Abstract

HSP90 and GRP94 are homologous cellular chaperones found in cytosol and endoplasmic reticulum, respectively. Several years ago, we discovered that members of the benzoquinone and ansamycin class of antibiotic, including herbimycin A and geldanamycin (GA) bound to HSP90 and GRP94 and disrupted certain multi-molecular complexes of which these proteins were a part. We have utilized pharmacologic disruption of HSP90 and GRP94 activity to study the function of these chaperones in cellular signal transduction. Multiple signal transduction proteins interact with these charperones, including the kinasesz src, erbB2 and c-raf-1, and mutated (but not wild type) p53. A general consequence of pharmacologic disruption of the chaperone/signal protein complex is the resultant marked instability and incorrect subcellular localization of the signalling protein. The instability is due to stimulation of targeted degradation of the signalling protein by the 26S proteasome proteolytic complex following chaperone dissociation. With respect to c-raf-1, no other members of the MAP kinase signalling pathway appear to be affected by GA. With respect to erbB2, it appears to be the most sensitive member of the EGF receptor family of tyrosine kinases to this drug. In the case of mutated p53, attainment of the mutated (but not wild type) conformation of the protein requires transient interaction with HSP90 and an accessory protein termed p23. GA treatment destroys the conformation and the function of mutated p53, providing evidence that pharmacologic manipulation of protein conformation is feasible. In collaboration with Pfizer Central Research, we have tested more than 35 benzoquinone ansamycin derivatives for their ability to bind HSP90/GRP94 and to affect the stability and function of mutant p53, c-raf-l and erbB2. Benzoquinone ansamycins are currently the only agents capable of specifically interfering in HSP90/GRP94 function and these drugs will be useful agents in further studying the role of these chaperones proteins in regulating the stability and function of oncogenes and other signalling proteins.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Intramural Research (Z01)
Project #
1Z01SC010074-01
Application #
2464563
Study Section
Special Emphasis Panel (CPB)
Project Start
Project End
Budget Start
Budget End
Support Year
1
Fiscal Year
1996
Total Cost
Indirect Cost

  Institution

Name
National Cancer Institute Division of Clinical Sciences
Department
Type
DUNS #
City
State
Country
United States
Zip Code

  Publications

Bachman, Ashleigh B; Keramisanou, Dimitra; Xu, Wanping et al. (2018) Phosphorylation induced cochaperone unfolding promotes kinase recruitment and client class-specific Hsp90 phosphorylation. Nat Commun 9:265
Yim, Kendrick H; Prince, Thomas L; Qu, Shiwei et al. (2016) Gambogic acid identifies an isoform-specific druggable pocket in the middle domain of Hsp90?. Proc Natl Acad Sci U S A 113:E4801-9
Calderwood, Stuart K; Neckers, Len (2016) Hsp90 in Cancer: Transcriptional Roles in the Nucleus. Adv Cancer Res 129:89-106
Prince, Thomas L; Kijima, Toshiki; Tatokoro, Manabu et al. (2015) Client Proteins and Small Molecule Inhibitors Display Distinct Binding Preferences for Constitutive and Stress-Induced HSP90 Isoforms and Their Conformationally Restricted Mutants. PLoS One 10:e0141786
Sourbier, Carole; Scroggins, Bradley T; Ratnayake, Ranjala et al. (2013) Englerin A stimulates PKC? to inhibit insulin signaling and to simultaneously activate HSF1: pharmacologically induced synthetic lethality. Cancer Cell 23:228-37
Alarcon, S V; Mollapour, M; Lee, M-J et al. (2012) Tumor-intrinsic and tumor-extrinsic factors impacting hsp90- targeted therapy. Curr Mol Med 12:1125-41
Xu, Wanping; Neckers, Len (2012) The double edge of the HSP90-CDC37 chaperone machinery: opposing determinants of kinase stability and activity. Future Oncol 8:939-42
Mollapour, Mehdi; Neckers, Len (2012) Post-translational modifications of Hsp90 and their contributions to chaperone regulation. Biochim Biophys Acta 1823:648-55
Mollapour, Mehdi; Tsutsumi, Shinji; Truman, Andrew W et al. (2011) Threonine 22 phosphorylation attenuates Hsp90 interaction with cochaperones and affects its chaperone activity. Mol Cell 41:672-81
Wang, Suiquan; Pashtan, Itai; Tsutsumi, Shinji et al. (2009) Cancer cells harboring MET gene amplification activate alternative signaling pathways to escape MET inhibition but remain sensitive to Hsp90 inhibitors. Cell Cycle 8:2050-6

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