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乙醇对灌注大鼠肝脏细胞内蛋白质降解的抑制作用。

Inhibition of intracellular protein degradation by ethanol in perfused rat liver.

作者信息

Pösö A R, Surmacz C A, Mortimore G E

出版信息

Biochem J. 1987 Mar 1;242(2):459-64. doi: 10.1042/bj2420459.

Abstract

Ethanol (50 mM) inhibited proteolysis in the perfused rat liver during stringent amino acid deprivation and also in the presence of normal and 10 times normal concentrations of plasma amino acids. The concentration-response curve of ethanol reached a plateau after 5 mM in both the presence and the absence of normal plasma amino acids, suggesting inhibition by oxidation products of ethanol. Intracellular glutamine, tyrosine and proline increased in concentration with ethanol, but the increases were too small to explain the observed inhibition of proteolysis. The uptake of 125I-asialofetuin was slightly decreased and the output of ammonia increased in the presence of ethanol. These, together with a significant suppression of basal proteolysis in the presence of amino acids, suggest that lysosomal function was directly affected. Electron-microscopic examination of lysosomal components showed that the aggregate volume of autophagosomes (initial vacuoles) were significantly smaller in livers perfused with ethanol than in controls. However, the equivalent volume of autolysosomes (degradative vacuoles) was the same in both groups. According to these results, ethanol inhibits protein degradation in the liver by two discrete mechanisms: one decreasing the formation of autophagic vacuoles and the other involving lysosomotropic inhibition, possibly via ammonia.

摘要

在严格的氨基酸缺乏期间以及存在正常浓度和正常浓度10倍的血浆氨基酸时,乙醇(50 mM)抑制灌注大鼠肝脏中的蛋白水解。无论有无正常血浆氨基酸,乙醇的浓度-反应曲线在5 mM后均达到平台期,提示乙醇的氧化产物起抑制作用。细胞内谷氨酰胺、酪氨酸和脯氨酸的浓度随乙醇升高,但升高幅度太小,无法解释观察到的蛋白水解抑制现象。在乙醇存在下,125I-去唾液酸胎球蛋白的摄取略有下降,氨的输出增加。这些结果,连同在氨基酸存在下基础蛋白水解的显著抑制,提示溶酶体功能受到直接影响。对溶酶体成分的电子显微镜检查显示,用乙醇灌注的肝脏中自噬体(初始液泡)的总体积明显小于对照组。然而,两组中自溶酶体(降解液泡)的等效体积相同。根据这些结果,乙醇通过两种不同机制抑制肝脏中的蛋白质降解:一种是减少自噬液泡的形成,另一种可能是通过氨的溶酶体亲和性抑制。

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Effects of alcohol on hepatic transport of proteins.
Annu Rev Med. 1982;33:281-92. doi: 10.1146/annurev.me.33.020182.001433.

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