Your search keyword '"Rickert KW"' showing total 28 results

1. Development and validation of a multiplex immunoassay for the simultaneous quantification of type-specific IgG antibodies to E6/E7 oncoproteins of HPV16 and HPV18.

Author

Layman H, Rickert KW, Wilson S, Aksyuk AA, Dunty JM, Natrakul D, Swaminathan N, and DelNagro CJ

Subjects

Animals, Antibody Specificity, Cross Reactions, DNA-Binding Proteins immunology, Electrochemical Techniques, Enzyme-Linked Immunosorbent Assay, Female, High-Throughput Screening Assays methods, High-Throughput Screening Assays statistics & numerical data, Humans, Immunoassay statistics & numerical data, Limit of Detection, Luminescent Measurements methods, Luminescent Measurements statistics & numerical data, Macaca fascicularis, Oncogene Proteins, Viral immunology, Papillomavirus E7 Proteins immunology, Repressor Proteins immunology, Uterine Cervical Neoplasms immunology, Uterine Cervical Neoplasms virology, Antibodies, Viral blood, Human papillomavirus 16 immunology, Human papillomavirus 18 immunology, Immunoassay methods, Immunoglobulin G blood

Abstract

More than 170 types of human papilloma viruses (HPV) exist with many causing proliferative diseases linked to malignancy in indications such as cervical cancer and head and neck squamous cell carcinoma. Characterization of antibody levels toward HPV serology is challenging due to complex biology of oncoproteins, pre-existing titers to multiple HPV types, cross-reactivity, and low affinity, polyclonal responses. Using multiplex technology from MSD, we have developed an assay that simultaneously characterizes antibodies against E6 and E7 oncoproteins of HPV16 and 18, the primary drivers of HPV-associated oncogenesis. We fusion tagged our E6 and E7 proteins with MBP via two-step purification, spot-printed an optimized concentration of protein into wells of MSD 96-well plates, and assayed various cynomolgus monkey, human and HPV+ cervical cancer patient serum to validate the assay. The dynamic range of the assay covered 4-orders of magnitude and antibodies were detected in serum at a dilution up to 100,000-fold. The assay was very precise (n = 5 assay runs) with median CV of human serum samples ~ 5.3% and inter-run variability of 11.4%. The multiplex serology method has strong cross-reactivity between E6 oncoproteins from human serum samples as HPV18 E6 antigens neutralized 5 of 6 serum samples as strongly as HPV16 E6. Moderate concordance (Spearman's Rank = 0.775) was found between antibody responses against HPV16 E7 in the multiplex assay compared to standard ELISA serology methods. These results demonstrate the development of a high-throughput, multi-plex assay that requires lower sample quantity input with greater dynamic range to detect type-specific anti-HPV concentrations to E6 and E7 oncoproteins of HPV16 and 18., Competing Interests: HL, KAR, SW, NS, CJD are current or former employees of AstraZeneca. They received compensation in the form of salary and stock as employees. AAA, JMD, and DN are current or former employees of Meso Scale Diagnostics LLC and receive compensation in the form of salary and stock. The commercial affiliations of AstraZeneca and Meso Scale Diagnostics LLC does not alter any adherence to PLOS ONE policies on sharing data and materials.

Published

2020

2. Antibody Fragment F(ab') 2 Targeting Caveolae-Associated Protein PV1 for Selective Kidney Targeting and Retention.

Author

Li Q, Peterson N, Hanna RN, Kuszpit K, White J, Allen KL, Barnes A, Rickert KW, Shan L, Wu H, Dall'Acqua WF, Tsui P, and Borrok MJ

Subjects

Animals, Antibodies, Monoclonal administration & dosage, Antibodies, Monoclonal pharmacokinetics, Antibody Affinity, Drug Carriers administration & dosage, Female, HEK293 Cells, Humans, Immunoglobulin Fab Fragments administration & dosage, Kidney metabolism, Lung drug effects, Lung metabolism, Mice, Mice, Inbred BALB C, Tissue Distribution, Antibodies, Monoclonal immunology, Caveolae metabolism, Drug Carriers pharmacokinetics, Immunoglobulin Fab Fragments immunology, Kidney drug effects, Membrane Proteins immunology

Abstract

Targeted strategies to deliver and retain drugs to kidneys are needed to improve drug accumulation and efficacy in a myriad of kidney diseases. These drug delivery systems show potential for improving the therapeutic windows of drugs acting in the kidney. Biodistribution of antibody-based therapeutics in vivo is governed by several factors including binding affinity, size, and valency. Investigations of how the biophysical and biochemical properties of biologics enable them to overcome biological barriers and reach kidneys are therefore of interest. Although renal accumulation of antibody fragments in cancer diagnostics and treatment has been observed, reports on effective delivery of antibody fragments to the kidneys remain scarce. Previously, we demonstrated that targeting plasmalemma vesicle-associated protein (PV1), a caveolae-associated protein, can promote accumulation of antibodies in both the lungs and the kidneys. Here, by fine-tuning the binding affinity of an antibody toward PV1, we observe that the anti-PV1 antibody with reduced binding affinity lost the capability for kidney targeting while retaining the lung targeting activity, suggesting that binding affinity is a critical factor for kidney targeting of the anti-PV1 antibody. We next use the antibody fragment F(ab') 2 targeting PV1 to assess the dual effects of rapid kidney filtration and PV1 targeting on kidney-selective targeting. Ex vivo fluorescence imaging results demonstrated that after rapidly accumulating in kidneys at 4 h, PV1-targeted F(ab') 2 was continually retained in the kidney at 24 h, whereas the isotype control F(ab') 2 underwent urinary elimination with significantly reduced signaling in the kidney. Confocal imaging studies confirmed the localization of PV1-targeted F(ab') 2 in the kidney. In addition, the monovalent antibody fragment (Fab-C4) lost the capability for kidney homing, indicating that the binding avidity of anti-PV1 F(ab') 2 is important for kidney targeting. Our findings suggest that PV1-targeted F(ab') 2 might be useful as a drug carrier for renal targeting and highlight the importance of affinity optimization for tissue targeting antibodies.

Published

2020

3. Experimentally guided computational antibody affinity maturation with de novo docking, modelling and rational design.

Author

Cannon DA, Shan L, Du Q, Shirinian L, Rickert KW, Rosenthal KL, Korade M 3rd, van Vlerken-Ysla LE, Buchanan A, Vaughan TJ, Damschroder MM, and Popovic B

Subjects

Amino Acid Sequence, Animals, Antibodies chemistry, Chemokine CCL20, Computer Simulation, Drug Design, Immunoglobulin Variable Region, Mice, Models, Molecular, Protein Binding, Protein Conformation, Antibody Affinity physiology, Computational Biology methods

Abstract

Antibodies are an important class of therapeutics that have significant clinical impact for the treatment of severe diseases. Computational tools to support antibody drug discovery have been developing at an increasing rate over the last decade and typically rely upon a predetermined co-crystal structure of the antibody bound to the antigen for structural predictions. Here, we show an example of successful in silico affinity maturation of a hybridoma derived antibody, AB1, using just a homology model of the antibody fragment variable region and a protein-protein docking model of the AB1 antibody bound to the antigen, murine CCL20 (muCCL20). In silico affinity maturation, together with alanine scanning, has allowed us to fine-tune the protein-protein docking model to subsequently enable the identification of two single-point mutations that increase the affinity of AB1 for muCCL20. To our knowledge, this is one of the first examples of the use of homology modelling and protein docking for affinity maturation and represents an approach that can be widely deployed., Competing Interests: I have read the journal's policy and the authors of this manuscript have the following competing interests: All authors were employees of MedImmune at the time that this work was performed and had stock ownership or interests and/or stock options in AstraZeneca.

