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灌注恒河猴肝脏产生的脂蛋白的特性分析

Characterization of lipoprotein produced by the perfused rhesus monkey liver.

作者信息

Jones L A, Teramoto T, Juhn D J, Goldberg R B, Rubenstein A H, Getz G S

出版信息

J Lipid Res. 1984 Apr;25(4):319-35.

PMID:6427376
Abstract

Isolated livers from rhesus monkeys (Macaca mulatta) were perfused in order to asses the nature of newly synthesized hepatic lipoprotein. Perfusate containing [3H]leucine was recirculated for 1.5 hr, followed by an additional 2.5-hr perfusion with fresh perfusate. Equilibrium density gradient ultracentrifugation clearly separated VLDL from LDL. The apoprotein composition of VLDL secreted by the liver was similar to that of serum VLDL. The perfusate LDL contained some poorly radiolabeled, apoB-rich material, which appeared to be contaminating serum LDL. There was also some material of an LDL-like density, which was rich in radiolabeled apoE. Rate zonal density gradient ultracentrifugation fractionated HDL. All perfusate HDL fractions had a decreased cholesteryl ester/unesterified cholesterol ratio, compared to serum HDL. Serum HDL distributed in one symmetric peak near the middle of the gradient, with coincident peaks of apoA-I and apoA-II. The least dense fractions of the perfusate gradient were rich in radiolabeled apoE. The middle of the perfusate gradient contained particles rich in radiolabeled apoA-I and apoA-II. The peak of apoA-I was offset from the apoA-II peak towards the denser end of the gradient. The dense end of the HDL gradient contained lipoprotein-free apoA-I, apoE, and small amounts of apoA-II, probably resulting from the relative instability of nascent lipoprotein compared to serum lipoprotein. Perfusate HDL apoA-I isoforms were more basic than serum apoA-I isoforms. Preliminary experiments, using noncentrifugal methods, suggest that some hepatic apoA-I is secreted in a lipoprotein-free form. In conclusion, the isolated rhesus monkey liver produces VLDL similar to serum VLDL, but produces LDL and HDL which differ in several important aspects from serum LDL and HDL.

摘要

为了评估新合成的肝脏脂蛋白的性质,对恒河猴(猕猴)的离体肝脏进行灌注。含有[3H]亮氨酸的灌注液循环1.5小时,随后用新鲜灌注液再灌注2.5小时。平衡密度梯度超速离心法可清晰地将极低密度脂蛋白(VLDL)与低密度脂蛋白(LDL)分离。肝脏分泌的VLDL的载脂蛋白组成与血清VLDL相似。灌注液中的LDL含有一些放射性标记较差、富含载脂蛋白B的物质,这些物质似乎是污染的血清LDL。也有一些类似LDL密度的物质,富含放射性标记的载脂蛋白E。速率区带密度梯度超速离心法对高密度脂蛋白(HDL)进行分级分离。与血清HDL相比,所有灌注液HDL组分的胆固醇酯/未酯化胆固醇比值均降低。血清HDL分布在梯度中部附近的一个对称峰中,载脂蛋白A-I(apoA-I)和载脂蛋白A-II(apoA-II)的峰重合。灌注液梯度中密度最低的组分富含放射性标记的载脂蛋白E。灌注液梯度的中部含有富含放射性标记的apoA-I和apoA-II的颗粒。apoA-I的峰从apoA-II的峰向梯度的较密端偏移。HDL梯度的较密端含有无脂蛋白的apoA-I、apoE和少量的apoA-II,这可能是由于新生脂蛋白与血清脂蛋白相比相对不稳定所致。灌注液HDL的apoA-I异构体比血清apoA-I异构体碱性更强。使用非离心方法的初步实验表明,一些肝脏apoA-I以无脂蛋白的形式分泌。总之,离体恒河猴肝脏产生的VLDL与血清VLDL相似,但产生的LDL和HDL在几个重要方面与血清LDL和HDL不同。

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