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铁通过代谢乙醇的大鼠肝细胞介导中性粒细胞趋化因子的产生。

Iron mediates production of a neutrophil chemoattractant by rat hepatocytes metabolizing ethanol.

作者信息

Hultcrantz R, Bissell D M, Roll F J

机构信息

Liver Center Laboratory, San Francisco General Hospital, California 94110.

出版信息

J Clin Invest. 1991 Jan;87(1):45-9. doi: 10.1172/JCI114999.

Abstract

Ethanol metabolism in hepatocytes is accompanied by release of a potent lipid chemoattractant for neutrophils. Production of the factor may initiate the inflammation associated with alcoholic hepatitis. In previous studies with a cytosol system from liver, production was blocked by iron chelators as well as by catalase and superoxide dismutase, suggesting the involvement of oxyradicals in formation of the chemoattractant. These studies have examined the role of iron in intact hepatocytes using cells from rats fed an iron-deficient diet, a control diet or a diet containing 3% carbonyl iron. The iron content averaged 1.4 nmol/mg protein in iron-deficient cells, 6.3 in controls and 135.3 in iron-loaded cells. Hepatocytes from all groups were established in primary culture and incubated with ethanol (10 mM); the medium was assayed for chemoattractant activity for human neutrophils. Cultures from chow-fed or iron-loaded animals produced chemoattractant as previously reported. By contrast, chemoattractant production was undetectable in the iron-deficient cultures. Addition of ferric citrate (10 microM) restored chemoattractant production while increasing cellular iron in the deficient cells less than 50% (to 2.3 nmol/mg protein). Addition of desferrioxamine mesylate to cultures of iron-loaded cells ablated chemoattractant production. The data provide evidence for the importance of hepatocellular iron in production of this alcohol-related lipid chemoattractant and suggest that a small intracellular pool of "free" iron plays a critical role.

摘要

肝细胞中的乙醇代谢伴随着一种对中性粒细胞具有强大脂质趋化作用的物质的释放。该因子的产生可能引发与酒精性肝炎相关的炎症。在先前使用肝脏胞浆系统进行的研究中,铁螯合剂、过氧化氢酶和超氧化物歧化酶均可阻断该物质的产生,这表明氧自由基参与了趋化因子的形成。这些研究使用了喂食缺铁饮食、对照饮食或含3%羰基铁饮食的大鼠的细胞,来研究铁在完整肝细胞中的作用。缺铁细胞中铁含量平均为1.4 nmol/mg蛋白质,对照细胞为6.3,铁负荷细胞为135.3。将所有组的肝细胞进行原代培养,并与乙醇(10 mM)一起孵育;检测培养基对人中性粒细胞的趋化活性。如先前报道,喂食普通饲料或铁负荷动物的培养物产生趋化因子。相比之下,在缺铁培养物中未检测到趋化因子的产生。添加柠檬酸铁(10 microM)可恢复趋化因子的产生,同时使缺铁细胞中的细胞铁增加不到50%(至2.3 nmol/mg蛋白质)。向铁负荷细胞的培养物中添加去铁胺甲磺酸盐可消除趋化因子的产生。这些数据证明了肝细胞铁在这种与酒精相关的脂质趋化因子产生中的重要性,并表明一小部分细胞内“游离”铁起着关键作用。

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