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Macrophage cholesterol removal by triglyceride-phospholipid emulsions
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Vol. 155, No. 2, 1988
Pages 709-713
September 15, 1988
MACROPHAGE CHOLESTEROL REMOVAL BY TRICLYCERIDE-PHOSPHOLIPID EMULSIONS Michael Aviram~ Kevin Jon Williams, and Richard J. Deckelbaum Columbia University, College of Physicians & Surgeons New York, New York 10032 Received May 25, 1988
SUMMARY: Phospholipid liposomes were previously shown to mobilize cholesterol from cultured macrophage foam cells. Because Intralipid, a clinically available triglyceride-phospholipid emulsion, contains both phospholipid liposomes and triglyceride-emulsion particles, we sought to study its effect on macrophage clholesterol mobilization. Following an 18h incubation of J774 macrophages in serum-free medium supplemented with Intralipid, cholesteryl ester content decreased by up to 50% in previously cholesterol-loaded cells, and by 25% in non-loaded cells. Both components of Intralipid, liposomes and emulsion particles, independently caused reductions in cellular cholesteryl ester. We conclude that clinically available triglyceride-phospholipid emulsions can mobilize macrophage cholesterol in vitro. © 1988 AcademicPress, Inc.
Removal of "accepter"
cholesterol from
particles,
cultured cells
including
HDL
is mediated by
(i),
red
a variety
blood
cells
apoprotein-phospholipid disks (3), and cholesterol-poor phospholipid (4).
of cholesteryl
ester
membrane (2,3).
Of
the
phospholipid liposomes
the cells, uptake of the freely
the accepter, and to make
up for
loss of
cholesterol at
particles studied
definitively shown
the
floating
hydrolysis of intracellular
the
various accepter
have been
the cell
diffusion of the accepter particle into
unstirred water layer that surrounds cholesterol molecule by
(2),
liposomes
The process involves spontaneous desorption of cholesterol from
membrane into the aqueous medium,
of
stores
the
cell
in vitro,
only
to mobilize
cholesterol
from endogenous stores in the whole animal (5,6). In
the
current
study,
we
sought
to
determine
if
Intralipid,
triglyceride-phospholipid emulsion that is commonly administered to humans, macrophages. component is
can
mobilize
cholesterol
Intralipid
contains
cholesteryl
phospholipid
triglyceride-emulsion particles
size (approximately 500nm into the unstirred cholesterol.
and
water layer, and
However,
liposomes,
(5-7).
diameter), emulsion
Because
from but
cultured its
of their
particles would diffuse
hence have poor
emulsion particles
ester
have
access to cell
a large
a
intravenously
capacity
major large poorly
membrane to
carry
*Dr. Aviram was a visiting scientist from the Lipid Research Laboratory, Rambam Medical Center, Haifa, Israel, where reprint requests should be sent. Abbreviations: DMEM, Dulbeceo's Modified Eagle's lipoprotein; HDL, high-density lipoprotein.
709
Medium;
LDL,
low-density
0006-291X/88 $1.50 Copyright © 1988 by Academic Press, Inc. All rights of reproduction in any form reserved.
