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2. Preclinical characterization of the Toll-like receptor 7/8 antagonist MHV370 for lupus therapy

Author

Hawtin, Stuart, André, Cédric, Collignon-Zipfel, Géraldine, Appenzeller, Simone, Bannert, Bettina, Baumgartner, Lea, Beck, Damian, Betschart, Claudia, Boulay, Thomas, Brunner, Hermine I., Ceci, Melanie, Deane, Jonathan, Feifel, Roland, Ferrero, Enrico, Kyburz, Diego, Lafossas, Frederique, Loetscher, Pius, Merz-Stoeckle, Christina, Michellys, Pierre, Nuesslein-Hildesheim, Barbara, Raulf, Friedrich, Rush, James S., Ruzzante, Giulia, Stein, Thomas, Zaharevitz, Samantha, Wieczorek, Grazyna, Siegel, Richard, Gergely, Peter, Shisha, Tamas, and Junt, Tobias

Published
2023
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3. Discovery of the TLR7/8 Antagonist MHV370 for Treatment of Systemic Autoimmune Diseases

Author

Alper, Phil, primary, Betschart, Claudia, additional, André, Cédric, additional, Boulay, Thomas, additional, Cheng, Dai, additional, Deane, Jonathan, additional, Faller, Michael, additional, Feifel, Roland, additional, Glatthar, Ralf, additional, Han, Dong, additional, Hemmig, Rene, additional, Jiang, Tao, additional, Knoepfel, Thomas, additional, Maginnis, Jillian, additional, Mutnick, Daniel, additional, Pei, Wei, additional, Ruzzante, Giulia, additional, Syka, Peter, additional, Zhang, Guobao, additional, Zhang, Yi, additional, Zink, Florence, additional, Zipfel, Géraldine, additional, Hawtin, Stuart, additional, Junt, Tobias, additional, and Michellys, Pierre-Yves, additional

Published
2023
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4. A root cause analysis to identify the mechanistic drivers of immunogenicity against the anti-VEGF biotherapeutic brolucizumab

Author

Kearns, Jeffrey D., primary, Wassmann, Paul, additional, Olgac, Ufuk, additional, Fichter, Marie, additional, Christen, Brigitte, additional, Rubic-Schneider, Tina, additional, Koepke, Stephan, additional, Cochin de Billy, Benjamin, additional, Ledieu, David, additional, Andre, Cedric, additional, Hawtin, Stuart, additional, Fischer, Benoit, additional, Moretti, Francesca, additional, Hug, Christian, additional, Bepperling, Alexander, additional, Brannetti, Barbara, additional, Mendez-Garcia, Celia, additional, Littlewood-Evans, Amanda, additional, Clemens, Andreas, additional, Grosskreutz, Cynthia L., additional, Mehan, Pawan, additional, Schmouder, Robert L., additional, Sasseville, Vito, additional, Brees, Dominique, additional, and Karle, Anette C., additional

Published
2023
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5. Nonhematopoietic IRAK1 drives arthritis via neutrophil chemoattractants

Author

Hoyler, Thomas, primary, Bannert, Bettina, additional, André, Cédric, additional, Beck, Damian, additional, Boulay, Thomas, additional, Buffet, David, additional, Caesar, Nadja, additional, Calzascia, Thomas, additional, Dawson, Janet, additional, Kyburz, Diego, additional, Hennze, Robert, additional, Huppertz, Christine, additional, Littlewood-Evans, Amanda, additional, Loetscher, Pius, additional, Mertz, Kirsten D., additional, Niwa, Satoru, additional, Robert, Gautier, additional, Rush, James S., additional, Ruzzante, Giulia, additional, Sarret, Sophie, additional, Stein, Thomas, additional, Touil, Ismahane, additional, Wieczorek, Grazyna, additional, Zipfel, Geraldine, additional, Hawtin, Stuart, additional, and Junt, Tobias, additional

Published
2022
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6. Structure-Based Optimization of a Fragment-like TLR8 Binding Screening Hit to an In Vivo Efficacious TLR7/8 Antagonist

