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Monitoring Equilibria and Kinetics of Protein Folding/Unfolding Reactions by Capillary Zone Electrophoresis

✍ Scribed by Barbara Verzola; Fabrizio Chiti; Giampaolo Manao; Pier Giorgio Righetti


Publisher
Elsevier Science
Year
2000
Tongue
English
Weight
92 KB
Volume
282
Category
Article
ISSN
0003-2697

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✦ Synopsis


A method is described here for studying conformational transitions of proteins due to denaturing agents: capillary zone electrophoresis (CZE) in acidic, isoelectric buffers. The sample is run in 50 mM isoelectric glutamic acid (pH ‫؍‬ pI ‫؍‬ 3.2) added with 1 mM oligoamine (tetraethylene pentamine) for quenching protein interaction to the capillary wall (final pH ‫؍‬ 3.3). Muscle acylphosphatase (AcP), in this buffer, exhibited a free solution mobility of 2.63 Ψ‹ 10 ؊4 cm 2 V ؊1 s ؊1 . By studying the unfolding kinetics, as a function of time of incubation in 7 M urea, it was possible to measure the rate constant of the unfolding reaction, estimated to be 0.00030 ؎ 0.00006 s ؊1 . The same measurements, when repeated via spectroscopic monitoring of intrinsic fluorescence, gave a value of 0.00034 ؎ 0.00002 s ؊1 , thus in excellent agreement with CZE data. By equilibrium unfolding CZE studies, it was possible to construct the typical sigmoidal transition of unfolding vs urea molarity: the midpoint of this transition, at which the folded and unfolded states should be equally populated, was estimated to be at 4.56 M urea. Similar experiments by fluorometric analysis gave a value of 4.60 M urea as midpoint of the unfolding curve.


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Folding/unfolding/refolding of proteins:
✍ Pier Giorgio Righetti; Barbara Verzola πŸ“‚ Article πŸ“… 2001 πŸ› John Wiley and Sons 🌐 English βš– 200 KB πŸ‘ 1 views

## Folding/unfolding/refolding of proteins: Present methodologies in comparison with capillary zone electrophoresis A series of techniques for monitoring protein folding/unfolding/misfolding equilibria are here assessed and compared with capillary zone electrophoresis (CZE). They include spectrosc