Vol. 155, No. 2, 1988
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
unesterified cholesterol, which can distribute to the phospholipid surface
and
to the triglyceride core (8). MATERIALS & METHODS Egg phospholipid liposomes were prepared by prolonged sonication (9). 10% and 20% Intralipid were purchased from KabiVitrum (Alameda, CA). Each deciliter of 10% Intralipid contains 10g triglyceride emulsified with 1.2g of phospholipid; 20% Intralipid contains twice the triglyceride (20g/dl) but the same amount of phospholipid (l.2g/dl). Triglyceride emulsion particles were purified from 20% Intralipid by separation from the liposome-rich fraction by ultracentrifugal floatation at d=l.OO6g/ml, to yield "washed" Intralipid (7). Murine J774 macrophage-like cells were maintained in DMEM supplemented with 10% fetal calf serum. Cholesterol-loaded foam cells were prepared by an 18~ incubation with LDL (0.6mg proteig/ml); to cholesterol-label cells, [(-H)-cholesteryl ester]-LDL was added (I0 cpm/ml) (i0,ii). All experiments involved 18h incubations at 37°C in DMEM supplemented with 0.5% bovine serum albumin and the various lipid dispersions described above. To avoid confounding effects from lipoproteins and apolipoproteins, the experimental media contained no serum. Following the experimental incubations, the cells were washed, then analyzed for protein (12), unesterified cholesterol, and cholesteryl ester mass (13). Radioactivity r~tained by the choles~erol-labeled macrophages was determined. Cellular [~H]-cholesterol and [~H]-cholesteryl ester were separated by thin-layer chromatography (14) .±~., Cellular cholesterol synthesis [W~c]aSsessed by the conversion of [1,2- C]-sodium acetate (i0 Ci/ml) into -cholesterol and cholesteryl ester. All data are displayed as means ± standard error of the mean, n=6. RESULTS An 18h
incubation
with 10%
Intralipid
cellular cholesteryl ester mass, in
A.
o5
IOO
Fc
reductions At
B. CHOLESTEROLLOADED CELLS
NONLOADED CELLS
o.'i
caused pronounced
a dose-dependent fashon (fig. i).
2OO
i
~=E so
Ioo
..I .J i,i 0
O TRIG .YCERIDE
I
I
I
I
I00
200
I00
200
PHO~;PHOLIPID
12
24
12
24
0
INTRALIP1D CONCENTRATION (mg/dl)
Figure !. Effect of a triglyceride-phospholipid emulsion on the cholesterol content of macrophages. J774 cells were incubated for 18h with 10% Intralipid at the indicated concentrations in serum-free media. Cells were then analyzed for unesterified (e) and esterified (0) cholesterol contents. A: Cells not pre-leaded; B: cells pre-loaded with cholesterol.
710
in the
Vol. 155, NO. 2, 1988
BIOCHEMICAL A N D BIOPHYSICAL RESEARCH COMMUNICATIONS
g.
A.
CHOLESTEROL LOADED
NONLOADED CELLS
pz ~ I.-
z o ,£,)~ n-
~ .~ELLS
IO0
IOO
FCj,
o
p-,._ if) o
~
s0
50
7"-O _.1 --I U.I rO I
'
0
12
I
24
I
12
0
24
PHOSPI-IOIIPID CONCENTRATION (mg/dl)
EMULSION
Figure 2. Effect of emulsion phospholipid concentrations on maorophage cholesterol. J774 cells were incubated for 18h in media containing 200mg of emulsion triglyceride/dl and the indicated concentrations of emulsion phospholipid. Cells were then analyzed for unesterified (e) and esterified (0) cholesterol contents. A: Cells not pre-loaded; B: cells pre-loaded with cholesterol. Washed, 20%, and 10% Intralipid were used to achieve the phospholipid concentrations of 6, 12, and 24mg/dl of medium, respectively.
highest
concentration
of
Intralipid
tested,
J774
cells
ester and cells
preloaded
with
that had not
been
cholesterol lost: 55%
of their cholesteryl
pre-loaded lost 28%.
Free cholesterol content also decreased (fig. i).
Triglyeeride-emulsions particles, without liposomes, reducing cellular cholesteryl
ester mass
were also capable
(fig. 2A and
2B, leftmost
At the same triglyceride concentration, 20% and 10% Intralipid (24 phospholipid/dl of
medium,
cellular cholesterol phospholipid/dl),
respectively)
and cholesteryl
indicating
were
ester
more
than was
additive effects
effective
and 12mg of at
removing
washed Intralipid
from the
of
points).
content of
(6mg
liposomes
(fig. 2). Similarly,
in
comparing
lipid
concentration, those with higher
dispersions
of
constant
phospholipid
triglyceride concentrations effected
losses of cellular cholesterol and cholesteryl ester (fig. 3). pre-loaded cells,
media containing
media, 12mg phospholipid/dl) mass
than
did
phospholipid/dl) Reduction in
media
containing
liposomes
macrophage cholesterol (fig.
