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用于β-丙氨酸生产的依赖于吡哆醛-5'-磷酸的 l-天冬氨酸-α-脱羧酶的蛋白质工程。

Protein Engineering of a Pyridoxal-5'-Phosphate-Dependent l-Aspartate-α-Decarboxylase from for β-Alanine Production.

机构信息

Key Laboratory of Bioorganic Synthesis of Zhejiang Province, College of Biotechnology and Bioengineering, Zhejiang University of Technology, No.18, Chaowang Road, Hangzhou 310014, China.

出版信息

Molecules. 2020 Mar 12;25(6):1280. doi: 10.3390/molecules25061280.

Abstract

In the present study, a pyridoxal-5'-phosphate (PLP)-dependent L-aspartate-α-decarboxylase from (TcPanD) was selected for protein engineering to efficiently produce β-alanine. A mutant PanD-R98H/K305S with a 2.45-fold higher activity than the wide type was selected through error-prone PCR, site-saturation mutagenesis, and 96-well plate screening technologies. The characterization of purified enzyme TcPanD-R98H/K305S showed that the optimal cofactor PLP concentration, temperature, and pH were 0.04% (), 50 °C, and 7.0, respectively. The 1mM of Na, Ni, Co, K, and Ca stimulated the activity of TcPanD-R98H/K305S, while only 5 mM of Ni and Na could increase its activity. The kinetic analysis indicated that TcPanD-R98H/K305S had a higher substrate affinity and enzymatic reaction rate than the wild enzyme. A total of 267 g/L substrate l-aspartic acid was consumed and 170.5 g/L of β-alanine with a molar conversion of 95.5% was obtained under the optimal condition and 5-L reactor fermentation.

摘要

在本研究中,选择来自 (TcPanD)的依赖于吡哆醛-5'-磷酸(PLP)的 L-天冬氨酸-α-脱羧酶进行蛋白质工程,以高效生产β-丙氨酸。通过易错 PCR、定点饱和突变和 96 孔板筛选技术,选择了一种突变体 PanD-R98H/K305S,其比野生型的酶活提高了 2.45 倍。对纯化的酶 TcPanD-R98H/K305S 的特性研究表明,最佳辅因子 PLP 浓度、温度和 pH 值分别为 0.04%()、50°C 和 7.0。1mM 的 Na、Ni、Co、K 和 Ca 均能刺激 TcPanD-R98H/K305S 的活性,而只有 5mM 的 Ni 和 Na 能提高其活性。动力学分析表明,TcPanD-R98H/K305S 对底物的亲和力和酶促反应速率均高于野生酶。在最佳条件和 5-L 发酵罐发酵下,共消耗 267g/L 的底物 L-天冬氨酸,获得 170.5g/L 的β-丙氨酸,摩尔转化率为 95.5%。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3b4b/7143960/65856bfaae3b/molecules-25-01280-g001.jpg

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