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分离的正常和转化肝细胞中脂肪酸过氧化与α-生育酚消耗之间的关系。

The relationship between fatty acid peroxidation and alpha-tocopherol consumption in isolated normal and transformed hepatocytes.

作者信息

Cogrel P, Morel I, Lescoat G, Chevanne M, Brissot P, Cillard P, Cillard J

机构信息

Laboratory of Cellular Biology and Botany, Faculty of Pharmacy, Rennes, France.

出版信息

Lipids. 1993 Feb;28(2):115-9. doi: 10.1007/BF02535774.

Abstract

The response of normal and transformed rat hepatocytes to oxidative stress was investigated. Isolated normal rat hepatocytes and differentiated hepatoma cells (the Fao cell line was derived from the Reuber H 35 rat hepatoma) in suspension were incubated with the ADP/Fe3+ chelate for 30 min at 37 degrees C. Membrane lipid oxidation was assessed by measuring (i) free malondialdehyde (MDA) production by a high-performance liquid chromatography (HPLC) procedure, (ii) membrane fatty acid disappearance as judged by capillary gas chromatography, and (iii) alpha-tocopherol oxidation as determined by HPLC and electrochemical detection. The addition of iron led to increased MDA production in normal as well as in transformed cells, and to simultaneous consumption of polyunsaturated fatty acids (PUFA) and alpha-tocopherol. In addition, in Fao cells more alpha-tocopherol was consumed during lipid peroxidation while less PUFA was oxidized. Lipid peroxidation was lower in tumoral hepatocytes than in normal cells. This could be due to a difference in membrane lipid composition because of a lower PUFA content and a higher alpha-tocopherol level in Fao cells. During oxidation, Fao cells produced 1.5 to 2 times less MDA than normal cells, while in the tumoral cells the amount of oxidized PUFA having 3 or more double bonds was 7 to 8 times lower. Therefore, measuring MDA alone as an index of lipid peroxidation did not allow for proper comparison of the membrane lipid oxidizability of transformed cells vs. the membrane lipid oxidizability of normal cells.

摘要

研究了正常和转化的大鼠肝细胞对氧化应激的反应。将分离的正常大鼠肝细胞和悬浮培养的分化肝癌细胞(Fao细胞系源自Reuber H 35大鼠肝癌)与ADP/Fe3+螯合物在37℃下孵育30分钟。通过以下方法评估膜脂质氧化:(i)采用高效液相色谱(HPLC)法测定游离丙二醛(MDA)的生成量;(ii)通过毛细管气相色谱法判断膜脂肪酸的消失情况;(iii)采用HPLC和电化学检测法测定α-生育酚的氧化情况。铁的添加导致正常细胞和转化细胞中MDA生成量增加,同时多不饱和脂肪酸(PUFA)和α-生育酚被消耗。此外,在Fao细胞中,脂质过氧化过程中消耗的α-生育酚更多,而被氧化的PUFA更少。肿瘤肝细胞中的脂质过氧化水平低于正常细胞。这可能是由于膜脂质组成的差异,因为Fao细胞中PUFA含量较低,α-生育酚水平较高。在氧化过程中,Fao细胞产生的MDA比正常细胞少1.5至2倍,而在肿瘤细胞中,具有3个或更多双键的氧化PUFA的量低7至8倍。因此,仅将MDA作为脂质过氧化的指标,无法对转化细胞与正常细胞的膜脂质氧化能力进行恰当比较。

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