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Loss of hydroxyl groups from the ceramide moiety can modify the lateral diffusion of membrane proteins in S. cerevisiae

机译:神经酰胺部分的羟基丢失会改变酿酒酵母中膜蛋白的横向扩散

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摘要

In the yeast Saccharomyces cerevisiae, structural diversities of complex sphingolipids [inositol phosphorylceramide (IPC), mannosylinositol phosphorylceramide, and mannosyldiinositol phosphorylceramide] are often observed in the presence or absence of hydroxyl groups on the C-4 position of long-chain base (C4-OH) and the C-2 position of very long-chain fatty acids (C2-OH), but the biological significance of these groups remains unclear. Here, we evaluated cellular membrane fluidity in hydroxyl group-defective yeast mutants by fluorescence recovery after photobleaching. The lateral diffusion of enhanced green fluorescent protein-tagged hexose transporter 1 (Hxt1-EGFP) was influenced by the absence of C4-OH and/or C2-OH. Notably, the fluorescence recovery of Hxt1-EGFP was dramatically decreased in the sur2Δ mutant (absence of C4-OH) under the csg1Δcsh1Δ background, in which mannosylation of IPC is blocked leading to IPC accumulation, while the recovery in the scs7Δ mutant (absence of C2-OH) under the same background was modestly decreased. In addition, the amount of low affinity tryptophan transporter 1 (Tat1)-EGFP was markedly decreased in the sur2Δcsg1Δcsh1Δ mutant and accumulated in intracellular membranes in the scs7Δcsg1Δcsh1Δ mutant without altering its protein expression. These results suggest that C4-OH and C2-OH are most probably critical factors for maintaining membrane fluidity and proper turnover of membrane molecules in yeast containing complex sphingolipids with only one hydrophilic head group.
机译:在酿酒酵母中,通常在长链碱基的C-4位置(C4- OH)和非常长链脂肪酸(C2-OH)的C-2位置,但这些基团的生物学意义仍不清楚。在这里,我们通过光漂白后的荧光恢复评估了羟基缺陷型酵母突变体中的细胞膜流动性。增强的绿色荧光蛋白标记的己糖转运蛋白1(Hxt1-EGFP)的横向扩散受到不存在C4-OH和/或C2-OH的影响。值得注意的是,在csg1Δcsh1Δ背景下的sur2Δ突变体(C4-OH缺失)中,Hxt1-EGFP的荧光恢复显着降低,其中IPC的甘露糖基化被阻止导致IPC积累,而在scs7Δ突变体中(在缺少C4-OH的情况下)恢复。在相同背景下的C2-OH)有所降低。此外,在sur2Δcsg1Δcsh1Δ突变体中低亲和力色氨酸转运蛋白1(Tat1)-EGFP的量明显减少,并在scs7Δcsg1Δcsh1Δ突变体中积累在细胞内膜中,而不会改变其蛋白表达。这些结果表明,C4-OH和C2-OH最可能是维持含有仅具有一个亲水头基的复杂鞘脂的酵母中的膜流动性和膜分子适当更新的关键因素。

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