Published

2019

4. Improved Inhibition of Tumor Growth by Diabody-Drug Conjugates via Half-Life Extension.

Author

Li Q, Barrett A, Vijayakrishnan B, Tiberghien A, Beard R, Rickert KW, Allen KL, Christie RJ, Marelli M, Harper J, Howard P, Wu H, Dall'Acqua WF, Tsui P, Gao C, and Borrok MJ

Subjects

Animals, Antineoplastic Agents chemistry, Antineoplastic Agents pharmacokinetics, Binding, Competitive, Cell Line, Tumor, Cell Proliferation drug effects, Drug Screening Assays, Antitumor, Enzyme-Linked Immunosorbent Assay, Female, Half-Life, Humans, Immunoconjugates chemistry, Immunoconjugates pharmacokinetics, Mice, Mice, Nude, Polyethylene Glycols chemistry, Xenograft Model Antitumor Assays, Antineoplastic Agents therapeutic use, Immunoconjugates therapeutic use

Abstract

Despite some clinical success with antibody-drug conjugates (ADCs) in patients with solid tumors and hematological malignancies, improvements in ADC design are still desirable due to the narrow therapeutic window of these compounds. Tumor-targeting antibody fragments have distinct advantages over monoclonal antibodies, including more rapid tumor accumulation and enhanced penetration, but are subject to rapid clearance. Half-life extension technologies such as PEGylation and albumin-binding domains (ABDs) have been widely used to improve the pharmacokinetics of many different types of biologics. PEGylation improves pharmacokinetics by increasing hydrodynamic size to reduce renal clearance, whereas ABDs extend half-life via FcRn-mediated recycling. In this study, we used an anti-oncofetal antigen 5T4 diabody conjugated with a highly potent cytotoxic pyrrolobenzodiazepine (PBD) warhead to assess and compare the effects of PEGylation and albumin binding on the in vivo efficacy of antibody fragment drug conjugates. Conjugation of 2× PEG20K to a diabody improved half-life from 40 min to 33 h, and an ABD-diabody fusion protein exhibited a half-life of 45 h in mice. In a xenograft model of breast cancer MDA-MB-436, the ABD-diabody-PBD showed greater tumor growth suppression and better tolerability than either PEG-diabody-PBD or diabody-PBD. These results suggest that the mechanism of half-life extension is an important consideration for designing cytotoxic antitumor agents.

Published

2019

5. Targeted drug delivery via caveolae-associated protein PV1 improves lung fibrosis.

Author

Marchetti GM, Burwell TJ, Peterson NC, Cann JA, Hanna RN, Li Q, Ongstad EL, Boyd JT, Kennedy MA, Zhao W, Rickert KW, Grimsby JS, Dall'Acqua WF, Wu H, Tsui P, Borrok MJ, and Gupta R

Subjects

Animals, Biomarkers, Bleomycin adverse effects, Dinoprostone metabolism, Disease Models, Animal, Gene Expression, Humans, Idiopathic Pulmonary Fibrosis etiology, Idiopathic Pulmonary Fibrosis pathology, Immunohistochemistry, Kidney metabolism, Kidney pathology, Lung drug effects, Lung metabolism, Lung pathology, Membrane Proteins chemistry, Membrane Proteins genetics, Mice, Drug Carriers, Drug Delivery Systems, Idiopathic Pulmonary Fibrosis drug therapy, Membrane Proteins metabolism

Abstract

Systemic administration of bio-therapeutics can result in only a fraction of drug reaching targeted tissues, with the majority of drug being distributed to tissues irrelevant to the drug's site of action. Targeted delivery to specific organs may allow for greater accumulation, better efficacy, and improved safety. We investigated how targeting plasmalemma vesicle-associated protein (PV1), a protein found in the endothelial caveolae of lungs and kidneys, can promote accumulation in these organs. Using ex vivo fluorescence imaging, we show that intravenously administered αPV1 antibodies localize to mouse lungs and kidneys. In a bleomycin-induced idiopathic pulmonary fibrosis (IPF) mouse model, αPV1 conjugated to Prostaglandin E 2 (PGE 2 ), a known anti-fibrotic agent, significantly reduced collagen content and fibrosis whereas a non-targeted PGE 2 antibody conjugate failed to slow fibrosis progression. Our results demonstrate that PV1 targeting can be utilized to deliver therapeutics to lungs and this approach is potentially applicable for various lung diseases., Competing Interests: All authors, with the exception of G.M.M., P.T., and R.G. are employees of the AstraZeneca group of companies. G.M.M., P.T., and R.G. are former employees of MedImmune, a company of the AstraZeneca group. All authors may have stocks/stock options in AstraZeneca.

Published

2019

6. Tumor uptake of pegylated diabodies: Balancing systemic clearance and vascular transport.

Author

Li Q, White JB, Peterson NC, Rickert KW, Lloyd CO, Allen KL, Rosenthal K, Gao X, Wu H, Dall'Acqua WF, Borrok MJ, and Tsui P

Subjects

Animals, Biological Transport, Cell Line, Tumor, Female, Half-Life, Humans, Hydrodynamics, Immunoglobulin Fragments chemistry, Immunoglobulin Fragments metabolism, Mice, Mice, Nude, Molecular Weight, Positron-Emission Tomography, Tissue Distribution, Drug Delivery Systems, Immunoglobulin Fragments administration & dosage, Neoplasms metabolism, Polyethylene Glycols chemistry

Abstract

The accumulation, dissemination and clearance of monoclonal antibody-based therapeutics or imaging reagents targeting tumor associated antigens is governed by several factors including affinity, size, charge, and valency. Tumor targeting antibody fragments have distinct advantages over intact monoclonal antibodies such as enhanced penetration within the tumor and rapid accumulation but are subject to rapid clearance. Polyethylene glycol (PEG)-modified antibody fragments can provide a way to balance tumor penetration and accumulation with improved serum persistence. In this study, we use a diabody, the dimeric antibody fragment, targeting the 5T4 antigen to assess the impact of PEGs of distinct size and shape on tumor accumulation and pharmacokinetics (PK). We show that PEG-modified diabodies improved the PK of the parental diabody from a half-life of 40 min to over 40 h for the higher molecular weight PEG conjugated diabodies. This improvement correlates with the increasing hydrodynamic size of pegylated diabodies, and can serve as a better predictor of the PK behavior of pegylated molecules than molecular weight alone. Tumor uptake profiles determined by quantitative PET imaging differed significantly based on PEG size and shape with diabody-PEG5K showing peak accumulation early on, but with the larger diabody-PEG20K showing better sustained tumor uptake at later time points. In addition, we demonstrate that a diabody-PEG20K-B with a hydrodynamic radius (Rh) of 6 nm had superior tumor uptake than the larger diabody-PEG40K-B with Rh of 12 nm, indicating that beyond 6 nm, larger pegylated diabodies have a slower tumor uptake rate while having comparable clearance kinetics. Our data demonstrate that pegylated diabodies with Rh of ~6 nm have an optimal size and PK profile for tumor uptake. Understanding the impact of pegylation on PK and tumor uptake could facilitate the development of pegylated diabodies as therapeutics., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2018

