Your search keyword '"Thompson PR"' showing total 18 results

1. Development of a Suicide Inhibition-Based Protein Labeling Strategy for Nicotinamide N-Methyltransferase.

Author

Sen S, Mondal S, Zheng L, Salinger AJ, Fast W, Weerapana E, and Thompson PR

Subjects

Catalysis, HEK293 Cells, Humans, Kinetics, Methylation, Nicotinamide N-Methyltransferase antagonists & inhibitors, Nicotinamide N-Methyltransferase metabolism, Proteins metabolism

Abstract

Nicotinamide N-methyltransferase (NNMT) catalyzes the S-adenosyl-l-methionine-dependent methylation of nicotinamide to form N-methylnicotinamide. This enzyme detoxifies xenobiotics and regulates NAD + biosynthesis. Additionally, NNMT is overexpressed in various cancers. Herein, we describe the first NNMT-targeted suicide substrates. These compounds, which include 4-chloropyridine and 4-chloronicotinamide, exploit the broad substrate scope of NNMT; methylation of the pyridine nitrogen enhances the electrophilicity of the C4 position, thereby promoting an aromatic nucleophilic substitution by C159, a noncatalytic cysteine. On the basis of this activity, we developed a suicide inhibition-based protein labeling strategy using an alkyne-substituted 4-chloropyridine that selectively labels NNMT in vitro and in cells. In total, this study describes the first NNMT-directed activity-based probes.

Published

2019

2. Citrullination Inactivates Nicotinamide- N-methyltransferase.

Author

Nemmara VV, Tilvawala R, Salinger AJ, Miller L, Nguyen SH, Weerapana E, and Thompson PR

Subjects

Enzyme Activation, Humans, Kinetics, Methylation, Models, Molecular, Mutagenesis, Site-Directed, Niacinamide analogs & derivatives, Niacinamide metabolism, Nicotinamide N-Methyltransferase chemistry, Nicotinamide N-Methyltransferase genetics, Protein Conformation, Citrullination, Nicotinamide N-Methyltransferase metabolism

Abstract

Nicotinamide- N-methyltransferase (NNMT) catalyzes the irreversible methylation of nicotinamide (NAM) to form N-methyl nicotinamide using S-adenosyl methionine as a methyl donor. NNMT is implicated in several chronic disease conditions, including cancers, kidney disease, cardiovascular disease, and Parkinson's disease. Although phosphorylation of NNMT in gastric tumors is reported, the functional effects of this post-translational modification has not been investigated. We previously reported that citrullination of NNMT by Protein Arginine Deiminases abolished its methyltransferase activity. Herein, we investigate the mechanism of inactivation. Using tandem mass spectrometry, we identified three sites of citrullination in NNMT. With this information in hand, we used a combination of site-directed mutagenesis, kinetics, and circular dichoism experiments to demonstrate that citrullination of R132 leads to a structural perturbation that ultimately promotes NNMT inactivation.

Published

2018

3. Photochemical Control of Protein Arginine Deiminase (PAD) Activity.

Author

Mondal S, Parelkar SS, Nagar M, and Thompson PR

Subjects

Azo Compounds, Enzyme Inhibitors pharmacology, Humans, Hydrolases, Isomerism, Ornithine analogs & derivatives, Protein-Arginine Deiminase Type 1, Protein-Arginine Deiminase Type 2, Protein-Arginine Deiminases metabolism, Photochemical Processes, Protein-Arginine Deiminases antagonists & inhibitors

Abstract

Protein arginine deiminases (PADs) play an important role in the pathogenesis of various diseases, including rheumatoid arthritis, multiple sclerosis, lupus, ulcerative colitis, and breast cancer. Therefore, the development of PAD inhibitors has drawn significant research interest in recent years. Herein, we describe the development of the first photoswitchable PAD inhibitors. These compounds possess an azobenzene photoswitch to optically control PAD activity. Screening of a series of inhibitors structurally similar to BB-Cl-amidine afforded compounds 1 and 2 as the most promising candidates for the light-controlled inhibition of PAD2; the cis isomer of 1 is 10-fold more potent than its trans isomer, whereas the trans isomer of 2 is 45-fold more potent than the corresponding cis isomer. The altered inhibitory potency upon photoisomerization has been confirmed in a competitive activity-based protein profiling (ABPP) assay. Further investigations indicate that the trans isomer of 2 is an irreversible inhibitor, whereas the cis isomer acts as a competitive inhibitor. In cells, the trans isomer of compound 1 is completely inactive, whereas the cis isomer inhibits histone H3-citrullination in a dose-dependent manner. Taken together, 1 serves as the foundation for developing photopharmaceuticals that can be activated at the desired tissue, using light, to treat diseases where PAD activity is dysregulated.

