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155. A Networked Mass Spectrometry Information System.

Author

Shah, Nikhil, Teeter, Steven, Fitch, William L., Wilgus, Rob L., and Koch, Charlie

Subjects
COMPUTER software, MASS spectrometry, LIQUID chromatography, PHARMACEUTICAL chemistry
Abstract

Presents information on the networked mass spectrometry information system used by pharmaceutical company Affymax. Application of liquid chromatography with ultraviolet and mass spectrometry detectors in identifying compounds from a chemical reaction; Description of the infrastructure for the networked mass spectrometry laboratory at Affymax; Use of Capture, a software invented at Glaxo Wellcome.

Published
2001

167. Liquid chromatography/mass spectrometry methods for measuring dipeptide abundance in non-small-cell lung cancer.

Author

Wu, Manhong, Xu, Yue, Fitch, William L., Zheng, Ming, Merritt, Robert E., Shrager, Joseph B., Zhang, Weiruo, Dill, David L., Peltz, Gary, and Hoang, Chuong D.

Subjects
*LIQUID chromatography, *LUNG cancer, *BIOMOLECULES, *CHEMICAL ecology, *BIOLOGICAL products
Abstract

RATIONALE Metabolomic profiling is a promising methodology of identifying candidate biomarkers for disease detection and monitoring. Although lung cancer is among the leading causes of cancer-related mortality worldwide, the lung tumor metabolome has not been fully characterized. METHODS We utilized a targeted metabolomic approach to analyze discrete groups of related metabolites. We adopted a dansyl [5-(dimethylamino)-1-naphthalene sulfonamide] derivatization with liquid chromatography/mass spectrometry (LC/MS) to analyze changes of metabolites from paired tumor and normal lung tissues. Identification of dansylated dipeptides was confirmed with synthetic standards. A systematic analysis of retention times was required to reliably identify isobaric dipeptides. We validated our findings in a separate sample cohort. RESULTS We produced a database of the LC retention times and MS/MS spectra of 361 dansyl dipeptides. Interpretation of the spectra is presented. Using this standard data, we identified a total of 279 dipeptides in lung tumor tissue. The abundance of 90 dipeptides was selectively increased in lung tumor tissue compared to normal tissue. In a second set of validation tissues, 12 dipeptides were selectively increased. CONCLUSIONS A systematic evaluation of certain metabolite classes in lung tumors may identify promising disease-specific metabolites. Our database of all possible dipeptides will facilitate ongoing translational applications of metabolomic profiling as it relates to lung cancer. Copyright © 2013 John Wiley & Sons, Ltd. [ABSTRACT FROM AUTHOR]

Published
2013
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168. Solvation in Electrospray Mass Spectrometry: Effects on the Reaction Kinetics of Fragmentation Mediated by Ion-Neutral Complexes.

Author

Ya-Ping Tu, Limin He, Fitch, William, and Lam, Michelle

Subjects
*IONIZATION (Atomic physics), *MASS spectrometers, *SOLUTION (Chemistry), *CHEMICAL reactions, *ORGANIC chemistry
Abstract

In electrospray ionization (ESI) on a triple quadrupole mass spectrometer, benzydamine, a molecule with an N,N-dimethylaminopropoxyl side chain, showed a fragmentation pattern in Q1 scans that is dramatically different from the mass-selected collision-induced dissociation (CID) of its MH+ ion. The N,N-dimethylimmonium ion, which dominates in Q1 scans at higher energies, is only a minor product in all CID spectra. By using a smaller model molecule, N,N,N',N'-tetramethyl-1,3propanediamine, with the kinetic energy release measured for the corresponding reaction, we have demonstrated that an ion-neutral complex composed of the N,N-dimethylazetidine cation and a neutral counterpart is involved. When the ion-neutral complex intermediate evolves toward elimination to form the immonium ion, the transition state is stabilized by the neutral species. Solvation of the ion-neutral complex, which obstructs the separation of the two partners by the resulting tighter enclosure, facilitates the elimination by enhancing the stabilization of the transition state. Therefore, the prevalence of the immonium ion in Q1 scans was a result of solvation in the ESI source. In CID reactions, where the decomposing ions are mass-selected and thus solvation does not exist, the immonium ion was a minor product, and the separation of the ion-neutral complex became dominant. [ABSTRACT FROM AUTHOR]

Published
2005
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169. Selection on vocal output affects laryngeal morphology in rats.

Author

Lesch, Raffaela, Schwaha, Thomas, Orozco, Andrea, Shilling, Margaret, Brunelli, Susan, Hofer, Myron, Bowling, Daniel L., Zimmerberg, Betty, and Fitch, William Tecumseh

Subjects
*LARYNX, *TRACHEAL cartilage, *ENERGY dispersive X-ray spectroscopy, *VOCAL cords, *MORPHOLOGY, *VIDEOFLUOROSCOPY, *ULTRASONIC effects
Abstract

Although laryngeal morphology often reflects adaptations for vocalization, the structural consequences of selection for particular aspects of vocal behavior remain poorly understood. In this study, we investigated the effects of increased ultrasonic calling in pups on the adult larynx morphology in selectively bred rat lines. Laryngeal morphology was assessed using multiple techniques: mineralized cartilage volumes were compared in 3D‐models derived from microCT scans, internal structure was compared using clearing and staining procedures combined with microscopy, cellular structure was compared using histology and microscopy, and element composition was assessed with scanning energy dispersive X‐ray spectroscopy. Our results show that adult rats from lines bred to produce ultrasonic calls at higher rates as pups have shorter vocal folds and a more mineralized thyroid cartilage compared to rats bred to produce ultrasonic calls at lower rates. The change in vocal fold length appears to account for differences in low‐frequency calls in these two rat lines. We suggest that the observed increases in mineralization of the thyroid cartilage in the high‐ultrasound lineage provide increased reinforcement of the laryngeal structure during ultrasonic call production. Our findings therefore demonstrate an effect of selection for vocal behavior on laryngeal morphology, with acoustic consequences. [ABSTRACT FROM AUTHOR]

Published
2021
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172. Safety and activity of RRx-001 in patients with advanced cancer: a first-in-human, open-label, dose-escalation phase 1 study.