7. A hingeless Fc fusion system for site-specific cleavage by IdeS.

Author

Novarra S, Grinberg L, Rickert KW, Barnes A, Wilson S, and Baca M

Subjects

Chromatography, Gel, Chromatography, Liquid, Hinge Exons, Humans, Immunoglobulin Fc Fragments genetics, Immunoglobulin G genetics, Mass Spectrometry, Protein Domains, Recombinant Fusion Proteins genetics, Substrate Specificity, Bacterial Proteins chemistry, Immunoglobulin Fc Fragments chemistry, Immunoglobulin G chemistry, Proteolysis, Recombinant Fusion Proteins chemistry

Abstract

Fusion of proteins to the Fc region of IgG is widely used to express cellular receptors and other extracellular proteins, but cleavage of the fusion partner is sometimes required for downstream applications. Immunoglobulin G-degrading enzyme of Streptococcus pyogenes (IdeS) is a protease with exquisite specificity for human IgG, and it can also cleave Fc-fusion proteins at a single site in the N-terminal region of the CH2 domain. However, the site of IdeS cleavage results in the disulfide-linked hinge region partitioning with the released protein, complicating downstream usage of the cleaved product. To tailor the Fc fragment for release of partner proteins by IdeS treatment, we investigated the effect of deleting regions of IgG-derived sequence that are upstream of the cleavage site. Elimination of the IgG-derived hinge sequence along with several residues of the CH2 domain had negligible effects on expression and purity of the fusion protein, while retaining efficient processing by IdeS. An optimal Fc fragment comprising residues 235-447 of the human IgG1 heavy chain sufficed for efficient production of fusion proteins and minimized the amount of residual Ig-derived sequence on the cleavage product following IdeS treatment. Pairing of this truncated Fc fragment with IdeS cleavage enables highly specific cleavage of Fc-fusion proteins, thus eliminating the need to engineer extraneous cleavage sequences. This system should be helpful for producing Fc-fusion proteins requiring downstream cleavage, particularly those that are sensitive to internal miscleavage if treated with alternative proteases.

Published

2016

8. Integration of Affinity Selection-Mass Spectrometry and Functional Cell-Based Assays to Rapidly Triage Druggable Target Space within the NF-κB Pathway.

Author

Kutilek VD, Andrews CL, Richards MP, Xu Z, Sun T, Chen Y, Hashke A, Smotrov N, Fernandez R, Nickbarg EB, Chamberlin C, Sauvagnat B, Curran PJ, Boinay R, Saradjian P, Allen SJ, Byrne N, Elsen NL, Ford RE, Hall DL, Kornienko M, Rickert KW, Sharma S, Shipman JM, Lumb KJ, Coleman K, Dandliker PJ, Kariv I, and Beutel B

Subjects

Ligands, Mass Spectrometry methods, NF-kappa B chemistry, Protein Binding, Signal Transduction drug effects, TNF Receptor-Associated Factor 5 antagonists & inhibitors, TNF Receptor-Associated Factor 5 chemistry, Transcription Factor RelA antagonists & inhibitors, Transcription Factor RelA chemistry, Drug Discovery, High-Throughput Screening Assays methods, NF-kappa B antagonists & inhibitors, Structure-Activity Relationship

Abstract

The primary objective of early drug discovery is to associate druggable target space with a desired phenotype. The inability to efficiently associate these often leads to failure early in the drug discovery process. In this proof-of-concept study, the most tractable starting points for drug discovery within the NF-κB pathway model system were identified by integrating affinity selection-mass spectrometry (AS-MS) with functional cellular assays. The AS-MS platform Automated Ligand Identification System (ALIS) was used to rapidly screen 15 NF-κB proteins in parallel against large-compound libraries. ALIS identified 382 target-selective compounds binding to 14 of the 15 proteins. Without any chemical optimization, 22 of the 382 target-selective compounds exhibited a cellular phenotype consistent with the respective target associated in ALIS. Further studies on structurally related compounds distinguished two chemical series that exhibited a preliminary structure-activity relationship and confirmed target-driven cellular activity to NF-κB1/p105 and TRAF5, respectively. These two series represent new drug discovery opportunities for chemical optimization. The results described herein demonstrate the power of combining ALIS with cell functional assays in a high-throughput, target-based approach to determine the most tractable drug discovery opportunities within a pathway., (© 2016 Society for Laboratory Automation and Screening.)

Published

2016

9. Combining phage display with de novo protein sequencing for reverse engineering of monoclonal antibodies.

Author

Rickert KW, Grinberg L, Woods RM, Wilson S, Bowen MA, and Baca M

Subjects

Animals, Mice, Rats, Tumor Necrosis Factor Receptor Superfamily, Member 9 antagonists & inhibitors, Tumor Necrosis Factor Receptor Superfamily, Member 9 chemistry, Peptide Library, Protein Engineering methods, Sequence Analysis, Protein, Single-Chain Antibodies chemistry, Single-Chain Antibodies genetics

Abstract

The enormous diversity created by gene recombination and somatic hypermutation makes de novo protein sequencing of monoclonal antibodies a uniquely challenging problem. Modern mass spectrometry-based sequencing will rarely, if ever, provide a single unambiguous sequence for the variable domains. A more likely outcome is computation of an ensemble of highly similar sequences that can satisfy the experimental data. This outcome can result in the need for empirical testing of many candidate sequences, sometimes iteratively, to identity one which can replicate the activity of the parental antibody. Here we describe an improved approach to antibody protein sequencing by using phage display technology to generate a combinatorial library of sequences that satisfy the mass spectrometry data, and selecting for functional candidates that bind antigen. This approach was used to reverse engineer 2 commercially-obtained monoclonal antibodies against murine CD137. Proteomic data enabled us to assign the majority of the variable domain sequences, with the exception of 3-5% of the sequence located within or adjacent to complementarity-determining regions. To efficiently resolve the sequence in these regions, small phage-displayed libraries were generated and subjected to antigen binding selection. Following enrichment of antigen-binding clones, 2 clones were selected for each antibody and recombinantly expressed as antigen-binding fragments (Fabs). In both cases, the reverse-engineered Fabs exhibited identical antigen binding affinity, within error, as Fabs produced from the commercial IgGs. This combination of proteomic and protein engineering techniques provides a useful approach to simplifying the technically challenging process of reverse engineering monoclonal antibodies from protein material.