Published

2018

4. The Development of Benzimidazole-Based Clickable Probes for the Efficient Labeling of Cellular Protein Arginine Deiminases (PADs).

Author

Nemmara VV, Subramanian V, Muth A, Mondal S, Salinger AJ, Maurais AJ, Tilvawala R, Weerapana E, and Thompson PR

Subjects

Autoimmune Diseases, Citrulline, Click Chemistry, Fluoroacetates pharmacology, Protein-Arginine Deiminases antagonists & inhibitors, Proteomics, Benzimidazoles chemistry, Molecular Probes chemistry, Protein-Arginine Deiminases analysis, Staining and Labeling methods

Abstract

Citrullination is the post-translational hydrolysis of peptidyl-arginines to form peptidyl-citrulline, a reaction that is catalyzed by the protein arginine deiminases (PADs), a family of calcium-regulated enzymes. Aberrantly increased protein citrullination is associated with a slew of autoimmune diseases (e.g., rheumatoid arthritis (RA), multiple sclerosis, lupus, and ulcerative colitis) and certain cancers. Given the clear link between increased PAD activity and human disease, the PADs are therapeutically relevant targets. Herein, we report the development of next generation cell permeable and "clickable" probes (BB-Cl-Yne and BB-F-Yne) for covalent labeling of the PADs both in vitro and in cell-based systems. Using advanced chemoproteomic technologies, we also report the off targets of both BB-Cl-Yne and BB-F-Yne. The probes are highly specific for the PADs, with relatively few off targets, especially BB-F-Yne, suggesting the preferential use of the fluoroacetamidine warhead in next generation irreversible PAD inhibitors. Notably, these compounds can be used in a variety of modalities, including the identification of off targets of the parent compounds and as activity-based protein profiling probes in target engagement assays to demonstrate the efficacy of PAD inhibitors.

Published

2018

5. Citrullination/Methylation Crosstalk on Histone H3 Regulates ER-Target Gene Transcription.

Author

Clancy KW, Russell AM, Subramanian V, Nguyen H, Qian Y, Campbell RM, and Thompson PR

Subjects

Citrulline metabolism, Gene Expression Regulation, Neoplastic, Histones metabolism, Humans, Hydrolases, Methylation, Models, Theoretical, Polycomb Repressive Complex 2, Protein-Arginine Deiminase Type 2, Protein-Arginine Deiminases, Transcriptional Activation, Histones physiology, Receptor Cross-Talk, Transcription, Genetic

Abstract

Posttranslational modifications of histone tails are a key contributor to epigenetic regulation. Histone H3 Arg26 and Lys27 are both modified by multiple enzymes, and their modifications have profound effects on gene expression. Citrullination of H3R26 by PAD2 and methylation of H3K27 by PRC2 have opposing downstream impacts on gene regulation; H3R26 citrullination activates gene expression, and H3K27 methylation represses gene expression. Both of these modifications are drivers of a variety of cancers, and their writer enzymes, PAD2 and EZH2, are the targets of drug therapies. After biochemical and cell-based analysis of these modifications, a negative crosstalk interaction is observed. Methylation of H3K27 slows citrullination of H3R26 30-fold, whereas citrullination of H3R26 slows methylation 30,000-fold. Examination of the mechanism of this crosstalk interaction uncovered a change in structure of the histone tail upon citrullination which prevents methylation by the PRC2 complex. This mechanism of crosstalk is reiterated in cell lines using knockdowns and inhibitors of both enzymes. Based our data, we propose a model in which, after H3 Cit26 formation, H3K27 demethylases are recruited to the chromatin to activate transcription. In total, our studies support the existence of crosstalk between citrullination of H3R26 and methylation of H3K27.

