highly viscous fermentation broth was developed. After incubation of the fermentation broth with a fructose-polymer cleaving enzyme preparation (Fructozyme, Novozymes, DK) for 48 h, levansucrase precipitated as aggregates and was redissolved in a 3 M urea solution. By ongoing size-exclusion chromatography on Sephacryl S-300 the final levansucrase preparation was purified 100-fold and exhibited a specific activity of 25-35 U/mg(protein). The levansucrase was stable in 3 M urea solution for at least four months without inactivation. To maximize the enzyme yield the dynamic changes of extracellular levansucrase activity during fermentation were investigated. The highest levansucrase activity was observed during the logarithmic phase of growth (15-19 h of fermentation).
机译:开发了一种从高粘度发酵液中纯化运动发酵单胞菌胞外葡聚糖的新方法。将发酵液与果糖聚合物裂解酶制剂(果糖酶,Novozymes,DK)孵育48小时后,左蔗糖酶沉淀为聚集体,并重新溶解在3 M尿素溶液中。通过正在进行的Sephacryl S-300尺寸排阻色谱法,最终的蔗糖酶制剂纯化了100倍,并显示出25-35 U / mg(蛋白质)的比活性。葡聚糖蔗糖酶在3M尿素溶液中稳定至少四个月而没有失活。为了使酶的产量最大化,研究了发酵过程中细胞外葡聚糖酶活性的动态变化。在对数生长期(发酵15-19小时)观察到最高的蔗糖酶活性。

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