Defective metabolism of hypertriglyceridemic low density lipoprotein in cultured human skin fibroblasts. Normalization with bezafibrate therapy.

Kleinman, Yosef; Eisenberg, Shlomo; Oschry, Yitzchak; Gavish, Dov; Stein, O.; Stein, Y.

doi:10.1172/jci111892

Cited by 125 publications

(38 citation statements)

References 45 publications

(27 reference statements)

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“…Our data (Table III) confirm the previous reports ofreduced uptake of LDL derived from hypertriglyceridemic subjects in fibroblast culture (8,44). In contrast, with HepG2 cells there was enhanced uptake of native and in vitro hypertriglyceridemic LDL (Figs.…”

Section: Discussionsupporting

confidence: 92%

Plasma triglycerides determine low density lipoprotein composition, physical properties, and cell-specific binding in cultured cells.

McKeone¹,

Patsch²,

Pownall³

1993

J. Clin. Invest.

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The relationship between the plasma triglycerides and the LDL triglycerides of 30 normal and 48 hypertriglyceridemic subjects has been quantified; the data fit a simple adsorption isotherm, LDL triglyceride/(LDL triglyceride + LDL cholesterol ester) = 0.65 plasma triglyceride/(464 + plasma triglyceride). In vitro transfer of triglyceride from concentrated VLDL to VLDL-depleted plasma produced triglyceride-rich LDL that had similar properties. LDL uptake by HepG2 cells increased with LDL triglyceride content whereas the reverse was found with skin fibroblasts. At 370C, the cores of both normal and hypertriglyceridemic LDL were isotropic liquids. Circular dichroic spectra revealed no difference in the secondary structure of normal and triglyceride-rich LDL. The affinity of monoclonal antibody MB47, which binds to the receptor ligand of apo B-100 was independent of LDL triglyceride content. MB3, which binds near residue 1022 ofapo B-100, showed a triglyceride-dependent decrease in affinity for LDL from hypertriglyceridemic subjects and from in vitro incubations. LDL with an elevated triglyceride content formed in vitro had reduced proteolytic cleavage of apo B-100 by Staphylococcus aureus V8 protease. From these data, we infer that (a) LDL triglyceride is a predictable function of plasma triglyceride, (b) triglyceride induces subtle changes in apo B-100 structure at a site that is remote from the putative receptor binding ligand, and (c) the triglyceride-dependent receptor-binding determinants of apo B-100 are recognized differently by fibroblasts and HepG2

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Section: Discussionsupporting

confidence: 92%

Plasma triglycerides determine low density lipoprotein composition, physical properties, and cell-specific binding in cultured cells.

McKeone¹,

Patsch²,

Pownall³

1993

J. Clin. Invest.

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“…Human skin fibroblasts were prepared from skin biopsies obtained from the medial part of the forearm of normal adult male donors (21 (12) except that the cells were grown in 35-mm dishes as above.…”

Section: Methodsmentioning

confidence: 99%

“…Binding, cell association, and proteolytic degradation of 123I-labeled lipoproteins were determined as previously described (21). On the day ofexperiment, the fresh medium was removed and the cells were incubated at 37°C with LPDS medium containing lipolyzed or control 1251I-VLDL-I, -II, or -III (apo B-100 equivalent to 10 gg protein/ml).…”

Section: Methodsmentioning

confidence: 99%

Lipolysis exposes unreactive endogenous apolipoprotein E-3 in human and rat plasma very low density lipoprotein.

et al. 1991

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Endogenous apolipoprotein E in VLDL is poorly expressed in receptor binding processes The ligand responsible for receptor interaction of lipolyzed VLDL (apo E or apo B-100) and its source (endogenous or transferred) was studied with monoclonal antibodies and with lipoproteins from E-3/3 and E-2/2 subjects. The data unequivocally proved that lipolysis causes exposure of unreactive endogenous apo E-3 at the VLDL surface, possibly by a change of conformation of the protein. Apo B-100 becomes biologically expressed only in lipolyzed VLDL-III. Lipolyzed VLDL, however, is less reactive to exogenous apo E-3 than control VLDL indicating that endogenous and exogenous apo E are oriented differently in VLDL. It is proposed that VLDL delivers triglycerides to tissues when apo E is unreactive but becomes a remnant after the protein becomes exposed and directs the particles from lipoprotein lipase sites to cellular receptors. (J. Clin. Invest. 1991. 88:553-560.)

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“…Fibrates lower triglycerides by limiting substrate availability for triglyceride synthesis in the liver [23,24] , promoting the action of lipoprotein lipase [25,26] , enhancing LDL receptor/ligand interaction [27] , promoting cholesterol excretion via bile [28] and stimulating reverse cholesterol transport [29] . The ultimate result is a reduction in triglyceride and LDL-C levels, but the data on HDL-C are varied.…”

Section: Leptinmentioning

confidence: 99%

Pharmacological effects of lipid-lowering drugs on circulating adipokines

Wanders

Plaisance²,

Judd³

2010

WJD

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The cardioprotective effects of lipid-lowering drugs have been primarily attributed to their effects on blood lipid metabolism. However, emerging evidence indicates that lipid-lowering drugs also modulate the synthesis and secretion of adipose tissue-secreted proteins referred to as adipokines. Adipokines influence energy homeostasis and metabolism and have also been shown to modulate the vascular inflammatory cascade. The purpose of this review will be to examine the reported effects of commonly used lipid-lowering drugs (statins, fibrates, niacin and omega-3-fatty acids) on the circulating concentrations of leptin, adiponectin, tumor necrosisfactor-α (TNF-α), Retinol binding protein 4 (RBP4) and resistin. Overall, the lipid-lowering drugs reviewed have minimal effects on leptin and resistin concentrations. Conversely, circulating adiponectin concentrations are consistently increased by each lipid-lowering drug reviewed with the greatest effects produced by niacin. Studies that have examined the effects of statins, niacin and omega-3-fatty acids on TNF-α demonstrate that these agents have little effect on circulating TNF-α concentrations. Niacin and fibrates appear to lower RBP4 but not resistin concentrations. The results of the available studies suggest that a strong relationship exists between pharmacological reductions in blood lipids and adiponectin that is not obvious for other adipokines reviewed.

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Defective metabolism of hypertriglyceridemic low density lipoprotein in cultured human skin fibroblasts. Normalization with bezafibrate therapy.

Cited by 125 publications

References 45 publications

Plasma triglycerides determine low density lipoprotein composition, physical properties, and cell-specific binding in cultured cells.

Plasma triglycerides determine low density lipoprotein composition, physical properties, and cell-specific binding in cultured cells.

Lipolysis exposes unreactive endogenous apolipoprotein E-3 in human and rat plasma very low density lipoprotein.

Pharmacological effects of lipid-lowering drugs on circulating adipokines

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