Article
Mechanisms of protein solubilization in reverse micelles
Article first published online: 19 FEB 2004
DOI: 10.1002/bit.260400114
Copyright © 1992 John Wiley & Sons, Inc.
Additional Information
How to Cite
Matzke, S. F., Creagh, A. L., Haynes, C. A., Prausnitz, J. M. and Blanch, H. W. (1992), Mechanisms of protein solubilization in reverse micelles. Biotechnol. Bioeng., 40: 91–102. doi: 10.1002/bit.260400114
Publication History
- Issue published online: 19 FEB 2004
- Article first published online: 19 FEB 2004
- Manuscript Accepted: 7 JAN 1992
- Manuscript Received: 10 JUL 1991
- Abstract
- References
- Cited By
Keywords:
- reverse micelle;
- solubilization;
- light scattering;
- chymotrypsin;
- LADH
Abstract
Solubilization properties of α-chymotrypsin and alcohol dehydrogenase (LADH) in reverse micelles are reported for three different solubilization techniques. The solubilization properties for these two proteins depend on the method used for protein addition. The addition of a dry protein powder to a reverse-micelle-containing organic phase does not appreciably solubilize the protein until the diameter of the reverse micelle is similar to that of the protein. However, when an aqueous protein solution is injected an organic phase, protein solubilization is not strongly dependent on micelle size. For chymotrypsin, multiple protein occupancy occurs at large micelle size, with as many as 11 chymotrypsin molecules solubilized in one reverse micelle. The solubilization of chymotrypsin using a phase-transter technique with a positively charged surfactant follows the expected traned based on protein-surfactant electrostatic interactions. When a negatively charged sufactants is used for phase transfer, at low pH the solubilization data do not fit this electrostatic interaction mechanism. In this case, proteinsurfactant aggregation may be occurring at the aqueousorganic interface.

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