Author

Reid, Tony, Oronsky, Bryan, Scicinski, Jan, Scribner, Curt L, Knox, Susan J, Ning, Shoucheng, Peehl, Donna M, Korn, Ron, Stirn, Meaghan, Carter, Corey A, Oronsky, Arnold, Taylor, Michael J, Fitch, William L, Cabrales, Pedro, Kim, Michelle M, 3rdBurris, Howard A, Lao, Christopher D, Abrouk, Nacer E D, Fanger, Gary R, and Infante, Jeffrey R

Subjects
*CANCER chemotherapy, *CANCER treatment, *CARCINOGENS, *ONCOLOGY, *MEDICAL care, *CLINICAL trials, *COMPARATIVE studies, *DRUG dosage, *DOSE-effect relationship in pharmacology, *DRUG side effects, *DRUG toxicity, *GENES, *HETEROCYCLIC compounds, *RESEARCH methodology, *MEDICAL cooperation, *ORGANIC compounds, *PROGNOSIS, *RESEARCH, *RESEARCH funding, *TUMORS, *EVALUATION research, *TREATMENT effectiveness
Abstract

Background: Epigenetic alterations have been strongly associated with tumour formation and resistance to chemotherapeutic drugs, and epigenetic modifications are an attractive target in cancer research. RRx-001 is activated by hypoxia and induces the generation of reactive oxygen and nitrogen species that can epigenetically modulate DNA methylation, histone deacetylation, and lysine demethylation. The aim of this phase 1 study was to assess the safety, tolerability, and pharmacokinetics of RRx-001.Methods: In this open-label, dose-escalation, phase 1 study, we recruited adult patients (aged >18 years) with histologically or cytologically confirmed diagnosis of advanced, malignant, incurable solid tumours from University of California at San Diego, CA, USA, and Sarah Cannon Research Institute, Nashville, TN, USA. Key eligibility criteria included evaluable disease, Eastern Cooperative Group performance status of 2 or less, an estimated life expectancy of at least 12 weeks, adequate laboratory parameters, discontinuation of all previous antineoplastic therapies at least 6 weeks before intervention, and no residual side-effects from previous therapies. Patients were assigned to receive intravenous infusions of RRx-001 at increasing doses (10 mg/m(2), 16·7 mg/m(2), 24·6 mg/m(2), 33 mg/m(2), 55 mg/m(2), and 83 mg/m(2)) either once or twice-weekly for at least 4 weeks, with at least three patients per dose cohort and allowing a 2-week observation period before dose escalation. Samples for safety and pharmacokinetics analysis, including standard chemistry and haematological panels, were taken on each treatment day. The primary objective was to assess safety, tolerability, and dose-limiting toxic effects of RRx-001, to determine single-dose pharmacokinetics, and to identify a recommended dose for phase 2 trials. All analyses were done per protocol. Accrual is complete and follow-up is still on-going. This trial is registered with ClinicalTrials.gov, number NCT01359982.Findings: Between Oct 10, 2011, and March 18, 2013, we enrolled 25 patients and treated six patients in the 10 mg/m(2) cohort, three patients in the 16·7 mg/m(2) cohort, three patients in the 24·6 mg/m(2) cohort, four patients in the 33 mg/m(2) cohort, three patients in the 55 mg/m(2), and six patients in the 83 mg/m(2) cohort. Pain at the injection site, mostly grade 1 and grade 2, was the most common adverse event related to treatment, experienced by 21 (84%) patients. Other common drug-related adverse events included arm swelling or oedema (eight [32%] patients), and vein hardening (seven [28%] patients). No dose-limiting toxicities were observed. Time constraints related to management of infusion pain from RRx-001 resulted in a maximally feasible dose of 83 mg/m(2). Of the 21 evaluable patients, one (5%) patient had a partial response, 14 (67%) patients had stable disease, and six (29%) patients had progressive disease; all responses were across a variety of tumour types. Four patients who had received RRx-001 were subsequently rechallenged with a treatment that they had become refractory to; all four responded to the rechallenge.Interpretation: RRx-001 is a well-tolerated novel compound without clinically significant toxic effects at the tested doses. Preliminary evidence of activity is promising and, on the basis of all findings, a dose of 16·7 mg/m(2) was recommended as the targeted dose for phase 2 trials.Funding: EpicentRx (formerly RadioRx). [ABSTRACT FROM AUTHOR]

Published
2015
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173. Identification of drug targets by chemogenomic and metabolomic profiling in yeast.

Author

Wu, Manhong, Zheng, Ming, Zhang, Weiruo, Suresh, Sundari, Schlecht, Ulrich, Fitch, William L., Aronova, Sofia, Baumann, Stephan, Davis, Ronald, St.onge, Robert, Dill, David L., and Peltz, Gary

Abstract

To advance our understanding of disease biology, the characterization of the molecular target for clinically proven or new drugs is very important. Because of its simplicity and the availability of strains with individual deletions in all of its genes, chemogenomic profiling in yeast has been used to identify drug targets. As measurement of drug-induced changes in cellular metabolites can yield considerable information about the effects of a drug, we investigated whether combining chemogenomic and metabolomic profiling in yeast could improve the characterization of drug targets.We used chemogenomic and metabolomic profiling in yeast to characterize the target for five drugs acting on two biologically important pathways. A novel computational method that uses a curated metabolic network was also developed, and it was used to identify the genes that are likely to be responsible for the metabolomic differences found.The combination of metabolomic and chemogenomic profiling, along with data analyses carried out using a novel computational method, could robustly identify the enzymes targeted by five drugs. Moreover, this novel computational method has the potential to identify genes that are causative of metabolomic differences or drug targets. [ABSTRACT FROM AUTHOR]

Published
2012
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174. Exploration of piperidine-4-yl-aminopyrimidines as HIV-1 reverse transcriptase inhibitors. N-Phenyl derivatives with broad potency against resistant mutant viruses

Author

Tang, Guozhi, Kertesz, Denis J., Yang, Minmin, Lin, Xianfeng, Wang, Zhanguo, Li, Wentao, Qiu, Zongxing, Chen, Junli, Mei, Jianghua, Chen, Li, Mirzadegan, Taraneh, Harris, Seth F., Villaseñor, Armando G., Fretland, Jennifer, Fitch, William L., Hang, Julie Qi, Heilek, Gabrielle, and Klumpp, Klaus