cellular
losses.
cholesterol
4A).
cholesterol mobilization by lipid from the cells (fig. 4B). the
(200mg triglyceride/dl
lower cellular cholesteryl (no
of
ester
triglyceride,
12mg
(fig. 3B).
cholesterol synthesis
paralleled
20% Intralipid
produced a 30%
greater
In cholesterol
patterns
phospholipid concentration
content was not
Synthesis The
mechanism
caused by
increased
to
responsible
compensate for
macrophage
(12mg/dl
cholesterol
of medium),
dispersions with higher triglyceride contents. 711
more
mass: loss was
for
macrophage
dispersions was enhanced cholesterol
The patterns for retained cholesterol for
decreased
efflux
radioactivity at
a
fixed
produced
by
Vol. 155, No. 2, 1988
A.
l,.-
z bJ l-Z 0
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
NONLOADEDCELLS
B. CHOLESTEROL LOADED
I00
IOO
50
50
J~
w
F-,,.
mo -r .-1 -J
0
I
I
0
I
I00
200
I
I
0
I
IOO
200
EMULSION TRIGLYCERIDE CONCENTRATION (mg/dl) Figure 3. Effect of triglyceride concentrations on macrophage cholesterol. Cells (A: not pre-loaded; B: pre-loaded with cholesterol) were incubated in media containing 12mg of phospholipid/dl and the indicated concentrations of triglyceride. Cells were analyzed for unesterified cholesterol (I) and esterified cholesterol (0). Pure phospholipid liposomes, 10% Intralipid, and 20% Intralipid were used to achieve the triglyceride concentrations of 0, i00, and 200mg/dl, respectively.
DISCUSSION We
have
emulsion,
shown
Intralipid,
cultured macrophages. which were
that can
a
clinically
available
substantially
triglyceride-phospholipid
reduce the
cholesterol
The effect was m o s t p r o n o u n c e d
pre-loaded with
m e d i a t e d b y an e n h a n c e m e n t
cholesterol. of
Cellular
cholesterol
in our
cholesterol
reduction
e f f l u x b y the emulsion.
g. ..J 0
~
content
of
m o d e l foam cells,
Both
was types
CHOLESTEROL EFFLUX
I0,-
w I-
A.
w _J
=
z
7
CHOLESTEROL SYNTHESIS
Q.
w"
'
~u m o-r
~
2
~ Control 0
Z
-1
/ ufl t.9
-x
IOO
20
3OO
~ EMULSION TRIGLYCERIDE CONCENTRATION (rng/dl)
o i
Oontrol 0
i
I00
i
i
200
300
EMULSION TRIGLYCERIDE CONCENTRATION (rag/all)
Figure 4. Effect of lipid dispersions on m~crophage cholesterol synthesis and efflux.- J774 cells were pre-loaded with [ H]-cholesterol, then incubated for 18h in lipid-free medium (control) or in media supplemented with 12mg of phospholipid/dl and the indicated concentrations of triglyceride. Cells were then analyzed f o r cholesterol 3synthesis rate (A) and retained radioactivity (B). [ H]-cholesterol, |; [ H]-cholesteryl ester, 0. Pure phospholipid liposomes, 10% Intralipid, 20% Intralipid, and washed Intralipid were used to achieve the triglyceride concentrations of 0, i00, 200, and 250mg/dl, respectively.
712
Vol. 155, No. 2, 1988
of
particles
particles,
in
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Intralipid,
liposomes
and
large
triglyeeride-emulsion
contributed to the effect.
Our results with pure
triglyeeride-emulsion particles show that, in
spite
of their large size, they were extremely effective cholesterol accepters.
Per
unit mass of phospholipid, macrophages.
