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1. Supplementary Tables 1 through 4 and Supplementary Figures 1 through 5 from In Vitro and In Vivo Characterization of Irreversible Mutant-Selective EGFR Inhibitors That Are Wild-Type Sparing

Author

Juswinder Singh, Andrew Allen, Russell C. Petter, William F. Westlin, Mariana Nacht, Deqiang Niu, Thomas C. Harding, Andrew D. Simmons, Mitch Raponi, Jeff Etter, Henry Haringsma, Yixuan Ren, Prasoon Chaturvedi, Aravind Medikonda, Russell Karp, Richland Tester, Zhendong Zhu, Matthew T. Labenski, Thia St. Martin, Michael Sheets, Aleksandr Dubrovskiy, Annette O. Walter, Kwangho Lee, and Robert Tjin Tham Sjin

Abstract

PDF - 252K, Supplemental Table 1. Mass spectrometry on EGFR-L858R/T790M protein. Supplemental Table 2. EGFR modulation in A431, H1975 and HCC827 cells by compound 3. Supplemental Table 3. Kinase selectivity profile of compound 3, afatinib and WZ4002 at 1 ?M. Supplemental Table 4.Multi-dose level PK/PD study in H1975 tumor-bearing mice. Supplemental Figure 1. Signaling inhibition in EGFR wild-type (A431) and mutant EGFR NSCLC cells (H1975 and HCC827). Supplemental Figure 2. Prolonged duration of action on EGFR-L858R/T790M (A) and EGFR-DelE746-A750 (B) proteins. Supplemental Figure 3. Protein degradation (t1/2) of EGFR-L858R/T790M (A) and EGFR-DelE746-A750 (B) in H1975 and HCC827 cells, respectively. Supplemental Figure 4. Prolonged duration of action on EGFR-DelE746-A750 protein by erlotinib. Supplemental Figure 5. Time-dependent inhibition in EGFR mutant H1975 (A) and HCC827 (B) cells.

Published
2023
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2. Data from In Vitro and In Vivo Characterization of Irreversible Mutant-Selective EGFR Inhibitors That Are Wild-Type Sparing

Author

Juswinder Singh, Andrew Allen, Russell C. Petter, William F. Westlin, Mariana Nacht, Deqiang Niu, Thomas C. Harding, Andrew D. Simmons, Mitch Raponi, Jeff Etter, Henry Haringsma, Yixuan Ren, Prasoon Chaturvedi, Aravind Medikonda, Russell Karp, Richland Tester, Zhendong Zhu, Matthew T. Labenski, Thia St. Martin, Michael Sheets, Aleksandr Dubrovskiy, Annette O. Walter, Kwangho Lee, and Robert Tjin Tham Sjin

Abstract

Patients with non–small cell lung carcinoma (NSCLC) with activating mutations in epidermal growth factor receptor (EGFR) initially respond well to the EGFR inhibitors erlotinib and gefitinib. However, all patients relapse because of the emergence of drug-resistant mutations, with T790M mutations accounting for approximately 60% of all resistance. Second-generation irreversible EGFR inhibitors are effective against T790M mutations in vitro, but retain affinity for wild-type EGFR (EGFRWT). These inhibitors have not provided compelling clinical benefit in T790M-positive patients, apparently because of dose-limiting toxicities associated with inhibition of EGFRWT. Thus, there is an urgent clinical need for therapeutics that overcome T790M drug resistance while sparing EGFRWT. Here, we describe a lead optimization program that led to the discovery of four potent irreversible 2,4-diaminopyrimidine compounds that are EGFR mutant (EGFRmut) selective and have been designed to have low affinity for EGFRWT. Pharmacokinetic and pharmacodynamic studies in H1975 tumor–bearing mice showed that exposure was dose proportional resulting in dose-dependent EGFR modulation. Importantly, evaluation of normal lung tissue from the same animals showed no inhibition of EGFRWT. Of all the compounds tested, compound 3 displayed the best efficacy in EGFRL858R/T790M-driven tumors. Compound 3, now renamed CO-1686, is currently in a phase I/II clinical trial in patients with EGFRmut-advanced NSCLC that have received prior EGFR-directed therapy. Mol Cancer Ther; 13(6); 1468–79. ©2014 AACR.

Published
2023
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3. Supplementary Materials and Methods and Supplementary Figure Legends from In Vitro and In Vivo Characterization of Irreversible Mutant-Selective EGFR Inhibitors That Are Wild-Type Sparing

Author

Juswinder Singh, Andrew Allen, Russell C. Petter, William F. Westlin, Mariana Nacht, Deqiang Niu, Thomas C. Harding, Andrew D. Simmons, Mitch Raponi, Jeff Etter, Henry Haringsma, Yixuan Ren, Prasoon Chaturvedi, Aravind Medikonda, Russell Karp, Richland Tester, Zhendong Zhu, Matthew T. Labenski, Thia St. Martin, Michael Sheets, Aleksandr Dubrovskiy, Annette O. Walter, Kwangho Lee, and Robert Tjin Tham Sjin

Abstract

PDF - 91K, Supplemental Materials and Methods and Legends for Supplementary Figures 1 through 5.

Published
2023
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4. SMaSh: A Streptavidin Mass Shift Assay for Rapidly Quantifying Target Occupancy by Irreversible Inhibitors

Author

Susan Cantin, Alan F. Corin, Matthew T. Labenski, Lukas T. Voortman, Lixin Qiao, Giulia Giammo, and Leslie A. Bateman

Subjects
MAPK/ERK pathway, Streptavidin, Molecular Structure, biology, Chemistry, Ligand (biochemistry), Biochemistry, Structure-Activity Relationship, chemistry.chemical_compound, Covalent bond, Cell Line, Tumor, Agammaglobulinaemia Tyrosine Kinase, Leukocytes, Mononuclear, biology.protein, Biophysics, Humans, Bruton's tyrosine kinase, Biological Assay, Target protein, Protein kinase A, Protein Kinase Inhibitors, Tyrosine kinase
Abstract

The streptavidin mass shift (SMaSh) assay is a robust and fast approach for quantifying target protein occupancy by a covalent inhibitor or ligand. It exploits the biotin-streptavidin bond using the Simple Western platform. One measurement on a single sample determines both total and occupied target protein simultaneously and is, therefore, self-normalizing. The approach works in diverse and complex biological matrices and, with no need for matched vehicle-treated controls, readily applies to tissues from animal pharmacology models. Assessing occupancy is critical in the development of targeted covalent drugs. We demonstrate its use by characterizing and validating a variety of chemical probes for Bruton's tyrosine kinase (BTK, UniprotKB Q10607) and mitogen-activated protein kinase (ERK1/2/MAPK1/2, UniprotKB P28482 and P27361) and determining target engagement of covalent inhibitors for both targets and off-target engagement for ERK. We demonstrated that it works in cell lysates, tissues, and human peripheral blood mononuclear cells. The SMaSh assay is superior to traditional methods and broadly useful as a tool in assessing covalent biological probes or targeted covalent inhibitors.

