Hwang J, Menon K M
J Biol Chem. 1985 May 10;260(9):5660-8.
To determine the apolipoprotein specificity of high density lipoprotein (HDL) receptor, apolipoprotein A-I (apo-AI) and apolipoprotein A-II (apo-AII) purified from high density lipoprotein3 (HDL3) were reconstituted into dimyristoyl phosphatidylcholine vesicles (DMPC) and their ability to bind to luteinized rat ovarian membranes was examined. Both 125I-apo-A-I.DMPC and 125I-apo-A-II.DMPC were shown to bind to ovarian membranes with Kd = 2.87 and 5.70 micrograms of protein/ml, respectively. The binding of both 125I-apo-A-I.DMPC and 125I-apo-A-II.DMPC was inhibited by unlabeled HDL3, apo-A-I.DMPC, apo-A-II.DMPC, apo-C-I.DMPC, apo-C-II.DMPC, apo-C-III1.DMPC, and apo-C-III2.DMPC, but not by DMPC vesicles, bovine serum albumin.DMPC or low density lipoprotein. Since the binding labeled apo-A-I.DMPC and apo-A-II.DMPC was inhibited by the DMPC complexes of apo-C groups, the direct binding of 125I-apo-C-III1.DMPC was also demonstrated with Kd = 9.6 micrograms of protein/ml. In addition, unlabeled apo-A-I.DMPC, and apo-A-II.DMPC, as well as apo-C.DMPC, inhibited 125I-HDL3 binding. 125I-apo-A-I, 125I-apo-A-II, and 125I-apo-C-III1 in the absence of DMPC also bind to the membranes. These results suggest that HDL receptor recognizes apolipoprotein AI, AII, and the C group and that the binding specificity of the reconstituted lipoproteins is conferred by their apolipoprotein moiety rather than the lipid environment. In vivo pretreatment of rats with human chorionic gonadotropin resulted in an increase of 125I-apo-A-I.DMPC, 125I-apo-A-II.DMPC, and 125I-apo-C-III1.DMPC binding activities. However, no induction of binding activity was observed when the apolipoprotein was not included in DMPC vesicles. An examination of the equilibrium dissociation constant and binding capacity for 125I-apo-A-I.DMPC and 125I-apo-A-II.DMPC after human chorionic gonadotropin treatment revealed that the increase in binding activity was due to an increase in the number of binding sites rather than a change in the binding affinity. These results further support our contention that apo-A-I, apo-A-II, and the apo-C group bind to HDL receptor. In conclusion, the HDL receptor of luteinized rat ovary recognizes apolipoproteins A-I, A-II, and the C group but not low density lipoprotein, and the binding is induced by human chorionic gonadotropin in vivo.
为确定高密度脂蛋白(HDL)受体的载脂蛋白特异性,将从高密度脂蛋白3(HDL3)中纯化的载脂蛋白A-I(apo-AI)和载脂蛋白A-II(apo-AII)重组成二肉豆蔻酰磷脂酰胆碱囊泡(DMPC),并检测它们与黄体化大鼠卵巢膜结合的能力。结果显示,125I-apo-A-I.DMPC和125I-apo-A-II.DMPC均能与卵巢膜结合,其解离常数(Kd)分别为2.87和5.70微克蛋白质/毫升。未标记的HDL3、apo-A-I.DMPC、apo-A-II.DMPC、apo-C-I.DMPC、apo-C-II.DMPC、apo-C-III1.DMPC和apo-C-III2.DMPC均可抑制125I-apo-A-I.DMPC和125I-apo-A-II.DMPC的结合,但DMPC囊泡、牛血清白蛋白.DMPC或低密度脂蛋白则无此作用。由于apo-C组的DMPC复合物可抑制标记的apo-A-I.DMPC和apo-A-II.DMPC的结合,因此也证实了125I-apo-C-III1.DMPC的直接结合,其Kd为9.6微克蛋白质/毫升。此外,未标记的apo-A-I.DMPC、apo-A-II.DMPC以及apo-C.DMPC均可抑制125I-HDL3的结合。在无DMPC的情况下,125I-apo-A-I、125I-apo-A-II和125I-apo-C-III1也可与膜结合。这些结果表明,HDL受体可识别载脂蛋白AI、AII和C组,重组脂蛋白的结合特异性由其载脂蛋白部分而非脂质环境决定。用人绒毛膜促性腺激素对大鼠进行体内预处理,可导致125I-apo-A-I.DMPC、125I-apo-A-II.DMPC和125I-apo-C-III1.DMPC的结合活性增加。然而,当载脂蛋白不包含在DMPC囊泡中时,未观察到结合活性的诱导。对人绒毛膜促性腺激素处理后的125I-apo-A-I.DMPC和125I-apo-A-II.DMPC的平衡解离常数和结合容量进行检测发现,结合活性的增加是由于结合位点数量的增加而非结合亲和力的改变。这些结果进一步支持了我们关于apo-A-I、apo-A-II和apo-C组与HDL受体结合的观点。总之,黄体化大鼠卵巢的HDL受体可识别载脂蛋白A-I、A-II和C组,但不识别低密度脂蛋白,且体内人绒毛膜促性腺激素可诱导这种结合。
