首页> 外文期刊>Analytical chemistry >Mesoporous TiO_(2)-Based Experimental Layout for On-Target Enrichment and Separation of Multi- and Monophosphorylated Peptides Prior to Analysis with Matrix-Assisted Laser Desorption-Ionization Mass Spectrometry
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Mesoporous TiO_(2)-Based Experimental Layout for On-Target Enrichment and Separation of Multi- and Monophosphorylated Peptides Prior to Analysis with Matrix-Assisted Laser Desorption-Ionization Mass Spectrometry

机译:基于中孔TiO_(2)的实验布局,用于目标富集和分离多和单磷酸化肽,然后进行基质辅助激光解吸电离质谱分析

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摘要

A simple method for on-target enrichment and subsequent separation and analysis of phosphorylated peptides is presented. The tryptic digest of a phosphorylated protein, in this case beta-casein, is loaded onto a spot on a thin stripe made of mesoporous TiO_(2) sintered onto a conductive glass surface. After washing with a salicylic buffer in order to remove the nonphosphorylated peptides, the stripe is placed in an elution chamber containing a phosphate solution. In a way analogous to thin layer chromatography (TLC), the phosphate solution acts as an eluent, clearly separating multi- and monophosphorylated peptides. By performing matrix-assisted laser desorption-ionization mass spectrometry (MALDI-MS) along the stripe, the detection of all phosphorylated peptides present in the digest is facilitated, as they are isolated from each other. The method was also tested on commercial drinking milk, achieving successful separation between multi- and monophosphorylated peptides, as well as a detection limit in the femtomole range. As the enrichment, separation, and analysis take place in the same substrate, sample handling and risk of contamination and sample loss is minimized. The results obtained suggest that the method, once optimized, may successfully provide a complete phosphoproteome.
机译:提出了一种简单的方法,可进行靶标富集,然后分离和分析磷酸化的肽。磷酸化蛋白的胰蛋白酶消化物(在这种情况下为β-酪蛋白)被加载到由细孔的TiO_(2)制成的细条上的斑点上,该细条被烧结到导电玻璃表面上。用水杨酸缓冲液洗涤以除去未磷酸化的肽后,将条带置于含有磷酸盐溶液的洗脱室中。以类似于薄层色谱法(TLC)的方式,磷酸盐溶液充当洗脱液,清楚地分离出多磷酸化和单磷酸化的肽。通过沿着条带执行基质辅助激光解吸电离质谱(MALDI-MS),可以方便地检测消化液中存在的所有磷酸化肽,因为它们彼此分离。该方法还在商用牛奶中进行了测试,成功实现了多磷酸化肽段和单磷酸化肽段之间的成功分离,以及飞摩尔范围内的检出限。由于富集,分离和分析都在同一底物中进行,因此样品处理以及污染和样品损失的风险得以最小化。获得的结果表明,该方法一旦优化,就可以成功提供完整的磷酸化蛋白质组。

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