Published
2021
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5. Labeling Preferences of Diazirines with Protein Biomolecules

Author

Andrew C. Huang, Lyn H. Jones, Giovanni Muncipinto, Christina M. Woo, Hung-Yi Wu, Matthew T Labenski, and Alexander V West

Subjects
Proteome, Protein Conformation, Photoaffinity Labels, 010402 general chemistry, 01 natural sciences, Biochemistry, Catalysis, chemistry.chemical_compound, Colloid and Surface Chemistry, Protein structure, Humans, Reactivity (chemistry), Amino Acids, Alkyl, chemistry.chemical_classification, Binding Sites, Photoaffinity labeling, Chemistry, Biomolecule, Voltage-Dependent Anion Channel 1, Proteins, General Chemistry, Diazonium Compounds, Hydrogen-Ion Concentration, Combinatorial chemistry, 0104 chemical sciences, Amino acid, Diazomethane, Diazirine, Diazo
Abstract

Diazirines are widely used in photoaffinity labeling (PAL) to trap noncovalent interactions with biomolecules. However, design and interpretation of PAL experiments is challenging without a molecular understanding of the reactivity of diazirines with protein biomolecules. Herein, we report a systematic evaluation of the labeling preferences of alkyl and aryl diazirines with individual amino acids, single proteins, and in the whole cell proteome. We find that alkyl diazirines exhibit preferential labeling of acidic amino acids in a pH-dependent manner that is characteristic of a reactive alkyl diazo intermediate, while the aryl-fluorodiazirine labeling pattern reflects reaction primarily through a carbene intermediate. From a survey of 32 alkyl diazirine probes, we use this reactivity profile to rationalize why alkyl diazirine probes preferentially enrich highly acidic proteins or those embedded in membranes and why probes with a net positive charge tend to produce higher labeling yields in cells and in vitro. These results indicate that alkyl diazirines are an especially effective chemistry for surveying the membrane proteome and will facilitate design and interpretation of biomolecular labeling experiments with diazirines.

Published
2021

6. Labeling Preferences of Diazirines with Protein Biomolecules

Author

Alexander West, Giovanni Muncipinto, Hung-Yi Wu, Andrew Huang, Matthew T. Labenski, and Christina Woo

Abstract

Diazirines are widely used in photoaffinity labeling (PAL) to trap non-covalent interactions with biomolecules. However, design and interpretation of PAL experiments is challenging without a molecular understanding of the reactivity of diazirines with protein biomolecules. Here, we report a systematic evaluation of the labeling preferences of alkyl and aryl diazirines with individual amino acids, single proteins, and in the whole cell proteome. We find that aryl-fluorodiazirines react primarily through a carbene intermediate, while alkyl diazirines generate a reactive alkyl diazo intermediate on route to the carbene. The generation of a reactive diazo intermediate leads to preferential labeling of acidic amino acids in a pH-dependent manner. From a survey of 32 alkyl diazirine probes, we use this reactivity profile to rationalize why these probes preferentially enrich highly acidic proteins or those embedded in membranes and why probes with a net positive-charge tend to produce higher labeling yields. These results indicate that alkyl diazirines are an especially effective chemistry for surveying the membrane proteome, and will facilitate probe design and interpretation of biomolecular labeling experiments with diazirines.

Published
2020
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7. Transcriptional and post-translational modifications of B-Raf in quinol-thioether induced tuberous sclerosis renal cell carcinoma

Author

Terrence J. Monks, Ryan Canatsey, Matthew T. Labenski, Nicholas J. Mastrandrea, Serrine S. Lau, and Jennifer D. Cohen

Subjects
0301 basic medicine, MAPK/ERK pathway, Cancer Research, Mutation, Kinase, Biology, medicine.disease_cause, Molecular biology, Proto-Oncogene Proteins B-raf, 03 medical and health sciences, 030104 developmental biology, Protein kinase domain, Cell culture, medicine, Phosphorylation, Proto-Oncogene Proteins c-raf, Molecular Biology
Abstract

Increased activity of B-Raf has been identified in approximately 7% of human cancers. Treatment of Eker rats (Tsc-2(EK/+) ), bearing a mutation in one allele of the tuberous sclerosis-2 (Tsc-2) gene, with the nephrocarcinogen 2,3,5-tris-(glutathion-S-yl) hydroquinone (TGHQ) results in loss of the wild-type allele of Tsc-2 in renal preneoplastic lesions and tumors. These tumors have increased protein expression of B-Raf, C-Raf (Raf-1), and increased expression and activity of ERK kinase. Similar changes are observed in Raf kinases following TGHQ-mediated transformation of primary renal epithelial cells derived from Tsc-2(EK/+) rats (QTRRE cells), cells that are also null for tuberin. Herein, we utilized LC-MS/MS to identify constitutive phosphorylation of S345 and S483 in both 100- and 95-kDa forms of B-Raf in QTRRE cells. Using microRotofor liquid-phase isoelectric focusing, we identified four fractions of B-Raf that contain different post-translational modification profiles in QTRRE cells. Amplification of the kinase domain of B-Raf from QTRRE cells, outer-stripe of the outer medulla of 8-month TGHQ- or vehicle-treated Tsc-2(+/+) and Tsc-2(EK/+) rats, as well as tumors excised from 8-month TGHQ-treated Tsc-2(EK/+) rats revealed three splice variants of B-Raf within the kinase domain. These splice variants differed by approximately 340, 544, and 600 bp; confirmed by sequencing. No point mutations within the kinase domain of B-Raf were identified. In addition, B-Raf/Raf-1/14-3-3 complex formation in the QTRRE cells was decreased by sorafenib, with concomitant selective decreases in p-ERK levels. Transcriptional and post-translational characterization of critical kinases, such as B-Raf, may contribute to the progression of tuberous sclerosis RCC. (246/250) © 2015 Wiley Periodicals, Inc.

Published
2015
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8. Inhibition of Btk with CC-292 Provides Early Pharmacodynamic Assessment of Activity in Mice and Humans

Author

Prasoon Chaturvedi, Erica Evans, Russell Karp, Matthew T. Labenski, Heather Lounsbury, Martin I. Freed, Steven Richard Witowski, Hormoz Mazdiyasni, Richland Wayne Tester, M. Nacht, Sharon Aslanian, Michael Sheets, Russell C. Petter, Juswinder Singh, Zhendong Zhu, Alex Dubrovskiy, and William F. Westlin

Subjects
B-cell receptor, Receptors, Antigen, B-Cell, Pharmacology, Biology, Arthritis, Rheumatoid, Mice, Double-Blind Method, hemic and lymphatic diseases, Agammaglobulinaemia Tyrosine Kinase, medicine, Animals, Humans, Bruton's tyrosine kinase, B cell, Acrylamides, B-Lymphocytes, Drug discovery, breakpoint cluster region, Protein-Tyrosine Kinases, BCR Signaling Pathway, Arthritis, Experimental, Pyrimidines, medicine.anatomical_structure, biology.protein, Molecular Medicine, Signal transduction, Tyrosine kinase, Signal Transduction
Abstract

Targeted therapies that suppress B cell receptor (BCR) signaling have emerged as promising agents in autoimmune disease and B cell malignancies. Bruton's tyrosine kinase (Btk) plays a crucial role in B cell development and activation through the BCR signaling pathway and represents a new target for diseases characterized by inappropriate B cell activity. N-(3-(5-fluoro-2-(4-(2-methoxyethoxy)phenylamino)pyrimidin-4-ylamino)phenyl)acrylamide (CC-292) is a highly selective, covalent Btk inhibitor and a sensitive and quantitative assay that measures CC-292-Btk engagement has been developed. This translational pharmacodynamic assay has accompanied CC-292 through each step of drug discovery and development. These studies demonstrate the quantity of Btk bound by CC-292 correlates with the efficacy of CC-292 in vitro and in the collagen-induced arthritis model of autoimmune disease. Recently, CC-292 has entered human clinical trials with a trial design that has provided rapid insight into safety, pharmacokinetics, and pharmacodynamics. This first-in-human healthy volunteer trial has demonstrated that a single oral dose of 2 mg/kg CC-292 consistently engaged all circulating Btk protein and provides the basis for rational dose selection in future clinical trials. This targeted covalent drug design approach has enabled the discovery and early clinical development of CC-292 and has provided support for Btk as a valuable drug target for B-cell mediated disorders.

