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Investigation of the Amycolatopsis sp. Strain ATCC 39116 Vanillin Dehydrogenase and Its Impact on the Biotechnical Production of Vanillin

机译:支链淀粉菌的调查。 ATCC 39116香兰素脱氢酶及其对香兰素生物技术生产的影响

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摘要

The actinomycete Amycolatopsis sp. strain ATCC 39116 is capable of synthesizing large amounts of vanillin from ferulic acid, which is a natural cell wall component of higher plants. The desired intermediate vanillin is subject to undesired catabolism caused by the metabolic activity of a hitherto unknown vanillin dehydrogenase (VDHATCC 39116). In order to prevent the oxidation of vanillin to vanillic acid and thereby to obtain higher yields and concentrations of vanillin, the responsible vanillin dehydrogenase in Amycolatopsis sp. ATCC 39116 was investigated for the first time by using data from our genome sequence analysis and further bioinformatic approaches. The vdh gene was heterologously expressed in Escherichia coli, and the encoded vanillin dehydrogenase was characterized in detail. VDHATCC 39116 was purified to apparent electrophoretic homogeneity and exhibited NAD+-dependent activity toward vanillin, coniferylaldehyde, cinnamaldehyde, and benzaldehyde. The enzyme showed its highest level of activity toward vanillin at pH 8.0 and at a temperature of 44°C. In a next step, a precise vdh deletion mutant of Amycolatopsis sp. ATCC 39116 was generated. The mutant lost its ability to grow on vanillin and did not show vanillin dehydrogenase activity. A 2.3-times-higher vanillin concentration and a substantially reduced amount of vanillic acid occurred with the Amycolatopsis sp. ATCC 39116 Δvdh::Kmr mutant when ferulic acid was provided for biotransformation in a cultivation experiment on a 2-liter-bioreactor scale. Based on these results and taking further metabolic engineering into account, the Amycolatopsis sp. ATCC 39116 Δvdh::Kmr mutant represents an optimized and industrially applicable platform for the biotechnological production of natural vanillin.
机译:放线菌淀粉样芽胞杆菌。 ATCC 39116菌株能够从阿魏酸合成大量香兰素,阿魏酸是高等植物的天然细胞壁成分。所需的中间香兰素由于迄今未知的香兰素脱氢酶(VDHATCC 39116)的代谢活性而导致不希望的分解代谢。为了防止香兰素氧化为香兰酸,从而获得更高的产量和浓度的香兰素,在霉菌属菌种中负责的香兰素脱氢酶。通过使用我们的基因组序列分析和其他生物信息学方法获得的数据,首次对ATCC 39116进行了研究。 vdh基因在大肠杆菌中异源表达,并详细描述了编码的香兰素脱氢酶。 VDHATCC 39116纯化至明显的电泳均一性,并且对香兰素,松柏树醛,肉桂醛和苯甲醛表现出NAD + 依赖性活性。该酶在pH 8.0和44°C的温度下对香草醛具有最高活性。下一步,是精确的Amycolatopsis sp。的vdh缺失突变体。生成了ATCC 39116。该突变体失去了在香草醛上生长的能力,并且没有显示香草醛脱氢酶活性。支链淀粉菌种的香草醛浓度升高了2.3倍,香草酸含量大大降低。当在2升生物反应器规模的培养实验中提供阿魏酸进行生物转化时,ATCC 39116Δvdh:: Km r 突变体。基于这些结果,并考虑到进一步的代谢工程,Amycolatopsis sp。 ATCC 39116Δvdh:: Km r 突变体代表了天然香兰素生物技术生产的优化和工业应用平台。

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