Subjects
*REVERSE transcriptase, *HIV, *ENZYME inhibitors, *PIPERIDINE, *ORGANIC synthesis, *STRUCTURE-activity relationships, *CRYSTALLOGRAPHY
Abstract

Abstract: Further investigation of the recently reported piperidine-4-yl-aminopyrimidine class of non-nucleoside reverse transcriptase inhibitors (NNRTIs) has been carried out. Thus, preparation of a series of N-phenyl piperidine analogs resulted in the identification of 3-carboxamides as a particularly active series. Analogs such as 28 and 40 are very potent versus wild-type HIV-1 and a broad range of NNRTI-resistant mutant viruses. Synthesis, structure–activity relationship (SAR), clearance data, and crystallographic evidence for the binding motif are discussed. [Copyright &y& Elsevier]

Published
2010
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175. Incidence and severity of sexual adverse experiences in finasteride and placebo-treated men with benign prostatic hyperplasia

Author

Wessells, Hunter, Roy, Johnny, Bannow, John, Grayhack, John, Matsumoto, Alvin M., Tenover, Lisa, Herlihy, Richard, Fitch, William, Labasky, Richard, Auerbach, Stephen, Parra, Raul, Rajfer, Jacob, Culbertson, Jennifer, Lee, Michael, Bach, Mark A., Waldstreicher, Joanne, and PLESS Study Group

Subjects
*HYPERPLASIA, *PLACEBOS
Abstract

: ObjectivesTo evaluate the incidence and resolution of sexual adverse experiences (AEs) in men with benign prostatic hyperplasia treated with finasteride 5 mg compared with placebo.: MethodsThe Proscar Long-term Efficacy and Safety Study (PLESS) was a 4-year, randomized, double-blind, placebo-controlled trial assessing the efficacy and safety of finasteride 5 mg in 3040 men, aged 45 to 78 years, with symptomatic benign prostatic hyperplasia, enlarged prostates, and no evidence of prostate cancer. Patients completed a questionnaire at screening regarding their history of sexual dysfunction. During treatment, spontaneously self-reported sexual AEs were recorded.: ResultsAt screening, 46% of patients in each treatment group reported some history of sexual dysfunction. During year 1 of the study, 15% of finasteride-treated patients and 7% of placebo-treated patients had sexual AEs that were considered drug related by the investigator (P <0.001). During years 2 to 4, no between-group difference was noted in the incidence of new sexual AEs (7% in each group). The drug-related sexual AE profile for finasteride was similar for men with or without a history of sexual dysfunction. Sexual AEs resolved while continuing therapy in 12% of finasteride patients and 19% of placebo patients. Only 4% of finasteride and 2% of placebo patients discontinued the study because of sexual AEs. In men who discontinued with a sexual AE, 50% and 41% experienced resolution of their sexual AE after discontinuing finasteride or placebo therapy, respectively.: ConclusionsCompared with placebo, men treated with finasteride experienced new drug-related sexual AEs with an increased incidence only during the first year of therapy. [Copyright &y& Elsevier]

Published
2003
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176. Discovery of G2019S-Selective Leucine Rich Repeat Protein Kinase 2 inhibitors with in vivo efficacy.

Author

Leśniak, Robert K., Nichols, R. Jeremy, Schonemann, Marcus, Zhao, Jing, Gajera, Chandresh R., Fitch, William L., Lam, Grace, Nguyen, Khanh C., Smith, Mark, and Montine, Thomas J.

Subjects
*PROTEIN kinase inhibitors, *LEUCINE, *PROTEIN kinases, *DARDARIN, *PARKINSON'S disease
Abstract

Mutations in the Leucine Rich Repeat Protein Kinase 2 gene (LRRK2) are the most common genetic causes of Parkinson's Disease (PD). The G2019S mutation is the most common inherited LRRK2 mutation, occurs in the kinase domain, and results in increased kinase activity. We report the discovery and development of compound 38 , an indazole-based, G2019S-selective (>2000-fold vs. WT) LRRK2 inhibitor capable of entering rodent brain (K p = 0.5) and selectively inhibiting G2019S-LRRK2. The compounds disclosed herein present a starting point for further development of brain penetrant G2019S selective inhibitors that hopefully reduce lung phenotype side-effects and pave the way to providing a precision medicine for people with PD who carry the G2019S mutation. [Display omitted] [ABSTRACT FROM AUTHOR]

Published
2022
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178. Complex Metabolism of the Novel Neurosteroid, Ganaxolone, in Humans: A Unique Challenge for Metabolites in Safety Testing Assessment.

Author

Fitch WL, Smith S, Saporito M, Busse G, Zhang M, Ren J, Fitzsimmons ME, Yi P, English S, Carter A, and Baillie TA

Subjects
Animals, Humans, Male, Pregnanolone analysis, Mass Spectrometry, Chromatography, Liquid, Chromatography, High Pressure Liquid, Feces chemistry, Neurosteroids analysis
Abstract

The human pharmacokinetics, metabolism, and excretion of [ 14 C]-ganaxolone (GNX) were characterized in healthy male subjects ( n = 8) following a single 300-mg (150 μ Ci) oral dose. GNX exhibited a short half-life of 4 hours in plasma, whereas total radioactivity had a half-life of 413 hours indicating extensive metabolism to long-lived metabolites. Identification of the major GNX circulating metabolites required extensive isolation and purification for liquid chromatography-tandem mass spectrometry analysis, together with in vitro studies, NMR spectroscopy, and synthetic chemistry support. This revealed that the major routes of GNX metabolism involved hydroxylation at the 16 α -hydroxy position, stereoselective reduction of the 20-ketone to afford the corresponding 20 α -hydroxysterol, and sulfation of the 3 α -hydroxy group. This latter reaction yielded an unstable tertiary sulfate, which eliminated the elements of H 2 SO 4 to introduce a double bond in the A ring. A combination of these pathways, together with oxidation of the 3 β -methyl substituent to a carboxylic acid and sulfation at the 20 α position, led to the major circulating metabolites in plasma, termed M2 and M17. These studies, which led to the complete or partial identification of no less than 59 metabolites of GNX, demonstrated the high complexity of the metabolic fate of this drug in humans and demonstrated that the major circulating products in plasma can result from multiple sequential processes that may not be easily replicated in animals or with animal or human in vitro systems. SIGNIFICANCE STATEMENT: Studies on the metabolism of [ 14 C]-ganaxolone in humans revealed a complex array of products that circulated in plasma, the two major components of which were formed via an unexpected multi-step pathway. Complete structural characterization of these (disproportionate) human metabolites required extensive in vitro studies, along with contemporary mass spectrometry, NMR spectroscopy, and synthetic chemistry efforts, which served to underscore the limitations of traditional animal studies in predicting major circulating metabolites in man., (Copyright © 2023 by The American Society for Pharmacology and Experimental Therapeutics.)

