60 results on '"Louis Grenier"'
Search Results
2. Discovery of a Selective Phosphoinositide-3-Kinase (PI3K)-γ Inhibitor (IPI-549) as an Immuno-Oncology Clinical Candidate
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Christian M. Martin, Jennifer Proctor, Patrick O'Hearn, Janid A. Ali, Andre Lescarbeau, Jennifer Hoyt, Jonathan P. DiNitto, Ann M. Rowley, Thomas T. Tibbitts, Catherine A. Evans, Martin R. Tremblay, Tao Liu, Vito J. Palombella, John Soglia, Johan A. Pradeilles, Somarajan J. Nair, Melissa Pink, David G. Winkler, Stanley Goldstein, Quentin Glenadel, Erin L. O’Hearn, Culver Cheung, Erin Brophy, Alfredo C. Castro, and Louis Grenier
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0301 basic medicine ,Phosphoinositide 3-kinase ,biology ,Kinase ,Organic Chemistry ,Pharmacology ,Biochemistry ,03 medical and health sciences ,030104 developmental biology ,Pharmacokinetics ,In vivo ,hemic and lymphatic diseases ,Drug Discovery ,biology.protein ,NEUTROPHIL MIGRATION ,Clinical evaluation ,PI3K/AKT/mTOR pathway - Abstract
Optimization of isoquinolinone PI3K inhibitors led to the discovery of a potent inhibitor of PI3K-γ (26 or IPI-549) with >100-fold selectivity over other lipid and protein kinases. IPI-549 demonstrates favorable pharmacokinetic properties and robust inhibition of PI3K-γ mediated neutrophil migration in vivo and is currently in Phase 1 clinical evaluation in subjects with advanced solid tumors.
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- 2016
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3. Development of a Multi Kilogram-Scale, Tandem Cyclopropanation Ring-Expansion Reaction en Route to Hedgehog Antagonist IPI-926
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Michael Foley, Andre Lescarbeau, Martin R. Tremblay, Lombardy Richard John, Grogan Michael John, Andrew B. Hague, Kristopher M. Depew, Jimin Xiong, Joseph Helble, Priscilla L. White, Julian Adams, Brian C. Austad, Caroline D. Lory, Somarajan J. Nair, Stéphane Peluso, Lin-Chen Yu, Alfredo C. Castro, André B. Charette, Benjamin S. Lane, Jeanne Shaffer, Louis Grenier, James R. Porter, Matthew Campbell, Koney Nii O, and Mark L. Behnke
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Tandem ,010405 organic chemistry ,Cyclopropanation ,Stereochemistry ,Chemistry ,Aryl ,Organic Chemistry ,Carbocation ,010402 general chemistry ,Ring (chemistry) ,01 natural sciences ,Semisynthesis ,0104 chemical sciences ,chemistry.chemical_compound ,Reagent ,Stereoselectivity ,Physical and Theoretical Chemistry - Abstract
The formation of the d-homocyclopamine ring system in IPI-926 is the key step in its semisynthesis and proceeds via a chemoselective cyclopropanation followed by a stereoselective acid-catalyzed carbocation rearrangement. In order to perform large-scale cyclopropanation reactions, we developed new iodomethylzinc bis(aryl)phosphate reagents that were found to be both effective and safe. These soluble reagents can be prepared under mild conditions and are stable during the course of the reaction. Importantly, they have favorable energetics relative to other cyclopropanating agents such as EtZnCH2I. Herein, we describe the process optimization studies that led to successful large-scale production of the d-homocyclopamine core necessary for IPI-926.
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- 2016
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4. A Design of Experiments Approach to a Robust Final Deprotection and Reactive Crystallization of IPI-926, A Novel Hedgehog Pathway Inhibitor
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Martin Trudeau, Louis Grenier, Kristopher M. Depew, Daniel G. Genov, Alexandre Côté, Brian C. Austad, Lin-Chen Yu, Andre Lescarbeau, Theodore A. Martinot, Priscilla L. White, Joseph Helble, and Somarajan J. Nair
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business.industry ,Chemistry ,Design of experiments ,Organic Chemistry ,Nanotechnology ,law.invention ,law ,Scientific method ,Physical and Theoretical Chemistry ,Crystallization ,Robust control ,Process engineering ,business ,Salt formation - Abstract
A design of experiments (DoE) approach was taken to optimize purity and reaction yield of the final debenzylation and hydrochloride salt formation of IPI-926. The study involved a careful dissection of the different process steps to enable an independent investigation of these steps while ensuring that process streams were representative. The results enabled a streamlined process from the final chemical transformation to the salting and isolation and led to the elimination of variability in the process as well as a robust control of impurities. The optimized process was applied to production and demonstrated on the kilogram scale.
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- 2015
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5. Pharmaceutical development of IPI-504, an Hsp90 inhibitor and clinical candidate for the treatment of cancer
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John Lee, Roger H. Pak, Louis Grenier, Vince Ammoscato, Michael Curtis, Kaiming Li, John Henderson, Matthew Campbell, Denise Mayes, Jason Kropp, Natalie Goltz, Bennett Carter, Johan Sebastian Basuki, Bradley Maurer, Gary Baker, James R. Wright, David Rusch, Rebecca Ahn, Brian C. Austad, Kris Depew, Joseph Helble, Jie Ge, Jason J. Piotrowski, Marlene R. Booth, Julian Adams, Mark Douglas, Steven G. Wong, Laila Kott, James R. Porter, Geoff E. Sylvester, Dumitru Ionescu, Jennifer R. Porter, and Brendan Arsenault
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Drug ,Hydroquinone ,Hydrochloride ,media_common.quotation_subject ,Cancer ,Pharmacology ,medicine.disease ,Hsp90 inhibitor ,Quinone ,Clinical trial ,chemistry.chemical_compound ,chemistry ,In vivo ,Drug Discovery ,medicine ,media_common - Abstract
IPI-504 (retaspimycin hydrochloride) is an Hsp90 inhibitor that is the subject of multiple clinical trials for the treatment of cancer. IPI-504 is an aqueous soluble (>200 mg/ml) hydroquinone hydrochloride salt of 17-(allylamino)-17-demethoxygeldanamycin (17-AAG), a quinone derivative also undergoing clinical evaluation, albeit with suboptimal formulations that address its inferior aqueous solubility (∼50 µg/ml). IPI-504 interconverts with 17-AAG in vivo through oxidation-reduction reactions that result in a dynamic redox equilibrium. The development challenges associated with redox active molecules are significant due to the pH, oxygen, and temperature sensitivities associated with such chemotypes. The API and sterile drug product manufacturing processes thus warrant the monitoring and control of these key variables. Furthermore, the pharmaceutical development challenges associated with cancer agents that are often fast-tracked due to unmet medical needs mandate a rapid development cycle with associated regulatory hurdles. Drug Dev Res 71: 429–438, 2010. © 2010 Wiley-Liss, Inc.
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- 2010
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6. Semisynthetic Cyclopamine Analogues as Potent and Orally Bioavailable Hedgehog Pathway Antagonists
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Matthew Campbell, Caroline N. Woodward, Jens Sydor, Alfredo C. Castro, James R. Porter, Margaret A. Read, Kerrie Faia, Kerry White, Martin R. Tremblay, Jill Cushing, Julian Adams, Lin-Chen Yu, Mark L. Behnke, Jennifer Hoyt, Vito J. Palombella, Karen McGovern, Somarajan J. Nair, Jeffrey K. Tong, Margit Hagel, Marta Nevalainen, Louis Grenier, and Michael Foley
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Molecular Structure ,Cyclopamine ,Stereochemistry ,Alkaloid ,Veratrum Alkaloids ,Administration, Oral ,Chemical synthesis ,Hedgehog signaling pathway ,Veratrum alkaloid ,Structure-Activity Relationship ,chemistry.chemical_compound ,chemistry ,Drug Discovery ,Molecular Medicine ,Structure–activity relationship ,Hedgehog Proteins ,Hedgehog ,Enone ,Signal Transduction - Abstract
Herein is reported the synthesis of a novel class of hedgehog antagonists derived from cyclopamine. The acid sensitive D-ring of cyclopamine was homologated utilizing a sequence of chemoselective cyclopropanation and stereoselective acid-catalyzed rearrangement. Further modification of the A/B-ring homoallylic alcohol to the conjugated ketone led to the discovery of new cyclopamine analogues with improved pharmaceutical properties and in vitro potency (EC 50) ranging from 10 to 1000 nM.
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- 2008
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7. Development of 17-allylamino-17-demethoxygeldanamycin hydroquinone hydrochloride (IPI-504), an anti-cancer agent directed against Hsp90
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Roger H. Pak, Louis Grenier, Julian Adams, Jeffrey K. Tong, James D. Wright, Janid A. Ali, Courtney Penders, Emmanuel Normant, Jens R. Sydor, Jon S. Patterson, Melissa Pink, Jie Ge, Jebecka Hudak, Marlene Dembski, Yilong Zhang, Jim Sang, Christine S. Pien, Caroline N. Woodward, James R. Porter, Margaret Read, John A. Barrett, David Grayzel, and Vito J. Palombella
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Lactams, Macrocyclic ,Antineoplastic Agents ,Biology ,Tanespimycin ,Pharmacology ,Hsp90 inhibitor ,Mice ,chemistry.chemical_compound ,In vivo ,Cell Line, Tumor ,Neoplasms ,hemic and lymphatic diseases ,Benzoquinones ,polycyclic compounds ,medicine ,Animals ,Humans ,HSP90 Heat-Shock Proteins ,Cell Proliferation ,Mice, Inbred BALB C ,Multidisciplinary ,Bortezomib ,Cell growth ,Biological activity ,Biological Sciences ,Xenograft Model Antitumor Assays ,Hsp90 ,chemistry ,Microsomes, Liver ,biology.protein ,Proteasome inhibitor ,medicine.drug - Abstract
Heat shock protein 90 (Hsp90) is an emerging therapeutic target of interest for the treatment of cancer. Its role in protein homeostasis and the selective chaperoning of key signaling proteins in cancer survival and proliferation pathways has made it an attractive target of small molecule therapeutic intervention. 17-Allylamino-17-demethoxygeldanamycin (17-AAG), the most studied agent directed against Hsp90, suffers from poor physical-chemical properties that limit its clinical potential. Therefore, there exists a need for novel, patient-friendly Hsp90-directed agents for clinical investigation. IPI-504, the highly soluble hydroquinone hydrochloride derivative of 17-AAG, was synthesized as an Hsp90 inhibitor with favorable pharmaceutical properties. Its biochemical and biological activity was profiled in an Hsp90-binding assay, as well as in cancer-cell assays. Furthermore, the metabolic profile of IPI-504 was compared with that of 17-AAG, a geldanamycin analog currently in clinical trials. The anti-tumor activity of IPI-504 was tested as both a single agent as well as in combination with bortezomib in myeloma cell lines andin vivoxenograft models, and the retention of IPI-504 in tumor tissue was determined. In conclusion, IPI-504, a potent inhibitor of Hsp90, is efficacious in cellular and animal models of myeloma. It is synergistically efficacious with the proteasome inhibitor bortezomib and is preferentially retained in tumor tissues relative to plasma. Importantly, it was observed that IPI-504 interconverts with the known agent 17-AAGin vitroandin vivovia an oxidation-reduction equilibrium, and we demonstrate that IPI-504 is the slightly more potent inhibitor of Hsp90.