It
has
they are more effective than liposomes
been
shown
elsewhere
partitions into the
triglyceride core
large
core
triglyceride
triglyceride-emulsion
can
act
that
unesterified
of emulsion particles
as
a
cholesterol
at unloading cholesterol
( 8 ) . Thus,
sink.
the
Efficacy
particles as cholesterol accepters in vivo, however,
be limited by t]heir short
residence time in the circulation (15), which
of may
would
limit the time to equilibrate with endogenous cholesterol stores (3,5,6). Overall,
we
have
shown
that
intravenously into humans, can vitro. particles,
Recent and
studies
have
Intralipid
atherogenie lipoproteins
Intralipid,
which
is
promote cholesterol efflux shown
can
that
also
liposomes,
block
influx
into model foam cells (11,16).
commonly
infused
from foam cells
i_nn
triglyceride-emulsion of
cholesterol
These results
from suggest
a possible anti.-atherogenic role for emulsions. ACKNOWLEDGEMENTS This work was supported by grants HL38956, HL21006, and HL40404 from the National Institutes of Health. K.J. Williams is a recipient of a Clinician-Scientist Award from the American Heart Association, with funds contributed in part by the AHA-New York City Affiliate.
REFERENCES i. Baily, J.M. (1965) Exp. Cell Res. 37,175-182. 2, He, Y.K., Brown, M.S., and Goldstein, J.L. (1980) J. Lipid Res. 21,391-398. 3. Phillips, M.C., Johnson, W.J., and Rothblat, G.H. (1987) Biochim. Biophys. Aeta 906,223-276. 4. Yau-Young, A.O., Rothblat, G.H., and Small, D.M. (1982) Biochim. Biophys. Acta 710,181-187. 5. Williams, K.J., and Scanu, A.M. (1986) Biochim. Biopbys. Aeta 875,183-194. 6. Williams, K.J., Vallabhajosula, S., Rahman, I.U. Dcnnelly, T.M., Parker, T.S., Weinraueh, M., and Goldsmith, S.J. (1987) P~oc. Natl. Acad. Sci. USA 85,242-246. 7. Granot, E., Deckelbaum, R.J., Eisenberg, S., Oschry, Y., and Olivecrona, G.B. (1985) Biochim. Biophys. Acta 833,308.~;[5 8. Miller, K.W., and Small, D.M. (1982) J. Ce!!~id. Inter. Sci. 89,466-478. 9. Huang, C., and Thompson, T.E. (1974) Methods Enzymol. 32,485-489. I0. Tabas, I., Weiland, D.A., and Tall. A.R. (1985) Prec. Natl. Acad. Sci. USA 82,416-420. ii. Williams, K.J., Tall, A.R., Bisgaier, C., and Broeia, R. (1987) J. Clin. Invest. 79,1466-1472. 12. Lowry, O.H., Rosebrough, N.J., Farr, A.L., and Randall~, R.J. (1951) J. Biol. Chem. 193,265-275. 13. Ishikawa, T.T., MacGee, J., Morrison, J.A., and Glueck, C.J. (1974) J. Lipid Res. 15,286-291. 14. Mangold, H.K. (1969) In Thin-layer Chromatography. A Laboratory Handbook. (E. Stahl, Ed.), pp. 363-421. Springer-Verlag, New York. 15. Untraeht, S.H. (1982) Bioehim. Biophys. Acta 711,176-192. 16. Aviram, M., Williams, K.J., MeIntosh, R.A., Carpentier, Y., Tall, A., and Deckelbaum, R.J. (1988) Arteriosclerosis, in press.
713
Vol. 155, No. 2, 1988
Pages 709-713
September 15, 1988
MACROPHAGE CHOLESTEROL REMOVAL BY TRICLYCERIDE-PHOSPHOLIPID EMULSIONS Michael Aviram~ Kevin Jon Williams, and Richard J. Deckelbaum Columbia University, College of Physicians & Surgeons New York, New York 10032 Received May 25, 1988
SUMMARY: Phospholipid liposomes were previously shown to mobilize cholesterol from cultured macrophage foam cells. Because Intralipid, a clinically available triglyceride-phospholipid emulsion, contains both phospholipid liposomes and triglyceride-emulsion particles, we sought to study its effect on macrophage clholesterol mobilization. Following an 18h incubation of J774 macrophages in serum-free medium supplemented with Intralipid, cholesteryl ester content decreased by up to 50% in previously cholesterol-loaded cells, and by 25% in non-loaded cells. Both components of Intralipid, liposomes and emulsion particles, independently caused reductions in cellular cholesteryl ester. We conclude that clinically available triglyceride-phospholipid emulsions can mobilize macrophage cholesterol in vitro. © 1988 AcademicPress, Inc.
