Physical and spectroscopic methods for the evaluation of the interactions of antimitotic agents with tubulin

Physical and spectroscopic methods for the evaluation of the interactions of antimitotic agents with tubulin

The physico-chemical methods for the study of the binding of ligands to tubulin are examined in-depth, emphasizing the assumptions on which they are based and their limitations. The criteria of specificity and linkage to protein self-association are presented. It is shown that, of the direct equilib...

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Veröffentlicht in:Pharmacology & therapeutics (Oxford) 1991-11, Vol.52 (2), p.191-210
Hauptverfasser: Timasheff, Serge N., Andreu, JoséM., Na, George C.
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Antineoplastic agents
Antineoplastic Agents - pharmacology
binding
Biological and medical sciences
colchicine
General aspects
Humans
Kinetics
measurements
Medical sciences
methodology
Pharmacology. Drug treatments
Protein Binding
reviews
tubulin
Tubulin - drug effects
Tubulin - metabolism
Tubulin - physiology
vinblastine
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Zusammenfassung:The physico-chemical methods for the study of the binding of ligands to tubulin are examined in-depth, emphasizing the assumptions on which they are based and their limitations. The criteria of specificity and linkage to protein self-association are presented. It is shown that, of the direct equilibrium binding techniques, Hummel-Dreyer gel permeation chromatography and rapid ultracentrifugation are applicable only when binding is not linked to protein self-association. Disc filtration is valid only when the reverse unbinding reaction is very slow. Binding linked to protein self-association can be measured by batch gel permeation or by dialysis equilibrium. The indirect techniques, such as fluorescence perturbation or difference absorption spectroscopy are discussed in terms of the assumptions on which they are based. They are shown to be used best only after characterization of the binding by direct techniques. Equilibrium binding parameters can also be deduced from careful kinetic experiments. Comparison of calorimetrically measured enthalpies of binding to van't Hoff enthalpies derived from equilibrium measurements indicates that the method of choice is calorimetric, while comparison with van't Hoff analysis can reveal the existence of reaction steps not detected by equilibrium measurements. Use of other indirect approaches, such as titration of an enzymic activity, can also lead to the detection of additional steps. The criteria are set up for the proper data analysis of ligand binding linked to protein self-association and the selection of the proper mode of linkage. It is shown how the thermodynamic contributions of various moieties of a Ligand can be established by a rational structural modification of the ligand and the proper analysis of the binding measurements, in which all non-specific entropic contributions are taken into account. It is demonstrated also how a similar analysis of binding data can lead to conclusions about the reaction pathway from a comparison of equilibrium thermodynamic measurements on judiciously modified ligand molecules.
ISSN:0163-7258
1879-016X
DOI:10.1016/0163-7258(91)90008-A