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Journal of Lipid Research, Vol 29, 1367-1377, Copyright © 1988 by Lipid Research, Inc.
Interaction of plasma-derived lipid transfer protein with macrophages in culture
RE Morton
Department of Brain and Vascular Research, Research Institute of the Cleveland Clinic Foundation, OH 44106.
This study investigates the ability of human plasma-derived lipid transfer
protein to facilitate lipid transfer to and from intact viable cells in
culture. Mouse peritoneal macrophages or J774 macrophages were preincubated
with acetylated low density lipoprotein and [3H]oleate/albumin to promote
the intracellular synthesis and accumulation of cholesteryl [3H]oleate and
3H-labeled triglyceride. The addition of partially purified lipid transfer
protein to cultures of lipid-loaded macrophages resulted in a time and
concentration-dependent transfer of radiolabeled cholesteryl ester and
triglyceride from macrophages to the medium. At 48 hr, lipid transfer
protein facilitated the net transfer of 16 and 11% of cellular cholesteryl
ester and triglyceride radioactivity, respectively, to the medium; transfer
in the absence of the lipid transfer protein was less than 2%. The transfer
of cholesteryl ester radioactivity was accompanied by a similar decrease in
cellular cholesteryl ester mass indicating a net transfer event. Lipid
transfer from cells was not dependent on the presence of a lipoprotein
acceptor in the medium; however, low and high density lipoproteins present
at 200 micrograms cholesterol/ml did significantly stimulate the transfer
protein-facilitated efflux of these lipids. Lipid transfer protein did not
appear capable of transferring radiolabeled lipid from low density or high
density lipoprotein to macrophages. Radiolabeled cholesteryl ester and
triglyceride transferred from cells to the medium by lipid transfer protein
were associated with large molecular weight (greater than 2 x 10(6))
components in the medium with an average density greater than 1.21 g/ml;
these lipids were not associated with lipid transfer protein itself.
However, these radiolabeled lipids were readily incorporated into low or
high density lipoproteins when these lipoproteins were added to the medium
either during or after its incubation with cells. It is concluded that
lipid transfer protein can facilitate the net efflux of cholesteryl esters
from intact, living macrophages. These studies suggest a novel and
potentially antiatherogenic role for lipid transfer protein.

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Copyright © 1988 by the American Society for Biochemistry and Molecular Biology.
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