Detection and analysis of protein-ligand binding sites is an important area of research in drug discovery. The FTMap web server is an established computational method for detection of binding hot spots, or regions on the protein surface that contribute disproportionately to the ligand binding free energy. This body of work primarily focuses on the utilization and advancement of FTMap for the study of protein-ligand interactions and their applications to drug discovery. First, the driving forces behind why some proteins require compounds beyond Lipinski’s rule-of-five (bRo5) guidelines are evaluated for 37 protein targets. Three types of proteins are identified on the basis of their binding hot spots, described by FTMap, and their ligand binding affinity profiles. We describe the multifaceted motivations for bRo5 drug discovery for each group of targets, including increased binding affinity, improved selectivity, decreased toxicity, and decreased off-target effects. Second, the conservation of surface binding properties in protein models is evaluated, with particular emphasis on their utility in drug discovery. Here, the probe-binding locations determined by FTMap are used to generate a binding fingerprint, and the Pearson correlation between the binding fingerprint of an experimental structure and a predicted model indicates the level of surface property conservation, without any knowledge of the protein function a priori. This analysis was performed on the protein models submitted to the Critical Assessment of Techniques for Protein Structure Prediction (CASP) rounds 12 and 14, and results were correlated with well-established structure quality metrics. Third, development of the publicly-available FTMove web server (https://ftmove.bu.edu) is described for detection of binding sites and their respective strengths across multiple different conformations of a protein. FTMove was tested on 22 proteins with known allosteric binding sites, and reliably identified both the orthosteric and allosteric binding sites as highly ranked binding sites. The results yield important insight into the dynamics and druggability of such binding sites. Finally, high throughput affinity purified, mass spectrometry data is evaluated for identification of protein-metabolite interactions (PMIs) in Escherichia coli. A detailed search for known PMIs in both the Protein Data Bank and KEGG database is described, and the resulting curated sets of 21 recovered and 37 potentially novel PMIs in E. Coli are presented. Finally, high confidence novel PMIs were evaluated with the template-based small molecule docking program, LigTBM. / 2023-01-26T00:00:00Z
Identifer | oai:union.ndltd.org:bu.edu/oai:open.bu.edu:2144/43710 |
Date | 26 January 2022 |
Creators | Egbert, Megan E. |
Contributors | Vajda, Sandor |
Source Sets | Boston University |
Language | en_US |
Detected Language | English |
Type | Thesis/Dissertation |
Rights | Attribution 4.0 International, http://creativecommons.org/licenses/by/4.0/ |
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