CE detection of N‐(3‐dimethylaminopropyl)‐N‐carbodiimide/N‐hydroxysuccinimide‐coupled proteins after homo‐ and hetero‐crosslinking reactions

Protein–protein conjugates formed by carbodiimide crosslinking reactions have been analyzed for the first time using CE. Lysozyme and BSA were chosen as model proteins to study the efficacy of N‐(3‐dimethylaminopropyl)‐N‐ethylcarbodiimide and N‐hydroxysuccinimide as crosslinkers. Detection of the molecular mass increase was checked by SDS‐PAGE. Commercially available, PVA‐coated capillaries showed appropriate selection, while phospho‐deactivated and dynamic PVA‐coated capillaries did not give suitable resolution. CE was found to be an efficient tool to characterize homo‐ (lysozyme–lysozyme) and hetero‐ (lysozyme–BSA) protein coupling by suitable variations of electrophoretic mobilities.