Removal of "accepter"
cholesterol from
particles,
cultured cells
including
HDL
is mediated by
(i),
red
a variety
blood
cells
apoprotein-phospholipid disks (3), and cholesterol-poor phospholipid (4).
of cholesteryl
ester
membrane (2,3).
Of
the
phospholipid liposomes
the cells, uptake of the freely
the accepter, and to make
up for
loss of
cholesterol at
particles studied
definitively shown
the
floating
hydrolysis of intracellular
the
various accepter
have been
the cell
diffusion of the accepter particle into
unstirred water layer that surrounds cholesterol molecule by
(2),
liposomes
The process involves spontaneous desorption of cholesterol from
membrane into the aqueous medium,
of
stores
the
cell
in vitro,
only
to mobilize
cholesterol
from endogenous stores in the whole animal (5,6). In
the
current
study,
we
sought
to
determine
if
Intralipid,
triglyceride-phospholipid emulsion that is commonly administered to humans, macrophages. component is
can
mobilize
cholesterol
Intralipid
contains
cholesteryl
phospholipid
triglyceride-emulsion particles
size (approximately 500nm into the unstirred cholesterol.
and
water layer, and
However,
liposomes,
(5-7).
diameter), emulsion
Because
from but
cultured its
of their
particles would diffuse
hence have poor
emulsion particles
ester
have
access to cell
a large
a
intravenously
capacity
major large poorly
membrane to
carry
*Dr. Aviram was a visiting scientist from the Lipid Research Laboratory, Rambam Medical Center, Haifa, Israel, where reprint requests should be sent. Abbreviations: DMEM, Dulbeceo's Modified Eagle's lipoprotein; HDL, high-density lipoprotein.
709
Medium;
LDL,
low-density
0006-291X/88 $1.50 Copyright © 1988 by Academic Press, Inc. All rights of reproduction in any form reserved.
Vol. 155, No. 2, 1988
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
unesterified cholesterol, which can distribute to the phospholipid surface
and
to the triglyceride core (8). MATERIALS & METHODS Egg phospholipid liposomes were prepared by prolonged sonication (9). 10% and 20% Intralipid were purchased from KabiVitrum (Alameda, CA). Each deciliter of 10% Intralipid contains 10g triglyceride emulsified with 1.2g of phospholipid; 20% Intralipid contains twice the triglyceride (20g/dl) but the same amount of phospholipid (l.2g/dl). Triglyceride emulsion particles were purified from 20% Intralipid by separation from the liposome-rich fraction by ultracentrifugal floatation at d=l.OO6g/ml, to yield "washed" Intralipid (7). Murine J774 macrophage-like cells were maintained in DMEM supplemented with 10% fetal calf serum. Cholesterol-loaded foam cells were prepared by an 18~ incubation with LDL (0.6mg proteig/ml); to cholesterol-label cells, [(-H)-cholesteryl ester]-LDL was added (I0 cpm/ml) (i0,ii). All experiments involved 18h incubations at 37°C in DMEM supplemented with 0.5% bovine serum albumin and the various lipid dispersions described above. To avoid confounding effects from lipoproteins and apolipoproteins, the experimental media contained no serum. Following the experimental incubations, the cells were washed, then analyzed for protein (12), unesterified cholesterol, and cholesteryl ester mass (13). Radioactivity r~tained by the choles~erol-labeled macrophages was determined. Cellular [~H]-cholesterol and [~H]-cholesteryl ester were separated by thin-layer chromatography (14) .±~., Cellular cholesterol synthesis [W~c]aSsessed by the conversion of [1,2- C]-sodium acetate (i0 Ci/ml) into -cholesterol and cholesteryl ester. All data are displayed as means ± standard error of the mean, n=6. RESULTS An 18h
incubation
with 10%
Intralipid
cellular cholesteryl ester mass, in
A.
o5
IOO
Fc
reductions At
B. CHOLESTEROLLOADED CELLS
NONLOADED CELLS
o.'i
caused pronounced
a dose-dependent fashon (fig. i).
