Your search keyword '"Underbakke ES"' showing total 21 results

1. Activation loop phosphorylation tunes conformational dynamics underlying Pyk2 tyrosine kinase activation

Author

Palhano Zanela, TM, primary, Woudenberg, A, additional, Romero Bello, KG, additional, and Underbakke, ES, additional

Published

2022

2. Mapping the Intersubunit Interdomain FMN-Heme Interactions in Neuronal Nitric Oxide Synthase by Targeted Quantitative Cross-Linking Mass Spectrometry.

Author

Jiang T, Wan G, Zhang H, Gyawali YP, Underbakke ES, and Feng C

Subjects

Animals, Rats, Binding Sites, Calmodulin metabolism, Calmodulin chemistry, Cross-Linking Reagents chemistry, Models, Molecular, Protein Binding, Protein Domains, Flavin Mononucleotide metabolism, Flavin Mononucleotide chemistry, Heme metabolism, Heme chemistry, Mass Spectrometry, Nitric Oxide Synthase Type I metabolism, Nitric Oxide Synthase Type I chemistry

Abstract

Nitric oxide synthase (NOS) in mammals is a family of multidomain proteins in which interdomain electron transfer (IET) is controlled by domain-domain interactions. Calmodulin (CaM) binds to the canonical CaM-binding site in the linker region between the FMN and heme domains of NOS and allows tethered FMN domain motions, enabling an intersubunit FMN-heme IET in the output state for NO production. Our previous cross-linking mass spectrometric (XL MS) results demonstrated site-specific protein dynamics in the CaM-responsive regions of rat neuronal NOS (nNOS) reductase construct, a monomeric protein [Jiang et al., Biochemistry , 2023, 62, 2232-2237]. In this work, we have extended our combined approach of XL MS structural mapping and AlphaFold structural prediction to examine the homodimeric nNOS oxygenase/FMN (oxyFMN) construct, an established model of the NOS output state. We employed parallel reaction monitoring (PRM) based quantitative XL MS (qXL MS) to assess the CaM-induced changes in interdomain dynamics and interactions. Intersubunit cross-links were identified by mapping the cross-links onto top AlphaFold structural models, which was complemented by comparing their relative abundances in the cross-linked dimeric and monomeric bands. Furthermore, contrasting the CaM-free and CaM-bound nNOS samples shows that CaM enables the formation of the intersubunit FMN-heme docking complex and that CaM binding induces extensive, allosteric conformational changes across the NOS regions. Moreover, the observed cross-links sites specifically respond to changes in ionic strength. This indicates that interdomain salt bridges are responsible for stabilizing and orienting the output state for efficient FMN-heme IET. Taken together, our targeted qXL MS results have revealed that CaM and ionic strength modulate specific dynamic changes in the CaM/FMN/heme complexes, particularly in the context of intersubunit interdomain FMN-heme interactions.

Published

2024

3. Molecularly imprinted nanoparticles reveal regulatory scaffolding features in Pyk2 tyrosine kinase.

Author

Zanela TMP, Zangiabadi M, Zhao Y, and Underbakke ES

Abstract

Pyk2 is a multi-domain non-receptor tyrosine kinase that serves dual roles as a signaling enzyme and scaffold. Pyk2 activation involves a multi-stage cascade of conformational rearrangements and protein interactions initiated by autophosphorylation of a linker site. Linker phosphorylation recruits Src kinase, and Src-mediated phosphorylation of the Pyk2 activation loop confers full activation. The regulation and accessibility of the initial Pyk2 autophosphorylation site remains unclear. We employed peptide-binding molecularly imprinted nanoparticles (MINPs) to probe the regulatory conformations controlling Pyk2 activation. MINPs differentiating local structure and phosphorylation state revealed that the Pyk2 autophosphorylation site is protected in the autoinhibited state. Activity profiling of Pyk2 variants implicated FERM and linker residues responsible for constraining the autophosphorylation site. MINPs targeting each Src docking site disrupt the higher-order kinase interactions critical for activation complex maturation. Ultimately, MINPs targeting key regulatory motifs establish a useful toolkit for probing successive activational stages in the higher-order Pyk2 signaling complex., Competing Interests: The authors declare no competing interests., (This journal is © The Royal Society of Chemistry.)

