Fig. 5.
![Fig. 5. Metabolism of [3H]Sph in HUVECs. (Upper panel) HUVECs were incubated with [3H]Sph for various durations. Lipids were then extracted from cells or media and analyzed for [3H]sphingolipids by TLC autoradiography. Locations of standard lipids are indicated on the left. SM, sphingomyelin; O, origin. (Lower panel) HUVECs and human platelets were incubated with [3H]Sph for 4 hours and, after the autoradiography, silica gel areas containing radiolabeled sphingolipids were scraped off and counted using a liquid scintillation counter. Radioactivity was expressed as a percentage of the value of [3H]Sph at time 0. Columns and error bars represent the mean ± SD (n = 3).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/93/12/10.1182_blood.v93.12.4293/4/blod41226005w.jpeg?Expires=1724235064&Signature=FbFiXHkv6r53X7M6s9s8wzxJsiIdW3egt9FX~3MZHnbDC2~RUtoYuOjynmSw2knwHxiHfm231fMYnyXACwuaJn-uksQ4d3CaPYA2obNMBGCaNBiSzStJgcqhTrJdeK8pMjhqFAQQ7zCJ8~xeBOpKRWDwjmfqwqEfceDJ49w7uh6WpMqC8ZkkUwMYTszX2xEg7vffwG3H9oSleRsCjQo1uR3s1Hy6ARvIb9wLrqrGxx29zjqrnhonIazH8MJS9ktz88a2oSPTOqsQHnnT-lOHooJ6drsop4RE4M0D~F8YtI--4-J9T86LHiHBe2ppbfD~dg~1hUsUbd1feGxIG~QF-g__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Metabolism of [3H]Sph in HUVECs. (Upper panel) HUVECs were incubated with [3H]Sph for various durations. Lipids were then extracted from cells or media and analyzed for [3H]sphingolipids by TLC autoradiography. Locations of standard lipids are indicated on the left. SM, sphingomyelin; O, origin. (Lower panel) HUVECs and human platelets were incubated with [3H]Sph for 4 hours and, after the autoradiography, silica gel areas containing radiolabeled sphingolipids were scraped off and counted using a liquid scintillation counter. Radioactivity was expressed as a percentage of the value of [3H]Sph at time 0. Columns and error bars represent the mean ± SD (n = 3).
