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A screen for over-secretion of proteins by yeast based on a dual component cellular phosphatase and immuno-chromogenic stain for exported bacterial alkaline phosphatase reporter

机译:基于双组分细胞磷酸酶和免疫显色染料的酵母过分泌蛋白筛查用于输出细菌碱性磷酸酶报道分子

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摘要

BackgroundTo isolate over-secretors, we subjected to saturation mutagenesis, a strain of P.pastoris exporting E. coli alkaline phosphatase (EAP) fused to the secretory domain of the yeast α factor pheromone through cellular PHO1/KEX2 secretory processing signals as the α-sec-EAP reporter protein. Direct chromogenic staining for α-sec-EAP activity is non-specific as its NBT/BCIP substrate cross-reacts with cellular phosphatases which can be inhibited with Levulinic acid. However, the parental E(P) strain only exports detectable levels of α-sec-EAP at 69 hours and not within the 36 hour period post-seeding required for effective screening with the consequent absence of a reference for secretion. We substituted the endogenous cellular phosphatase activity as a comparative reference for secretion rate and levels as well as for colony alignment while elevating specificity and sensitivity of detection of the exported protein with other innovative modifications of the immuno-chromogenic staining application for screening protein export mutants.
机译:背景为了分离过分泌物,我们进行了饱和诱变,这是一种通过细胞PHO1 / KEX2分泌加工信号将酵母碱性磷酸酶(EAP)菌株通过细胞PHO1 / KEX2分泌加工信号与酵母α因子信息素的分泌结构域融合为α- sec-EAP报告蛋白。 α-sec-EAP活性的直接显色染色是非特异性的,因为其NBT / BCIP底物与细胞磷酸酶发生交叉反应,而磷酸酶可以被Levulinic acid抑制。然而,亲本E(P)菌株仅在69小时输出可检测水平的α-sec-EAP,而不在有效筛选所需的播种后36小时内输出,因此没有分泌参考。我们用内源性细胞磷酸酶的活性作为分泌速率和水平以及菌落排列的比较参考,同时提高了输出蛋白检测的特异性和灵敏度,同时对免疫显色染色应用进行了其他创新性修饰,以筛选蛋白输出突变体。

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