Published

2024

4. Probing Protein Dynamics in Neuronal Nitric Oxide Synthase by Quantitative Cross-Linking Mass Spectrometry.

Author

Jiang T, Wan G, Zhang H, Gyawali YP, Underbakke ES, and Feng C

Abstract

Nitric oxide synthase (NOS) is responsible for the biosynthesis of nitric oxide (NO), an important signaling molecule controlling diverse physiological processes such as neurotransmission and vasodilation. Neuronal NOS (nNOS) is a calmodulin (CaM)-controlled enzyme. In the absence of CaM, several intrinsic control elements, along with NADP + binding, suppress electron transfer across the NOS domains. CaM binding relieves the inhibitory factors to promote the electron transport required for NO production. The regulatory dynamics of nNOS control elements are critical to governing NO signaling, yet mechanistic questions remain, because the intrinsic dynamics of NOS thwart traditional structural biology approaches. Here, we have employed cross-linking mass spectrometry (XL MS) to probe regulatory dynamics in nNOS, focusing on the CaM-responsive control elements. Quantitative XL MS revealed conformational changes differentiating the nNOS reductase (nNOSred) alone, nNOSred with NADP + , nNOS-CaM, and nNOS-CaM with NADP + . We observed distinct effects of CaM vs NADP + on cross-linking patterns in nNOSred. CaM induces striking global changes, while the impact of NADP + is primarily localized to the NADPH-binding subdomain. Moreover, CaM increases the abundance of intra-nNOS cross-links that are related to the formation of the inter-CaM-nNOS cross-links. Taken together, these XL MS results demonstrate that CaM and NADP + site-specifically alter the nNOS conformational landscape.

Published

2023

5. Activation loop phosphorylation tunes conformational dynamics underlying Pyk2 tyrosine kinase activation.

Author

Palhano Zanela TM, Woudenberg A, Romero Bello KG, and Underbakke ES

Subjects

Phosphorylation, src-Family Kinases genetics, src-Family Kinases metabolism, Molecular Conformation, Focal Adhesion Kinase 2 genetics, Focal Adhesion Kinase 2 chemistry, Focal Adhesion Kinase 2 metabolism, Tyrosine metabolism

Abstract

Pyk2 is a multidomain non-receptor tyrosine kinase that undergoes a multistage activation mechanism. Activation is instigated by conformational rearrangements relieving autoinhibitory FERM domain interactions. The kinase autophosphorylates a central linker residue to recruit Src kinase. Pyk2 and Src mutually phosphorylate activation loops to confer full activation. While the mechanisms of autoinhibition are established, the conformational dynamics associated with autophosphorylation and Src recruitment remain unclear. We employ hydrogen/deuterium exchange mass spectrometry and kinase activity profiling to map the conformational dynamics associated with substrate binding and Src-mediated activation loop phosphorylation. Nucleotide engagement stabilizes the autoinhibitory interface, while phosphorylation deprotects both FERM and kinase regulatory surfaces. Phosphorylation organizes active site motifs linking catalytic loop with activation segment. Dynamics of the activation segment anchor propagate to EF/G helices to prevent reversion of the autoinhibitory FERM interaction. We employ targeted mutagenesis to dissect how phosphorylation-induced conformational rearrangements elevate kinase activity above the basal autophosphorylation rate., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2023 Elsevier Ltd. All rights reserved.)

Published

2023

6. Intricate coupling between the transactivation and basic-leucine zipper domains governs phosphorylation of transcription factor ATF4 by casein kinase 2.

