Abstract

We propose to develop and validate a technology that will enable unequivocal genome-wide functional identification of cancer-related genes using either a positive or negative selection in conditions of either low or high stringency. This will extend the reach of forward genetics to a principally new set of phenomena. Identification of the genes and their products, which form the molecular basis of cellular phenotypes, is the fundamental problem in molecular analysis of cancer. The cellular factors that control proliferation, death, response to therapy, motility, interaction with other cells and the environment have emerged as the diagnostic and prognostic markers, as well as the targets of therapeutic intervention. Forward genetics is a popular methodology that uses genetic tools to uncover the modulators of various biological processes. Insertional mutagenesis based on random insertion of a strong and regulated promoter is a versatile, cost-efficient, unbiased and comprehensive approach to forward genetics in somatic cells. However, the current implementations of this approach apply exclusively to the conditions of stringent positive selection, and are inapplicable to a wider range of clinically-significant phenomena. Moreover, large-scale mapping and validation of multiple relevant insertional targets remains the technical bottleneck of the whole approach. To overcome these limitations, we will develop a new technology, which combines the elements of insertional mutagenesis with those of microarray analysis. The microarray component will allow high-throughput mapping of the inserts in a highly complex pool of cells. Positive or negative changes in the representation of individual inserts could be used to identify the loci, which affect the cell behavior under various selective conditions. The dependence of the changes on the function of the inserted promoter could be used for large-scale validation of the findings. We will construct a series of appropriate lentiviral vectors and will confirm their activity as insertional mutagens. We will optimize the procedure to monitor the frequency of individual mutant alleles in a high-throughput format. Finally, we will apply the newly developed tools and procedures to the discovery of genes whose products determine the response of prostate carcinoma to Taxol, the only chemotherapeutic compound known to extend the life of patients with androgen-independent prostate cancer. We will identify the events that either sensitize or protect cells from the drug. The clinical significance of these findings will be pursued in future studies, while our data, tools and procedures will be shared with the research community.

Public Health Relevance

Development of diagnostic, prognostic and therapeutic strategies depend on our understanding of the molecular factors that determine various traits of the cancer cell. We propose a new genetic technology that could be used to discover such factors, including the ones that cannot be readily identified by other techniques. To test this approach, we will identify what determines the response of prostate cancer cells to Taxol, the drug that prolongs survival of the patients, but ultimately fails due to tumor resistance.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Exploratory/Developmental Grants (R21)
Project #
3R21CA137708-03S1
Application #
8322939
Study Section
Special Emphasis Panel (ZCA1-SRLB-Q (O1))
Program Officer
Ogunbiyi, Peter
Project Start
2009-07-01
Project End
2013-05-31
Budget Start
2011-08-01
Budget End
2013-05-31
Support Year
3
Fiscal Year
2011
Total Cost
$54,547
Indirect Cost

  Institution

Name
Roswell Park Cancer Institute Corp
Department
Type
DUNS #
824771034
City
Buffalo
State
NY
Country
United States
Zip Code
14263

  Publications

Babagana, Mahamat; Johnson, Sydney; Slabodkin, Hannah et al. (2017) P21-activated kinase 1 regulates resistance to BRAF inhibition in human cancer cells. Mol Carcinog 56:1515-1525
Zynda, Evan R; Matveev, Vitaliy; Makhanov, Michael et al. (2014) Protein kinase A type II-? regulatory subunit regulates the response of prostate cancer cells to taxane treatment. Cell Cycle 13:3292-301
Das Gupta, Jaydip; Luk, Ka-Cheung; Tang, Ning et al. (2012) Absence of XMRV and closely related viruses in primary prostate cancer tissues used to derive the XMRV-infected cell line 22Rv1. PLoS One 7:e36072
Yang, Jiawen; Battacharya, Partho; Singhal, Ruchi et al. (2011) Xenotropic murine leukemia virus-related virus (XMRV) in prostate cancer cells likely represents a laboratory artifact. Oncotarget 2:358-62
Singhal, Ruchi; Deng, Xiaotao; Chenchik, Alex A et al. (2011) Long-distance effects of insertional mutagenesis. PLoS One 6:e15832