Published

2016

10. Structure and Function of the Hypertension Variant A486V of G Protein-coupled Receptor Kinase 4.

Author

Allen SJ, Parthasarathy G, Darke PL, Diehl RE, Ford RE, Hall DL, Johnson SA, Reid JC, Rickert KW, Shipman JM, Soisson SM, Zuck P, Munshi SK, and Lumb KJ

Subjects

Amino Acid Sequence, Crystallography, X-Ray, G-Protein-Coupled Receptor Kinase 4 genetics, Humans, Models, Molecular, Molecular Sequence Data, Phosphorylation, Protein Conformation, Sequence Homology, Amino Acid, Substrate Specificity, G-Protein-Coupled Receptor Kinase 4 chemistry, G-Protein-Coupled Receptor Kinase 4 metabolism, Hypertension genetics

Abstract

G-protein-coupled receptor (GPCR) kinases (GRKs) bind to and phosphorylate GPCRs, initiating the process of GPCR desensitization and internalization. GRK4 is implicated in the regulation of blood pressure, and three GRK4 polymorphisms (R65L, A142V, and A486V) are associated with hypertension. Here, we describe the 2.6 Å structure of human GRK4α A486V crystallized in the presence of 5'-adenylyl β,γ-imidodiphosphate. The structure of GRK4α is similar to other GRKs, although slight differences exist within the RGS homology (RH) bundle subdomain, substrate-binding site, and kinase C-tail. The RH bundle subdomain and kinase C-terminal lobe form a strikingly acidic surface, whereas the kinase N-terminal lobe and RH terminal subdomain surfaces are much more basic. In this respect, GRK4α is more similar to GRK2 than GRK6. A fully ordered kinase C-tail reveals interactions linking the C-tail with important determinants of kinase activity, including the αB helix, αD helix, and the P-loop. Autophosphorylation of wild-type GRK4α is required for full kinase activity, as indicated by a lag in phosphorylation of a peptide from the dopamine D1 receptor without ATP preincubation. In contrast, this lag is not observed in GRK4α A486V. Phosphopeptide mapping by mass spectrometry indicates an increased rate of autophosphorylation of a number of residues in GRK4α A486V relative to wild-type GRK4α, including Ser-485 in the kinase C-tail., (© 2015 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2015

11. Tricyclic 1,5-naphthyridinone oxabicyclooctane-linked novel bacterial topoisomerase inhibitors as broad-spectrum antibacterial agents-SAR of left-hand-side moiety (Part-2).

Author

Singh SB, Kaelin DE, Wu J, Miesel L, Tan CM, Black T, Nargund R, Meinke PT, Olsen DB, Lagrutta A, Lu J, Patel S, Rickert KW, Smith RF, Soisson S, Sherer E, Joyce LA, Wei C, Peng X, Wang X, Fukuda H, Kishii R, Takei M, Takano H, Shibasaki M, Yajima M, Nishimura A, Shibata T, and Fukuda Y

Subjects

Anti-Bacterial Agents chemical synthesis, Anti-Bacterial Agents chemistry, Cyclooctanes chemical synthesis, Cyclooctanes chemistry, Dose-Response Relationship, Drug, Gram-Negative Bacteria enzymology, Gram-Positive Bacteria enzymology, Microbial Sensitivity Tests, Models, Molecular, Molecular Structure, Naphthyridines chemical synthesis, Naphthyridines chemistry, Structure-Activity Relationship, Topoisomerase II Inhibitors chemical synthesis, Topoisomerase II Inhibitors chemistry, Anti-Bacterial Agents pharmacology, Cyclooctanes pharmacology, DNA Topoisomerases, Type II metabolism, Gram-Negative Bacteria drug effects, Gram-Positive Bacteria drug effects, Naphthyridines pharmacology, Topoisomerase II Inhibitors pharmacology

Abstract

Novel bacterial topoisomerase inhibitors (NBTIs) represent a new class of broad-spectrum antibacterial agents targeting bacterial Gyrase A and ParC and have potential utility in combating antibiotic resistance. A series of novel oxabicyclooctane-linked NBTIs with new tricyclic-1,5-naphthyridinone left hand side moieties have been described. Compounds with a (R)-hydroxy-1,5-naphthyridinone moiety (7) showed potent antibacterial activity (e.g., Staphylococcus aureus MIC 0.25 μg/mL), acceptable Gram-positive and Gram-negative spectrum with rapidly bactericidal activity. The compound 7 showed intravenous and oral efficacy (ED50) at 3.2 and 27 mg/kg doses, respectively, in a murine model of bacteremia. Most importantly they showed significant attenuation of functional hERG activity (IC50 >170 μM). In general, lower logD attenuated hERG activity but also reduced Gram-negative activity. The co-crystal structure of a hydroxy-tricyclic NBTI bound to a DNA-gyrase complex exhibited a binding mode that show enantiomeric preference for R isomer and explains the activity and SAR. The discovery, synthesis, SAR and X-ray crystal structure of the left-hand-side tricyclic 1,5-naphthyridinone based oxabicyclooctane linked NBTIs are described., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

12. Oxabicyclooctane-linked novel bacterial topoisomerase inhibitors as broad spectrum antibacterial agents.

Author

Singh SB, Kaelin DE, Wu J, Miesel L, Tan CM, Meinke PT, Olsen D, Lagrutta A, Bradley P, Lu J, Patel S, Rickert KW, Smith RF, Soisson S, Wei C, Fukuda H, Kishii R, Takei M, and Fukuda Y

Abstract

Bacterial resistance is eroding the clinical utility of existing antibiotics necessitating the discovery of new agents. Bacterial type II topoisomerase is a clinically validated, highly effective, and proven drug target. This target is amenable to inhibition by diverse classes of inhibitors with alternative and distinct binding sites to quinolone antibiotics, thus enabling the development of agents that lack cross-resistance to quinolones. Described here are novel bacterial topoisomerase inhibitors (NBTIs), which are a new class of gyrase and topo IV inhibitors and consist of three distinct structural moieties. The substitution of the linker moiety led to discovery of potent broad-spectrum NBTIs with reduced off-target activity (hERG IC50 > 18 μM) and improved physical properties. AM8191 is bactericidal and selectively inhibits DNA synthesis and Staphylococcus aureus gyrase (IC50 = 1.02 μM) and topo IV (IC50 = 10.4 μM). AM8191 showed parenteral and oral efficacy (ED50) at less than 2.5 mg/kg doses in a S. aureus murine infection model. A cocrystal structure of AM8191 bound to S. aureus DNA-gyrase showed binding interactions similar to that reported for GSK299423, displaying a key contact of Asp83 with the basic amine at position-7 of the linker.

Published

2014

13. Structure of the bacterial deacetylase LpxC bound to the nucleotide reaction product reveals mechanisms of oxyanion stabilization and proton transfer.

