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Cloning of the Membrane-Bound Aldehyde Dehydrogenase Gene of Acetobacter polyoxogenes and Improvement of Acetic Acid Production by Use of the Cloned Gene

机译:多产醋杆菌膜结合醛脱氢酶基因的克隆及利用该克隆基因提高乙酸产量

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摘要

A genomic clone bank of Acetobacter polyoxogenes NBI1028 constructed in Escherichia coli by use of the expression vector pUC18 was screened with antibody raised against membrane-bound aldehyde dehydrogenase (ALDH; 75 kilodaltons [kDa]) from A. polyoxogenes NBI1028. A clone that synthesized a 41-kDa protein cross-reactive with anti-ALDH antibody was isolated. For cloning of the full-length ALDH structural gene, a cosmid gene bank was screened by Southern blot hybridization with the cloned DNA as a probe, and subcloning from the positive cosmid clone was performed with shuttle vector pMV24. Plasmid pAL25, containing the full-length ALDH structural gene, was isolated and expressed in both E. coli and Acetobacter aceti to produce a fused protein (78 kDa) with a short NH2-terminal β-galactosidase peptide. pAL25 conferred ALDH production on a mutant of A. aceti lacking the enzyme activity. Transformation of A. aceti subsp. xylinum NBI2099 with pAL25 caused 2- and 1.4-fold increases in the production rate and in the maximum concentration of acetic acid in submerged fermentation, respectively.
机译:利用表达载体pUC18在大肠杆菌中构建的多氧醋杆菌醋杆菌NBI1028的基因组克隆库,用针对多氧合酶杆菌NBI1028的膜结合醛脱氢酶(ALDH; 75道尔顿[kDa])产生的抗体进行筛选。分离出合成了与抗ALDH抗体交叉反应的41 kDa蛋白的克隆。为了克隆全长ALDH结构基因,通过以所克隆的DNA作为探针的Southern印迹杂交来筛选粘粒基因库,并用穿梭载体pMV24从阳性粘粒克隆中进行亚克隆。分离出含有全长ALDH结构基因的质粒pAL25,并在大肠杆菌和醋杆菌中表达,以产生具有短NH 2末端β-半乳糖苷酶肽的融合蛋白(78 kDa)。 pAL25赋予缺乏酶活性的醋曲霉突变体ALDH产生。乙酰丙酮杆菌亚种的转化带有pAL25的木霉NBI2099分别导致淹没式发酵的生产率和最大乙酸浓度分别提高2倍和1.4倍。

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