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首页> 外文期刊>Applied biochemistry and biotechnology, Part A. enzyme engineering and biotechnology >Hydrolysis of Lactose by #beta#-Glycosidase CelB from Hyperthermophilic Archaeon Pyrococcus furiosus (Comparison of Hollow-Fiber Membrane and Packed-Bed Immobilized Enzyme Reactors for Continuous Processing of Ultrahigh Temperature-Treated Skim Milk)
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Hydrolysis of Lactose by #beta#-Glycosidase CelB from Hyperthermophilic Archaeon Pyrococcus furiosus (Comparison of Hollow-Fiber Membrane and Packed-Bed Immobilized Enzyme Reactors for Continuous Processing of Ultrahigh Temperature-Treated Skim Milk)

机译:嗜热古生热球菌#beta#-糖苷酶CelB水解乳糖(中空纤维膜和填充床固定酶反应器连续处理超高温脱脂牛奶的比较)

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摘要

Recombinant #beta#-glycosidase CelB from the hyperthermophilic archaeon Pyrococcus furiosus was produced through expression of the plasmid-encoded gene in Escherichia coli. Bioreactor cultivations of E. coli in the presence of the inductor isopropyl-1-thio-#beta#-D-galactoside (0.1 mM) gave approx 100,000 U of enzyme activity/L of culture medium after 8 h of growth. A technical-grade enzyme for the hydrolysis of lacatose was prepared by precipitating the mesophilic protein at 80 deg C. A hollow-fiber membrane reactor was developed, and its performance during continuous processing of ultrahigh temperature-treated (UHT) skin milk at 70 deg C was analyzed regarding long-term stability, productivity, and diffusional limitation thereof. CelB was covalently attached onto Eupergit C in yields of 80%, and a packed-bed immobilized enzyme reactor was used for the continuous hydrolysis of lactose in UHT skim milk at 70 deg C. The packed-bed reactor was approx = 10-fold more stable and gave about the same productivity at 80% substrate conversion as the hollow-fiber reactor at 60% substrate conversion. The marked difference in the stability of free and immobilized CelB seems to reflect mainly binding of the soluble enzyme to the membrane surface of the hollow-fiber module. Under these bound conditions, CelB is essentially inactive. CelB is essentially inactive. Microbial contamination of the reactors did not occur during reaction times of up to 39d, given that UHT skim milk and not pasteurized skim milk was used as the substrate.
机译:通过在大肠杆菌中表达质粒编码的基因,产生了来自超嗜热古生热球菌的重组#β#-糖苷酶CelB。在诱导剂异丙基-1-硫代-#β#-D-半乳糖苷(0.1 mM)存在下,大肠杆菌的生物反应器培养在生长8小时后,每培养基的酶活性约为100,000U。通过在80℃下沉淀嗜温蛋白来制备用于水解拉卡糖的工业级酶。开发了一种中空纤维膜反应器,其在70℃超高温处理(UHT)皮肤乳的连续加工过程中的性能分析了C的长期稳定性,生产率及其扩散极限。将CelB共价连接到Eupergit C上,产率为80%,并使用固定床固定化酶反应器在70℃下连续水解UHT脱脂乳中的乳糖。该固定床反应器的数量大约是原来的10倍稳定,在80%的底物转化率下获得的生产率与中空纤维反应器在60%的底物转化率下的生产率相同。游离的和固定的CelB的稳定性的明显差异似乎主要反映了可溶性酶与中空纤维组件膜表面的结合。在这些约束条件下,CelB本质上是不活动的。 CelB本质上是不活动的。假定使用UHT脱脂乳而不是巴氏杀菌脱脂乳作为底物,在长达39d的反应时间内不会发生反应器的微生物污染。

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