Your search keyword '"David Stout"' showing total 228 results

1. Follistatin promotes adipocyte differentiation, browning, and energy metabolism[S]

Author

Melissa Braga, Srinivasa T. Reddy, Laurent Vergnes, Shehla Pervin, Victor Grijalva, David Stout, John David, Xinmin Li, Venina Tomasian, Christopher B. Reid, Keith C. Norris, Sherin U. Devaskar, Karen Reue, and Rajan Singh

Subjects

mouse embryonic fibroblast, myostatin, brown fat, energy expenditure, uncoupling protein 1, mitochondria, Biochemistry, QD415-436

Abstract

Follistatin (Fst) functions to bind and neutralize the activity of members of the transforming growth factor-β superfamily. Fst has a well-established role in skeletal muscle, but we detected significant Fst expression levels in interscapular brown and subcutaneous white adipose tissue, and further investigated its role in adipocyte biology. Fst expression was induced during adipogenic differentiation of mouse brown preadipocytes and mouse embryonic fibroblasts (MEFs) as well as in cold-induced brown adipose tissue from mice. In differentiated MEFs from Fst KO mice, the induction of brown adipocyte proteins including uncoupling protein 1, PR domain containing 16, and PPAR gamma coactivator-1α was attenuated, but could be rescued by treatment with recombinant FST. Furthermore, Fst enhanced thermogenic gene expression in differentiated mouse brown adipocytes and MEF cultures from both WT and Fst KO groups, suggesting that Fst produced by adipocytes may act in a paracrine manner. Our microarray gene expression profiling of WT and Fst KO MEFs during adipogenic differentiation identified several genes implicated in lipid and energy metabolism that were significantly downregulated in Fst KO MEFs. Furthermore, Fst treatment significantly increases cellular respiration in Fst-deficient cells. Our results implicate a novel role of Fst in the induction of brown adipocyte character and regulation of energy metabolism.

Published

2014

2. Guidance for Methods Descriptions Used in Preclinical Imaging Papers

Author

David Stout, Stuart S. Berr, Amy LeBlanc, Joseph D. Kalen, Dustin Osborne, Julie Price, Wynne Schiffer, Claudia Kuntner, and Jonathan Wall

Subjects

Biology (General), QH301-705.5, Medical technology, R855-855.5

Abstract

Preclinical molecular imaging is a rapidly growing field, where new imaging systems, methods, and biological findings are constantly being developed or discovered. Imaging systems and the associated software usually have multiple options for generating data, which is often overlooked but is essential when reporting the methods used to create and analyze data. Similarly, the ways in which animals are housed, handled, and treated to create physiologically based data must be well described in order that the findings be relevant, useful, and reproducible. There are frequently new developments for metabolic imaging methods. Thus, specific reporting requirements are difficult to establish; however, it remains essential to adequately report how the data have been collected, processed, and analyzed. To assist with future manuscript submissions, this article aims to provide guidelines of what details to report for several of the most common imaging modalities. Examples are provided in an attempt to give comprehensive, succinct descriptions of the essential items to report about the experimental process.

Published

2013

3. Fully Automated Chemical Synthesis: Toward the Universal Synthesizer

Author

Jeremiah P. Malerich, David Krieger, Peter D. Karp, Judy Szeto, Michael Deleo, Markus Krummenacker, David Stout, Sahana Mallya, Jason D. White, Vi-Anh Vu, Nathan Collins, Mario Latendresse, Yonael Gorfu, Peter B. Madrid, Kristina Rucker, Leslie A. Hokama, and Jin-Ping Lim

Subjects

Synthetic biology, Fully automated, 010405 organic chemistry, Oligonucleotide, Chemistry, Organic Chemistry, Nanotechnology, Flow chemistry, Physical and Theoretical Chemistry, 010402 general chemistry, 01 natural sciences, Chemical synthesis, 0104 chemical sciences

Abstract

Automated peptide and oligonucleotide synthesizers enabled a revolution in molecular biology and helped pave the way to modern synthetic biology. Similarly, fully automated synthetic chemistry coul...

Published

2020

4. In vivo imaging of mitochondrial membrane potential in non-small-cell lung cancer

Author

Anthony E. Jones, Adrian M. Gomez, Milica Momcilovic, Carla M. Koehler, Jason T. Lee, Saman Sadeghi, Travis Holloway, Heather R. Christofk, Rui Li, Orian S. Shirihai, Sean T. Bailey, Linsey Stiles, Michael C. Fishbein, David Stout, Steven M. Dubinett, Christopher M. Waldmann, Deepa V. Dabir, David B. Shackelford, Gihad Abdelhady, and Ernst W. Schmid

Subjects

0301 basic medicine, Lung Neoplasms, General Science & Technology, 1.1 Normal biological development and functioning, Oxidative phosphorylation, Mitochondrion, Membrane Potential, Transgenic, Mice, 03 medical and health sciences, Organophosphorus Compounds, 0302 clinical medicine, Underpinning research, In vivo, medicine, Animals, Humans, Non-Small-Cell Lung, Lung, Cancer, Membrane potential, screening and diagnosis, Multidisciplinary, Chemistry, Cell growth, Carcinoma, Lung Cancer, medicine.disease, Mitochondrial, 4.1 Discovery and preclinical testing of markers and technologies, Cell biology, Detection, 030104 developmental biology, A549 Cells, Positron-Emission Tomography, 030220 oncology & carcinogenesis, Cancer cell, Biomedical Imaging, Generic health relevance, Preclinical imaging

Abstract

Mitochondria are essential regulators of cellular energy and metabolism, and have a crucial role in sustaining the growth and survival of cancer cells. A central function of mitochondria is the synthesis of ATP by oxidative phosphorylation, known as mitochondrial bioenergetics. Mitochondria maintain oxidative phosphorylation by creating a membrane potential gradient that is generated by the electron transport chain to drive the synthesis of ATP1. Mitochondria are essential for tumour initiation and maintaining tumour cell growth in cell culture and xenografts2,3. However, our understanding of oxidative mitochondrial metabolism in cancer is limited because most studies have been performed in vitro in cell culture models. This highlights a need for in vivo studies to better understand how oxidative metabolism supports tumour growth. Here we measure mitochondrial membrane potential in non-small-cell lung cancer in vivo using a voltage-sensitive, positron emission tomography (PET) radiotracer known as 4-[18F]fluorobenzyl-triphenylphosphonium (18F-BnTP)4. By using PET imaging of 18F-BnTP, we profile mitochondrial membrane potential in autochthonous mouse models of lung cancer, and find distinct functional mitochondrial heterogeneity within subtypes of lung tumours. The use of 18F-BnTP PET imaging enabled us to functionally profile mitochondrial membrane potential in live tumours. A positron emission tomography imaging tracer is developed to image mitochondrial function in vivo, and application of this tracer to a mouse model of lung cancer identifies distinct functional mitochondrial heterogeneity between tumour cells.

Published

2019

5. Integration of flow synthesis hardware with on-line purification

Author

Dominique Tartar, Peter Madrid, Jeremiah Malerich, and David Stout

Published

2020

6. High resolution structure of the ba3 cytochrome c oxidase from Thermus thermophilus in a lipidic environment.

Author

Theresa Tiefenbrunn, Wei Liu, Ying Chen, Vsevolod Katritch, C David Stout, James A Fee, and Vadim Cherezov

Subjects

Medicine, Science

Abstract

The fundamental chemistry underpinning aerobic life on Earth involves reduction of dioxygen to water with concomitant proton translocation. This process is catalyzed by members of the heme-copper oxidase (HCO) superfamily. Despite the availability of crystal structures for all types of HCO, the mode of action for this enzyme is not understood at the atomic level, namely how vectorial H(+) and e(-) transport are coupled. Toward addressing this problem, we report wild type and A120F mutant structures of the ba(3)-type cytochrome c oxidase from Thermus thermophilus at 1.8 Å resolution. The enzyme has been crystallized from the lipidic cubic phase, which mimics the biological membrane environment. The structures reveal 20 ordered lipid molecules that occupy binding sites on the protein surface or mediate crystal packing interfaces. The interior of the protein encloses 53 water molecules, including 3 trapped in the designated K-path of proton transfer and 8 in a cluster seen also in A-type enzymes that likely functions in egress of product water and proton translocation. The hydrophobic O(2)-uptake channel, connecting the active site to the lipid bilayer, contains a single water molecule nearest the Cu(B) atom but otherwise exhibits no residual electron density. The active site contains strong electron density for a pair of bonded atoms bridging the heme Fe(a3) and Cu(B) atoms that is best modeled as peroxide. The structure of ba(3)-oxidase reveals new information about the positioning of the enzyme within the membrane and the nature of its interactions with lipid molecules. The atomic resolution details provide insight into the mechanisms of electron transfer, oxygen diffusion into the active site, reduction of oxygen to water, and pumping of protons across the membrane. The development of a robust system for production of ba(3)-oxidase crystals diffracting to high resolution, together with an established expression system for generating mutants, opens the door for systematic structure-function studies.

