Electron capture dissociation distinguishes a single D-amino acid in a protein and probes the tertiary structure

被引:89
作者
Adams, CM
Kjeldsen, F
Zubarev, RA
Budnik, BA
Haselmann, KF
机构
[1] Uppsala Univ, Uppsala Biomed Ctr, Lab Biol & Med Mass Spectrometry, S-75123 Uppsala, Sweden
[2] Univ So Denmark, Dept Chem, Odense, Denmark
关键词
D O I
10.1016/j.jasms.2004.04.026
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
First results are reported on the application of ECD in analysis of 2+ and 3+ ions of stereoisomers of Trp-cage (NLYIQWLKDGGPSSGRPPPS), the smallest and fastest-folding protein, which exhibits a tightly folded tertiary structure in solution. The chiral recognition based on the ratios of the abundances of z(18) and z(19) fragments in ECD of 2+ ions was excellent even for a single amino acid (Tyr) D-substitution (R-chiral = 8.6). The chiral effect decreased with an increase of temperature at the electrospray ion source, as well as at a higher degree of ionization, 3+ ions (R-chiral = 1.5). A general approach is suggested for charge localization in n+ ions by analysis of ECD mass spectra of (n + 1)+ ions. Application of this approach to 3+ Trp-cage ions revealed the protonation probability order in 2+ ions: Arg(16) much greater than Gln(5) >approximate to N-terminus. The ECD results for native form of the 2+ ions favor the preservation of the solution-phase tertiary structure, and chiral recognition through the interaction between the charges and the neutral bond network. Conversely, ECD of 3+ ions supports the dominance of ionic hydrogen bending which determines a different gas-phase structure than found in solution. Vibrational activation of 2+ ions indicated greater stability of the native form, but the fragmentation patterns did not provide stereoisomer differentiation, thus underlying the special position of ECD among other MS/MS fragmentation techniques. Further ECD studies should yield more structural information as well as quantitative single-amino acid D/L content measurements in proteins. (C) 2004 American Society for Mass Spectrometry.
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页码:1087 / 1098
页数:12
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