Materials Map

Discover the materials research landscape. Find experts, partners, networks.

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The Materials Map is an open tool for improving networking and interdisciplinary exchange within materials research. It enables cross-database search for cooperation and network partners and discovering of the research landscape.

The dashboard provides detailed information about the selected scientist, e.g. publications. The dashboard can be filtered and shows the relationship to co-authors in different diagrams. In addition, a link is provided to find contact information.

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The Materials Map is still under development. In its current state, it is only based on one single data source and, thus, incomplete and contains duplicates. We are working on incorporating new open data sources like ORCID to improve the quality and the timeliness of our data. We will update Materials Map as soon as possible and kindly ask for your patience.

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University of Bristol

in Cooperation with on an Cooperation-Score of 37%

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Publications (4/4 displayed)

  • 2020A Multipronged Screening Approach Targeting Inhibition of ETV6 PNT Domain Polymerization3citations
  • 2019343-LB: The Type 2 Diabetes-Associated Lipid Binding Protein STARD10 Controls Insulin Secretory Granule Biogenesiscitations
  • 2014Computational design of water-soluble α-helical barrels332citations
  • 2014Molecular dynamics simulations reveal a dielectric-responsive coronal structure in protein-polymer surfactant hybrid nanoconstructs43citations

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Zhang, Si Miao
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Balgi, Aruna D.
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Gerak, Chloe A. N.
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Roberge, Michel
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Sadowski, Ivan J.
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Leclerc, Isabelle
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Rutter, Guy A.
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Alpy, Fabien
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Co-Authors (by relevance)

  • Zhang, Si Miao
  • Balgi, Aruna D.
  • Gerak, Chloe A. N.
  • Mcintosh, Lawrence P.
  • Roberge, Michel
  • Sadowski, Ivan J.
  • Leclerc, Isabelle
  • Rutter, Guy A.
  • Alpy, Fabien
  • Kong, Alice P.
  • Cakebread, Andrew
  • Hodson, David
  • Distaso, Walter
  • Stylianides, Theodoros
  • Salem, Victoria
  • Pullen, Timothy J.
  • Georgiadou, Eleni
  • Tomas, Alejandra
  • Piunti, Alexandra
  • Haataja, Leena
  • Arvan, Peter
  • Carrat, Gaelle
  • Haythorne, Elizabeth
  • Fung, Annie
  • Burton, Antony J.
  • Bartlett, Gail J.
  • Brady, R. Leo
  • Woolfson, Derek N.
  • Thomson, Andrew R.
  • Wood, Christopher
  • Brogan, Alex P. S.
  • Mann, Stephen
  • Perriman, Adam Willis
OrganizationsLocationPeople

article

A Multipronged Screening Approach Targeting Inhibition of ETV6 PNT Domain Polymerization

  • Zhang, Si Miao
  • Balgi, Aruna D.
  • Gerak, Chloe A. N.
  • Sessions, Richard B.
  • Mcintosh, Lawrence P.
  • Roberge, Michel
  • Sadowski, Ivan J.
Abstract

ETV6 is an ETS family transcriptional repressor for which head-to-tail polymerization of its PNT domain facilitates cooperative binding to DNA by its ETS domain. Chromosomal translocations frequently fuse the ETV6 PNT domain to one of several protein tyrosine kinases. The resulting chimeric oncoproteins undergo ligand-independent self-association, autophosphorylation, and aberrant stimulation of downstream signaling pathways, leading to a variety of cancers. Currently, no small-molecule inhibitors of ETV6 PNT domain polymerization are known and no assays targeting PNT domain polymerization have been described. In this study, we developed complementary experimental and computational approaches for identifying such inhibitory compounds. One mammalian cellular approach utilized a mutant PNT domain heterodimer system covalently attached to split Gaussia luciferase fragments. In this protein–fragment complementation assay, inhibition of PNT domain heterodimerization reduces luminescence. A yeast assay took advantage of activation of the reporter HIS3 gene upon heterodimerization of mutant PNT domains fused to DNA-binding and transactivation domains. In this two-hybrid screen, inhibition of PNT domain heterodimerization prevents cell growth in medium lacking histidine. The Bristol University Docking Engine (BUDE) was used to identify virtual ligands from the ZINC8 library predicted to bind the PNT domain polymerization interfaces. More than 75 hits from these three assays were tested by nuclear magnetic resonance spectroscopy for binding to the purified ETV6 PNT domain. Although none were found to bind, the lessons learned from this study may facilitate future approaches for developing therapeutics that act against ETV6 oncoproteins by disrupting PNT domain polymerization.

Topics
  • impedance spectroscopy
  • compound
  • activation
  • Nuclear Magnetic Resonance spectroscopy
  • luminescence