Published

2011

7. The effect of certain colloidal substances on the growth of wheat seedlings ...

Author

Jennings, David Stout, 1885- [fr, Library of Congress, and Jennings, David Stout, 1885- [fr

Subjects

Seedlings, Wheat

Published

1919

8. The effect of certain colloidal substances on the growth of wheat seedlings

Author

Jennings, David Stout, 1885, Library of Congress, and Jennings, David Stout, 1885

Subjects

Seedlings, Wheat

9. The Kidnap Years : The Astonishing True History of the Forgotten Epidemic That Shook Depression-Era America

Author

David Stout and David Stout

Subjects

Kidnapping--United States--History--20th century, Crime--United States--History--20th century

Abstract

A chilling true crime book that chronicles the wave of abductions that terrorized the U.S. during the Great Depression, including the most infamous kidnapping case in American history.'A thrilling account that puts the 1932 Lindbergh baby kidnapping case, billed as'the crime of the century,'in the context of the thousands of other kidnappings that occurred in the U.S. during the Prohibition and Depression eras...will enthrall true crime fans.'—Publishers Weekly, STARRED reviewThe Great Depression was a time of desperation in America—parents struggled to feed their children and unemployment was at a record high. Adding to the lawlessness of the decade, thugs with submachine guns and corrupt law-enforcement officers ran rampant. But amidst this panic, there was one sure-fire way to make money, one used by criminals and resourceful civilians alike: kidnapping.Jump into this forgotten history with Edgar Award-winning author David Stout as he explores the reports of missing people that inundated newspapers at the time. Learn the horrifying details of these abduction cases, from the methods used and the investigative processes to the personal histories of the culprits and victims. All of this culminates with the most infamous kidnapping in American history, the one that targeted an international celebrity and changed legislation forever: the Lindbergh kidnapping.The Kidnap Years is a gritty, visceral, thoughtfully reported page-turner that chronicles the sweep of abductions that afflicted all corners of the country as desperate people were pushed to do the unthinkable.'A fascinating crime book like no other.'—David Cay Johnston, Pulitzer Prize-winning journalist

Published

2021

10. Sanctioned to Survive: How Foreign Firms Perform when Economic Sanctions Affect their Business Relationships—A Study of Contemporary Economic Sanction Actions and their Impact

Author

Blaine David Stout

Subjects

021110 strategic, defence & security studies, Health (social science), 05 social sciences, Geography, Planning and Development, 0211 other engineering and technologies, 02 engineering and technology, International economics, Foreign direct investment, Development, Affect (psychology), Outcome (game theory), 0506 political science, Education, Economic sanctions, Sovereignty, Sustainability, 050602 political science & public administration, Sanctions, Business, Economic system, Social Sciences (miscellaneous), Divestment

Abstract

The intent of this study is to examine the effects of economic sanctions on companies with significant fdi operating in the sanctioned country. Using case study methodology, we consider the impact of sanctions imposed on the Russian Federation (rf) by the United States of America for its intrusion into the sovereign rights of Ukraine. Past sanction events in South Africa and pre-rf formation are reviewed. Two measurable frameworks are developed to study strategies based on ‘divestment and non-divestment’ (Malone and Goodin 1997) dimensions and coupled with variables related to ‘direct and indirect’ effects on financial performance, forgone potential, (Losman 1988) and foreign direct investment (Biglaiser and Lektzian 2011). This research also relies on the historical accounts of Hufbauer et al. (2007) for the compilation of facts related to economic sanctions. Through literature review, the study asks: 1) Strategically, how does a company respond to the economic sanctions imposed by its home country on the sanctioned country in which it has significant fdi? 2) Financially, how do economic sanctions affect the company’s performance and fdi? and 3) Organizationally, how do economic sanctions affect the relationships with those recipient companies of fdi? The study focus is on the energy industry in which the rf economy relies upon for 40 percent of its sustainability and the company of focus is Exxon Mobil (xom). The author readily acknowledges that a single case study may not provide the degree of conclusiveness found in a cross-case study format. However, the outcome of the study does provide a template for use in future case reviews.

Published

2017

11. Other facets of workplace abuse: An exploratory study

Author

Alan A. Cavaiola and David Stout

Subjects

Distress, Social Psychology, Exploratory research, Psychology, General Business, Management and Accounting, Applied Psychology, Clinical psychology

Published

2017

12. Image Sonification—A Practitioner’s Account

Author

David Stout

Subjects

Computer science, business.industry, Sonification, Computer vision, Artificial intelligence, business, Image (mathematics)

Published

2019

13. Purification and crystallization of N-terminally truncated forms of microsomal cytochrome P450 2C5

Author

Wester, Michael R., primary, David Stout, C., additional, and Johnson, Eric E., additional

Published

2002

14. Role of the Conserved Valine 236 in Access of Ligands to the Active Site of Thermus thermophilus ba3 Cytochrome Oxidase

Author

Ying Chen, Yang Li, Ólöf Einarsdóttir, C. David Stout, Chie Funatogawa, Istvan Szundi, William McDonald, and James A. Fee

Subjects

0301 basic medicine, 030102 biochemistry & molecular biology, biology, Ligand, Stereochemistry, Active site, Thermus thermophilus, biology.organism_classification, Biochemistry, 03 medical and health sciences, chemistry.chemical_compound, Heme B, Crystallography, 030104 developmental biology, chemistry, Valine, biology.protein, Cytochrome c oxidase, Heme, Bond cleavage

Abstract

Knowledge of the role of conserved residues in the ligand channel of heme-copper oxidases is critical for understanding how the protein scaffold modulates the function of these enzymes. In this study, we investigated the role of the conserved valine 236 in the ligand channel of ba3 cytochrome c oxidase from Thermus thermophilus by mutating the residue to a more polar (V236T), smaller (V236A), or larger (V236I, V236N, V236L, V236M, and V236F) residue. The crystal structures of the mutants were determined, and the effects of the mutations on the rates of CO, O2, and NO binding were investigated. O2 reduction and NO binding were unaffected in V236T, while the oxidation of heme b during O–O bond cleavage was not detected in V236A. The V236A results are attributed to a decrease in the rate of electron transfer between heme b and heme a3 during O–O bond cleavage in V236A, followed by faster re-reduction of heme b by CuA. This interpretation is supported by classical molecular dynamics simulations of diffusion o...

Published

2016

15. Coumarin Derivatives as Substrate Probes of Mammalian Cytochromes P450 2B4 and 2B6: Assessing the Importance of 7-Alkoxy Chain Length, Halogen Substitution, and Non-Active Site Mutations

Author

Qinghai Zhang, Manish B. Shah, C. David Stout, James R. Halpert, P. Ross Wilderman, and Jingbao Liu

Subjects

Models, Molecular, 0301 basic medicine, Alkylation, Halogenation, Protein Conformation, Stereochemistry, Molecular Conformation, Ligands, Biochemistry, Article, Protein Structure, Secondary, Substrate Specificity, 03 medical and health sciences, chemistry.chemical_compound, Protein structure, Coumarins, Catalytic Domain, Humans, Binding site, Cytochrome P450 Family 2, Binding Sites, Trifluoromethyl, Molecular Structure, 030102 biochemistry & molecular biology, biology, Ligand, Active site, Substrate (chemistry), Recombinant Proteins, Cytochrome P-450 CYP2B6, Kinetics, 030104 developmental biology, Amino Acid Substitution, chemistry, Mutation, Mutagenesis, Site-Directed, biology.protein, Alkoxy group, Aryl Hydrocarbon Hydroxylases

Abstract

Using a combined structural and biochemical approach, the functional importance of a recently described peripheral pocket bounded by the E-, F-, G-, and I-helices in CYP2B4 and 2B6 was probed. Three series of 4-substituted-7-alkoxycoumarin derivatives with a -H, -CH3, or -CF3 at the 4 position of the coumarin core were used initially to monitor functional differences between CYP2B4 and 2B6. 7-Ethoxy-4-(trifluoromethyl)coumarin (7-EFC) displayed the highest catalytic efficiency among these substrates. Mutants were made to alter side-chain polarity (V/E194Q) or bulk (F/Y244W) to alter access to the peripheral pocket. Modest increases in catalytic efficiency of 7-EFC O-deethylation by the mutants were magnified considerably by chlorination or bromination of the substrate ethoxy chain. A structure of CYP2B6 Y244W in complex with (+)-α-pinene was solved at 2.2 Å and showed no CYMAL-5 in the peripheral pocket. A ligand free structure of CYP2B4 F244W was solved at 3.0 Å with CYMAL-5 in the peripheral pocket. In both instances, comparison of the respective wild-type and mutant CYP2B enzymes revealed that CYMAL-5 occupancy of the peripheral pocket had little effect on the topology of active site residue side-chains, despite the fact that the peripheral pocket and active site are located on opposite sides of the I-helix. Analysis of available CYP2B structures suggest that the effect of the amino acid substitutions within the peripheral pocket derive from altered interactions between the F and G helices.

Published

2016

16. Influence of Animal Handling and Housing on Multimodality Imaging

Author

David Stout

Subjects

business.industry, Computer science, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Computer vision, Artificial intelligence, business, Multimodality

Abstract

Development of small-animal imaging systems for functional and anatomical measurements resulted in a fundamental shift toward smaller animals being used for medical research. Rodents, in particular rats and mice, have become the most commonly used species due in part to their low cost, ability to image large numbers quickly, and ease of handling. This had led to the development of support devices such as imaging chambers and specialized anesthesia systems. These imaging chambers provide physiological and physical support for imaging animals, which in turn facilitates imaging animals multiple times and in multiple imaging systems. The ability to reproducibly position animals greatly aids in image analysis, making it easier to co-register and fuse images, draw and reuse regions of interest across studies, and create uniformly positioned images for presentation.

Published

2018

17. Optical Bioluminescence Protocol for Imaging Mice

Author

David, Stout and John, David

Subjects

Mice, Neoplasms, Luminescent Measurements, Optical Imaging, Tumor Cells, Cultured, Animals, Humans, Mice, Nude, Luciferases, Xenograft Model Antitumor Assays

Abstract

The presence, growth, or decline of transfected cell populations expressing the enzyme Luciferase can be followed in live mice using bioluminescence optical imaging techniques. This protocol describes how to verify the imaging equipment, options for injecting the substrate Luciferin into mice, image acquisition considerations, and commonly used data analysis techniques.

