ABSTRACT
Methylation/demethylation of cytosines in DNA is central to epigenetics, which plays crucial roles in the regulation of about half of all human genes. Although the methylation mechanism, which downregulates gene expression, has been sufficiently decoded; the demethylation pathway, which upregulates gene expression, still holds questions to be answered. Demethylation of 5-methylcytosine by ten-eleven translocation (TET) enzymes yields understudied but epigenetically relevant intermediates, 5-hydroxymethyl (5-hmC), 5-formyl (5-fC), and 5-carboxyl (5-caC) cytosines. Here we report an iron complex, FeIIITAML (TAML = tetraamido macrocyclic ligand), which can facilitate selective oxidation of 5-hmC to its oxidative derivatives by forming a high-valent Fe-oxo intermediate in the presence of H2O2 under physiologically relevant conditions. Detailed HPLC analyses supported by a wide reaction condition optimization for the 5-hmC â 5-fC oxidation provides us with a chemical model of the TET enzyme. This study shines light on future efforts for a better understanding of the roles of 5-hmC and the TET enzyme mechanism and potentially novel therapeutic methods.
Subject(s)
Cytosine , Models, Chemical , Humans , Hydrogen Peroxide , DNA Methylation , 5-Methylcytosine/analysis , 5-Methylcytosine/metabolism , Oxidation-ReductionABSTRACT
Copper can act as a double-edged sword as it can cause fatal diseases when in excess or shortage. Precise control of copper homeostasis is maintained by a complex machinery inside cells. To overcome imbalances in copper concentration, we have developed a simple system to control the cellular copper concentration by using a photocaged chelator and light. This photocaged chelator allowed us to control cellular copper concentration in a spatiotemporal manner.
Subject(s)
Chelating Agents , Copper , Animals , Homeostasis , MammalsABSTRACT
SARS-CoV-2 main protease (Mpro/3CLpro) is a crucial target for therapeutics, which is responsible for viral polyprotein cleavage and plays a vital role in virus replication and survival. Recent studies suggest that 2-phenylbenzisoselenazol-3(2H)-one (ebselen) is a potent covalent inhibitor of Mpro, which affects its enzymatic activity and virus survival. Herein, we synthesized various ebselen derivatives to understand the mechanism of Mpro inhibition by ebselen. Using ebselen derivatives, we characterized the detailed interaction mechanism with Mpro. We discovered that modification of the parent ebselen inhibitor with an electron-withdrawing group (NO2) increases the inhibition efficacy by 2-fold. We also solved the structure of an Mpro complex with an ebselen derivative showing the mechanism of inhibition by blocking the catalytic Cys145 of Mpro. Using a combination of crystal structures and LC-MS data, we showed that Mpro hydrolyzes the new ebselen derivative and leaves behind selenium (Se) bound with Cys145 of the catalytic dyad of Mpro. We also described the binding profile of ebselen-based inhibitors using molecular modeling predictions supported by binding and inhibition assays. Furthermore, we have also solved the crystal structure of catalytically inactive mutant H41N-Mpro, which represents the inactive state of the protein where the substrate binding pocket is blocked. The inhibited structure of H41N-Mpro shows gatekeeper residues in the substrate binding pocket responsible for blocking the substrate binding; mutation of these gatekeeper residues leads to hyperactive Mpro.