Published

2017

6. Protein Arginine Methylation and Citrullination in Epigenetic Regulation.

Author

Fuhrmann J and Thompson PR

Subjects

Arginine genetics, Chromatin physiology, Humans, Methylation, Arginine metabolism, Citrulline metabolism, Epigenesis, Genetic physiology

Abstract

The post-translational modification of arginine residues represents a key mechanism for the epigenetic control of gene expression. Aberrant levels of histone arginine modifications have been linked to the development of several diseases including cancer. In recent years, great progress has been made in understanding the physiological role of individual arginine modifications and their effects on chromatin function. The present review aims to summarize the structural and functional aspects of histone arginine modifying enzymes and their impact on gene transcription. We will discuss the potential for targeting these proteins with small molecules in a variety of disease states.

Published

2016

7. Chemical Proteomic Platform To Identify Citrullinated Proteins.

Author

Lewallen DM, Bicker KL, Subramanian V, Clancy KW, Slade DJ, Martell J, Dreyton CJ, Sokolove J, Weerapana E, and Thompson PR

Subjects

Enzyme-Linked Immunosorbent Assay, HEK293 Cells, Histones chemistry, Humans, Molecular Structure, Citrulline chemistry, Proteins analysis, Proteins metabolism, Proteomics methods

Abstract

Anti-citrullinated protein antibodies (ACPAs) are a hallmark of rheumatoid arthritis (RA) and are routinely used for disease diagnosis. Protein citrullination is also increased in cancer and other autoimmune disorders, suggesting that citrullinated proteins may serve as biomarkers for diseases beyond RA. To identify these citrullinated proteins, we developed biotin-conjugated phenylglyoxal (biotin-PG). Using this probe and our platform technology, we identified >50 intracellular citrullinated proteins. More than 20 of these are involved in RNA splicing, suggesting, for the first time, that citrullination modulates RNA biology. Overall, this chemical proteomic platform will play a key role in furthering our understanding of protein citrullination in rheumatoid arthritis and potentially a wider spectrum of inflammatory diseases.

Published

2015

8. Protein arginine deiminase 2 binds calcium in an ordered fashion: implications for inhibitor design.

Author

Slade DJ, Fang P, Dreyton CJ, Zhang Y, Fuhrmann J, Rempel D, Bax BD, Coonrod SA, Lewis HD, Guo M, Gross ML, and Thompson PR

Subjects

Amino Acid Sequence, Benzimidazoles chemistry, Benzimidazoles pharmacology, Catalytic Domain, Crystallography, X-Ray, Cysteine chemistry, Cysteine metabolism, Deuterium Exchange Measurement, Enzyme Activation, Enzyme Inhibitors chemistry, Humans, Hydrolases antagonists & inhibitors, Molecular Docking Simulation, Molecular Sequence Data, Protein Conformation, Protein-Arginine Deiminase Type 2, Protein-Arginine Deiminases, Calcium metabolism, Hydrolases chemistry, Hydrolases metabolism

Abstract

Protein arginine deiminases (PADs) are calcium-dependent histone-modifying enzymes whose activity is dysregulated in inflammatory diseases and cancer. PAD2 functions as an Estrogen Receptor (ER) coactivator in breast cancer cells via the citrullination of histone tail arginine residues at ER binding sites. Although an attractive therapeutic target, the mechanisms that regulate PAD2 activity are largely unknown, especially the detailed role of how calcium facilitates enzyme activation. To gain insights into these regulatory processes, we determined the first structures of PAD2 (27 in total), and through calcium-titrations by X-ray crystallography, determined the order of binding and affinity for the six calcium ions that bind and activate this enzyme. These structures also identified several PAD2 regulatory elements, including a calcium switch that controls proper positioning of the catalytic cysteine residue, and a novel active site shielding mechanism. Additional biochemical and mass-spectrometry-based hydrogen/deuterium exchange studies support these structural findings. The identification of multiple intermediate calcium-bound structures along the PAD2 activation pathway provides critical insights that will aid the development of allosteric inhibitors targeting the PADs.

