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Journal of Lipid Research, Vol 38, 1649-1659, Copyright © 1997 by Lipid Research, Inc.
CE MacPhee, RY Chan, WH Sawyer, WF Stafford and GJ Howlett
The central function of lipoprotein lipase (LpL) is to hydrolyze
triacylglycerols in chylomicrons and very low density lipoproteins. We have
examined the binding of purified milk lipoprotein lipase to homogeneous
synthetic lipid emulsions. Emulsions composed of either naturally occurring
ester-linked lipids or the non-hydrolyzable ether analogues were prepared
by sonication and pressure extrusion, and fractionated by sucrose density
gradient centrifugation. Flotation analysis using the analytical
ultracentrifuge indicated that the individual fractions were relatively
homogeneous with respect to size with flotation coefficients and molecular
weights for the separated fractions ranging from 100 to 1100 S and 5.2 x
10(7) to 6.0 x 10(8), respectively. Purified milk lipoprotein lipase bound
with high affinity and in a saturable manner to emulsions prepared from the
non- hydrolyzable ether-linked lipid analogues of 1-oleoyl, 2-palmitoyl
phosphatidylcholine and triolein. At low concentrations of LpL, the enzyme
caused aggregation of the emulsion particles by interparticle
cross-linking. At higher LpL concentrations, the flotation coefficient of
the emulsions decreased significantly with a concomitant increase in
particle density. At saturation, the number of LpL monomers bound to lipid
particles of radii 67, 75, and 79 nm was 1315, 1449, and 1466,
respectively. The results demonstrate close packing of LpL on the lipid
surface and are consistent with there being little disruption to the
overall structure of the emulsion particle.
ARTICLES
Interaction of lipoprotein lipase with homogeneous lipid emulsions
Russell Grimwade School of Biochemistry and Molecular Biology, University of Melbourne, Parkville, Victoria, Australia.
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