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GPI anchor attachment is required for Gas1p transport from the endoplasmic reticulum in COP II vesicles.

机译:在COP II囊泡中从内质网运输Gas1p时需要GPI锚定附件。

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摘要

Inositol starvation of auxotrophic yeast interrupts glycolipid biosynthesis and prevents lipid modification of a normally glycosyl phosphatidylinositol (GPI)-linked protein, Gas1p. The unanchored Gas1p precursor undergoes progressive modification in the endoplasmic reticulum (ER), but is not modified by Golgi-specific glycosylation. Starvation-induced defects in anchor assembly and protein processing are rapid, and occur without altered maturation of other proteins. Cells remain competent to manufacture anchor components and to process Gas1p efficiently once inositol is restored. Newly synthesized Gas1p is packaged into vesicles formed in vitro from perforated yeast spheroplasts incubated with either yeast cytosol or the purified Sec proteins (COP II) required for vesicle budding from the ER. In vitro synthesized vesicles produced by inositol-starved membranes do not contain detectable Gas1p. These studies demonstrate that COP II components fulfill the soluble protein requirements for packaging a GPI-anchored protein into ER-derived transport vesicles. However, GPI anchor attachment is required for this packaging to occur.
机译:营养缺陷型酵母的肌醇饥饿会中断糖脂的生物合成,并阻止通常与糖基磷脂酰肌醇(GPI)相连的蛋白Gas1p的脂质修饰。未锚定的Gas1p前体在内质网(ER)中进行渐进修饰,但未被高尔基体特异性糖基化修饰。饥饿诱导的锚蛋白装配和蛋白质加工缺陷很快发生,并且在其他蛋白质成熟度不变的情况下发生。肌醇恢复后,细胞仍然具有制造锚定成分和有效处理Gas1p的能力。将新合成的Gas1p包装到体外培养的小泡中,这些小泡是由穿孔的酵母原生质球与酵母细胞溶质或从ER囊泡出芽所需的纯化Sec蛋白(COP II)一起孵育而成的。由肌醇饥饿的膜产生的体外合成囊泡不含可检测的Gas1p。这些研究表明,COP II组分满足了将GPI锚定的蛋白包装到ER衍生的运输小泡中的可溶性蛋白要求。但是,需要使用GPI锚定附件才能进行此包装。

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