Author

Siang S, Underbakke ES, and Roche J

Subjects

Phosphorylation, Transcriptional Activation, Activating Transcription Factor 4 genetics, Activating Transcription Factor 4 metabolism, Casein Kinase II genetics, Casein Kinase II metabolism, Leucine Zippers

Abstract

Most transcription factors possess at least one long intrinsically disordered transactivation domain that binds to a variety of coactivators and corepressors and plays a key role in modulating the transcriptional activity. Despite the crucial importance of these domains, the structural and functional basis of transactivation remains poorly understood. Here, we focused on activating transcription factor 4 (ATF4)/cAMP response element-binding protein-2, an essential transcription factor for cellular stress adaptation. Bioinformatic sequence analysis of the ATF4 transactivation domain sequence revealed that the first 125 amino acids have noticeably less propensity for structural disorder than the rest of the domain. Using solution nuclear magnetic resonance spectroscopy complemented by a range of biophysical methods, we found that the isolated transactivation domain is predominantly yet not fully disordered in solution. We also observed that a short motif at the N-terminus of the transactivation domain has a high helical propensity. Importantly, we found that the N-terminal region of the transactivation domain is involved in transient long-range interactions with the basic-leucine zipper domain involved in DNA binding. Finally, in vitro phosphorylation assays with the casein kinase 2 show that the presence of the basic-leucine zipper domain is required for phosphorylation of the transactivation domain. This study uncovers the intricate coupling existing between the transactivation and basic-leucine zipper domains of ATF4, highlighting its potential regulatory significance., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2022 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2022

7. Structural basis for ALK2/BMPR2 receptor complex signaling through kinase domain oligomerization.

Author

Agnew C, Ayaz P, Kashima R, Loving HS, Ghatpande P, Kung JE, Underbakke ES, Shan Y, Shaw DE, Hata A, and Jura N

Subjects

Activin Receptors, Type I genetics, Bone Morphogenetic Protein Receptors metabolism, Bone Morphogenetic Protein Receptors, Type II genetics, Bone Morphogenetic Proteins metabolism, Familial Primary Pulmonary Hypertension metabolism, Humans, Ligands, Models, Molecular, Mutation, Phosphorylation, Protein Binding, Protein Domains, Pulmonary Arterial Hypertension, Scattering, Small Angle, Signal Transduction genetics, Smad Proteins metabolism, X-Ray Diffraction, Activin Receptors, Type I chemistry, Activin Receptors, Type I metabolism, Bone Morphogenetic Protein Receptors, Type II chemistry, Bone Morphogenetic Protein Receptors, Type II metabolism, Signal Transduction physiology

Abstract

Upon ligand binding, bone morphogenetic protein (BMP) receptors form active tetrameric complexes, comprised of two type I and two type II receptors, which then transmit signals to SMAD proteins. The link between receptor tetramerization and the mechanism of kinase activation, however, has not been elucidated. Here, using hydrogen deuterium exchange mass spectrometry (HDX-MS), small angle X-ray scattering (SAXS) and molecular dynamics (MD) simulations, combined with analysis of SMAD signaling, we show that the kinase domain of the type I receptor ALK2 and type II receptor BMPR2 form a heterodimeric complex via their C-terminal lobes. Formation of this dimer is essential for ligand-induced receptor signaling and is targeted by mutations in BMPR2 in patients with pulmonary arterial hypertension (PAH). We further show that the type I/type II kinase domain heterodimer serves as the scaffold for assembly of the active tetrameric receptor complexes to enable phosphorylation of the GS domain and activation of SMADs., (© 2021. The Author(s).)

Published

2021

8. Controlling Kinase Activities by Selective Inhibition of Peptide Substrates.

Author

Li X, Palhano Zanela TM, Underbakke ES, and Zhao Y

Subjects

Humans, Models, Molecular, Molecular Structure, Peptides chemistry, Phosphorylation, Phosphotransferases metabolism, Protein Processing, Post-Translational, Substrate Specificity, Peptides pharmacology, Phosphotransferases antagonists & inhibitors

Abstract

Phosphorylation is the most common reversible post-translational modification (PTM) of proteins. Because a given kinase often has many substrates in a cell and is involved in numerous functions, traditional inhibition of the enzyme leads to unintended consequences. Here we report synthetic receptors to manipulate kinase phosphorylation precisely for the first time, utilizing the receptors' abilities to bind peptides with high affinity and specificity. The inhibition enables selective phosphorylation of peptides with identical consensus motifs in a mixture. A particular phosphosite can be inhibited while other sites in the same substrate undergo phosphorylation. The receptors may work either individually on their targeted strands or in concert to protect segments of a long sequence. The binding-derived inhibition is able to compete with protein-protein interactions within a multidomain kinase, enabling controlled PTM to be performed in a previously unavailable manner.