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- 2006
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8. Protein-rich diet attenuates cyclosporin A-induced renal tubular damage in rats
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Marie Simard, Pierrette Gourde, Denis Beauchamp, Louise Thibault, Louis Grenier, Isabelle Plante, Michel LeBrun, Gaston Labrecque, and Marianne Pons
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medicine.medical_specialty ,Drinking ,Medicine (miscellaneous) ,Diuresis ,Urine ,Acute nephrotoxicity ,Kidney Tubules, Proximal ,Rats, Sprague-Dawley ,Excretion ,chemistry.chemical_compound ,Internal medicine ,Cyclosporin a ,Acetylglucosaminidase ,Animals ,Medicine ,Gamma-glutamyltransferase ,Diet, Fat-Restricted ,Creatinine ,Kidney ,Nutrition and Dietetics ,biology ,business.industry ,Body Weight ,Caseins ,gamma-Glutamyltransferase ,beta-Galactosidase ,Immunohistochemistry ,Rats ,Endocrinology ,medicine.anatomical_structure ,chemistry ,Nephrology ,Cyclosporine ,biology.protein ,Female ,Kidney Diseases ,Dietary Proteins ,Energy Intake ,business - Abstract
The objective of the present study was to look at the effect of a protein-rich diet on cyclosporine A (CsA)-induced acute nephrotoxicity in rodents using markers of tubular damage.Female Sprague-Dawley rats were conditioned to either a standard or a casein-rich diet for 2 weeks. Then, they were given CsA intraperitoneally (25 mg/kg/24 h or an equivalent volume of vehicle (Cremophor EL; Sigma Chemical Co, St. Louis, MO) for 7 days at 7 AM.During CsA treatment, bodyweight, caloric consumption, water intake, and urine output were not significantly different in animals fed with the standard Rat Chow and those on the high-protein feeding. On days 1 and 7, the 24-hour urine excretion of N-acetyl-beta-d-glucosaminidase (NAG) and beta-galactosidase (beta-GAL) were significantly (P.001) lower in CsA-treated rats on the high-protein diet than in those on the standard Rat Chow. After 7 days of treatment with CsA, no significant difference in the renal function level was found between rats fed with the standard or the casein-rich diet. The post-necrotic cellular regeneration in renal cortex was significantly lower (p0.001) in CsA-treated rats on the high-protein than on the standard diet. In CsA-treated rats on the standard diet, immunogold labeling showed a massive and specific concentration of the drug into lysosomes of proximal tubular cells. Contrastingly, no gold particle was found over the lysosomes of animals given the rich-protein feeding.In our current experimental conditions, a protective effect of high-casein diet against CsA-induced proximal tubular damage was observed in Sprague-Dawley rats.
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- 2003
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9. Multiplex PCR assays for the detection of clinically relevant antibiotic resistance genes in staphylococci isolated from patients infected after cardiac surgery
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Louis Grenier, Marc Ouellette, François J. Picard, Michel G. Bergeron, Paul H. Roy, and Francis Martineau
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Adult ,Microbiology (medical) ,Staphylococcus aureus ,Erythromycin ,Microbial Sensitivity Tests ,Drug resistance ,Biology ,Staphylococcal infections ,medicine.disease_cause ,Polymerase Chain Reaction ,Microbiology ,Staphylococcus epidermidis ,Multiplex polymerase chain reaction ,medicine ,Humans ,Surgical Wound Infection ,Pharmacology (medical) ,Coronary Artery Bypass ,Pharmacology ,Staphylococcal Infections ,medicine.disease ,biology.organism_classification ,Drug Resistance, Multiple ,Penicillin ,Infectious Diseases ,Gentamicin ,medicine.drug - Abstract
Multiresistant staphylococci (82 Staphylococcus aureus and 114 coagulase-negative staphylococci) were characterized by testing with rapid multiplex polymerase chain reaction (PCR) assays for species identification and detection of associated antibiotic resistance genes. These 196 staphylococci were isolated from 149 adult patients who developed wound infection after elective coronary artery bypass grafts and/or valve surgery. The multiplex PCR assays allowed identification of the most common staphylococcal species with S. aureus- and Staphylococcus epidermidis-specific primers as well as the detection of the erythromycin resistance genes ermA, ermB, ermC and msrA, the aminoglycoside resistance gene aac(6')-aph(2"), the oxacillin resistance gene mecA and the penicillin resistance gene blaZ. There was a very good correlation between the genotypic analysis by PCR and the phenotype determined by standard methods of susceptibility testing and identification of staphylococcal species: 100% for erythromycin resistance, 98.0% for gentamicin resistance, 99.0% for oxacillin resistance, 100% for penicillin resistance and 100% for S. aureus and S. epidermidis species identification. This study suggests that the incidence and distribution of the tested clinically relevant antibiotic resistance genes in staphylococci associated with infections after cardiac surgery do not differ from those in strains from other infections. These multiplex PCR assays may be used as diagnostic tools to replace or complement standard methods of susceptibility testing and identification of staphylococci.
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- 2000
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10. A Novel and Efficient Synthesis of a Highly Active Analogue of clasto-Lactacystin β-Lactone
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Julian Adams, Teresa A. McCormack, Francois Soucy, Louis Grenier, Mark L. Behnke, Louis Plamondon, and Antonia T. Destree
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Colloid and Surface Chemistry ,Stereochemistry ,Chemistry ,Convergent synthesis ,Clasto-lactacystin beta-lactone ,macromolecular substances ,General Chemistry ,Biochemistry ,Catalysis - Abstract
Herein, we describe a new convergent synthesis of a more potent analogue of clasto-lactacystin β-lactone (2), PS-519 compound 4, which is currently in preclinical development for the treatment of i...
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- 1999
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11. Potent and selective inhibitors of the proteasome: Dipeptidyl boronic acids
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Louis Plamondon, Shaowu Chen, Janice M. Klunder, Amy A. Cruickshank, Julian Adams, Yu-Ting Ma, Lawrence R. Dick, Mark L. Behnke, Louis Grenier, and Ross L. Stein
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inorganic chemicals ,Proteasome Endopeptidase Complex ,Clinical Biochemistry ,Pharmaceutical Science ,Biochemistry ,Chemical synthesis ,chemistry.chemical_compound ,Multienzyme Complexes ,Drug Discovery ,Peptide synthesis ,Protease Inhibitors ,Molecular Biology ,chemistry.chemical_classification ,Dipeptide ,Molecular Structure ,biology ,Organic Chemistry ,Boronic Acids ,In vitro ,Cysteine Endopeptidases ,Enzyme ,chemistry ,Proteasome ,Enzyme inhibitor ,biology.protein ,Molecular Medicine ,Boronic acid - Abstract
Potent and selective dipeptidyl boronic acid proteasome inhibitors are described. As compared to peptidyl aldehyde compounds, boronic acids in this series display dramatically enhanced potency. Compounds such as 15 are promising new therapeutics for treatment of cancer and inflammatory diseases.
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- 1998
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12. Preparation of enantiopure 4-oxygenated pipecolic acid derivatives
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Paul C. Anderson, Yves Bousquet, Ingrid Guse, Jean-Simon Duceppe, Louis Grenier, and Tibor Bogri
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Decarboxylation ,Organic Chemistry ,Biochemistry ,Dieckmann condensation ,chemistry.chemical_compound ,Enantiopure drug ,chemistry ,Intramolecular force ,Drug Discovery ,Michael reaction ,Organic chemistry ,Stereoselectivity ,Piperidine ,Pipecolic acid - Abstract
Two approaches to enantiopure 4-oxo- and 4-( R )-hydroxypipecolic acid derivatives from protected L-aspartic acid were developed. The first route exploits an intramolecular Michael addition on the stable enaminone 8 . Hydrogenation and concomitant decarboxylation gave the 4-oxo derivative 11 which was reduced selectively to the 4-( R )-hydroxy derivative 12 . The second route starts with a Michael addition followed by an intramolecular Dieckmann condensation to build the piperidine ring. The 4-oxo derivatives 11 and 19 are thus obtained in an expeditious manner on large scale without any chromatographic purification. Both sequences proved to be highly stereoselective.
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- 1997
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13. Active Site-directed Inhibitors of Rhodococcus 20 S Proteasome
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Frank Zühl, Louis Plamondon, Bikash C. Pramanik, Lawrence Dick, Clive A. Slaughter, Louis Grenier, Teresa Mc Cormack, Carolyn R. Moomaw, Ross L. Stein, Francois Soucy, and Wolfgang Baumeister
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chemistry.chemical_classification ,biology ,Stereochemistry ,Active site ,Peptide ,Cell Biology ,biology.organism_classification ,Biochemistry ,Small molecule ,Amino acid ,chemistry ,Proteasome ,biology.protein ,Threonine ,Binding site ,Molecular Biology ,Rhodococcus - Abstract
We have studied the mechanism of inhibition of the recombinant Rhodococcus proteasome by four different chemical classes of active site-directed small molecule inhibitors.Clasto-lactacystin β-lactone is a time-dependent inhibitor of the Rhodococcusproteasome’s ability to hydrolyze Suc-Leu-Leu-Val-Tyr-AMC, a substrate for this proteasome’s single type of active site, and proceeds with ak inact/[I] of 1,700m −1 s−1. Using peptide mapping of tryptic digests, LC/MS, and amino acid sequence analysis, we have established that the Oγ of the hydroxyl group on the N-terminal threonine of the β-subunit is the sole modification made by the β-lactone. Active site titrations of the Rhodococcus proteasome with reversible peptide aldehydes show the expected stoichiometry of one inhibitor molecule per β-subunit. Prior modification with β-lactone completely abrogates the binding of peptidyl boronic acid inhibitors, suggesting that these inhibitors also inactivate the enzyme by reacting with the Oγ moiety on Thr1. High performance liquid chromatography analysis of peptidyl vinyl sulfone-modified intactRhodococcus proteasome β-subunit and its tryptic peptides suggests that the peptidyl vinyl sulfone modifies a residue in the N-terminal 20 amino acids. This modification is also blocked by prior treatment with β-lactone.