Published
2013
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9. Discovery of a Potent and Isoform-Selective Targeted Covalent Inhibitor of the Lipid Kinase PI3Kα

Author

Hormoz Mazdiyasni, Prasoon Chaturvedi, Aravind Prasad Medikonda, Lixin Qiao, Thia St Martin, Juswinder Singh, Russell C. Petter, Deqiang Niu, Zhendong Zhu, William F. Westlin, Michael Sheets, Deepa Bhavsar, Matthew T. Labenski, Russell Karp, and M. Nacht

Subjects
Male, chemistry.chemical_classification, Kinase, Drug design, Molecular biology, Mass Spectrometry, Amino acid, Isoenzymes, Mice, Inbred C57BL, Mice, Phosphatidylinositol 3-Kinases, chemistry, Biochemistry, In vivo, Covalent bond, Drug Discovery, Animals, Molecular Medicine, Transferase, Signal transduction, Nuclear Magnetic Resonance, Biomolecular, Protein Kinase Inhibitors, Phosphoinositide-3 Kinase Inhibitors, Signal Transduction, Cysteine
Abstract

PI3Kα has been identified as an oncogene in human tumors. By use of rational drug design, a targeted covalent inhibitor 3 (CNX-1351) was created that potently and specifically inhibits PI3Kα. We demonstrate, using mass spectrometry and X-ray crystallography, that the selective inhibitor covalently modifies PI3Kα on cysteine 862 (C862), an amino acid unique to the α isoform, and that PI3Kβ, -γ, and -δ are not covalently modified. 3 is able to potently (EC(50) < 100 nM) and specifically inhibit signaling in PI3Kα-dependent cancer cell lines, and this leads to a potent antiproliferative effect (GI(50) < 100 nM). A covalent probe, 8 (CNX-1220), which selectively bonds to PI3Kα, was used to investigate the duration of occupancy of 3 with PI3Kα in vivo. This is the first report of a PI3Kα-selective inhibitor, and these data demonstrate the biological impact of selectively targeting PI3Kα.

Published
2013
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10. The Frequency of 1,4-Benzoquinone-Lysine Adducts in Cytochrome c Correlate with Defects in Apoptosome Activation

Author

John D. Chapman, Shawn B. Bratton, Ashley A. Fisher, Terrence J. Monks, Serrine S. Lau, Srinivas Malladi, and Matthew T. Labenski

Subjects
Models, Molecular, Circular dichroism, Cytochrome, Protein Conformation, Lysine, Toxicology, DNA Adducts, Molecular Toxicology, Tandem Mass Spectrometry, Apoptosomes, Benzoquinones, Animals, Horses, Protein Structure, Quaternary, biology, Caspase 3, Chemistry, Isoelectric focusing, Circular Dichroism, Cytochrome c, Cytochromes c, Isoelectric point, Biochemistry, Coenzyme Q – cytochrome c reductase, biology.protein, Apoptosome, Isoelectric Focusing, Protein Processing, Post-Translational, Chromatography, Liquid
Abstract

Electrophile-mediated post-translational modifications (PTMs) are known to cause tissue toxicities and disease progression. These effects are mediated via site-specific modifications and structural disruptions associated with such modifications. 1,4-Benzoquinone (BQ) and its quinone-thioether metabolites are electrophiles that elicit their toxicity via protein arylation and the generation of reactive oxygen species. Site-specific BQ-lysine adducts are found on residues in cytochrome c that are necessary for protein-protein interactions, and these adducts contribute to interferences in its ability to facilitate apoptosome formation. To further characterize the structural and functional impact of these BQ-mediated PTMs, the original mixture of BQ-adducted cytochrome c was fractionated by liquid isoelectric focusing to provide various fractions of BQ-adducted cytochrome c species devoid of the native protein. The fractionation process separates samples based on their isoelectric point (pI), and because BQ adducts form predominantly on lysine residues, increased numbers of BQ adducts on cytochrome c correlate with a lower protein pI. Each fraction was analyzed for structural changes, and each was also assayed for the ability to support apoptosome-mediated activation of caspase-3. Circular dichroism revealed that several of the BQ-adducted cytochrome c species maintained a slightly more rigid structure in comparison to native cytochrome c. BQ-adducted cytochrome c also failed to activate caspase-3, with increasing numbers of BQ-lysine adducts corresponding to a greater inability to activate the apoptosome. In summary, the specific site of the BQ-lysine adducts, and the nature of the adduct, are important determinants of the subsequent structural changes to cytochrome c. In particular, adducts at sites necessary for protein-protein interactions interfere with the proapoptotic function of cytochrome c.

Published
2011
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11. Carbamate Analogues of Fumagillin as Potent, Targeted Inhibitors of Methionine Aminopeptidase-2

Author

Paolo A. Centrella, Christopher C. Arico-Muendel, Gary M. Olson, Jennifer L Svendsen, Matthew T. Labenski, Steven R. Skinner, Charles D. Thompson, Christopher L. Paradise, Dennis Benjamin, Barbara C. Sluboski, Kenneth E Lind, Brooke D. Contonio, Teresa M Caiazzo, Christopher Self, Gerhard Hannig, Barry A. Morgan, William F. Westlin, Elisabeth Doyle, Charles M. Cook, Kerry White, and Lily Lee Searle

Subjects
Models, Molecular, Methionyl aminopeptidase, Cell Growth Processes, Aminopeptidases, Chemical synthesis, Structure-Activity Relationship, chemistry.chemical_compound, Cyclohexanes, Drug Discovery, medicine, Animals, Humans, Structure–activity relationship, Fumagillin, Amino Acids, Methionine, biology, Endothelial Cells, Metalloendopeptidases, METAP2, chemistry, Biochemistry, Enzyme inhibitor, Fatty Acids, Unsaturated, biology.protein, Molecular Medicine, Cattle, Carbamates, Sesquiterpenes, Lead compound, medicine.drug
Abstract

Inhibition of methionine aminopeptidase-2 (MetAP2) represents a novel approach to antiangiogenic therapy. We describe the synthesis and activity of fumagillin analogues that address the pharmacokinetic and safety liabilities of earlier candidates in this compound class. Two-step elaboration of fumagillol with amines yielded a diverse series of carbamates at C6 of the cyclohexane spiroepoxide. The most potent of these compounds exhibited subnanomolar inhibition of cell proliferation in HUVEC and BAEC assays. Although a range of functionalities were tolerated at this position, alpha-trisubstituted amines possessed markedly decreased inhibitory activity, and this could be rationalized by modeling based on the known fumagillin-MetAP2 crystal structure. The lead compound resulting from these studies, (3R,4S,5S,6R)-5-methoxy-4-((2R,3R)-2-methyl-3-(3-methylbut-2-enyl)oxiran-2-yl)-1-oxaspiro[2.5]octan-6-yl (R)-1-amino-3-methyl-1-oxobutan-2-ylcarbamate, (PPI-2458), demonstrated an improved pharmacokinetic profile relative to the earlier clinical candidate TNP-470, and has advanced into phase I clinical studies in non-Hodgkin's lymphoma and solid cancers.

