Abstract

Data from seminal studies on the functional roles of polyoma gene products along with recent results from cancer genomics have converged to highlight the multimeric enzyme protein phosphatase PP2A as an important tumor suppressor which is frequently mutated in a variety of human cancers. The overriding objective of the Functional Proteomics Core (FPC) is to provide state-of-the-art proteomic approaches for tandem affinity purification followed by mass spectrometry (TAP-MS) as well as quantitative proteomic/phosphoproteomic technologies. Data from these studies will advance our understanding of how ST/MT alter PP2A protein associations, as well as host cell signaling networks and protein expression profiles, ultimately contributing to cellular transformation and human cancers. The FPC will serve as a technical and intellectual resource where researchers within all Projects can collaborate, compare, and interpret their proteomic data within the context of human cancer. We will work collaboratively with Program members through two specific aims:
Aim 1. Utilize tandem affinity purification followed by mass spectrometry (TAP-MS) to characterize ST/MT-mediated alterations in PP2A protein complexes. We will utilize our proven platform for TAP-MS platform to: (Project 2) quantify the dynamics of YAP-PP2A complexes as a function of ST or MT expression; (Project 3) compare protein binding partners of PP2A A? and PP2A A?; (Project 4) quantify changes in the assembly of PP2A-STRIPAK multi-component protein complexes as a function of ST expression.
Aim 2. Utilize quantitative mass spectrometry to interrogate alterations in protein expression and PP2A-associated signaling cascades resulting from expression of ST/MT gene products. We will use our DEEP SEQ quantitative mass spectrometry platform to: (Project 1) identify signaling pathways influenced by expression of Merkel ST and determine whether these oppose or work synergistically with mTOR in the context of cellular proliferation and oncogenic transformation; (Project 2) quantify changes in PP2A signaling that result from ST/MT-mediated changes in YAP protein complexes; (Project 3) quantify perturbations in phosphorylation that result from ST/MT targeting of PP2A-A?; (Project 4) identify changes in phosphorylation sites associated with expression of SV40 ST or depletion of specific PP2A subunits. In addition we will work with Project 1 to interrogate alterations in protein expression resulting from MCPyV ST. These data will be integrated with the DeCaprio Lab?s RNA-seq results to prioritize metabolic regulators for further study. In addition our DEEP SEQ proteomic data may reveal transcription-independent mechanisms by which MCPyV ST commandeers cellular pathways.

Public Health Relevance

The Functional Proteomics Core (FPC) will provide state-of-the-art mass spectrometry-based assays to quantify disruptions in host cell PP2A protein complexes, signaling cascades, and protein expression resulting from expression of polyoma small-T (ST) or middle-T (MT) antigens. Given the difficulty of characterizing tumor suppressors in general, and the protein phosphatase PP2A in particular, ST/MT will serve as effective probes to interrogate the function of this important tumor suppressor. These data may reveal important mechanisms by which the repertoire of PP2A mutations revealed through recent cancer genomics studies lead to transformation.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Program Projects (P01)
Project #
1P01CA203655-01A1
Application #
9358183
Study Section
Special Emphasis Panel (ZCA1)
Project Start
Project End
Budget Start
2017-08-01
Budget End
2018-07-31
Support Year
1
Fiscal Year
2017
Total Cost
Indirect Cost

  Institution

Name
Dana-Farber Cancer Institute
Department
Type
DUNS #
076580745
City
Boston
State
MA
Country
United States
Zip Code
02215

  Publications

Tarnita, Roxana M; Wilkie, Adrian R; DeCaprio, James A (2018) Contribution of DNA replication to the FAM111A-mediated simian virus 40 host range phenotype. J Virol :
Becker, Jürgen C; Stang, Andreas; DeCaprio, James A et al. (2017) Merkel cell carcinoma. Nat Rev Dis Primers 3:17077
Zhang, Jing; Gao, Xueliang; Schmit, Fabienne et al. (2017) CRKL Mediates p110?-Dependent PI3K Signaling in PTEN-Deficient Cancer Cells. Cell Rep 20:549-557
Cheng, Jingwei; Park, Donglim Esther; Berrios, Christian et al. (2017) Merkel cell polyomavirus recruits MYCL to the EP400 complex to promote oncogenesis. PLoS Pathog 13:e1006668
Kang, Un-Beom; Alexander, William M; Marto, Jarrod A (2017) Interrogating the hidden phosphoproteome. Proteomics 17:
Ni, Jing; Xie, Shaozhen; Ramkissoon, Shakti H et al. (2017) Tyrosine receptor kinase B is a drug target in astrocytomas. Neuro Oncol 19:22-30
Tsherniak, Aviad; Vazquez, Francisca; Montgomery, Phil G et al. (2017) Defining a Cancer Dependency Map. Cell 170:564-576.e16
Hsu, Jessie Hao-Ru; Hubbell-Engler, Benjamin; Adelmant, Guillaume et al. (2017) PRMT1-Mediated Translation Regulation Is a Crucial Vulnerability of Cancer. Cancer Res 77:4613-4625
Rouleau, Cecile; Pores Fernando, Arun T; Hwang, Justin H et al. (2016) Transformation by Polyomavirus Middle T Antigen Involves a Unique Bimodal Interaction with the Hippo Effector YAP. J Virol 90:7032-7045
Odajima, Junko; Saini, Siddharth; Jung, Piotr et al. (2016) Proteomic Landscape of Tissue-Specific Cyclin E Functions in Vivo. PLoS Genet 12:e1006429