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Ligand-exchange detection of phosphorylated peptides using liquid chromatography electrospray mass spectrometry

机译:液相色谱电喷雾质谱法检测磷酸化肽的配体交换

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Electrospray ionization mass spectrometry (ESI-MS) is used to selectively detect analytes with a high affinity for metal ions. The detection method is based on the selective monitoring of a competing ligand at its specific m/z value that is released during the ligand-exchange reaction of a metal-ligand complex with analyte(s) eluting from a reversed-phase liquid chromatography column. The ligand-exchange reaction proceeds in a postcolumn reaction detection system placed prior to the inlet of the electrospray MS interface. The feasibility of metal affinity detection by ESI-MS is demonstrated using phosphorylated peptides and iron(III)methylcalcein blue as reactant, as a model system. Methylcalcein blue (MCB) released upon interaction with phosphorylated peptides is detected at m/z 278. The ligand-exchange detection is coupled to a C8 reversed-phase column to separate several nonphosphorylated enkephalins and the phosphorylated peptides pp60 c-src (P) and M2170. Detection limits of 2 muM were obtained for pp60 c-src (P) and M2170. The linearity of the detection method is tested in the range of 2-80 mumol/L phosphorylated compounds (r(2) = 0.9996), and a relative standard deviation of less than 8% (n = 3) for all MCB responses of the different concentrations of phosphorylated compounds was obtained. The presented method showed specificity for phosphorylated peptides and may prove a useful tool for studying other ligand-exchange reactions and metal-protein interactions. [References: 49]
机译:电喷雾电离质谱(ESI-MS)用于选择性地检测对金属离子具有高亲和力的分析物。该检测方法基于选择性监测竞争配体的特定m / z值,该比值在金属-配体络合物与从反相液相色谱柱洗脱的分析物的配体交换反应过程中释放。配体交换反应在放置在电喷雾MS接口入口之前的柱后反应检测系统中进行。使用磷酸化的肽和铁(III)甲基钙黄绿素蓝作为反应物,通过ESI-MS进行金属亲和力检测的可行性作为模型系统得到了证明。在m / z 278处检测到与磷酸化肽相互作用后释放的甲基钙钙蛋白蓝(MCB)。配体交换检测与C8反相色谱柱相连,以分离出几种非磷酸化脑啡肽和磷酸化肽pp60 c-src(P)和M2170。 pp60 c-src(P)和M2170的检测限为2μM。测试方法的线性在2-80μmol/ L磷酸化化合物(r(2)= 0.9996)的范围内进行测试,对于所有MCB响应,相对标准偏差均小于8%(n = 3)。获得了不同浓度的磷酸化化合物。提出的方法显示出对磷酸化肽的特异性,并且可以证明是研究其他配体交换反应和金属-蛋白质相互作用的有用工具。 [参考:49]

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