Published
2009
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12. Protein Electrophile-Binding Motifs: Lysine-Rich Proteins Are Preferential Targets of Quinones

Author

Matthew T. Labenski, Terrence J. Monks, Ashley A. Fisher, Herng Hsiang Lo, and Serrine S. Lau

Subjects
Male, Amino Acid Motifs, Blotting, Western, Lysine, Pharmaceutical Science, Plasma protein binding, Tandem mass spectrometry, Mass Spectrometry, Western blot, medicine, Animals, Amino Acid Sequence, Peptide sequence, Pharmacology, Gel electrophoresis, Molecular Structure, medicine.diagnostic_test, Chemistry, Quinones, Proteins, Articles, Rats, Blot, Biochemistry, Electrophile, Protein Processing, Post-Translational, Chromatography, Liquid, Protein Binding
Abstract

Quinones represent an important class of endogenous compounds such as neurotransmitters and coenzyme Q10, electrophilic xenobiotics, and environmental toxicants that have known reactivity based on their ability to redox cycle and generate oxidative stress, as well as to alkylate target proteins. It is likely that topological, chemical, and physical features combine to determine which proteins become targets for chemical adduction. Chemical-induced post-translational modification of certain critical proteins causes a change in structure/function that contributes to the toxicological response to chemical exposure. In this study, we have identified a number of proteins that are modified by quinone-thioethers after administration of 2-(glutathion-S-yl)HQ. Parallel one-dimensional gel electrophoresis was performed, and the Coomassie-stained gel was aligned with the corresponding Western blot, which was probed for adductions. Immunopositive bands were then subjected to trypsin digestion and analyzed via liquid chromatography/tandem mass spectrometry. The proteins that were subsequently identified contained a higher than average (9.7 versus 5.5%) lysine content and numerous stretches of lysine run-ons, which is a presumed electrophile binding motif. Approximately 50% of these proteins have also been identified as targets for electrophilic adduction by a diverse group of chemicals by other investigators, implying overlapping electrophile adductomes. By identifying a motif targeted by electrophiles it becomes possible to make predictions of proteins that may be targeted for adduction and possible sites on these proteins that are adducted. An understanding of proteins targeted for adduction is essential to unraveling the toxicity produced by these electrophiles.

Published
2009
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13. An inhibitor of methionine aminopeptidase type-2, PPI-2458, ameliorates the pathophysiological disease processes of rheumatoid arthritis

Author

A. B. Rogers, Matthew T. Labenski, E. G. Doyle, E. J. Clark, D. D. Lazarus, R. M. Karp, W. F. Westlin, G. Hannig, S. G. Bernier, J. D. Wakefield, J. Lorusso, Charles D. Thompson, and J. G. Hoyt

Subjects
medicine.medical_specialty, Immunology, Osteoclasts, Arthritis, Disease, Pharmacology, Aminopeptidases, Aminopeptidase, Arthritis, Rheumatoid, Mice, Osteoclast, Internal medicine, medicine, Animals, Protease Inhibitors, Bone Resorption, Cells, Cultured, Clinical pathology, business.industry, Body Weight, Metalloendopeptidases, Cell Differentiation, Valine, medicine.disease, Pathophysiology, Rheumatology, Rats, medicine.anatomical_structure, Rats, Inbred Lew, Rheumatoid arthritis, Epoxy Compounds, Female, Joints, business
Abstract

To elucidate the role of methionine aminopeptidase type-2 (MetAP-2) in the clinical pathology of rheumatoid arthritis, arthritis was induced in rats by administration of peptidoglycan-polysaccharide (PG-PS).The inhibitor of MetAP-2, PPI-2458, was administered orally at 5 mg/kg every other day during 3 distinct phases of the disease. In vitro studies were performed to clarify in vivo findings.Ankle swelling was completely alleviated by MetAP-2 inhibition. Inhibition of MetAP-2 in blood and tissues correlated with protection against PG-PS-induced arthritis. Histopathology of the tarsal joints improved following PPI-2458 administration, including a significant improvement of bone structure. In in vitro studies, osteoclast formation and activity were inhibited by PPI-2458, a mechanism not previously attributed to MetAP-2 inhibition.The important role that MetAP-2 has in the pathophysiological disease processes of PG-PS arthritis provides a strong rationale for evaluating PPI-2458 as a disease modifying antirheumatic treatment for rheumatoid arthritis.

Published
2008
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14. A Novel Methionine Aminopeptidase-2 Inhibitor, PPI-2458, Inhibits Non–Hodgkin's Lymphoma Cell Proliferation In vitro and In vivo

Author

Matthew T. Labenski, Edward Clark, Michael J. Murray, Nazbeh Taghizadeh, William F. Westlin, Russell Karp, Andrew C. Cooper, Gerhard Hannig, Jennifer G. Hoyt, and Charles D. Thompson

Subjects
Cancer Research, medicine.medical_specialty, Lymphoma, B-Cell, Time Factors, Blotting, Western, Spleen, Mice, SCID, Biology, Aminopeptidases, Mice, In vivo, Cell Line, Tumor, Internal medicine, medicine, Animals, Humans, Lymphocyte Count, Fumagillin, Cell Proliferation, B-Lymphocytes, Dose-Response Relationship, Drug, Cell growth, Lymphoma, Non-Hodgkin, Metalloendopeptidases, Germinal center, Valine, Germinal Center, medicine.disease, Xenograft Model Antitumor Assays, In vitro, METAP2, Non-Hodgkin's lymphoma, Macaca fascicularis, medicine.anatomical_structure, Endocrinology, Proto-Oncogene Proteins c-bcl-2, Oncology, Cancer research, Epoxy Compounds, Female, medicine.drug
Abstract

Purpose: Fumagillin and related compounds have potent antiproliferative activity through inhibition of methionine aminopeptidase-2 (MetAP-2). It has recently been reported that MetAP-2 is highly expressed in germinal center B cells and germinal center–derived non–Hodgkin's lymphomas (NHL), suggesting an important role for MetAP-2 in proliferating B cells. Therefore, we determined the importance of MetAP-2 in normal and transformed germinal center B cells by evaluating the effects of MetAP-2 inhibition on the form and function of germinal centers and germinal center–derived NHL cells. Experimental Design: To examine the activity of PPI-2458 on germinal center morphology, spleen sections from cynomolgus monkeys treated with oral PPI-2458 were analyzed. Antiproliferative activity of PPI-2458 was assessed on germinal center–derived NHL lines in culture. A MetAP-2 pharmacodynamic assay was used to determine cellular MetAP-2 inhibition following PPI-2458 treatment. Finally, inhibition of MetAP-2 and proliferation by PPI-2458 was examined in the human SR NHL line in culture and in implanted xenografts. Results: Oral PPI-2458 caused a reduction in germinal center size and number in lymphoid tissues from treated animals. PPI-2458 potently inhibited growth (GI50 = 0.2-1.9 nmol/L) of several NHL lines in a manner that correlated with MetAP-2 inhibition. Moreover, orally administered PPI-2458 significantly inhibited SR tumor growth, which correlated with inhibition of tumor MetAP-2 (>85% at 100 mg/kg) in mice. Conclusions: These results show the potent antiproliferative activity of PPI-2458 on NHL lines in vitro and oral antitumor activity in vivo and suggest the therapeutic potential of PPI-2458 as a novel agent for treatment of NHL should be evaluated in the clinical setting.

Published
2006
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15. S-adenosyl-l-methionine protection of acetaminophen mediated oxidative stress and identification of hepatic 4-hydroxynonenal protein adducts by mass spectrometry

Author

Monica A. Valentovic, Serrine S. Lau, Matthew T. Labenski, Christopher L. Kuhlman, James Mike Brown, Andre Benja Lamyaithong, John G. Ball, and Marcus V. Terneus

Subjects
Male, S-Adenosylmethionine, Protein Carbonylation, Sarcosine Dehydrogenase, Carbamoyl-Phosphate Synthase (Ammonia), Mitochondria, Liver, Mitochondrion, Pharmacology, Toxicology, medicine.disease_cause, Antioxidants, Article, chemistry.chemical_compound, Tandem Mass Spectrometry, Carbamoyl phosphate, medicine, Animals, Acetaminophen, Aldehydes, Mice, Inbred BALB C, Methionine, Chemistry, digestive, oral, and skin physiology, Disease Models, Animal, Oxidative Stress, Biochemistry, Sarcosine dehydrogenase, Liver, Cytoprotection, Toxicity, Chemical and Drug Induced Liver Injury, Protein Processing, Post-Translational, Oxidative stress, medicine.drug, Chromatography, Liquid
Abstract

