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细胞蛋白质的脂肪酸酰化特异性

Specificity of fatty acid acylation of cellular proteins.

作者信息

Olson E N, Towler D A, Glaser L

出版信息

J Biol Chem. 1985 Mar 25;260(6):3784-90.

PMID:3972848
Abstract

Labeling of the BC3H1 muscle cell line with [3H] palmitate and [3H]myristate results in the incorporation of these fatty acids into a broad spectrum of different proteins. The patterns of proteins which are labeled with palmitate and myristate are distinct, indicating a high degree of specificity of fatty acylation with respect to acyl chain length. The protein-linked [3H]palmitate is released by treatment with neutral hydroxylamine or by alkaline methanolysis consistent with a thioester linkage or a very reactive ester linkage. In contrast, only a small fraction of the [3H]myristate which is attached to proteins is released by treatment with hydroxylamine or alkaline methanolysis, suggesting that myristate is linked to proteins primarily through amide bonds. The specificity of fatty acid acylation has also been examined in 3T3 mouse fibroblasts and in PC12 cells, a rat pheochromacytoma cell line. In both cells, palmitate is primarily linked to proteins by a hydroxylamine-labile linkage while the major fraction of the myristic acid (60-70%) is linked to protein via amide linkage and the remainder via an ester linkage. Major differences were noted in the rate of fatty acid metabolism in these cells; in particular in 3T3 cells only 33% of the radioactivity incorporated from myristic acid into proteins is in the form of fatty acids. The remainder is presumably the result of conversion of label to amino acids. In BC3H1 cells, palmitate- and myristate-containing proteins also exhibit differences in subcellular localization. [3H]Palmitate-labeled proteins are found almost exclusively in membranes, whereas [3H]myristate-labeled proteins are distributed in both the soluble and membrane fractions. These results demonstrate that fatty acid acylation is a covalent modification common to a wide range of cellular proteins and is not restricted solely to membrane-associated proteins. The major acylated proteins in the various cell lines examined appear to be different, suggesting that the acylated proteins are concerned with specialized cell functions. The linkages through which fatty acids are attached to proteins also appear to be highly specific with respect to the fatty acid chain length.

摘要

用[3H]棕榈酸酯和[3H]肉豆蔻酸酯标记BC3H1肌肉细胞系,会使这些脂肪酸掺入到广泛的不同蛋白质中。用棕榈酸酯和肉豆蔻酸酯标记的蛋白质模式各不相同,这表明就酰基链长度而言,脂肪酸酰化具有高度特异性。与硫酯键或非常活泼的酯键一致,通过用中性羟胺处理或碱性甲醇解可释放与蛋白质相连的[3H]棕榈酸酯。相比之下,用羟胺或碱性甲醇解处理后,只有一小部分与蛋白质结合的[3H]肉豆蔻酸酯被释放,这表明肉豆蔻酸主要通过酰胺键与蛋白质相连。在3T3小鼠成纤维细胞和PC12细胞(一种大鼠嗜铬细胞瘤细胞系)中也研究了脂肪酸酰化的特异性。在这两种细胞中,棕榈酸主要通过对羟胺不稳定的键与蛋白质相连,而大部分肉豆蔻酸(60 - 70%)通过酰胺键与蛋白质相连,其余部分通过酯键相连。在这些细胞中脂肪酸代谢速率存在显著差异;特别是在3T3细胞中,从肉豆蔻酸掺入到蛋白质中的放射性只有33%是以脂肪酸的形式存在。其余部分可能是标记物转化为氨基酸的结果。在BC3H1细胞中,含棕榈酸和肉豆蔻酸的蛋白质在亚细胞定位上也存在差异。[3H]棕榈酸酯标记的蛋白质几乎只存在于膜中,而[3H]肉豆蔻酸酯标记的蛋白质分布在可溶性部分和膜部分。这些结果表明,脂肪酸酰化是广泛的细胞蛋白质共有的一种共价修饰,并不局限于与膜相关的蛋白质。在所检测的各种细胞系中,主要的酰化蛋白质似乎不同,这表明酰化蛋白质与特定的细胞功能有关。就脂肪酸链长度而言,脂肪酸与蛋白质相连的键也似乎具有高度特异性。

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