Your search keyword '"Steven D. Bull"' showing total 8 results

1. Fluorescent probe for the imaging of superoxide and peroxynitrite during drug-induced liver injury†

Author

Steven D. Bull, Robin R. Groleau, Luling Wu, Jihong Liu, Xue Tian, Tony D. James, Bo Tang, and Ping Li

Subjects

chemistry.chemical_classification, Liver injury, Reactive oxygen species, Fluorophore, Superoxide, General Chemistry, medicine.disease, Fluorescence, chemistry.chemical_compound, Chemistry, chemistry, medicine, Biophysics, Molecular probe, Reactive nitrogen species, Peroxynitrite

Abstract

Drug-induced liver injury (DILI) is an important cause of potentially fatal liver disease. Herein, we report the development of a molecular probe (LW-OTf) for the detection and imaging of two biomarkers involved in DILI. Initially, primary reactive oxygen species (ROS) superoxide (O2˙−) selectively activates a near-infrared fluorescence (NIRF) output by generating fluorophore LW-OH. The C Created by potrace 1.16, written by Peter Selinger 2001-2019 C linker of this hemicyanine fluorophore is subsequently oxidized by reactive nitrogen species (RNS) peroxynitrite (ONOO−), resulting in cleavage to release xanthene derivative LW-XTD, detected using two-photon excitation fluorescence (TPEF). An alternative fluorescence pathway can occur through cleavage of LW-OTf by ONOO− to non-fluorescent LW-XTD-OTf, which can react further with the second analyte O2˙− to produce the same LW-XTD fluorescent species. By combining NIRF and TPEF, LW-OTf is capable of differential and simultaneous detection of ROS and RNS in DILI using two optically orthogonal channels. Probe LW-OTf could be used to detect O2˙− or O2˙− and ONOO− in lysosomes stimulated by 2-methoxyestradiol (2-ME) or 2-ME and SIN-1 respectively. In addition, we were able to monitor the chemoprotective effects of tert-butylhydroxyanisole (BHA) against acetaminophen (APAP) toxicity in living HL-7702 cells. More importantly, TPEF and NIRF imaging confirmed an increase in levels of both O2˙− and ONOO− in mouse livers during APAP-induced DILI (confirmed by hematoxylin and eosin (H&E) staining)., Drug-induced liver injury (DILI) is an important cause of potentially fatal liver disease.

Published

2021

2. Pinkment: a synthetic platform for the development of fluorescent probes for diagnostic and theranostic applications†

Author

Maria Weber, Amanda B. Mackenzie, Tony D. James, Jia Li, Maria L. Odyniec, Xiao-Peng He, Yi Zang, Bo Han Li, Charlotte E.F. Jarman, Adam C. Sedgwick, Hai Hao Han, and Steven D. Bull

Subjects

Chemistry, Bioconjugation, Biological species, Nanotechnology, General Chemistry, Fluorescence, Biomarker (cell)

Abstract

Reaction-based fluorescent-probes have proven successful for the visualisation of biological species in various cellular processes. Unfortunately, in order to tailor the design of a fluorescent probe to a specific application (i.e. organelle targeting, material and theranostic applications) often requires extensive synthetic efforts and the synthetic screening of a range of fluorophores to match the required synthetic needs. In this work, we have identified Pinkment-OH as a unique “plug-and-play” synthetic platform that can be used to develop a range of ONOO− responsive fluorescent probes for a variety of applications. These include theranostic-based applications and potential material-based/bioconjugation applications. The as prepared probes displayed an excellent sensitivity and selectivity for ONOO− over other ROS. In vitro studies using HeLa cells and RAW 264.7 macrophages demonstrated their ability to detect exogenously and endogenously produced ONOO−. Evaluation in an LPS-induced inflammation mouse model illustrated the ability to monitor ONOO− production in acute inflammation. Lastly, theranostic-based probes enabled the simultaneous evaluation of indomethacin-based therapeutic effects combined with the visualisation of an inflammation biomarker in RAW 264.7 cells., Pinkment, a resorufin based ONOO− selective and sensitive ‘plug and play’ fluorescence-based platform for in vitro and in vivo use, enables facile functionalisation for various imaging and theranostic applications.

