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Dive into the research topics where Heather J. Montgomery is active.

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Featured researches published by Heather J. Montgomery.


Bioorganic & Medicinal Chemistry | 2002

Photo-control of nitric oxide synthase activity using a caged isoform specific inhibitor.

Heather J. Montgomery; Basil Perdicakis; Dan Fishlock; Gilles A. Lajoie; Eric Jervis; J. Guy Guillemette

Nitric oxide (NO) plays a critical role in a number of physiological processes and is produced in mammalian cells by nitric oxide synthase (NOS) isozymes. Because of the diverse functions of NO, pharmaceutical interventions which seek to abrogate adverse effects of excess NOS activity must not interfere with the normal regulation of NO levels in the body. A method has been developed for the control of NOS enzyme activity using the localized photochemical release of a caged isoform-specific NOS inhibitor. The caged form of an iNOS inhibitor has been synthesized and tested for photosensitivity and potency. UV and multiphoton uncaging were verified using a hemoglobin-based assay. IC(50) values were determined for the inhibitor (70+/-11 nM), the caged inhibitor (1098+/-172 nM), the UV uncaged inhibitor (67+/-26 nM) and the multiphoton uncaged inhibitor (73+/-11 nM). UV irradiation of the caged inhibitor resulted in a 86% reduction in iNOS activity after 5 min. Multiphoton uncaging had an apparent first order time constant of 0.007+/-0.001 min(-1). A therapeutic range exists, with molar excess of inhibitor to enzyme from 3- to 7-fold, over which the full dynamic range of the inhibition can be exploited.


Bioorganic & Medicinal Chemistry | 2003

Synthesis and evaluation of trans 3,4-cyclopropyl l-arginine analogues as isoform selective inhibitors of nitric oxide synthase

Dan Fishlock; Basil Perdicakis; Heather J. Montgomery; J. Guy Guillemette; Eric Jervis; Gilles A. Lajoie

Four optically pure conformationally restricted L-arginine analogues syn- 1 and anti- 2 trans-3,4-cyclopropyl L-arginine, and syn- 3 and anti-trans-3,4-cyclopropyl N-(1-iminoethyl) L-ornithine 4 were synthesized. These compounds were tested as potential inhibitors against the three isoforms of nitric oxide synthase (NOS). Compound 1 was determined to be a poor substrate of NOS, while compound 2 was determined to be a poor mixed type inhibitor and did not exhibit any isoform selectivity. Syn- 3 and anti-trans-3,4-cyclopropyl N-(1-iminoethyl) L-ornithine 4 were found to be competitive inhibitors of NOS. These compounds were time dependent inhibitors of inducible NOS (iNOS), but not of neuronal NOS (nNOS) or endothelial NOS (eNOS). Compound 3 was 10- to 100-fold more potent an inhibitor than 4, exhibited a 5-fold increase in nNOS/iNOS and eNOS/iNOS selectivity over 4, and displayed tight binding characteristics against iNOS. These results indicate that the relative configuration of the cyclopropyl ring in the L-arginine analogues significantly affects their inhibitory potential and NOS isoform selectivity.


Biochemistry Research International | 2010

Cloning, Expression, and Purification of a Nitric Oxide Synthase-Like Protein from Bacillus cereus

Heather J. Montgomery; Andrea L. Dupont; Hilary E. Leivo; J. Guy Guillemette

The nitric oxide synthase-like protein from Bacillus cereus (bcNOS) has been cloned, expressed, and characterized. This small hemeprotein (356 amino acids in length) has a mass of 43 kDa and forms a dimer. The recombinant protein showed similar spectral shifts to the mammalian NOS proteins and could bind the substrates L-arginine and NG-hydroxy-L-arginine as well as the ligand imidazole. Low levels of activity were recorded for the hydrogen peroxide-dependent oxidation of NG-hydroxy-L-arginine and L-arginine by bcNOS, while a reconstituted system with the rat neuronal NOS reductase domain showed no activity. The recombinant bcNOS protein adds to the complement of bacterial NOS-like proteins that are used for the investigation of the mechanism and function of NO in microorganisms.


Journal of Biological Chemistry | 2000

Removal of a putative inhibitory element reduces the calcium-dependent calmodulin activation of neuronal nitric-oxide synthase.

Heather J. Montgomery; Vladimir Romanov; J. Guy Guillemette


Journal of Biological Chemistry | 2004

Differential Activation of Nitric-oxide Synthase Isozymes by Calmodulin-Troponin C Chimeras

Elena Newman; Donald E. Spratt; Jennifer Mosher; Bo Cheyne; Heather J. Montgomery; Denney L. Wilson; J. Brice Weinberg; Susan Smith; John C. Salerno; Dipak K. Ghosh; J. Guy Guillemette


Journal of Biological Chemistry | 2004

Thermodynamics of Oxidation-Reduction Reactions in Mammalian Nitric-oxide Synthase Isoforms

Ying Tong Gao; Susan M. E. Smith; J. Brice Weinberg; Heather J. Montgomery; Elena Newman; J. Guy Guillemette; Dipak K. Ghosh; Linda J. Roman; Pavel Martásek; John C. Salerno


Biochemistry | 2003

Activation of constitutive nitric oxide synthases by oxidized calmodulin mutants.

Heather J. Montgomery; Ryan K. Bartlett; Basil Perdicakis; Eric Jervis; Thomas C. Squier; J. Guy Guillemette


Molecular Therapy | 2007

Real-time Fluorescence Tracking of Dynamic Transgene Variegation in Stem Cells

John Ramunas; Heather J. Montgomery; Liam Kelly; Tanya Sukonnik; James Ellis; Eric Jervis


Bioorganic & Medicinal Chemistry | 2005

Photocontrol of nitric oxide production in cell culture using a caged isoform selective inhibitor.

Basil Perdicakis; Heather J. Montgomery; Glenn L. Abbott; Dan Fishlock; Gilles A. Lajoie; J. Guy Guillemette; Eric Jervis


Archives of Biochemistry and Biophysics | 1998

The reductase domain of the human inducible nitric oxide synthase is fully active in the absence of bound calmodulin.

Derek C. Newton; Heather J. Montgomery; J. Guy Guillemette

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Eric Jervis

University of Waterloo

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Liam Kelly

University of Waterloo

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