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Human MUC5AC mucin dimerizes in the rough endoplasmic reticulum similarly to the MUC2 mucin.

机译:与MUC2粘蛋白相似人MUC5AC粘蛋白在粗糙的内质网中二聚。

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摘要

Biosynthetic studies on the human MUC5AC mucin were performed by immunoprecipitations with antisera recognizing only the non-O-glycosylated apomucin in the colon adenocarcinoma cell line LS 174T. Pulse-chase studies and subcellular fractionations showed that MUC5AC formed dimers in the rough endoplasmic reticulum within 15 min of the initiation of biosynthesis. No non-O-glycosylated species larger than dimers were identified. The dimerization was N-glycosylation-dependent, because tunicamycin treatment significantly lowered the rate of dimerization. When the biosynthesis of MUC5AC apomucin was compared with that of MUC2 apomucin, also produced in the LS 174T cell line, both apomucins were assembled in similar ways with respect to their rates of dimerization with and without inhibition of N-glycosylation. No heterodimerization was observed between the human MUC5AC and the MUC2 apomucins despite the extensive sequence similarities in the positions of the cysteine residues in the C-termini proposed to be involved in mucin dimerization.
机译:对人MUC5AC粘蛋白的生物合成研究是通过免疫沉淀进行的,抗血清仅识别结肠腺癌细胞LS 174T中非O-糖基化的载脂蛋白。脉冲追踪研究和亚细胞分级分离显示,MUC5AC在生物合成开始后15分钟内在粗糙的内质网中形成了二聚体。没有发现大于二聚体的非O-糖基化物质。二聚化是N-糖基化依赖性的,因为衣霉素处理显着降低了二聚化速率。当将同样在LS 174T细胞系中生产的MUC5AC载脂蛋白的生物合成与MUC2载脂蛋白的生物合成进行比较时,两种载脂蛋白的二聚化速率(具有和不具有抑制N-糖基化的能力)的组装方式均相似。尽管有人提出参与粘蛋白二聚化的C-末端的半胱氨酸残基的位置具有广泛的序列相似性,但在人MUC5AC和MUC2载脂蛋白之间未观察到异二聚化。

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