Levels of plasma HDL are determined in part by catabolism in the liver. However, it is unclear how the hepatic catabolism of holo-HDL is regulated or mediated. Recently, we found that ob/ob mice have defective liver catabolism of HDL apoproteins in vivo that can be reversed by low-dose leptin treatment. Here we examined HDL catabolism and trafficking at the cellular level using isolated hepatocytes. We demonstrate that ob/ob hepatocytes have reduced binding, association, degradation, and resecretion of HDL apoproteins and 50% less selective lipid uptake relative to wild-type hepatocytes. In addition, HDL apoproteins were found to colocalize with transferrin in the general endosomal recycling compartment (ERC) in wild-type hepatocytes. However, the localization to the ERC was markedly reduced in ob/ob hepatocytes. Filipin staining of cellular cholesterol revealed decreased cholesterol in the ERC in ob/ob hepatocytes. Defects in HDL cell association and cholesterol distribution were reversed by leptin administration. The findings show a major defect in HDL uptake and recycling in ob/ob hepatocytes and suggest that HDL recycling through the ERC plays a role in the determination of plasma HDL protein and cholesterol levels.
David L. Silver, Nan Wang, Alan R. Tall
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A gene-expression screen identifies a non-toxic sumoylation inhibitor that mimics SUMO-less human LRH-1 in liver: ( A ) Schematic of hLRH-1 protein (NR5A2 isoform 1) showing the location of major sumoylation sites at K192 and K270, and the minor K44 site (top panel). WT and SUMO-less forms of hLRH-1 (3KR and 2KR) expressed in JEG3 and HepG2 cells are indicated as detected with anti-Flag antibody. Unsumoylated (hLRH-1) as well as sumoylated hLRH-1 species (1x, 2x, and 3x) are indicated in bottom panel by arrows. Additional bands observed in HepG2 cells that persist after mutating both K192 and K270 are indicated with asterisk (*). Strategy used to humanize mouse liver for expression of wild type or SUMO-less (2KR) hLRH-1. ( B ) Sumoylated hLRH-1 species detected by anti-Flag in harvested livers after first infecting with AAV8-vectors expressing eGFP, WT or 2KR. ( C ) Relative transcripts levels of hLRH-1 transcripts in mouse livers infected with recombinant AAV8-vectors expressing eGFP, wild-type hLRH-1 (WT) or SUMO-less hLRH-1 (2KR). ( D ) Staining for tagged-hLRH-1 as detected by immunofluorescence using anti-Flag (white arrows). Hepatocytes are prepared as described in ‘Materials and methods’ from harvested, perfused livers 2 weeks post retro-orbital viral-mediated infection
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1999 George Lyman Duff memorial lecture: lipid transfer proteins, HDL metabolism, and atherogenesis
AR Tall, X Jiang, Y Luo, D Silver |
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