Author

Betschart, Claudia, primary, Faller, Michael, additional, Zink, Florence, additional, Hemmig, René, additional, Blank, Jutta, additional, Vangrevelinghe, Eric, additional, Bourrel, Marjorie, additional, Glatthar, Ralf, additional, Behnke, Dirk, additional, Barker, Kerstin, additional, Heizmann, Andreas, additional, Angst, Daniela, additional, Nimsgern, Pierre, additional, Jacquier, Sébastien, additional, Junt, Tobias, additional, Zipfel, Géraldine, additional, Ruzzante, Giulia, additional, Loetscher, Pius, additional, Limonta, Sarah, additional, Hawtin, Stuart, additional, Andre, Cedric Bernard, additional, Boulay, Thomas, additional, Feifel, Roland, additional, and Knoepfel, Thomas, additional

Published
2022
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7. Discovery of potent, orally bioavailable in vivo efficacious antagonists of the TLR7/8 pathway

Author

Alper, Phil B., Deane, Jonathan, Betschart, Claudia, Buffet, David, Collignon Zipfel, Géraldine, Gordon, Perry, Hampton, Janice, Hawtin, Stuart, Ibanez, Maureen, Jiang, Tao, Junt, Tobias, Knoepfel, Thomas, Liu, Bo, Maginnis, Jillian, McKeever, Una, Michellys, Pierre-Yves, Mutnick, Daniel, Nayak, Bishnu, Niwa, Satoru, Richmond, Wendy, Rush, James S., Syka, Peter, Zhang, Yi, and Zhu, Xuefeng

Published
2020
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8. Agonist-specific, high-affinity binding epitopes are contributed by an arginine in the N-terminus of the human oxytocin receptor

Author

Wesley, Victoria J., Hawtin, Stuart R., Howard, Helen C., and Wheatley, Mark

Subjects
Peptide hormones -- Receptors, Oxytocin -- Research, Binding sites (Biochemistry) -- Analysis, Structure-activity relationships (Biochemistry) -- Analysis, Biological sciences, Chemistry
Abstract

Research demonstrates that within the N-terminus domain of the oxytocin rceptor, Arg34 is involved in the high-affinity agonist binding to the receptor as shown by a 2000-fold decrease in oxytocin affinity by removal or substitution of Arg34. Further, the arginyl residue is agonist-specific and is not essential for peptide or antagonist binding.

Published
2002

9. Target-Based Identification and Optimization of 5-Indazol-5-yl Pyridones as Toll-like Receptor 7 and 8 Antagonists Using a Biochemical TLR8 Antagonist Competition Assay

Author

Knoepfel, Thomas, primary, Nimsgern, Pierre, additional, Jacquier, Sébastien, additional, Bourrel, Marjorie, additional, Vangrevelinghe, Eric, additional, Glatthar, Ralf, additional, Behnke, Dirk, additional, Alper, Phil B., additional, Michellys, Pierre-Yves, additional, Deane, Jonathan, additional, Junt, Tobias, additional, Zipfel, Géraldine, additional, Limonta, Sarah, additional, Hawtin, Stuart, additional, Andre, Cedric, additional, Boulay, Thomas, additional, Loetscher, Pius, additional, Faller, Michael, additional, Blank, Jutta, additional, Feifel, Roland, additional, and Betschart, Claudia, additional

Published
2020
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10. Critical role of a subdomain of the N-terminus of the V(sub)1a vasopressin receptor for binding agonists but not antagonists; functional rescue by the oxytocin receptor N-terminus

Author

Hawtin, Stuart R., Wesley, Victoria J., Parslow, Rosmary A., Patel, Smita, and Wheatley, Mark

Subjects
Proteins -- Conformation, G proteins -- Physiological aspects, Vasopressin -- Analysis, Drug receptors -- Physiological aspects, Biological sciences, Chemistry
Abstract

Results demonstrate that a short segment of the N-terminus of the V(sub)1a vasopressin receptor is crucial for both agonist binding and receptor's ability to adopt for the agonist-induced conformational changes in the receptor.

Published
2000

16. Systematic analysis of the entire second extracellular loop of the V 1a vasopressin receptor :Key residues, conserved throughout a G-protein-coupled receptor family, identified

Author

Conner, Matthew, Hawtin, Stuart R., Simms, John, Wootten, Denise, Lawson, Zoe, Conner, Alex C., Parslow, Rosemary A., and Wheatley, Mark

