ETD Allows for Native Surface Mapping of a 150 kDa Noncovalent Complex on a Commercial Q-TWIMS-TOF Instrument

被引:75
作者
Lermyte, Frederik [1 ,2 ]
Konijnenberg, Albert [1 ]
Williams, Jonathan P. [3 ]
Brown, Jeffery M. [3 ]
Valkenborg, Dirk [2 ,4 ,5 ]
Sobott, Frank [1 ,2 ]
机构
[1] Univ Antwerp, Dept Chem, Biomol & Analyt Mass Spectrometry Grp, B-2020 Antwerp, Belgium
[2] Univ Antwerp, Ctr Prote CFP CeProMa, B-2020 Antwerp, Belgium
[3] Waters Corp, Manchester, Lancs, England
[4] Vlaamse Instelling Technol Onderzoek, B-2400 Mol, Belgium
[5] Hasselt Univ, Interuniv Inst Biostat & Stat Bioinformat, Diepenbeek, Belgium
基金
比利时弗兰德研究基金会;
关键词
Electron transfer dissociation; Mass spectrometry; Surface mapping; Protein tetramer; Noncovalent complex; Top-down sequencing; ELECTRON-CAPTURE DISSOCIATION; MOBILITY-MASS SPECTROMETRY; CHARGE-STATE; SUPERCHARGING REAGENTS; DOWN CHARACTERIZATION; IONIZATION; ANTIBODIES; PEPTIDE; MODEL;
D O I
10.1007/s13361-013-0798-3
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Top-down approaches for the characterization of intact proteins and macromolecular complexes are becoming increasingly popular, since they potentially simplify and speed up the assignment process. Here we demonstrate how, on a commercially available Q-TWIMS-TOF instrument, we performed top-down ETD of the native form of tetrameric alcohol dehydrogenase. We achieved good sequence coverage throughout the first 81 N-terminal amino acids of ADH, with the exception of a loop located on the inside of the protein. This is in agreement with the exposed parts of the natively folded protein according to the crystal structure. Choosing the right precursor charge state and applying supplemental activation were found to be key to obtaining a high ETD fragmentation efficiency. Finally, we briefly discuss opportunities to further increase the performance of ETD based on our results.
引用
收藏
页码:343 / 350
页数:8
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