工程化 L-谷氨酸氧化酶作为全细胞生物催化剂以提高 α-酮戊二酸的产量。
Engineering of L-glutamate oxidase as the whole-cell biocatalyst for the improvement of α-ketoglutarate production.
机构信息
Key Laboratory of Food Nutrition and Safety, Ministry of Education, Tianjin University of Science and Technology, Tianjin, 300457, PR China; Tianjin Institute of Industrial Biotechnology, Chinese Academy of Sciences, Tianjin 300308, PR China.
Tianjin Institute of Industrial Biotechnology, Chinese Academy of Sciences, Tianjin 300308, PR China; Key Laboratory of Systems Microbial Biotechnology, Tianjin Institute of Industrial Biotechnology, Chinese Academy of Sciences, Tianjin, 300308, PR China.
出版信息
Enzyme Microb Technol. 2020 May;136:109530. doi: 10.1016/j.enzmictec.2020.109530. Epub 2020 Jan 30.
L-glutamate oxidase (LGOX) catalyzes the oxidative deamination of l-glutamate to α-ketoglutarate (α-KG) with the formation of ammonia and hydrogen peroxide. Consequently, identifying a novel LGOX with high enzymatic activity is a prime target for industrial biotechnology. In this study, error-prone PCR mutagenesis of Streptomyces mobaraensis LGOX followed by high-throughput screening was performed to yield four single point mutants with improved enzymatic activity, termed F94L, S280T, I282M and H533R. Moreover, site-saturation mutagenesis at these four residues was employed, yielding two additionally improved mutants, termed I282L and H533L. Subsequently, we employed combinatorial mutagenesis of two, three and four point mutants, and the best mutant S280TH533L showed 90 % higher enzymatic activity than the wild-type control. The data also showed that the presence of these point mutations greatly enhanced enzymatic activity, but did not alter its optimum temperature and pH. Furthermore, the S280TH533L mutant had the maximal velocity (V) of 231.3 μmol/mg/min and the Michaelis-Menten constant (K) of 2.7 mM, which were the highest V and lowest K values of LGOX reported so far. Finally, we developed a whole-cell biocatalyst for α-KG production by co-expression of both S280TH533L mutant and KatE catalase. Randomized ribosome binding site (RBS) sequences were introduced to generate vectors with varying expression levels of S280TH533L and KatE, and two optimized co-expression strains were obtained after screening. The α-KG production reached a maximum titer of 181.9 g/L after 12 h conversation using the optimized whole-cell biocatalyst, with a molar conversion rate of substrate higher than 86.3 % in the absence of exogenous catalase, while the molar conversion rate of substrate using the wild-type biocatalyst was less than 30 %. Taken together, these data suggest that the engineering of LGOX has great potentials to enhance the industrial production of α-KG.
谷氨酸氧化酶(LGOX)催化 L-谷氨酸的氧化脱氨反应,生成 α-酮戊二酸(α-KG)、氨和过氧化氢。因此,鉴定具有高酶活性的新型 LGOX 是工业生物技术的首要目标。在这项研究中,对莫拉氏链霉菌 LGOX 进行易错 PCR 诱变,然后进行高通量筛选,得到了四个单点突变体,其酶活性得到了提高,分别命名为 F94L、S280T、I282M 和 H533R。此外,在这四个残基上进行定点饱和突变,得到了另外两个提高的突变体,分别命名为 I282L 和 H533L。随后,我们采用了两个、三个和四个点突变体的组合诱变,最佳突变体 S280TH533L 的酶活性比野生型对照提高了 90%。数据还表明,这些点突变的存在极大地提高了酶活性,但没有改变其最适温度和 pH 值。此外,S280TH533L 突变体的最大速度(V)为 231.3 μmol/mg/min,米氏常数(K)为 2.7 mM,这是迄今为止报道的 LGOX 中 V 最高和 K 最低的值。最后,我们通过共表达 S280TH533L 突变体和 KatE 过氧化氢酶,开发了一种用于 α-KG 生产的全细胞生物催化剂。引入随机核糖体结合位点(RBS)序列,生成了具有不同 S280TH533L 和 KatE 表达水平的载体,并通过筛选得到了两个优化的共表达菌株。优化后的全细胞生物催化剂在 12 小时的转化后,α-KG 的产量达到了 181.9 g/L 的最高浓度,在没有外源过氧化氢酶的情况下,底物的摩尔转化率高于 86.3%,而使用野生型生物催化剂时,底物的摩尔转化率低于 30%。综上所述,这些数据表明,LGOX 的工程改造具有很大的潜力,可以提高 α-KG 的工业生产。
Zotero 插件