Published

2021

9. N-terminal fusion of the N-terminal domain of bacterial enzyme I facilitates recombinant expression and purification of the human RNA demethylases FTO and Alkbh5.

Author

Khatiwada B, Purslow JA, Underbakke ES, and Venditti V

Subjects

Bacterial Proteins chemistry, Bacterial Proteins genetics, Chromatography, Liquid methods, Escherichia coli genetics, Expressed Sequence Tags, Mass Spectrometry methods, Protein Engineering methods, Recombinant Proteins, Solubility, AlkB Homolog 5, RNA Demethylase biosynthesis, AlkB Homolog 5, RNA Demethylase isolation & purification, Alpha-Ketoglutarate-Dependent Dioxygenase FTO biosynthesis, Alpha-Ketoglutarate-Dependent Dioxygenase FTO isolation & purification, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics

Abstract

Various fusion tags are commonly employed to increase the heterologous expression and solubility of aggregation-prone proteins within Escherichia coli. Herein, we present a protocol for efficient recombinant expression and purification of the human RNA demethylases Alkbh5 and FTO. Our method incorporates a novel fusion tag (the N-terminal domain of bacterial enzyme I, EIN) that dramatically increases the solubility of its fusion partner and is promptly removed upon digestion with a protease. The presented protocol allows for the production of mg amounts of Alkbh5 and FTO in 1L of both rich and minimal media. We developed a liquid chromatography-mass spectrometry (LC-MS)-based assay to confirm that both proteins are enzymatically active. Furthermore, the LC-MS method developed here is applicable to other members of the AlkB family of Fe(II)/α-ketoglutarate-dependent dioxygenases. The superior protein yield, afforded by our expression and purification method, will facilitate biochemical investigations into the biological function of the human RNA demethylases and endorse employment of EIN as a broadly applicable fusion tag for recombinant expression projects., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2020

10. Conformational Dynamics of FERM-Mediated Autoinhibition in Pyk2 Tyrosine Kinase.

Author

Loving HS and Underbakke ES

Subjects

Amino Acid Sequence, Amino Acid Substitution, Enzyme Assays, Focal Adhesion Kinase 2 genetics, Humans, Mutation, Protein Conformation, Focal Adhesion Kinase 2 antagonists & inhibitors, Focal Adhesion Kinase 2 chemistry, Protein Domains

Abstract

Pyk2 is a non-receptor tyrosine kinase that evolved from gene duplication of focal adhesion kinase (FAK) and subsequent functional specialization in the brain and hemopoietic cells. Pyk2 shares a domain organization with FAK, with an N-terminal regulatory FERM domain adjoining the kinase domain. FAK regulation involves integrin-mediated membrane clustering to relieve autoinhibitory interactions between FERM and kinase domains. Pyk2 regulation remains cryptic, involving Ca 2+ influx and protein scaffolding. While the mechanism of the FAK FERM domain in autoinhibition is well-established, the regulatory role of the Pyk2 FERM is ambiguous. We probed the mechanisms of FERM-mediated autoinhibition of Pyk2 using hydrogen/deuterium exchange mass spectrometry and kinase activity profiling. The results reveal FERM-kinase interfaces that are responsible for autoinhibition. Pyk2 autoinhibition impacts the activation loop conformation. In addition, the autoinhibitory FERM-kinase interface exhibits allosteric linkage with the FERM basic patch conserved in both FAK and Pyk2.

Published

2019

11. Recommendations for performing, interpreting and reporting hydrogen deuterium exchange mass spectrometry (HDX-MS) experiments.

