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艾氏腹水瘤细胞对脂质过氧化促进剂组氨酸亚铁的摄取。

Uptake of ferrous iron histidinate, a promoter of lipid peroxidation, by Ehrlich ascites tumor cells.

作者信息

Sharaf El Din M, Schaur R J, Schauenstein E

机构信息

Institute of Biochemistry, University of Graz, Austria.

出版信息

Biochim Biophys Acta. 1988 Sep 2;962(1):37-41. doi: 10.1016/0005-2760(88)90092-6.

Abstract

The kinetics of the uptake of Fe(II)-histidinate, a known promoter of lipid peroxidation, into Ehrlich ascites tumor (EAT) cells and the intracellular binding of iron were studied in vitro. EAT cells (27.10(6)/ml) were incubated in Hanks' balanced salts solution at 37 degrees C for various time intervals in the presence of FeSO4 (1 mM) and L-histidine (10 mM). Total iron was determined by the 1,10-phenanthroline/ascorbate method and ferric iron by reaction with 5-sulfosalicylic acid; the difference was ascribed to ferrous iron. Total iron decreased rapidly in the medium (242 nmol within the first 10 min), and a corresponding increase of total iron (saturation value 376 nmol after 60 min) was determined within the cells, after the cellular proteins had been solubilized with 6 M urea. In the absence of EAT cells, Fe(II)-histidinate was readily oxidized to Fe(III)-histidinate by oxygen, but this reaction was strongly retarded by the tumor cells. The uptake of iron histidinate occurred in the oxidized state, while an uptake of ferrous iron could not be proven unambiguously. When EAT cells were saturated with iron, it was found that 93% of intracellular iron was bound to water-insoluble proteins and 7% was associated with soluble proteins, while no unbound iron was detectable by the method used. It was concluded that, despite the high uptake of total iron, only a very small portion of the intracellular iron was available as a redox catalyst for lipid peroxidation.

摘要

研究了脂质过氧化的已知促进剂——组氨酸亚铁进入艾氏腹水瘤(EAT)细胞的动力学以及铁在细胞内的结合情况。将EAT细胞(27×10⁶个/ml)在含有硫酸亚铁(1 mM)和L - 组氨酸(10 mM)的汉克斯平衡盐溶液中于37℃孵育不同时间间隔。用邻菲罗啉/抗坏血酸法测定总铁,用与5 - 磺基水杨酸反应的方法测定三价铁;两者之差归为二价铁。培养基中的总铁迅速下降(最初10分钟内下降242 nmol),在用6 M尿素溶解细胞蛋白后,测定细胞内总铁相应增加(60分钟后饱和值为376 nmol)。在没有EAT细胞的情况下,组氨酸亚铁很容易被氧气氧化为组氨酸铁,但肿瘤细胞强烈抑制了该反应。组氨酸铁的摄取以氧化态发生,而二价铁的摄取无法明确证实。当EAT细胞铁饱和时,发现细胞内93%的铁与水不溶性蛋白结合,7%与可溶性蛋白结合,而用所用方法未检测到未结合的铁。得出的结论是,尽管总铁摄取量高,但细胞内只有非常小的一部分铁可作为脂质过氧化的氧化还原催化剂。

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