![Figure 6. [14C]4F-GalNAc distribution in culture media and glycoproteins. Cell culture media containing [14C]4F-GalNAc (0.5 μCi/mL, 100μM) was placed under standard growth conditions either in the presence or absence of HL-60 cells for 38 hours. Growth media and cells were harvested separately. (A-B) Culture media harvested from cultures with (A) and without HL-60 (B) separated on Biogel P-2 column. (C) Samples at the void volume (samples 1 and 4), peak fractions in panel A (samples 2 and 3) and panel B (sample 5) were separated using TLC with chloroform/methanol (5:1) as mobile phase. Phosphorimaging detected radioactivity on TLC plates. Nonradiolabeled, nonacetylated 4F-GalNAc (lane 6) and per-acetylated 4F-GalNAc (lane 7) standards were run in parallel and developed using ethanol/sulfuric acid spray followed by charring. Addition of acetylated 4F-GalNAc to HL-60 cells leads to deacetylation as evidenced by prominent peak 3 in the chromatogram. (D) PSGL-1 was immunoprecipitated from HL-60 lysates cultured with [14C]4F-GalNAc using Ab H-300. This immunoprecipitate and PSGL-1–depleted cell lysate were resolved on a sodium dodecyl sulfate–polyacrylamide gel electrophoresis gel and blotted onto nitrocellulose membrane. Radioactivity was measured using scintillation counter in panels A and B; and using phosphorimaging in panels C and D. 4F-GalNAc is incorporated into leukocyte PSGL-1 and other glycoproteins.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/115/6/10.1182_blood-2009-07-231480/4/zh89990948290006.jpeg?Expires=1724268256&Signature=ErTiQ3nDiVngqvymKCClKbanGOGOYbSKY4dRUxkegO515vA9-XhZT7jHmmiNK7xd13j0qo7c4-C7wJFMTP4r3pEVTEHh3jnXj3zrmYRGB4gdGq~EcGcCvvaqlHpK~5jT8lUgwzipHErvT0VtvMTYFuPhwa1kC59P~GuKMx72uxDnw3GYu48gWGHLV6h6GHV9yrhqwF7V~vJ096K-dmaE~L~Tz43L~~0VkT6wP~8IwKYMiTmyrww0x7k2nAJMmK4v7~9~pMcdZHAW5cqQ3ipEDEmDxUBQ3ta8zM-Zn32rU~zjrQ5Mm3cssUQOvaRUikt1p-FNGhItMGXt324OyaDrDQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
[14C]4F-GalNAc distribution in culture media and glycoproteins. Cell culture media containing [14C]4F-GalNAc (0.5 μCi/mL, 100μM) was placed under standard growth conditions either in the presence or absence of HL-60 cells for 38 hours. Growth media and cells were harvested separately. (A-B) Culture media harvested from cultures with (A) and without HL-60 (B) separated on Biogel P-2 column. (C) Samples at the void volume (samples 1 and 4), peak fractions in panel A (samples 2 and 3) and panel B (sample 5) were separated using TLC with chloroform/methanol (5:1) as mobile phase. Phosphorimaging detected radioactivity on TLC plates. Nonradiolabeled, nonacetylated 4F-GalNAc (lane 6) and per-acetylated 4F-GalNAc (lane 7) standards were run in parallel and developed using ethanol/sulfuric acid spray followed by charring. Addition of acetylated 4F-GalNAc to HL-60 cells leads to deacetylation as evidenced by prominent peak 3 in the chromatogram. (D) PSGL-1 was immunoprecipitated from HL-60 lysates cultured with [14C]4F-GalNAc using Ab H-300. This immunoprecipitate and PSGL-1–depleted cell lysate were resolved on a sodium dodecyl sulfate–polyacrylamide gel electrophoresis gel and blotted onto nitrocellulose membrane. Radioactivity was measured using scintillation counter in panels A and B; and using phosphorimaging in panels C and D. 4F-GalNAc is incorporated into leukocyte PSGL-1 and other glycoproteins.