Published

2015

9. A FluoPol-ABPP PAD2 high-throughput screen identifies the first calcium site inhibitor targeting the PADs.

Author

Lewallen DM, Bicker KL, Madoux F, Chase P, Anguish L, Coonrod S, Hodder P, and Thompson PR

Subjects

Binding Sites, Biological Assay, Drug Evaluation, Preclinical, Enzyme Inhibitors pharmacology, Hydrolases antagonists & inhibitors, Molecular Structure, Protein Binding drug effects, Protein-Arginine Deiminases, Calcium chemistry, Drug Delivery Systems, Hydrolases metabolism, Ruthenium Red chemistry, Ruthenium Red pharmacology

Abstract

The protein arginine deiminases (PADs) catalyze the post-translational hydrolysis of peptidyl-arginine to form peptidyl-citrulline in a process termed deimination or citrullination. PADs likely play a role in the progression of a range of disease states because dysregulated PAD activity is observed in a host of inflammatory diseases and cancer. For example, recent studies have shown that PAD2 activates ERα target gene expression in breast cancer cells by citrullinating histone H3 at ER target promoters. To date, all known PAD inhibitors bind directly to the enzyme active site. PADs, however, also require calcium ions to drive a conformational change between the inactive apo-state and the fully active calcium bound holoenzyme, suggesting that it would be possible to identify inhibitors that bind the apoenzyme and prevent this conformational change. As such, we set out to develop a screen that can identify PAD2 inhibitors that bind to either the apo or calcium bound form of PAD2. Herein, we provide definitive proof of concept for this approach and report the first PAD inhibitor, ruthenium red (Ki of 17 μM), to preferentially bind the apoenzyme.

Published

2014

10. Using unnatural amino acid mutagenesis to probe the regulation of PRMT1.

Author

Rust HL, Subramanian V, West GM, Young DD, Schultz PG, and Thompson PR

Subjects

Amino Acid Substitution, Benzophenones metabolism, Cross-Linking Reagents chemistry, Histones metabolism, Humans, Immunoprecipitation, K562 Cells, Methylation, Phenylalanine genetics, Phenylalanine metabolism, Phosphorylation, Protein Processing, Post-Translational, Substrate Specificity, Tyrosine metabolism, Mutagenesis, Site-Directed, Phenylalanine analogs & derivatives, Protein-Arginine N-Methyltransferases genetics, Protein-Arginine N-Methyltransferases metabolism, Repressor Proteins genetics, Repressor Proteins metabolism, Tyrosine genetics

Abstract

Protein arginine methyltransferase 1 (PRMT1)-dependent methylation contributes to the onset and progression of numerous diseases (e.g., cancer, heart disease, ALS); however, the regulatory mechanisms that control PRMT1 activity are relatively unexplored. We therefore set out to decipher how phosphorylation regulates PRMT1 activity. Curated mass spectrometry data identified Tyr291, a residue adjacent to the conserved THW loop, as being phosphorylated. Natural and unnatural amino acid mutagenesis, including the incorporation of p-carboxymethyl-l-phenylalanine (pCmF) as a phosphotyrosine mimic, were used to show that Tyr291 phosphorylation alters the substrate specificity of PRMT1. Additionally, p-benzoyl-l-phenylalanine (pBpF) was incorporated at the Tyr291 position, and cross-linking experiments with K562 cell extracts identified several proteins (e.g., hnRNPA1 and hnRNP H3) that bind specifically to this site. Moreover, we also demonstrate that Tyr291 phosphorylation impairs PRMT1's ability to bind and methylate both proteins. In total, these studies demonstrate that Tyr291 phosphorylation alters both PRMT1 substrate specificity and protein-protein interactions.

Published

2014

11. Inhibiting AMPylation: a novel screen to identify the first small molecule inhibitors of protein AMPylation.

Author

Lewallen DM, Sreelatha A, Dharmarajan V, Madoux F, Chase P, Griffin PR, Orth K, Hodder P, and Thompson PR

Subjects

Adenosine Monophosphate antagonists & inhibitors, Adenosine Triphosphate antagonists & inhibitors, Anti-Bacterial Agents chemistry, Bacterial Proteins metabolism, Drug Discovery, High-Throughput Screening Assays, Humans, Small Molecule Libraries chemistry, Vibrio Infections drug therapy, Vibrio Infections microbiology, Adenosine Monophosphate metabolism, Adenosine Triphosphate metabolism, Anti-Bacterial Agents pharmacology, Bacterial Proteins antagonists & inhibitors, Small Molecule Libraries pharmacology, Vibrio parahaemolyticus drug effects, Vibrio parahaemolyticus metabolism