Published

2020

3. An 'OFF-ON-OFF' fluorescence protein-labeling probe for real-time visualization of the degradation of short-lived proteins in cellular systems

Author

Shahi Imam Reja, Yuichiro Hori, Takuya Kamikawa, Kohei Yamasaki, Miyako Nishiura, Steven D. Bull, and Kazuya Kikuchi

Subjects

General Chemistry

Abstract

The ability to monitor proteolytic pathways that remove unwanted and damaged proteins from cells is essential for understanding the multiple processes used to maintain cellular homeostasis. In this study, we have developed a new protein-labeling probe that employs an 'OFF-ON-OFF' fluorescence switch to enable real-time imaging of the expression (fluorescence ON) and degradation (fluorescence OFF) of PYP-tagged protein constructs in living cells. Fluorescence switching is modulated by intramolecular contact quenching interactions in the unbound probe (fluorescence OFF) being disrupted upon binding to the PYP-tag protein, which turns fluorescence ON. Quenching is then restored when the PYP-tag-probe complex undergoes proteolytic degradation, which results in fluorescence being turned OFF. Optimization of probe structures and PYP-tag mutants has enabled this fast reacting 'OFF-ON-OFF' probe to be used to fluorescently image the expression and degradation of short-lived proteins.

Published

2021

4. A fluorescent ESIPT-based benzimidazole platform for the ratiometric two-photon imaging of ONOO−in vitro and ex vivo

Author

Emily C. Webb, Juyoung Yoon, Hwan Myung Kim, Steven D. Bull, Adam C. Sedgwick, Sang Jun Park, Jordan E. Gardiner, Tony D. James, and Maria L. Odyniec

Subjects

inorganic chemicals, chemistry.chemical_compound, Benzimidazole, Fluorophore, Imaging Tool, Two-photon excitation microscopy, chemistry, cardiovascular system, Biophysics, General Chemistry, Fluorescence, Ex vivo, In vitro

Abstract

In this work, we have developed an ESIPT-based benzimidazole platform (MO-E1 and MO-E2) for the two-photon cell imaging of ONOO- and a potential ONOO--activated theranostic scaffold (MO-E3). Each benzimidazole platform, MO-E1-3, were shown to rapidly detect ONOO- at micromolar concentrations (LoD = 0.28 μM, 6.53 μM and 0.81 μM respectively). The potential theranostic MO-E3 was shown to release the parent fluorophore and drug indomethacin in the presence of ONOO- but unfortunately did not perform well in vitro due to low solubility. Despite this, the parent scaffold MO-E2 demonstrated its effectiveness as a two-photon imaging tool for the ratiometric detection of endogenous ONOO- in RAW264.7 macrophages and rat hippocampus tissue. These results demonstrate the utility of this ESIPT benzimidazole-based platform for theranostic development and bioimaging applications.

Published

2020

5. Fluorogenic probes for detecting deacylase and demethylase activity towards post-translationally-modified lysine residues

Author

Steven D. Bull, Kazuya Kikuchi, Miyako Nishiura, Reisuke Baba, Yuichiro Hori, and Tomomi Tao

Subjects

chemistry.chemical_classification, 0303 health sciences, Enzyme catalyzed, Lysine, Peptide, General Chemistry, 010402 general chemistry, 01 natural sciences, Fluorescence, 0104 chemical sciences, Turn (biochemistry), 03 medical and health sciences, Chemistry, Enzyme, chemistry, Biochemistry, Demethylase activity, 030304 developmental biology

Abstract

Reversible enzymatic post-translational modification of the ε-amino groups of lysine residues (e.g. N-acylation reactions) plays an important role in regulating the cellular activities of numerous proteins. This study describes how enzyme catalyzed N-deprotection of lysine residues of non-fluorescent peptide-coumarin probes can be used to generate N-deprotected peptides that undergo spontaneous O- to N-ester transfer reactions (uncatalyzed) to generate a highly fluorescent N-carbamoyl peptide. This enables detection of enzyme catalyzed N-deacetylation, N-demalonylation, N-desuccinylation and N-demethylation reactions activities towards the N-modified lysine residues of these probes using simple ‘turn on’ fluorescent assays., We developed “turn-on” fluorescent probes that detect enzymatic lysine deacylation and demethylation critical for epigenetic and other cellular phenomena, using intramolecular O- to N-ester transfer reactions.

Published

2021

6. Protein encapsulation: a new approach for improving the capability of small-molecule fluorogenic probes

Author

Tony D. James, He Tian, Hai Hao Han, Na Li, Xiao Peng He, James T. Brewster, Maria Weber, Yi Zang, Steven D. Bull, Maria L. Odyniec, Jonathan L. Sessler, Adam C. Sedgwick, Jia Li, Ying Shang, Bo Han Li, Tingting Liu, and Kunqian Yu

Subjects

biology, Chemistry, Cell, General Chemistry, biology.organism_classification, Human serum albumin, Fluorescence, Small molecule, In vitro, HeLa, medicine.anatomical_structure, In vivo, Biophysics, medicine, Preclinical imaging, medicine.drug

