Rotational Dynamics of Calcium-Free Calmodulin Studied by 15N-NMR Relaxation Measurements
- 1 June 1995
- journal article
- Published by Wiley in European Journal of Biochemistry
- Vol. 230 (3) , 1014-1024
- https://doi.org/10.1111/j.1432-1033.1995.tb20650.x
Abstract
The backbone motions of calcium-free Xenopus calmodulin have been characterized by measurements of the 15N longitudinal relaxation times (T1) at 51 and 61 MHz, and by conducting transverse relaxation (T2), spin-locked transverse relaxation (T1 rho), and 15N-[1H] heteronuclear NOE measurements at 61 MHz 15N frequency. Although backbone amide hydrogen exchange experiments indicate that the N-terminal domain is more stable than calmodulin's C-terminal half, slowly exchanging backbone amide protons are found in all eight alpha-helices and in three of the four short beta-strands. This confirms that the calcium-free form consists of stable secondary structure and does not adopt a 'molten globule' type of structure. However, the C-terminal domain of calmodulin is subject to conformational exchange on a time scale of about 350 microseconds, which affects many of the C-terminal domain residues. This results in significant shortening of the 15N T2 values relative to T1 rho, whereas the T1 rho and T2 values are of similar magnitude in the N-terminal half of the protein. A model in which the motion of the protein is assumed to be isotropic suggests a rotational correlation time for the protein of about 8 ns but quantitatively does not agree with the magnetic field dependence of the T1 values and does not explain the different T2 values found for different alpha-helices in the N-terminal domain. These latter parameters are compatible with a flexible dumb-bell model in which each of calmodulin's two domains freely diffuse in a cone with a semi-angle of about 30 degrees and a time constant of about 3 ns, whereas the overall rotation of the protein occurs on a much slower time scale of about 12 ns. The difference in the transverse relaxation rates observed between the amides in helices C and D suggests that the change in interhelical angle upon calcium binding is less than predicted by Herzberg et al. Strynadka and James [Strynadka, N. C. J. & James, M. N. G. (1988) Proteins Struct. Funct. Genet. 3, 1-17].Keywords
This publication has 51 references indexed in Scilit:
- Backbone Dynamics of a Highly Disordered 131 Residue Fragment of Staphylococcal NucleaseJournal of Molecular Biology, 1994
- Investigation of the backbone dynamics of the igg‐binding domain of streptococcal protein g by heteronuclear two‐dimensional 1H‐15N nuclear magnetic resonance spectroscopyProtein Science, 1994
- Effects of ion binding on the backbone dynamics of calbindin D9k determined by nitrogen-15 NMR relaxationBiochemistry, 1993
- Primary structure effects on peptide group hydrogen exchangeProteins-Structure Function and Bioinformatics, 1993
- Optimized recording of heteronuclear multidimensional NMR spectra using pulsed field gradientsJournal of Magnetic Resonance (1969), 1992
- Backbone dynamics of calmodulin studied by nitrogen-15 relaxation using inverse detected two-dimensional NMR spectroscopy: the central helix is flexibleBiochemistry, 1992
- Deviations from the simple two-parameter model-free approach to the interpretation of nitrogen-15 nuclear magnetic relaxation of proteinsJournal of the American Chemical Society, 1990
- Structure of calmodulin refined at 2.2 Å resolutionJournal of Molecular Biology, 1988
- Three-dimensional structure of calmodulinNature, 1985
- Comparative studies on thermostability of calmodulin, skeletal muscle troponin C and their tryptic fragmentsFEBS Letters, 1983