Published

2018

18. Cost Management ISE

Author

Edward Blocher, David Stout, Paul Juras, Steven Smith, Edward Blocher, David Stout, Paul Juras, and Steven Smith

Abstract

Cost Management: A Strategic Emphasis, by Blocher/Stout/Juras/Smith is dedicated to answering the question: Why Cost Management? It answers this question by providing cost-management tools and techniques needed to support an organization's competitiveness, improve its performance, and help the organization accomplish its strategy. The text is written to help students understand the broader role of cost accounting in helping an organization succeed - not just the measurement of costs. While the text does include coverage of traditional costing topics (e.g., job-order costing, process costing, service-department cost allocations, and accounting for joint and by-products), its primary strength is the linkage of these topics, as well as more contemporary topics, to an organization's strategy. And with Connect, an easy-to-use homework and learning management solution that embeds learning science and award-winning adaptive tools to improve student outcomes, instructors receive a course solution that includes high quality content and assessment paired with assignments that help students build the skills they need to succeed.New Co-author: Steven D. Smith is an associate professor of accountancy and the Kristine V. and Randy J. Vest Fellow in the Marriott School of Business at Brigham Young University (BYU). Professor Smith's expertise is in the areas of management control systems, focusing on the provision of incentives and performance measurement.

Published

2018

19. The Impact of Social Support and Attachment Style on Quality of Life and Readiness to Change in a Sample of Individuals Receiving Medication-Assisted Treatment for Opioid Dependence

Author

David Stout, Alan A. Cavaiola, and Barbara A Fulmer

Subjects

Adult, Male, media_common.quotation_subject, Medicine (miscellaneous), Ambivalence, Young Adult, Social support, Quality of life (healthcare), Adaptation, Psychological, Opiate Substitution Treatment, medicine, Attachment theory, Humans, Aged, media_common, Addiction, Social Support, Middle Aged, Abstinence, Opioid-Related Disorders, Object Attachment, Analgesics, Opioid, Psychiatry and Mental health, Treatment Outcome, Scale (social sciences), Quality of Life, Female, Psychology, Methadone, medicine.drug, Clinical psychology

Abstract

Background A basic principle within the addictions treatment field is that social support is a vital ingredient in the recovery process. This study examines the nature of social support in a sample of opioid-dependent men and women who are currently being treated in a medication-assisted treatment program (methadone). This research examines the types of social support behaviors that the opioid-dependent individuals consider helpful and explores whether attachment style (i.e., secure, ambivalent, or anxious attachment) was a determining factor in whether social support was perceived as helpful. The dependent variables included readiness to change addictive behaviors and abstinence from other mood-altering drugs. Methods Participants ( N = 159) completed a demographic questionnaire, the Significant Others Scale, the Experiences in Close Relationships Scale, the Multidimensional Scale of Perceived Social Support Assessment, the Readiness to Change Scale, and an Attachment Style Questionnaire. The demographic questionnaire included subjective ratings of self-improvement. Results Social support predicted perceived improvement in all of the areas examined (e.g., health, family/social relationships) and abstinence; however, attachment style did not predict improvement or with readiness to change. Conclusions Social support is an important factor in one's recovery from substance use disorders. Yet attachment style (i.e., anxious, avoidant, or secure) did not predict abstinence or overall improvement in functioning.

Published

2015

20. Night of the Ice Storm

Author

David Stout and David Stout

Abstract

The night of the ice storm in tiny Bessemer, New York, is memorable for more than just the savage weather. That same frigid January evening, a young Catholic priest, Father John Barrow, is brutally bludgeoned to death by an unknown assailant. Two decades later the case remains unsolved, and a group of former employees of the local newspaper hold a reunion and listen to a tape recording made at an earlier celebration when the storm and the terrible crime were the talk of the day. But something police beat reporter Ed Speri hears on the recording compels him to take a closer look at the now ice-cold trail – a decision that ultimately leads to tragedy. Suddenly the stakes have gotten much too high to ignore for Marlee West, the reporter who originally made the damning tape, and her colleague Jenniferurley Hurley. The darkness that fell over their small town on that awful winter night two decades earlier has never truly lifted. A murderer still walks among them, ready to kill and to kill again, and is closer than anyone could have imagined.

Published

2017

21. A Child Is Missing

Author

David Stout and David Stout

Abstract

Long Creek in New York's Hill County is an angry place – depressed, suspicious, and unforgiving. In the aftermath of a late-November snowstorm, one of the town's youngest citizens, five-year-old Jamie Brokow, the son of wealthy divorced parents, is abducted. His family pays the kidnappers their ransom, but the boy is never returned – and soon afterward, Fran Spicer, the local reporter covering the case, dies as the result of a mysterious car crash that the police are all too eager to attribute to alcohol. Will Schafer edits a newspaper in a neighboring county, and he's less willing to dismiss the death of his friend Spicer so easily. Schafer won't find much local support for his investigation, however – strangers like him are not welcome in Long Creek. Still, he is determined to uncover the truth and see that justice is served, for Fran and for little Jamie. But the hunt could have powerful, unanticipated consequences for everyone involved: Schafer, the townspeople, the police, the devastated family... and an odd, disfigured hermit, drawn from his solitude in the forest by the frightened cries of a small child in the night.

Published

2017

22. In Vitro Methods for In Vivo Quantitation of PET and SPECT Imaging Probes: Autoradiography and Gamma Counting

Author

David Stout and Cinthia Pastuskovas

Published

2017

23. Structural and Thermodynamic Basis of (+)-α-Pinene Binding to Human Cytochrome P450 2B6

Author

P. Ross Wilderman, C. David Stout, James R. Halpert, Manish B. Shah, and Hyun-Hee Jang

Subjects

Models, Molecular, Stereochemistry, Biochemistry, Article, Catalysis, Colloid and Surface Chemistry, Oxidoreductase, Humans, Molecule, Binding site, Bicyclic Monoterpenes, chemistry.chemical_classification, Binding Sites, Molecular Structure, biology, Chemistry, Active site, Cooperative binding, Isothermal titration calorimetry, General Chemistry, Aryl Hydrocarbon Hydroxylases, Cytochrome P-450 CYP2B6, Monoterpenes, biology.protein, Thermodynamics, Entropy (order and disorder)

Abstract

Despite recent advances in atomic level understanding of drug and inhibitor interactions with human cytochromes P450, the decades-old questions of chemical and structural determinants of hydrocarbon binding are still unanswered. (+)-α-Pinene is a monoterpene hydrocarbon that is widely distributed in the environment and a potent P450 2B inhibitor. Therefore, a combined biophysical and structural analysis of human P450 2B6 interactions with (+)-α-pinene was undertaken to elucidate the basis of the very high affinity binding. Binding of (+)-α-pinene to the P450 active site was demonstrated by a Type I spectral shift. Thermodynamics of ligand binding were explored using isothermal titration calorimetry and compared to those of P450 2A6, which is much less flexible than 2B6 based on comparison of multiple X-ray crystal structures. Consistent with expectation, entropy is the major driving force for hydrocarbon binding to P450 2A6, as evidenced by the calorimetric results. However, formation of the 2B6-(+)-α-pinene complex has a significant enthalpic component. A 2.0 Å resolution crystal structure of this enzyme ligand complex reveals that the highly plastic 2B6 utilizes previously unrecognized rearrangements of protein motifs. The results indicate that the specific components of enthalpic contribution to ligand binding are closely tied to the degree of enzyme flexibility.

Published

2013

24. The novel purification and biochemical characterization of a reversible CYP24A1:adrenodoxin complex

Author

Andrew J. Annalora, C. David Stout, and Kimberly A. Hartfield

Subjects

Endocrinology, Diabetes and Metabolism, Molecular Sequence Data, Clinical Biochemistry, Biochemistry, Redox, Endocrinology, CYP24A1, Chaps, Adrenodoxin, Animals, Humans, Amino Acid Sequence, Vitamin D3 24-Hydroxylase, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Chemistry, Substrate (chemistry), Cell Biology, Peptide Fragments, Recombinant Proteins, Rats, Enzyme, Multiprotein Complexes, Critical micelle concentration, Steroid Hydroxylases, Biophysics, Molecular Medicine, Cattle, hormones, hormone substitutes, and hormone antagonists

Abstract

Novel paradigms for CYP24A1 inhibitor development are needed to circumvent existing efficacy and toxicity issues related to human therapeutics in this class. We hypothesize that improved structural knowledge of CYP24A1 in complex with natural substrates, inhibitors and/or its redox partner protein, adrenodoxin (Adx) is required to facilitate the next generation of CYP24A1 inhibitor design. To this end, we have developed truncated expression constructs for both rat CYP24A1 (Δ51) and bovine Adx (Δ108), which allow us to purify a stable and reversible state of the CYP24A1:Adx complex, for use in ongoing X-ray crystallographic studies. Spectral characterization of the reversible complex revealed that Adx binding enhanced the stability of the enzyme-substrate complex, despite lowering the ligand binding affinity of the free enzyme, for 1,25(OH)2D2, over 9-fold. Truncation of CYP24A1's flexible N-terminus (Δ51) improved the enzyme's ability to recruit substrate, without altering Adx's ability to stabilize the ligand-bound form. We also found that several common crystallization detergents, including CHAPS, inhibit ligand binding to the CYP24A1:Adx complex at concentrations well below their reported critical micelle concentration (CMC) values. Ultimately, this research provides a useful platform and framework for the study of conformationally complex, membrane-protein complexes, in the ligand-bound state.