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- 1997
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14. Practical, Stereoselective Synthesis of Palinavir, a Potent HIV Protease Inhibitor
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Jean-Simon Duceppe, Louis Plamondon, Yvan Guindon, Colette Boucher, Ingrid Guse, Serge Valois, Pierre L. Beaulieu, Christiane Yoakim, Yves Bousquet, and Dominik Wernic, Pierre Lavallee, Francois Soucy, Louis Grenier, James Gillard, A. Abraham, Chantal Grand-Maître, Paul C. Anderson, and Vida Gorys
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Peptidomimetic ,Chemistry ,Organic Chemistry ,HIV Protease Inhibitor ,Stereoselectivity ,Combinatorial chemistry - Abstract
Palinavir is a potent peptidomimetic-based HIV protease inhibitor. We have developed a highly convergent and stereoselective synthesis which is amenable to the preparation of multikilogram quantities of this compound. The synthetic sequence proceeds in 24 distinct chemical steps (with several integrated, multistep operations) from commercially available starting materials. No chromatographies are required throughout the process, and the final product is purified by crystallization of its dihydrochloride salt to >99% homogeneity.
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- 1997
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15. Mechanistic Studies on the Inactivation of the Proteasome by Lactacystin in Cultured Cells
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Antonia T. Destree, Louis Plamondon, Amy A. Cruikshank, Vito J. Palombella, Sandra L. Nunes, Lawrence R. Dick, Teresa A. McCormack, Lana A. Parent, Francesco D. Melandri, Ross L. Stein, and Louis Grenier
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Proteasome Endopeptidase Complex ,Lactacystin ,macromolecular substances ,Cysteine Proteinase Inhibitors ,Biology ,Biochemistry ,Lactones ,chemistry.chemical_compound ,Multienzyme Complexes ,Tumor Cells, Cultured ,medicine ,Humans ,Molecular Biology ,Oligopeptide ,Biological Transport ,Cell Biology ,Glutathione ,Pyrrolidinones ,In vitro ,Acetylcysteine ,Cell biology ,Cysteine Endopeptidases ,Cytosol ,chemistry ,Proteasome ,Proteasome inhibitor ,Oligopeptides ,HeLa Cells ,medicine.drug - Abstract
The natural product lactacystin exerts its cellular antiproliferative effects through a mechanism involving acylation and inhibition of the proteasome, a cytosolic proteinase complex that is an essential component of the ubiquitin-proteasome pathway for intracellular protein degradation. In vitro, lactacystin does not react with the proteasome; rather, it undergoes a spontaneous conversion (lactonization) to the active proteasome inhibitor, clasto-lactacystin beta-lactone. We show here that when the beta-lactone is added to mammalian cells in culture, it rapidly enters the cells, where it can react with the sulfhydryl of glutathione to form a thioester adduct that is both structurally and functionally analogous to lactacystin. We call this adduct lactathione, and like lactacystin, it does not react with the proteasome, but can undergo lactonization to yield back the active beta-lactone. We have studied the kinetics of this reaction under appropriate in vitro conditions as well as the kinetics of lactathione accumulation and proteasome inhibition in cells treated with lactacystin or beta-lactone. The results indicate that only the beta-lactone (not lactacystin) can enter cells and suggest that the formation of lactathione serves to concentrate the inhibitor inside cells, providing a reservoir for prolonged release of the active beta-lactone.
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- 1997
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16. Effects of fasting on temporal variations in nephrotoxicity of gentamicin in rats
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Denis Beauchamp, Michele Couture, P Collin, Michel LeBrun, Louis Grenier, Louise Thibault, Michel G. Bergeron, and Gaston Labrecque
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medicine.medical_specialty ,Time Factors ,Renal cortex ,medicine.medical_treatment ,Intraperitoneal injection ,Drinking ,Biology ,Kidney ,Kidney Function Tests ,Nephrotoxicity ,Rats, Sprague-Dawley ,Eating ,Internal medicine ,medicine ,Animals ,Pharmacology (medical) ,Saline ,Antibacterial agent ,Pharmacology ,Body Weight ,Aminoglycoside ,Fasting ,Immunohistochemistry ,Anti-Bacterial Agents ,Rats ,Microscopy, Electron ,Infectious Diseases ,Endocrinology ,medicine.anatomical_structure ,Toxicity ,Female ,Kidney Diseases ,Gentamicin ,Gentamicins ,Research Article ,medicine.drug - Abstract
Evidence for temporal variations in the nephrotoxicity of low doses of aminoglycosides were recently shown by using specific and sensitive parameters of renal toxicity. The aim of the present study was to evaluate the effect of a short period of fasting on the temporal variations in the renal toxicity of gentamicin. Twenty-eight normally fed (i.e., food and water were available ad libitum throughout the experiment) female Sprague-Dawley rats (weight, 175 to 220 g) and 28 fasted rats (i.e., only water was available during a 12-h fast before and a 24-h fast after gentamicin injection) were used. The animals were synchronized on a 14-h light, 10-h dark cycle (lights on at 0600 h) for 1 week before gentamicin administration. In July 1993, each group of animals was treated with a single intraperitoneal injection of saline (NaCl, 0.9%) or gentamicin (150 mg/kg of body weight) at either the peak (1400 h) or the trough (0200 h) of the previously determined toxicity. On day 1, the 24-h urinary excretion of beta-galactosidase, N-acetyl-beta-D-glucosaminidase, and gamma-glutamyltransferase was significantly higher in normally fed animals treated with gentamicin at 1400 h than in their time-matched controls and in normally fed animals treated at 0200 h (P < 0.01), which had normal levels of these enzymes. By contrast, the urinary excretion of these enzymes was significantly higher in both groups of gentamicin-treated, fasted rats than in their time-matched control groups (P < 0.01), reaching levels similar to those measured in normally fed rats treated at 1400 h. The accumulation of gentamicin was significantly lower in the renal cortex of normally fed rats treated at 0200 h than in rats treated at 1400 h (P < 0.05), but this time-dependent difference was not found in fasted rats treated at 0200 and 1400 h. Immunogold labeling done on ultrathin sections and observed by electron microscopy showed a similar subcellular localization of gentamicin in normally fed and fasted rats treated at either 1400 or 0200 h. These results suggest that the feeding period is of crucial importance in the temporal variations of the nephrotoxicity of gentamicin in rats.
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- 1996
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17. Mechanistic Studies on the Inactivation of the Proteasome by Lactacystin
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Amy A. Cruikshank, Sandra L. Nunes, Ross L. Stein, Lawrence R. Dick, Francesco D. Melandri, and Louis Grenier
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Metabolite ,Lactacystin ,macromolecular substances ,Cell Biology ,Biology ,biology.organism_classification ,Biochemistry ,Streptomyces ,Cysteine Proteinase Inhibitors ,Acetylcysteine ,chemistry.chemical_compound ,Hydrolysis ,chemistry ,Proteasome ,Cell culture ,medicine ,Molecular Biology ,medicine.drug - Abstract
Lactacystin is a Streptomyces metabolite that inhibits cell cycle progression and induces differentiation in a murine neuroblastoma cell line. The cellular target of lactacystin is the 20 S proteasome, also known as the multicatalytic proteinase complex, an essential component of the ubiquitin-proteasome pathway for intracellular protein degradation. In aqueous solution at pH 8, lactacystin undergoes spontaneous hydrolysis to yield N-acetyl-L-cysteine and the inactive lactacystin analog, clasto-lactacystin dihydroxy acid. We have studied the mechanism of lactacystin hydrolysis under these conditions and found that it proceeds exclusively through the intermediacy of the active lactacystin analog, clasto-lactacystin beta-lactone. Conditions that stabilize lactacystin (and thus prevent the transient accumulation of the intermediate beta-lactone) negate the ability of lactacystin to inactivate the proteasome. Together these findings suggest that lactacystin acts as a precursor for clasto-lactacystin beta-lactone and that the latter is the sole species that interacts with the proteasome.
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- 1996
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18. Nephrotoxicity of amphotericin b in rats: Effects of the time of administration
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Gaston Labrecque, Louis Grenier, Pierrette Gourde, Denis Beauchamp, Michel G. Bergeron, and Michel LeBrun
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Time Factors ,Renal cortex ,Significant difference ,General Medicine ,Pharmacology ,Biology ,Kidney ,General Biochemistry, Genetics and Molecular Biology ,Circadian Rhythm ,Rats ,Nephrotoxicity ,Rats, Sprague-Dawley ,medicine.anatomical_structure ,Amphotericin B ,Creatinine ,Darkness ,medicine ,Animals ,Female ,Circadian rhythm ,General Pharmacology, Toxicology and Pharmaceutics ,medicine.drug - Abstract
Amphotericin B is a potentially nephrotoxic agent used for the treatment of severe mycoses and numerous fungal infections. Temporal variation in the nephrotoxicity of amphotericin B was studied in rats maintained on a light-dark period of 14 hrs of light and 10 hrs of darkness (light on: 06h00). Subgroups of animals were treated with a single daily i.p. dose of either 5% dextrose or amphotericin B (10 mg/kg/day) given at either 07h00, 13h00, 19h00 or 01h00 for 4 and 10 days. On day 4, no significant difference was observed in any parameter studied. On day 10, the cellular regeneration ([3H]-thymidine incorporation into DNA of renal cortex)(p0.01), BUN levels (p0.05), serum creatinine (p0.05), and accumulation of amphotericin B in the renal cortex (p0.05) were significantly higher when animals were treated with similar subcellular localization of amphotericin B in the proximal tubular cells of the renal cortex. These results showed a temporal variation in the nephrotoxicity of amphotericin B (peak toxicity occurred at 07h00) which is different from that of other nephrotoxic antibiotics such as aminoglycosides.
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- 1996
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19. Preparation of (2S,4R)-4-Hydroxypipecolic Acid and Derivatives
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Paul C. Anderson, Pierre Lavallee, James Gillard, and Ingrid Guse, Tibor Bogri, Yves Bousquet, A. Abraham, Pierre L. Beaulieu, and Louis Grenier
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Chemistry ,Organic Chemistry ,4-hydroxypipecolic acid ,Organic chemistry - Published
- 1996
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20. Peptidomimetic inhibitors of herpes simplex virus ribonucleotide reductase: a new class of antiviral agents
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Robert Deziel, Dominik Wernic, Sylvie Goulet, Pierre L. Beaulieu, Raymond Plante, Jean-Simon Duceppe, Elsie Ghiro, Louis Grenier, Jean-Marie Ferland, Jean Gauthier, Neil Moss, and Montse Llinas-Brunet
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Herpesvirus 2, Human ,Protein subunit ,Herpesvirus 1, Human ,Virus Replication ,medicine.disease_cause ,Antiviral Agents ,Virus ,Cell Line ,Structure-Activity Relationship ,In vivo ,Cricetinae ,Ribonucleotide Reductases ,Drug Discovery ,medicine ,Animals ,Humans ,Structure–activity relationship ,biology ,Chemistry ,Virology ,In vitro ,Ribonucleotide reductase ,Herpes simplex virus ,Enzyme inhibitor ,biology.protein ,Molecular Medicine ,Oligopeptides - Abstract
We have been investigating a new class of antiviral compounds effective against herpes simplex virus (HSV) in vitro and in vivo. Antiviral activity results from inhibition of HSV ribonucleotide reductase (RR). The inhibitors are designed as mimics of the RR small subunit C-terminus, a region essential for RR subunit association and consequently enzymatic activity. Inhibition results from specific binding of the inhibitor to the HSV RR large subunit thereby preventing subunit association. This report details the structure--activity studies that lead to the indentification of BILD 1263, a potent inhibitor of HSV RR subunit association (IC50, 0.2 nM) that also inhibits the replication of HSV types 1 and 2 in cell culture (EC50, 3 and 4 microM) and reduces the severity of HSV-1-induced keratitis in a murine ocular model. The discovery of inhibitors with in vitro antiviral results from a combination of improving inhibitor potency in a RR binding assay and modifying inhibitor physicochemical properties. The importance and possible role of the new structural modifications introduced into this inhibitor series is discussed.
