Tubulin equilibrium unfolding followed by time-resolved fluorescence and fluorescence correlation spectroscopy

Sánchez, Susana A.; Brunet, Juan E.; Jameson, David M.; Lagos Mónaco, Rosalba; Monasterio Opazo, Octavio

Artículos de revistas

Fecha

2004

Registro en:

Protein Science, Volumen 13, Issue 1, 2018, Pages 81-88

09618368

10.1110/ps.03295604

https://repositorio.uchile.cl/handle/2250/158867

Autor

Sánchez, Susana A.

Brunet, Juan E.

Jameson, David M.

Lagos Mónaco, Rosalba

Monasterio Opazo, Octavio

Institución

Universidad de Chile

Resumen

The pathway for the in vitro equilibrium unfolding of the tubulin heterodimer by guanidinium chloride (GdmCl) has been studied using several spectroscopic techniques, specifically circular dichroism (CD), two-photon Fluorescence Correlation Spectroscopy (FCS), and time-resolved fluorescence, including lifetime and dynamic polarization. The results show that tubulin unfolding is characterized by distinct processes that occur in different GdmCl concentration ranges. From 0 to 0.5 M GdmCl, a slight alteration of the tubulin heterodimer occurs, as evidenced by a small, but reproducible increase in the rotational correlation time of the protein and a sharp decrease in the secondary structure monitored by CD. In the range 0.5-1.5 M GdmCl, significant decreases in the steady-state anisotropy and average lifetime of the intrinsic tryptophan fluorescence occur, as well as a decrease in the rotational correlation time, from 48 to 26 nsec. In the same GdmCl range, the number of protein molecules

Materias

FCS

GdmCl

Time-resolved fluorescence

Tubulin

Unfolding

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