Published

2013

25. Structural Diversity of Eukaryotic Membrane Cytochrome P450s

Author

C. David Stout and Eric F. Johnson

Subjects

Models, Molecular, Cytochrome, Mitochondrion, Biology, digestive system, Biochemistry, Protein Structure, Secondary, Protein structure, Cytochrome P-450 Enzyme System, Catalytic Domain, polycyclic compounds, Animals, Humans, Molecular Biology, Cytochrome b, Cell Membrane, Membrane Proteins, Cytochrome P450 reductase, Cytochrome P450, Minireviews, Cell Biology, Mitochondria, Transport protein, Cell biology, Protein Transport, Membrane protein, Inactivation, Metabolic, Carcinogens, biology.protein

Abstract

X-ray crystal structures are available for 29 eukaryotic microsomal, chloroplast, or mitochondrial cytochrome P450s, including two non-monooxygenase P450s. These structures provide a basis for understanding structure-function relations that underlie their distinct catalytic activities. Moreover, structural plasticity has been characterized for individual P450s that aids in understanding substrate binding in P450s that mediate drug clearance.

Published

2013

26. AutoDrug: fully automated macromolecular crystallography workflows for fragment-based drug discovery

Author

Britt Hedman, Bertram Ludaescher, Ana Gonzalez, Michael D. Feese, S. Michael Soltis, S.E. McPhillips, Yingssu Tsai, Aina E. Cohen, Timothy M. McPhillips, Keith O. Hodgson, David A. Bushnell, Daniel Zinn, C. David Stout, and Theresa Tiefenbrunn

Subjects

Models, Molecular, Computer science, Fragment-based lead discovery, Processing, Crystallography, X-Ray, Workflow, Computational science, Automation, User-Computer Interface, Software, Structural Biology, Drug Discovery, computer.programming_language, business.industry, Fragment (computer graphics), Process (computing), General Medicine, Research Papers, Pipeline (software), Crystallography, business, computer, Synchrotrons

Abstract

AutoDrug is software based upon the scientific workflow paradigm that integrates the Stanford Synchrotron Radiation Lightsource macromolecular crystallography beamlines and third-party processing software to automate the crystallo­graphy steps of the fragment-based drug-discovery process. AutoDrug screens a cassette of fragment-soaked crystals, selects crystals for data collection based on screening results and user-specified criteria and determines optimal data-collection strategies. It then collects and processes diffraction data, performs molecular replacement using provided models and detects electron density that is likely to arise from bound fragments. All processes are fully automated, i.e. are performed without user interaction or supervision. Samples can be screened in groups corresponding to particular proteins, crystal forms and/or soaking conditions. A single AutoDrug run is only limited by the capacity of the sample-storage dewar at the beamline: currently 288 samples. AutoDrug was developed in conjunction with RestFlow, a new scientific workflow-automation framework. RestFlow simplifies the design of AutoDrug by managing the flow of data and the organization of results and by orchestrating the execution of computational pipeline steps. It also simplifies the execution and interaction of third-party programs and the beamline-control system. Modeling AutoDrug as a scientific workflow enables multiple variants that meet the requirements of different user groups to be developed and supported. A workflow tailored to mimic the crystallography stages comprising the drug-discovery pipeline of CoCrystal Discovery Inc. has been deployed and successfully demonstrated. This workflow was run once on the same 96 samples that the group had examined manually and the workflow cycled successfully through all of the samples, collected data from the same samples that were selected manually and located the same peaks of unmodeled density in the resulting difference Fourier maps.

Published

2013

27. Small Molecule Regulation of Protein Conformation by Binding in the Flap of HIV Protease

Author

Arthur J. Olson, Stefano Forli, M. G. Finn, Theresa Tiefenbrunn, C. David Stout, Max W. Chang, Meaghan Happer, Ying-Chuan Lin, Bruce E. Torbett, Alexander L. Perryman, Jin Kyu Rhee, John H. Elder, and Michael M. Baksh

Subjects

Conformational change, Indoles, Protein Conformation, Stereochemistry, medicine.medical_treatment, HIV Infections, Crystallography, X-Ray, Biochemistry, Article, chemistry.chemical_compound, Protein structure, HIV Protease, Pepstatins, Hydrolase, medicine, Humans, HIV Protease Inhibitor, Protease, Chemistry, HIV Protease Inhibitors, General Medicine, AutoDock, Small molecule, Molecular Docking Simulation, Crystallography, HIV-1, Molecular Medicine, Propionates, Pepstatin

Abstract

The fragment indole-6-carboxylic acid (1F1), previously identified as a flap site binder in a fragment-based screen against HIV protease (PR), has been co-crystallized with pepstatin-inhibited PR and with apo-PR. Another fragment, 3-indolepropionic acid (1F1-N), predicted by AutoDock calculations and confirmed in a novel ‘inhibition of nucleation’ crystallization assay, exploits the same interactions in the flap site in two crystal structures. Both 1F1 and 1F1-N bind to the closed form of apo-PR and to pepstatin:PR. In solution, 1F1 and 1F1-N raise the Tm of apo-PR by 3.5–5 °C as assayed by differential scanning fluorimetry (DSF), and show equivalent low-micromolar binding constants to both apo-PR and pepstatin:PR, assayed by backscattering interferometry (BSI). The observed signal intensities in BSI are greater for each fragment upon binding to apo-PR than to pepstatin-bound PR, consistent with greater conformational change in the former binding event. Together, these data indicate that fragment binding in the flap site favors a closed conformation of HIV PR.

Published

2013

28. Binding of a Cyano- and Fluoro-containing Drug Bicalutamide to Cytochrome P450 46A1

Author

C. David Stout, Natalia Mast, Wenchao Zheng, and Irina A. Pikuleva

Subjects

biology, Nitrile, Stereochemistry, Active site, Cytochrome P450, Stereoisomerism, Cell Biology, Biochemistry, Enzyme structure, chemistry.chemical_compound, chemistry, biology.protein, Racemic mixture, Molecular Biology, Heme, Conformational isomerism

Abstract

Cytochrome P450 46A1 (CYP46A1) is the cholesterol 24-hydroxylase initiating the major pathways of cholesterol removal from the brain, and bicalutamide (BIC) is a drug of choice for the treatment of progressive androgen-dependent prostate cancer. We evaluated the interactions of BIC with CYP46A1 by x-ray crystallography and by conducting solution and mutagenesis studies. Because BIC is administered to patients as a racemic mixture of the S and R isomers, we studied all three, racemic BIC as well as the S and R isomers. Co-crystallization of CYP46A1 with racemic BIC led to structure determinations at 2.1 A resolution with the drug complexes exhibiting novel properties. Both BIC isomers bind to the CYP46A1 active site in very similar single orientation and adopt an energetically unfavorable folded conformation. This folded BIC conformation is correlated with drug-induced localized shifts of amino acid side chains in CYP46A1 and unusual interactions in the CYP46A1-BIC complex. One of these interactions involves a water molecule that is coordinated to the P450 heme iron and also hydrogen-bonded to the BIC nitrile. Due to polarization of the water in this environment, the heme elicits previously unreported types of P450 spectral responses. We also observed that access to the P450 active site was affected by differential recognition of S versus R isomers at the CYP46A1 surface arising from BIC conformational polymorphism. Background: Cytochrome P450 46A1 is important for normal brain function. Results: The x-ray structures of P450 46A1 were determined in complex with the R and S isomers of the anticancer drug bicalutamide. Conclusion: The cyano group of the folded bicalutamide conformer coordinates the heme iron via a water molecule. Significance: We demonstrate how conformational polymorphism affects drug entry and binding in the P450 active site.

Published

2013

29. Potent Mechanism-Based Inactivation of Cytochrome P450 2B4 by 9-Ethynylphenanthrene: Implications for Allosteric Modulation of Cytochrome P450 Catalysis

Author

Haoming Zhang, Sean C. Gay, Manish Shah, Maryam Foroozesh, Jiawang Liu, Yoichi Osawa, Qinghai Zhang, C. David Stout, James R. Halpert, and Paul F. Hollenberg

Subjects

chemistry.chemical_classification, biology, Chemistry, Stereochemistry, Electrospray ionization, Allosteric regulation, Active site, Cooperativity, Mass spectrometry, Biochemistry, Protein structure, Covalent bond, Oxidoreductase, biology.protein

Abstract

The mechanism-based inactivation of cytochrome P450 2B4 (CYP2B4) by 9-ethynylphenanthrene (9EP) has been investigated. The partition ratio and kinact are 0.2 and 0.25 min–1, respectively. Intriguingly, the inactivation exhibits sigmoidal kinetics with a Hill coefficient of 2.5 and an S50 of 4.5 μM indicative of homotropic cooperativity. Enzyme inactivation led to an increase in mass of the apo-CYP2B4 by 218 Da as determined by electrospray ionization liquid chromatography and mass spectrometry, consistent with covalent protein modification. The modified CYP2B4 was purified to homogeneity and its structure determined by X-ray crystallography. The structure showed that 9EP is covalently attached to Oγ of Thr 302 via an ester bond, which is consistent with the increased mass of the protein. The presence of the bulky phenanthrenyl ring resulted in inward rotations of Phe 297 and Phe 206, leading to a compact active site. Thus, binding of another molecule of 9EP in the active site is prohibited. However, resul...

