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高密度脂蛋白亚组分的组成与代谢

The composition and metabolism of high density lipoprotein subfractions.

作者信息

Schaefer E J, Foster D M, Jenkins L L, Lindgren F T, Berman M, Levy R I, Brewer H B

出版信息

Lipids. 1979 May;14(5):511-22. doi: 10.1007/BF02533471.

Abstract

The composition and metabolism of high density lipoprotein (HDL) subfractions were investigated in seven normal individuals. Mean HDL2 (d, 1.063-1.125 g/ml) composition (by weight) was 43% protein, 28% phospholipid, 23% cholesterol, and 6% triglyceride, and mean HDL3 (d, 1.125-1.21 g/ml) composition was 58% protein, 22% phospholipid, 14% cholesterol, and 5% triglyceride. The mean apoA-I; apoA-II weight ratio was 4.75 for HDL2 and 3.65 for HDL3. HDL2 protein was proportionally slightly richer in C apolipoproteins and higher molecular weight constituents (including apoE) than HDL3. Kinetic studies utilized radiolabeled HDLA (d, 1.09-1.21 g/ml), HDL2, and HDL3 demonstrated rapid exchange of apoA-I and apoA-II radioactivity among HDL subfractions, similar fractional rates of catabolism of apoA-I and apo A-II within HDL, and similar radioactivity decay within HDL subfractions. Mean plasma residence time was 5.74 days for radiolabeled HDL2 and 5.70 days for radiolabedled HDL3. Differences in HDL protein mass among individuals were largely due to alterations in catabolism, and in general both HDL2 and HDL3 were catabolized via a plasma and a nonplasma pathway. Data from simultaneous radiolabeled very low density lipoprotein and HDL studies in 2 individuals are consistent with the concept that apoC-II and apoC-III are catabolized at a different rate than are apo A-I and apo A-II within the HDL density range.

摘要

对7名正常个体的高密度脂蛋白(HDL)亚组分的组成和代谢进行了研究。平均HDL2(密度为1.063 - 1.125 g/ml)的组成(按重量计)为43%蛋白质、28%磷脂、23%胆固醇和6%甘油三酯,平均HDL3(密度为1.125 - 1.21 g/ml)的组成是58%蛋白质、22%磷脂、14%胆固醇和5%甘油三酯。HDL2的平均载脂蛋白A-I;载脂蛋白A-II重量比为4.75,HDL3为3.65。HDL2蛋白在C载脂蛋白和较高分子量成分(包括载脂蛋白E)方面比HDL3略丰富。动力学研究使用放射性标记的HDLA(密度为1.09 - 1.21 g/ml)、HDL2和HDL3,结果表明载脂蛋白A-I和载脂蛋白A-II的放射性在HDL亚组分之间快速交换,HDL内载脂蛋白A-I和载脂蛋白A-II的分解代谢分数率相似,且HDL亚组分内的放射性衰变相似。放射性标记的HDL2的平均血浆停留时间为5.74天,放射性标记的HDL3为5.70天。个体之间HDL蛋白质量的差异主要归因于分解代谢的改变,一般来说,HDL2和HDL3都是通过血浆和非血浆途径进行分解代谢的。在2名个体中同时进行的放射性标记极低密度脂蛋白和HDL研究的数据与以下概念一致:在HDL密度范围内,载脂蛋白C-II和载脂蛋白C-III的分解代谢速率与载脂蛋白A-I和载脂蛋白A-II不同。

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