A rapid ceramide synthase activity using NBD-sphinganine and solid phase extraction.

Ceramides are synthesized by six mammalian ceramide synthases (CerSs), each of which uses fatty acyl-CoAs of different chain lengths for N-acylation of the sphingoid long-chain base. We now describe a rapid and reliable CerS assay that uses a fluorescent N-[6-[(7-nitrobenzo-2-oxa-1,3-diazol-4-yl) (NBD) sphinganine substrate followed by separation of the NBD-lipid substrate and products using solid phase extraction (SPE) C18 chromatography. SPE chromatography is a quick and reliable alternative to TLC, and moreover, there is no degradation of either NBD-sphinganine or NBD-ceramide. We have optimized the assay for use with minimal amounts of protein in a minimal volume. This assay will prove useful for the analysis of CerS activity, which is of particular importance in light of the growing involvement of CerS in cell regulation and in the pathology of human diseases.

for CerS4. Both these results compare favorably with K m values obtained previously using [4, H]Sph ( 22 ) and NBD-Sph ( 21 ) (which were obtained using higher amounts of protein and/or longer reaction times). The need for lower amounts of protein could be particularly useful when only small amounts of tissue or cells are available, such as might be the case when using clinical samples.
Interestingly, whereas NBD-Sph was a good substrate for CerS, { N -[(7-nitro-2-1,3-benzoxadiazol-4-yl)-methyl] amino} palmitoyl coenzyme A (NBD-palmitoyl-CoA) did not act as a CerS5 substrate ( Fig. 2A ), nor did it act as a competitive inhibitor of CerS5 (data not shown), strengthening the notion ( 4 ) that CerSs are highly specifi c for the acyl-CoA donor but less specifi c for the sphingoid longchain base. Degradation products of NBD-Sph are readily apparent upon separation by TLC, which is of concern if low levels of CerS activity are assayed because some of the degradation products have Rf values similar to that of NBDceramide ( Fig. 2B ). To isolate the degradation products, we performed preparative TLC ( Fig. 2B ), followed by negative ion mode electrospray tandem mass spectrometry, Cell culture, transfection, and preparation of cell homogenates HEK 293T cells were cultured in Dulbecco's modifi ed Eagle's medium supplemented with 10% fetal calf serum, 100 IU/ml penicillin, 100 µg/ml streptomycin, and 110 µg /ml sodium pyruvate. Transfection was performed with the polyethylenimine reagent (Sigma-Aldrich) using 10 µg of plasmid per 10 cm culture dish. Thirty-six to 48 h after transfection, cells were removed from culture dishes and washed twice with phosphate-buffered saline. Cell homogenates were prepared in 20 mM HEPES-KOH, pH 7.2, 25 mM KCl, 250 mM sucrose, and 2 mM MgCl 2 containing a protease inhibitor cocktail (Sigma-Aldrich). Protein was determined using the Bradford reagent (Bio-Rad, Hercules, CA).

Optimizing conditions for use of NBD-Sph in the CerS assay
While NBD-Sph ( Fig. 1 ) has been used previously to assay CerS ( 17,18,21 ), no attempts have been made to minimize reaction volumes to allow the use of small amounts of biological material or to improve the mode of separating NBD-lipid substrates and products. We have now been able to decrease the reaction volume to a minimum of 20 µl, rather than the 100-250 µl used previously with [4, H]Sph ( 22 ) or with NBD-Sph ( 21 ), permitting the use of small amounts of protein for the assay. Thus, we could assay CerS5 activity using as little as 1 µg of protein and 5 min reaction time, and CerS4 activity using 10 ( Fig. 1B ) or 20 µg (not shown) of protein and 20 min reaction time; note that each CerS displays different specifi c activities, necessitating optimization of assay conditions for each CerS ( 22 ). Under these conditions, we obtained a K m of 2.0 ± 0.5 µM toward NBD-Sph for CerS5 and 3.4 ± 1.5 µM  and obtained predicted structures of the NBD-Sph degradation products ( Fig. 2C ).

