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脂蛋白(a)进入培养的成纤维细胞的过程独立于质膜低密度脂蛋白受体。

Lp(a) lipoprotein enters cultured fibroblasts independently of the plasma membrane low density lipoprotein receptor.

作者信息

Maartmann-Moe K, Berg K

出版信息

Clin Genet. 1981 Nov;20(5):352-62. doi: 10.1111/j.1399-0004.1981.tb01047.x.

DOI:10.1111/j.1399-0004.1981.tb01047.x
PMID:6277537
Abstract

Lp(a) lipoprotein shares the apoB antigen with low density lipoprotein (LDL). The Lp(a) antigen is unique for Lp(a) lipoprotein. Fibroblast association (i.e. plasma membrane binding plus intracellular accumulation), plasma membrane binding, intracellular accumulation and degradation of 125I-Lp(a) lipoprotein were studied in strains from subjects with or without autosomal dominant hypercholesterolemia (HC). Subjects without HC (non-HCs) have cell surface receptors for low density lipoprotein (LDL receptors). On the average, HC heterozygotes have half-normal LDL receptor activity and "receptor-negative" HC homozygous cell strains lack functional receptors. Fibroblast processing of 125I-Lp(a) lipoprotein was compared to fibroblast processing of 125I-LDL. LDL receptor-dependent processing of 125I-LDL was saturated at about 50 microgram apo 125I-LDL.ml-1 in non-HC fibroblasts. 125I-Lp(a) lipoprotein was, however, largely processed independently of receptor mechanisms by non-HC cells (highest concentration examined 150 microgram apo 125I-Lp(a) lipoprotein . ml-1). Lp(a) lipoprotein did not interfere with 125I-LDL for fibroblast association, but inhibited 125I-LDL degradation. The interference with 125I-LDL degradation was time dependent. Only slightly higher 125I-Lp(a) lipoprotein processing values were found in non-HC and HC heterozygous strains than in "receptor-negative" HC homozygous strains. However, non-HC cells had more than tenfold higher 125I-LDL processing values than "receptor-negative" HC homozygous cells.

摘要

脂蛋白(a)[Lp(a)]与低密度脂蛋白(LDL)共享载脂蛋白B抗原。Lp(a)抗原是Lp(a)脂蛋白所特有的。研究了来自有或无常染色体显性高胆固醇血症(HC)受试者的细胞株中125I-Lp(a)脂蛋白的成纤维细胞结合(即质膜结合加细胞内积聚)、质膜结合、细胞内积聚及降解情况。无HC的受试者(非HC者)具有低密度脂蛋白细胞表面受体(LDL受体)。平均而言,HC杂合子的LDL受体活性为正常的一半,而“受体阴性”的HC纯合细胞株缺乏功能性受体。将125I-Lp(a)脂蛋白的成纤维细胞处理过程与125I-LDL的成纤维细胞处理过程进行了比较。在非HC成纤维细胞中,125I-LDL的LDL受体依赖性处理在约50微克载脂蛋白125I-LDL·ml-1时达到饱和。然而,非HC细胞对125I-Lp(a)脂蛋白的处理很大程度上独立于受体机制(检测的最高浓度为150微克载脂蛋白125I-Lp(a)脂蛋白·ml-1)。Lp(a)脂蛋白不干扰125I-LDL与成纤维细胞的结合,但抑制125I-LDL的降解。对125I-LDL降解的干扰具有时间依赖性。在非HC和HC杂合细胞株中发现的125I-Lp(a)脂蛋白处理值仅比“受体阴性”的HC纯合细胞株略高。然而,非HC细胞的125I-LDL处理值比“受体阴性”的HC纯合细胞高十多倍。

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