Abstract

Herein, we report a protein-based hybridization strategy that exploits the host-guest chemistry of HSA (human serum albumin) to solubilize the otherwise cell impermeable ONOO− fluorescent probe Pinkment-OAc. Formation of a HSA/Pinkment-OAc supramolecular hybrid was confirmed by SAXS and solution-state analyses. This HSA/Pinkment-OAc hybrid provided an enhanced fluorescence response towards ONOO−versusPinkment-OAc alone, as determined by in vitro experiments. The HSA/Pinkment-OAc hybrid was also evaluated in RAW 264.7 macrophages and HeLa cancer cell lines, which displayed an enhanced cell permeability enabling the detection of SIN-1 and LPS generated ONOO− and the in vivo imaging of acute inflammation in LPS-treated mice. A remarkable 5.6 fold (RAW 264.7), 8.7-fold (HeLa) and 2.7-fold increased response was seen relative to Pinkment-OAc alone at the cellular level and in vivo, respectively. We anticipate that HSA/fluorescent probe hybrids will soon become ubiquitous and routinely applied to overcome solubility issues associated with hydrophobic fluorescent imaging agents designed to detect disease related biomarkers., Herein, we report a protein-based hybridization strategy that exploits the host–guest chemistry of HSA (human serum albumin) to solubilize the otherwise cell impermeable ONOO− fluorescent probe Pinkment-OAc.

Published

2021

7. The development of a novel AND logic based fluorescence probe for the detection of peroxynitrite and GSH

Author

Xiao-Peng He, Hai Hao Han, Jordan E. Gardiner, Steven D. Bull, Adam C. Sedgwick, and Tony D. James

Subjects

inorganic chemicals, Analyte, 010405 organic chemistry, Cellular imaging, General Chemistry, Glutathione, 010402 general chemistry, 01 natural sciences, Fluorescence, 0104 chemical sciences, chemistry.chemical_compound, chemistry, cardiovascular system, Biophysics, Fluorescein, Selectivity, Fluorescence response, Peroxynitrite

Abstract

We have developed a novel AND logic based fluorescence probe for the simultaneous detection of ONOO− and GSH (GSH-PF3). The GSH-PF3 probe was synthesised over three steps starting from commercially available fluorescein. The probe was constructed by attaching the GSH reactive motif, 2,4-dinitrobenzenesulfonyl, to the previously reported boronate fluorescence based probe, PF3. GSH-PF3 produced only a small fluorescence response towards the addition of GSH or ONOO− separately. However, when the probe was exposed to both analytes, there was a significant (40-fold) fluorescence enhancement. GSH-PF3 demonstrated an excellent selectivity towards both GSH and ONOO−. In cellular imaging experiments the probe was shown to be cell permeable with no ‘turn-on’ response observed for the addition of either GSH or ONOO− separately. However, in the presence of both analytes, a clear fluorescence response was observed in live cells. GSH-PF3 was further able to monitor the co-existence of metabolically produced ONOO− and GSH by exogenous stimulation.

Published

2018

8. Reaction-based Indicator displacement Assay (RIA) for the selective colorimetric and fluorometric detection of peroxynitrite

Author

John S. Fossey, Eric V. Anslyn, Tony D. James, Stephen E. Flower, Elena C. Ramsamy, Steven D. Bull, Xiaolong Sun, Karel Lacina, and Xuhong Qian

Subjects

inorganic chemicals, ALIZARIN RED, Viologen, General Chemistry, Photochemistry, Chemical reaction, Combinatorial chemistry, Nitric oxide, Chemistry, chemistry.chemical_compound, chemistry, medicine, sense organs, Phenylboronic acid, Hydrogen peroxide, Boronic acid, Peroxynitrite, medicine.drug

Abstract

Using the self-assembly of aromatic boronic acids with Alizarin Red S (ARS), we developed a new chemosensor for the selective detection of peroxynitrite., Using the self-assembly of aromatic boronic acids with Alizarin Red S (ARS), we developed a new chemosensor for the selective detection of peroxynitrite. Phenylboronic acid (PBA), benzoboroxole (BBA) and 2-(N,N-dimethylaminomethyl)phenylboronic acid (NBA) were employed to bind with ARS to form the complex probes. In particular, the ARS–NBA system with a high binding affinity can preferably react with peroxynitrite over hydrogen peroxide and other ROS/RNS due to the protection of the boron via the solvent-insertion B–N interaction. Our simple system produces a visible colorimetric change and on–off fluorescence response towards peroxynitrite. By coupling a chemical reaction that leads to an indicator displacement, we have developed a new sensing strategy, referred to herein as RIA (Reaction-based Indicator displacement Assay).

Published

2015