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使用NAD(H)或NADP(H)作为辅因子体外酶促生产2-酮基-L-古龙酸的数学建模。

Mathematical modeling of in vitro enzymatic production of 2-Keto-L-gulonic acid using NAD(H) or NADP(H) as cofactors.

作者信息

Banta Scott, Boston Matt, Jarnagin Alisha, Anderson Stephen

机构信息

Department of Chemical and Biochemical Engineering, Rutgers, The State University of New Jersey, Piscataway 08854, USA.

出版信息

Metab Eng. 2002 Oct;4(4):273-84. doi: 10.1006/mben.2002.0231.

Abstract

A 2-Keto-L-gulonic acid (2-KLG) production process using stationary Pantoea citrea cells and a Corynebacterium 2,5-diketo-D-gluconic acid (2,5-DKG) reductase enzyme has been developed which may represent an improved method of vitamin C biosynthesis. Experimental data was collected using the F22Y/A272G 2,5-DKG reductase mutant and NADP(H) as a cofactor. An extensive kinetic analysis was performed and a kinetic rate equation model for this process was developed. A recent protein engineering effort has resulted in several 2,5-DKG reductase mutants exhibiting improved activity with NADH as a cofactor. The use of NAD(H) in the bioreactor may be preferable due to its increased stability and lower cost. The kinetic parameters in the rate equation model have been replaced in order to predict 2-KLG production with NAD(H) as a cofactor. The model was also extended to predict 2-KLG production in the presence of a range of combined cofactor concentrations. This analysis suggests that the use of the F22Y/K232G/R238H/A272G 2,5-DKG reductase mutant with NAD(H) combined with a small amount of NADP(H) could provide a significant cost benefit for in vitro enzymatic 2-KLG production.

摘要

已经开发出一种使用固定化柑橘泛菌细胞和棒状杆菌2,5-二酮-D-葡萄糖酸(2,5-DKG)还原酶生产2-酮-L-古龙酸(2-KLG)的方法,这可能是一种改进的维生素C生物合成方法。使用F22Y/A272G 2,5-DKG还原酶突变体和NADP(H)作为辅因子收集了实验数据。进行了广泛的动力学分析,并建立了该过程的动力学速率方程模型。最近的蛋白质工程工作产生了几个以NADH作为辅因子表现出更高活性的2,5-DKG还原酶突变体。由于其稳定性提高和成本较低,在生物反应器中使用NAD(H)可能更可取。速率方程模型中的动力学参数已被替换,以便预测以NAD(H)作为辅因子时2-KLG的产量。该模型还被扩展以预测在一系列组合辅因子浓度存在下2-KLG的产量。该分析表明,使用F22Y/K232G/R238H/A272G 2,5-DKG还原酶突变体与NAD(H)并结合少量NADP(H)可为体外酶促生产2-KLG提供显著的成本效益。

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