Abstract

Enzymatic transfer of the AMP portion of ATP to substrate proteins has recently been described as an essential mechanism of bacterial infection for several pathogens. The first AMPylator to be discovered, VopS from Vibrio parahemolyticus, catalyzes the transfer of AMP onto the host GTPases Cdc42 and Rac1. Modification of these proteins disrupts downstream signaling events, contributing to cell rounding and apoptosis, and recent studies have suggested that blocking AMPylation may be an effective route to stop infection. To date, however, no small molecule inhibitors have been discovered for any of the AMPylators. Therefore, we developed a fluorescence-polarization-based high-throughput screening assay and used it to discover the first inhibitors of protein AMPylation. Herein we report the discovery of the first small molecule VopS inhibitors (e.g., calmidazolium, GW7647, and MK886) with Ki's ranging from 6 to 50 μM and upward of 30-fold selectivity versus HYPE, the only known human AMPylator.

Published

2014

12. Targeting the arginine phosphatase YwlE with a catalytic redox-based inhibitor.

Author

Fuhrmann J, Subramanian V, and Thompson PR

Subjects

Arginine metabolism, Bacillus chemistry, Bacillus genetics, Enzyme Inhibitors chemistry, Enzyme Inhibitors pharmacology, Mutagenesis, Site-Directed, Mutation, Organophosphorus Compounds metabolism, Oxidation-Reduction, Phosphoprotein Phosphatases antagonists & inhibitors, Phosphoprotein Phosphatases chemistry, Phosphoprotein Phosphatases genetics, Arginine analogs & derivatives, Bacillus enzymology, Phosphoprotein Phosphatases metabolism

Abstract

Protein phosphatases are critical regulators of cellular signaling in both eukaryotes and prokaryotes. The majority of protein phosphatases dephosphorylate phosphoserine/phosphothreonine or phosphotyrosine residues. Recently, however, YwlE, a member of the low-molecular weight protein tyrosine phosphatase (LMW-PTP) family, was shown to efficiently target phosphoarginine. YwlE shares several sequence motifs with this family including the C(X)4 CR(S/T) motif that is crucial for catalysis and redox regulation of the enzyme. Herein we confirm that Cys9 and Cys14 play important roles in YwlE catalysis and regulation. On the basis of these observations, we designed and synthesized a YwlE inhibitor, denoted cyc-SeCN-amidine, that irreversibly inhibits YwlE (kinact/KI = 310 M(-1) min(-1)) by inducing disulfide bond formation between the two active site cysteine residues. Interestingly, inactivation appears to be catalytic, since the compound is neither destroyed nor altered after enzyme inhibition. Although the exact mechanism of disulfide induction remains elusive, we propose several potential mechanisms accounting for the cyc-SeCN-amidine mediated inhibition of YwlE. These findings could stimulate the design of similar selenium-based compounds targeting other redox-sensitive enzymes.

Published

2013

13. Design, synthesis, and kinetic characterization of protein N-terminal acetyltransferase inhibitors.

Author

Foyn H, Jones JE, Lewallen D, Narawane R, Varhaug JE, Thompson PR, and Arnesen T

Subjects

Acetylation, Acetyltransferases metabolism, Amino Acid Sequence, Humans, Kinetics, Models, Molecular, Peptides chemistry, Peptides pharmacology, Substrate Specificity, Acetyltransferases antagonists & inhibitors, Drug Design, Enzyme Inhibitors chemistry, Enzyme Inhibitors pharmacology

Abstract

The N-termini of 80-90% of human proteins are acetylated by the N-terminal acetyltransferases (NATs), NatA-NatF. The major NAT complex, NatA, and particularly the catalytic subunit hNaa10 (ARD1) has been implicated in cancer development. For example, knockdown of hNaa10 results in cancer cell death and the arrest of cell proliferation. It also sensitized cancer cells to drug-induced cytotoxicity. Human NatE has a distinct substrate specificity and is essential for normal chromosome segregation. Thus, NAT inhibitors may potentially be valuable anticancer therapeutics, either directly or as adjuvants. Herein, we report the design and synthesis of the first inhibitors targeting these enzymes. Using the substrate specificity of the enzymes as a guide, we synthesized three bisubstrate analogues that potently and selectively inhibit the NatA complex (CoA-Ac-SES4; IC50 = 15.1 μM), hNaa10, the catalytic subunit of NatA (CoA-Ac-EEE4; Ki = 1.6 μM), and NatE/hNaa50 (CoA-Ac-MLG7; Ki* = 8 nM); CoA-Ac-EEE4 is a reversible competitive inhibitor of hNaa10, and CoA-Ac-MLG7 is a slow tight binding inhibitor of hNaa50. Our demonstration that it is possible to develop NAT selective inhibitors should assist future efforts to develop NAT inhibitors with more drug-like properties that can be used to chemically interrogate in vivo NAT function.