Published
2023
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180. The evolution of the British Journal of Anaesthesia: the first 100 years.

Author

Fitch W, Smith G, Hunter JM, Reilly CS, Mahajan RP, and Hemmings HC Jr

Subjects
Humans, Critical Care, Anesthesiology, Anesthesia
Abstract

At this centenary of the British Journal of Anaesthesia (BJA) in 2023, six of its 12 editors/editors-in-chief detail developments over the decades that have led to the BJA becoming a high-impact international scientific journal. As a charity, the BJA supports academic research and training in anaesthesia, critical care, and pain medicine including funding of research grants and postgraduate education. Building on this foundation, the BJA continues to innovate as it aims to become fully electronic, expand into open access publishing, and increase the diversity of its editorial board., (Copyright © 2022 British Journal of Anaesthesia. Published by Elsevier Ltd. All rights reserved.)

Published
2023
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181. Tunable Enzymatic Synthesis of the Immunomodulator Lipid IV A To Enable Structure-Activity Analysis.

Author

Sankaranarayanan K, Antaris XX, Palanski BA, El Gamal A, Kao CM, Fitch WL, Fischer CR, and Khosla C

Subjects
Anti-Inflammatory Agents pharmacology, Cell Line, Escherichia coli enzymology, Glycolipids pharmacology, Humans, Immunologic Factors pharmacology, Lipid A chemical synthesis, Lipid A pharmacology, Molecular Structure, Structure-Activity Relationship, Anti-Inflammatory Agents chemical synthesis, Enzymes chemistry, Escherichia coli Proteins chemistry, Glycolipids chemical synthesis, Immunologic Factors chemical synthesis, Lipid A analogs & derivatives
Abstract

The Lipid A family of glycolipids, found in the outer membranes of all Gram-negative bacteria, exhibits considerable structural diversity in both lipid and glycan moieties. The lack of facile methods to prepare analogues of these natural products represents a major roadblock in understanding the relationship between their structure and immunomodulatory activities. Here we present a modular, cell-free multienzymatic platform to access these structure-activity relationships. By individually purifying 19 Escherichia coli proteins and reconstituting them in vitro in the presence of acetyl-CoA, UDP- N-acetylglucosamine, NADPH, and ATP, we have developed a system capable of synthesizing Lipid IV A , the first bioactive intermediate in the Lipid A pathway. Our reconstituted multienzyme system revealed considerable promiscuity for orthologs with distinct substrate specificity, as illustrated by swapping enzymes from distantly related cyanobacterial and Pseudomonas species. Analysis of the agonistic and antagonistic activities of the resulting products against the THP-1 human monocytic cell line revealed hitherto unrecognized trends, while opening the door to harnessing the potent biological activities of these complex glycolipid natural products.

Published
2019
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182. In vitro and in vivo metabolite identification of a novel benzimidazole compound ZLN005 by liquid chromatography/tandem mass spectrometry.

Author

Sun W, Nguyen KD, Fitch WL, Banister SD, Tang H, Zhang X, Yu L, Engleman EG, and Rajadas J

Abstract

Rationale: A novel benzimidazole compound ZLN005 was previously identified as a transcriptional activator of peroxisome proliferator-activated receptor γ coactivator 1α (PGC-1α) in certain metabolic tissues. Upregulation of PGC-1α by ZLN005 has been shown to have a beneficial effect in a diabetic mouse model and in a coronary artery disease model in vitro. ZLN005 could also have therapeutic potential in neurodegenerative diseases involving down-regulation of PGC-1α. Given the phenotypic efficacy of ZLN005 in several animal models of human disease, its metabolic profile was investigated to guide the development of novel therapeutics using ZLN005 as the lead compound., Methods: ZLN005 was incubated with both rat and human liver microsomes and S9 fractions to identify in vitro metabolites. Urine from rats dosed with ZLN005 was used to identify in vivo metabolites. Extracted metabolites were analyzed by liquid chromatography/tandem mass spectrometry (LC/MS/MS) using a hybrid linear ion trap triple quadrupole mass spectrometer in full scan, enhanced product ion scan, neutral loss scan and precursor scan modes. Metabolites in plasma and brain of ZLN005-treated rats were also profiled using multiple reaction monitoring., Results: Identified in vitro transformations of ZLN005 include mono- and dihydroxylation, further oxidation to carboxylic acids, and mono-O-glucuronide and sulfate conjugation to hydroxy ZLN005 as well as glutathione conjugation. Identified in vivo metabolites are mainly glucuronide and sulfate conjugates of dihydroxyl, carboxyl, and hydroxy acid of the parent compound. The parent compound as well as several major phase I metabolites were found in rat plasma and brain., Conclusions: Using both in vitro and in vivo methods, we elucidated the metabolic pathway of ZLN005. Phase I metabolites with hydroxylation and carboxylation, as well as phase II metabolites with glucuronide, sulfate and glutathione conjugation, were identified., (Copyright © 2018 John Wiley & Sons, Ltd.)

Published
2018
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183. Using LC Retention Times in Organic Structure Determination: Drug Metabolite Identification.