2OO
i
~=E so
Ioo
..I .J i,i 0
O TRIG .YCERIDE
I
I
I
I
I00
200
I00
200
PHO~;PHOLIPID
12
24
12
24
0
INTRALIP1D CONCENTRATION (mg/dl)
Figure !. Effect of a triglyceride-phospholipid emulsion on the cholesterol content of macrophages. J774 cells were incubated for 18h with 10% Intralipid at the indicated concentrations in serum-free media. Cells were then analyzed for unesterified (e) and esterified (0) cholesterol contents. A: Cells not pre-leaded; B: cells pre-loaded with cholesterol.
710
in the
Vol. 155, NO. 2, 1988
BIOCHEMICAL A N D BIOPHYSICAL RESEARCH COMMUNICATIONS
g.
A.
CHOLESTEROL LOADED
NONLOADED CELLS
pz ~ I.-
z o ,£,)~ n-
~ .~ELLS
IO0
IOO
FCj,
o
p-,._ if) o
~
s0
50
7"-O _.1 --I U.I rO I
'
0
12
I
24
I
12
0
24
PHOSPI-IOIIPID CONCENTRATION (mg/dl)
EMULSION
Figure 2. Effect of emulsion phospholipid concentrations on maorophage cholesterol. J774 cells were incubated for 18h in media containing 200mg of emulsion triglyceride/dl and the indicated concentrations of emulsion phospholipid. Cells were then analyzed for unesterified (e) and esterified (0) cholesterol contents. A: Cells not pre-loaded; B: cells pre-loaded with cholesterol. Washed, 20%, and 10% Intralipid were used to achieve the phospholipid concentrations of 6, 12, and 24mg/dl of medium, respectively.
highest
concentration
of
Intralipid
tested,
J774
cells
ester and cells
preloaded
with
that had not
been
cholesterol lost: 55%
of their cholesteryl
pre-loaded lost 28%.
Free cholesterol content also decreased (fig. i).
Triglyeeride-emulsions particles, without liposomes, reducing cellular cholesteryl
ester mass
were also capable
(fig. 2A and
2B, leftmost
At the same triglyceride concentration, 20% and 10% Intralipid (24 phospholipid/dl of
medium,
cellular cholesterol phospholipid/dl),
respectively)
and cholesteryl
indicating
were
ester
more
than was
additive effects
effective
and 12mg of at
removing
washed Intralipid
from the
of
points).
content of
(6mg
liposomes
(fig. 2). Similarly,
in
comparing
lipid
concentration, those with higher
dispersions
of
constant
phospholipid
triglyceride concentrations effected
losses of cellular cholesterol and cholesteryl ester (fig. 3). pre-loaded cells,
media containing
media, 12mg phospholipid/dl) mass
than
did
phospholipid/dl) Reduction in
media
containing
liposomes
macrophage cholesterol (fig.
cellular
losses.
cholesterol
4A).
cholesterol mobilization by lipid from the cells (fig. 4B). the
(200mg triglyceride/dl
lower cellular cholesteryl (no
of
ester
triglyceride,
12mg
(fig. 3B).
cholesterol synthesis
paralleled
20% Intralipid
produced a 30%
greater
In cholesterol
patterns
phospholipid concentration
content was not
Synthesis The
mechanism
caused by
increased
to
responsible
compensate for
macrophage
(12mg/dl
cholesterol
of medium),
dispersions with higher triglyceride contents. 711
more
mass: loss was
for
macrophage
dispersions was enhanced cholesterol
The patterns for retained cholesterol for
decreased
efflux
radioactivity at
a
fixed
produced
by
Vol. 155, No. 2, 1988
A.