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- 1995
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21. Protection against gentamicin nephrotoxicity by daptomycin in nephrectomized rats
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Michel G. Bergeron, Marie Simard, Louis Grenier, Denis Beauchamp, and Nathalie Thibault
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medicine.medical_specialty ,Kidney Cortex ,medicine.medical_treatment ,Pharmacology ,Nephrectomy ,General Biochemistry, Genetics and Molecular Biology ,Nephrotoxicity ,Kidney Tubules, Proximal ,Rats, Sprague-Dawley ,Daptomycin ,polycyclic compounds ,medicine ,Animals ,General Pharmacology, Toxicology and Pharmaceutics ,Microscopy, Immunoelectron ,Saline ,business.industry ,General Medicine ,biochemical phenomena, metabolism, and nutrition ,bacterial infections and mycoses ,Rats ,Surgery ,carbohydrates (lipids) ,Sphingomyelin Phosphodiesterase ,Creatinine ,Concomitant ,Toxicity ,Female ,Kidney Diseases ,lipids (amino acids, peptides, and proteins) ,Gentamicin ,Gentamicins ,Lysosomes ,business ,medicine.drug - Abstract
Daptomycin was previously shown to reduce gentamicin renal toxicity and this toxicity was not delayed by the concomitant injection of daptomycin (Thibault N., L. Grenier, M. Simard, M. G. Bergeron, and D. Beauchamp, Antimicrob. Agents Chemother., 38 1027-1035 (1994)). The protective effect of daptomycin against gentamicin toxicity was evaluated in 96 female Sprague-Dawley rats. Normal and nephrectomized rats were treated with saline (NaCl, 0.9%), gentamicin (30 mg/kg/12 hrs, i.p.), daptomycin (10 mg/kg/12 hrs, s.c.) or with a combination of daptomycin plus gentamicin during 4 and 10 days. On day 4, gentamicin and daptomycin cortical levels were higher in nephrectomized gentamicin-daptomycin-treated rats (p0.05) as compared to all other groups. The accumulation of gentamicin or daptomycin in nephrectomized gentamicin-daptomycin-treated or gentamicin-saline-treated rats was higher on day 4 (p0.01) than on day 10. Other parameters such as the sphingomyelinase activity in the renal cortex, the serum creatinine, and the histopathology showed significantly fewer changes in daptomycin-gentamicin-treated rats as compared to animals given gentamicin alone. On the other hand, the protection of daptomycin was less extensive in nephrectomized rats as compared to normal rats. Daptomycin and gentamicin were localized in the lysosomes of proximal tubular cells of animals treated with daptomycin and gentamicin given alone or in combination. These results suggest that daptomycin protects against gentamicin toxicity in nephrectomized rats but to a lesser extent than in normal rats.
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- 1995
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22. Circadian Variation in the Intracortical Accumulation Kinetics of Tobramycin in Conscious Rats
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Michel G. Bergeron, Michel LeBrun, Louis Grenier, Denis Beauchamp, Lesheng Lin, Chantal Guimont, and Gaston Labrecque
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Chronobiology ,medicine.medical_specialty ,Kidney ,Physiology ,Aminoglycoside ,Biology ,medicine.anatomical_structure ,Endocrinology ,Pharmacokinetics ,Physiology (medical) ,Internal medicine ,Toxicity ,medicine ,Tobramycin ,Circadian rhythm ,Antibacterial agent ,medicine.drug - Abstract
The time-dependent variation in the renal accumulation of aminoglycosides has not been extensively investigated. The aim of the present study was to better characterize the temporal variation in the intracortical accumulation kinetics of tobramycin. Female Sprague-Dawley rats weighing 210–254 g were maintained in a 14 h light/10 h dark cycle (light on 06h00–20h00). They were infused for 6 h with tobramycin to achieve individual steady-state serum levels of 0.5–15 μg/ml over four different periods of the day (02h00–08h00; 08h00–14h00; 14h00–20h00; and 20h00–02h00). As previously reported, the steady-state elevation of serum tobramycin concentrations was associated with a linear increase of the cortical concentration in all groups. The tobramycin accumulation rate was significantly lower in animals infused at 20h00–02h00 compared to rats infused at 08h00–14h00 (p < 0.001). The data suggest that the lower rate of tobramycin accumulation during the dark period might be responsible for the lower toxicity obser...
- Published
- 1995
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23. Temporal changes of pharmacokinetics, nephrotoxicity, and subcellular distribution of tobramycin in rats
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Louis Grenier, Denis Beauchamp, Marie Simard, Michel G. Bergeron, Yves Bergeron, Gaston Labrecque, and Lesheng Lin
- Subjects
medicine.medical_specialty ,Kidney Cortex ,Time Factors ,Biology ,Acetylglucosamine ,Nephrotoxicity ,Rats, Sprague-Dawley ,Bolus (medicine) ,Pharmacokinetics ,Internal medicine ,Acetylglucosaminidase ,medicine ,Tobramycin ,Animals ,Pharmacology (medical) ,Circadian rhythm ,Antibacterial agent ,Pharmacology ,Body Weight ,Immunohistochemistry ,Rats ,Infectious Diseases ,Endocrinology ,Toxicity ,Female ,Kidney Diseases ,medicine.symptom ,Weight gain ,Research Article ,Subcellular Fractions ,Thymidine ,medicine.drug - Abstract
The present study was designed to determine the temporal changes in tobramycin nephrotoxicity during the dark and the light periods of the day and to look for the mechanisms of such changes. Female Sprague-Dawley rats (9 to 11 weeks old) were housed in a 14-h-light-10-h-dark cycle (lights on 0600 to 2000 h). A bolus of tobramycin (60 mg/kg of body weight) was intravenously injected into a first group of 15 rats, at either 1400 or 0200 h. Six blood samples were taken from each rat, 30 to 210 min after the bolus injection. The total clearance of the drug was reduced during the rest period (1400 h) of rats compared with the activity period (0200 h) (P = 0.0007). Another group of 99 rats was given intraperitoneally a single dose of tobramycin (40 mg/kg), and renal cortices were collected 2 to 222 h after injection. The cortical drug levels were always higher in animals injected at 1400 h than in those injected at 0200 h. A last group of 32 rats was used in the studies of tobramycin (30 mg/kg/day, once daily for 10 days, intraperitoneally) nephrotoxicity and subcellular distribution. Weight gain in the rats receiving tobramycin (both 1400 and 0200 h) was significantly (P = 0.028) less than that in the controls. Nephrotoxicity, indicated by the incorporation of [3H]thymidine into cortical DNA and urinary excretion of N-acetyl-beta-D-glucosaminidase, was significantly higher in animals treated at 1400 h than in those treated at 0200 h. No difference in the subcellular distribution of tobramycin was observed. The data indicate that the reduction in the clearance of tobramycin during the rest period is in part responsible for the higher nephrotoxicity in rats.
- Published
- 1994
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24. ChemInform Abstract: Asymmetric Selenomethoxylation of Olefins Involving a Chiral C2 Symmetrical Electrophilic Organoselenium Reagent
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Josée Bordeleau, Sylvie Goulet, Julie Bernier, Louis Grenier, and Robert Deziel
- Subjects
Addition reaction ,chemistry.chemical_compound ,Chemistry ,Stereochemistry ,Reagent ,Electrophile ,General Medicine ,Methanol ,Selectivity ,Combinatorial chemistry ,Adduct - Abstract
A new chiral C 2 symmetrical organoselenium reagent has been synthesized; this compound, in the presence of methanol, reacts with high facial selectivity with olefins to afford the anti selenomethoxylated adducts in very good yields
- Published
- 2010
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25. ChemInform Abstract: Inhibition of Herpes Simplex Virus Type 1 Ribonucleotide Reductase by Substituted Tetrapeptide Derivatives
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Ghiro Elise, Norman Aubry, Murray D. Bailey, Dominik Wernic, Jean Gauthier, Jean Marie Ferland, Julian Adams, Pierre Lavallee, Francois Soucy, Yvan Guindon, C. Lepine‐Frenette, Pierre L. Beaulieu, Sumanas Rakhit, Robert Deziel, Sylvie Goulet, M. Baillet, John Dimaio, Raymond Plante, N. Moss, Jean-Simon Duceppe, and Louis Grenier
- Subjects
Herpes simplex virus ,Ribonucleotide reductase ,Tetrapeptide ,Biochemistry ,Chemistry ,medicine ,General Medicine ,medicine.disease_cause - Published
- 2010
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- View/download PDF
26. ChemInform Abstract: Preparation of (2S,4R)-4-Hydroxypipecolic Acid and Derivatives
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A. Abraham, Yves Bousquet, Ingrid Guse, Pierre Lavallee, J. Gilllard, Louis Grenier, Paul C. Anderson, Pierre L. Beaulieu, and Tibor Bogri
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chemistry.chemical_classification ,Chemistry ,Stereochemistry ,4-hydroxypipecolic acid ,Organic chemistry ,General Medicine ,Amino acid - Published
- 2010
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- View/download PDF
27. ChemInform Abstract: A Practical and Diastereoselective Synthesis of Ketomethylene Dipeptide Isosteres of the Type AAψ(COCH2)Asp
- Author
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Montse Llinas-Brunet, Eric Malenfant, Louis Grenier, Robert Deziel, Raymond Plante, N. Moss, Jean-Simon Duceppe, and V. Caron
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chemistry.chemical_classification ,chemistry.chemical_compound ,Dipeptide ,chemistry ,Stereochemistry ,Organic chemistry ,General Medicine ,Amino acid - Published
- 2010
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- View/download PDF
28. ChemInform Abstract: Practical, Stereoselective Synthesis of Palinavir, a Potent HIV Protease Inhibitor
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Ingrid Guse, Pierre Lavallee, A. Abraham, Louis Plamondon, Yves Bousquet, Chantal Grand-Maître, Jean-Simon Duceppe, Serge Valois, Colette Boucher, Paul C. Anderson, Dominik Wernic, Pierre L. Beaulieu, Francois Soucy, Yvan Guindon, Vida Gorys, Louis Grenier, James Gillard, and Christiane Yoakim
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Chemistry ,Stereochemistry ,HIV Protease Inhibitor ,Stereoselectivity ,General Medicine ,Combinatorial chemistry - Published
- 2010
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29. ChemInform Abstract: Preparation of Enantiopure 4-Oxygenated Pipecolic Acid Derivatives
- Author
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Tibor Bogri, Yves Bousquet, Louis Grenier, Ingrid Guse, Paul C. Anderson, and Jean-Simon Duceppe
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chemistry.chemical_compound ,Enantiopure drug ,chemistry ,Decarboxylation ,Intramolecular force ,Michael reaction ,Organic chemistry ,Stereoselectivity ,General Medicine ,Piperidine ,Dieckmann condensation ,Pipecolic acid - Abstract
Two approaches to enantiopure 4-oxo- and 4-( R )-hydroxypipecolic acid derivatives from protected L-aspartic acid were developed. The first route exploits an intramolecular Michael addition on the stable enaminone 8 . Hydrogenation and concomitant decarboxylation gave the 4-oxo derivative 11 which was reduced selectively to the 4-( R )-hydroxy derivative 12 . The second route starts with a Michael addition followed by an intramolecular Dieckmann condensation to build the piperidine ring. The 4-oxo derivatives 11 and 19 are thus obtained in an expeditious manner on large scale without any chromatographic purification. Both sequences proved to be highly stereoselective.