Acetaminophen (APAP) hepatotoxicity is protected by S-adenosyl-L-methionine (SAMe) treatment 1 hour (h) after APAP in C57/Bl6 mice. This study examined protein carbonylation as well as mitochondrial and cytosolic protein adduction by 4-hydroxynonenal (4-HNE) using mass spectrometry (MS) analysis. Additional studies investigated the leakage of mitochondrial proteins and 4-HNE adduction of these proteins. Male C57/Bl6 mice (n=5/group) were divided into the following groups and treated as indicated: Veh (15 ml/kg water, ip), SAMe (1.25 mmol/kg, ip), APAP (250 mg/kg), and SAMe given 1 h after APAP (S+A). APAP toxicity was confirmed by an increase (p

Published
2014

16. In vitro and in vivo characterization of irreversible mutant-selective EGFR inhibitors that are wild-type sparing

Author

Annette O Walter, Michael Sheets, Thia St Martin, Henry J. Haringsma, Zhendong Zhu, Andrew R. Allen, Robert Tjin Tham Sjin, Deqiang Niu, Mitch Raponi, Russell C. Petter, Prasoon Chaturvedi, Kwangho Lee, Yixuan Ren, Thomas C. Harding, M. Nacht, Aleksandr Dubrovskiy, Aravind Prasad Medikonda, Richland Wayne Tester, Russell Karp, Matthew T. Labenski, Andrew D Simmons, Juswinder Singh, William F. Westlin, and Jeff Etter

Subjects
Cancer Research, Pharmacology, In Vitro Techniques, T790M, Mice, Gefitinib, In vivo, Carcinoma, Non-Small-Cell Lung, Cell Line, Tumor, medicine, Animals, Humans, Epidermal growth factor receptor, 4-Aminopyridine, EGFR inhibitors, Cell Proliferation, Clinical Trials as Topic, biology, business.industry, Wild type, Xenograft Model Antitumor Assays, In vitro, respiratory tract diseases, ErbB Receptors, Oncology, Drug Resistance, Neoplasm, Mutation, biology.protein, Erlotinib, Neoplasm Recurrence, Local, business, medicine.drug
Abstract

Patients with non–small cell lung carcinoma (NSCLC) with activating mutations in epidermal growth factor receptor (EGFR) initially respond well to the EGFR inhibitors erlotinib and gefitinib. However, all patients relapse because of the emergence of drug-resistant mutations, with T790M mutations accounting for approximately 60% of all resistance. Second-generation irreversible EGFR inhibitors are effective against T790M mutations in vitro, but retain affinity for wild-type EGFR (EGFRWT). These inhibitors have not provided compelling clinical benefit in T790M-positive patients, apparently because of dose-limiting toxicities associated with inhibition of EGFRWT. Thus, there is an urgent clinical need for therapeutics that overcome T790M drug resistance while sparing EGFRWT. Here, we describe a lead optimization program that led to the discovery of four potent irreversible 2,4-diaminopyrimidine compounds that are EGFR mutant (EGFRmut) selective and have been designed to have low affinity for EGFRWT. Pharmacokinetic and pharmacodynamic studies in H1975 tumor–bearing mice showed that exposure was dose proportional resulting in dose-dependent EGFR modulation. Importantly, evaluation of normal lung tissue from the same animals showed no inhibition of EGFRWT. Of all the compounds tested, compound 3 displayed the best efficacy in EGFRL858R/T790M-driven tumors. Compound 3, now renamed CO-1686, is currently in a phase I/II clinical trial in patients with EGFRmut-advanced NSCLC that have received prior EGFR-directed therapy. Mol Cancer Ther; 13(6); 1468–79. ©2014 AACR.

Published
2014

17. Selective irreversible inhibition of a protease by targeting a noncatalytic cysteine

Author

Thia St. Martin, Hugues Bernard, Deqiang Niu, Margit Hagel, Michael Sheets, Zhendong Zhu, Lixin Qiao, Mariana Nacht, Matthew T. Labenski, Prasoon Chaturvedi, Russell Karp, William F. Westlin, Petter Russell C, and Juswinder Singh

Subjects
Proteases, Protease, Chemistry, medicine.medical_treatment, A protein, Hepacivirus, Cell Biology, Cysteine Proteinase Inhibitors, Crystallography, X-Ray, Biochemistry, chemistry.chemical_compound, Drug Design, Virology, Hcv protease, Biocatalysis, medicine, Cysteine, Pharmacophore, Oligopeptides, Molecular Biology, Cysteine metabolism
Abstract

Designing selective inhibitors of proteases has proven problematic, in part because pharmacophores that confer potency exploit the conserved catalytic apparatus. We developed a fundamentally different approach by designing irreversible inhibitors that target noncatalytic cysteines that are structurally unique to a target in a protein family. We have successfully applied this approach to the important therapeutic target HCV protease, which has broad implications for the design of other selective protease inhibitors.

Published
2010
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18. Discovery of a mutant-selective covalent inhibitor of EGFR that overcomes T790M-mediated resistance in NSCLC

Author

Aleksander Dubrovskiy, Prasoon Chaturvedi, Annette O Walter, Deqiang Niu, Kadoaki Ohashi, Michael Sheets, Andrew E. Allen, M. Nacht, Terry Van Dyke, Thomas Harding, Zoe Weaver, Mitch Raponi, Jing Sun, William Pao, Kwangho Lee, Zhendong Zhu, William F. Westlin, Dan van Kalken, Russell C. Petter, Thia St Martin, Matthew T. Labenski, Russell Karp, Henry J. Haringsma, Robert Tjin Tham Sjin, Zhigang Wang, Andrew Simmons, Sarah Jaw-Tsai, Kevin K. Lin, Juswinder Singh, and Jeff Etter

Subjects
Epithelial-Mesenchymal Transition, Lung Neoplasms, Mutant, Administration, Oral, Mice, Nude, Antineoplastic Agents, Mice, Transgenic, medicine.disease_cause, Article, T790M, Mice, Carcinoma, Non-Small-Cell Lung, Cell Line, Tumor, medicine, Animals, Humans, Rociletinib, Epithelial–mesenchymal transition, Epidermal growth factor receptor, Molecular Targeted Therapy, Protein Kinase Inhibitors, Cell Proliferation, Mutation, Acrylamides, Mice, Inbred BALB C, biology, Cell growth, Kinase, Molecular biology, Xenograft Model Antitumor Assays, respiratory tract diseases, ErbB Receptors, HEK293 Cells, Pyrimidines, Oncology, Drug Resistance, Neoplasm, biology.protein, Female, Mutant Proteins, Drug Screening Assays, Antitumor
Abstract

Patients with non–small cell lung cancer (NSCLC) with activating EGF receptor (EGFR) mutations initially respond to first-generation reversible EGFR tyrosine kinase inhibitors. However, clinical efficacy is limited by acquired resistance, frequently driven by the EGFRT790M mutation. CO-1686 is a novel, irreversible, and orally delivered kinase inhibitor that specifically targets the mutant forms of EGFR, including T790M, while exhibiting minimal activity toward the wild-type (WT) receptor. Oral administration of CO-1686 as single agent induces tumor regression in EGFR-mutated NSCLC tumor xenograft and transgenic models. Minimal activity of CO-1686 against the WT EGFR receptor was observed. In NSCLC cells with acquired resistance to CO-1686 in vitro, there was no evidence of additional mutations or amplification of the EGFR gene, but resistant cells exhibited signs of epithelial–mesenchymal transition and demonstrated increased sensitivity to AKT inhibitors. These results suggest that CO-1686 may offer a novel therapeutic option for patients with mutant EGFR NSCLC. Significance: We report the preclinical development of a novel covalent inhibitor, CO-1686, that irreversibly and selectively inhibits mutant EGFR, in particular the T790M drug-resistance mutation, in NSCLC models. CO-1686 is the first drug of its class in clinical development for the treatment of T790M-positive NSCLC, potentially offering potent inhibition of mutant EGFR while avoiding the on-target toxicity observed with inhibition of the WT EGFR. Cancer Discov; 3(12); 1404–15. ©2013 AACR. This article is highlighted in the In This Issue feature, p. 1317

