Abstract

Synthetic lethal approaches for `personalized' therapy of specific cancer subsets is a strategy that can attack the initial drivers of genetic instability, possibly eliminating tumor heterogeneity, as well as the emergence of resistant and metastatic cancer cells. We recently discovered that cancer cells that lost one allele of the RPRD1B/Kub5-Hera (K-H) gene, corresponding to ~50+% loss of protein, exhibit atypical elevations of PARP1 activities and a ?BRCAness? phenotype in BRCA-proficient cancer cells. We hypothesize that K-H binds to the C-terminal domain (CTD) of RNA polymerase II (RNAPII) to preferentially direct transcription of genes containing sequence-specific CHR-motif promoters, most importantly cyclin-dependent kinase 1 (CDK1). CDK1, in turn, stimulates BRCA1 phosphorylation and HR function. K-H loss in breast or nonsmall cell lung cancers (NSCLC), by copy number variation (CNV), mRNA expression or specific SNPs in patient tumors, results in a unique `cancer vulnerability of persistent R-loop formation and HR deficiency', whereby cells are dependent on PARP1- driven alternative non-homologous end joining (alt-NHEJ) repair. While this drives genetic instability due to elevated R-loops, a BRCA deficiency and a dependency on error-prone alt-NHEJ, the `vulnerability in genetic instability' can be exploited using PARP inhibitors (PARPis) that block redundant DSB repair and cause lethality during replication. We will complete two specific aims:
Aim 1 : To perform structure/function analyses using rationally-derived K-H mutation(s) and patient- derived tumor SNPs to delineate the mechanism by which aberrant K-H mutations alter PARP1 activity and CDK1 levels that, in turn, affect downstream BRCA1-HR function and cellular responses to PARP1is or IR. (Years 1-5).
Aim 2 : To optimize antitumor efficacy of breast or NSCLC cancer xenografts expressing mutant or loss of K-H protein expression using clinically-relevant PARPis or IR (Years 1-5). Completion of the proposed research will define the mechanism by which K-H directs RNAPII-driven CHR motif-specific gene expression and CDK1-BRCA1 HR function. In turn, understanding this mechanism will allow exploitation of the consequences of K-H loss and optimization of synthetic lethal approaches using PARPis or IR for treatment of specific cancer subsets. The studies will also reveal additional, exploitable cancer vulnerabilities. Our studies are novel as they define how a RNA transcription termination factor can direct transcription and DNA repair, revealing exploitable cancer vulnerabilities that can be translated.

Public Health Relevance

When cancers originate from normal cells, they commit themselves to fundamental genetic instability processes that appear to be specific for each individual, possibly because of a lack of understanding of the initiation process. In their genesis, cancer cells inadvertently become vulnerable by committing themselves to specific survival pathways that when inhibited can lead to their death. When lost (even one allele that leads to loss of protein), the RPRD1B/Kub5-Hera (K-H) gene leads to a heightened carcinogenic state after stress (e.g., after exposure to low doses of ionizing radiation). By defining mechanisms of how cells that have lost K-H become genetically unstable, we have discovered their specific vulnerability ? a BRCAness phenotype wherein cells become hypersensitive to IR or inhibitors of poly(ADP-ribose) polymerase (PARPis). Completing the proposed research in this grant will reveal, for the first time, the mechanism by which an RNA transcriptional termination factor can regulate homologous recombination, and thereby be exploited (when lost in breast and nonsmall cell lung cancers/tumors) on an individual basis for synthetic lethal, tumor-selective therapy using PARPis or IR. Our studies will allow development of K-H gene and protein levels as a predictor of response.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA210489-04
Application #
9513472
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Buchsbaum, Jeffrey
Project Start
2016-07-05
Project End
2021-06-30
Budget Start
2018-07-01
Budget End
2019-06-30
Support Year
4
Fiscal Year
2018
Total Cost
Indirect Cost

  Institution

Name
Indiana University-Purdue University at Indianapolis
Department
Biochemistry
Type
Schools of Medicine
DUNS #
603007902
City
Indianapolis
State
IN
Country
United States
Zip Code
46202

  Publications

Motea, Edward A; Fattah, Farjana J; Xiao, Ling et al. (2018) Kub5-Hera RPRD1B Deficiency Promotes ""BRCAness"" and Vulnerability to PARP Inhibition in BRCA-proficient Breast Cancers. Clin Cancer Res :
Patidar, Praveen L; Motea, Edward A; Fattah, Farjana J et al. (2016) The Kub5-Hera/RPRD1B interactome: a novel role in preserving genetic stability by regulating DNA mismatch repair. Nucleic Acids Res 44:1718-31
Morales, Julio C; Richard, Patricia; Patidar, Praveen L et al. (2016) XRN2 Links Transcription Termination to DNA Damage and Replication Stress. PLoS Genet 12:e1006107
Kahanda, Dimithree; Chakrabarti, Gaurab; Mcwilliams, Marc A et al. (2016) Using DNA devices to track anticancer drug activity. Biosens Bioelectron 80:647-653
Norbury, John W; Schimmerling, Walter; Slaba, Tony C et al. (2016) Galactic cosmic ray simulation at the NASA Space Radiation Laboratory. Life Sci Space Res (Amst) 8:38-51