Mapping protein–protein interactions by mass spectrometry

The shielding of lysine groups from acetylation by acetic anhydride has been used to identify the regions of calmodulin in contact with melittin in the 1:1 complex. The estimation of the degree of acetylation was done by examining cyanogen bromide and cyanogen bromide/trypsin digests by mass spectro

Mass spectrometry is capable of examining very large, dynamic proteins and this ability, coupled with its relatively high throughput and low sample requirements, is reflected by its increasing importance for the characterisation of protein structure. Recent developments in mass spectrometry, in part

Microarray technology allows the analysis of a large number of different parameters simultaneously by using a variety of readout systems based on fluorescence, chemiluminescence, electrochemistry, radioactivity, or mass spectrometry (MS). [1] Of these readout systems mass spectrometry is unique, sin

## Abstract The utility of biomolecular interaction analysis–mass spectrometry (BIA/MS) in screening for protein–protein interactions was explored in this work. Experiments were performed in which proteins served as ligands for screening of possible interactions with other proteins from human plasm