Published
2013

19. Metabolites of PPI-2458, a selective, irreversible inhibitor of methionine aminopeptidase-2: structure determination and in vivo activity

Author

Gary K. O’Donovan, Steven R. Skinner, Barry A. Morgan, Bruce Belanger, Matthew T. Labenski, Kerry White, Dennis Benjamin, Paolo A. Centrella, Elisabeth Doyle, Heather S. Blanchette, Ulrike Gradhand, Nazbeh Taghizadeh, Sarah T Griffin, Teresa M Caiazzo, Kavirayani R. Prasad, James Wakefield, William F. Westlin, Jennifer L. DeLorey, Susan E. Hill, Charles D. Thompson, and Christopher C. Arico-Muendel

Subjects
Pharmaceutical Science, Angiogenesis Inhibitors, Thymus Gland, Pharmacology, Aminopeptidases, Drug Administration Schedule, chemistry.chemical_compound, Structure-Activity Relationship, In vivo, medicine, Leukocytes, Animals, Humans, Fumagillin, Methionine, biology, Lymphoma, Non-Hodgkin, Cytochrome P450, Metalloendopeptidases, Valine, In vitro, METAP2, Rats, Metabolic pathway, chemistry, Biochemistry, biology.protein, Microsomes, Liver, Epoxy Compounds, Lymph Nodes, Ex vivo, medicine.drug
Abstract

The natural product fumagillin exhibits potent antiproliferative and antiangiogenic properties. The semisynthetic analog PPI-2458, [(3R,4S,5S,6R)-5-methoxy-4-[(2R,3R)-2-methyl-3-(3-methylbut-2-enyl)oxiran-2-yl]-1-oxaspiro[2.5]octan-6-yl] N-[(2R)-1-amino-3-methyl-1-oxobutan-2-yl]carbamate, demonstrates rapid inactivation of its molecular target, methionine aminopeptidase-2 (MetAP2), and good efficacy in several rodent models of cancer and inflammation with oral dosing despite low apparent oral bioavailability. To probe the basis of its in vivo efficacy, the metabolism of PPI-2458 was studied in detail. Reaction phenotyping identified CYP3A4/5 as the major source of metabolism in humans. Six metabolites were isolated from liver microsomes and characterized by mass spectrometry and nuclear resonance spectroscopy, and their structures were confirmed by chemical synthesis. The synthetic metabolites showed correlated inhibition of MetAP2 enzymatic activity and vascular endothelial cell growth. In an ex vivo experiment, MetAP2 inhibition in white blood cells, thymus, and lymph nodes in rats after single dosing with PPI-2458 and the isolated metabolites was found to correlate with the in vitro activity of the individual species. In a phase 1 clinical study, PPI-2458 was administered to patients with non-Hodgkin lymphoma. At 15 mg administered orally every other day, MetAP2 in whole blood was 80% inactivated for up to 48 hours, although the exposure of the parent compound was only ∼10% that of the summed cytochrome P450 metabolites. Taken together, the data confirm the participation of active metabolites in the in vivo efficacy of PPI-2458. The structures define a metabolic pathway for PPI-2458 that is distinct from that of TNP-470 ([(3R,4S,5S,6R)-5-methoxy-4-[(2R,3R)-2-methyl-3-(3-methylbut-2-enyl)oxiran-2-yl]-1-oxaspiro[2.5]octan-6-yl] N-(2-chloroacetyl)carbamate). The high level of MetAP2 inhibition achieved in vivo supports the value of fumagillin-derived therapeutics for angiogenic diseases.

Published
2013

20. Orally active fumagillin analogues: transformations of a reactive warhead in the gastric environment

Author

Teresa M. Caiazzo, Elisabeth G. Doyle, Steven R. Johnson, Christopher C. Arico-Muendel, Dennis R. Benjamin, Charles D. Thompson, Gary O’Donovan, Steven Skinner, Amy A. Sarjeant, Sarah T. Griffin, Matthew T. Labenski, Barry Morgan, Paolo A. Centrella, Kerry White, Jennifer DeLorey, Heather Blanchette, and William Westlin

Subjects
Methionine, Stereochemistry, Organic Chemistry, Diol, Epoxide, Biology, Biochemistry, METAP2, chemistry.chemical_compound, chemistry, Covalent bond, Drug Discovery, medicine, Fumagillin, Target protein, Ex vivo, medicine.drug
Abstract

Semisynthetic analogues of fumagillin, 1, inhibit methionine aminopeptidase-2 (MetAP2) and have entered the clinic for the treatment of cancer. An optimized fumagillin analogue, 3 (PPI-2458), was found to be orally active, despite containing a spiroepoxide function that formed a covalent linkage to the target protein. In aqueous acid, 3 underwent ring-opening addition of water and HCl, leading to four products, 4-7, which were characterized in detail. The chlorohydrin, but not the diol, products inhibited MetAP2 under weakly basic conditions, suggesting reversion to epoxide as a step in the mechanism. In agreement, chlorohydrin 6 was shown to revert rapidly to 3 in rat plasma. In an ex vivo assay, rats treated with purified acid degradants demonstrated inhibition of MetAP2 that correlated with the biochemical activity of the compounds. Taken together, the results indicate that degradation of the parent compound was compensated by the formation of active equivalents leading to a pharmacologically useful level of MetAP2 inhibition.

Published
2012

21. Identification of Chemical-Adducted Proteins in Urine by Multi-dimensional Protein Identification Technology (LC/LC–MS/MS)

Author

Matthew T. Labenski, Ashley A. Fisher, Serrine S. Lau, and Terrence J. Monks

Subjects
chemistry.chemical_classification, Lysis, Statistics as Topic, Reproducibility of Results, Peptide, Mass spectrometry, Tandem mass spectrometry, High-performance liquid chromatography, Article, Hydroquinones, Rats, Adduct, Proteinuria, Biochemistry, chemistry, Tandem Mass Spectrometry, Nat, Proteome, Animals, Databases, Protein, Protein Processing, Post-Translational, Chromatography, Liquid
Abstract

Recent technological advancements in mass spectrometry facilitate the detection of chemical-induced posttranslational modifications (PTMs) that may alter cell signaling pathways or alter the structure and function of the modified proteins. To identify such protein adducts (Kleiner et al., Chem Res Toxicol 11:1283–1290, 1998), multi-dimensional protein identification technology (MuDPIT) has been utilized. MuDPIT was first described by Link et al. as a new technique useful for protein identification from a complex mixture of proteins (Link et al., Nat Biotechnol 17:676–682, 1999). MuDPIT utilizes two different HPLC columns to further enhance peptide separation, increasing the number of peptide hits and protein coverage. The technology is extremely useful for proteomes, such as the urine proteome, samples from immunoprecipitations, and 1D gel bands resolved from a tissue homogenate or lysate. In particular, MuDPIT has enhanced the field of adduct hunting for adducted peptides, since it is more capable of identifying lesser abundant peptides, such as those that are adducted, than the more standard LC–MS/MS. The site-specific identification of covalently adducted proteins is a prerequisite for understanding the biological significance of chemical-induced PTMs and the subsequent toxicological response they elicit.