- Published
- 2010
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30. ChemInform Abstract: Potent and Selective Inhibitors of the Proteasome: Dipeptidyl Boronic Acids
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Mark L. Behnke, Lawrence R. Dick, Ross L. Stein, Yu-Ting Ma, Shaowu Chen, Louis Plamondon, Julian Adams, Janice M. Klunder, Amy A. Cruickshank, and Louis Grenier
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inorganic chemicals ,chemistry.chemical_classification ,chemistry.chemical_compound ,chemistry ,Proteasome ,Biochemistry ,medicine ,Potency ,Cancer ,General Medicine ,medicine.disease ,Aldehyde ,Boronic acid - Abstract
Potent and selective dipeptidyl boronic acid proteasome inhibitors are described. As compared to peptidyl aldehyde compounds, boronic acids in this series display dramatically enhanced potency. Compounds such as 15 are promising new therapeutics for treatment of cancer and inflammatory diseases.
- Published
- 2010
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31. ChemInform Abstract: A Novel and Efficient Synthesis of a Highly Active Analogue of clasto-Lactacystin β-Lactone
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Louis Plamondon, Julian Adams, Mark L. Behnke, Antonia T. Destree, Francois Soucy, Teresa A. McCormack, and Louis Grenier
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chemistry.chemical_classification ,chemistry.chemical_compound ,Addition reaction ,chemistry ,Lactacystin ,General Medicine ,Combinatorial chemistry ,Lactone - Published
- 2010
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32. Lunar Underground Mining and Construction: A Terrestrial Vision Enabling Space Exploration and Commerce
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Greg Baiden, Brad Blair, and Louis Grenier
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Engineering ,Underground mining (soft rock) ,business.industry ,Commercial enterprise ,business ,Space exploration ,Construction engineering ,Remote sensing - Abstract
As early as 1959 the US army considered a permanent underground base on the moon. While the original underground idea has significant merit, space agencies have strayed from this sensible concept, focusing instead on short-term touch and go missions and relying on the expendable paradigm. Newly disclosed advances in underground telerobotic mining technology for terrestrial purposes provides a foundation for an emerging opportunity for international space programs to conceptualize, design, build and implement an underground lunar habitat and polar volatile mining and processing operation. This paper discusses an emerging uniquely Canadian concept for a permanent manned outpost on the moon, an outpost that could enable a longer-term commercial enterprise. The paper offers rationale for an underground lunar outpost, and discusses how it might be constructed as well as the terrestrial technologies that could enable a radiationprotected underground habitat to made and later utilized to mine lunar volatiles.
- Published
- 2010
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33. Abstract 4973: A novel cellular class I phosphoinositide-3-kinase (PI3K) isoform-specific occupancy assay demonstrates a direct correlation between PI3K isoform activity and phospho-AKT levels
- Author
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Lina Gu, Bonnie Tillotson, Jonathan P. DiNitto, Erin Brophy, Janid A. Ali, Louis Grenier, and Erin S. Murphy
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Gene isoform ,Cancer Research ,Phosphoinositide 3-kinase ,Oncology ,biology ,Chemistry ,biology.protein ,Phospho akt ,PI3K/AKT/mTOR pathway ,Cell biology - Abstract
Background: AKT phosphorylation is a widely used pharmacodynamic indicator for Class I PI3K activity in cells and tumors; however, the direct correlation of pAKT with PI3K activity has not been carefully examined. We have developed a novel, direct isoform specific occupancy assay for PI3K to determine if intracellular isoform specific inhibition of PI3K is quantitatively equivalent to inhibition of pAKT formation. Methods: A biotin-conjugated derivative of the irreversible pan-PI3K inhibitor, wortmannin, was synthesized. All four class I PI3K isoforms could be pulled down using this biotin-probe. ATP-competitive PI3K inhibitor binding prevented probe binding in a dose dependent manner, and hence pull-down of PI3K. Inhibition isotherms monitoring the decrease in PI3K pulled down with increasing inhibitor concentrations were generated via western blot with PI3K isoform specific antibodies. The affinity of a given inhibitor against PI3K-β, -δ, and -γ was determined in various cell lines and compared to inhibition of pAKT levels measured by ELISA or western blotting in unstimulated 786.0 cells, IgM-stimulated Raji cells, and C5a-stimulated RAW264.7 cells. Results: We utilized the occupancy assay on these cell lines with compounds that have differential biochemical PI3K isoform inhibition profiles. All of these cell lines significantly express more than one PI3K isoform, with Raji and 786.0 cells expressing PI3K-δ and -β, and RAW264.7 cells expressing PI3K-δ and -γ. In unstimulated 786.0 cells, PI3K-β and PI3K-δ occupancy IC50s were obtained and compared with pAKT IC50s. PI3K-β occupancy IC50s, but not PI3K-δ occupancy IC50s, correlated well with pAKT IC50s, indicating that in 786.0 cells, PI3K-β is the main driver for pAKT formation. Similarly, PI3K-β and PI3K-δ occupancy IC50s were obtained in anti-IgM stimulated Raji cells. Here pAKT IC50s correlated with PI3K-δ, and not PI3K-β occupancy IC50s, indicating that PI3K-δ is the major signaling isoform responding to this stimulus. The PI3K-δ occupancy IC50s were similar in C5a-stimulated RAW264.7 cells, but here the PI3K-γ occupancy IC50 was equivalent to pAKT IC50, confirming that PI3K-γ is the major PI3K signaling isoform downstream of C5a in RAW264.7 cells. Interestingly, PI3K-δ and PI3K-γ occupancy IC50s were similar between stimulated or unstimulated Raji or RAW264.7 cells. Therefore, PI3K occupancy is unaffected by PI3K migration to the cell membrane after stimulation. Conclusions: To our knowledge, this is the first demonstration that occupancy of membrane-recruited Class I PI3K isoforms by PI3K inhibitors directly correlates with the inhibition of pAKT. These results also indicate a predominant PI3K signaling isoform is responsible for downstream pAKT formation in these cell lines, validating them for PI3K isoform specific cell based assays. Citation Format: Lina Gu, Erin Brophy, Erin Murphy, Bonnie Tillotson, Jonathan DiNitto, Louis Grenier, Janid Ali. A novel cellular class I phosphoinositide-3-kinase (PI3K) isoform-specific occupancy assay demonstrates a direct correlation between PI3K isoform activity and phospho-AKT levels. [abstract]. In: Proceedings of the 106th Annual Meeting of the American Association for Cancer Research; 2015 Apr 18-22; Philadelphia, PA. Philadelphia (PA): AACR; Cancer Res 2015;75(15 Suppl):Abstract nr 4973. doi:10.1158/1538-7445.AM2015-4973
- Published
- 2015
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34. Design, synthesis, and biological evaluation of hydroquinone derivatives of 17-amino-17-demethoxygeldanamycin as potent, water-soluble inhibitors of Hsp90
- Author
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Asimina T. Georges, Julian Adams, James R Porter, Janid A. Ali, Emmanuel Normant, Yun Gao, Roger H. Pak, Jie Ge, Vito J. Palombella, Thomas T. Tibbitts, Louis Grenier, Marlene S Dembski, Jeffrey K. Tong, Jon Patterson, and Jens Sydor
- Subjects
Models, Molecular ,Glucose-regulated protein ,Receptor, ErbB-2 ,Lactams, Macrocyclic ,Antineoplastic Agents ,Fluorescence Polarization ,Chemical synthesis ,Binding, Competitive ,Structure-Activity Relationship ,Dogs ,Heat shock protein ,Cell Line, Tumor ,Drug Discovery ,polycyclic compounds ,Benzoquinones ,Structure–activity relationship ,Animals ,Humans ,Protein Isoforms ,HSP70 Heat-Shock Proteins ,HSP90 Heat-Shock Proteins ,biology ,Chemistry ,Endoplasmic reticulum ,Membrane Proteins ,Water ,Biological activity ,Hsp90 ,Hydroquinones ,Biochemistry ,Rifabutin ,Solubility ,Chaperone (protein) ,biology.protein ,Molecular Medicine ,Drug Screening Assays, Antitumor - Abstract
17-Allylamino-17-demethoxygeldanamycin (17-AAG)1 is a semisynthetic inhibitor of the 90 kDa heat shock protein (Hsp90) currently in clinical trials for the treatment of cancer. However, 17-AAG faces challenging formulation issues due to its poor solubility. Here we report the synthesis and evaluation of a highly soluble hydroquinone hydrochloride derivative of 17-AAG, 1a (IPI-504), and several of the physiological metabolites. These compounds show comparable binding affinity to human Hsp90 and its endoplasmic reticulum (ER) homologue, the 94 kDa glucose regulated protein (Grp94). Furthermore, the compounds inhibit the growth of the human cancer cell lines SKBR3 and SKOV3, which overexpress Hsp90 client protein Her2, and cause down-regulation of Her2 as well as induction of Hsp70 consistent with Hsp90 inhibition. There is a clear correlation between the measured binding affinity of the compounds and their cellular activities. Upon the basis of its potent activity against Hsp90 and a significant improvement in solubility, 1a is currently under evaluation in Phase I clinical trials for cancer.
