Literature DB >> 24041654

Reversible inhibitors of regulators of G-protein signaling identified in a high-throughput cell-based calcium signaling assay.

Andrew J Storaska1, Jian P Mei, Meng Wu, Min Li, Susan M Wade, Levi L Blazer, Benita Sjögren, Corey R Hopkins, Craig W Lindsley, Zhihong Lin, Joseph J Babcock, Owen B McManus, Richard R Neubig.   

Abstract

Regulator of G-protein signaling (RGS) proteins potently suppress G-protein coupled receptor (GPCR) signal transduction by accelerating GTP hydrolysis on activated heterotrimeric G-protein α subunits. RGS4 is enriched in the CNS and is proposed as a therapeutic target for treatment of neuropathological states including epilepsy and Parkinson's disease. Therefore, identification of novel RGS4 inhibitors is of interest. An HEK293-FlpIn cell-line stably expressing M3-muscarinic receptor with doxycycline-regulated RGS4 expression was employed to identify compounds that inhibit RGS4-mediated suppression of M3-muscarinic receptor signaling. Over 300,000 compounds were screened for an ability to enhance Gαq-mediated calcium signaling in the presence of RGS4. Compounds that modulated the calcium response in a counter-screen in the absence of RGS4 were not pursued. Of the 1365 RGS4-dependent primary screen hits, thirteen compounds directly target the RGS-G-protein interaction in purified systems. All thirteen compounds lose activity against an RGS4 mutant lacking cysteines, indicating that covalent modification of free thiol groups on RGS4 is a common mechanism. Four compounds produce >85% inhibition of RGS4-G-protein binding at 100μM, yet are >50% reversible within a ten-minute time frame. The four reversible compounds significantly alter the thermal melting temperature of RGS4, but not G-protein, indicating that inhibition is occurring through interaction with the RGS protein. The HEK cell-line employed for this study provides a powerful tool for efficiently identifying RGS-specific modulators within the context of a GPCR signaling pathway. As a result, several new reversible, cell-active RGS4 inhibitors have been identified for use in future biological studies.
© 2013.

Entities:  

Keywords:  BSA; DMSO; FCPIA; G-protein coupled receptors; GAP; GTPase accelerating protein; High-throughput screen; M(3) muscarinic acetylcholine receptor; MBP; PPI; RGS; Regulator of G-protein signaling; Small molecule inhibitor; T(m); bovine serum albumin; dimethyl sulfoxide; flow cytometry protein interaction assay; maltose binding protein; melting temperature; protein–protein interaction; regulator of G-protein signaling

Mesh:

Substances:

Year:  2013        PMID: 24041654      PMCID: PMC3848259          DOI: 10.1016/j.cellsig.2013.09.007

Source DB:  PubMed          Journal:  Cell Signal        ISSN: 0898-6568            Impact factor:   4.315


  52 in total

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2.  N-terminal residues control proteasomal degradation of RGS2, RGS4, and RGS5 in human embryonic kidney 293 cells.

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7.  Development of a bimolecular luminescence complementation assay for RGS: G protein interactions in cells.

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8.  Mixed-solvent molecular dynamics simulation-based discovery of a putative allosteric site on regulator of G protein signaling 4.

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10.  Evaluation of the Selectivity and Cysteine Dependence of Inhibitors across the Regulator of G Protein-Signaling Family.

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