A fluorescence‐based sensor for calibrated measurement of protein kinase stability in live cells

Author:

Paul Joseph W.12ORCID,Muratcioğlu Serena3,Kuriyan John34ORCID

Affiliation:

1. Department of Molecular and Cell Biology University of California Berkeley California USA

2. California Institute for Quantitative Bioscience (QB3) University of California Berkeley California USA

3. Department of Biochemistry Vanderbilt University School of Medicine Nashville Tennessee USA

4. Department of Chemistry Vanderbilt University Nashville Tennessee USA

Abstract

AbstractOncogenic mutations can destabilize signaling proteins, resulting in increased or unregulated activity. Thus, there is considerable interest in mapping the relationship between mutations and the stability of signaling proteins, to better understand the consequences of oncogenic mutations and potentially inform the development of new therapeutics. Here, we develop a tool to study protein‐kinase stability in live mammalian cells and the effects of the HSP90 chaperone system on the stability of these kinases. We determine the expression levels of protein kinases by monitoring the fluorescence of fluorescent proteins fused to those kinases, normalized to that of co‐expressed reference fluorescent proteins. We used this tool to study the dependence of Src‐ and Raf‐family kinases on the HSP90 system. We demonstrate that this sensor reports on destabilization induced by oncogenic mutations in these kinases. We also show that Src‐homology 2 and Src‐homology 3 domains, which are required for autoinhibition of Src‐family kinases, stabilize these kinase domains in the cell. Our expression‐calibrated sensor enables the facile characterization of the effects of mutations and small‐molecule drugs on protein‐kinase stability.

Funder

National Institutes of Health

National Institute of Allergy and Infectious Diseases

Howard Hughes Medical Institute

School of Medicine, Vanderbilt University

National Science Foundation

Publisher

Wiley

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