[Expression Of DNA-Encoded Antidote to Organophosphorus Toxins in the Methylotrophic Yeast Pichia Pastoris].

S S Terekhov, T V Bobik, Yu A Mokrushina, A V Stepanova, N M Aleksandrova, I V Smirnov, A A Belogurov, N A Ponomarenko, A G Gabibov
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Abstract

A platform for the cloning and expression of active human butyrylcholinesterase (BuChE) in the yeast Pichia pastoris is first presented. Genetic constructs for BuChE gene expression, separately and in conjunction with a proline-rich peptide called proline-rich attachment domain (PRAD), are based on the vector pPICZαA. It is shown that the highest level of production is achieved in the expression of a BuChE gene without PRAD pPICZαA. It is found that one can obtain up to 125 mg of active enzyme from 1 L of culture medium at an optimal pH environment (pH 7.6), an optical seed culture density of 3 o.u., and an optimum methanol addition mode of (0.5% methanol in the first day and 0.2% thereafter from the second day).

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[甲基营养酵母毕赤酵母中有机磷毒素解毒剂的dna编码表达]。
本文首次提出了酵母毕赤酵母中活性人丁基胆碱酯酶(BuChE)的克隆和表达平台。BuChE基因表达的遗传构建,单独或与富含脯氨酸的肽称为脯氨酸-富附着域(PRAD)结合,基于载体ppicz - α a。结果表明,不含PRAD的BuChE基因ppicz - α a的表达量最高。研究发现,在最佳pH环境(pH 7.6)下,从1 L培养基中可以获得高达125 mg的酶,光学种子培养密度为3 μ u,最佳甲醇添加模式为(第一天添加0.5%甲醇,第二天添加0.2%甲醇)。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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