Abstract

The roles of extracellular residues of G-protein-coupled receptors (GPCRs) are not well defined compared with residues in transmembrane helices. Nevertheless, it has been established that extracellular domains of both peptide-GPCRs and amine-GPCRs incorporate functionally important residues. Extracellular loop 2 (ECL2) has attracted particular interest, because the x-ray structure of bovine rhodopsin revealed that ECL2 projects into the binding crevice within the transmembrane bundle. Our study provides the first comprehensive investigation into the role of the individual residues comprising the entire ECL2 domain of a small peptide-GPCR. Using the V1a vasopressin receptor, systematic substitution of all of the ECL2 residues by Ala generated 30 mutant receptors that were characterized pharmacologically. The majority of these mutant receptor constructs (24 in total) had essentially wild-type ligand binding and intracellular signaling characteristics, indicating that these residues are not critical for normal receptor function. However, four aromatic residues Phe189, Trp206, Phe209, and Tyr218 are important for agonist binding and receptor activation and are highly conserved throughout the neurohypophysial hormone subfamily of peptide-GPCRs. Located in the middle of ECL2, juxtaposed to the highly conserved disulfide bond, Trp206 and Phe209 project into the binding crevice. Indeed, Phe209 is part of the Cys-X-X-X-Ar (where Ar is an aromatic residue) motif, which is well conserved in both peptide-GPCRs and amine-GPCRs. In contrast, Phe189 and Tyr218, located at the extreme ends of ECL2, may be important for determining the position of the ECL2 cap over the binding crevice. This study provides mechanistic insight into the roles of highly conserved ECL2 residues.

Published
2007

20. Charged extracellular residues, conserved throughout a G-protein-coupled receptor family, are required for ligand binding, receptor activation, and cell-surface expression

Author

Hawtin, Stuart R., Simms, John, Conner, Matthew, Lawson, Zoe, Parslow, Rosemary A., Trim, Julie, Sheppard, Andrew, Wheatley, Mark, Hawtin, Stuart R., Simms, John, Conner, Matthew, Lawson, Zoe, Parslow, Rosemary A., Trim, Julie, Sheppard, Andrew, and Wheatley, Mark

Abstract

For G-protein-coupled receptors (GPCRs) in general, the roles of extracellular residues are not well defined compared with residues in transmembrane helices (TMs). Nevertheless, extracellular residues are important for various functions in both peptide-GPCRs and amine-GPCRs. In this study, the V1a vasopressin receptor was used to systematically investigate the role of extracellular charged residues that are highly conserved throughout a subfamily of peptide-GPCRs, using a combination of mutagenesis and molecular modeling. Of the 13 conserved charged residues identified in the extracellular loops (ECLs), Arg116 (ECL1), Arg125 (top of TMIII), and Asp204 (ECL2) are important for agonist binding and/or receptor activation. Molecular modeling revealed that Arg125 (and Lys 125) stabilizes TMIII by interacting with lipid head groups. Charge reversal (Asp125) caused re-ordering of the lipids, altered helical packing, and increased solvent penetration of the TM bundle. Interestingly, a negative charge is excluded at this locus in peptide-GPCRs, whereas a positive charge is excluded in amine-GPCRs. This contrasting conserved charge may reflect differences in GPCR binding modes between peptides and amines, with amines needing to access a binding site crevice within the receptor TM bundle, whereas the binding site of peptide-GPCRs includes more extracellular domains. A conserved negative charge at residue 204 (ECL2), juxtaposed to the highly conserved disulfide bond, was essential for agonist binding and signaling. Asp204 (and Glu204) establishes TMIII contacts required for maintaining the α-hairpin fold of ECL2, which if broken (Ala204 or Arg204) resulted in ECL2 unfolding and receptor dysfunction. This study provides mechanistic insight into the roles of conserved extracellular residues.

Published
2006

38. Systematic Analysis of the Entire Second Extracellular Loop of the V1a Vasopressin Receptor.

Author

Conner, Matthew, Hawtin, Stuart R., Simms, John, Wootten, Denise, Lawson, Zoe, Conner, Alex C., Parslow, Rosemary A., and Wheatley, Mark

Subjects
*G proteins, *PHARMACOLOGY, *PEPTIDES, *VASOPRESSIN, *CHEMICAL bonds
Abstract

