Expression of human hepatic lipase negatively impacts apolipoprotein A-Ⅰ production in primary hepat

来源 :The Journal of Biomedical Research | 被引量 : 0次 | 上传用户:lengxiang520
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This study aimed to examine whether expression of human hepatic lipase(hHL) exerted an intracellular effect on hepatic production of apolipoprotein(apo) A-I.The levels of secreted and cell-associated apoA-I were contrasted between primary hepatocytes isolated from Lipc-nuW and C57BL/6 mice,and between Lipc-nuW hepatocytes transfected with either hHL-encoding or control adenovirus.An HSPG-binding deficient hHL protein(hHLmt) was used to determine the impact of cell surface binding on HL action.Accumulation of apoA-I in conditioned media of primary hepatocytes isolated from Lipc-nuW mice was increased as compared to that from C57BL/6 mice.Metabolic labeling experiments showed that secretion of ’’S-apoA-I from Lipc-nuW cells was significantly higher than that from C57BL/6 cells.Expression of hHL in Lipc-nuW hepatocytes,through adenovirus-mediated gene transfer,resulted in decreased synthesis and secretion of ’S-apoA-I,but not S-apoE,as compared with cells transfected with control adenovirus.Expression of HSPG-binding deficient hHLmt in Lipc-nuW cells also exerted an inhibitory effect on apoA-I production,even though hHLmt displayed impaired exit from the endoplasmic reticulum as compared with hHL.Subcellular fractionation revealed that expression of hHL or hHLmt led to increased microsome-association of apoA-I relative to non-transfected control.Expression of hHL negatively impacts hepatic production of apoA-I. This study aimed to examine whether expression of human hepatic lipase (hHL) exerted an intracellular effect on hepatic production of apolipoprotein (apo) AI. These levels of secreted and cell-associated apoA-I were contrasted between primary hepatocytes isolated from Lipc-nuW and C57BL / 6 mice, and between Lipc-nuW hepatocytes transfected with either hHL-encoding or control adenovirus. An HSPG-binding deficient hHL protein (hHLmt) was used to determine the impact of cell surface binding on HL action. in conditioned media of primary hepatocytes isolated from Lipc-nuW mice was increased as compared to that from C57BL / 6 mice. Metabolic labeling experiments showed that secretion of ’S-apoA-I from Lipc-nuW cells was significantly higher than that from C57BL / 6 cells. Expression of hHL in Lipc-nuW hepatocytes, through adenovirus-mediated gene transfer, resulted in decreased synthesis and secretion of ’S-apoA-I, but not S-apoE, as compared with cells transfected with control adenovir us. Expression of HSPG-binding deficient hHLmt in Lipc-nuW cells also exerted an inhibitory effect on apoA-I production, even though hHLmt displayed impaired exit from the endoplasmic reticulum as compared with hHL. Subcellular fractionation revealed that that hlL or hHLmt led to increased microsome-association of apoA-I relative to non-transfected control. Expression of hHL negatively productive hepatic production of apoA-I.
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