Expansion of time window for mass spectrometric measurement of amide hydrogen/deuterium exchange reactions

被引:64
作者
Coales, Stephen J. [1 ]
E, Sook Yen [1 ]
Lee, Jessica E. [1 ]
Ma, Anita [1 ]
Morrow, Jeffrey A. [2 ]
Hamuro, Yoshitomo [1 ]
机构
[1] ExSAR Corp, Monmouth Jct, NJ 08852 USA
[2] Sierra Analyt Inc, Modesto, CA 95356 USA
关键词
ELECTRON-CAPTURE DISSOCIATION; HYDROGEN-EXCHANGE; PROTEIN-STRUCTURE; DEUTERIUM EXCHANGE; DYNAMICS; DETERMINANTS; RESOLUTION; KINETICS; NMR;
D O I
10.1002/rcm.4814
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Backbone amide hydrogen exchange rates can be used to describe the dynamic properties of a protein. Amide hydrogen exchange rates in a native protein may vary from milliseconds (ms) to several years. Ideally, the rates of all amide hydrogens of the analyte protein can be determined individually. To achieve this goal, monitoring of a wider time window is critical, in addition to high sequence coverage and high sequence resolution. Significant improvements have been made to hydrogen/deuterium exchange mass spectrometry methods in the past decade for better sequence coverage and higher sequence resolution. On the other hand, little effort has been made to expand the experimental time window to accurately determine exchange rates of amide hydrogens. Many fast exchanging amide hydrogens are completely exchanged before completion of a typical short exchange time point (10-30 s) and many slow exchanging amide hydrogens do not start exchanging before a typical long exchanging time point (1-3 h). Here various experimental conditions, as well as a quenched-flow apparatus, are utilized to monitor cytochrome c amide hydrogen exchange behaviors over more than eight orders of magnitude (0.0044-1 000 000 s), when converted into the standard exchange condition (pH 7 and 23 degrees C). Copyright (c) 2010 John Wiley & Sons, Ltd.
引用
收藏
页码:3585 / 3592
页数:8
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