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一种“荧光开关”技术提高了蛋白质组学检测和鉴定 S-亚硝基化蛋白质的灵敏度。

A "fluorescence switch" technique increases the sensitivity of proteomic detection and identification of S-nitrosylated proteins.

机构信息

Servicio de Inmunología, Hospital de La Princesa, Madrid, Spain.

出版信息

Proteomics. 2009 Dec;9(23):5359-70. doi: 10.1002/pmic.200900070.

DOI:10.1002/pmic.200900070
PMID:19798666
Abstract

Protein S-nitrosylation is a reversible post-translational modification of protein cysteines that is increasingly being considered as a signal transduction mechanism. The "biotin switch" technique marked the beginning of the study of the S-nitrosoproteome, based on the specific replacement of the labile S-nitrosylation by a more stable biotinylation that allowed further detection and purification. However, its application for proteomic studies is limited by its relatively low sensitivity. Thus, typical proteomic experiments require high quantities of protein extracts, which precludes the use of this method in a number of biological settings. We have developed a "fluorescence switch" technique that, when coupled to 2-DE proteomic methodologies, allows the detection and identification of S-nitrosylated proteins by using limited amounts of starting material, thus significantly improving the sensitivity. We have applied this methodology to detect proteins that become S-nitrosylated in endothelial cells when exposed to S-nitroso-L-cysteine, a physiological S-nitrosothiol, identifying already known S-nitrosylation targets, as well as proteins that are novel targets. This "fluorescence switch" approach also allowed us to identify several proteins that are denitrosylated by thioredoxin in cytokine-activated RAW264.7 (murine macrophage) cells. We believe that this method represents an improvement in order to approach the identification of S-nitrosylated proteins in physiological conditions.

摘要

蛋白质 S-亚硝基化是一种蛋白质半胱氨酸的可逆翻译后修饰,它越来越被认为是一种信号转导机制。“生物素开关”技术标志着 S-亚硝酰蛋白组学研究的开始,该技术基于不稳定的 S-亚硝酰化的特异性替代,形成更稳定的生物素化,从而允许进一步的检测和纯化。然而,由于其相对较低的灵敏度,其在蛋白质组学研究中的应用受到限制。因此,典型的蛋白质组学实验需要大量的蛋白质提取物,这使得该方法无法在许多生物学环境中使用。我们开发了一种“荧光开关”技术,当与 2-DE 蛋白质组学方法结合使用时,可以通过使用有限数量的起始材料来检测和鉴定 S-亚硝酰化蛋白质,从而显著提高了灵敏度。我们已经应用这种方法来检测内皮细胞在暴露于 S-亚硝基-L-半胱氨酸(一种生理 S-亚硝酰硫醇)时发生 S-亚硝酰化的蛋白质,鉴定已经已知的 S-亚硝酰化靶标,以及新的靶标。这种“荧光开关”方法还使我们能够鉴定出几种在细胞因子激活的 RAW264.7(鼠巨噬细胞)细胞中被硫氧还蛋白还原的蛋白质。我们相信,这种方法是在生理条件下鉴定 S-亚硝酰化蛋白质的一种改进。

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