Martin O C, Pagano R E
Department of Embryology, Carnegie Institution of Washington, Baltimore, Maryland 21210-3399.
J Cell Biol. 1994 May;125(4):769-81. doi: 10.1083/jcb.125.4.769.
We examined the uptake and intracellular transport of the fluorescent glucosylceramide analogue N-[5-(5,7-dimethyl BODIPYTM)-1-pentanoyl]-glucosyl sphingosine (C5-DMB-GlcCer) in human skin fibroblasts, and we compared its behavior to that of the corresponding fluorescent analogues of sphingomyelin, galactosylceramide, and lactosylceramide. All four fluorescent analogues were readily transferred from defatted BSA to the plasma membrane during incubation at 4 degrees C. When cells treated with C5-DMB-GlcCer were washed, warmed to 37 degrees C, and subsequently incubated with defatted BSA to remove fluorescent lipid at the cell surface, strong fluorescence was observed at the Golgi apparatus, as well as weaker labeling at the nuclear envelope and other intracellular membranes. Similar results were obtained with C5-DMB-galactosylceramide, except that labeling of the Golgi apparatus was weaker than with C5-DMB-GlcCer. Internalization of C5-DMB-GlcCer was not inhibited by various treatments, including ATP depletion or warming to 19 degrees C, and biochemical analysis demonstrated that the lipid was not metabolized during its internalization. However, accumulation of C5-DMB-GlcCer at the Golgi apparatus was reduced when cells were treated with a nonfluorescent analogue of glucosylceramide, suggesting that accumulation of C5-DMB-GlcCer at the Golgi apparatus was a saturable process. In contrast, cells treated with C5-DMB-analogues of sphingomyelin or lactosylceramide internalized the fluorescent lipid into a punctate pattern of fluorescence during warming at 37 degrees C, and this process was temperature and energy dependent. These results with C5-DMB-sphingomyelin and C5-DMB-lactosylceramide were analogous to those obtained with another fluorescent analogue of sphingomyelin in which labeling of endocytic vesicles and plasma membrane lipid recycling were documented (Koval, M., and R. E. Pagano. 1990. J. Cell Biol. 111:429-442). Incubation of perforated cells with C5-DMB-sphingomyelin resulted in prominent labeling of the nuclear envelope and other intracellular membranes, similar to the pattern observed with C5-DMB-GlcCer in intact cells. These observations are consistent with the transbilayer movement of fluorescent analogues of glucosylceramide and galactosylceramide at the plasma membrane and early endosomes of human skin fibroblasts, and suggest that both endocytic and nonendocytic pathways are used in the internalization of these lipids from the plasma membrane.
我们检测了荧光葡糖神经酰胺类似物N-[5-(5,7-二甲基BODIPYTM)-1-戊酰基]-葡糖基鞘氨醇(C5-DMB-GlcCer)在人皮肤成纤维细胞中的摄取及细胞内转运情况,并将其行为与鞘磷脂、半乳糖神经酰胺和乳糖神经酰胺的相应荧光类似物进行了比较。在4℃孵育期间,所有这四种荧光类似物都很容易从脱脂牛血清白蛋白转移至质膜。用C5-DMB-GlcCer处理的细胞经洗涤、升温至37℃,随后与脱脂牛血清白蛋白一起孵育以去除细胞表面的荧光脂质后,在高尔基体观察到强荧光,在核膜和其他细胞内膜也有较弱的标记。C5-DMB-半乳糖神经酰胺也得到了类似结果,只是高尔基体的标记比C5-DMB-GlcCer弱。C5-DMB-GlcCer的内化不受包括ATP耗竭或升温至19℃在内的各种处理的抑制,生化分析表明该脂质在其内化过程中未被代谢。然而,当用葡糖神经酰胺的非荧光类似物处理细胞时,C5-DMB-GlcCer在高尔基体的积累减少,这表明C5-DMB-GlcCer在高尔基体的积累是一个可饱和过程。相比之下,用鞘磷脂或乳糖神经酰胺的C5-DMB类似物处理的细胞在37℃升温期间将荧光脂质内化为点状荧光模式,且该过程依赖于温度和能量。C5-DMB-鞘磷脂和C5-DMB-乳糖神经酰胺的这些结果与用另一种鞘磷脂荧光类似物得到的结果相似,后者记录了内吞小泡和质膜脂质循环的标记情况(科瓦尔,M.,和R.E.帕加诺。1990。《细胞生物学杂志》111:429 - 442)。用C5-DMB-鞘磷脂孵育穿孔细胞导致核膜和其他细胞内膜出现明显标记,类似于在完整细胞中用C5-DMB-GlcCer观察到的模式。这些观察结果与葡糖神经酰胺和半乳糖神经酰胺的荧光类似物在人皮肤成纤维细胞质膜和早期内体中的跨膜运动一致,并表明内吞和非内吞途径都用于这些脂质从质膜的内化。