Author

Masson GR, Burke JE, Ahn NG, Anand GS, Borchers C, Brier S, Bou-Assaf GM, Engen JR, Englander SW, Faber J, Garlish R, Griffin PR, Gross ML, Guttman M, Hamuro Y, Heck AJR, Houde D, Iacob RE, Jørgensen TJD, Kaltashov IA, Klinman JP, Konermann L, Man P, Mayne L, Pascal BD, Reichmann D, Skehel M, Snijder J, Strutzenberg TS, Underbakke ES, Wagner C, Wales TE, Walters BT, Weis DD, Wilson DJ, Wintrode PL, Zhang Z, Zheng J, Schriemer DC, and Rand KD

Subjects

Data Analysis, Hydrogen-Ion Concentration, Deuterium Exchange Measurement methods, Mass Spectrometry methods

Abstract

Hydrogen deuterium exchange mass spectrometry (HDX-MS) is a powerful biophysical technique being increasingly applied to a wide variety of problems. As the HDX-MS community continues to grow, adoption of best practices in data collection, analysis, presentation and interpretation will greatly enhance the accessibility of this technique to nonspecialists. Here we provide recommendations arising from community discussions emerging out of the first International Conference on Hydrogen-Exchange Mass Spectrometry (IC-HDX; 2017). It is meant to represent both a consensus viewpoint and an opportunity to stimulate further additions and refinements as the field advances.

Published

2019

12. Calmodulin-induced Conformational Control and Allostery Underlying Neuronal Nitric Oxide Synthase Activation.

Author

Hanson QM, Carley JR, Gilbreath TJ, Smith BC, and Underbakke ES

Subjects

Allosteric Regulation, Catalytic Domain, Deuterium Exchange Measurement, Enzyme Activation, Humans, Protein Conformation, Calmodulin metabolism, Nitric Oxide Synthase Type I chemistry, Nitric Oxide Synthase Type I metabolism

Abstract

Nitric oxide synthase (NOS) is the primary generator of nitric oxide signals controlling diverse physiological processes such as neurotransmission and vasodilation. NOS activation is contingent on Ca 2+ /calmodulin binding at a linker between its oxygenase and reductase domains to induce large conformational changes that orchestrate inter-domain electron transfer. However, the structural dynamics underlying activation of full-length NOS remain ambiguous. Employing hydrogen-deuterium exchange mass spectrometry, we reveal mechanisms underlying neuronal NOS activation by calmodulin and regulation by phosphorylation. We demonstrate that calmodulin binding orders the junction between reductase and oxygenase domains, exposes the FMN subdomain, and elicits a more dynamic oxygenase active site. Furthermore, we demonstrate that phosphorylation partially mimics calmodulin activation to modulate neuronal NOS activity via long-range allostery. Calmodulin binding and phosphorylation ultimately promote a more dynamic holoenzyme while coordinating inter-domain communication and electron transfer., (Copyright © 2018 Elsevier Ltd. All rights reserved.)

Published

2018

13. Nitric oxide-induced conformational changes in soluble guanylate cyclase.

Author

Underbakke ES, Iavarone AT, Chalmers MJ, Pascal BD, Novick S, Griffin PR, and Marletta MA

Subjects

Amino Acid Sequence, Catalytic Domain, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Guanylate Cyclase genetics, Humans, Models, Molecular, Molecular Sequence Data, Protein Binding, Protein Folding, Protein Multimerization, Protein Structure, Secondary, Protein Subunits genetics, Receptors, Cytoplasmic and Nuclear genetics, Recombinant Proteins chemistry, Recombinant Proteins genetics, Soluble Guanylyl Cyclase, Cyclic GMP chemistry, Guanylate Cyclase chemistry, Nitric Oxide chemistry, Protein Subunits chemistry, Receptors, Cytoplasmic and Nuclear chemistry

Abstract

Soluble guanylate cyclase (sGC) is the primary mediator of nitric oxide (NO) signaling. NO binds the sGC heme cofactor stimulating synthesis of the second messenger cyclic-GMP (cGMP). As the central hub of NO/cGMP signaling pathways, sGC is important in diverse physiological processes such as vasodilation and neurotransmission. Nevertheless, the mechanisms underlying NO-induced cyclase activation in sGC remain unclear. Here, hydrogen/deuterium exchange mass spectrometry (HDX-MS) was employed to probe the NO-induced conformational changes of sGC. HDX-MS revealed NO-induced effects in several discrete regions. NO binding to the heme-NO/O2-binding (H-NOX) domain perturbs a signaling surface implicated in Per/Arnt/Sim (PAS) domain interactions. Furthermore, NO elicits striking conformational changes in the junction between the PAS and helical domains that propagate as perturbations throughout the adjoining helices. Ultimately, NO binding stimulates the catalytic domain by contracting the active site pocket. Together, these conformational changes delineate an allosteric pathway linking NO binding to activation of the catalytic domain., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published

