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固定化核糖核酸酶对核糖核酸的降解作用。

Degradation of ribonucleic acid by immobilized ribonuclease.

作者信息

Dale B E, White D H

出版信息

Biotechnol Bioeng. 1979 Sep;21(9):1639-48. doi: 10.1002/bit.260210910.

DOI:10.1002/bit.260210910
PMID:40630
Abstract

An immobilized enzyme (pancreatic ribonuclease bound to porous titania) was investigated for the degradation of purified yeast ribonucleic acid as a substrate. The immobilized enzyme is active and stable in the pH range 4--8. Dependence of enzymatic activity on ionic strength, pH, temperature, fluid flow rate, and substrate concentration were investigated. A cumulative fluid residence time of 6 sec is sufficient for 50% substrate conversion at 25 degrees C and pH 7.0. The critical flow rate (i.e., the fluid flow rate necessary to remove film diffusion resistance) approximately doubles with each 10 degree C rise in reaction temperature. The critical flow rates obtained in this study are about 40 times greater than those obtained for a similar study on immobilized glucose oxidase. Arrhenius plots gave activation energies of -9.6 and -7.1 kcal/g mol at pH 4.6 and 7.0, respectively. The work reported herein is a bench-scale investigation of an immobilized enzyme with primary emphasis on the mass transfer and kinetic characteristics of the system. The rapid reaction rates obtainable at relatively low temperatures offer a potential alternative method of purifying yeast single cell protein (SCP) with miminum loss of desired protein. The key questions are how such a system would react in a yeast homogenate, what conditions in such a system must be controlled, and what type of immobilized reactor should be utilized, if such further work continued to show promise.

摘要

研究了一种固定化酶(结合在多孔二氧化钛上的胰腺核糖核酸酶)对纯化的酵母核糖核酸作为底物的降解作用。该固定化酶在pH值4 - 8范围内具有活性且稳定。研究了酶活性对离子强度、pH值、温度、流体流速和底物浓度的依赖性。在25℃和pH值7.0时,累积流体停留时间为6秒足以实现50%的底物转化。临界流速(即消除膜扩散阻力所需的流体流速)随着反应温度每升高10℃大约增加一倍。本研究中获得的临界流速比类似的固定化葡萄糖氧化酶研究中获得的临界流速大约大40倍。阿累尼乌斯曲线分别在pH值4.6和7.0时给出的活化能为 -9.6和 -7.1千卡/克分子。本文报道的工作是对固定化酶的实验室规模研究,主要侧重于系统的传质和动力学特性。在相对较低温度下可获得的快速反应速率为以最小的所需蛋白质损失纯化酵母单细胞蛋白(SCP)提供了一种潜在的替代方法。关键问题是这样的系统在酵母匀浆中会如何反应,在这样的系统中必须控制哪些条件,以及如果进一步的工作继续显示出前景,应该使用哪种类型的固定化反应器。

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