Published

2013

14. Synthesis and screening of a haloacetamidine containing library to identify PAD4 selective inhibitors.

Author

Jones JE, Slack JL, Fang P, Zhang X, Subramanian V, Causey CP, Coonrod SA, Guo M, and Thompson PR

Subjects

Amidines pharmacology, Biotinylation, Enzyme Inhibitors pharmacology, Humans, Hydrocarbons, Fluorinated pharmacology, Hydrolases chemistry, Hydrolases metabolism, Isoenzymes antagonists & inhibitors, Isoenzymes chemistry, Isoenzymes metabolism, Kinetics, Models, Molecular, Molecular Probes chemical synthesis, Ornithine chemical synthesis, Ornithine pharmacology, Protein Structure, Tertiary, Protein-Arginine Deiminase Type 4, Protein-Arginine Deiminases, Recombinant Proteins antagonists & inhibitors, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Small Molecule Libraries pharmacology, Substrate Specificity, Amidines chemical synthesis, Enzyme Inhibitors chemical synthesis, Hydrocarbons, Fluorinated chemical synthesis, Hydrolases antagonists & inhibitors, Ornithine analogs & derivatives, Small Molecule Libraries chemical synthesis

Abstract

Protein arginine deiminase activity (PAD) is increased in cancer, rheumatoid arthritis, and ulcerative colitis. Although the link between abnormal PAD activity and disease is clear, the relative contribution of the individual PADs to human disease is not known; there are 5 PAD isozymes in humans. Building on our previous development of F- and Cl-amidine as potent pan-PAD irreversible inhibitors, we describe herein a library approach that was used to identify PAD-selective inhibitors. Specifically, we describe the identification of Thr-Asp-F-amidine (TDFA) as a highly potent PAD4 inactivator that displays ≥15-fold selectivity for PAD4 versus PAD1 and ≥50-fold versus PADs 2 and 3. This compound is active in cells and can be used to inhibit PAD4 activity in cellulo. The structure of the PAD4·TDFA complex has also been solved, and the structure and mutagenesis data indicate that the enhanced potency is due to interactions between the side chains of Q346, R374, and R639. Finally, we converted TDFA into a PAD4-selective ABPP and demonstrated that this compound, biotin-TDFA, can be used to selectively isolate purified PAD4 in vitro. In total, TDFA and biotin-TDFA represent PAD4-selective chemical probes that can be used to study the physiological roles of this enzyme.

Published

2012

15. Activity-based protein profiling of protein arginine methyltransferase 1.

Author

Obianyo O, Causey CP, Jones JE, and Thompson PR

Subjects

Breast Neoplasms drug therapy, Breast Neoplasms enzymology, Cell Line, Tumor, Female, Humans, Inhibitory Concentration 50, Drug Design, Enzyme Inhibitors chemistry, Enzyme Inhibitors pharmacology, Protein-Arginine N-Methyltransferases antagonists & inhibitors, Protein-Arginine N-Methyltransferases metabolism, Repressor Proteins antagonists & inhibitors, Repressor Proteins metabolism

Abstract

The protein arginine methyltransferases (PRMTs) are SAM-dependent enzymes that catalyze the mono- and dimethylation of peptidyl arginine residues. PRMT1 is the founding member of the PRMT family, and this isozyme is responsible for methylating ∼85% of the arginine residues in mammalian cells. Additionally, PRMT1 activity is aberrantly upregulated in heart disease and cancer. As a part of a program to develop isozyme-specific PRMT inhibitors, we recently described the design and synthesis of C21, a chloroacetamidine bearing histone H4 tail analogue that acts as an irreversible PRMT1 inhibitor. Given the covalent nature of the interaction, we set out to develop activity-based probes (ABPs) that could be used to characterize the physiological roles of PRMT1. Herein, we report the design, synthesis, and characterization of fluorescein-conjugated C21 (F-C21) and biotin-conjugated C21 (B-C21) as PRMT1-specific ABPs. Additionally, we provide the first evidence that PRMT1 activity is negatively regulated in a spatial and temporal fashion.

