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Resumen de New insights into sphingolipid metabolism and functions by using chemical tools

Francesca Cingolani

  • Sphingolipids (SLs), essential components of cell membranes, are bioactive molecules involved in the regulation of a variety of cellular processes. Ceramide and sphingosine generally mediate anti-proliferative stimuli, while sphingosine-1-phospate plays an opposite role. The bioactive role of dihydroceramide has also been recently described, showing its involvement in processes like apoptosis and autophagy. Alteration of SLs levels is involved in different disease, including cancer. Sphingolipid metabolism is a complex network of anabolic and catabolic reactions catalyzed by specific enzymes. Consistent with the key role of sphingolipids in cell biology, the modulation of keyenzyme of the sphingolipid metabolism such as dihydroceramide desaturase (Des1), ceramide synthase (CerS), ceramidases (CDases) and sphingosine kinase (SK) represent a strategy to better understand the role of SLs in physiophatological processes. During this PhD thesis three different studies that show the use of SL analogues and SL metabolism inhibitors as pharmacological tools for biomedical investigation in cancer cells were performed. The first study was focused on the alteration of sphingolipid metabolism and cytotoxic effect induced by Jaspine B (JB) in cancer cells. JB, a natural sphingolipid analogue from marine origin, is cytotoxic in a variety of cancer cell lines, including HGC-27 gastric cancer cells. JB induces changes in the sphingolipidome in this cell line, mainly the accumulation of dihydrosphingosine (dhSo) and sphingosine (So), and their phosphorylated forms. Moreover lipidomic analysis show the formation of acyl-JB. These effects appear to be due to inhibitory action of JB on CerS that use the natural sphingolipid as substrate. The hallmark of JB cytotoxicity in HGC-27 cells is the formation of cytoplasmic vacuoles in a time and dose-dependent manner. Apoptosis is not involved in cytoplasmic vacuolation and JB induced cytotoxicity. In addition, despite the accumulation of the autophagic marker LC3-II, autophagy is probably not activated by JB treatment. The micropinocytic nature of vacuoles suggest the involvement of methuosis in JB-induced cell death. The second study was focused on SKI II is a well-known SK inhibitor. In a study on HGC-27 cells we show that SKI II is also an uncompetitive inhibitor of Des1. Des1 inhibition in intact cells is not connected to protein degradation. SKI II, but not the SK1-specific inhibitor PF-543, provoked a remarkable accumulation of dhCers and their metabolites, while both SKI II and PF-543 reduced S1P to almost undetectable levels. SKI II, but not PF-543, reduced cell proliferation, with accumulation of cells in the G0/G1 phase. Similarly SKI II, but not PF543 increases LC3-II levels in HGC-27 cells, suggesting autophagy induction. These overall findings indicate that some of the effects attributed to decreased S1P may actually be caused by augmented dhCers and/or their metabolites. The use of ceramide analogues as chemical tool for ceramidases investigation is the topic of the third study. RBM14 are coumarinic ceramide analogues that differ from the acyl chain length. Among them RBM14C12 was reported as the best substrate for acid ceramidase. In this study it was shown that RBM14 molecules are also hydrolyzed by neutral and alkaline ceramidase. Neutral ceramidase from Pseudomonas aeuriginosa prefers C12 and C14 analogues, while human recombinant NC better hydrolyze RBM14C14 and RBM14C16 molecules. RBM14 substrates are hydrolyzed by MEF cells lacking NC, whit higher activity at basic pH, suggesting alkaline ceramidase activity. SABRAC and RBM1-12 have been designed to inhibit the cysteine protease AC. In this study it was shown that papain, a protein belonging to the same protein family, is not inhibited by SABRAC and RBM1-12. Moreover preliminary studies suggest an irreversible inhibition of AC. These molecules can be used in combination with RBM14C12 substrate as a suitable tool for AC activity determination in intact cancer cells.


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