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A Single Mutation in the Activation Site of Bovine Trypsinogen Enhances Its Accumulation in the Fermentation Broth of the Yeast Pichia pastoris

机译:牛胰蛋白酶原激活位点的单一突变会增加其在酵母毕赤酵母发酵液中的积累

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摘要

We produced bovine trypsinogen in the yeast Pichia pastoris. Little or no trypsinogen was detected when the gene with its native leader sequence was expressed under the control of the strong aox1 promoter, suggesting that expression of the wild-type bovine trypsinogen was toxic to the cells. We altered the trypsinogen native propeptide sequence by replacing the lysine at position 6 with an aspartic acid, thus destroying the site in the propeptide cleaved by enterokinase and by trypsin. This mutant accumulated up to 10 mg of trypsinogen per liter in shake flask cultures and about 40 mg/liter in 6-liter fermentors. Trypsinogen could be activated in vitro with a dipeptidyl-aminopeptidase, which selectively removed the modified trypsinogen propeptide; the resulting trypsin was fully active and showed evidence of glycosylation. Thus, we have developed a novel protein production scheme that can be used for the expression of proteins, such as proteases, that are deleterious to the producing organism. This system relies on the expression of a zymogen that cannot be activated in vivo coupled with its in vitro purification and activation.
机译:我们在巴斯德毕赤酵母中产生了牛胰蛋白酶原。当具有其天然前导序列的基因在强aox1启动子的控制下表达时,几乎没有检测到胰蛋白酶原,这表明野生型牛胰蛋白酶原的表达对细胞有毒性。我们通过用天冬氨酸替换6位上的赖氨酸来改变胰蛋白酶原的天然前肽序列,从而破坏了经肠激酶和胰蛋白酶切割的前肽中的位点。该突变体在摇瓶培养物中每升累积高达10 mg胰蛋白酶原,在6升发酵罐中累积约40 mg / L。胰蛋白酶原可以在体外用二肽基氨基肽酶激活,该酶选择性地除去修饰的胰蛋白酶原前肽。所得的胰蛋白酶具有充分的活性,并显示出糖基化的迹象。因此,我们开发了一种新颖的蛋白质生产方案,该方案可用于表达对生产生物有害的蛋白质,例如蛋白酶。该系统依赖不能在体内被激活的酶原的表达及其体外纯化和激活。

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