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The goal of this theoretical study of infrared spectra was to ascertain to what degree molecules may be identified from their IR spectra and which spectral regions are best suited for this purpose. The frequencies considered range from the lowest frequency molecular vibrations in the far-IR, terahertz region (below ~3

The goal of this theoretical study of infrared spectra was to ascertain to what degree molecules may be identified from their IR spectra and which spectral regions are best suited for this purpose. The frequencies considered range from the lowest frequency molecular vibrations in the far-IR, terahertz region (below ~3 THz or 100 cm-1) up to the highest frequency vibrations (~120 THz or 4000 cm-1). An emphasis was placed on the IR spectra of chemical and biological threat molecules in the interest of detection and prevention. To calculate IR spectra, the technique of normal mode analysis was applied to organic molecules ranging in size from 8 to 11,352 atoms. The IR intensities of the vibrational modes were calculated in terms of the derivative of the molecular dipole moment with respect to each normal coordinate. Three sets of molecules were studied: the organophosphorus G- and V-type nerve agents and chemically related simulants (15 molecules ranging in size from 11 to 40 atoms); 21 other small molecules ranging in size from 8 to 24 atoms; and 13 proteins ranging in size from 304 to 11,352 atoms. Spectra for the first two sets of molecules were calculated using quantum chemistry software, the last two sets using force fields. The "middle" set used both methods, allowing for comparison between them and with experimental spectra from the NIST/EPA Gas-Phase Infrared Library. The calculated spectra of proteins, for which only force field calculations are practical, reproduced the experimentally observed amide I and II bands, but they were shifted by approximately +40 cm-1 relative to experiment. Considering the entire spectrum of protein vibrations, the most promising frequency range for differentiating between proteins was approximately 600-1300 cm-1 where water has low absorption and the proteins show some differences.
ContributorsMott, Adam J (Author) / Rez, Peter (Thesis advisor) / Ozkan, Banu (Committee member) / Shumway, John (Committee member) / Thorpe, Michael (Committee member) / Vaiana, Sara (Committee member) / Arizona State University (Publisher)
Created2012
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Proteins are the machines of living systems that carry out a diverse set of essential biochemical functions. Furthermore, the diversity of their functions has grown overtime via molecular evolution. This thesis aims to explore fundamental questions in protein science regarding the mechanisms of protein evolution particularly addressing how substitutions in

Proteins are the machines of living systems that carry out a diverse set of essential biochemical functions. Furthermore, the diversity of their functions has grown overtime via molecular evolution. This thesis aims to explore fundamental questions in protein science regarding the mechanisms of protein evolution particularly addressing how substitutions in sequence modulate function through structure and structural dynamics. In the work presented here, the first goal is to develop a set of tools which connect the sequence-structure relationship which are implemented in two major projects of protein structural refinement and protein structural design. Both of these two works highlight the importance of capturing important pairwise interactions within a given protein system.The second major goal of this work is to understand how sequence and structural dynamics give rise to protein function, and, importantly, how Nature can utilize allostery to evolve towards a new function. Here I employ several in-house and novel computational tools to shed light onto the mechanisms of allostery, and, particularly dynamic allostery in the absence of structural rearrangements. This analysis is applied to several different protein systems including Pin1, LacI, CoV-1 and CoV-2 and TEM-1. I show that the dynamics of protein systems may be altered fundamentally by distal perturbations such as ligand binding or point mutations. These peturbations lead to change in local interactions which cascade within the 3-D network of interaction of a protein and give rise to flexibility changes of distal sites, particularly those of functional/active residues positions thereby altering the protein function. This networking picture of the protein is further explored through asymmetric dynamic coupling which shows to be a marker of allosteric interactions between distal residue pairs. Within the networking picture, the concept of sequence context dependence upon mutation becomes critical in understanding the functional outcome of these mutations. Here I design a computational tool, EpiScore, which is able to capture these effects and correlate them to measured experimental epistasis in two protein systems, dihydrofolate reductase (DHFR) and TEM-1. Ultimately, the work provided in this thesis shows that both allostery and epistasis may be considered, and accurately modeled, as intrinsic properties of anisotropic networks.
Contributorscampitelli, paul (Author) / Ozkan, Banu (Thesis advisor) / Ghirlanda, Giovanna (Committee member) / Hariadi, Rizal (Committee member) / Thorpe, Michael (Committee member) / Arizona State University (Publisher)
Created2021