胆固醇氧化产物进入细胞脂质及其对培养心肌细胞增殖的影响。

Cardioscience Pub Date : 1995-06-01
A Bordoni, S Hrelia, M F Caboni, G Lercker, P L Biagi
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引用次数: 0

摘要

我们研究了胆固醇氧化产物与心肌细胞脂质的结合,并将其与细胞增殖的变化联系起来,通过测量细胞蛋白质含量来评估。在新生大鼠心室细胞的原代培养中补充了几种胆固醇氧化产物(胆甾-5 α, 6 α -环氧-3- β -醇,5 α -胆甾-3 β, 5,6 β -三醇,5-胆甾-3 β, 4 - β -二醇,5-胆甾-3 β -7- 1和5-胆甾-3- 1)的标量浓度。虽然所有的胆固醇氧化产物在浓度高于0.5微米的培养基中加入心肌细胞脂质中,但不同胆固醇氧化产物的加入程度不同,这取决于培养基中的浓度和化合物的化学结构。胆固醇氧化产物对细胞蛋白含量的影响也各不相同:5-胆甾醇-3 β、5,6 -三醇是最有效的细胞增殖抑制剂,其次是胆甾醇-5 α、6 -环氧-3 - β -醇、5-胆甾醇-3 β、4 - β -二醇和5-胆甾醇-3 - β -醇-7- 1。5-胆甾醇-3- 1不影响细胞蛋白含量。胆固醇氧化产物抑制细胞增殖的能力,以及它们增加质膜对钙的渗透性的能力,可能对心脏细胞有害。
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Incorporation of cholesterol oxidation products into cell lipids and their influence on the proliferation of cultured cardiomyocytes.

We have investigated the incorporation of cholesterol oxidation products into cardiomyocyte lipids and related this to changes in cell proliferation, evaluated by measuring cellular protein content. Primary cultures of neonatal rat ventricular cells were supplemented with scalar concentrations of several cholesterol oxidation products (cholestan-5 alpha, 6 alpha-epoxy-3 beta-ol, 5 alpha-cholestane-3 beta, 5, 6 beta-triol, 5-cholesten-3 beta, 4 beta-diol, 5-cholesten-3 beta-ol-7-one, and 5-cholesten-3-one). Although all the cholesterol oxidation products were incorporated into the cardiomyocyte lipids when added to the medium at a concentration higher than 0.5 microM, the extent of the incorporation of the different cholesterol oxidation products differed, depending on the concentration in the culture medium and on the chemical structure of the compound. The effects of the cholesterol oxidation products on the cellular protein content were also different: 5 alpha-cholestane-3 beta, 5, 6 beta-triol was shown to be the most potent inhibitor of cell proliferation, followed by cholestan-5 alpha, 6 alpha-epoxy-3 beta-ol, 5-cholesten-3 beta, 4 beta-diol and 5-cholesten-3 beta-ol-7-one. 5-Cholesten-3-one did not affect the cellular protein content. The ability of cholesterol oxidation products to inhibit cell proliferation, and their capacity to increase the permeability of the plasma membrane to calcium, could be deleterious for cardiac cells.

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