2014

14. Single-particle EM reveals the higher-order domain architecture of soluble guanylate cyclase.

Author

Campbell MG, Underbakke ES, Potter CS, Carragher B, and Marletta MA

Subjects

Animals, Cloning, Molecular, Enzyme Activators metabolism, Guanylate Cyclase metabolism, Image Processing, Computer-Assisted, Microscopy, Electron, Transmission, Protein Binding, Protein Structure, Tertiary, Rats, Receptors, Cytoplasmic and Nuclear metabolism, Soluble Guanylyl Cyclase, Guanylate Cyclase chemistry, Guanylate Cyclase ultrastructure, Models, Molecular, Protein Conformation, Receptors, Cytoplasmic and Nuclear chemistry, Receptors, Cytoplasmic and Nuclear ultrastructure

Abstract

Soluble guanylate cyclase (sGC) is the primary nitric oxide (NO) receptor in mammals and a central component of the NO-signaling pathway. The NO-signaling pathways mediate diverse physiological processes, including vasodilation, neurotransmission, and myocardial functions. sGC is a heterodimer assembled from two homologous subunits, each comprised of four domains. Although crystal structures of isolated domains have been reported, no structure is available for full-length sGC. We used single-particle electron microscopy to obtain the structure of the complete sGC heterodimer and determine its higher-order domain architecture. Overall, the protein is formed of two rigid modules: the catalytic dimer and the clustered Per/Art/Sim and heme-NO/O2-binding domains, connected by a parallel coiled coil at two hinge points. The quaternary assembly demonstrates a very high degree of flexibility. We captured hundreds of individual conformational snapshots of free sGC, NO-bound sGC, and guanosine-5'-[(α,β)-methylene]triphosphate-bound sGC. The molecular architecture and pronounced flexibility observed provides a significant step forward in understanding the mechanism of NO signaling.

Published

2014

15. Nitric oxide synthase domain interfaces regulate electron transfer and calmodulin activation.

Author

Smith BC, Underbakke ES, Kulp DW, Schief WR, and Marletta MA

Subjects

Animals, Calmodulin metabolism, Deuterium Exchange Measurement, Dimerization, Electron Transport, Electrophoresis, Polyacrylamide Gel, Flavin Mononucleotide metabolism, Flavin-Adenine Dinucleotide metabolism, Fluorescence, Heme metabolism, Mass Spectrometry, Nitric Oxide Synthase Type II genetics, Nitric Oxide Synthase Type II metabolism, Species Specificity, Calmodulin chemistry, Models, Molecular, Nitric Oxide Synthase Type II chemistry, Protein Conformation

Abstract

Nitric oxide (NO) produced by NO synthase (NOS) participates in diverse physiological processes such as vasodilation, neurotransmission, and the innate immune response. Mammalian NOS isoforms are homodimers composed of two domains connected by an intervening calmodulin-binding region. The N-terminal oxidase domain binds heme and tetrahydrobiopterin and the arginine substrate. The C-terminal reductase domain binds FAD and FMN and the cosubstrate NADPH. Although several high-resolution structures of individual NOS domains have been reported, a structure of a NOS holoenzyme has remained elusive. Determination of the higher-order domain architecture of NOS is essential to elucidate the molecular underpinnings of NO formation. In particular, the pathway of electron transfer from FMN to heme, and the mechanism through which calmodulin activates this electron transfer, are largely unknown. In this report, hydrogen-deuterium exchange mass spectrometry was used to map critical NOS interaction surfaces. Direct interactions between the heme domain, the FMN subdomain, and calmodulin were observed. These interaction surfaces were confirmed by kinetic studies of site-specific interface mutants. Integration of the hydrogen-deuterium exchange mass spectrometry results with computational docking resulted in models of the NOS heme and FMN subdomain bound to calmodulin. These models suggest a pathway for electron transfer from FMN to heme and a mechanism for calmodulin activation of this critical step.