Author

Clayton GM, Klein DJ, Rickert KW, Patel SB, Kornienko M, Zugay-Murphy J, Reid JC, Tummala S, Sharma S, Singh SB, Miesel L, Lumb KJ, and Soisson SM

Subjects

Amidohydrolases metabolism, Crystallography, X-Ray, Lipopolysaccharides biosynthesis, Lipopolysaccharides chemistry, Myristic Acids metabolism, Protein Structure, Tertiary, Uridine Diphosphate N-Acetylglucosamine chemistry, Uridine Diphosphate N-Acetylglucosamine metabolism, Amidohydrolases chemistry, Escherichia coli enzymology, Myristic Acids chemistry, Protons, Uridine Diphosphate N-Acetylglucosamine analogs & derivatives

Abstract

The emergence of antibiotic-resistant strains of pathogenic bacteria is an increasing threat to global health that underscores an urgent need for an expanded antibacterial armamentarium. Gram-negative bacteria, such as Escherichia coli, have become increasingly important clinical pathogens with limited treatment options. This is due in part to their lipopolysaccharide (LPS) outer membrane components, which dually serve as endotoxins while also protecting Gram-negative bacteria from antibiotic entry. The LpxC enzyme catalyzes the committed step of LPS biosynthesis, making LpxC a promising target for new antibacterials. Here, we present the first structure of an LpxC enzyme in complex with the deacetylation reaction product, UDP-(3-O-(R-3-hydroxymyristoyl))-glucosamine. These studies provide valuable insight into recognition of substrates and products by LpxC and a platform for structure-guided drug discovery of broad spectrum Gram-negative antibiotics.

Published

2013

14. Discovery of 1-[3-(1-methyl-1H-pyrazol-4-yl)-5-oxo-5H-benzo[4,5]cyclohepta[1,2-b]pyridin-7-yl]-N-(pyridin-2-ylmethyl)methanesulfonamide (MK-8033): A Specific c-Met/Ron dual kinase inhibitor with preferential affinity for the activated state of c-Met.

Author

Northrup AB, Katcher MH, Altman MD, Chenard M, Daniels MH, Deshmukh SV, Falcone D, Guerin DJ, Hatch H, Li C, Lu W, Lutterbach B, Allison TJ, Patel SB, Reilly JF, Reutershan M, Rickert KW, Rosenstein C, Soisson SM, Szewczak AA, Walker D, Wilson K, Young JR, Pan BS, and Dinsmore CJ

Subjects

Animals, Benzocycloheptenes chemistry, Cell Line, Tumor, Dogs, Enzyme Activation drug effects, Female, Humans, Mice, Models, Molecular, Protein Conformation, Protein Kinase Inhibitors chemistry, Protein Kinase Inhibitors metabolism, Protein Kinase Inhibitors pharmacology, Proto-Oncogene Proteins c-met chemistry, Rats, Substrate Specificity, Sulfonamides chemistry, Xenograft Model Antitumor Assays, Benzocycloheptenes metabolism, Benzocycloheptenes pharmacology, Drug Discovery, Proto-Oncogene Proteins c-met antagonists & inhibitors, Proto-Oncogene Proteins c-met metabolism, Receptor Protein-Tyrosine Kinases antagonists & inhibitors, Sulfonamides metabolism, Sulfonamides pharmacology

Abstract

This report documents the first example of a specific inhibitor of protein kinases with preferential binding to the activated kinase conformation: 5H-benzo[4,5]cyclohepta[1,2-b]pyridin-5-one 11r (MK-8033), a dual c-Met/Ron inhibitor under investigation as a treatment for cancer. The design of 11r was based on the desire to reduce time-dependent inhibition of CYP3A4 (TDI) by members of this structural class. A novel two-step protocol for the synthesis of benzylic sulfonamides was developed to access 11r and analogues. We provide a rationale for the observed selectivity based on X-ray crystallographic evidence and discuss selectivity trends with additional examples. Importantly, 11r provides full inhibition of tumor growth in a c-Met amplified (GTL-16) subcutaneous tumor xenograft model and may have an advantage over inactive form kinase inhibitors due to equal potency against a panel of oncogenic activating mutations of c-Met in contrast to c-Met inhibitors without preferential binding to the active kinase conformation.

Published

2013

15. Discovery of a 5H-benzo[4,5]cyclohepta[1,2-b]pyridin-5-one (MK-2461) inhibitor of c-Met kinase for the treatment of cancer.

Author

Katz JD, Jewell JP, Guerin DJ, Lim J, Dinsmore CJ, Deshmukh SV, Pan BS, Marshall CG, Lu W, Altman MD, Dahlberg WK, Davis L, Falcone D, Gabarda AE, Hang G, Hatch H, Holmes R, Kunii K, Lumb KJ, Lutterbach B, Mathvink R, Nazef N, Patel SB, Qu X, Reilly JF, Rickert KW, Rosenstein C, Soisson SM, Spencer KB, Szewczak AA, Walker D, Wang W, Young J, and Zeng Q

Subjects

Animals, Antineoplastic Agents pharmacokinetics, Antineoplastic Agents pharmacology, Benzocycloheptenes pharmacokinetics, Benzocycloheptenes pharmacology, Cell Line, Tumor, Crystallography, X-Ray, Dogs, Drug Screening Assays, Antitumor, Female, Haplorhini, Humans, Mice, Mice, Nude, Models, Molecular, Mutation, Neoplasm Transplantation, Phosphorylation, Protein Binding, Pyrazoles chemical synthesis, Pyrazoles pharmacokinetics, Pyrazoles pharmacology, Pyridines pharmacokinetics, Pyridines pharmacology, Rats, Receptor Protein-Tyrosine Kinases genetics, Structure-Activity Relationship, Sulfonamides chemical synthesis, Sulfonamides pharmacokinetics, Sulfonamides pharmacology, Transplantation, Heterologous, Antineoplastic Agents chemical synthesis, Benzocycloheptenes chemical synthesis, Pyridines chemical synthesis, Receptor Protein-Tyrosine Kinases antagonists & inhibitors

Abstract

c-Met is a transmembrane tyrosine kinase that mediates activation of several signaling pathways implicated in aggressive cancer phenotypes. In recent years, research into this area has highlighted c-Met as an attractive cancer drug target, triggering a number of approaches to disrupt aberrant c-Met signaling. Screening efforts identified a unique class of 5H-benzo[4,5]cyclohepta[1,2-b]pyridin-5-one kinase inhibitors, exemplified by 1. Subsequent SAR studies led to the development of 81 (MK-2461), a potent inhibitor of c-Met that was efficacious in preclinical animal models of tumor suppression. In addition, biochemical studies and X-ray analysis have revealed that this unique class of kinase inhibitors binds preferentially to the activated (phosphorylated) form of the kinase. This report details the development of 81 and provides a description of its unique biochemical properties.

