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内皮型一氧化氮合酶中氨基末端共价结合肉豆蔻酸的鉴定。

Identification of covalently bound amino-terminal myristic acid in endothelial nitric oxide synthase.

作者信息

Liu J, Sessa W C

机构信息

Molecular Cardiobiology Program, Boyer Center for Molecular Medicine, Yale University School of Medicine, New Haven, Connecticut 06536-0812.

出版信息

J Biol Chem. 1994 Apr 22;269(16):11691-4.

PMID:7512951
Abstract

Endothelial nitric oxide synthase (eNOS) is unique among the nitric oxide synthase family of proteins due to the presence of an N-myristoylation consensus sequence elucidated from the cloning of its cDNA. Although eNOS was metabolically labeled with [3H]myristic acid and mutation of glycine 2 in the N-myristoylation consensus sequence changed the particulate localization of the enzyme to a cytosolic form, the definitive characterization of eNOS as an N-myristoylprotein has not been demonstrated. Therefore, the purpose of the present study was to determine the nature of the fatty acid incorporated into eNOS. Wild-type or G2A mutant (mutation of glycine 2, the myristic acid acceptor site, to alanine) eNOS-transfected COS cells and bovine aortic endothelial cells (BAEC) were metabolically labeled with [3H]myristic acid for 5 h. The radiolabel was primarily incorporated into membrane-associated eNOS from wild-type transfected COS cells and cultured BAEC but not into the mutant eNOS from G2A-transfected COS cells. Qualitatively similar amounts of immunoreactive protein were found in wild-type and G2A-transfected cells. In addition, linkage of the radiolabel to eNOS was insensitive to hydroxylamine treatment, and incorporation of the radiolabel into eNOS was abolished by cyclo-heximide. Chemical analysis of the fatty acid released by acid methanolysis of labeled eNOS verified the 3H-labeled fatty acid as protein-bound myristic acid. These results unequivocally demonstrate that eNOS incorporates myristic acid via an amide linkage with the amino-terminal glycine of the enzyme as a co-translational modification.

摘要

内皮型一氧化氮合酶(eNOS)在一氧化氮合酶蛋白家族中独具特色,这是因为其cDNA克隆揭示了一个N-肉豆蔻酰化共有序列。尽管eNOS能用[3H]肉豆蔻酸进行代谢标记,且N-肉豆蔻酰化共有序列中甘氨酸2的突变会使该酶的颗粒定位转变为胞质形式,但eNOS作为N-肉豆蔻酰化蛋白的确切特征尚未得到证实。因此,本研究的目的是确定掺入eNOS的脂肪酸的性质。用[3H]肉豆蔻酸对野生型或G2A突变体(肉豆蔻酸接受位点的甘氨酸2突变为丙氨酸)eNOS转染的COS细胞和牛主动脉内皮细胞(BAEC)进行5小时的代谢标记。放射性标记主要掺入野生型转染COS细胞和培养的BAEC的膜相关eNOS中,而未掺入G2A转染COS细胞的突变型eNOS中。在野生型和G2A转染细胞中发现了定性相似量的免疫反应性蛋白。此外,放射性标记与eNOS的连接对羟胺处理不敏感,放线菌酮可消除放射性标记掺入eNOS。对标记的eNOS进行酸甲醇解释放的脂肪酸的化学分析证实,3H标记的脂肪酸为与蛋白质结合的肉豆蔻酸。这些结果明确表明,eNOS通过与该酶氨基末端甘氨酸的酰胺键掺入肉豆蔻酸,作为一种共翻译修饰。

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