Published

2013

30. Role of the Conserved Valine 236 in Access of Ligands to the Active Site of Thermus thermophilus ba

Author

Chie, Funatogawa, Yang, Li, Ying, Chen, William, McDonald, Istvan, Szundi, James A, Fee, C David, Stout, and Ólöf, Einarsdóttir

Subjects

Carbon Monoxide, Binding Sites, Thermus thermophilus, Mutation, Missense, Valine, Heme, Molecular Dynamics Simulation, Crystallography, X-Ray, Cytochrome b Group, Ligands, Nitric Oxide, Electron Transport Complex IV, Oxygen, Kinetics, Bacterial Proteins, Protein Domains, Spectrophotometry, Catalytic Domain, Crystallization, Oxidation-Reduction, Protein Binding

Abstract

Knowledge of the role of conserved residues in the ligand channel of heme-copper oxidases is critical for understanding how the protein scaffold modulates the function of these enzymes. In this study, we investigated the role of the conserved valine 236 in the ligand channel of ba

Published

2016

31. Effect of Detergent Binding on Cytochrome P450 2B4 Structure as Analyzed by X-ray Crystallography and Deuterium-Exchange Mass Spectrometry

Author

James R. Halpert, P. Ross Wilderman, Sheng Li, Qinghai Zhang, Hyun-Hee Jang, C. David Stout, Manish B. Shah, and David Lee

Subjects

0301 basic medicine, Models, Molecular, Structural similarity, Detergents, Biophysics, Ether, Crystal structure, Mass spectrometry, Crystallography, X-Ray, Biochemistry, Article, Mass Spectrometry, Protein Structure, Secondary, 03 medical and health sciences, chemistry.chemical_compound, Glucosides, Catalytic Domain, Molecule, Animals, Humans, Cytochrome P450 Family 2, 030102 biochemistry & molecular biology, biology, Chemistry, Organic Chemistry, Active site, Substrate (chemistry), Deuterium Exchange Measurement, Protein Structure, Tertiary, Crystallography, 030104 developmental biology, Mutation, biology.protein, Hydrogen–deuterium exchange, Aryl Hydrocarbon Hydroxylases, Protein Binding

Abstract

Multiple crystal structures of CYP2B4 have demonstrated the binding of the detergent 5-cyclohexyl-1-pentyl-β-D-maltoside (CYMAL-5) in a peripheral pocket located adjacent to the active site. To explore the consequences of detergent binding, X-ray crystal structures of the peripheral pocket mutant CYP2B4 F202W were solved in the presence of hexaethylene glycol monooctyl ether (C8E6) and CYMAL-5. The structure in the presence of CYMAL-5 illustrated a closed conformation indistinguishable from the previously solved wild-type. In contrast, the F202W structure in the presence of C8E6 revealed a detergent molecule that coordinated the heme-iron and extended to the protein surface through the substrate access channel 2f. Despite the overall structural similarity of these detergent complexes, remarkable differences were observed in the A, A', and H helices, the F-G cassette, the C-D and β4 loop region. Hydrogen-deuterium exchange mass spectrometry (DXMS) was employed to probe these differences and to test the effect of detergents in solution. The presence of either detergent increased the H/D exchange rate across the plastic regions, and the results obtained by DXMS in solution were consistent in general with the relevant structural snapshots. The study provides insight into effect of detergent binding and the interpretation of associated conformational dynamics of CYP2B4.

Published

2016

32. Structural Characterization of Human Cytochrome P450 2C19

Author

C. David Stout, Eric F. Johnson, R. Leila Reynald, and Stefaan Sansen

Subjects

chemistry.chemical_classification, biology, Stereochemistry, Substrate (chemistry), Active site, Cytochrome P450, Cell Biology, computer.file_format, Protein Data Bank, Biochemistry, Enzyme, Protein structure, chemistry, Oxidoreductase, Helix, biology.protein, Molecular Biology, computer

Abstract

To identify the structural features underlying the distinct substrate and inhibitor profiles of P450 2C19 relative to the closely related human enzymes, P450s 2C8 and 2C9, the atomic structure (Protein Data Bank code 4GQS) of cytochrome P450 2C19 complexed with the inhibitor (2-methyl-1-benzofuran-3-yl)-(4-hydroxy-3,5-dimethylphenyl)methanone (Protein Data Bank chemical component 0XV) was determined to 2.87 A resolution by x-ray crystallography. The conformation of the peptide backbone of P450 2C19 is most similar to that of P450 2C8, but the substrate-binding cavity of P450 2C8 is much larger than that of P450 2C19 due to differences in the amino acid residues that form the substrate-binding cavities of the two enzymes. In contrast, the substrate-binding cavity of P450 2C19 is much more similar in size to that of the structure of the P450 2C9 flurbiprofen complex than to that of a modified P450 2C9 or that of P450 2C8. The cavities of the P450 2C19 0XV complex and the P450 2C9 flurbiprofen complex differ, however, because the helix B-C loops of the two enzymes are dissimilar. These conformational differences reflect the effects of adjacent structural elements that interact with the B-C loops and that differ between the two enzymes. The availability of a structure for 2C19 will facilitate computational approaches for predictions of substrate and inhibitor binding to this enzyme.

Published

2012

33. Conformational Adaptation of Human Cytochrome P450 2B6 and Rabbit Cytochrome P450 2B4 Revealed upon Binding Multiple Amlodipine Molecules

Author

Qinghai Zhang, P. Ross Wilderman, Manish B. Shah, James R. Halpert, C. David Stout, and Jaime Pascual

Subjects

Stereochemistry, Plasma protein binding, Crystallography, X-Ray, Biochemistry, Article, Protein Structure, Secondary, Substrate Specificity, Protein structure, Animals, Humans, Cytochrome P450 Family 2, chemistry.chemical_classification, biology, Chemistry, Active site, Cytochrome P450, Substrate (chemistry), Oxidoreductases, N-Demethylating, Calcium Channel Blockers, Protein Structure, Tertiary, Cytochrome P-450 CYP2B6, Enzyme, Helix, biology.protein, Amlodipine, Aryl Hydrocarbon Hydroxylases, Rabbits, Protein Binding

Abstract

Structures of human cytochrome P450 2B6 and rabbit cytochrome P450 2B4 in complex with two molecules of the calcium channel blocker amlodipine have been determined by X-ray crystallography. The presence of two drug molecules suggests clear substrate access channels in each P450. According to a previously established nomenclature, amlodipine molecules were trapped in access pathway 2f in P450 2B6 and in pathway 2a or 2f in P450 2B4. These pathways overlap for part of the length and then diverge as they extend toward the protein surface. A previously described solvent channel was also found in each enzyme. The results indicate that key residues located on the surface and at the entrance of the substrate access channels in each of these P450s may play a crucial role in guiding substrate entry. In addition, the region of P450 2B6 and 2B4 involving helices B', F, F', and G' and part of helix G is substantially more open in the amlodipine complexes than in the corresponding 4-(4-chlorophenyl)imidazole complexes. The increased active site volume observed results from the major retraction of helices F, F', and B' and the β4 sheet region located close to the binding cavity to accommodate amlodipine. These structures demonstrate novel insight into distinct conformational states not observed with previous P450 2B structures and provide clear evidence of the substrate access channels in two drug-metabolizing P450s. In addition, the structures exhibit the versatility that can be exploited via in silico studies with other P450 2B6 ligands as large as raloxifene and itraconazole.

Published

2012

34. In Silico and Intuitive Predictions of CYP46A1 Inhibition by Marketed Drugs with Subsequent Enzyme Crystallization in Complex with Fluvoxamine

Author

Natalia Mast, Irina A. Pikuleva, Jeffrey S. Wiseman, Matthew Clark, C. David Stout, and Marlin Linger

Subjects

Models, Molecular, Stereochemistry, Entropy, Quantitative Structure-Activity Relationship, Plasma protein binding, In Vitro Techniques, Crystallography, X-Ray, Hydroxylation, chemistry.chemical_compound, In vivo, Microsomes, Cholesterol 24-Hydroxylase, Animals, Humans, Computer Simulation, Protease Inhibitors, Heme, Enzyme Assays, Pharmacology, chemistry.chemical_classification, Molecular Structure, biology, Brain, Water, Cytochrome P450, Active site, Substrate (chemistry), Stereoisomerism, Articles, Antidepressive Agents, Recombinant Proteins, Cholesterol, Enzyme, chemistry, Fluvoxamine, Steroid Hydroxylases, biology.protein, Molecular Medicine, Cattle, Tranylcypromine, Crystallization, Protein Binding

Abstract

Cytochrome P450 46A1 (cholesterol 24-hydroxylase) is an important brain enzyme that may be inhibited by structurally distinct pharmaceutical agents both in vitro and in vivo. To identify additional inhibitors of CYP46A1 among U.S. Food and Drug Administration-approved therapeutic agents, we used in silico and intuitive predictions and evaluated some of the predicted binders in the enzyme and spectral binding assays. We tested a total of 298 marketed drugs for the inhibition of CYP46A1-mediated cholesterol hydroxylation in vitro and found that 13 of them reduce CYP46A1 activity by >50%. Of these 13 inhibitors, 7 elicited a spectral response in CYP46A1 with apparent spectral K(d) values in a low micromolar range. One of the identified tight binders, the widely used antidepressant fluvoxamine, was cocrystallized with CYP46A1. The structure of this complex was determined at a 2.5 A resolution and revealed the details of drug binding to the CYP46A1 active site. The NH(2)-containing arm of the Y-shaped fluvoxamine coordinates the CYP46A1 heme iron, whereas the methoxy-containing arm points away from the heme group and has multiple hydrophobic interactions with aliphatic amino acid residues. The CF(3)-phenyl ring faces the entrance to the substrate access channel and has contacts with the aromatic side chains. The crystal structure suggests that only certain drug conformers can enter the P450 substrate access channel and reach the active site. Once inside the active site, the conformer probably further adjusts its configuration and elicits the movement of the protein side chains.