- Published
- 2006
35. A Practical and Diastereoselective Synthesis of Ketomethylene Dipeptide Isosteres of the Type AAΨ[COCH2]Asp
- Author
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Raymond Plante, Jean-Simon Duceppe, Neil Moss, Eric Malenfant, Robert Deziel, Louis Grenier, Montse Llinas-Brunet, and Valérie Caron
- Subjects
chemistry.chemical_compound ,Dipeptide ,chemistry ,Stereochemistry ,Organic Chemistry - Published
- 1996
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36. Novel IKK inhibitors: beta-carbolines
- Author
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Christine S. Pien, Julian Adams, Lana A. Parent, Francois Soucy, Maria Hottelet, Luan C. Dang, Hormoz Mazdiyasni, Vito Palombella, Alfredo C. Castro, and Louis Grenier
- Subjects
IKappaB Kinase ,Clinical Biochemistry ,Blotting, Western ,Pharmaceutical Science ,Endogeny ,Electrophoretic Mobility Shift Assay ,IκB kinase ,Protein Serine-Threonine Kinases ,Biochemistry ,environment and public health ,chemistry.chemical_compound ,Structure-Activity Relationship ,Drug Discovery ,Structure–activity relationship ,Humans ,Enzyme Inhibitors ,CHUK ,Protein kinase A ,Molecular Biology ,Natural product ,biology ,Organic Chemistry ,I-Kappa-B Kinase ,General Medicine ,Precipitin Tests ,Cell biology ,I-kappa B Kinase ,enzymes and coenzymes (carbohydrates) ,chemistry ,Enzyme inhibitor ,IKK complex ,biology.protein ,Molecular Medicine ,Phosphorylation ,Signal transduction ,biological phenomena, cell phenomena, and immunity ,Carbolines ,HeLa Cells - Abstract
Inhibitors of IkappaB kinase (IKK) have long been sought as specific regulators of NF-kappaB. A screening effort of the endogenous IKK complex allowed us to identify 5-bromo-6-methoxy-beta-carboline as a nonspecific IKK inhibitor. Optimization of this beta-carboline natural product derivative resulted in a novel class of selective IKK inhibitors with IC(50)s in the nanomolar range. In addition, we show that one of these beta-carboline analogues inhibits the phosphorylation of IkappaBalpha and subsequent activation of NF-kappaB in whole cells, as well as blocking TNF-alpha release in LPS-challenged mice.
- Published
- 2003
37. Asymmetric selenomethoxylation of olefins involving a chiral C2 symmetrical electrophilic organoselenium reagent
- Author
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Julie Bernier, Josée Bordeleau, Louis Grenier, Sylvie Goulet, and Robert Deziel
- Subjects
chemistry.chemical_classification ,Addition reaction ,chemistry.chemical_compound ,Ketone ,chemistry ,Reagent ,Organic Chemistry ,Electrophile ,Ether ,Selectivity ,Asymmetric induction ,Combinatorial chemistry ,Catalysis - Abstract
A new chiral C 2 symmetrical organoselenium reagent has been synthesized; this compound, in the presence of methanol, reacts with high facial selectivity with olefins to afford the anti selenomethoxylated adducts in very good yields
- Published
- 1993
- Full Text
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38. Effect of fasting on temporal variation in the nephrotoxicity of amphotericin B in rats
- Author
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Michel G. Bergeron, Louis Grenier, Denis Beauchamp, Louise Thibault, Gaston Labrecque, and Michel LeBrun
- Subjects
medicine.medical_specialty ,Antifungal Agents ,Kidney Cortex ,Time Factors ,Renal function ,Biology ,Kidney Function Tests ,Nephrotoxicity ,Blood Urea Nitrogen ,Excretion ,Rats, Sprague-Dawley ,chemistry.chemical_compound ,Internal medicine ,Amphotericin B ,Acetylglucosaminidase ,medicine ,Animals ,Pharmacology (medical) ,Blood urea nitrogen ,Triglycerides ,Pharmacology ,Creatinine ,Cholesterol, HDL ,Fasting ,medicine.disease ,beta-Galactosidase ,Rats ,Infectious Diseases ,Endocrinology ,chemistry ,Toxicity ,Female ,Kidney Diseases ,Kidney disease ,medicine.drug - Abstract
Evidence for temporal variation in the nephrotoxicity of amphotericin B was recently reported in experimental animals. The role of food in these variations was determined by studying the effect of a short fasting period on the temporal variation in the renal toxicity of amphotericin B. Twenty-eight normally fed and 28 fasted female Sprague-Dawley rats were used. Food was available ad libitum to the fed rats, while the fasted animals were fasted 12 h before and 24 h after amphotericin B injection to minimize stress for the animals. Water was available ad libitum to both groups of rats, which were maintained on a 14-h light, 10-h dark regimen (light on at 0600 h). Renal toxicity was determined by comparing the levels of excretion of renal enzyme and the serum creatinine and blood urea nitrogen (BUN) levels at the time of the maximal (0700 h) or the minimal (1900 h) nephrotoxicity after the intraperitoneal administration of a single dose of dextrose (5%; control group) or amphotericin B (50 mg/kg of body weight; treated group) to the rats. The nephrotoxicities obtained after amphotericin B administration at both times of day were compared to the nephrotoxicities observed for time-matched controls. In fed animals, the 24-h urinary excretion of N -acetyl-β- d -glucosaminidase and β-galactosidase was significantly higher when amphotericin B was injected at 0700 and 1900 h. The excretion of these two enzymes was reduced significantly ( P < 0.05) in fasting rats, and this effect was larger at 0700 h ( P < 0.05) than at 1900 h. The serum creatinine level was also significantly higher ( P < 0.05) in fed animals treated at 0700 h than in fed animals treated at 1900 h. Fasting reduced significantly ( P < 0.05) the increase in the serum creatinine level, and this effect was larger in the animals treated at 0700 h. Similar data were obtained for BUN levels. Amphotericin B accumulation was significantly higher ( P < 0.05) in the renal cortexes of fed rats than in those of fasted animals, but there was no difference according to the time of injection. These results demonstrated that fasting reduces the nephrotoxicity of amphotericin B and that food availability is of crucial importance in the temporal variation in the renal toxicity of amphotericin B in rats.
- Published
- 1999
39. Kinetic studies of the branched chain amino acid preferring peptidase activity of the 20S proteasome: development of a continuous assay and inhibition by tripeptide aldehydes and clasto-lactacystin beta-lactone
- Author
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Francesco D. Melandri, Ross L. Stein, Lawrence R. Dick, Amy A. Cruikshank, Sandra L. Nunes, Louis Plamondon, Teresa A. McCormack, and Louis Grenier
- Subjects
Proteasome Endopeptidase Complex ,Stereochemistry ,Branched-chain amino acid ,Lactacystin ,Peptide ,Tripeptide ,Cysteine Proteinase Inhibitors ,Biochemistry ,Mass Spectrometry ,Substrate Specificity ,chemistry.chemical_compound ,Hydrolysis ,Lactones ,Multienzyme Complexes ,Endopeptidases ,Animals ,Protease Inhibitors ,chemistry.chemical_classification ,Aldehydes ,Amino acid ,Cysteine Endopeptidases ,Kinetics ,chemistry ,Proteasome ,Rabbits ,Oligopeptides ,Lactone ,Amino Acids, Branched-Chain - Abstract
We have developed an assay to continuously monitor the branched amino acid preferring peptidase (BrAAP) activity of the proteasome. This assay is based on the hydrolysis of the fluorogenic peptide, Abz-Gly-Pro-Ala-Leu-Ala-Nba (Abz is 2-aminobenzoyl and Nba is 4-nitrobenzylamide) which is cleaved exclusively at the Leu-Ala bond by the 20S proteasome with a kc/Km value of 13 000 M-1 s-1. Hydrolysis of this peptide is accompanied by an increase in fluorescence intensity (lambda ex = 340 nm, lambda em = 415 nm) due to release of the internally quenched 2-aminobenzoyl fluorescence that accompanies diffusion apart of the hydrolysis products, Abz-Gly-Pro-Ala-Leu and Ala-Nba. Using this assay, we examined inhibition of the BrAAP activity of the proteasome by a series of tripeptide aldehydes, Z-Leu-Leu-Xaa-H. When Xaa = Phe, (p-Cl)Phe, and Trp we observe biphasic or partial inhibition of the BrAAP activity. In contrast, when Xaa = Nva and Leu, simple inhibition kinetics are observed and allow us to calculate Ki values of 120 nM and 12 nM, respectively. The inhibitors that exhibit simple inhibition kinetics for BrAAP activity are also approximately equipotent for inhibition of the chymotrypsin-like (ChT-L) and peptidyl-glutamyl peptide hydrolyzing (PGPH) activities, dissociation constants varying by less than 25-fold, whereas the inhibitors that exhibit biphasic inhibition kinetics for BrAAP activity are300-fold more potent for inhibiting ChT-L activity than for PGPH activity. Inactivation of the BrAAP activity of the proteasome by clasto-lactacystin beta-lactone is also biphasic. beta-Lactone inactivates approximately 60% of the BrAAP activity rapidly, with kinetics indistinguishable from its inactivation of the chymotrypsin-like activity. The remaining 40% of the BrAAP activity is inactivated by beta-lactone at a 50-fold slower rate, with kinetics indistinguishable from its inactivation of the PGPH activity. These results suggest a mechanism in which hydrolysis of Abz-Gly-Pro-Ala-Leu-Ala-Nba (i.e., BrAAP activity) occurs at two different active sites in the 20S proteasome, and that these two active sites are the same ones that catalyze the previously described ChT-L and PGPH activities.
- Published
- 1998
40. Time-restricted feeding schedules modify temporal variation of gentamicin experimental nephrotoxicity
- Author
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Pierrette Gourde, Chantal Guimont, Denis Beauchamp, Michel LeBrun, Louise Thibault, Gaston Labrecque, Michel G. Bergeron, D Tardif, and Louis Grenier
- Subjects
medicine.medical_specialty ,Drug Evaluation, Preclinical ,Pharmacology ,Biology ,Nephrotoxicity ,Rats, Sprague-Dawley ,chemistry.chemical_compound ,Internal medicine ,medicine ,Animals ,Pharmacology (medical) ,Dosing ,Blood urea nitrogen ,Kidney ,Creatinine ,Analysis of Variance ,Aminoglycoside ,Anti-Bacterial Agents ,Circadian Rhythm ,Rats ,Infectious Diseases ,medicine.anatomical_structure ,Endocrinology ,chemistry ,Food ,Toxicity ,Multivariate Analysis ,Gentamicin ,Female ,Kidney Diseases ,Gentamicins ,medicine.drug ,Research Article - Abstract
The effect of timing of gentamicin dosing relative to food access periods was evaluated in experimental animals. Female Sprague-Dawley rats were treated for 4 and 10 days with gentamicin (40 mg/kg of body weight/day) intraperitoneally at either 0700, 1300, 1900, or 0100 h according to three food presentation schedules: food was available from 0800 to 1600 h in the first group, from 1600 to 0000 h in the second group, and from 0000 to 0800 h in the last group. Animals were thus subjected to a restricted feeding period. Results indicate that time-restricted feeding schedules displace the peak and the trough of gentamicin-induced renal toxicity, as evaluated by changes in the inhibition of sphingomyelinase activity, cellular regeneration (incorporation of [3H]thymidine into DNA of renal cortex), and blood urea nitrogen and serum creatinine levels, as well as histopathological lesions observed after 10 days of treatment. In fact, the toxicity was minimal when gentamicin was injected during the feeding period, while the maximal toxicity was found when gentamicin was administered during the fasting period. It is concluded that the feeding period can modulate aminoglycoside nephrotoxicity. The time of dosing of gentamicin relative to the time of feeding seems to be a more important modulator of gentamicin nephrotoxicity than the light-dark cycle.