Published
2010
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22. Utilization of LC-MS/MS Analyses to Identify Site-Specific Chemical Protein Adducts In Vitro

Author

Ashley A. Fisher, Matthew T. Labenski, Serrine S. Lau, and Terrence J. Monks

Subjects
Binding Sites, Chemistry, Molecular Sequence Data, Reactive intermediate, Lysine, Cytochromes c, Proteins, Tandem mass spectrometry, Article, Substrate Specificity, Xenobiotics, Adduct, Biochemistry, Tandem Mass Spectrometry, Electrophile, Benzoquinones, Animals, Amino Acid Sequence, Target protein, Binding site, Protein Processing, Post-Translational, Peptide sequence, Chromatography, Liquid
Abstract

Biologically reactive intermediates are formed following metabolism of xenobiotics, and during normal oxidative metabolism. These reactive species are electrophilic in nature and are capable of forming stable adducts with target proteins. These covalent protein modifications can initiate processes that lead to acute tissue injury or chronic disease. Recent advancements in mass spectrometry techniques and data analysis has permitted a more detailed investigation of site-specific protein modifications by reactive electrophiles. Knowledge from such analyses will assist in providing a better understanding of how specific classes of electrophiles produce toxicity and disease progression via site-selective protein-specific covalent modification. Hydroquinone (HQ) is a known environmental toxicant, and its quinone–thioether metabolites, formed via the intermediate generation of 1,4-benzoquinone (1,4-BQ), elicit their toxic response via the covalent modification of target proteins and the generation of reactive oxygen species. We have utilized a model protein, cytochrome c, to guide us in identifying 1,4-BQ- and 1,4-BQ-thioether derived site-specific protein modifications. LC-MS/MS analyses reveals that these modifications occur selectively on lysine and glutamic acid residues of the target protein, and that these modifications occur within identifiable “electrophile binding motifs” within the protein. These motifs are found within lysine-rich regions of the protein and appear to be target sites of 1,4-BQ-thioether adduction. These residues also appear to dictate the nature of post-adduction chemistry and the final structure of the adduct. This model system will provide critical insight for in vivo adduct hunting following exposure to 1,4-BQ-thioethers, but the general approaches can also be extended to the identification of protein adducts derived from other classes of reactive electrophiles.

Published
2010
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23. Utilization of MALDI-TOF to Determine Chemical-Protein Adduct Formation In Vitro

Author

Ashley A. Fisher, Terrence J. Monks, Matthew T. Labenski, and Serrine S. Lau

Subjects
Metabolite, Reactive intermediate, medicine.disease_cause, Article, Substrate Specificity, chemistry.chemical_compound, medicine, Animals, Amino Acid Sequence, biology, Cytochrome c, Proteins, Metabolism, Protein tertiary structure, Hydroquinones, Quinone, Pharmaceutical Preparations, chemistry, Biochemistry, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, biology.protein, Cattle, Peptides, Xenobiotic, Protein Processing, Post-Translational, Oxidative stress
Abstract

Biological reactive intermediates can be created via metabolism of xenobiotics during the process of chemical elimination. They can also be formed as by-products of cellular metabolism, which produces reactive oxygen and nitrogen species. These reactive intermediates tend to be electrophilic in nature, which enables them to interact with tissue macromolecules, disrupting cellular signaling processes and often producing acute and chronic toxicities. Quinones are a well-known class of electrophilic species. Many natural products contain quinones as active constituents, and the quinone moiety exists in a number of chemotherapeutic agents. Quinones are also frequently formed as electrophilic metabolites from a variety of xeno- and endobiotics. Hydroquinone (HQ) is present in the environment from various sources, and it is also a known metabolite of benzene. HQ is converted in the body to 1,4-benzoqui-none, which subsequently gives rise to hematotoxic and nephrotoxic quinone–thioether metabolites. The toxicity of these metabolites is dependent upon their ability to arylate proteins and to produce oxidative stress. Protein tertiary structure and protein amino acid sequence combine to determine which proteins are targets of these electrophilic quinone–thioether metabolites. We have used cytochrome c and model peptides to view adduction profiles of quinone–thioether metabolites, and have determined by MALDI-TOF analysis that these electrophiles target specific residues within these model systems.

Published
2010
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24. One-Dimensional Western Blotting Coupled to LC-MS/MS Analysis to Identify Chemical-Adducted Proteins in Rat Urine

Author

Ashley A. Fisher, Serrine S. Lau, Terrence J. Monks, and Matthew T. Labenski

Subjects
Blotting, Western, Statistics as Topic, Article, Adduct, chemistry.chemical_compound, Western blot, Tandem Mass Spectrometry, medicine, Animals, Electrophoresis, Gel, Two-Dimensional, Hydroquinone, biology, medicine.diagnostic_test, Glutathione, Hydroquinones, Rats, Blot, Proteinuria, chemistry, Biochemistry, Covalent bond, biology.protein, Electrophoresis, Polyacrylamide Gel, Environmental Pollutants, Antibody, Protein Processing, Post-Translational, Chromatography, Liquid, Toxicant
Abstract

The environmental toxicant hydroquinone (HQ) and its glutathione conjugates (GSHQs) cause renal cell necrosis via a combination of redox cycling and the covalent adduction of proteins within the S3 segment of the renal proximal tubules in the outer stripe of the outer medulla (OSOM). Following administration of 2-(glutathion-S-yl)HQ (MGHQ) (400 µmol/kg, i.v., 2 h) to Long Evans (wild-type Eker) rats, Western analysis utilizing an antibody specific for quinol–thioether metabolites of HQ revealed the presence of large amounts of chemical–protein adducts in both the OSOM and urine. By aligning the Western blot film with a parallel gel stained for protein, we can isolate the adducted proteins for LC-MS/MS analysis. Subsequent database searching can identify the specific site(s) of chemical adduction within these proteins. Finally, a combination of software programs can validate the identity of the adducted peptides. The site-specific identification of covalently adducted and oxidized proteins is a prerequisite for understanding the biological significance of chemical-induced posttranslational modifications (PTMs) and their toxicological significance.

Published
2010
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25. Binary selectivity for HCV NS3/4A protease versus host proteases via irreversible inactivation at a non‐catalytic cysteine

Author

Juswinder Singh, Thia St. Martin, Deqiang Niu, Matthew T. Labenski, Petter Russell C, Zhendong Zhu, Mariana Nacht, Michael Sheets, Hugues Bernhard, Russell Karp, Prasson Chaturvedi, Margit Hagel, William F. Westlin, and Lixin Qiao

Subjects
Proteases, Protease, Host (biology), Chemistry, medicine.medical_treatment, Biochemistry, Genetics, medicine, Non catalytic, Selectivity, Molecular Biology, Biotechnology, Cysteine
Published
2010
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28. Quinone electrophiles selectively adduct 'electrophile binding motifs' within cytochrome c

Author

Rania S. Milleron, Ashley A. Fisher, Terrence J. Monks, Srinivas Malladi, Vijay Gokhale, Serrine S. Lau, Martina E. Bowen, Matthew T. Labenski, and Shawn B. Bratton

Subjects
Models, Molecular, Cytochrome, Stereochemistry, Protein Conformation, Amino Acid Motifs, Molecular Sequence Data, Biochemistry, Protein Structure, Secondary, Nucleophile, Tandem Mass Spectrometry, Apoptosomes, Cell Line, Tumor, Benzoquinones, Animals, Humans, Amino Acid Sequence, Horses, Mercapturic acid, biology, Molecular Structure, Chemistry, Caspase 3, Cytochrome c, Circular Dichroism, Cytochromes c, Glutamic acid, Hydrogen-Ion Concentration, Benzoquinone, Caspase 9, Quinone, Acetylcysteine, Protein Structure, Tertiary, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Electrophile, biology.protein, Chromatography, Liquid, Protein Binding
Abstract

Electrophiles generated endogenously, or via the metabolic bioactivation of drugs and other environmental chemicals, are capable of binding to a variety of nucleophilic sites within proteins. Factors that determine site selective susceptibility to electrophile-mediated post-translational modifications, and the consequences of such alterations, remain largely unknown. To identify and characterize chemical-mediated protein adducts, electrophiles with known toxicity were utilized. Hydroquinone, and its mercapturic acid pathway metabolites, cause renal proximal tubular cell necrosis and nephrocarcinogenicity in rats. The adverse effects of HQ and its thioether metabolites are in part a consequence of their oxidation to the corresponding electrophilic 1,4-benzoquinones (BQ). We now report that BQ and 2-(N-acetylcystein-S-yl)benzoquinone (NAC-BQ) preferentially bind to solvent-exposed lysine-rich regions within cytochrome c. Furthermore, we have identified specific glutamic acid residues within cytochrome c as novel sites of NAC-BQ adduction. The microenvironment at the site of adduction governs both the initial specificity and the structure of the final adduct. The solvent accessibility and local pKa of the adducted and neighboring amino acids contribute to the selectivity of adduction. Postadduction chemistry subsequently alters the nature of the final adduct. Using molecular modeling, the impact of BQ and NAC-BQ adduction on cytochrome c was visualized, revealing the spatial rearrangement of critical residues necessary for protein-protein interactions. Consequently, BQ-adducted cytochrome c fails to initiate caspase-3 activation in native lysates and also inhibits Apaf-1 oligomerization into an apoptosome complex in a purely reconstituted system. In summary, a combination of mass spectroscopic, molecular modeling, and biochemical approaches confirms that electrophile-protein adducts produce structural alterations that influence biological function.

