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利用点击化学优化炔基脂肪酸类似物掺入法检测脂肪酰化蛋白

Optimized Incorporation of Alkynyl Fatty Acid Analogs for the Detection of Fatty Acylated Proteins using Click Chemistry.

作者信息

Liao Lucia M Q, Gray Rachel A V, Martin Dale D O

机构信息

Department of Biology, University of Waterloo.

Department of Biology, University of Waterloo;

出版信息

J Vis Exp. 2021 Apr 9(170). doi: 10.3791/62107.

Abstract

Fatty acylation, the covalent addition of saturated fatty acids to protein substrates, is important in regulating a myriad of cellular functions in addition to its implications in cancer and neurodegenerative diseases. Recent developments in fatty acylation detection methods have enabled efficient and non-hazardous detection of fatty acylated proteins, particularly through the use of click chemistry with bio-orthogonal labeling. However, click chemistry detection can be limited by the poor solubility and potential toxic effects of adding long chain fatty acids to cell culture. Described here is a labeling approach with optimized delivery using saponified fatty acids in combination with fatty-acid free BSA, as well as delipidated media, which can improve detection of hard to detect fatty acylated proteins. This effect was most pronounced with the alkynyl-stearate analog, 17-ODYA, which has been the most commonly used fatty acid analog in click chemistry detection of acylated proteins. This modification will improve cellular incorporation and increase sensitivity to acylated protein detection. In addition, this approach can be applied in a variety of cell types and combined with other assays such as pulse-chase analysis, stable isotope labeling with amino acids in cell culture, and mass spectrometry for quantitative profiling of fatty acylated proteins.

摘要

脂肪酰化是指将饱和脂肪酸共价添加到蛋白质底物上,除了在癌症和神经退行性疾病中的影响外,在调节众多细胞功能方面也很重要。脂肪酰化检测方法的最新进展使得能够高效且无害地检测脂肪酰化蛋白质,特别是通过使用具有生物正交标记的点击化学方法。然而,点击化学检测可能会受到向细胞培养物中添加长链脂肪酸时溶解度差和潜在毒性作用的限制。本文描述了一种标记方法,该方法使用皂化脂肪酸与无脂肪酸的牛血清白蛋白(BSA)以及脱脂培养基进行优化递送,可改善对难以检测的脂肪酰化蛋白质的检测。这种效果在炔基硬脂酸酯类似物17-ODYA中最为明显,它是点击化学检测酰化蛋白质中最常用的脂肪酸类似物。这种修饰将改善细胞摄取并提高对酰化蛋白质检测的灵敏度。此外,这种方法可应用于多种细胞类型,并可与其他检测方法结合使用,如脉冲追踪分析、细胞培养中氨基酸的稳定同位素标记以及用于脂肪酰化蛋白质定量分析的质谱分析。

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