| Literature DB >> 25278616 |
Mikhail M Savitski1, Friedrich B M Reinhard2, Holger Franken2, Thilo Werner2, Maria Fälth Savitski2, Dirk Eberhard2, Daniel Martinez Molina3, Rozbeh Jafari3, Rebecca Bakszt Dovega3, Susan Klaeger4, Bernhard Kuster4, Pär Nordlund5, Marcus Bantscheff1, Gerard Drewes1.
Abstract
The thermal stability of proteins can be used to assess ligand binding in living cells. We have generalized this concept by determining the thermal profiles of more than 7000 proteins in human cells by means of mass spectrometry. Monitoring the effects of small-molecule ligands on the profiles delineated more than 50 targets for the kinase inhibitor staurosporine. We identified the heme biosynthesis enzyme ferrochelatase as a target of kinase inhibitors and suggest that its inhibition causes the phototoxicity observed with vemurafenib and alectinib. Thermal shifts were also observed for downstream effectors of drug treatment. In live cells, dasatinib induced shifts in BCR-ABL pathway proteins, including CRK/CRKL. Thermal proteome profiling provides an unbiased measure of drug-target engagement and facilitates identification of markers for drug efficacy and toxicity.Entities:
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Year: 2014 PMID: 25278616 DOI: 10.1126/science.1255784
Source DB: PubMed Journal: Science ISSN: 0036-8075 Impact factor: 47.728