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Analysis of intact proteins on a chromatographic time scale by electron transfer dissociation tandem mass spectrometry

机译:电子转移解离串联质谱在色谱时间尺度上分析完整蛋白

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摘要

Direct analysis of intact proteins on a chromatographic time scale is demonstrated on a modified linear ion trap mass spectrometer using sequential ion/ion reactions, electron transfer and proton transfer, to dissociate the sample and to convert the resulting peptide fragments to a mixture of singly and doubly charged species. Proteins are converted to gas-phase, multiply-charged, positive ions by electrospray ionization and then allowed to react with fluoranthene radical anions. Electron transfer to the multiply charged protein promotes random fragmentation of amide bonds along the protein backbone. Multiply charged fragment ions are then deprotonated in a second ion/ion reaction with even-electron benzoate anions. M/z values for the resulting singly and doubly charged ions are used to read a sequence of 15-40 amino acids at both the N-terminus and the C-terminus of the protein. This information, along with the measured mass of the intact protein, are employed to identify known proteins and to detect the presence of post-translational modifications. In this study, we analyze intact proteins from the Escherchia coli 70S ribosomal protein complex and identify 46 of the 55 known unique components in a single, 90 min, on-line, chromatography experiment. Truncated versions of the above proteins along with several post-translational modifications are also detected.
机译:在改良的线性离子阱质谱仪上,使用顺序的离子/离子反应,电子转移和质子转移,以离解样品并将所得的肽片段单独和转化为混合物,证明了在色谱时间尺度上完整蛋白质的直接分析。双电荷物种。通过电喷雾电离将蛋白质转换为气相,多电荷的正离子,然后使其与荧蒽自由基阴离子反应。电子转移到带多重电荷的蛋白质上会促进酰胺键沿蛋白质主链的随机断裂。然后,在第二个离子/离子反应中,带电荷的碎片离子与偶数电子苯甲酸酯阴离子去质子化。所产生的单电荷和双电荷离子的M / z值用于读取蛋白质N端和C端的15-40个氨基酸序列。该信息与完整蛋白质的测定质量一起用于鉴定已知蛋白质并检测翻译后修饰的存在。在这项研究中,我们分析了大肠杆菌70S核糖体蛋白复合物中的完整蛋白,并在一次90分钟的在线色谱实验中鉴定了55种已知独特组分中的46种。还检测到上述蛋白的截短形式以及几种翻译后修饰。

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