Schneider W J, Kovanen P T, Brown M S, Goldstein J L, Utermann G, Weber W, Havel R J, Kotite L, Kane J P, Innerarity T L, Mahley R W
J Clin Invest. 1981 Oct;68(4):1075-85. doi: 10.1172/jci110330.
Patients with familial dysbetalipoproteinemia (F. Dys.), also called familial type 3 hyperlipoproteinemia, are homozygous for a mutant allele, Ed, that specifies an abnormal form of apoprotein (apo) E, a prominent constituent of remnant lipoproteins derived from very low density lipoproteins (VLDL) and chylomicrons. Apo E is thought to mediate the removal of remnant lipoproteins from the plasma by virtue of its ability to bind to hepatic lipoprotein receptors. In F. Dys. patients, remnant-like lipoproteins accumulate, apparently because of delayed clearance by the liver. In the current studies, we show that the abnormal protein specified by the Ed allele (apo E-D) from some, but not all, patients with F. Dys. has a markedly deficient ability to bind to low density lipoprotein (LDL) receptors. Apo E was isolated from eight control subjects and nine patients with F. Dys. and incorporated into phospholipid complexes. The complexes were tested for their ability to compete with human 125I-LDL or rabbit 125I-beta-VLDL fo binding to LDL receptors in four assay systems: cultured human fibroblasts, solubilized receptors from bovine adrenal cortex, liver membranes from rats treated with 17 alpha-ethinyl estradiol, and liver membranes from normal rabbits. The apo E-D from six of the nine patients with F. Dys. showed binding affinities for LDL receptors that were reduced by greater than 98% in all receptor assays (group 1 patients). All of these group 1 patients were unequivocally of phenotype apo E-D/D by the criterion of isoelectric focussing. The apo E from the three other F. Dys. patients showed a near normal binding ability in all four of the receptor assays (group 2 patients). One of these group 2 patients appeared to have the apo E-D/D phenotype by isoelectric focussing. In the other two patients in group 2, apo E-D was the predominant protein (phenotype, apo E-D/D), but traces of protein in the region corresponding to normal apo E (apo E-N) were also present. The difference between group 1 and group 2 patients was also apparent when the apo E was iodinated and tested directly for binding to liver membranes from rats treated with 17 alpha-ethinyl estradiol. The 125I-labeled apo E from a group 2 patient, but not a group 1 patient, showed enhanced uptake when perfused through the liver of an estradiol-treated rate, indicating that the receptor binding ability of apo E correlated with uptake in the intact liver. The current studies allow the subdivision of patients with F. Dys. into two groups. In group 1, the elevated plasma level of remnants appears to be due to a diminished receptor binding activity of the abnormal protein specified by the Ed allele; in group 2 patients, the cause of the elevated plasma level of remnants remains to be explained.
家族性异常β脂蛋白血症(F.Dys.)患者,也称为家族性Ⅲ型高脂蛋白血症患者,是突变等位基因Ed的纯合子,该等位基因编码一种异常形式的载脂蛋白(apo)E,apo E是源自极低密度脂蛋白(VLDL)和乳糜微粒的残余脂蛋白的主要成分。apo E被认为凭借其与肝脂蛋白受体结合的能力介导血浆中残余脂蛋白的清除。在F.Dys.患者中,残余样脂蛋白会积聚,显然是因为肝脏清除延迟。在当前的研究中,我们发现,部分(但并非全部)F.Dys.患者中由Ed等位基因指定的异常蛋白(apo E-D)与低密度脂蛋白(LDL)受体结合的能力明显不足。从8名对照受试者和9名F.Dys.患者中分离出apo E,并将其整合到磷脂复合物中。在四个检测系统中测试这些复合物与人类125I-LDL或兔125I-β-VLDL竞争结合LDL受体的能力:培养的人类成纤维细胞、牛肾上腺皮质的可溶性受体、用17α-乙炔雌二醇处理的大鼠的肝膜以及正常兔的肝膜。9名F.Dys.患者中有6名的apo E-D在所有受体检测中显示与LDL受体的结合亲和力降低了98%以上(第1组患者)。根据等电聚焦标准,所有这些第1组患者明确为apo E-D/D表型。其他3名F.Dys.患者的apo E在所有四种受体检测中均显示出接近正常的结合能力(第2组患者)。通过等电聚焦,这些第2组患者中有1名似乎具有apo E-D/D表型。在第2组的其他两名患者中,apo E-D是主要蛋白(表型,apo E-D/D),但也存在与正常apo E(apo E-N)相对应区域的微量蛋白。当apo E碘化并直接检测其与用17α-乙炔雌二醇处理的大鼠肝膜的结合时,第1组和第2组患者之间的差异也很明显。来自第2组患者而非第1组患者的125I标记的apo E在灌注经过雌二醇处理的大鼠肝脏时显示摄取增强,这表明apo E与完整肝脏中的摄取相关。当前的研究允许将F.Dys.患者细分为两组。在第1组中,残余物血浆水平升高似乎是由于Ed等位基因指定的异常蛋白的受体结合活性降低;在第2组患者中,残余物血浆水平升高的原因仍有待解释。