Author

Fitch WL, Khojasteh C, Aliagas I, and Johnson K

Subjects
Biotransformation, Demethylation, Humans, Hydrogen Bonding, Hydrophobic and Hydrophilic Interactions, Hydroxylation, Mass Spectrometry, Microsomes, Liver metabolism, Molecular Structure, Oxidation-Reduction, Quantitative Structure-Activity Relationship, Time Factors, Workflow, Atorvastatin metabolism, Carbanilides metabolism, Chromatography, Liquid methods
Abstract

Background: There is a continued need for improvements in the efficiency of metabolite structure elucidation., Objective: We propose to take LC Retention Time (RT) into consideration during the process of structure determination., Methods: Herein, we develop a simple methodology that employs a Chromatographic Hydrophobicity Index (CHI) framework for standardizing LC conditions and introduce and utilize the concept of a predictable CHI change upon Phase 1 biotransformation (CHIbt). Through the analysis of literature examples, we offer a Quantitative Structure-Retention Relationship (QSRR) for several types of biotransformation (especially hydroxylation) using physicochemical properties (clogP, hydrogen bonding)., Results: The CHI system for retention indexing is shown to be practical and simple to implement. A database of CHIbt values has been created from re-incubation of 3 compounds and from analysis of an additional 17 datasets from the literature. Application of this database is illustrated., Conclusion: In our experience, this simple methodology allows complementing the discovery efforts that saves resources for in-depth characterization using NMR., (Copyright© Bentham Science Publishers; For any queries, please email at epub@benthamscience.org.)

Published
2018
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184. Small-Volume Injections: Evaluation of Volume Administration Deviation From Intended Injection Volumes.

Author

Muffly MK, Chen MI, Claure RE, Drover DR, Efron B, Fitch WL, and Hammer GB

Subjects
Calibration standards, Humans, Injections, Pharmaceutical Preparations chemistry, Tuberculin administration & dosage, Tuberculin chemistry, Anesthesiologists standards, Drug Compounding methods, Drug Compounding standards, Nurses standards, Pharmaceutical Preparations standards, Syringes standards
Abstract

Background: In the perioperative period, anesthesiologists and postanesthesia care unit (PACU) nurses routinely prepare and administer small-volume IV injections, yet the accuracy of delivered medication volumes in this setting has not been described. In this ex vivo study, we sought to characterize the degree to which small-volume injections (≤0.5 mL) deviated from the intended injection volumes among a group of pediatric anesthesiologists and pediatric postanesthesia care unit (PACU) nurses. We hypothesized that as the intended injection volumes decreased, the deviation from those intended injection volumes would increase., Methods: Ten attending pediatric anesthesiologists and 10 pediatric PACU nurses each performed a series of 10 injections into a simulated patient IV setup. Practitioners used separate 1-mL tuberculin syringes with removable 18-gauge needles (Becton-Dickinson & Company, Franklin Lakes, NJ) to aspirate 5 different volumes (0.025, 0.05, 0.1, 0.25, and 0.5 mL) of 0.25 mM Lucifer Yellow (LY) fluorescent dye constituted in saline (Sigma Aldrich, St. Louis, MO) from a rubber-stoppered vial. Each participant then injected the specified volume of LY fluorescent dye via a 3-way stopcock into IV tubing with free-flowing 0.9% sodium chloride (10 mL/min). The injected volume of LY fluorescent dye and 0.9% sodium chloride then drained into a collection vial for laboratory analysis. Microplate fluorescence wavelength detection (Infinite M1000; Tecan, Mannedorf, Switzerland) was used to measure the fluorescence of the collected fluid. Administered injection volumes were calculated based on the fluorescence of the collected fluid using a calibration curve of known LY volumes and associated fluorescence.To determine whether deviation of the administered volumes from the intended injection volumes increased at lower injection volumes, we compared the proportional injection volume error (loge [administered volume/intended volume]) for each of the 5 injection volumes using a linear regression model. Analysis of variance was used to determine whether the absolute log proportional error differed by the intended injection volume. Interindividual and intraindividual deviation from the intended injection volume was also characterized., Results: As the intended injection volumes decreased, the absolute log proportional injection volume error increased (analysis of variance, P < .0018). The exploratory analysis revealed no significant difference in the standard deviations of the log proportional errors for injection volumes between physicians and pediatric PACU nurses; however, the difference in absolute bias was significantly higher for nurses with a 2-sided significance of P = .03., Conclusions: Clinically significant dose variation occurs when injecting volumes ≤0.5 mL. Administering small volumes of medications may result in unintended medication administration errors.

Published
2017
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185. RRx-001: a systemically non-toxic M2-to-M1 macrophage stimulating and prosensitizing agent in Phase II clinical trials.

Author

Oronsky B, Paulmurugan R, Foygel K, Scicinski J, Knox SJ, Peehl D, Zhao H, Ning S, Cabrales P, Summers TA Jr, Reid TR, Fitch WL, Kim MM, Trepel JB, Lee MJ, Kesari S, Abrouk ND, Day RM, Oronsky A, Ray CM, and Carter CA

Subjects
Animals, Antineoplastic Agents adverse effects, Antineoplastic Agents pharmacology, Antineoplastic Agents therapeutic use, Azetidines adverse effects, Azetidines pharmacology, Cell Death drug effects, Drug Resistance, Neoplasm, Humans, Macrophages metabolism, Neoplasms pathology, Nitro Compounds adverse effects, Nitro Compounds pharmacology, Azetidines therapeutic use, Macrophages drug effects, Neoplasms drug therapy, Nitro Compounds therapeutic use
Abstract

Introduction: According to Hanahan and Weinberg, cancer manifests as six essential physiologic hallmarks: (1) self-sufficiency in growth signals, (2) insensitivity to growth-inhibitory signals, (3) evasion of programmed cell death, (4) limitless replicative potential, (5) sustained angiogenesis, and (6) invasion and metastasis. As a facilitator of these traits as well as immunosuppression and chemoresistance, the presence of tumor-associated macrophages (TAMs) may serve as the seventh hallmark of cancer. Anticancer agents that successfully reprogram TAMs to target rather than support tumor cells may hold the key to better therapeutic outcomes. Areas covered: This article summarizes the characteristics of the macrophage-stimulating agent RRx-001, a molecular iconoclast, sourced from the aerospace industry, with a particular emphasis on the cell-to-cell transfer mechanism of action (RBCs to TAMs) underlying its antitumor activity as well as its chemo and radioprotective properties, consolidated from various preclinical and clinical studies. Expert opinion: RRx-001 is macrophage-stimulating agent with the potential to synergize with chemotherapy, radiotherapy and immunotherapy while simultaneously protecting normal tissues from their cytotoxic effects. Given the promising indications of activity in multiple tumor types and these normal tissue protective properties, RRx-001 may be used to treat a broad spectrum of malignancies, if it is approved in the future.

