二氢神经酰胺去饱和酶在人神经母细胞瘤细胞周期进程中的作用。
Involvement of dihydroceramide desaturase in cell cycle progression in human neuroblastoma cells.
作者信息
Kraveka Jacqueline M, Li Li, Szulc Zdzislaw M, Bielawski Jacek, Ogretmen Besim, Hannun Yusuf A, Obeid Lina M, Bielawska Alicja
机构信息
Division of Hematology/Oncology, Department of Pediatrics, Medical University of South Carolina, Charleston, South Carolina 29425, USA.
出版信息
J Biol Chem. 2007 Jun 8;282(23):16718-28. doi: 10.1074/jbc.M700647200. Epub 2007 Feb 5.
The role of dihydroceramide desaturase as a key enzyme in the de novo pathway of ceramide generation was investigated in human neuroblastoma cells (SMS-KCNR). A novel assay using water-soluble analogs of dihydroceramide, dihydroceramidoids (D-erythro-dhCCPS analogs), was used to measure desaturase activity in situ. Conversion of D-erythro-2-N-[12'-(1''-pyridinium)-dodecanoyl]-4,5-dihydrosphingosine bromide (C(12)-dhCCPS) to its 4,5-desaturated counterpart, D-erythro-2-N-[12'-(1''-pyridinium)dodecanoyl]sphingosine bromide (C(12)-CCPS), was determined by liquid chromatography/mass spectrometry analysis. The validity of the assay was confirmed using C(8)-cyclopropenylceramide, a competitive inhibitor of dihydroceramide desaturase. A human homolog (DEGS-1) of the Drosophila melanogaster des-1 gene was recently identified and reported to have desaturase activity. Transfection of SMS-KCNR cells with small interfering RNA to DEGS-1 significantly blocked the conversion of C(12)-dhCCPS to C(12)-CCPS. The associated accumulation of endogenous dihydroceramides confirmed DEGS-1 as the main active dihydroceramide desaturase in these cells. The partial loss of DEGS-1 inhibited cell growth, with cell cycle arrest at G(0)/G(1). This was accompanied by a significant decrease in the amount of phosphorylated retinoblastoma protein. This hypophosphorylation was inhibited by tautomycin and not by okadaic acid, suggesting the involvement of protein phosphatase 1. Additionally, we found that treatment of SMS-KCNR cells with fenretinide inhibited desaturase activity in a dose-dependent manner. An increase in dihydroceramides (but not ceramides) paralleled this process as measured by liquid chromatography/mass spectrometry. There were no effects on the mRNA or protein levels of DEGS-1, suggesting that fenretinide acts at the post-translational level as an inhibitor of this enzyme. Tautomycin was also able to block the hypophosphorylation of the retinoblastoma protein observed upon fenretinide treatment. These findings suggest a novel biological function for dihydroceramides.
在人神经母细胞瘤细胞(SMS-KCNR)中研究了二氢神经酰胺去饱和酶作为神经酰胺从头合成途径中关键酶的作用。使用二氢神经酰胺的水溶性类似物二氢神经酰胺类似物(D-赤藓糖-dhCCPS类似物)的一种新型测定法来原位测量去饱和酶活性。通过液相色谱/质谱分析确定D-赤藓糖-2-N-[12'-(1''-吡啶鎓)-十二烷酰基]-4,5-二氢鞘氨醇溴化物(C(12)-dhCCPS)向其4,5-去饱和对应物D-赤藓糖-2-N-[12'-(1''-吡啶鎓)十二烷酰基]鞘氨醇溴化物(C(12)-CCPS)的转化。使用二氢神经酰胺去饱和酶的竞争性抑制剂C(8)-环丙烯基神经酰胺证实了该测定法的有效性。最近鉴定并报道了果蝇des-1基因的人同源物(DEGS-1)具有去饱和酶活性。用针对DEGS-1的小干扰RNA转染SMS-KCNR细胞可显著阻断C(12)-dhCCPS向C(12)-CCPS的转化。内源性二氢神经酰胺的相关积累证实DEGS-1是这些细胞中主要的活性二氢神经酰胺去饱和酶。DEGS-1的部分缺失抑制细胞生长,细胞周期停滞在G(0)/G(1)期。这伴随着视网膜母细胞瘤蛋白磷酸化量的显著减少。这种低磷酸化被 tautomycin抑制而不被冈田酸抑制,提示蛋白磷酸酶1的参与。此外,我们发现用维甲酸处理SMS-KCNR细胞以剂量依赖性方式抑制去饱和酶活性。通过液相色谱/质谱测定,二氢神经酰胺(而非神经酰胺)的增加与该过程平行。对DEGS-1的mRNA或蛋白质水平没有影响,提示维甲酸在翻译后水平作为该酶的抑制剂起作用。Tautomycin也能够阻断维甲酸处理后观察到的视网膜母细胞瘤蛋白的低磷酸化。这些发现提示了二氢神经酰胺的一种新的生物学功能。
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