STAT3 differential scanning fluorimetry and differential scanning light scattering assays: Addressing a missing link in the characterization of STAT3 inhibitor interactions

Matthieu Desroses; Sander Busker; Juan Astorga-Wells; Sanaz Attarha; Iryna Kolosenko; Roman A Zubarev; Thomas Helleday; Dan Grandér; Brent D G Page

doi:10.1016/j.jpba.2018.07.018

STAT3 differential scanning fluorimetry and differential scanning light scattering assays: Addressing a missing link in the characterization of STAT3 inhibitor interactions

J Pharm Biomed Anal. 2018 Oct 25:160:80-88. doi: 10.1016/j.jpba.2018.07.018. Epub 2018 Jul 17.

Authors

Matthieu Desroses¹, Sander Busker², Juan Astorga-Wells³, Sanaz Attarha¹, Iryna Kolosenko², Roman A Zubarev³, Thomas Helleday¹, Dan Grandér², Brent D G Page⁴

Affiliations

¹ Karolinska Institute, Science for Life Laboratory, Department of Oncology and Pathology, 171 21, Stockholm, Sweden.
² Karolinska Institute, Department of Oncology-Pathology, Cancer Center Karolinska, R8:03, 171 76, Stockholm, Sweden.
³ Karolinska Institute, Medical Biochemistry and Biophysics, 171 65, Stockholm, Sweden.
⁴ Karolinska Institute, Science for Life Laboratory, Department of Oncology and Pathology, 171 21, Stockholm, Sweden. Electronic address: brent.page@scilifelab.se.

PMID: 30086509
DOI: 10.1016/j.jpba.2018.07.018

Abstract

STAT3 protein is an established target for the development of new cancer therapeutic agents. Despite lacking a traditional binding site for small molecule inhibitors, many STAT3 inhibitors have been identified and explored for their anti-cancer activity. Because STAT3 signaling is mediated by protein-protein interactions, indirect methods are often employed to determine if proposed STAT3 inhibitors bind to STAT3 protein. While established STAT3 inhibition assays (such as the fluorescence polarization assay, electrophoretic mobility shift assay and ELISAs) have been used to identify novel inhibitors of STAT3 signaling, methods that directly assess STAT3 protein-inhibitor interactions could facilitate the development of novel inhibitors. In this context, we herein report new STAT3 binding assays based on differential scanning fluorimetry (DSF) and differential scanning light scattering (DSLS) to characterize interactions between STAT3 protein and inhibitors. Several peptide and small molecule STAT3 inhibitors have been evaluated, and new insight into how these compounds may interact with STAT3 is provided.

Keywords: Differential scanning fluorimetry; Differential scanning light scattering; Protein truncations; STAT3; Thermal stability assays.

MeSH terms

Binding Sites
Cyclic S-Oxides / chemistry
Cyclic S-Oxides / pharmacology
Drug Development / methods*
Fluorometry / methods*
High-Throughput Screening Assays / methods
Light
Peptides / chemistry
Peptides / pharmacology*
Protein Binding
Protein Domains
Protein Stability
Recombinant Proteins / chemistry
Recombinant Proteins / isolation & purification
STAT3 Transcription Factor / antagonists & inhibitors*
STAT3 Transcription Factor / chemistry
STAT3 Transcription Factor / isolation & purification
Scattering, Radiation
Temperature

Substances

Cyclic S-Oxides
Peptides
Recombinant Proteins
STAT3 Transcription Factor
stattic