Published

2011

16. Structural basis for selective small molecule kinase inhibition of activated c-Met.

Author

Rickert KW, Patel SB, Allison TJ, Byrne NJ, Darke PL, Ford RE, Guerin DJ, Hall DL, Kornienko M, Lu J, Munshi SK, Reid JC, Shipman JM, Stanton EF, Wilson KJ, Young JR, Soisson SM, and Lumb KJ

Subjects

Animals, Cell Line, Crystallography, X-Ray, Drug Design, Humans, Phosphorylation, Protein Binding, Protein Structure, Secondary, Protein Structure, Tertiary, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins metabolism, Receptor Protein-Tyrosine Kinases genetics, Receptor Protein-Tyrosine Kinases metabolism, Spodoptera, Structure-Activity Relationship, c-Mer Tyrosine Kinase, Protein Kinase Inhibitors chemistry, Proto-Oncogene Proteins antagonists & inhibitors, Proto-Oncogene Proteins chemistry, Receptor Protein-Tyrosine Kinases antagonists & inhibitors, Receptor Protein-Tyrosine Kinases chemistry

Abstract

The receptor tyrosine kinase c-Met is implicated in oncogenesis and is the target for several small molecule and biologic agents in clinical trials for the treatment of cancer. Binding of the hepatocyte growth factor to the cell surface receptor of c-Met induces activation via autophosphorylation of the kinase domain. Here we describe the structural basis of c-Met activation upon autophosphorylation and the selective small molecule inhibiton of autophosphorylated c-Met. MK-2461 is a potent c-Met inhibitor that is selective for the phosphorylated state of the enzyme. Compound 1 is an MK-2461 analog with a 20-fold enthalpy-driven preference for the autophosphorylated over unphosphorylated c-Met kinase domain. The crystal structure of the unbound kinase domain phosphorylated at Tyr-1234 and Tyr-1235 shows that activation loop phosphorylation leads to the ejection and disorder of the activation loop and rearrangement of helix αC and the G loop to generate a viable active site. Helix αC adopts a orientation different from that seen in activation loop mutants. The crystal structure of the complex formed by the autophosphorylated c-Met kinase domain and compound 1 reveals a significant induced fit conformational change of the G loop and ordering of the activation loop, explaining the selectivity of compound 1 for the autophosphorylated state. The results highlight the role of structural plasticity within the kinase domain in imparting the specificity of ligand binding and provide the framework for structure-guided design of activated c-Met inhibitors.

Published

2011

17. Structural definition and substrate specificity of the S28 protease family: the crystal structure of human prolylcarboxypeptidase.

Author

Soisson SM, Patel SB, Abeywickrema PD, Byrne NJ, Diehl RE, Hall DL, Ford RE, Reid JC, Rickert KW, Shipman JM, Sharma S, and Lumb KJ

Subjects

Amino Acid Sequence, Binding Sites, Carboxypeptidases genetics, Carboxypeptidases metabolism, Catalytic Domain, Crystallography, X-Ray, Humans, Molecular Sequence Data, Protein Structure, Tertiary, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sequence Alignment, Sequence Homology, Amino Acid, Substrate Specificity, Carboxypeptidases chemistry

Abstract

Background: The unique S28 family of proteases is comprised of the carboxypeptidase PRCP and the aminopeptidase DPP7. The structural basis of the different substrate specificities of the two enzymes is not understood nor has the structure of the S28 fold been described., Results: The experimentally phased 2.8 A crystal structure is presented for human PRCP. PRCP contains an alpha/beta hydrolase domain harboring the catalytic Asp-His-Ser triad and a novel helical structural domain that caps the active site. Structural comparisons with prolylendopeptidase and DPP4 identify the S1 proline binding site of PRCP. A structure-based alignment with the previously undescribed structure of DPP7 illuminates the mechanism of orthogonal substrate specificity of PRCP and DPP7. PRCP has an extended active-site cleft that can accommodate proline substrates with multiple N-terminal residues. In contrast, the substrate binding groove of DPP7 is occluded by a short amino-acid insertion unique to DPP7 that creates a truncated active site selective for dipeptidyl proteolysis of N-terminal substrates., Conclusion: The results define the structure of the S28 family of proteases, provide the structural basis of PRCP and DPP7 substrate specificity and enable the rational design of selective PRCP modulators.

Published

2010

18. Expression, purification and crystallization of human prolylcarboxypeptidase.

Author

Abeywickrema PD, Patel SB, Byrne NJ, Diehl RE, Hall DL, Ford RE, Rickert KW, Reid JC, Shipman JM, Geissler WM, Pryor KD, SinhaRoy R, Soisson SM, Lumb KJ, and Sharma S

Subjects

Animals, CHO Cells, Carboxypeptidases genetics, Carboxypeptidases isolation & purification, Cricetinae, Cricetulus, Crystallization, Crystallography, X-Ray, Gene Expression, Glycosylation, Humans, Carboxypeptidases chemistry

Abstract

Prolylcarboxypeptidase (PrCP) is a lysosomal serine carboxypeptidase that cleaves a variety of C-terminal amino acids adjacent to proline and has been implicated in diseases such as hypertension and obesity. Here, the robust production, purification and crystallization of glycosylated human PrCP from stably transformed CHO cells is described. Purified PrCP yielded crystals belonging to space group R32, with unit-cell parameters a = b = 181.14, c = 240.13 A, that diffracted to better than 2.8 A resolution.

Published

2010

19. Structure of human prostasin, a target for the regulation of hypertension.

Author

Rickert KW, Kelley P, Byrne NJ, Diehl RE, Hall DL, Montalvo AM, Reid JC, Shipman JM, Thomas BW, Munshi SK, Darke PL, and Su HP

Subjects

Amino Acid Sequence, Apoproteins chemistry, Benzamidines, Crystallography, X-Ray methods, Escherichia coli metabolism, Guanidines chemistry, Humans, Molecular Conformation, Molecular Sequence Data, Protein Conformation, Protein Folding, Protein Renaturation, Sequence Homology, Amino Acid, Serine Endopeptidases genetics, Substrate Specificity, Hypertension metabolism, Serine Endopeptidases chemistry

Abstract

Prostasin (also called channel activating protease-1 (CAP1)) is an extracellular serine protease implicated in the modulation of fluid and electrolyte regulation via proteolysis of the epithelial sodium channel. Several disease states, particularly hypertension, can be affected by modulation of epithelial sodium channel activity. Thus, understanding the biochemical function of prostasin and developing specific agents to inhibit its activity could have a significant impact on a widespread disease. We report the expression of the prostasin proenzyme in Escherichia coli as insoluble inclusion bodies, refolding and activating via proteolytic removal of the N-terminal propeptide. The refolded and activated enzyme was shown to be pure and monomeric, with kinetic characteristics very similar to prostasin expressed from eukaryotic systems. Active prostasin was crystallized, and the structure was determined to 1.45 A resolution. These apoprotein crystals were soaked with nafamostat, allowing the structure of the inhibited acyl-enzyme intermediate structure to be determined to 2.0 A resolution. Comparison of the inhibited and apoprotein forms of prostasin suggest a mechanism of regulation through stabilization of a loop which interferes with substrate recognition.

Published

2008

20. Discovery and biochemical characterization of selective ATP competitive inhibitors of the human mitotic kinesin KSP.

Author

Rickert KW, Schaber M, Torrent M, Neilson LA, Tasber ES, Garbaccio R, Coleman PJ, Harvey D, Zhang Y, Yang Y, Marshall G, Lee L, Walsh ES, Hamilton K, and Buser CA

Subjects

Adenosine Triphosphate chemistry, Allosteric Site, Binding, Competitive, Drug Design, Humans, Kinesins metabolism, Models, Biological, Models, Chemical, Nucleotides chemistry, Phenotype, Protein Binding, Thiazoles pharmacology, Adenosine Triphosphate metabolism, Biochemistry methods, Kinesins antagonists & inhibitors, Kinesins chemistry, Mitosis

Abstract

The kinesin spindle protein (KSP, also known as Eg5) is essential for the proper separation of spindle poles during mitosis, and inhibition results in mitotic arrest and the formation of characteristic monoaster spindles. Several distinct classes of KSP inhibitors have been described previously in the public and patent literature. However, most appear to share a common induced-fit allosteric binding site, suggesting a common mechanism of inhibition. In a high-throughput screen for inhibitors of KSP, a novel class of thiazole-containing inhibitors was identified. Unlike the previously described allosteric KSP inhibitors, the thiazoles described here show ATP competitive kinetic behavior, consistent with binding within the nucleotide binding pocket. Although they bind to a pocket that is highly conserved across kinesins, these molecules exhibit significant selectivity for KSP over other kinesins and other ATP-utilizing enzymes. Several of these compounds are active in cells and produce a phenotype similar to that observed with previously published allosteric inhibitors of KSP.