Published

2012

35. Crystal Structure of Human Cytochrome P450 2D6 with Prinomastat Bound

Author

C. David Stout, A. Wang, Üzen Savas, Mei-Hui Hsu, and Eric F. Johnson

Subjects

Models, Molecular, Prinomastat, Stereochemistry, Beta sheet, Crystallography, X-Ray, Ligands, Biochemistry, Turn (biochemistry), Protein structure, Catalytic Domain, Cytochrome P-450 CYP2D6 Inhibitors, Humans, Enzyme Inhibitors, Organic Chemicals, Molecular Biology, biology, Chemistry, Active site, Cell Biology, computer.file_format, Protein Data Bank, Enzyme structure, Crystallography, Cytochrome P-450 CYP2D6, Helix, Enzymology, biology.protein, computer, Protein Binding

Abstract

Human cytochrome P450 2D6 contributes to the metabolism of >15% of drugs used in clinical practice. This study determined the structure of P450 2D6 complexed with a substrate and potent inhibitor, prinomastat, to 2.85 A resolution by x-ray crystallography. Prinomastat binding is well defined by electron density maps with its pyridyl nitrogen bound to the heme iron. The structure of ligand-bound P450 2D6 differs significantly from the ligand-free structure reported for the P450 2D6 Met-374 variant (Protein Data Bank code 2F9Q). Superposition of the structures reveals significant differences for β sheet 1, helices A, F, F′, G″, G, and H as well as the helix B-C loop. The structure of the ligand complex exhibits a closed active site cavity that conforms closely to the shape of prinomastat. The closure of the open cavity seen for the 2F9Q structure reflects a change in the direction and pitch of helix F and introduction of a turn at Gly-218, which is followed by a well defined helix F′ that was not observed in the 2F9Q structure. These differences reflect considerable structural flexibility that is likely to contribute to the catalytic versatility of P450 2D6, and this new structure provides an alternative model for in silico studies of substrate interactions with P450 2D6.

Published

2012

36. Investigation by site-directed mutagenesis of the role of cytochrome P450 2B4 non-active-site residues in protein-ligand interactions based on crystal structures of the ligand-bound enzyme

Author

P. Ross Wilderman, Sean C. Gay, Hyun-Hee Jang, Qinghai Zhang, C. David Stout, and James R. Halpert

Subjects

chemistry.chemical_classification, Trifluoromethyl, biology, Chemistry, Stereochemistry, Cytochrome P450, Active site, Cell Biology, Ligand (biochemistry), Biochemistry, chemistry.chemical_compound, Enzyme, Oxidoreductase, biology.protein, Site-directed mutagenesis, Molecular Biology, Protein ligand

Abstract

Residues located outside the active site of cytochromes P450 2B have exhibited importance in ligand binding, structural stability and drug metabolism. However, contributions of non-active-site residues to the plasticity of these enzymes are not known. Thus, a systematic investigation was undertaken of unique residue-residue interactions found in crystal structures of P450 2B4 in complex with 4-(4-chlorophenyl)imidazole (4-CPI), a closed conformation, or in complex with bifonazole, an expanded conformation. Nineteen mutants distributed over 11 sites were constructed, expressed in Escherichia coli and purified. Most mutants showed significantly decreased expression, especially in the case of interactions found in the 4-CPI structure. Six mutants (H172A, H172F, H172Q, L437A, E474D and E474Q) were chosen for detailed functional analysis. Among these, the K(s) of H172F for bifonazole was ∼ 20 times higher than for wild-type 2B4, and the K(s) of L437A for 4-CPI was ∼ 50 times higher than for wild-type, leading to significantly altered inhibitor selectivity. Enzyme function was tested with the substrates 7-ethoxy-4-(trifluoromethyl)coumarin, 7-methoxy-4-(trifluoromethyl)coumarin and 7-benzyloxyresorufin (7-BR). H172F was inactive with all three substrates, and L437A did not turn over 7-BR. Furthermore, H172A, H172Q, E474D and E474Q showed large changes in k(cat)/K(M) for each of the three substrates, in some cases up to 50-fold. Concurrent molecular dynamics simulations yielded distances between some of the residues in these putative interaction pairs that are not consistent with contact. The results indicate that small changes in the protein scaffold lead to large differences in solution behavior and enzyme function.

Published

2011

37. Structures of Cytochrome P450 2B6 Bound to 4-Benzylpyridine and 4-(4-Nitrobenzyl)pyridine: Insight into Inhibitor Binding and Rearrangement of Active Site Side Chains

Author

Manish B. Shah, Jaime Pascual, James R. Halpert, C. David Stout, and Qinghai Zhang

Subjects

Protein Conformation, Pyridines, Stereochemistry, Molecular Sequence Data, Plasma protein binding, Crystallography, X-Ray, chemistry.chemical_compound, Residue (chemistry), Protein structure, Catalytic Domain, Side chain, Humans, Imidazole, Amino Acid Sequence, Enzyme Inhibitors, Histidine, Pharmacology, biology, Chemistry, Hydrogen bond, Active site, Oxidoreductases, N-Demethylating, Articles, Cytochrome P-450 CYP2B6, biology.protein, Molecular Medicine, Aryl Hydrocarbon Hydroxylases, Protein Binding

Abstract

The biochemical, biophysical, and structural analysis of the cytochrome P450 2B subfamily of enzymes has provided a wealth of information regarding conformational plasticity and substrate recognition. The recent X-ray crystal structure of the drug-metabolizing P450 2B6 in complex with 4-(4-chlorophenyl)imidazole (4-CPI) yielded the first atomic view of this human enzyme. However, knowledge of the structural basis of P450 2B6 specificity and inhibition has remained limited. In this study, structures of P450 2B6 were determined in complex with the potent inhibitors 4-benzylpyridine (4-BP) and 4-(4-nitrobenzyl)pyridine (4-NBP). Comparison of the present structures with the previous P450 2B6-4-CPI complex showed that reorientation of side chains of the active site residue Phe206 on the F-helix and Phe297 on the I-helix was necessary to accommodate the inhibitors. However, P450 2B6 does not require any major side chain rearrangement to bind 4-NBP compared with 4-BP, and the enzyme provides no hydrogen-bonding partners for the polar nitro group of 4-NBP within the hydrophobic active site. In addition, on the basis of these new structures, substitution of residue 172 with histidine as observed in the single nucleotide polymorphism Q172H and in P450 2B4 may contribute to a hydrogen bonding network connecting the E- and I-helices, thereby stabilizing active site residues on the I-helix. These results provide insight into the role of active site side chains upon inhibitor binding and indicate that the recognition of the benzylpyridines in the closed conformation structure of P450 2B6 is based solely on hydrophobicity, size, and shape.

Published

2011

38. Structural Characterization of the Complex between α-Naphthoflavone and Human Cytochrome P450 1B1

Author

A. Wang, Eric F. Johnson, Uzen Savas, and C. David Stout

Subjects

Subfamily, Stereochemistry, Plasma protein binding, Crystallography, X-Ray, Biochemistry, Protein Structure, Secondary, Protein structure, Cytochrome P-450 Enzyme System, Oxidoreductase, Catalytic Domain, Humans, Molecular Biology, Benzoflavones, chemistry.chemical_classification, biology, Active site, Cell Biology, Amino acid, Crystallography, Enzyme, chemistry, Protein Structure and Folding, Cytochrome P-450 CYP1B1, Helix, biology.protein, Aryl Hydrocarbon Hydroxylases, Protein Binding

Abstract

The atomic structure of human P450 1B1 was determined by x-ray crystallography to 2.7 Å resolution with α-naphthoflavone (ANF) bound in the active site cavity. Although the amino acid sequences of human P450s 1B1 and 1A2 have diverged significantly, both enzymes exhibit narrow active site cavities, which underlie similarities in their substrate profiles. Helix I residues adopt a relatively flat conformation in both enzymes, and a characteristic distortion of helix F places Phe(231) in 1B1 and Phe(226) in 1A2 in similar positions for π-π stacking with ANF. ANF binds in a distinctly different orientation in P450 1B1 from that observed for 1A2. This reflects, in part, divergent conformations of the helix B'-C loop that are stabilized by different hydrogen-bonding interactions in the two enzymes. Additionally, differences between the two enzymes for other amino acids that line the edges of the cavity contribute to distinct orientations of ANF in the two active sites. Thus, the narrow cavity is conserved in both P450 subfamily 1A and P450 subfamily 1B with sequence divergence around the edges of the cavity that modify substrate and inhibitor binding. The conservation of these P450 1B1 active site amino acid residues across vertebrate species suggests that these structural features are conserved.

Published

2011

39. Three Clusters of Conformational States in P450cam Reveal a Multistep Pathway for Closing of the Substrate Access Channel

Author

Edith C. Glazer, David B. Goodin, Richard Wilson, C. David Stout, and Young Tae Lee

Subjects

Camphor 5-Monooxygenase, biology, Protein Conformation, Pseudomonas putida, Stereochemistry, Chemistry, Active site, Substrate (chemistry), Plasma protein binding, Crystallography, X-Ray, Ligand (biochemistry), Biochemistry, Article, Substrate Specificity, Crystallography, Protein structure, Bacterial Proteins, Catalytic Domain, Helix, biology.protein, Molecular imprinting, Linker, Protein Binding

Abstract

Conformational changes in the substrate access channel have been observed for several forms of cytochrome P450, but the extent of conformational plasticity exhibited by a given isozyme has not been completely characterized. Here we present crystal structures of P450cam bound to a library of 12 active site probes containing a substrate analog tethered to a variable linker. The structures provide a unique view of the range of protein conformations accessible during substrate binding. Principal component analysis of a total of 30 structures reveals three discrete clusters of conformations; closed (P450cam-C), intermediate (P450cam-I) and fully open (P450cam-O). Relative to P450cam-C, the P450cam-I state results predominantly from a retraction of the F-helix, while both F and G helices move in concert to reach the fully open P450cam-O state. Both P450cam-C and P450cam-I are well defined states, while P450cam-O shows evidence for a somewhat broader distribution of conformations, and includes the open form recently seen in the absence of substrate. The observed clustering of protein conformations over a wide range of ligand variants suggests a multi-step closure of the enzyme around the substrate that begins by conformational selection from an ensemble of open conformations and proceeds through a well defined intermediate, P450cam-I, before full closure to the P450cam-C state in the presence of small substrates. This multi-step pathway may have significant implications for a full understanding of substrate specificity, kinetics and coupling of substrate binding to P450 function.