The roles of extracellular residues of G-protein-coupled receptors (GPCRs) are not well defined compared with residues in transmembrane helices. Nevertheless, it has been established that extracellular domains of both peptide-GPCRs and amine- GPCRs incorporate functionally important residues. Extracellular loop 2 (ECL2) has attracted particular interest, because the x-ray structure of bovine rhodopsin revealed that ECL2 projects into the binding crevice within the transmembrane bundle. Our study provides the first comprehensive investigation into the role of the individual residues comprising the entire ECL2 domain of a small peptide-GPCR. Using the V1a vasopressin receptor, systematic substitution of all of the ECL2 residues by Ala generated 30 mutant receptors that were characterized pharmacologically. The majority of these mutant receptor constructs (24 in total) had essentially wild-type ligand binding and intracellular signaling characteristics, indicating that these residues are not critical for normal receptor function. However, four aromatic residues Phe189, Trp206, Phe209, and Tyr218 are important for agonist binding and receptor activation and are highly conserved throughout the neurohypophysial hormone subfamily of peptide-GPCRs. Located in the middle of ECL2, juxtaposed to the highly conserved disulfide bond, Trp206 and Phe209 project into the binding crevice. Indeed, Phe209 is part of the Cys-X-X-X-Ar (where Ar is an aromatic residue) motif, which is well conserved in both peptide-GPCRs and amine- GPCRs. In contrast, Phe189 and Tyr218, located at the extreme ends of ECL2, may be important for determining the position of the ECL2 cap over the binding crevice. This study provides mechanistic insight into the roles of highly conserved ECL2 residues. [ABSTRACT FROM AUTHOR]

Published
2007
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39. Pharmacological Chaperone Activity of SR49059 to Functionally Recover Misfolded Mutations of the Vasopressin Via Receptor.

Author

Hawtin, Stuart R.

Subjects
*VASOPRESSIN, *ENZYME-linked immunosorbent assay, *GENETIC mutation, *HORMONE receptors, *G proteins, *LIGANDS (Biochemistry), *DISEASES
Abstract

Pharmacological chaperones represent a new class of ligand with the potential to facilitate the delivery of misfolded, but still active, G-protein-coupled receptors to the cell surface. Using transfected HEK 293T cells, treatment with a nonpeptide antagonist, SR49059, dramatically increased (∼60-fold) the surface expression of a misfolded, nonfunctional and intracellularly localized vasopressin V1a receptor (V1aR) mutant (D148A). This rescue of surface expression (111 ± 7%) was almost identical to wild type assessed by confocal microscopy and quantitative enzyme-linked immunosorbent assay-based techniques. Recovery was not specific to D148A, since other surface-impaired mutations, D148N and D148E, and wild type were also increased following SR49059 exposure. However, surface delivery was specific to SR49059, since V1aR-selective peptide ligands or unrelated ligands were unable to mimic this action, suggesting that SR49059 acts intracellularly. SR49059-mediated surface rescue was time-, mutant-, and concentration-dependent but not directly related to its binding affinity. Maximal recovery was achieved following 12 h of treatment and did not involve de novo receptor synthesis or a consequence of preventing endogenous constitutive activity and/or internalization. Once at the surface, all mutants displayed enhanced signaling ability, and D148A was able to undergo agonist-mediated internalization. SR49059 was not effectively removed from the receptor, since signaling (EC50) of both wild type and D148A was reduced ∼40-fold. This is the first report of a pharmacological chaperone ligand to act on misfolded mutant V1aRs. This work provides an excellent model to understand the mechanistic action of an important new class of drug that may have potential in the treatment of diseases caused by inherited mutations. [ABSTRACT FROM AUTHOR]

Published
2006
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40. A Gly/Ala switch contributes to high affinity binding of benzoxazinone-based non-peptide oxytocin receptor antagonists

Author

Hawtin, Stuart R., Ha, Sookhee N., Pettibone, Douglas J., and Wheatley, Mark

Subjects
*PEPTIDES, *OXYTOCIN, *PHARMACOLOGY, *VASOPRESSIN
Abstract

Abstract: Non-peptide antagonists of the oxytocin receptor (OTR) have been developed to prevent pre-term labour. The benzoxazinone-based antagonists L-371,257 and L-372,662 display pronounced species-dependent pharmacology with respect to selectivity for the OTR over the V1a vasopressin receptor. Examination of receptor sequences from different species identified Ala318 in helix 7 of the human OTR as a candidate discriminator required for high affinity binding. The mutant receptor [A318G]OTR was engineered and characterised using ligands representing many different chemical classes. Of all the ligands investigated, only the benzoxazinone-based antagonists had decreased affinity for [A318G]OTR. Molecular modelling revealed that Ala318 provides a direct hydrophobic contact with a methoxy group of L-371,257 and L-372,662. [Copyright &y& Elsevier]

Published
2005
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41. An arginyl in the N-terminus of the V1a vasopressin receptor is part of the conformational switch controlling activation by agonist.