Published

2008

21. Potent 2-[(pyrimidin-4-yl)amine}-1,3-thiazole-5-carbonitrile-based inhibitors of VEGFR-2 (KDR) kinase.

Author

Sisko JT, Tucker TJ, Bilodeau MT, Buser CA, Ciecko PA, Coll KE, Fernandes C, Gibbs JB, Koester TJ, Kohl N, Lynch JJ, Mao X, McLoughlin D, Miller-Stein CM, Rodman LD, Rickert KW, Sepp-Lorenzino L, Shipman JM, Thomas KA, Wong BK, and Hartman GD

Subjects

Animals, Dogs, Macaca mulatta, Molecular Structure, Nitriles chemistry, Protein Kinase Inhibitors chemistry, Pyrimidines chemistry, Rats, Sensitivity and Specificity, Structure-Activity Relationship, Thiazoles chemistry, Vascular Endothelial Growth Factor Receptor-2 metabolism, Nitriles chemical synthesis, Nitriles pharmacology, Protein Kinase Inhibitors chemical synthesis, Protein Kinase Inhibitors pharmacology, Pyrimidines chemical synthesis, Pyrimidines pharmacology, Thiazoles chemical synthesis, Thiazoles pharmacology, Vascular Endothelial Growth Factor Receptor-2 antagonists & inhibitors

Abstract

Pyrimidino-thiazolyl carbonitriles were prepared that are potent VEGFR-2 (KDR) kinase inhibitors. The modification of lead structures resulted in 3m which exhibited the best overall profile in KDR inhibitory activity, iv/po pharmacokinetics, and reduced hERG affinity.

Published

2006

22. Potent N-(1,3-thiazol-2-yl)pyridin-2-amine vascular endothelial growth factor receptor tyrosine kinase inhibitors with excellent pharmacokinetics and low affinity for the hERG ion channel.

Author

Bilodeau MT, Balitza AE, Koester TJ, Manley PJ, Rodman LD, Buser-Doepner C, Coll KE, Fernandes C, Gibbs JB, Heimbrook DC, Huckle WR, Kohl N, Lynch JJ, Mao X, McFall RC, McLoughlin D, Miller-Stein CM, Rickert KW, Sepp-Lorenzino L, Shipman JM, Subramanian R, Thomas KA, Wong BK, Yu S, and Hartman GD

Subjects

Administration, Oral, Aminopyridines pharmacokinetics, Aminopyridines pharmacology, Animals, Biological Availability, Cell Line, Dogs, ERG1 Potassium Channel, Electrocardiography drug effects, Ether-A-Go-Go Potassium Channels, In Vitro Techniques, Lung enzymology, Macaca mulatta, Male, Mice, Microsomes, Liver metabolism, Phosphorylation, Pyridines pharmacokinetics, Pyridines pharmacology, Radioligand Assay, Rats, Rats, Sprague-Dawley, Thiazoles pharmacokinetics, Thiazoles pharmacology, Tissue Distribution, Vascular Endothelial Growth Factor Receptor-2 metabolism, Aminopyridines chemical synthesis, Potassium Channels, Voltage-Gated metabolism, Pyridines chemical synthesis, Receptors, Vascular Endothelial Growth Factor antagonists & inhibitors, Thiazoles chemical synthesis

Abstract

A series of N-(1,3-thiazol-2-yl)pyridin-2-amine KDR kinase inhibitors have been developed that possess optimal properties. Compounds have been discovered that exhibit excellent in vivo potency. The particular challenges of overcoming hERG binding activity and QTc increases in vivo in addition to achieving good pharmacokinetics have been acomplished by discovering a unique class of amine substituents. These compounds have a favorable kinase selectivity profile that can be accentuated with appropriate substitution.

Published

2004

23. The discovery of N-(1,3-thiazol-2-yl)pyridin-2-amines as potent inhibitors of KDR kinase.

Author

Bilodeau MT, Rodman LD, McGaughey GB, Coll KE, Koester TJ, Hoffman WF, Hungate RW, Kendall RL, McFall RC, Rickert KW, Rutledge RZ, and Thomas KA

Subjects

Amines chemical synthesis, Binding Sites, Enzyme Inhibitors chemical synthesis, Enzyme Inhibitors pharmacology, Humans, Inhibitory Concentration 50, Models, Molecular, Protein Binding, Protein Conformation drug effects, Structure-Activity Relationship, Thermodynamics, Vascular Endothelial Growth Factor Receptor-2 chemistry, Amines pharmacology, Vascular Endothelial Growth Factor Receptor-2 antagonists & inhibitors

Abstract

An azo-dye lead was modified to a novel N-(1,3-thiazol-2-yl)pyridin-2-amine series of KDR kinase inhibitors through the use of rapid analog libraries. This new class has been found to be potent, selective, and of low molecular weight. Molecular modeling has postulated an interesting conformational preference and binding mode for these compounds in the active site of the enzyme.

Published

2004

24. 2,4-disubstituted pyrimidines: a novel class of KDR kinase inhibitors.

Author

Manley PJ, Balitza AE, Bilodeau MT, Coll KE, Hartman GD, McFall RC, Rickert KW, Rodman LD, and Thomas KA

Subjects

Angiogenesis Inhibitors pharmacology, Antineoplastic Agents chemical synthesis, Antineoplastic Agents pharmacology, Cells, Cultured, Enzyme Inhibitors chemical synthesis, Enzyme Inhibitors pharmacology, Humans, Inhibitory Concentration 50, Pyrimidines chemical synthesis, Structure-Activity Relationship, Angiogenesis Inhibitors chemical synthesis, Pyrimidines pharmacology, Vascular Endothelial Growth Factor Receptor-2 antagonists & inhibitors

Abstract

2,4-Disubstituted pyrimidines were synthesized as a novel class of KDR kinase inhibitors. Evaluation of the SAR of the screening lead compound 1 (KDR IC(50)=105 nM, Cell IC(50)=8% inhibition at 500 nM) led to the potent 3,5-dimethylaniline derivative 2d (KDR IC(50)=6 nM, cell IC(50)=19 nM).