Published

2011

16. Kinase consensus sequences: a breeding ground for crosstalk.

Author

Rust HL and Thompson PR

Subjects

Amino Acids metabolism, Consensus Sequence, Humans, Phosphorylation, Signal Transduction, Protein Kinases metabolism

Abstract

The best characterized examples of crosstalk between two or more different post-translational modifications (PTMs) occur with respect to histones. These examples demonstrate the critical roles that crosstalk plays in regulating cell signaling pathways. Recently, however, non-histone crosstalk has been observed between serine/threonine phosphorylation and the modification of arginine and lysine residues within kinase consensus sequences. Interestingly, many kinase consensus sequences contain critical arginine/lysine residues surrounding the substrate serine/threonine residue. Therefore, we hypothesize that non-histone crosstalk between serine/threonine phosphorylation and arginine/lysine modifications is a global mechanism for the modulation of cellular signaling. In this review, we discuss several recent examples of non-histone kinase consensus sequence crosstalk, as well as provide the biophysical basis for these observations. In addition, we predict likely examples of crosstalk between protein arginine methyltransferase 1 (PRMT1) and Akt and discuss the future implications of these findings.

Published

2011

17. Development and use of clickable activity based protein profiling agents for protein arginine deiminase 4.

Author

Slack JL, Causey CP, Luo Y, and Thompson PR

Subjects

Biotin analogs & derivatives, Enzyme Activation, Fluorescent Dyes, Humans, Hydrolases antagonists & inhibitors, Limit of Detection, Protein Array Analysis, Protein-Arginine Deiminase Type 4, Protein-Arginine Deiminases, Triazoles chemistry, Amidines pharmacology, Hydrolases metabolism

Abstract

The protein arginine deiminases (PADs), which catalyze the hydrolysis of peptidyl-arginine to form peptidyl-citrulline, are potential targets for the development of a rheumatoid arthritis (RA) therapeutic, as well as other human diseases including colitis and cancer. Additionally, these enzymes, and in particular PAD4, appear to play important roles in a variety of cell signaling pathways including apoptosis, differentiation, and transcriptional regulation. To better understand the factors that regulate in vivo PAD4 activity, we set out to design and synthesize a series of activity-based protein profiling (ABPP) reagents that target this enzyme. Herein we describe the design, synthesis, and evaluation of six ABPPs including (i) FITC-conjugated F-amidine (FFA1 and 2) and Cl-amidine (FCA1 and 2), and (ii) biotin-conjugated F-amidine (BFA) and Cl-amidine (BCA). We further demonstrate the utility of these probes for labeling PAD4 in cells, as well as for isolating PAD4 and PAD4 binding proteins. These probes will undoubtedly prove to be powerful tools that can be used to dissect the factors controlling the dynamics of PAD4 expression, activity, and function.

Published

2011

18. Histone citrullination by protein arginine deiminase: is arginine methylation a green light or a roadblock?

Author

Thompson PR and Fast W

Subjects

Chemistry methods, Hydrolases metabolism, Methylation, Models, Chemical, Models, Molecular, Multigene Family, Protein Conformation, Protein Processing, Post-Translational, Protein-Arginine Deiminases, Proteomics methods, Arginine chemistry, Citrulline chemistry, Gene Expression Regulation, Enzymologic, Histones chemistry, Hydrolases chemistry

Abstract

Protein citrullination, a once-obscure post-translational modification (PTM) of peptidylarginine, has recently become an area of significant interest because of its suspected role in human disease states, including rheumatoid arthritis and multiple sclerosis, and also because of its newfound role in gene regulation. One protein isozyme responsible for this modification, protein arginine deiminase 4 (PAD4), has also been proposed to "reverse" epigenetic histone modifications made by the protein arginine methyltransferases. Here, we review the in vivo and in vitro studies of transcriptional regulation by PAD4, evaluate conflicting evidence for its ability to use methylated peptidylarginine as a substrate, and highlight promising areas of future work. Understanding the interplay of multiple arginine PTMs is an emerging area of importance in health and disease and is a topic best addressed by novel tools in proteomics and chemical biology.

Published

2006