Published
2017
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186. Novel Series of Dihydropyridinone P2X7 Receptor Antagonists.

Author

Lopez-Tapia F, Walker KA, Brotherton-Pleiss C, Caroon J, Nitzan D, Lowrie L, Gleason S, Zhao SH, Berger J, Cockayne D, Phippard D, Suttmann R, Fitch WL, Bourdet D, Rege P, Huang X, Broadbent S, Dvorak C, Zhu J, Wagner P, Padilla F, Loe B, Jahangir A, and Alker A

Subjects
Aniline Compounds chemistry, Aniline Compounds pharmacology, Halogenation, Humans, Purinergic P2X Receptor Antagonists chemistry, Purinergic P2X Receptor Antagonists pharmacology, Pyridones chemistry, Pyridones pharmacology, Receptors, Purinergic P2X7 metabolism
Abstract

Identification of singleton P2X7 inhibitor 1 from HTS gave a pharmacophore that eventually turned into potential clinical candidates 17 and 19. During development, a number of issues were successfully addressed, such as metabolic stability, plasma stability, GSH adduct formation, and aniline mutagenicity. Thus, careful modification of the molecule, such as conversion of the 1,4-dihydropyridinone to the 1,2-dihydropyridinone system, proper substitution at C-5″, and in some cases addition of fluorine atoms to the aniline ring allowed for the identification of a novel class of potent P2X7 inhibitors suitable for evaluating the role of P2X7 in inflammatory, immune, neurologic, or musculoskeletal disorders.

Published
2015
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187. Development of methods for the bioanalysis of RRx-001 and metabolites.

Author

Scicinski J, Oronsky B, Cooper V, Taylor M, Alexander M, Hadar R, Cosford R, Fleischmann T, and Fitch WL

Subjects
Animals, Antineoplastic Agents pharmacokinetics, Azetidines pharmacokinetics, Calibration, Chromatography, Liquid, Dogs, Humans, Nitro Compounds pharmacokinetics, Rats, Tandem Mass Spectrometry, Antineoplastic Agents metabolism, Azetidines metabolism, Nitro Compounds metabolism
Abstract

Background: Bioanalytical methods were required to study the novel anticancer drug, RRx-001 preclinically and for clinical pharmacokinetic analysis; however, RRx-001 quickly and completely disappeared on intravenous administration in preclinical species., Results: Quantification of RRx-001 directly or by derivatization was unsuccessful. On exposure to whole blood, RRx-001 formed the glutathione (GSH) adduct very rapidly, suggesting this metabolite as the bioanalyte. However, rapid enzymatic degradation in the blood matrix of RRx-001-GSH posed significant technical problems. Herein, we describe a novel and broadly applicable solution to stabilize GSH conjugates in blood samples by inhibiting the degrading enzyme. Liquid chromatography-tandem mass spectrometry methods for analysis of RRx-001-GSH in rat, dog and human plasma were developed and successfully validated to good laboratory practice standards., Conclusion: Extensive breakdown of RRx-001-GSH was effectively stopped by addition of the enzyme inhibitor, acivicin. The developed liquid chromatography-tandem mass spectrometry assay for RRx-001-GSH was validated for use in preclinical toxicology studies and the Phase I first-in-human clinical trial.

Published
2014
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188. Metabolomic-derived novel cyst fluid biomarkers for pancreatic cysts: glucose and kynurenine.

Author

Park WG, Wu M, Bowen R, Zheng M, Fitch WL, Pai RK, Wodziak D, Visser BC, Poultsides GA, Norton JA, Banerjee S, Chen AM, Friedland S, Scott BA, Pasricha PJ, Lowe AW, and Peltz G

Subjects
Adult, Aged, Aged, 80 and over, Carcinoma, Pancreatic Ductal diagnosis, Carcinoma, Pancreatic Ductal metabolism, Cohort Studies, Cystadenocarcinoma diagnosis, Cystadenocarcinoma, Mucinous diagnosis, Cystadenocarcinoma, Mucinous metabolism, Cystadenoma diagnosis, Cystadenoma, Mucinous diagnosis, Cystadenoma, Mucinous metabolism, Cystadenoma, Serous diagnosis, Cystadenoma, Serous metabolism, Female, Humans, Male, Metabolomics, Middle Aged, Pancreatic Cyst diagnosis, Pancreatic Neoplasms diagnosis, Pancreatic Pseudocyst diagnosis, Pancreatic Pseudocyst metabolism, Retrospective Studies, Sensitivity and Specificity, Biomarkers, Tumor metabolism, Cyst Fluid metabolism, Cystadenocarcinoma metabolism, Cystadenoma metabolism, Glucose metabolism, Kynurenine metabolism, Pancreatic Cyst metabolism, Pancreatic Neoplasms metabolism
Abstract

Background: Better pancreatic cyst fluid biomarkers are needed., Objective: To determine whether metabolomic profiling of pancreatic cyst fluid would yield clinically useful cyst fluid biomarkers., Design: Retrospective study., Setting: Tertiary-care referral center., Patients: Two independent cohorts of patients (n = 26 and n = 19) with histologically defined pancreatic cysts., Intervention: Exploratory analysis for differentially expressed metabolites between (1) nonmucinous and mucinous cysts and (2) malignant and premalignant cysts was performed in the first cohort. With the second cohort, a validation analysis of promising identified metabolites was performed., Main Outcome Measurements: Identification of differentially expressed metabolites between clinically relevant cyst categories and their diagnostic performance (receiver operating characteristic [ROC] curve)., Results: Two metabolites had diagnostic significance-glucose and kynurenine. Metabolomic abundances for both were significantly lower in mucinous cysts compared with nonmucinous cysts in both cohorts (glucose first cohort P = .002, validation P = .006; and kynurenine first cohort P = .002, validation P = .002). The ROC curve for glucose was 0.92 (95% confidence interval [CI], 0.81-1.00) and 0.88 (95% CI, 0.72-1.00) in the first and validation cohorts, respectively. The ROC for kynurenine was 0.94 (95% CI, 0.81-1.00) and 0.92 (95% CI, 0.76-1.00) in the first and validation cohorts, respectively. Neither could differentiate premalignant from malignant cysts. Glucose and kynurenine levels were significantly elevated for serous cystadenomas in both cohorts., Limitations: Small sample sizes., Conclusion: Metabolomic profiling identified glucose and kynurenine to have potential clinical utility for differentiating mucinous from nonmucinous pancreatic cysts. These markers also may diagnose serous cystadenomas., (Copyright © 2013 American Society for Gastrointestinal Endoscopy. Published by Mosby, Inc. All rights reserved.)

