Selective Enrichment and Direct Analysis of Protein S-Palmitoylation Sites

棕榈酰化 脂锚定蛋白 酰化 生物化学 脂肪酸 化学 半胱氨酸 硫酯 生物 自噬 催化作用 细胞凋亡
作者
Emmanuelle Thinon,Joseph Fernandez,Henrik Molina,Howard C. Hang
出处
期刊:Journal of Proteome Research [American Chemical Society]
卷期号:17 (5): 1907-1922 被引量:44
标识
DOI:10.1021/acs.jproteome.8b00002
摘要

S-Fatty-acylation is the covalent attachment of long chain fatty acids, predominately palmitate (C16:0, S-palmitoylation), to cysteine (Cys) residues via a thioester linkage on proteins. This post-translational and reversible lipid modification regulates protein function and localization in eukaryotes and is important in mammalian physiology and human diseases. While chemical labeling methods have improved the detection and enrichment of S-fatty-acylated proteins, mapping sites of modification and characterizing the endogenously attached fatty acids are still challenging. Here, we describe the integration and optimization of fatty acid chemical reporter labeling with hydroxylamine-mediated enrichment of S-fatty-acylated proteins and direct tagging of modified Cys residues to selectively map lipid modification sites. This afforded improved enrichment and direct identification of many protein S-fatty-acylation sites compared to previously described methods. Notably, we directly identified the S-fatty-acylation sites of IFITM3, an important interferon-stimulated inhibitor of virus entry, and we further demonstrated that the highly conserved Cys residues are primarily modified by palmitic acid. The methods described here should facilitate the direct analysis of protein S-fatty-acylation sites and their endogenously attached fatty acids in diverse cell types and activation states important for mammalian physiology and diseases.
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