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受体途径对人类低密度脂蛋白分解代谢的作用。定量分析的新方法。

Contribution of the receptor pathway to low density lipoprotein catabolism in humans. New methods for quantitation.

作者信息

Slater H R, McKinney L, Packard C J, Shepherd J

出版信息

Arteriosclerosis. 1984 Nov-Dec;4(6):604-13. doi: 10.1161/01.atv.4.6.604.

DOI:10.1161/01.atv.4.6.604
PMID:6439178
Abstract

Receptor-mediated catabolism of low density lipoprotein (LDL) by cultured cells depends on the presence of functionally significant arginine and lysine residues on the lipoprotein apoprotein. When these are blocked, the recognition process is abolished, and catabolism of the modified lipoprotein is restricted to other mechanisms. Accurate discrimination between the activities of the receptor and nonreceptor pathways in vivo depends critically on the metabolic properties of this chemically modified lipoprotein. Here we report our experiences with two lysine-modified LDL tracers, glucosylated LDL (GLC-LDL) and 2-hydroxyacetaldehyde-treated LDL (HOET-LDL). The fractional clearance rate of GLC-LDL (0.25 +/- 0.05 pools/day, n = 5) was 50% of that of control material (0.51 +/- 0.09 pools/day) injected simultaneously into normal subjects. The HOET-LDL was also retarded in its clearance. Here, however, the fractional clearances of the control (0.37 +/- 0.06 pools/day, n = 6) and modified lipoprotein (0.19 +/- 0.03 pools/day) were lower than those obtained by the glucosylation procedure. We suspect that the prolonged incubation required for glucosylation of LDL artifactually accelerated its catabolism. The HOET-LDL does not suffer from this defect and seems to be a better tracer of the receptor-independent pathway. In a group of 10 subjects, HOET-LDL was metabolically indistinguishable from 1,2 cyclohexanedione-treated, arginine-modified LDL.

摘要

培养细胞通过受体介导的低密度脂蛋白(LDL)分解代谢取决于脂蛋白载脂蛋白上功能显著的精氨酸和赖氨酸残基的存在。当这些残基被阻断时,识别过程就会被消除,修饰后脂蛋白的分解代谢就会局限于其他机制。在体内准确区分受体途径和非受体途径的活性关键取决于这种化学修饰脂蛋白的代谢特性。在此,我们报告了我们使用两种赖氨酸修饰的LDL示踪剂,即糖基化LDL(GLC-LDL)和2-羟基乙醛处理的LDL(HOET-LDL)的经验。同时注射到正常受试者体内的GLC-LDL的分数清除率(0.25±0.05池/天,n = 5)是对照物质(0.51±0.09池/天)的50%。HOET-LDL的清除也有所延迟。然而,在此对照物(0.37±0.06池/天,n = 6)和修饰脂蛋白(0.19±0.03池/天)的分数清除率低于糖基化过程所获得的清除率。我们怀疑LDL糖基化所需的长时间孵育人为地加速了其分解代谢。HOET-LDL不存在这一缺陷,似乎是受体非依赖途径的更好示踪剂。在一组10名受试者中,HOET-LDL在代谢上与1,2-环己二酮处理的、精氨酸修饰的LDL无法区分。

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Contribution of the receptor pathway to low density lipoprotein catabolism in humans. New methods for quantitation.受体途径对人类低密度脂蛋白分解代谢的作用。定量分析的新方法。
Arteriosclerosis. 1984 Nov-Dec;4(6):604-13. doi: 10.1161/01.atv.4.6.604.
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Comparison of glucosylated low density lipoprotein with methylated or cyclohexanedione-treated low density lipoprotein in the measurement of receptor-independent low density lipoprotein catabolism.在测量非受体依赖型低密度脂蛋白分解代谢中,糖基化低密度脂蛋白与甲基化或环己二酮处理的低密度脂蛋白的比较。
J Clin Invest. 1983 Apr;71(4):960-4. doi: 10.1172/jci110850.
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Receptor-mediated catabolism of low density lipoprotein in man. Quantitation using glucosylated low density lipoprotein.人类中低密度脂蛋白的受体介导分解代谢。使用糖基化低密度脂蛋白进行定量分析。
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Receptor-independent low-density lipoprotein catabolism. Evaluation of 2-hydroxyacetaldehyde-treated lipoprotein as a probe for its measurement.非受体依赖性低密度脂蛋白分解代谢。评估经2-羟基乙醛处理的脂蛋白作为其测量探针的情况。
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Inhibition of receptor-mediated clearance of lysine and arginine-modified lipoproteins from the plasma of rats and monkeys.抑制大鼠和猴血浆中赖氨酸和精氨酸修饰脂蛋白的受体介导清除。
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Receptor-mediated low density lipoprotein catabolism in man.人类中受体介导的低密度脂蛋白分解代谢
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