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Investigating the role of ERAD on antibody processing in glycoengineered Saccharomyces cerevisiae

机译:调查Erad对甘油酵母酿酒酵母群抗体加工的作用

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N-glycosylation plays an important role in the endoplasmic reticulum quality control (ERQC). N-glycan biosynthesis pathways have been engineered in yeasts and fungi to enable the production of therapeutic glycoproteins with human-compatible N-glycosylation, and some glycoengineering approaches alter the synthesis of the lipid-linked oligosaccharide (LLO). Because the effects of LLO engineering on ERQC are currently unknown, we characterized intracellular processing of IgG in glycoengineered Delta alg3 Delta alg11 Saccharomyces cerevisiae strain and analyzed how altered LLO structures affect endoplasmic reticulum-associated degradation (ERAD). Intracellular IgG light and heavy chain molecules expressed in Delta alg3 Delta alg11 strain are ERAD substrates and targeted to ERAD independently of Yos9p and Htm1p, whereas in the presence of ALG3 ERAD targeting is dependent on Yos9p but does not require Htm1p. Blocking of ERAD accumulated ER and post-Golgi forms of IgG and increased glycosylation of mat alpha secretion signal but did not improve IgG secretion. Our results show ERAD targeting of a heterologous glycoprotein in yeast, and suggest that proteins in the ER can be targeted to ERAD via other mechanisms than the Htm1p-Yos9p-dependent route when the LLO biosynthesis is altered.
机译:N-糖基化在内质网质量控制(ERQC)中起重要作用。 N-聚糖生物合成途径已在酵母和真菌中设计,以使得能够用人类相容的N-糖基化产生治疗性糖蛋白,并且一些甘油化方法改变了脂质连接的寡糖(LLO)的合成。由于LLO工程对ERQC的影响目前未知,所以我们表征了甘油替辛δ血糖11阶段IgG的IgG内加工,并分析了LLO结构改变如何影响内质网相关的降解(ERAD)。在Delta ALG3 Delta ALG11菌株中表达的细胞内IgG光和重链分子是Erad基材,并且靶向以YOS9P和HTM1P独立于ERAD,而在ALG3的存在中,ERAD靶向取决于YOS9P,但不需要HTM1P。阻断ERAD累积的ER和后GOLGI形式的IgG和增加乳头α分泌信号的糖基化,但未改善IgG分泌。我们的结果显示Erad靶向酵母中异源糖蛋白的靶向,并表明ER中的蛋白质可以在改变LLO生物合成的情况下通过其他机制来靶向ERAD。

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