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Monitoring Lipase/Esterase Activity by Stopped Flow in a Sequential Injection Analysis System Using p-Nitrophenyl Butyrate

机译:在使用对硝基苯基丁酸的顺序注射分析系统中通过停止流动监测脂肪酶/酯酶的活性

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摘要

Lipases and esterases are biocatalysts used at the laboratory and industrial level. To obtain the maximum yield in a bioprocess, it is important to measure key variables, such as enzymatic activity. The conventional method for monitoring hydrolytic activity is to take out a sample from the bioreactor to be analyzed off-line at the laboratory. The disadvantage of this approach is the long time required to recover the information from the process, hindering the possibility to develop control systems. New strategies to monitor lipase/esterase activity are necessary. In this context and in the first approach, we proposed a lab-made sequential injection analysis system to analyze off-line samples from shake flasks. Lipase/esterase activity was determined using p-nitrophenyl butyrate as the substrate. The sequential injection analysis allowed us to measure the hydrolytic activity from a sample without dilution in a linear range from 0.05–1.60 U/mL, with the capability to reach sample dilutions up to 1000 times, a sampling frequency of five samples/h, with a kinetic reaction of 5 min and a relative standard deviation of 8.75%. The results are promising to monitor lipase/esterase activity in real time, in which optimization and control strategies can be designed.
机译:脂肪酶和酯酶是在实验室和工业水平上使用的生物催化剂。为了在生物过程中获得最大产量,重要的是测量关键变量,例如酶活性。监测水解活性的常规方法是从生物反应器中取出要在实验室离线分析的样品。这种方法的缺点是从过程中恢复信息需要很长时间,从而阻碍了开发控制系统的可能性。监测脂肪酶/酯酶活性的新策略是必要的。在这种情况下,在第一种方法中,我们提出了一种实验室制造的顺序进样分析系统来分析摇瓶中的离线样品。使用对硝基苯基丁酸酯作为底物测定脂肪酶/酯酶活性。顺序进样分析使我们能够以0.05–1.60 U / mL的线性范围测量未经稀释的样品的水解活性,能够达到高达1000倍的样品稀释度,采样频率为五个样品/小时, 5分钟的动力学反应和8.75%的相对标准偏差。该结果有望实时监测脂肪酶/酯酶活性,从而可以设计优化和控制策略。

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