Structural dynamics studies of human calcium binding protein S100A12 and T4 lysozyme

The work presented here was conceived with two main objectives. The first one, more general, involved the implementation of a new methodology for the study of conformational changes in proteins, i.e., its structural dynamics. The technique of Site-directed Spin Labeling combined with Electronic Paramagnetic Resonance (SDSL-EPR) are the pillars of this new method, which is now part of the set of techniques available at the Grupo de Biofísica Molecular Sérgio Mascarenhas, Instituto de Física de São Carlos (USP). The second objective, more specific, represented the path actually taken to achieve the overall goal. Therefore, it was proposed to study the structure-function correlation in two interesting biological systems. The first involved the study of the movement of the helices that form the structure of the human calcium binding protein S100A12 (HS100A12) induced by calcium and zinc ions. Knowing that, besides Ca+2, human S100A12 has also affinity for other divalent metals, such as Zn+2 and Cu+2 ions, and that the formation of different protein oligomers is governed by the concentration of Ca+2 and Zn+2, we performed spectroscopic studies using circular dichroism (CD) to investigate the thermal stability of protein HS100A12 in the presence and absence of calcium and zinc. Conformational changes in the structure of HS100A12 were monitored by producing a series of mutants (singles and doubles) in which residues in helices B, C and D were replaced by cysteine and subsequently labeled with a magnetic probe MTSSL and then analyzed via SDSL-EPR. The latter consisted of the EPR spectra measurement of many mutants at room temperature to study the effects of the presence of ions on the dynamics experienced by the probe in different positions. In addition, we performed measurements of the distance between two probes inserted in the protein structure, thereby, seeking to improve the understanding of the effect of the ions presence on the protein. Finally, due to the fact that HS100A12 is involved in some events of cell signaling and interaction with the Receptor for Advanced Glycation End Products (RAGE), we also decided to study the interaction of protein with models of biomembranes using Langmuir monolayers. In the other problem of interest, we used a variety of mutants of the enzyme T4 lysozyme, a protein standard, in order to obtain more details about its structure-function correlation and make more solid the understanding of SDSL technique. Initially, we conducted a study about the alleged creation of a cavity in the hydrophobic C-terminal portion of the enzyme, when we replaced the Leu 133 by Ala and/or Gly, or when we changed a large residue for a smaller one, because it is believed that the protein undergoes a structural adjustment in order to fill the gap created by this substitution. For this, we studied by SDSL the α-helix H motion, inserting the spin label in a neighbor position of the mutated residue. Additionally, we performed an experiment of \"transmutation\" with the enzyme T4L in order to investigate the nature of contributions for different dynamic modes experienced by the spin label when it is introduced in topologically similar sites. (AU)