Abstract
Glucosylceramide synthase (GCS or GlcT-1), converting ceramide to glucosylceramide, is a key enzyme for the synthesis of glycosphingolipids. Due to its diverse roles in physiology and diseases, GCS may be a disease marker and drug target. Current assays for enzymes including GCS are based on reactions conducted in a test tube using enzyme preparations. Measurement of enzyme activity in laboratory-made conditions cannot directly evaluate the role of GCS in cells. Here, we introduce a new approach to determine GCS cellular activity using fluorescent NBD C6-ceramide in vivo. Cellular GCS transfers UDP-glucose to NBD C6-ceramide and produces NBD C6-glucosylceramide. C6-glucosylceramide is then separated from C6-ceramide by thin-layer chromatography and both are then quantitated by spectrophotometer. This cell-based method is able to quantitate glucosylceramide in pmol range, produced by approximately 50,000 cells or 1.0 mg tissue. This method has been used successfully to evaluate the degrees of GCS enzyme in cells and in tumors subjected to gene manipulation and chemical inhibition. These data indicate that this cell-based fluorescent method is direct, reproducible, and simple for assessing ceramide glycosylation. It is applicable to validate GCS activity in drug-resistant cancers and in other disorders.
Highlights
Glucosylceramide synthase (GCS or GlcT-1), converting ceramide to glucosylceramide, is a key enzyme for the synthesis of glycosphingolipids
Quantitation of Cer glycosylation in cells In this study, commercially available fluorescent substrate NBD C6-Cer was used as an acceptor for glucose conversion catalyzed by GCS
We developed a simple and reliable method to directly quantitate ceramide glycosylation catalyzed by GCS in cells and in tissues
Summary
Glucosylceramide synthase (GCS or GlcT-1), converting ceramide to glucosylceramide, is a key enzyme for the synthesis of glycosphingolipids. Different from test tube assay in vitro, NBD C6-Cer, a substrate for GCS in cells, is not under saturation once glycosylation starts. Consistence with GCS protein levels, GlcCer/Cer ratio was increased to 124% (3.1 vs 2.5, P < 0.05) in NCI/ADR-RES/GCS and decreased to 60% (1.5 vs 2.5, P < 0.05) in NCI/ADR-RES asGCS cells, respectively, as compared with NCI/ADR-RES cells.
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