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Journal of Lipid Research, Vol 28, 1335-1341, Copyright © 1987 by Lipid Research, Inc.
RA Coleman and EB Haynes
In order to determine whether placental cells can synthesize and release
fatty acids, trophoblast cells from term human placentas were established
in monolayer culture. The cells continued to secrete placental lactogen and
progesterone and maintained specific activities of critical enzymes of
triacylglycerol and phosphatidylcholine biosynthesis for 24 to 72 hr in
culture. Fatty acid was rapidly synthesized from [14C]acetate and released
by the cells. Palmitoleic, palmitic, and oleic acids were the major fatty
acids synthesized from [14C]acetate and released. Small amounts of lauric,
myristic, and stearic acids were also identified. [14C]acetate was also
incorporated into cellular triacylglycerol, phospholipid, and cholesterol,
but radiolabeled free fatty acid did not accumulate intracellularly. In a
pulse-chase experiment, cellular glycerolipids were labeled with [1-
14C]oleate; trophoblast cells then released 14C-labeled fatty acid into the
media as the cellular content of labeled phospholipid and triacylglycerol
decreased without intracellular accumulation of free fatty acid. Twenty
percent of the 14C-label lost from cellular glycerolipid could not be
recovered as a chloroform-extractable product, suggesting that some of the
hydrolyzed fatty acid had been oxidized. These data indicate that cultured
placenta trophoblast cells can release fatty acids that have either been
synthesized de novo or that have been hydrolyzed from cellular
glycerolipids. Trophoblast cells in monolayer culture should provide an
excellent model for molecular studies of placental fatty acid metabolism
and release.
ARTICLES
Synthesis and release of fatty acids by human trophoblast cells in culture
Department of Pediatrics, Duke University Medical Center, Durham, NC 27710.
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