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Metabolically programmed quality control system for dolichol-linked oligosaccharides

机译:代谢性程序化质量控制体系用于与链烷醇连接的低聚糖

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摘要

The glycolipid Glc3Man9GlcNAc2-pyrophosphate-dolichol serves as the precursor for asparagine (N)-linked protein glycosylation in mammals. The biosynthesis of dolichol-linked oligosaccharides (DLOs) is arrested in low-glucose environments via unknown mechanisms, resulting in abnormal N-glycosylation. Here, we show that under glucose deprivation, DLOs are prematurely degraded during the early stages of DLO biosynthesis by pyrophosphatase, leading to the release of singly phosphorylated oligosaccharides into the cytosol. We identified that the level of GDP-mannose (Man), which serves as a donor substrate for DLO biosynthesis, is substantially reduced under glucose deprivation. We provide evidence that the selective shutdown of the GDP-Man biosynthetic pathway is sufficient to induce the release of phosphorylated oligosaccharides. These results indicate that glucose-regulated metabolic changes in the GDP-Man biosynthetic pathway cause the biosynthetic arrest of DLOs and facilitate their premature degradation by pyrophosphatase. We propose that this degradation system may avoid abnormal N-glycosylation with premature oligosaccharides under conditions that impair efficient DLO biosynthesis.
机译:糖脂Glc3Man9GlcNAc2-焦磷酸二氢乙醇用作哺乳动物中与天冬酰胺(N)连接的蛋白质糖基化的前体。在低葡萄糖环境中,通过未知机制阻止了与直链连接的寡糖(DLO)的生物合成,从而导致异常的N-糖基化。在这里,我们显示在葡萄糖剥夺下,DLO在焦磷酸酶DLO生物合成的早期阶段过早降解,导致单个磷酸化的寡糖释放到细胞质中。我们发现,在葡萄糖剥夺下,作为DLO生物合成供体的GDP-甘露糖(Man)的水平已大大降低。我们提供的证据表明,GDP-Man生物合成途径的选择性关闭足以诱导磷酸化寡糖的释放。这些结果表明,GDP-Man生物合成途径中葡萄糖调节的代谢变化会导致DLO的生物合成停滞,并促进焦磷酸酶使其过早降解。我们建议该降解系统可以避免在损害有效DLO生物合成的条件下,过早的寡糖发生异常的N-糖基化。

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