Barnes G, Hansen W J, Holcomb C L, Rine J
Mol Cell Biol. 1984 Nov;4(11):2381-8. doi: 10.1128/mcb.4.11.2381-2388.1984.
Asparagine-linked glycosylation is a form of covalent modification that distinguishes proteins that are either membrane bound or are in cellular compartments topologically outside of the cell from those proteins that remain soluble in the cytoplasm. This type of glycosylation occurs stepwise, with core oligosaccharide added in the endoplasmic reticulum and subsequent modifications occurring in the golgi. We used tunicamycin, an inhibitor of one of the earliest steps in the synthesis of N-linked oligosaccharide, to select for mutants that are resistant to this antibiotic. Genetic, biochemical, and physiological experiments led to the following conclusions. The synthesis of N-linked oligosaccharide is an essential function in cells. In contrast to mammalian cells, yeast cells do not transport tunicamycin by a glucosamine transport function. We identified a gene, ALG7, that is probably the structural gene for UDP-N-acetylglucosamine-1-P transferase, the enzyme inhibited by tunicamycin. Dominant mutations in this gene result in increased activity of the transferase and loss of the ability of the cell to sporulate. In addition, we identified another gene, TUN1, in which recessive mutations result in resistance to tunicamycin. The ALG7 and TUN1 genes both map on chromosome VII.
天冬酰胺连接的糖基化是一种共价修饰形式,它将膜结合蛋白或细胞拓扑结构上位于细胞外的细胞区室中的蛋白与那些仍溶于细胞质的蛋白区分开来。这种类型的糖基化是逐步发生的,核心寡糖在内质网中添加,随后的修饰发生在高尔基体中。我们使用衣霉素(一种N-连接寡糖合成最早步骤之一的抑制剂)来筛选对这种抗生素具有抗性的突变体。遗传学、生物化学和生理学实验得出了以下结论。N-连接寡糖的合成是细胞中的一项基本功能。与哺乳动物细胞不同,酵母细胞不会通过葡糖胺转运功能转运衣霉素。我们鉴定出一个基因ALG7,它可能是被衣霉素抑制的酶UDP-N-乙酰葡糖胺-1-P转移酶的结构基因。该基因中的显性突变导致转移酶活性增加以及细胞形成孢子能力的丧失。此外,我们鉴定出另一个基因TUN1,其中的隐性突变导致对衣霉素具有抗性。ALG7和TUN1基因都位于第七条染色体上。
