Literature DB >> 19196702

High-throughput screening for small-molecule inhibitors of LARG-stimulated RhoA nucleotide binding via a novel fluorescence polarization assay.

Chris R Evelyn1, Timothy Ferng, Rafael J Rojas, Martha J Larsen, John Sondek, Richard R Neubig.   

Abstract

Guanine nucleotide exchange factors (GEFs) stimulate guanine nucleotide exchange and the subsequent activation of Rho-family proteins in response to extracellular stimuli acting upon cytokine, tyrosine kinase, adhesion, integrin, and G-protein-coupled receptors (GPCRs). Upon Rho activation, several downstream events occur, such as morphological and cytoskeletal changes, motility, growth, survival, and gene transcription. The leukemia-associated RhoGEF (LARG) is a member of the regulators of G-protein signaling homology domain (RH) family of GEFs originally identified as a result of chromosomal translocation in acute myeloid leukemia. Using a novel fluorescence polarization guanine nucleotide-binding assay using BODIPY-Texas Red-GTPgammaS (BODIPY-TR-GTPgammaS), the authors performed a 10,000-compound high-throughput screen for inhibitors of LARG-stimulated RhoA nucleotide binding. Five compounds identified from the high-throughput screen were confirmed in a nonfluorescent radioactive guanine nucleotide-binding assay measuring LARG-stimulated [( 35)S] GTPgammaS binding to RhoA, thus ruling out nonspecific fluorescent effects. All 5 compounds selectively inhibited LARG-stimulated RhoA [( 35)S] GTPgammaS binding but had little to no effect on RhoA or Galpha( o) [(35)S] GTPgammaS binding. Therefore, these 5 compounds should serve as promising starting points for the development of small-molecule inhibitors of LARG-mediated nucleotide exchange as both pharmacological tools and therapeutics. In addition, the fluorescence polarization guanine nucleotide-binding assay described here should serve as a useful approach for both high-throughput screening and general biological applications.

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Year:  2009        PMID: 19196702      PMCID: PMC2698131          DOI: 10.1177/1087057108328761

Source DB:  PubMed          Journal:  J Biomol Screen        ISSN: 1087-0571


  36 in total

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2.  Fluorescent BODIPY-GTP analogs: real-time measurement of nucleotide binding to G proteins.

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Review 3.  Fluorescence polarization and anisotropy in high throughput screening: perspectives and primer.

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4.  Structure of Galphaq-p63RhoGEF-RhoA complex reveals a pathway for the activation of RhoA by GPCRs.

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5.  Leukemia-associated Rho guanine nucleotide exchange factor, a Dbl family protein found mutated in leukemia, causes transformation by activation of RhoA.

Authors:  G W Reuther; Q T Lambert; M A Booden; K Wennerberg; B Becknell; G Marcucci; J Sondek; M A Caligiuri; C J Der
Journal:  J Biol Chem       Date:  2001-05-23       Impact factor: 5.157

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  21 in total

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2.  A conserved hydrophobic surface of the LARG pleckstrin homology domain is critical for RhoA activation in cells.

Authors:  Mohamed Aittaleb; Guang Gao; Chris R Evelyn; Richard R Neubig; John J G Tesmer
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4.  Combined rational design and a high throughput screening platform for identifying chemical inhibitors of a Ras-activating enzyme.

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6.  Identification of influenza endonuclease inhibitors using a novel fluorescence polarization assay.

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Review 7.  Ras superfamily GEFs and GAPs: validated and tractable targets for cancer therapy?

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Review 10.  Druggable targets in the Rho pathway and their promise for therapeutic control of blood pressure.

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