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细胞和脂蛋白胆固醇含量对成纤维细胞与高密度脂蛋白之间胆固醇通量的影响。

The influence of cellular and lipoprotein cholesterol contents on the flux of cholesterol between fibroblasts and high density lipoprotein.

作者信息

Johnson W J, Mahlberg F H, Chacko G K, Phillips M C, Rothblat G H

机构信息

Department of Physiology and Biochemistry, Medical College of Pennsylvania, Philadelphia 19129.

出版信息

J Biol Chem. 1988 Oct 5;263(28):14099-106.

PMID:2844757
Abstract

Previous studies indicate that free cholesterol moves passively between high density lipoprotein (HDL) and cell plasma membranes by uncatalyzed diffusion of cholesterol molecules in the extracellular aqueous phase. By this mechanism, the rate constants for free cholesterol influx (Cli) and efflux (ke) should not be very sensitive to the free cholesterol content of cells or HDL. Thus, at a given HDL concentration, the unidirectional influx and efflux of cholesterol mass (Fi, Fe) should be proportional to the cholesterol content of HDL and cells, respectively, and net efflux of cholesterol mass (Fe-Fi greater than 0) should occur when either cells are enriched with cholesterol or HDL is depleted of cholesterol. We have examined the influence of cell and HDL free cholesterol contents on the bidirectional flux of free cholesterol between HDL and human fibroblasts and also attempted to detect some dependence of flux on the binding of HDL to the cells. In the range of HDL concentrations from 1 to 1000 micrograms of protein/ml, ke for cell free cholesterol approximately doubled for every 10-fold increase in HDL concentration, reaching 0.04 h-1 at 1000 micrograms of HDL/ml. ke and Cli were not influenced by the doubling of fibroblast free cholesterol content (from 31 +/- 5 to 62 +/- 13 micrograms of cholesterol/mg of protein). There was an approximate exchange of cholesterol between HDL and the unenriched fibroblasts (e.g. at [HDL] = 100 micrograms/ml, Fe and Fi = 3.2 and 3.0 micrograms of cholesterol/[4 h.mg of cell protein], respectively). In contrast, there was substantial net efflux from the enriched cells (at [HDL] = 100 micrograms/ml, Fe and Fi = 5.5 and 3.1 micrograms of cholesterol/[4 h.mg of cell protein], respectively). The rate constants for cholesterol flux were not influenced by changing the free cholesterol content of HDL, so that there was net efflux of cell cholesterol in the presence of cholesterol-depleted HDL and net influx from cholesterol-rich HDL. The Kd of HDL binding to fibroblasts was reduced from 1.7 to 0.9 micrograms/ml by the enrichment of the cells with free cholesterol; this increase in affinity for HDL was not reflected in enhanced rate constants for cholesterol flux. The inhibition of specific HDL binding by treatment of the lipoprotein with dimethyl suberimidate did not affect cholesterol flux using either control or cholesterol-rich cells at any HDL concentration in the range 1-1000 micrograms/ml. The above results are consistent with the concept that net movement of free cholesterol between cells and HDL occurs by passive, mass-action effects.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

先前的研究表明,游离胆固醇通过胆固醇分子在细胞外水相中的无催化扩散,在高密度脂蛋白(HDL)和细胞质膜之间被动移动。通过这种机制,游离胆固醇流入(Cli)和流出(ke)的速率常数对细胞或HDL中的游离胆固醇含量不应非常敏感。因此,在给定的HDL浓度下,胆固醇质量的单向流入和流出(Fi,Fe)应分别与HDL和细胞中的胆固醇含量成正比,当细胞富含胆固醇或HDL中的胆固醇耗尽时,应发生胆固醇质量的净流出(Fe-Fi大于0)。我们研究了细胞和HDL游离胆固醇含量对HDL与人成纤维细胞之间游离胆固醇双向通量的影响,并试图检测通量对HDL与细胞结合的某种依赖性。在HDL浓度从1至1000微克蛋白质/毫升的范围内,HDL浓度每增加10倍,细胞游离胆固醇的ke大约增加一倍,在1000微克HDL/毫升时达到0.04 h-1。ke和Cli不受成纤维细胞游离胆固醇含量加倍(从31±5至62±13微克胆固醇/毫克蛋白质)的影响。在HDL与未富集的成纤维细胞之间存在近似的胆固醇交换(例如,在[HDL]=100微克/毫升时,Fe和Fi分别为3.2和3.0微克胆固醇/[4小时·毫克细胞蛋白质])。相比之下,在富集的细胞中有大量的净流出(在[HDL]=100微克/毫升时,Fe和Fi分别为5.5和3.1微克胆固醇/[4小时·毫克细胞蛋白质])。胆固醇通量的速率常数不受改变HDL游离胆固醇含量的影响,因此在存在胆固醇耗尽的HDL时细胞胆固醇有净流出,而从富含胆固醇的HDL有净流入。通过用辛二酸二甲酯处理脂蛋白来抑制特异性HDL结合,在1至1000微克/毫升范围内的任何HDL浓度下,使用对照细胞或富含胆固醇的细胞时均不影响胆固醇通量。上述结果与游离胆固醇在细胞和HDL之间的净移动是通过被动的质量作用效应发生的这一概念一致。(摘要截短至400字)

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