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Sphingomyelinase D, a novel probe for cellular sphingomyelin

机译:鞘磷脂酶D,一种用于细胞鞘鞘素的新型探针

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摘要

Sphingomyelin (SM) and free cholesterol (FC) are concentrated in the plasma membranes of eukaryotes; however, the physiological significance of their association is unclear. A common tool for studying the role of membrane SM is digestion with bacterial sphingomyelinase (SMase) C, which hydrolyzes SM to ceramide. However, it is not known whether the observed effects of SMase C treatment are due to the loss of SM per se or to the signaling effects of ceramide. In this study, we tested SMase D from Corynebacterium pseudotuberculosis, which hydrolyzes SM to ceramide phosphate, as an alternative probe. This enzyme specifically hydrolyzed SM in fibroblasts without causing accumulation of ceramide. Treatment of fibroblasts with SMase D stimulated translocation of PM FC to intracellular sites by <20% of the rate observed after SMase C digestion. The cells regenerated SM nearly completely within 5 h after SMase C treatment. However, even after 20 h, no regeneration occurred following SMase D digestion.These findings suggest that the translocation of PM FC caused by SMase C digestion is due to the cellular effects of ceramide rather than the loss of SM. Since ceramide phosphate does not appear to have such effects, we suggest that SMase D is a useful probe of membrane SM.
机译:鞘磷脂(SM)和游离胆固醇(Fc)浓缩在真核生物的血浆膜中;然而,他们的关联的生理意义尚不清楚。用于研究膜SM的作用的常见工具是用细菌鞘氨氨基酶(SMASE)C的消化,其将SM水解为神经酰胺。然而,尚不清楚观察到的Smase C治疗的影响是由于SM本身的损失或神经酰胺的信号效应。在这项研究中,我们从棒状杆菌的Smase D测试了诸如磷酸酯的源于磷酸盐,作为替代探针。该酶特异性地在成纤维细胞中水解SM而不会引起神经酰胺的积累。通过在SMASE C消化后观察到的20%观察到的血液D刺激PM Fc转化为细胞内部位的成纤维细胞。在Smase C处理后,细胞几乎完全再生SM。然而,即使在20小时后,SMASE D消化后也不会发生再生。这些发现表明,由SMASE C消化引起的PM FC的易位是由于神经酰胺的细胞效应而不是SM的损失。由于神经酰胺磷酸盐似乎没有具有这样的效果,因此SMASE D是膜SM的有用探针。

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