de Rijke Y B, van Berkel T J
Division of Biopharmaceutics, Leiden-Amsterdam Center for Drug Research, Sylvius Laboratories, University of Leiden, The Netherlands.
J Biol Chem. 1994 Jan 14;269(2):824-7.
The liver is the major organ responsible for the uptake of oxidized low density lipoproteins (Ox-LDL) from the blood circulation with Kupffer cells as major cellular uptake site. Candidate binding proteins for Ox-LDL on membranes from Kupffer and endothelial liver cells were identified with ligand blots. Under nonreducing conditions, a major binding protein with an estimated molecular mass of 95 kDa and a minor stained protein of 220 kDa were detected on Kupffer cell membranes, while endothelial cell membranes expressed only a 220-kDa binding protein. Both the 95-kDa protein of Kupffer cell membranes and the 220-kDa protein of endothelial membranes displayed saturable binding of 125I-Ox-LDL with a Kd of 15 and 5 micrograms/ml, respectively. LDL was a weak competitor for the binding of 125I-Ox-LDL to the 95-kDa protein, while the degree of competition appeared to be dependent on the oxidation grade of LDL with a complete competition with LDL oxidized for 20 h with 10 microM Cu2+. We conclude that the 95-kDa binding protein, highly concentrated on rat Kupffer cells, forms the most likely candidate for mediating the in vivo uptake of Ox-LDL from the blood circulation.
肝脏是负责从血液循环中摄取氧化型低密度脂蛋白(Ox-LDL)的主要器官,库普弗细胞是主要的细胞摄取部位。通过配体印迹法鉴定了库普弗细胞和肝内皮细胞膜上Ox-LDL的候选结合蛋白。在非还原条件下,在库普弗细胞膜上检测到一种估计分子量为95 kDa的主要结合蛋白和一种220 kDa的次要染色蛋白,而内皮细胞膜仅表达一种220 kDa的结合蛋白。库普弗细胞膜上的95 kDa蛋白和内皮细胞膜上的220 kDa蛋白均显示对125I-Ox-LDL的饱和结合,其解离常数(Kd)分别为15和5微克/毫升。低密度脂蛋白(LDL)是125I-Ox-LDL与95 kDa蛋白结合的弱竞争者,而竞争程度似乎取决于LDL的氧化程度,与用10 microM Cu2+氧化20小时的LDL完全竞争。我们得出结论,高度集中在大鼠库普弗细胞上的95 kDa结合蛋白最有可能是介导从血液循环中体内摄取Ox-LDL的候选蛋白。
