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Glycosyl-phosphatidylinositol anchor attachment in a yeast in vitro system.

机译:糖基磷脂酰肌醇锚定在酵母体外系统中。

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摘要

The yeast mating pheromone precursor prepro-alpha factor was fused to C-terminal signals for glycosyl-phosphatidylinositol (GPI) anchor attachment, based on the sequence of the Saccharomyces cerevisiae protein Gas1p. Maturation of fusion proteins expressed in vivo required the presence of both a functional GPI attachment site and the synthesis of GPI precursors. Constructs were translated in vitro for use in cell-free studies of glycolipid attachment. The radiolabelled polypeptides were post-translationally translocated into yeast microsomes, where at least one third of the molecules received a GPI anchor. This approach offers distinct advantages over anchor attachment reactions that require co-translational translocation of secretory peptide substrates.
机译:根据酿酒酵母蛋白Gas1p的序列,将酵母交配信息素前体前原α因子融合到糖基磷脂酰肌醇(GPI)锚定附件的C端信号上。体内表达的融合蛋白的成熟需要功能性GPI附着位点和GPI前体的合成。将构建体体外翻译以用于糖脂附着的无细胞研究。放射性标记的多肽被翻译后转移到酵母微粒体内,其中至少三分之一的分子接受了GPI锚。与需要分泌肽底物进行共翻译易位的锚定附着反应相比,该方法具有明显的优势。

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