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培养细胞对鞘脂的摄取:细胞鞘脂与血清蛋白和脂蛋白形成的复合聚集体会迅速被分解代谢。

Sphingolipid uptake by cultured cells: complex aggregates of cell sphingolipids with serum proteins and lipoproteins are rapidly catabolized.

作者信息

Chigorno Vanna, Giannotta Claudia, Ottico Elena, Sciannamblo Mariateresa, Mikulak Joanna, Prinetti Alessandro, Sonnino Sandro

机构信息

Center of Excellence on Neurodegenerative Diseases, Department of Medical Chemistry, Biochemistry, and Biotechnology, University of Milan, 20090 Segrate, Italy.

出版信息

J Biol Chem. 2005 Jan 28;280(4):2668-75. doi: 10.1074/jbc.M407749200. Epub 2004 Nov 17.

Abstract

Human fibroblasts, rat neurons, and murine neuroblastoma cells, cultured in the presence of fetal calf serum, were fed with [1-(3)H]sphingosine to radiolabel sphingolipids. The fate of cell sphingolipids, the release of sphingolipids in the culture medium, the interaction of sphingolipids with the proteins and lipoproteins of fetal calf serum, and the fate of sphingolipids taken up by the cells were investigated. For this latter purpose, the culture medium containing radioactive sphingolipids was delivered to nonlabeled cells. The presence of tritium at position 1 of sphingosine allowed us to follow the extent of sphingolipid catabolism by measuring the production of radioactive phosphatidylethanolamine and proteins by recycling the radioactive ethanolamine formed during sphingosine catabolism and the production of tritiated water. We confirmed that in cells the recycling of sphingosine occurred to a high extent and that only a minor portion of cell sphingolipids was catabolized to the small fragments of ethanolamine and water. Cell sphingolipids were released in the culture medium, where they formed large lipoproteic aggregates at a rate of about 12% per day. Released sphingolipids were taken up by the cells and catabolized to the sphingosine and then to ethanolamine, and recycling of sphingosine was not observed. This suggests that in the presence of fetal calf serum in the culture medium, exogenous sphingolipids directly reach the lysosomes, were they are entirely catabolized. Thus, the trafficking of sphingolipids from cells to the extracellular environment and from this to other cells does not allow the modification of the plasma membrane composition.

摘要

在胎牛血清存在的情况下培养的人成纤维细胞、大鼠神经元和小鼠神经母细胞瘤细胞,用[1-(3)H]鞘氨醇喂养以对鞘脂进行放射性标记。研究了细胞鞘脂的命运、鞘脂在培养基中的释放、鞘脂与胎牛血清蛋白质和脂蛋白的相互作用以及细胞摄取的鞘脂的命运。为了达到后一个目的,将含有放射性鞘脂的培养基输送到未标记的细胞中。鞘氨醇1位上氚的存在使我们能够通过测量放射性磷脂酰乙醇胺和蛋白质的产生来追踪鞘脂分解代谢的程度,放射性磷脂酰乙醇胺和蛋白质是通过回收鞘氨醇分解代谢过程中形成的放射性乙醇胺以及产生的氚化水来产生的。我们证实,在细胞中鞘氨醇的再循环程度很高,并且只有一小部分细胞鞘脂被分解代谢为乙醇胺和水的小片段。细胞鞘脂释放到培养基中,在那里它们以每天约12%的速率形成大的脂蛋白聚集体。释放的鞘脂被细胞摄取并分解代谢为鞘氨醇,然后再分解代谢为乙醇胺,未观察到鞘氨醇的再循环。这表明,在培养基中存在胎牛血清的情况下,外源性鞘脂直接到达溶酶体,并在那里被完全分解代谢。因此,鞘脂从细胞到细胞外环境以及从细胞外环境到其他细胞的运输不允许质膜组成发生改变。

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