Abstract
In isolated cell studies, the internalization and degradation of hepatic lipase (HL) has been linked to its binding to the low density lipoprotein receptor-related protein (LRP). We have utilized the receptor-associated protein (RAP), a universal inhibitor of high affinity ligand binding to LRP, to evaluate the participation of LRP in the endocytosis of HL and lipoprotein lipase (LPL). We isolated a total endosome fraction from rat livers after a 30-min infusion of recombinant RAP, administered as a glutathione S-transferase conjugate (GST-RAP). GST-RAP infusion had no effect on the concentration of HL in liver homogenates, but its concentration in blood plasma increased progressively by 20%, and enrichment over homogenate of HL in endosomes was reduced by 50% as compared with infusion of GST alone. The concentrations of LPL in liver and plasma were 1.4 and 0.5%, respectively, those of HL, but endosomal enrichment of the two enzymes was similar ( approximately 10-fold). GST-RAP infusion had no effect on the concentration of LPL in liver but increased its concentration in blood plasma by 250% and reduced its endosomal enrichment by 95% or greater. GST-RAP infusion also reduced endosomal enrichment of LRP by 40%, but enrichment of several other endocytic receptors was unaffected. Endosomal enrichment of several membrane trafficking proteins associated with the endocytic pathway in hepatocytes was unaffected by GST-RAP with the exception of early endosome endosome antigen 1, which was reduced by 85%. We conclude that HL is partially and LPL almost exclusively taken up into rat hepatocytes after binding to the endocytic receptor LRP.
Highlights
Hepatic lipase (HL)1 is synthesized by hepatocytes and resides on liver cell surfaces, presumably bound to heparan sul
In light of these observations in cultured cells, we have pursued our earlier observation [16] that HL is concentrated in hepatocytic endosomes from rat liver, and we report here evidence that lipoprotein receptor-related protein (LRP) contributes in vivo to the endocytosis of HL destined for lysosomal degradation
We have determined the effect of glutathione S-transferase (GST)-receptor-associated protein (RAP) upon the concentration of HL and lipoprotein lipase (LPL) in endosomes isolated from rat liver in order to evaluate the role of LRP in the endocytosis of these lipolytic enzymes
Summary
Reagents and Antibodies—␣2-Macroglobulin (␣2MG) (Sigma) was activated with methylamine and radioiodinated (125I) as described [18]. Isolation of Endosomes—Initial experiments to evaluate the presence and distribution of HL in endosomes were carried out in male Sprague-Dawley rats treated with 17-␣-ethinyl estradiol, which highly induces LDL receptors in hepatocytes. To determine the effect of administering RAP upon the endocytosis of HL and LPL, we used untreated male Sprague-Dawley rats weighing 230 –270 g, from which we isolated a total endosome fraction from liver homogenates. Livers were removed, weighed, and immediately placed in ice-cold 0.15 M NaCl. Routinely, four rats were studied in a given day, receiving GST-RAP and GST alternately, and two livers were used from each group to isolate endosomes. Selection of Dose of GST-RAP—Untreated rats, anesthetized as described above and with cannulated carotid arteries, were injected with various amounts of GST-RAP, administered as a pulse followed by a constant infusion.
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