Multifaceted studies into the bioinorganic chemistry of ruthenium(II) arene anticancer complexes
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USyd Access
Type
ThesisThesis type
Doctor of PhilosophyAuthor/s
Stewart, Thomas JefferyAbstract
Ru(II) arene complexes are attractive anticancer drugs but their mechanisms of action and biological targets are not fully known, and new aspects of their modes of action are a focus of this thesis. A Ru(II) arene complex library covering a variety of ligands and diverse antitumour ...
See moreRu(II) arene complexes are attractive anticancer drugs but their mechanisms of action and biological targets are not fully known, and new aspects of their modes of action are a focus of this thesis. A Ru(II) arene complex library covering a variety of ligands and diverse antitumour activities was investigated using spectroscopic techniques, biochemical assays and live cell analyses, to elucidate their mechanisms of action and biological targets. These studies were conducted on two breast cancer cell lines, the aggressive TNBC cell line, MDA-MB-231, and less aggressive epithelial cell line, MCF-7. A large complex-dependent range of antiproliferative activities and cell line sensitivities were observed. In the first study of EV biochemistry changes, the FTIR spectra of the mainly microvesicle and mainly exosome fractions released by these cells following Ru arene complex treatment showed biochemical content varied greatly by proposed drug modes of action. The first research on the Ru anticancer drug interactions with proteoglycans comprised studies on the interactions of the library, and well-studied Ru(III) drugs NAMI-A and KP1019, with the heparan sulfate mimetic fondaparinux, using NSI-MS, UV-Vis reporter assays and heparinase II inhibition assays. The interactions depended on the initial complex charges, as fondaparinux has a large negative charge, and ligand exchange rates. Ligand exchange reactions were studied by XAS on the RAPTA and RAED complexes, which provided strong evidence for ligand-exchange of non-arene ligands with sulfur-donor ligands in both cells and cell medium and with the serum albumin protein. XFM and FTIR microscopy mapping experiments were performed on the two cell lines treated with RAPTA-C and RAED-C. This provided complementary information about intracellular distribution of these drugs and their biochemical impact on cells. RAPTA-C had strongest interactions with the cell surface region, while RAED-C targeted intracellular interactions.
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See moreRu(II) arene complexes are attractive anticancer drugs but their mechanisms of action and biological targets are not fully known, and new aspects of their modes of action are a focus of this thesis. A Ru(II) arene complex library covering a variety of ligands and diverse antitumour activities was investigated using spectroscopic techniques, biochemical assays and live cell analyses, to elucidate their mechanisms of action and biological targets. These studies were conducted on two breast cancer cell lines, the aggressive TNBC cell line, MDA-MB-231, and less aggressive epithelial cell line, MCF-7. A large complex-dependent range of antiproliferative activities and cell line sensitivities were observed. In the first study of EV biochemistry changes, the FTIR spectra of the mainly microvesicle and mainly exosome fractions released by these cells following Ru arene complex treatment showed biochemical content varied greatly by proposed drug modes of action. The first research on the Ru anticancer drug interactions with proteoglycans comprised studies on the interactions of the library, and well-studied Ru(III) drugs NAMI-A and KP1019, with the heparan sulfate mimetic fondaparinux, using NSI-MS, UV-Vis reporter assays and heparinase II inhibition assays. The interactions depended on the initial complex charges, as fondaparinux has a large negative charge, and ligand exchange rates. Ligand exchange reactions were studied by XAS on the RAPTA and RAED complexes, which provided strong evidence for ligand-exchange of non-arene ligands with sulfur-donor ligands in both cells and cell medium and with the serum albumin protein. XFM and FTIR microscopy mapping experiments were performed on the two cell lines treated with RAPTA-C and RAED-C. This provided complementary information about intracellular distribution of these drugs and their biochemical impact on cells. RAPTA-C had strongest interactions with the cell surface region, while RAED-C targeted intracellular interactions.
See less
Date
2024Rights statement
The author retains copyright of this thesis. It may only be used for the purposes of research and study. It must not be used for any other purposes and may not be transmitted or shared with others without prior permission.Faculty/School
Faculty of Science, School of ChemistryAwarding institution
The University of SydneyShare