Published

2003

25. Nature of hydrogen transfer in soybean lipoxygenase 1: separation of primary and secondary isotope effects.

Author

Rickert KW and Klinman JP

Subjects

Catalysis, Deuterium, Electron Transport, Hydrogen chemistry, Kinetics, Linoleic Acid chemistry, Linoleic Acid metabolism, Lipoxygenase chemistry, Lipoxygenase genetics, Models, Chemical, Models, Molecular, Mutagenesis, Site-Directed, Plant Proteins chemistry, Plant Proteins metabolism, Stereoisomerism, Hydrogen metabolism, Lipoxygenase metabolism, Glycine max enzymology

Abstract

Previous measurements of the kinetics of oxidation of linoleic acid by soybean lipoxygenase 1 have indicated very large deuterium isotope effects, but have not been able to distinguish the primary isotope effect from the alpha-secondary effect. To address this question, singly deuterated linoleic acid was prepared, and enantiomerically resolved using the enzyme itself. Noncompetitive measurements of the primary deuterium isotope effect give a value of ca. 40 which is temperature-independent. The enthalpy of activation is low and isotope-independent, and there is a large isotope effect on the Arrhenius prefactor. A very large apparent secondary isotope effect (ca. 2.1) is measured with deuterium in the primary position, but a greatly reduced value (1.1) is observed with protium in the primary position. Mutagenesis of the active site leads to a significant reduction in k(cat) and perturbed isotope effects, in particular, a secondary effect of 5.6 when deuterium is in the primary position. The anomalous secondary isotope effects are shown to arise from imperfect stereoselectivity of hydrogen abstraction which, for the mutant, is attributed to a combination of inverse substrate binding and increased flexibility at the reactive carbon. After correction, a very large primary (76-84) and small secondary (1.1-1.2) kinetic isotope effects are calculated for both mutant and wild-type enzymes. The weight of the evidence is taken to favor hydrogen tunneling as the primary mechanism of hydrogen transfer.

Published

1999

26. Analysis of the conserved glycosylation site in the nicotinic acetylcholine receptor: potential roles in complex assembly.

Author

Rickert KW and Imperiali B

Subjects

Amino Acid Sequence, Animals, Circular Dichroism, Conserved Sequence, Disulfides, Glycopeptides chemistry, Glycosylation, Kinetics, Molecular Sequence Data, Nuclear Magnetic Resonance, Biomolecular, Protein Folding, Receptors, Nicotinic biosynthesis, Swine, Thermodynamics, Receptors, Nicotinic metabolism

Abstract

Background: Assembly of the functional nicotinic acetylcholine receptor (nAChR) is dependent on a series of exquisitely coordinated events including polypeptide synthesis and processing, side-chain elaboration through post-translational modifications, and subunit oligomerization. A 17-residue sequence that includes a cystine disulfide and an N-linked glycosylation site is conserved in the extracellular domain of each of the nAChR subunits, and is involved in intersubunit interactions that are critical for assembly of intact, pentameric complexes. A polypeptide representing the relevant sequence from the alpha-subunit of the nAChR (Ac-Tyr-Cys-Glu-Ile-Ile-Val-Thr-His-Phe-Pro-Phe-Asp-Gln-Gln Asn-Cys-Thr-NH2) is small enough to allow detailed structural analysis, which may provide insight into the role of glycosylation in the maturation process that leads to ion-channel assembly. We therefore investigated the effect of N-linked glycosylation on the structure of this heptadecapeptide., Results: Thermodynamic analysis shows that glycosylation alters disulfide formation in the loop peptide, shifting the equilibrium in favor of the disulfide. Spectroscopic studies reveal that the cis/trans amide isomer ratio of the proline is also affected by the modification, with a resultant shift in the equilibrium in favor of the trans isomer, even though the proline is several residues removed from the glycosylation site. Two-dimensional NMR analysis of the glycopeptide does not indicate the presence of any specific interactions between the carbohydrate and the peptide., Conclusions: These studies demonstrate that glycosylation can have a significant influence on disulfide formation and proline isomerization in a local peptide sequence. As both these processes are considered slow steps in protein folding, it is evident that N-linked glycosylation has important indirect roles that influence the folding of the receptor subunit and assembly of the pentameric complex.

Published

1995

27. Conformational implications of asparagine-linked glycosylation.

Author

Imperiali B and Rickert KW

Subjects

Amino Acid Sequence, Fluorescent Dyes, Glycoproteins chemical synthesis, Glycosylation, Hemagglutinins chemistry, Immunoglobulin A chemistry, Immunoglobulin Fab Fragments chemistry, Indicators and Reagents, Kinetics, Molecular Sequence Data, Oligopeptides chemical synthesis, Solvents, Spectrometry, Fluorescence, Spectrophotometry, Ultraviolet, Structure-Activity Relationship, Time Factors, Transferases, Asparagine, Glycopeptides chemistry, Glycoproteins chemistry, Hexosyltransferases, Membrane Proteins, Oligopeptides chemistry, Protein Conformation, Protein Folding

Abstract

The effects of cotranslational protein modification on the process of protein folding are poorly understood. Time-resolved fluorescence energy transfer has been used to assess the impact of glycosylation on the conformational dynamics of flexible oligopeptides. The peptide sequences examined are selected from glycoproteins of known three-dimensional structure. The energy transfer modulation associated with N-linked glycosylation is consistent with the glycopeptides sampling different conformational profiles in water. Results show that glycosylation causes the modified peptides to adopt a different ensemble of conformations, and for some peptides this change may lead to conformations that are more compact and better approximate the conformation of these peptides in the final folded protein. This result further implies that cotranslational glycosylation can trigger the timely formation of structural nucleation elements and thus assist in the complex process of protein folding.

Published

1995

28. Mechanism of irreversible inhibition of O2 evolution in photosystem II by Tris(hydroxymethyl)aminomethane.

Author

Rickert KW, Sears J, Beck WF, and Brudvig GW

Subjects

Electron Spin Resonance Spectroscopy, Kinetics, Manganese analysis, Oxygen metabolism, Photosystem II Protein Complex, Photosynthetic Reaction Center Complex Proteins antagonists & inhibitors, Plants metabolism, Tromethamine pharmacology

Abstract

The dark reaction of tris(hydroxymethyl)aminomethane (Tris) with the O2-evolving center of photosystem II (PSII) in the S1 state causes irreversible inhibition of O2 evolution. Similar inhibition is observed for several other amines: NH3, CH3NH2, (CH3)2NH, ethanolamine, and 2-amino-2-ethyl-1,3-propanediol. In PSII membranes, both depleted of the 17- and 23-kDa polypeptides and undepleted, the rate of reaction of Tris depends inversely upon the Cl- concentration. However, the rate of reaction of Tris is about 2-fold greater with PSII membranes depleted of the 17- and 23-kDa polypeptides than with undepleted PSII membranes. We have used low-temperature electron paramagnetic resonance (EPR) spectroscopy to study the effect of Tris on the oxidation state of the Mn complex in the O2-evolving center, to monitor the electron-donation reactions in Tris-treated samples, and to observe any loss of the Mn complex (forming Mn2+ ions) after Tris treatment. We find that Tris treatment causes loss of electron-donation ability from the Mn complex at the same rate as inhibition of O2 evolution and that Mn2+ ions are released. We conclude that Tris reduces the Mn complex to labile Mn2+ ions, without generating any kinetically stable, partially reduced intermediates, and that the reaction occurs at the Cl(-)-sensitive site previously characterized in studies of the reversible inhibition of O2 evolution by amines.

Published

1991