[No authors listed]
Choline is used to synthesize phospholipids and a lack of choline induces a number of liverârelated diseases, including nonâalcoholic steatohepatitis. The current study characterized the choline uptake system, at molecular and functional levels, in the immortalized human hepatic cell line, Fa2Nâ4, to identify the specific choline transporter involved in choline uptake. The present study also assesed whether choline deficiency or the inhibited choline uptake affected cell viability and apoptosis. Reverse transcriptionâquantitative polymerase chain reaction (PCR) revealed choline transporterâlike protein 1 (CTL1) and CTL2 mRNA and protein expression in Fa2Nâ4 cells. [Methylâ3H]choline studies revealed choline uptake was saturable and mediated by a single transport system that functioned in a Na+âindependent but pHâdependent manner, which was similar to CTL1. Hemicholiniumâ3 (HCâ3), which is a choline uptake inhibitor, and choline deficiency inhibited cell viability, increased caspaseâ3 and â7 activities, and increased fluorescein isothiocyanateâAnnexin V immunofluorescent staining indicated apoptosis. Immunofluorescent staining also revealed CTL1 and CTL2 localized in plasma and mitochondrial membranes, respectively. [Methylâ3H]choline uptake was enhanced by a protein activator, phorbolâ12âmyristate 13âacetate (PMA). Immunofluorescence staining and western blot analysis demonstrated increased CTL1 expression on the cell membrane following PMA treatment. The results of current study indicated that extracellular choline is primarily transported via CTL1, relying on a direct H+ gradient that functions as a driving force in Fa2Nâ4 cells. Furthermore, it was hypothesized that CTL1 and the choline uptake system are strongly associated with cell survival, and that the choline uptake system is modulated by signaling via increased CTL1 expression on the cell surface. These findings provide further insights into the pathogenesis of liver disease involving choline metabolism.
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