Published

2011

40. THINK AGAIN: THE BUSINESS OF ECONOMICS IS BUSINESS

Author

David Stout

Subjects

Economics, Econometrics and Finance (miscellaneous), Economics, Subject (philosophy), Business, Management and Accounting (miscellaneous), Marketing, Positive economics

Abstract

Advances in the subject have greatly developed the ways in which economists within a business can contribute to strategic decisions. In this 1997 article, David Stout draws on his experiences with Unilever to demonstrate the contribution economists can and should be making.

Published

2010

41. Plasticity of Cytochrome P450 2B4 as Investigated by Hydrogen-Deuterium Exchange Mass Spectrometry and X-ray Crystallography

Author

Qinghai Zhang, Tong Liu, P. Ross Wilderman, Simon Hsu, C. David Stout, Arthur G. Roberts, Sheng Li, Manish B. Shah, David R. Goodlett, James R. Halpert, and Virgil L. Woods

Subjects

Models, Molecular, Ligand, Chemistry, Deuterium Exchange Measurement, Cell Biology, Crystal structure, Crystallography, X-Ray, Mass spectrometry, Biochemistry, Mass Spectrometry, Protein Structure, Tertiary, Crystallography, Molecular dynamics, chemistry.chemical_compound, Protein structure, Protein Structure and Folding, Animals, Humans, Imidazole, Computer Simulation, Protein folding, Hydrogen–deuterium exchange, Aryl Hydrocarbon Hydroxylases, Cytochrome P450 Family 2, Molecular Biology

Abstract

Crystal structures of the xenobiotic metabolizing cytochrome P450 2B4 have demonstrated markedly different conformations in the presence of imidazole inhibitors or in the absence of ligand. However, knowledge of the plasticity of the enzyme in solution has remained scant. Thus, hydrogen-deuterium exchange mass spectrometry (DXMS) was utilized to probe the conformations of ligand-free P450 2B4 and the complex with 4-(4-chlorophenyl)imidazole (4-CPI) or 1-biphenyl-4-methyl-1H-imidazole (1-PBI). The results of DXMS indicate that the binding of 4-CPI slowed the hydrogen-deuterium exchange rate over the B′- and C-helices and portions of the F-G-helix cassette compared with P450 2B4 in the absence of ligands. In contrast, there was little difference between the ligand-free and 1-PBI-bound exchange sets. In addition, DXMS suggests that the ligand-free P450 2B4 is predominantly open in solution. Interestingly, a new high resolution structure of ligand-free P450 2B4 was obtained in a closed conformation very similar to the 4-CPI complex. Molecular dynamics simulations performed with the closed ligand-free structure as the starting point were used to probe the energetically accessible conformations of P450 2B4. The simulations were found to equilibrate to a conformation resembling the 1-PBI-bound P450 2B4 crystal structure. The results indicate that conformational changes observed in available crystal structures of the promiscuous xenobiotic metabolizing cytochrome P450 2B4 are consistent with its solution structural behavior.

Published

2010

42. KNOWLEDGE FLOW, INNOVATIVE CAPABILITIES AND BUSINESS SUCCESS: PERFORMANCE OF THE RELATIONSHIP BETWEEN SMALL WORLD NETWORKS TO PROMOTE INNOVATION

Author

Nitya Singh and Blaine David Stout

Subjects

Small-world network, Strategy and Management, Study methodology, 05 social sciences, Ethnic group, Subject matter, Knowledge flow, Management of Technology and Innovation, 0502 economics and business, Economics, 050207 economics, Business and International Management, Marketing, China, Research question, 050203 business & management

Abstract

The question of how innovation comes about, and the circumstances under which it prospers, is a question that has continued to be the focus of academic research on innovation creation. Recent works have focused on how the capacity to innovate hinges on the ability to form networks; hence, the importance of the research. The article therefore answers the research question of whether the network relationships between similar ethnic, education background, and geographically clustered groups plays a significant role in innovation creation or not? Using the theoretical concept of a Small World Network, we use case study methodology to study the origins of several companies from the technology sector, who in recent years have emerged as successful businesses. The article examines the small world network dimensions of ethnicity, education, geography and the binding subject matter interest that initially formed these relationships, as well as the impact that these relationships have on innovation creation and business success.

Published

2018

43. X-Ray Structures of the Hexameric Building Block of the HIV Capsid

Author

C. David Stout, Yuanzi Hua, Owen Pornillos, Barbie K. Ganser-Pornillos, Wesley I. Sundquist, Frank G. Whitby, Christopher P. Hill, Brian N. Kelly, and Mark Yeager

Subjects

Models, Molecular, MICROBIO, Viral protein, Polymers, viruses, Human immunodeficiency virus (HIV), Biology, 010402 general chemistry, medicine.disease_cause, Crystallography, X-Ray, 01 natural sciences, General Biochemistry, Genetics and Molecular Biology, Article, 03 medical and health sciences, Protein structure, Atomic resolution, medicine, 030304 developmental biology, 0303 health sciences, Rigid core, Extramural, Biochemistry, Genetics and Molecular Biology(all), Virology, 3. Good health, 0104 chemical sciences, Protein Structure, Tertiary, Capsid, Biophysics, HIV-1, Capsid Proteins

Abstract

SummaryThe mature capsids of HIV and other retroviruses organize and package the viral genome and its associated enzymes for delivery into host cells. The HIV capsid is a fullerene cone: a variably curved, closed shell composed of approximately 250 hexamers and exactly 12 pentamers of the viral CA protein. We devised methods for isolating soluble, assembly-competent CA hexamers and derived four crystallographically independent models that define the structure of this capsid assembly unit at atomic resolution. A ring of six CA N-terminal domains form an apparently rigid core, surrounded by an outer ring of C-terminal domains. Mobility of the outer ring appears to be an underlying mechanism for generating the variably curved lattice in authentic capsids. Hexamer-stabilizing interfaces are highly hydrated, and this property may be key to the formation of quasi-equivalent interactions within hexamers and pentamers. The structures also clarify the molecular basis for capsid assembly inhibition and should facilitate structure-based drug design strategies.

Published

2009

44. Crystal Structures of Cytochrome P450 2B4 in Complex with the Inhibitor 1-Biphenyl-4-methyl-1H-imidazole: Ligand-Induced Structural Response through α-Helical Repositioning

Author

Sean C. Gay, Ling Sun, Keiko Maekawa, James R. Halpert, and C. David Stout

Subjects

Stereochemistry, Bifonazole, Crystal structure, Crystallography, X-Ray, Ligands, Biochemistry, Protein Structure, Secondary, Article, chemistry.chemical_compound, Oxidoreductase, Catalytic Domain, medicine, Imidazole, Cytochrome P450 Family 2, Biphenyl, chemistry.chemical_classification, biology, Ligand, Escherichia coli Proteins, Biphenyl Compounds, Imidazoles, Active site, Biphenyl compound, Crystallography, chemistry, biology.protein, Aryl Hydrocarbon Hydroxylases, Protein Multimerization, Crystallization, Protein Binding, medicine.drug

Abstract

Two different ligand occupancy structures of cytochrome P450 2B4 (CYP2B4) in complex with 1-biphenyl-4-methyl-1H-imidazole (1-PBI) have been determined by X-ray crystallography. 1-PBI belongs to a series of tight binding, imidazole-based CYP2B4 inhibitors. 1-PBI binding to CYP2B4 yields a type II spectrum with a K(s) value of 0.23 microM and inhibits enzyme activity with an IC(50) value of 0.035 microM. Previous CYP2B4 structures have shown a large degree of structural movement in response to ligand size. With two phenyl rings, 1-PBI is larger than 1-(4-chlorophenyl)imidazole (1-CPI) and 4-(4-chlorophenyl)imidazole (4-CPI) but smaller than bifonazole, which is branched and contains three phenyl rings. The CYP2B4-1-PBI complex is a structural intermediate to the closed CPI and the open bifonazole structures. The B/C-loop reorganizes itself to include two short partial helices while closing one side of the active site. The F-G-helix cassette pivots over the I-helix in direct response to the size of the ligand in the active site. A cluster of Phe residues at the fulcrum of this pivot point allows for dramatic repositioning of the cassette with only a relatively small amount of secondary structure rearrangement. Comparisons of ligand-bound CYP2B4 structures reveal trends in plastic region mobility that could allow for predictions of their position in future structures based on ligand shape and size.