- Published
- 1997
41. Attenuation of gentamicin-induced nephrotoxicity in rats by fleroxacin
- Author
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Louis Grenier, Jeanine-Anne Heuson-Stiennon, Jacqueline Zanen, Denis Beauchamp, Pierrette Gourde, Michel G. Bergeron, and Guy Laurent
- Subjects
Fleroxacin ,Renal cortex ,Pharmacology ,Nephrotoxicity ,Blood Urea Nitrogen ,Rats, Sprague-Dawley ,Anti-Infective Agents ,medicine ,Animals ,Pharmacology (medical) ,Blood urea nitrogen ,Phospholipids ,Antibacterial agent ,Hyperplasia ,business.industry ,Aminoglycoside ,Anti-Bacterial Agents ,Rats ,Infectious Diseases ,medicine.anatomical_structure ,Creatinine ,Toxicity ,Gentamicin ,Female ,Kidney Diseases ,Gentamicins ,business ,medicine.drug ,Research Article - Abstract
The effect of fleroxacin on gentamicin-induced nephrotoxicity was evaluated with female Sprague-Dawley rats. Animals were injected during 4 or 10 days with saline (NaCl; 0.9%), gentamicin alone at doses of 10 and 40 mg/kg of body weight/12 h (subcutaneously), fleroxacin alone at a dose of 25 mg/kg/12 h (intraperitoneally), or the combination gentamicin-fleroxacin in the same regimen. Gentamicin induced a dose- and time-dependent renal toxicity as evaluated by gentamicin cortical levels, sphingomyelinase activity in the renal cortex, histopathologic and morphometric analysis, blood urea nitrogen and serum creatinine levels, and cellular regeneration ([3H]thymidine incorporation into DNA of cortical cells). The extent of these changes was significantly reduced when gentamicin was given in combination with fleroxacin. Although the mechanisms by which fleroxacin reduces the nephrotoxic potential of gentamicin are unknown, we propose that the fleroxacin-gentamicin combination enhances exocytosis activity in proximal tubular cells, as suggested by the higher excretion of urinary enzymes and lower cortical levels of gentamicin observed in animals treated with the combination fleroxacin-gentamicin compared with those treated with gentamicin alone. The protective effect of fleroxacin on gentamicin nephrotoxicity should be investigated further.
- Published
- 1997
42. Day-night treatment difference of tobramycin serum and intrarenal drug distribution and nephrotoxicity in rats: effects of fasting
- Author
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Louis Grenier, Louise Thibault, Denis Beauchamp, Lesheng Lin, Michel G. Bergeron, Michel LeBrun, and Gaston Labrecque
- Subjects
medicine.medical_specialty ,Light ,Physiology ,Biology ,Kidney ,Nephrotoxicity ,Rats, Sprague-Dawley ,Eating ,Pharmacokinetics ,Physiology (medical) ,Internal medicine ,medicine ,Tobramycin ,Animals ,Tissue Distribution ,Circadian rhythm ,Antibacterial agent ,Aminoglycoside ,Fasting ,Darkness ,beta-Galactosidase ,Circadian Rhythm ,Rats ,medicine.anatomical_structure ,Endocrinology ,Creatinine ,Toxicity ,Female ,medicine.drug - Abstract
The effects of short-term food deprivation on the serum and renal distribution and nephrotoxicity of tobramycin were studied in female Sprague-Dawley rats maintained on a 14-h light/10-h dark cycle (light on: 06:00). For the distribution study, a single injection of tobramycin (40 mg/kg, i.p.) was administered at 14:00 or 02:00 to normally fed animals or to animals fasted for 12 h before tobramycin injection; these treatment times correspond to the peak and trough of tobramycin nephrotoxicity as previously determined in other studies. The serum and cortical levels of tobramycin were significantly higher 60, 120, and 240 min after the injection in fasted animals treated at 02:00 compared with normally fed animals treated at the same time (p0.05). In animals injected at 14:00, similar levels of tobramycin were measured in both fasted and fed rats. In the nephrotoxicity study, female Sprague-Dawley rats were fasted for 12 h before and 24 h after the timed single injection of tobramycin (150 mg/kg, i.p.). The 24-h urinary excretion of beta-galactosidase was significantly higher in fasted animals treated at 02:00 than in fed rats treated at the same time of day. Seventy-two hours following tobramycin injection, serum creatinine levels and cortical levels of tobramycin were significantly higher in fasted rats treated at 14:00 than at 02:00 and in fed rats treated at 14:00. These data suggest that a short period of food deprivation modulates the temporal variations of tobramycin nephrotoxicity.
- Published
- 1996
43. Temporal variation in nephrotoxicity of low doses of isepamicin in rats
- Author
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Gaston Labrecque, Michel G. Bergeron, Louis Grenier, Denis Beauchamp, Lesheng Lin, Yuji Yoshiyama, Nathalie J. Morin, Pierrette Gourde, and Marie Simard
- Subjects
Male ,medicine.medical_specialty ,Kidney Cortex ,Time Factors ,medicine.medical_treatment ,Renal cortex ,Intraperitoneal injection ,Biology ,Nephrotoxicity ,Kidney Tubules, Proximal ,Rats, Sprague-Dawley ,Internal medicine ,medicine ,Animals ,Regeneration ,Pharmacology (medical) ,Saline ,Antibacterial agent ,Pharmacology ,Kidney ,Body Weight ,Immunohistochemistry ,Anti-Bacterial Agents ,Circadian Rhythm ,Rats ,Microscopy, Electron ,Infectious Diseases ,medicine.anatomical_structure ,Endocrinology ,Toxicity ,Kidney Diseases ,Isepamicin ,Gentamicins ,Injections, Intraperitoneal ,medicine.drug ,Thymidine ,Research Article - Abstract
The temporal variation in the nephrotoxicity of low doses of isepamicin was studied in male Sprague-Dawley rats treated with a single daily intraperitoneal injection of saline (NaCl, 0.9%) or isepamicin (80 mg/kg of body weight) at either 0800, 1400, 2000, or 0200 h for 4 and 10 days. On day 10, the cellular regeneration (incorporation of [3H] thymidine into DNA of renal cortex) and cortical accumulation of isepamicin were significantly higher in animals treated at 1400 h than at 0200 h (P < 0.01). Immunogold labeling studies showed that isepamicin was essentially localized in the lysosomes of proximal tubular cells in all treated groups, but the density of the gold particles over the lysosomes was higher in animals treated at 1400 than at 0200 h. The results of the present study show that the renal toxicity of isepamicin was maximal at 1400 h (midlight period) and minimal at 0200 h (middark period).
- Published
- 1996
44. Attenuation by daptomycin of gentamicin-induced experimental nephrotoxicity
- Author
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Louis Grenier, Marie Simard, Denis Beauchamp, Nathalie Thibault, and Michel G. Bergeron
- Subjects
Kidney Cortex ,Pharmacology ,Kidney ,Nephrotoxicity ,Rats, Sprague-Dawley ,chemistry.chemical_compound ,Daptomycin ,In vivo ,Tobramycin ,medicine ,Animals ,Pharmacology (medical) ,Antibacterial agent ,Creatinine ,business.industry ,DNA ,biochemical phenomena, metabolism, and nutrition ,Immunohistochemistry ,Rats ,Infectious Diseases ,Sphingomyelin Phosphodiesterase ,chemistry ,Toxicity ,Immunology ,Gentamicin ,lipids (amino acids, peptides, and proteins) ,Female ,Kidney Diseases ,Gentamicins ,business ,medicine.drug ,Research Article ,Subcellular Fractions ,Thymidine - Abstract
Previously, daptomycin was shown to reduce tobramycin nephrotoxicity in vivo (D. Beauchamp, M. Pellerin, P. Gourde, M. Pettigrew, and M. G. Bergeron, Antimicrob. Agents Chemother. 34:139-147, 1990; C. A. Wood, H. C. Finkbeiner, S. J. Kohlhepp, P. W. Kohnen, and D. C. Gilbert, Antimicrob. Agents Chemother. 33:1280-1285, 1989). Female Sprague-Dawley rats were treated with saline (NaCl, 0.9%), daptomycin (10 mg/kg of body weight every 12 h, subcutaneously), gentamicin (30 mg/kg/12 h, intraperitoneally) or with a combination of daptomycin plus gentamicin over a 10-day period. Animals were killed 4, 10, and 20 days after the end of treatment. Four days after the end of drug administration, gentamicin and daptomycin levels in the renal cortices of animals treated with the combination of daptomycin and gentamicin were significantly higher than in those of rats given gentamicin or daptomycin alone (P < 0.01). Despite the higher cortical concentrations of gentamicin, rats given the combination of gentamicin and daptomycin had less reduction in renal cortex sphingomyelinase activity, less evidence of regeneration of cellular cortical cells ([3H]thymidine incorporation into cortex DNA), lower creatinine concentration in serum, and less histopathologic evidence of injury than rats given gentamicin alone. By immunogold technique, both daptomycin and gentamicin were localized to the lysosomes of proximal tubular cells, regardless of whether animals received the drugs alone or in combination. Interestingly, myeloid body formation occurred in both those animals given gentamicin alone and those given daptomycin plus gentamicin. No significant changes were observed for all groups between 10 and 20 days after the end of therapy, suggesting that the toxicity of gentamicin was not delayed by the concomitant injection of daptomycin. The results confirm that daptomycin can attenuate experimental gentamicin nephrotoxicity.