Published

2013

16. Higher-order interactions bridge the nitric oxide receptor and catalytic domains of soluble guanylate cyclase.

Author

Underbakke ES, Iavarone AT, and Marletta MA

Subjects

Catalysis, Cyclic GMP metabolism, Deuterium Exchange Measurement, Kinetics, Mass Spectrometry, Nitric Oxide metabolism, Protein Structure, Tertiary, Soluble Guanylyl Cyclase, Guanylate Cyclase chemistry, Guanylate Cyclase metabolism, Models, Molecular, Receptors, Cytoplasmic and Nuclear chemistry, Receptors, Cytoplasmic and Nuclear metabolism, Signal Transduction physiology

Abstract

Nitric oxide (NO) signaling pathways mediate diverse physiological functions, including vasodilation and neurotransmission. Soluble guanylate cyclase (sGC), the primary NO receptor, triggers downstream signaling cascades by producing the second messenger cGMP. NO binds the sGC heme cofactor to stimulate cyclase activity, yet the molecular mechanisms of cyclase activation remain obscure. Although structural models of the individual sGC domains are available, the structure of the full sGC heterodimer is unknown. Understanding the higher-order domain architecture of sGC is a prerequisite to elucidating the mechanisms of NO activation. We used protein footprinting to map interdomain interaction surfaces of the sGC signaling domains. Hydrogen/deuterium exchange mass spectrometry revealed direct interactions between the Per/Arnt/Sim domain and the heme-associated signaling helix of the heme-NO/O2 binding (H-NOX) domain. Furthermore, interfaces between the H-NOX and catalytic domains were mapped using domain truncations and full-length sGC. The H-NOX domain buries surfaces of the α1 catalytic domain proximal to the cyclase active site, suggesting a signaling mechanism involving NO-induced derepression of catalytic activity. Together, our data reveal interdomain interactions responsible for communicating NO occupancy from H-NOX heme to the catalytic domain active site.

Published

2013

17. Heme-assisted S-nitrosation desensitizes ferric soluble guanylate cyclase to nitric oxide.

Author

Fernhoff NB, Derbyshire ER, Underbakke ES, and Marletta MA

Subjects

Alkylation, Animals, Catalytic Domain, Cysteine metabolism, Guanylate Cyclase chemistry, Humans, Hydroxides metabolism, Kinetics, Mutant Proteins metabolism, Nitrosation, Nucleotides metabolism, Oxidation-Reduction, Protein Binding, Rats, Receptors, Cytoplasmic and Nuclear chemistry, Soluble Guanylyl Cyclase, Sulfhydryl Compounds metabolism, Guanylate Cyclase metabolism, Heme metabolism, Iron metabolism, Nitric Oxide metabolism, Receptors, Cytoplasmic and Nuclear metabolism

Abstract

Nitric oxide (NO) signaling regulates key processes in cardiovascular physiology, specifically vasodilation, platelet aggregation, and leukocyte rolling. Soluble guanylate cyclase (sGC), the mammalian NO sensor, transduces an NO signal into the classical second messenger cyclic GMP (cGMP). NO binds to the ferrous (Fe(2+)) oxidation state of the sGC heme cofactor and stimulates formation of cGMP several hundred-fold. Oxidation of the sGC heme to the ferric (Fe(3+)) state desensitizes the enzyme to NO. The heme-oxidized state of sGC has emerged as a potential therapeutic target in the treatment of cardiovascular disease. Here, we investigate the molecular mechanism of NO desensitization and find that sGC undergoes a reductive nitrosylation reaction that is coupled to the S-nitrosation of sGC cysteines. We further characterize the kinetics of NO desensitization and find that heme-assisted nitrosothiol formation of β1Cys-78 and β1Cys-122 causes the NO desensitization of ferric sGC. Finally, we provide evidence that the mechanism of reductive nitrosylation is gated by a conformational change of the protein. These results yield insights into the function and dysfunction of sGC in cardiovascular disease.

Published

2012

18. Protein footprinting in a complex milieu: identifying the interaction surfaces of the chemotaxis adaptor protein CheW.