Published

2009

45. Recession in America and its World Wide Repercussion

Author

Randall Towner, David Stout, Ross Richmond, Antonio E. Morales-Pita, and Brian Cihlar

Subjects

World economy, Currency, media_common.quotation_subject, Economics, Credit crunch, Default, International economics, External debt, Recession, Global recession, Currency crisis, media_common

Abstract

The main objective of this paper is to analyze the influence of the American recession on the world economy, emphasizing that interdependence is both the cause and the possible solution to the global economic crisis. The paper is structured into five sections. The main conclusions indicate that the recession in America was basically due to domestic problems (the housing market slow down, over consumption and indebtedness of households partially due to the idiosyncrasy of the average American consumer and his reliance on housing and stock markets, the credit crunch resulting from the recession, and the banks' reluctance to lend after the defaults on the housing market and the credit industry). The situation was worsened by the twin deficits, and an increase in the foreign debt. Since most countries depend on America as their top export market and key location for capital outflows, the recession was extended to their economies. The paper also concludes that because of Chinese exports' role in the structure of its GDP and its dependence on American consumers, as well as China's role in funding the US deficits there is a mutual interdependence between China and the US. Despite America's present predicaments, the US dollar still remains as the primary currency in international trade.

Published

2009

46. Combined Microspectrophotometric and Crystallographic Examination of Chemically Reduced and X-ray Radiation-Reduced Forms of Cytochrome ba3 Oxidase from Thermus thermophilus: Structure of the Reduced Form of the Enzyme

Author

James A. Fee, Ying Chen, S. Michael Soltis, Tzanko Doukov, C. David Stout, and Bin Liu

Subjects

chemistry.chemical_classification, Oxidase test, biology, Chemistry, Stereochemistry, Thermus thermophilus, X-Rays, Cytochrome c, Electron Transport Complex IV, Crystallography, X-Ray, Cytochrome b Group, biology.organism_classification, Biochemistry, Article, Crystallography, Bacterial Proteins, Cytochrome C1, Oxidoreductase, Microspectrophotometry, biology.protein, Cytochrome c oxidase, Cytochrome aa3, Oxidation-Reduction

Abstract

In respiring organisms cytochrome c oxidase catalyzes proton translocation coupled to the reduction of O2 to water (1, 2). Cytochrome ba3 oxidase is one of two heme-copper oxidases isolated from T. thermophilus (3). It contains the dinuclear CuA center; a six-coordinated, low-spin, (6cLS) heme-B; and a (usually) five-coordinated, high-spin (5cHS) heme-As in close proximity to CuB ((3, 4) and references therein). The latter (heme-As and CuB) constitute the bimetallic site, and it is widely agreed that dioxygen binds to this site as the first step in O2-reduction and proton pumping. Two crystal structures of native and recombinant, oxidized ba3-type cytochrome c oxidase have been solved at

Published

2009

47. A Copper(I)-Catalyzed 1,2,3-Triazole Azide−Alkyne Click Compound Is a Potent Inhibitor of a Multidrug-Resistant HIV-1 Protease Variant

Author

Michael J. Giffin, John H. Elder, Ying-Chuan Lin, H. Heaslet, Chi-Huey Wong, Bruce E. Torbett, Ashraf Brik, C. David Stout, Gabrielle Cauvi, and Duncan E. McRee

Subjects

Models, Molecular, Azides, 1,2,3-Triazole, Stereochemistry, medicine.medical_treatment, Alkenes, Crystallography, X-Ray, Virus Replication, Article, Catalysis, Cell Line, chemistry.chemical_compound, Drug Resistance, Multiple, Viral, HIV Protease, HIV-1 protease, Drug Discovery, medicine, Protease inhibitor (pharmacology), Protease, Molecular Structure, biology, virus diseases, HIV Protease Inhibitors, Triazoles, Isoenzymes, Multiple drug resistance, Biochemistry, chemistry, Enzyme inhibitor, biology.protein, Click chemistry, Molecular Medicine, Azide, Copper, Protein Binding

Abstract

Treatment with HIV-1 protease inhibitors, a component of highly active antiretroviral therapy (HAART), often results in viral resistance. Structural and biochemical characterization of a 6X protease mutant arising from in vitro selection with compound 1, a C 2-symmetric diol protease inhibitor, has been previously described. We now show that compound 2, a copper(I)-catalyzed 1,2,3-triazole derived compound previously shown to be potently effective against wild-type protease (IC 50 = 6.0 nM), has low nM activity (IC 50 = 15.7 nM) against the multidrug-resistant 6X protease mutant. Compound 2 displays similar efficacy against wild-type and 6X HIV-1 in viral replication assays. While structural studies of compound 1 bound to wild type and mutant proteases revealed a progressive change in binding mode in the mutants, the 1.3 A resolution 6X protease-compound 2 crystal structure reveals nearly identical interactions for 2 as in the wild-type protease complex with very little change in compound 2 or protease conformation.

Published

2008

48. Crystal structures of substrate-bound and substrate-free cytochrome P450 46A1, the principal cholesterol hydroxylase in the brain

Author

Eric F. Johnson, Irina A. Pikuleva, Mark A. White, Natalia Mast, Ingemar Björkhem, and C. David Stout

Subjects

Brain Chemistry, Binding Sites, Multidisciplinary, biology, Protein Conformation, Chemistry, Cytochrome P450, Substrate (chemistry), Active site, Plasma protein binding, Biological Sciences, Crystallography, X-Ray, Ligands, Cholesterol 7 alpha-hydroxylase, Protein structure, Biochemistry, Steroid Hydroxylases, Cholesterol 24-Hydroxylase, biology.protein, Humans, Binding site, Cholesterol 24-hydroxylase, Protein Binding

Abstract

By converting cholesterol to 24S-hydroxycholesterol, cytochrome P450 46A1 (CYP46A1) initiates the major pathway for cholesterol removal from the brain. Two crystal structures of CYP46A1 were determined. First is the 1.9-Å structure of CYP46A1 complexed with a high-affinity substrate cholesterol 3-sulfate (CH-3S). The second structure is that of the substrate-free CYP46A1 at 2.4-Å resolution. CH-3S is bound in the productive orientation and occupies the entire length of the banana-shaped hydrophobic active-site cavity. A unique helix B′–C loop insertion (residues 116–120) contributes to positioning cholesterol for oxygenation catalyzed by CYP46A1. A comparison with the substrate-free structure reveals substantial substrate-induced conformational changes in CYP46A1 and suggests that structurally distinct compounds could bind in the enzyme active site. In vitro assays were performed to characterize the effect of different therapeutic agents on cholesterol hydroxylase activity of purified full-length recombinant CYP46A1, and several strong inhibitors and modest coactivators of CYP46A1 were identified. Structural and biochemical data provide evidence that CYP46A1 activity could be altered by exposure to some therapeutic drugs and potentially other xenobiotics.

Published

2008

49. Determinants of Cytochrome P450 2C8 Substrate Binding

Author

C. David Stout, Patrick M. Dansette, Stefaan Sansen, Eric F. Johnson, Guillaume A. Schoch, and Jason Yano

Subjects

biology, Chemistry, Stereochemistry, Active site, Substrate (chemistry), Cell Biology, Plasma protein binding, Biochemistry, chemistry.chemical_compound, Functional group, biology.protein, Molecule, Pharmacophore, Binding site, Molecular Biology, Heme

Abstract

Although a crystal structure and a pharmacophore model are available for cytochrome P450 2C8, the role of protein flexibility and specific ligand-protein interactions that govern substrate binding are poorly understood. X-ray crystal structures of P450 2C8 complexed with montelukast (2.8 A), troglitazone (2.7 A), felodipine (2.3 A), and 9-cis-retinoic acid (2.6 A) were determined to examine ligand-protein interactions for these chemically diverse compounds. Montelukast is a relatively large anionic inhibitor that exhibits a tripartite structure and complements the size and shape of the active-site cavity. The inhibitor troglitazone occupies the upper portion of the active-site cavity, leaving a substantial part of the cavity unoccupied. The smaller neutral felodipine molecule is sequestered with its dichlorophenyl group positioned close to the heme iron, and water molecules fill the distal portion of the cavity. The structure of the 9-cis-retinoic acid complex reveals that two substrate molecules bind simultaneously in the active site of P450 2C8. A second molecule of 9-cis-retinoic acid is located above the proximal molecule and can restrain the position of the latter for more efficient oxygenation. Solution binding studies do not discriminate between cooperative and noncooperative models for multiple substrate binding. The complexes with structurally distinct ligands further demonstrate the conformational adaptability of active site-constituting residues, especially Arg-241, that can reorient in the active-site cavity to stabilize a negatively charged functional group and define two spatially distinct binding sites for anionic moieties of substrates.

Published

2008

50. A Child Is Missing

Author

David Stout and David Stout

Subjects

Missing children--Fiction

Abstract

A newspaper editor in upstate New York is drawn into a deadly web of hatred and suspicion when he joins the hunt for a kidnapped little boy in this gritty and evocative thriller from an Edgar Award–winning authorLong Creek in New York's Hill County is an angry place—depressed, suspicious, and unforgiving. In the aftermath of a late-November snowstorm, one of the town's youngest citizens, five-year-old Jamie Brokow, the son of wealthy divorced parents, is abducted. His family pays the kidnappers their ransom, but the boy is never returned—and soon afterward, Fran Spicer, the local reporter covering the case, dies as the result of a mysterious car crash that the police are all too eager to attribute to alcohol. Will Schafer edits a newspaper in a neighboring county, and he's less willing to dismiss the death of his friend Spicer so easily. Schafer won't find much local support for his investigation, however—strangers like him are not welcome in Long Creek. Still, he is determined to uncover the truth and see that justice is served, for Fran and for little Jamie. But the hunt could have powerful, unanticipated consequences for everyone involved: Schafer, the townspeople, the police, the devastated family... and an odd, disfigured hermit, drawn from his solitude in the forest by the frightened cries of a small child in the night.

Published

2014