- Published
- 1994
45. Ceftriaxone protects against tobramycin nephrotoxicity
- Author
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Michel G. Bergeron, Louis Grenier, Denis Beauchamp, Yves Bergeron, Sylvie Perron, Guy Thériault, L Fontaine, and Pierrette Gourde
- Subjects
Kidney Cortex ,medicine.medical_treatment ,Renal cortex ,Pharmacology ,Nephrotoxicity ,Rats, Sprague-Dawley ,chemistry.chemical_compound ,medicine ,Tobramycin ,Animals ,Pharmacology (medical) ,Drug Interactions ,Saline ,Antibacterial agent ,Creatinine ,business.industry ,Ceftriaxone ,beta-Galactosidase ,Enzymes ,Rats ,carbohydrates (lipids) ,Microscopy, Electron ,Infectious Diseases ,medicine.anatomical_structure ,Sphingomyelin Phosphodiesterase ,chemistry ,Immunology ,Toxicity ,Female ,Kidney Diseases ,business ,medicine.drug ,Thymidine ,Research Article - Abstract
The effect of ceftriaxone on tobramycin-induced nephrotoxicity was investigated. Female Sprague-Dawley rats were treated during 4 and 10 days with saline (NaCl, 0.9%), ceftriaxone at a dose of 100 mg/kg of body weight/12 h subcutaneously, tobramycin at doses of 40 and 60 mg/kg/12 h intraperitoneally, or the combination ceftriaxone-tobramycin. Creatinine levels in serum were significantly higher in animals treated with tobramycin alone given at 60 mg/kg/12 h during 10 days, compared with control animals (P < 0.01) or animals receiving the combination tobramycin-ceftriaxone (P < 0.01). After 10 days of treatment, ceftriaxone did not accumulate in renal tissue but did reduce the renal intracortical accumulation of tobramycin (P < 0.05). Tobramycin given alone at either 40 or 60 mg/kg/12 h induced a significant inhibition of sphingomyelinase activity compared with control animals (P < 0.05). However, this enzyme activity was significantly less inhibited when tobramycin was injected in combination with ceftriaxone (P < 0.05). Ceftriaxone alone had no effect on the activity of this enzyme. The [3H]thymidine incorporation into the DNA of renal cortex was also significantly lower in animals treated with tobramycin-ceftriaxone compared with animals receiving tobramycin alone (P < 0.05). The 24-h urinary excretion of beta-galactosidase was significantly reduced in animals treated with the combination tobramycin-ceftriaxone compared with the administration of tobramycin alone at 40 and 60 mg/kg/12 h after 5 and 10 days (P < 0.05). Histologically, ceftriazone induced very few cellular alterations and reduced considerably the presence of typical signs of tobramycin nephrotoxicity. This investigation demonstrated that ceftriaxone protects animals against tobramycin-induced nephrotoxicity.
- Published
- 1994
46. Nephrotoxicity of low doses of tobramycin in rats: effect of the time of administration
- Author
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Yuji Yoshiyama, Pierrette Gourde, Louis Grenier, Lesheng Lin, Michel G. Bergeron, Gaston Labrecque, Guy Thériault, and Denis Beauchamp
- Subjects
Kidney Cortex ,Time Factors ,medicine.medical_treatment ,Renal cortex ,Physiology ,Pharmacology ,General Biochemistry, Genetics and Molecular Biology ,Nephrotoxicity ,Rats, Sprague-Dawley ,chemistry.chemical_compound ,medicine ,Tobramycin ,Animals ,Regeneration ,Circadian rhythm ,General Pharmacology, Toxicology and Pharmaceutics ,Saline ,Creatinine ,business.industry ,Low dose ,General Medicine ,DNA ,Circadian Rhythm ,Rats ,medicine.anatomical_structure ,chemistry ,Toxicity ,Female ,Seasons ,business ,medicine.drug - Abstract
The circadian and the cricannual variations of the nephrotoxicity of tobramycin were studied in female Sprague-Dawley rats. Animals were maintained on a light-dark period of 1410 hrs (light on: 06h00 to 20h00). They were injected once daily for 4 and 10 days with saline or tobramycin at a dose of 40 mg/kg/day i.p. at either 08h00, 14h00, 20h00 and 02h00, in April 1991, July 91, October 91, January 92. In April 91, tobramycin injected at 14h00 during 10 days induced a significant increase of [3H]-thymidine incorporation into DNA of renal cortex as compared to other groups (p < 0.01): toxicity was highest at 14h00 and lowest at 02h00. No temporal change was observed in the renal cortical accumulation of tobramycin, and in serum creatinine after the 4 or 10 days of treatment. In experiments done in April, July and October 1991 and in January 1992, no circannual variation was found in tobramycin cortical levels but peaks of toxicity were observed at 02h00 in April and October 1991 and at 14h00 in July 1991 and January 1992. There was no linear correlation between the toxicity and the tobramycin accumulation in the renal cortex (r=0.21). The data suggest that the circadian changes in tobramycin toxicity are due to temporal changes in the susceptibility of renal cells to tobramycin.
- Published
- 1994
47. A Design of Experiments Approach to a Robust FinalDeprotection and Reactive Crystallization of IPI-926, A Novel HedgehogPathway Inhibitor.
- Author
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Theodore A. Martinot, Brian C. Austad, Alexandre Côté, Kristopher M. Depew, Daniel Genov, Louis Grenier, Joseph Helble, Andre Lescarbeau, Somarajan Nair, Martin Trudeau, Priscilla White, and Lin-Chen Yu
- Published
- 2015
- Full Text
- View/download PDF
48. Synthesis and biological activity of atrial natriuretic factor analogues: effect of modifications to the disulfide bridge
- Author
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John DiMaio, Louis Grenier, Jorge Jaramillo, Julian Adams, Dominik Wernic, and Ewald Welchner
- Subjects
Stereochemistry ,Molecular Sequence Data ,Cystine ,Receptors, Cell Surface ,In Vitro Techniques ,chemistry.chemical_compound ,Structure-Activity Relationship ,Drug Discovery ,medicine ,Animals ,Humans ,Secretion ,Amino Acid Sequence ,Disulfides ,Receptor ,Protecting group ,chemistry.chemical_classification ,Aldosterone ,Biological activity ,Fibroblasts ,Cyclic peptide ,Rats ,medicine.anatomical_structure ,chemistry ,Biochemistry ,Zona glomerulosa ,Molecular Medicine ,Cattle ,Zona Glomerulosa ,Rabbits ,Receptors, Atrial Natriuretic Factor ,Atrial Natriuretic Factor - Abstract
A series of atrial natriuretic factor (ANF) analogues with modifications to the disulfide bridge and lacking the exocyclic N-terminal sequence was synthesized. The native cystine residue was substituted by isofunctional deamino carba, beta,beta-dimethyl carba and dehydro dicarba spanners that bridge residues 106 and 120. The compounds were prepared by segment condensation coupling using the base-labile (9-fluorenylmethyl)carboxyl protecting group. Biological evaluation revealed that the exocyclic N-terminal segment of ANF is not necessary for expression of high biological activity. The compounds retained high affinity for ANF receptors in bovine adrenal zona glomerulosa cells and were found to be potent antihypertensive and diuretic agents, indicating that the native disulfide bridge can be mimicked by isosteric spanning residues. It was noted that the reported analogues, unlike the endogenous hormone, show marked reduced inhibitory activity on PGE1-stimulated aldosterone secretion from adrenal zona glomerulosa cells. This lack of inhibition may be a contributing element to the low saluresis in spite of the high level of diuresis observed with some analogues.
- Published
- 1990
49. Anti-Tumor Activity of IPI-504, a Novel Hsp90 Inhibitor in Multiple Myeloma
- Author
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Jon Patterson, Vito J. Palombella, James H. Porter, David Grayzel, Asimina T. Georges, John P. Barrett, Christine Pien, Adams Julian, Jennie Ge, Jeffrey K. Tong, Kenneth C. Anderson, Kerry Spear, Roger H. Pak, Janid Ali, Jebecka Hudak, Constantine S. Mitsiades, Emmanuel Normant, James Homer Wright, Melissa Pink, Louis Grenier, Jens Sydor, Michael Foley, Yun Gao, and Junbiao Sang
- Subjects
biology ,Immunology ,Cell Biology ,Hematology ,Geldanamycin ,Immunoglobulin light chain ,Biochemistry ,Hsp90 ,In vitro ,Hsp90 inhibitor ,chemistry.chemical_compound ,chemistry ,In vivo ,hemic and lymphatic diseases ,Cancer cell ,polycyclic compounds ,Cancer research ,biology.protein ,Cytotoxic T cell - Abstract
IPI-504 is a novel inhibitor of Hsp90 based on the geldanamycin pharmacophore. When placed in rat, monkey, and human blood, IPI-504 rapidly converts to the known and well-studied compound 17-allylamino-17-demethoxy-geldanamycin (17-AAG). 17-AAG is the subject of multiple clinical trials for the treatment of hematologic and solid tumors. However, 17-AAG suffers from poor aqueous solubility necessitating the use of sub-optimal formulations to deliver this agent to patients. IPI-504 is over 1000-fold more soluble than 17-AAG in aqueous solution. In vitro, both 17-AAG and IPI-504 bind tightly to, and selectively inhibit Hsp90 derived from cancer cells. The cytotoxic effect of IPI-504, as well as its ability to stimulate the degradation of Hsp90 client proteins and increase the intracellular levels Hsp70, were monitored in two human multiple myeloma cells lines (RPMI-8226 and MM1.S). The effects of IPI-504 were compared to 17-AAG. We demonstrate that the actions of IPI-504 are bioequivalent to 17-AAG and that both compounds induce apoptosis in these cells and stimulate the degradation of HER2 and c-Raf. In addition, both agents stimulate Hsp70 protein levels. In all cases the EC50s are virtually the same for both molecules (~200–400 nM). Furthermore, IPI-504 inhibits the secretion of immunoglobulin light chain from the RPMI-8226 multiple myeloma cells (EC50 ~300 nM). Importantly, IPI-504 is active in tumor xenograft models of multiple myeloma. The data indicate that active metabolites of IPI-504 accumulate in these xenografts long after these metabolites are cleared from the plasma compartment, suggesting that they preferentially accumulate in tumor cells based on their increased affinity to Hsp90 derived from tumor cells. In conclusion, we have developed IPI-504 as a novel, potent inhibitor of Hsp90 with greatly increased solubility over 17-AAG, and that IPI-504 is an active anti-tumor agent in vitro and in vivo.
- Published
- 2004
- Full Text
- View/download PDF
50. Semisynthetic Cyclopamine Analogues as Potent and Orally Bioavailable Hedgehog Pathway Antagonists.
- Author
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Martin R. Tremblay, Marta Nevalainen, Somarajan J. Nair, James R. Porter, Alfredo C. Castro, Mark L. Behnke, Lin-Chen Yu, Margit Hagel, Kerry White, Kerrie Faia, Louis Grenier, Matthew J. Campbell, Jill Cushing, Caroline N. Woodward, Jennifer Hoyt, Michael A. Foley, Margaret A. Read, Jens R. Sydor, Jeffrey K. Tong, and Vito J. Palombella
- Published
- 2008
- Full Text
- View/download PDF
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