Author

Underbakke ES, Zhu Y, and Kiessling LL

Subjects

Bacterial Proteins chemistry, Bacterial Proteins metabolism, Chemotaxis physiology, Cysteine chemistry, Escherichia coli physiology, Escherichia coli Proteins metabolism, Histidine Kinase, Mass Spectrometry methods, Membrane Proteins chemistry, Membrane Proteins metabolism, Methyl-Accepting Chemotaxis Proteins, Models, Molecular, Protein Structure, Tertiary, Signal Transduction physiology, Escherichia coli Proteins chemistry, Isotope Labeling methods, Protein Footprinting methods, Protein Interaction Mapping methods

Abstract

Characterizing protein-protein interactions in a biologically relevant context is important for understanding the mechanisms of signal transduction. Most signal transduction systems are membrane associated and consist of large multiprotein complexes that undergo rapid reorganization--circumstances that present challenges to traditional structure determination methods. To study protein-protein interactions in a biologically relevant complex milieu, we employed a protein footprinting strategy based on isotope-coded affinity tag (ICAT) reagents. ICAT reagents are valuable tools for proteomics. Here, we show their utility in an alternative application--they are ideal for protein footprinting in complex backgrounds because the affinity tag moiety allows for enrichment of alkylated species prior to analysis. We employed a water-soluble ICAT reagent to monitor cysteine accessibility and thereby to identify residues involved in two different protein-protein interactions in the Escherichia coli chemotaxis signaling system. The chemotaxis system is an archetypal transmembrane signaling pathway in which a complex protein superstructure underlies sophisticated sensory performance. The formation of this superstructure depends on the adaptor protein CheW, which mediates a functionally important bridging interaction between transmembrane receptors and histidine kinase. ICAT footprinting was used to map the surfaces of CheW that interact with the large multidomain histidine kinase CheA, as well as with the transmembrane chemoreceptor Tsr in native E. coli membranes. By leveraging the affinity tag, we successfully identified CheW surfaces responsible for CheA-Tsr interaction. The proximity of the CheA and Tsr binding sites on CheW suggests the formation of a composite CheW-Tsr surface for the recruitment of the signaling kinase to the chemoreceptor complex., (Copyright © 2011 Elsevier Ltd. All rights reserved.)

Published

2011

19. Classifying chemoreceptors: quantity versus quality.

Author

Underbakke ES and Kiessling LL

Subjects

Bacteria metabolism, Chemoreceptor Cells metabolism, Chemotaxis physiology, Signal Transduction physiology, Chemoreceptor Cells classification

Published

2010

20. Isotope-coded affinity tags with tunable reactivities for protein footprinting.

Author

Underbakke ES, Zhu Y, and Kiessling LL

Subjects

Alkylation, Bacterial Proteins chemistry, Molecular Probes chemical synthesis, Protein Conformation, Protein Folding, Trypsin chemistry, Cysteine chemistry, Isotope Labeling, Molecular Probes chemistry, Protein Footprinting, Protein Interaction Mapping

Published

2008

21. Solid-phase synthesis of polymers using the ring-opening metathesis polymerization.

Author

Pontrello JK, Allen MJ, Underbakke ES, and Kiessling LL

Subjects

Esters chemistry, Immobilization, Molecular Structure, Polymers chemical synthesis

Abstract

We report a general method for the solid-phase synthesis of polymers via the ring-opening metathesis polymerization (ROMP). The method involves polymerization in solution to form a block copolymer, immobilization of the polymer via reaction of one block with a resin-bound functional group, modification of the other block, and liberation of the polymer from the resin. We demonstrated the utility of this approach by generating a block copolymer with an N-hydroxysuccinimidyl ester-substituted block (for on-resin functionalization) and a maleimide-substituted block (for conjugation to the resin). We showed that the Diels-Alder reaction can be employed to immobilize the polymers and that amines of diverse structure can be used to modify the resin-bound polymers. The reversibility of the furan-maleimide Diels-Alder adduct was exploited to liberate the polymer from the support. Specifically, treatment of the resin with cyclopentadiene resulted in complete polymer release. The resulting polymers are functional: they were as potent in assays with the lectin concanavalin A as polymers generated by traditional solution routes. We anticipate that this method can be used for the rapid synthesis of diverse polymers via ROMP.

Published

2005