Published
2007

29. Inhibition of melanoma tumor growth by a pharmacological inhibitor of MetAP-2, PPI-2458

Author

Gerhard, Hannig, Douglas D, Lazarus, Sylvie G, Bernier, Russell M, Karp, Jeanine, Lorusso, Daniel, Qiu, Matthew T, Labenski, Jim D, Wakefield, Charles D, Thompson, and William F, Westlin

Subjects
Cyclin-Dependent Kinase Inhibitor p21, Male, Melanins, Dose-Response Relationship, Drug, Blotting, Western, Melanoma, Experimental, Administration, Oral, Valine, Aminopeptidases, Cell Line, Mice, Inbred C57BL, Mice, Cell Line, Tumor, Animals, Epoxy Compounds, Humans, Methionyl Aminopeptidases, Cell Proliferation, Glycoproteins
Abstract

Over the past few decades, melanoma has shown the fastest growing incidence rate of all cancers. This malignancy is clinically defined by its potential to rapidly metastasize, and advanced metastatic melanomas are highly resistant to existing therapeutic regimens. Here, we report that PPI-2458, a novel, orally active agent of the fumagillin class of irreversible methionine aminopeptidase-2 (MetAP-2) inhibitors, potently inhibited the proliferation of B16F10 melanoma cells in vitro, with a growth inhibitory concentration 50% (GI50) of 0.2 nM. B16F10 growth inhibition was correlated with the inhibition of MetAP-2 enzyme, in a dose-dependent fashion, as determined by a pharmacodynamic assay, which measures the amount of uninhibited MetAP-2 following PPI-2458 treatment. Prolonged exposure of B16F10 cells to PPI-2458 at concentrations of up to 1 microM, 5,000-fold above the GI50, did not alter their sensitivity to PPI-2458 growth inhibition and no drug resistance was observed. Moreover, prolonged exposure to this agent induced melanogenesis, concomitant with the elevated expression of the melanocyte-specific enzymes tyrosinase and tyrosinase-related proteins (TRP) 1 and 2, a morphological feature associated with differentiated melanocytes. PPI-2458, when administered orally (p.o.), significantly inhibited B16F10 tumor growth in mice in a dose-dependent fashion, with a maximum inhibition of 62% at 100 mg/kg. This growth inhibition was directly correlated to the amount of irreversibly inhibited MetAP-2 (80% at 100 mg/kg PPI-2458) in tumor tissue. These data demonstrate that PPI-2458 has potent antiproliferative activity against B16F10 cells in vitro and in vivo, and that both activities are directly correlated with levels of MetAP-2 enzyme inhibition. This antiproliferative activity, coupled with additional observations from studies in vitro (absence of detectable resistance to PPI-2458 and induction of morphological features consistent with differentiated melanocytes), provides a rationale for assessing the therapeutic potential of PPI-2458 in the treatment of melanoma.

Published
2006

32. A methionine aminopeptidase-2 inhibitor, PPI-2458, for the treatment of rheumatoid arthritis

Author

Matthew T. Labenski, William F. Westlin, Edward A. Clark, Douglas Lazarus, Gerhard Hannig, Charles D. Thompson, Sylvie G. Bernier, and Beth Doyle

Subjects
Anti-Inflammatory Agents, Arthritis, Down-Regulation, Pharmacology, Aminopeptidases, Umbilical vein, Arthritis, Rheumatoid, chemistry.chemical_compound, In vivo, Cyclohexanes, Proliferating Cell Nuclear Antigen, medicine, Animals, Humans, Fumagillin, Enzyme Inhibitors, Cells, Cultured, Multidisciplinary, Synovial Membrane, Endothelial Cells, Metalloendopeptidases, Valine, Biological Sciences, medicine.disease, METAP2, Rats, Vascular endothelial growth factor, medicine.anatomical_structure, chemistry, Antirheumatic Agents, Immunology, Fatty Acids, Unsaturated, Epoxy Compounds, Growth inhibition, Synovial membrane, Sesquiterpenes, Cell Division, medicine.drug
Abstract

The hallmark of rheumatoid arthritis (RA) is the progressive destruction of articular joints, characterized by invasive synovial hyperplasia and pathological neovascularization. Here we report that PPI-2458, a member of the fumagillin class of irreversible methionine aminopeptidase-2 (MetAP-2) inhibitors, potently inhibits the proliferation of human fibroblast-like synoviocytes (HFLS-RA), derived from RA patients, with a growth inhibitory concentration 50 (GI50) of 0.04 nM and a maximum inhibition of >95% at 1 nM. Human umbilical vein endothelial cells (HUVEC) are similarly inhibited in proliferation by PPI-2458 (GI50, 0.2 nM). We developed a method to measure the level of MetAP-2 enzyme inhibition after exposure to PPI-2458 and demonstrate that growth inhibition of PPI-2458-sensitive HFLS-RA and HUVEC is linked to MetAP-2 enzyme inhibition, in a dose-dependent fashion. The secretion of several inflammatory mediators such as IL-6 and vascular endothelial growth factor from activated HFLS-RA was not inhibited by PPI-2458. The CNS toxicity profile of PPI-2458, determined by the incidence of seizures, is significantly improved over that of the parental compound TNP-470. In the rat model of peptidoglycan–polysaccharide-induced arthritis, PPI-2458 significantly attenuated paw swelling when therapeutically administered after the onset of chronic disease. We suggest that the mechanism of PPI-2458 action, highly selective and potent anti-proliferative activity on HFLS-RA and HUVECin vitro, a significantly improved CNS toxicity profile, and marked attenuation of chronic disease in the rat peptidoglycan–polysaccharide arthritis modelin vivo, positions this compound as a drug for the treatment of RA.

Published
2004

34. 93 Selective inhibition of PI3K alpha using a novel covalent compound

Author

Deqiang Niu, Matthew T. Labenski, T.St. Martin, Russell C. Petter, M. Nacht, Michael Sheets, Lixin Qiao, Juswinder Singh, Prasoon Chaturvedi, and William F. Westlin

Subjects
Cancer Research, Oncology, Covalent bond, Stereochemistry, Chemistry, Alpha (ethology), Selective inhibition, PI3K/AKT/mTOR pathway
Published
2010
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35. 764 AVL-181, A POTENT AND SELECTIVE IRREVERSIBLE HCV PROTEASE INHIBITOR, REQUIRES A HELPER AMINO ACID IN THE BINDING MICROENVIRONMENT TO FORM A COVALENT BOND WITH CYS-159

Author

Juswinder Singh, Margit Hagel, Russell C. Petter, Lixin Qiao, D. Niu, Matthew T. Labenski, M. Nacht, T. St. Martin, William F. Westlin, Prasoon Chaturvedi, and Michael Sheets

Subjects
chemistry.chemical_classification, Hepatology, Biochemistry, Kunitz STI protease inhibitor, Chemistry, Covalent bond, Hcv protease, Amino acid
Published
2010
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