Author

Hawtin, Stuart R., Wesley, Victoria J., Simms, John, Parslow, Rosemary A., Miles, Alice, McEwan, Kim, Keen, Mary, and Wheatley, Mark

Subjects
*PROTEINS, *VASOPRESSIN, *HORMONE receptors, *LIGAND binding (Biochemistry), *PEPTIDE hormones, *BIOCHEMISTRY
Abstract

Defining how the agonist–receptor interaction differs from that of the antagonist–receptor and understanding the mechanisms of receptor activation are fundamental issues in cell signalling. The V1a vasopressin receptor (V1aR) is a member of a family of related G-protein coupled receptors that are activated by neurohypophysial peptide hormones, including vasopressin (AVP). It has recently been reported that an arginyl in the distal N-terminus of the V1aR is critical for binding agonists but not antagonists. To determine specific features required at this locus to support high affinity agonist binding and second messenger generation, Arg46 was substituted by all other 19 encoded amino acids. Our data establish that there is an absolute requirement for arginyl, as none of the [R46X]V1aR mutant constructs supported high affinity agonist binding and all 19 had defective signalling. In contrast, all of the mutant receptors possessed wildtype binding for both peptide and nonpeptide antagonists. The ratio of Ki to EC50, an indicator of efficacy, was increased for all substitutions. Consequently, although [R46X]V1aR constructs have a lower affinity for agonist, once AVP has bound all 19 are more likely than the wildtype V1aR to become activated. Therefore, in the wildtype V1aR, Arg46 constrains the inactive conformation of the receptor. On binding AVP this constraint is alleviated, promoting the transition to active V1aR. Our findings explain why arginyl is conserved at this locus throughout the evolutionary lineage of the neurohypophysial peptide hormone receptor family of G-protein coupled receptors. [ABSTRACT FROM AUTHOR]

Published
2003
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42. Critical Role of a Subdomain of the N-Terminus of the V[sub 1a] Vasopressin Receptor for Binding....

Author

Hawtin, Stuart R. and Wesley, Victoria J.

Subjects
*VASOPRESSIN, *OXYTOCIN, *CHEMICAL agonists, *HORMONE receptors
Abstract

Examines the role of V[sub 1a] vasopressin receptor N-terminus subdomain for binding agonists. Comparison of the pharmacological profile between oxytocin and vasopressin receptor; Importance of subdomain in receptor activation and second messenger generation; Differences between agonist and antagonist interaction with peptide receptors.

Published
2000
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43. Palmitoylation of the Vasopressin V1aReceptor Reveals Different Conformational Requirements for Signaling, Agonist-induced Receptor Phosphorylation, and Sequestration*

Author

Hawtin, Stuart R., Tobin, Andrew B., Patel, Smita, and Wheatley, Mark

Abstract

In this study, we establish that the V1avasopressin receptor (V1aR) is palmitoylated, and we show that this modification has an important functional role. Palmitoylation of the V1aR occurs within the Cys371/Cys372couplet located in the proximal C-terminal tail domain. Substitution of these residues in a [C371G/C372G]V1aR construct effectively disrupted receptor palmitoylation. Our data also indicate an additional palmitoylation site at another locus in the receptor, as yet undefined. [3H]Palmitate incorporation was agonist-sensitive and increased following exposure to [Arg8]vasopressin (AVP). Given the hydrophobic nature of the acyl chain, palmitoylation of the C terminus of G-protein-coupled receptors has been proposed to form an additional intracellular loop. Consequently, palmitoylation/depalmitoylation will have a profound effect on the local conformation of this domain. The V1aR palmitoylation status regulated both phosphorylation and sequestration of the receptor, and furthermore, palmitoylation, phosphorylation, and sequestration were all regulated by AVP. The palmitoylation-defective construct [C371G/C372G]V1aR exhibited decreased phosphorylation compared to wild-type V1aR, under both basal and AVP-stimulated conditions, and was sequestered at a faster rate. In contrast, the binding of four different classes of ligand and intracellular signaling were not affected by palmitoylation. This study therefore establishes that there are different conformational requirements for signaling, agonist-induced phosphorylation, and sequestration of the V1aR.

Published
2001
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