SPE chromatography to separate NBD lipids
In order to simplify the CerS assay, and to limit the use of specialized equipment that might only be available in a lipid-oriented laboratory, as well as to make the assay compatible for use with large numbers of samples, we established a new method based on the separation of  containing NBD-Sph was discarded and replaced by roundbottom, black polypropylene 96-well plates (Nunc Thermo Scientifi c, Waltham, MA) (three plates were placed on top of each other so that the distance between the columns and the plates was short enough to avoid spillage of the eluates). NBD-ceramide was eluted from the columns with 2 × 150 µl and an additional 1 × 50 µl of 10 mM ammonium acetate in methanol-chloroform-water-formic acid (30:14:6:1) (30 s each) ( Fig. 3I ) followed by 2 min under vacuum. NBD-ceramide was quantifi ed using a fl uorescent ELISA reader. In contrast to separation on TLC plates, no degradation of NBD-Sph was detected after elution from the SPE column, and likewise, there was no degradation of NBD-ceramide ( Fig. 4 ).
The suitability of using SPE columns for the CerS assay was tested in nontransfected HEK cells using either C16:0acyl-CoA (to assay CerS5/6) or C24:1-acyl-CoA (to assay CerS2), with increasing amounts of protein. NBD-ceramide was quantifi ed using standard curves of NBD-Sph and compared with results obtained by TLC. The rate of the reaction was linear up to 20 µg of protein and was similar using both methods ( Fig. 5A ). HEK cells transfected with CerS5 were also assayed using either increasing amounts of protein ( Fig. 5B ) or reaction times ( Fig. 5C ), as were CerS2 or CerS4 (not shown), and similar results the best separation; the use of the vacuum was essential to achieve effi cient separation.
Optimal conditions were established as follows, as outlined schematically in Fig. 3 . Reactions were performed at 37°C using 15 µM NBD-Sph, 20 µM defatted BSA, and 50 µM acyl-CoA in a reaction volume of 20 µl ( Fig. 3A ). Reactions were terminated with 20 l methanol/1% (v/v) formic acid ( Fig. 3B ), followed by addition of 110 µl water/1% (v/v) formic acid ( Fig. 3C ). While columns were being activated (see below), samples were maintained at either room temperature or at Ϫ 20°C (prior to addition of water/1% (v/v) formic acid) if column preparation took more than a few minutes. Columns were placed in a vacuum manifold attached to a vacuum pump and washed with 150 µl methanol/1% formic acid with 30 s of vacuum ( Fig. 3D ), followed by 150 µl water/1% formic acid for an additional 30 s under vacuum ( Fig. 3E ). Samples from the reaction tubes (150 µl) were added, and the vacuum was applied for another 30 s ( Fig. 3F ). Two washes with 150 µl water/1% formic acid were applied for 30 s each, followed by 2 min under vacuum ( Fig. 3G ). NBD-Sph was eluted using three 150 l washes of 10 mM ammonium acetate in methanol-water-chloroform-formic acid (30:14:6:1, v/v/v/v) for 30 s each ( Fig. 3H ), followed by 2 min under vacuum. The waste container used to collect the initial washes the use of SPE-C18 columns provides a number of advantages, not least the accessibility of the method for laboratories that do not routinely assay enzymes of lipid metabolism. A major advantage of the SPE-C18 columns is the ability to assay up to 96 samples at once, whereas assaying 96 samples by TLC would require 10 or 11 TLC plates, thus saving considerable time and effort. In terms of time, assaying 96 samples by the classical TLC method, including quantifi cation (by either scraping the silica and counting in a fl uorimeter or analysis using a phosphorimager) and data analysis, could take as long as 3 days, whereas only 1 day is needed for the same number of reactions using SPE-C18 columns (due to the short times of separation on the columns, the possibility of running multiples samples together, and the ease of quantifi cation by placing the 96-well plate directly in a fl uorescent ELISA reader). Thus, although the SPE-C18 columns are somewhat more expensive than TLC plates, the time saved in personnel costs renders the SPE-C18 columns more effi cient and economical.
Because CerSs appear to be involved in the pathology of a number of human diseases (15)(16)(17)(18)(19), the assay that we have described in this study might prove useful in a clinical setting. Furthermore, SPE column chromatography could be were obtained using both methods with all three CerSs. Reactions were linear with respect to protein for amounts as low as 1-10 g for CerS5 and 1-20 g for CerS6, and up to 70 µg of protein for CerS2 and CerS4 ( Fig. 6A ). Likewise, reactions were linear with respect to time for up to 20 min with CerS5 and CerS6 and 60 min with CerS2 and CerS4 ( Fig. 6B ). Importantly, for CerSs that display high levels of activity, assays can be performed for as short a time as 5 min using as little as 5 µg of protein, which gives similar results to those obtained previously using [4, H] Sph ( 24 ). Some of the CerSs (i.e., CerS2 and CerS4), display lower activity than others (i.e., CerS5), as previously reported ( 10,22,25 ).
In summary, we have developed a rapid and reliable method for assaying CerS activity in small amounts of biological material using SPE column chromatography. Moreover, a large number of assays can be run simultaneously by using a multichamber pipettor and performing the activity in a 96-well PCR plate. The assay alleviates the need to use TLC as a separation method and thus requires much lower levels of organic solvents.
Although similar results were obtained in the current study using TLC separation and SPE-C18 column chromatography, Fig. 6. CerS activity using the optimized assay procedure. A: Assays were performed using different amounts of protein from HEK cells overexpressing the indicated CerS; the acyl-CoA was chosen according to the specifi city of the particular CerS (i.e., C24:1-CoA for CerS2, C20-CoA for CerS4, and C16-CoA for CerS5 and CerS6). CerS2 and CerS4 were assayed for 30 min, and CerS5 and CerS6 for 10 min.
Results are means ± SEM; n = 2-5. B: Assays were performed using different reaction times. CerS2 and CerS4 were assayed with 40 g of protein, and CerS5 and CerS6 with 10 µg of protein. Results are means ± SEM; n = 2-5. used to assay other enzymes of sphingolipid metabolism for which fl uorescent substrates ( 26 ) are available.