High-content, high-throughput analysis of cell cycle perturbations induced by the HSP90 inhibitor XL888

Susan K Lyman; Suzanne C Crawley; Ruoyu Gong; Joanne I Adamkewicz; Garth McGrath; Jason Y Chew; Jennifer Choi; Charles R Holst; Leanne H Goon; Scott A Detmer; Jana Vaclavikova; Mary E Gerritsen; Robert A Blake

doi:10.1371/journal.pone.0017692

High-content, high-throughput analysis of cell cycle perturbations induced by the HSP90 inhibitor XL888

PLoS One. 2011 Mar 7;6(3):e17692. doi: 10.1371/journal.pone.0017692.

Authors

Susan K Lyman¹, Suzanne C Crawley, Ruoyu Gong, Joanne I Adamkewicz, Garth McGrath, Jason Y Chew, Jennifer Choi, Charles R Holst, Leanne H Goon, Scott A Detmer, Jana Vaclavikova, Mary E Gerritsen, Robert A Blake

Affiliation

¹ Department of Molecular and Cellular Pharmacology, Exelixis, Inc., South San Francisco, California, United States of America. xl888.mail@gmail.com

Abstract

Background: Many proteins that are dysregulated or mutated in cancer cells rely on the molecular chaperone HSP90 for their proper folding and activity, which has led to considerable interest in HSP90 as a cancer drug target. The diverse array of HSP90 client proteins encompasses oncogenic drivers, cell cycle components, and a variety of regulatory factors, so inhibition of HSP90 perturbs multiple cellular processes, including mitogenic signaling and cell cycle control. Although many reports have investigated HSP90 inhibition in the context of the cell cycle, no large-scale studies have examined potential correlations between cell genotype and the cell cycle phenotypes of HSP90 inhibition.

Methodology/principal findings: To address this question, we developed a novel high-content, high-throughput cell cycle assay and profiled the effects of two distinct small molecule HSP90 inhibitors (XL888 and 17-AAG [17-allylamino-17-demethoxygeldanamycin]) in a large, genetically diverse panel of cancer cell lines. The cell cycle phenotypes of both inhibitors were strikingly similar and fell into three classes: accumulation in M-phase, G2-phase, or G1-phase. Accumulation in M-phase was the most prominent phenotype and notably, was also correlated with TP53 mutant status. We additionally observed unexpected complexity in the response of the cell cycle-associated client PLK1 to HSP90 inhibition, and we suggest that inhibitor-induced PLK1 depletion may contribute to the striking metaphase arrest phenotype seen in many of the M-arrested cell lines.

Conclusions/significance: Our analysis of the cell cycle phenotypes induced by HSP90 inhibition in 25 cancer cell lines revealed that the phenotypic response was highly dependent on cellular genotype as well as on the concentration of HSP90 inhibitor and the time of treatment. M-phase arrest correlated with the presence of TP53 mutations, while G2 or G1 arrest was more commonly seen in cells bearing wt TP53. We draw upon previous literature to suggest an integrated model that accounts for these varying observations.

MeSH terms

Azabicyclo Compounds / pharmacology*
Benzoquinones / pharmacology
Cell Cycle Proteins / metabolism
Cell Cycle* / drug effects
Cell Line
Flow Cytometry
HSP90 Heat-Shock Proteins / antagonists & inhibitors*
HSP90 Heat-Shock Proteins / metabolism
High-Throughput Screening Assays / methods*
Humans
Lactams, Macrocyclic / pharmacology
Phthalic Acids / pharmacology*
Polo-Like Kinase 1
Protein Serine-Threonine Kinases / metabolism
Proto-Oncogene Proteins / metabolism
Time Factors

Substances

Azabicyclo Compounds
Benzoquinones
Cell Cycle Proteins
HSP90 Heat-Shock Proteins
Lactams, Macrocyclic
Phthalic Acids
Proto-Oncogene Proteins
XL 888
tanespimycin
Protein Serine-Threonine Kinases