Published
2013
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189. Using chimeric mice with humanized livers to predict human drug metabolism and a drug-drug interaction.

Author

Nishimura T, Hu Y, Wu M, Pham E, Suemizu H, Elazar M, Liu M, Idilman R, Yurdaydin C, Angus P, Stedman C, Murphy B, Glenn J, Nakamura M, Nomura T, Chen Y, Zheng M, Fitch WL, and Peltz G

Subjects
Animals, Antiviral Agents blood, Antiviral Agents pharmacokinetics, Antiviral Agents therapeutic use, Benzimidazoles blood, Benzimidazoles pharmacokinetics, Benzimidazoles therapeutic use, Cytochrome P-450 CYP3A, Cytochrome P-450 CYP3A Inhibitors, Drug Evaluation, Preclinical, Drug Interactions, Enzyme Inhibitors metabolism, Enzyme Inhibitors pharmacokinetics, Enzyme Inhibitors pharmacology, Half-Life, Hepacivirus drug effects, Hepatitis C drug therapy, Hepatitis C enzymology, Hepatitis C virology, Hepatocytes drug effects, Hepatocytes enzymology, Hepatocytes metabolism, Humans, Male, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Microsomes, Liver drug effects, Microsomes, Liver enzymology, Microsomes, Liver metabolism, Predictive Value of Tests, Rats, Ritonavir metabolism, Ritonavir pharmacokinetics, Ritonavir pharmacology, Species Specificity, Virus Replication drug effects, Antiviral Agents metabolism, Benzimidazoles metabolism, Liver drug effects, Liver enzymology, Liver metabolism, Transplantation Chimera metabolism
Abstract

Interspecies differences in drug metabolism have made it difficult to use preclinical animal testing data to predict the drug metabolites or potential drug-drug interactions (DDIs) that will occur in humans. Although chimeric mice with humanized livers can produce known human metabolites for test substrates, we do not know whether chimeric mice can be used to prospectively predict human drug metabolism or a possible DDI. Therefore, we investigated whether they could provide a more predictive assessment for clemizole, a drug in clinical development for the treatment of hepatitis C virus (HCV) infection. Our results demonstrate, for the first time, that analyses performed in chimeric mice can correctly identify the predominant human drug metabolite before human testing. The differences in the rodent and human pathways for clemizole metabolism were of importance, because the predominant human metabolite was found to have synergistic anti-HCV activity. Moreover, studies in chimeric mice also correctly predicted that a DDI would occur in humans when clemizole was coadministered with a CYP3A4 inhibitor. These results demonstrate that using chimeric mice can improve the quality of preclinical drug assessment.

Published
2013
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190. A three-parameter model for classifying anurans into four genera based on advertisement calls.

Author

Gingras B and Fitch WT

Subjects
Animals, Anura classification, Logistic Models, Male, Multivariate Analysis, Phylogeny, Reproducibility of Results, Sound Spectrography, Species Specificity, Support Vector Machine, Time Factors, Algorithms, Anura physiology, Models, Statistical, Signal Processing, Computer-Assisted, Vocalization, Animal
Abstract

The vocalizations of anurans are innate in structure and may therefore contain indicators of phylogenetic history. Thus, advertisement calls of species which are more closely related phylogenetically are predicted to be more similar than those of distant species. This hypothesis was evaluated by comparing several widely used machine-learning algorithms. Recordings of advertisement calls from 142 species belonging to four genera were analyzed. A logistic regression model, using mean values for dominant frequency, coefficient of variation of root-mean square energy, and spectral flux, correctly classified advertisement calls with regard to genus with an accuracy above 70%. Similar accuracy rates were obtained using these parameters with a support vector machine model, a K-nearest neighbor algorithm, and a multivariate Gaussian distribution classifier, whereas a Gaussian mixture model performed slightly worse. In contrast, models based on mel-frequency cepstral coefficients did not fare as well. Comparable accuracy levels were obtained on out-of-sample recordings from 52 of the 142 original species. The results suggest that a combination of low-level acoustic attributes is sufficient to discriminate efficiently between the vocalizations of these four genera, thus supporting the initial premise and validating the use of high-throughput algorithms on animal vocalizations to evaluate phylogenetic hypotheses.

Published
2013
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191. Application of modern drug metabolism structure determination tools and assays to the in vitro metabolism of imiloxan.

Author

Fitch WL, Chen Y, Liu L, Paehler A, and Young M

Subjects
Animals, Biotransformation, Cytochrome P-450 Enzyme System metabolism, Hepatocytes metabolism, Humans, In Vitro Techniques, Liver metabolism, Microsomes, Liver metabolism, Protein Binding, Rats, Adrenergic alpha-2 Receptor Antagonists analysis, Adrenergic alpha-2 Receptor Antagonists metabolism, Imidazoles analysis, Imidazoles metabolism
Abstract

Imiloxan is an alpha2 adrenoceptor antagonist and was developed for depression in the 1980's. In Phase 1 clinical trials imiloxan dosing led to hypersensitivity reactions; the molecule's development was discontinued. The present study revisits the in vitro metabolism of imiloxan using modern analytical methods. Human and rat liver microsomes convert imiloxan into a variety of metabolites many of which are unstable and or reactive. Imiloxan also yields high protein covalent binding in microsomal assays. Imiloxan is a useful test molecule for defining the relationship between liver covalent binding and idiosyncratic toxicity.

Published
2010
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192. Analytical tools and approaches for metabolite identification in early drug discovery.

