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Chemical dephosphorylation for identification of multiply phosphorylated peptides and phosphorylation site determination

机译:化学去磷酸化用于鉴定多种磷酸化肽和磷酸化位点

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We have developed a novel strategy to improve the efficiency of identification of multiply phosphorylated peptides isolated by hydroxy acid modified metal oxide chromatography (HAMMOC). This strategy consists of alkali-induced chemical dephosphorylation (beta-elimination reaction) of phosphopeptides isolated by HAMMOC prior to analysis by liquid chromatography/mass spectrometry (LC/MS). This approach identified 1.9-fold more multiply phosphorylated peptides than the conventional approach without beta-elimination from a digested mixture of three standard phosphoproteins. In addition, the accuracy of phosphorylation site determination in synthetic phosphopeptides was significantly improved. Finally, we applied this approach to a cell lysate. By combining this dephosphorylation approach with the conventional approach, we successfully identified 1649 unique phosphopeptides, including 325 multiply phosphorylated phosphopeptides, from 200mg of cultured Arabidopsis cells. These results indicate that chemical dephosphorylation prior to LC/MS analysis increases the efficiency of identification of multiply phosphorylated peptides, as well as the accuracy of phosphorylation site determination.
机译:我们已经开发出一种新的策略,以提高通过羟基酸修饰的金属氧化物色谱(HAMMOC)分离的多重磷酸化肽的鉴定效率。该策略包括在通过液相色谱/质谱(LC / MS)分析之前,通过HAMMOC分离的磷酸肽的碱诱导的化学去磷酸化(β消除反应)。这种方法比没有从三种标准磷蛋白的消化混合物中进行β消除的常规方法鉴定的多磷酸化肽多1.9倍。另外,合成磷酸肽中磷酸化位点测定的准确性显着提高。最后,我们将这种方法应用于细胞裂解液。通过将此脱磷酸方法与常规方法相结合,我们成功地从200mg培养的拟南芥细胞中鉴定出1649种独特的磷酸肽,包括325种多重磷酸化的磷酸肽。这些结果表明,在LC / MS分析之前进行化学去磷酸化可提高鉴定多种磷酸化肽段的效率以及磷酸化位点确定的准确性。

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