l,.-
z bJ l-Z 0
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
NONLOADEDCELLS
B. CHOLESTEROL LOADED
I00
IOO
50
50
J~
w
F-,,.
mo -r .-1 -J
0
I
I
0
I
I00
200
I
I
0
I
IOO
200
EMULSION TRIGLYCERIDE CONCENTRATION (mg/dl) Figure 3. Effect of triglyceride concentrations on macrophage cholesterol. Cells (A: not pre-loaded; B: pre-loaded with cholesterol) were incubated in media containing 12mg of phospholipid/dl and the indicated concentrations of triglyceride. Cells were analyzed for unesterified cholesterol (I) and esterified cholesterol (0). Pure phospholipid liposomes, 10% Intralipid, and 20% Intralipid were used to achieve the triglyceride concentrations of 0, i00, and 200mg/dl, respectively.
DISCUSSION We
have
emulsion,
shown
Intralipid,
cultured macrophages. which were
that can
a
clinically
available
substantially
triglyceride-phospholipid
reduce the
cholesterol
The effect was m o s t p r o n o u n c e d
pre-loaded with
m e d i a t e d b y an e n h a n c e m e n t
cholesterol. of
Cellular
cholesterol
in our
cholesterol
reduction
e f f l u x b y the emulsion.
g. ..J 0
~
content
of
m o d e l foam cells,
Both
was types
CHOLESTEROL EFFLUX
I0,-
w I-
A.
w _J
=
z
7
CHOLESTEROL SYNTHESIS
Q.
w"
'
~u m o-r
~
2
~ Control 0
Z
-1
/ ufl t.9
-x
IOO
20
3OO
~ EMULSION TRIGLYCERIDE CONCENTRATION (rng/dl)
o i
Oontrol 0
i
I00
i
i
200
300
EMULSION TRIGLYCERIDE CONCENTRATION (rag/all)
Figure 4. Effect of lipid dispersions on m~crophage cholesterol synthesis and efflux.- J774 cells were pre-loaded with [ H]-cholesterol, then incubated for 18h in lipid-free medium (control) or in media supplemented with 12mg of phospholipid/dl and the indicated concentrations of triglyceride. Cells were then analyzed f o r cholesterol 3synthesis rate (A) and retained radioactivity (B). [ H]-cholesterol, |; [ H]-cholesteryl ester, 0. Pure phospholipid liposomes, 10% Intralipid, 20% Intralipid, and washed Intralipid were used to achieve the triglyceride concentrations of 0, i00, 200, and 250mg/dl, respectively.
712
Vol. 155, No. 2, 1988
of
particles
particles,
in
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Intralipid,
liposomes
and
large
triglyeeride-emulsion
contributed to the effect.
Our results with pure
triglyeeride-emulsion particles show that, in
spite
of their large size, they were extremely effective cholesterol accepters.
Per
unit mass of phospholipid, macrophages.
It
has
they are more effective than liposomes
been
shown
elsewhere
partitions into the
triglyceride core
large
core
triglyceride
triglyceride-emulsion
can
act
that
unesterified
of emulsion particles
as
a
cholesterol
at unloading cholesterol
( 8 ) . Thus,
sink.
the
Efficacy
particles as cholesterol accepters in vivo, however,
be limited by t]heir short
residence time in the circulation (15), which
of may
would
limit the time to equilibrate with endogenous cholesterol stores (3,5,6). Overall,
we
have
shown
that
intravenously into humans, can vitro. particles,
Recent and
studies
have
Intralipid
atherogenie lipoproteins
Intralipid,
which
is
promote cholesterol efflux shown
can
that
also
liposomes,
block
influx
into model foam cells (11,16).
commonly
infused
from foam cells
i_nn
triglyceride-emulsion of
cholesterol
These results
from suggest
a possible anti.-atherogenic role for emulsions. ACKNOWLEDGEMENTS This work was supported by grants HL38956, HL21006, and HL40404 from the National Institutes of Health. K.J. Williams is a recipient of a Clinician-Scientist Award from the American Heart Association, with funds contributed in part by the AHA-New York City Affiliate.
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