Author

Chen Y, Monshouwer M, and Fitch WL

Subjects
Animals, Biotransformation, Chromatography, High Pressure Liquid, Humans, Magnetic Resonance Spectroscopy, Mass Spectrometry, Pharmaceutical Preparations chemistry, Spectrophotometry, Ultraviolet, Pharmaceutical Preparations analysis, Pharmaceutical Preparations metabolism
Abstract

Determination of the chemical structures of metabolites is a critical part of the early pharmaceutical discovery process. Understanding the structures of metabolites is useful both for optimizing the metabolic stability of a drug as well as rationalizing the drug safety profile. This review describes the current state of the art in this endeavor. The likely outcome of metabolism is first predicted by comparison to the literature. Then metabolites are synthesized in a variety of in vitro systems. The various approaches to LC/UV/MS are applied to learn information about these metabolites and structure hypotheses are made. Structures are confirmed by synthesis or NMR. The special topic of reactive metabolite structure determination is briefly addressed.

Published
2007
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193. Agonists of the follicle stimulating hormone receptor from an encoded thiazolidinone library.

Author

Maclean D, Holden F, Davis AM, Scheuerman RA, Yanofsky S, Holmes CP, Fitch WL, Tsutsui K, Barrett RW, and Gallop MA

Subjects
Aldehydes chemistry, Amino Acids chemistry, Aminobenzoates chemical synthesis, Chromatography, High Pressure Liquid, Combinatorial Chemistry Techniques methods, Drug Design, Luciferases chemistry, Mass Spectrometry, Molecular Structure, Polystyrenes, Stereoisomerism, Receptors, FSH agonists, Thiazoles chemical synthesis
Abstract

The design, synthesis, characterization, and screening of a large, encoded thiazolidinone library are described. Three sets of 35 building blocks were combined by encoded split-pool synthesis to give a library containing more than 42 000 members. Building block selection was based in part on a novel small molecule follicle stimulating hormone receptor agonist hit and in part for diversity. HPLC/MS techniques were applied at the single-bead level to build confidence in the reliability of library construction. Application of two distinct screening strategies resulted in the identification of compounds with significantly improved potency over the initial hit. This work demonstrates the versatility of encoded libraries for preparing a large number of analogues of a given hit while simultaneously generating a large collection of compounds for screening against other targets.

Published
2004
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194. Software for automating analysis of encoded combinatorial libraries.

Author

Fitch WL, Zhang JJ, Shah N, Ouchi G, Wilgus RL, and Muskal S

Subjects
Diamines isolation & purification, Electronic Data Processing, Forms and Records Control, Robotics, Combinatorial Chemistry Techniques, Diamines chemical synthesis, Software
Abstract

This paper describes the applications which are used to automate the analysis of encoded combinatorial libraries. Commercial packages from MDL, Oracle and Agilent are linked with application software written in C/C++, in Microsoft Access and in ChemStation macro language. Encoding correspondence lists for each of up to three synthetic steps are conveniently associated with building block lists using the first application, CodeGen. The second application Decode allows the user to identify the individual beads picked onto a 96-well plate and the pool number for each bead. The decoding chromatography data for each well is then loaded into the program. The chromatography data is used to identify the tags used in the synthesis. Along with the building block information from ISIS/Host, the building block used in each step of the synthesis can be identified. A third routine, Code-to-Structure, takes the coded library building blocks and creates the connection table in ISIS for each structure found by the decode program. For quality control of encoded library synthesis, the decoded structures on a set of beads is compared to the LC/UV/MS data for the ligand cleaved from the same bead. CAPTURE, a GlaxoSmithKline proprietary application, is used to display and analyze the decoded structures and associated mass spectral data. This application uses simple isotopic composition and electrospray ionization rule sets to predict mass spectra and judge the concordance of a structure- mass spectrum data set. An ancillary program, EIC, is used to extract predicted single ion chromatograms from the full scan LC/MS data.

Published
2002
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195. Prediction of ultraviolet spectral absorbance using quantitative structure-property relationships.

Author

Fitch WL, McGregor M, Katritzky AR, Lomaka A, Petrukhin R, and Karelson M

Abstract

High performance liquid chromatography (HPLC) with ultraviolet (UV) spectrophotometric detection is a common method for analyzing reaction products in organic chemistry. This procedure would benefit from a computational model for predicting the relative response of organic molecules. Models are now reported for the prediction of the integrated UV absorbance for a diverse set of organic compounds using a quantitative structure-property relationship (QSPR) approach. A seven-descriptor linear correlation with a squared correlation coefficient (R2) of 0.815 is reported for a data set of 521 compounds. Using the sum of ZINDO oscillator strengths in the integration range as an additional descriptor allowed reduction in the number of descriptors producing a robust model for 460 compounds with five descriptors and a squared correlation coefficient 0.857. The descriptors used in the models are discussed with respect to the physical nature of the UV absorption process.

Published
2002
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199. Alkaloid and predation patterns in colorado lupine populations.

Author

Dolinger PM, Ehrlich PR, Fitch WL, and Breedlove DE

Abstract

Colorado populations of herbaceous perennial lupines show three distinct patterns of amounts, kinds, and individual variability of inflorescence alkaloids. These patterns, interpreted as alternative chemical defense strategies, can be related to the susceptibility of populations to attack by larvae of a small flower-feeding lycaenid butterfly, Glaucopsyche lygdamus.In situations ecologically unfavorable to G. lygdumus, lupine populations have "low" alkaloidal profiles, accumulating relatively low amounts of single, bicyclic alkaloids in their inflorescences, with little individual alkaloidal variability, Lupine populations which are quite available to G. lygdamus, on the other hand, accumulate much higher amounts of inflorescence alkaloids. Of these alkaloidally "high" populations, those which suffer only minor predation by G. lygdamus have individually variable mixtures of three or four inflorescence alkaloids, which are found to be isomers of lupanine and closely related tetracyclic compounds. In contrast, those which suffer heavy predation by G. lygdamus show a mixture of nine diverse alkaloidal components including lupanine, hydroxylupanine, and hydroxylupanine esters which is quite invariant from individual to individual.It is hypothesized that individual variability in alkaloids is an anti-specialist chemical defense mechanism. Such individual variability may be advantageous to plant populations by reducing the possibility of selection for strains of specialist herbivores capable of detoxifying or otherwise withstanding plant defensive compounds.

Published
1973
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