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Quantification of peptides for the monitoring of protease-catalyzed reactions by matrix-assisted laser desorption/ionization mass spectrometry using ionic liquid matrixes

机译:使用离子液体基质通过基质辅助激光解吸/电离质谱法对肽进行定量,以监测蛋白酶催化的反应

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摘要

Ionic liquid matrixes (ILM) have been shown to allow very homogeneous sample preparations, facilitating relative quantifications using internal standards in matrix-assisted laser desorption/ionization mass spectrometry (MALDI-MS). In the present work, the ability to perform quantifications of peptides without using internal standards in these matrixes was investigated. linear correlations between peptide amount and signal intensities could be observed when increased molar mabix-to-analyte ratios were applied. The dynamic range of linearity was similar to 1 order of magnitude. The method was applied successfully to monitor the time-dependent evolution of substrates and products in trypsin-catalyzed digests of single peptides and peptide mixtures. Thus, ionic liquid matrixes allow quantitative MALDI-MS without the need for internal standards, making the method a suitable tool for the fast screening of new enzymes or the search for substrates or inhibitors.
机译:离子液体基质(ILM)可以进行非常均匀的样品制备,从而在基质辅助激光解吸/电离质谱(MALDI-MS)中使用内标促进了相对定量。在本工作中,研究了无需在这些基质中使用内标物即可进行肽定量的能力。当应用增加的摩尔马比克斯与被分析物之比时,可以观察到肽量与信号强度之间的线性相关性。线性度的动态范围类似于1个数量级。该方法已成功应用于监测胰蛋白酶催化的单肽和肽混合物消化物中底物和产物的时间依赖性演化。因此,离子液体基质无需内部标准液即可进行定量MALDI-MS分析,使该方法成为快速筛选新酶或寻找底物或抑制剂的合适工具。

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