1. Inhibition of RNA polymerase I transcription activates targeted DNA damage response and enhances the efficacy of PARP inhibitors in high-grade serous ovarian cancer.
- Author
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Sanij, E, Hannan, K, Xuan, J, Yan, S, Ahern, JA, Trigos, AS, Brajanovski, N, Son, J, Chan, KT, Kondrashova, O, Lieschke, E, Wakefield, MJ, Ellis, S, Cullinane, C, Poortinga, G, Khanna, KK, Mileshkin, L, McArthur, GA, Soong, J, Berns, EM, Hannan, RD, Scott, CL, Sheppard, KE, Pearson, RB, Sanij, E, Hannan, K, Xuan, J, Yan, S, Ahern, JA, Trigos, AS, Brajanovski, N, Son, J, Chan, KT, Kondrashova, O, Lieschke, E, Wakefield, MJ, Ellis, S, Cullinane, C, Poortinga, G, Khanna, KK, Mileshkin, L, McArthur, GA, Soong, J, Berns, EM, Hannan, RD, Scott, CL, Sheppard, KE, and Pearson, RB
- Abstract
Introduction: PARP inhibitors (PARPi) have revolutionized disease management of patients with homologous recombination (HR) DNA repair-deficient high-grade serous ovarian cancer (HGSOC). However, acquired resistance to PARPi is a major challenge in the clinic. The specific inhibitor of RNA polymerase I (Pol I) transcription of ribosomal RNA genes (rDNA) has demonstrated single-agent antitumor activity in p53 wild-type and p53-mutant hematologic malignancies (first-in-human trial, dose escalation study of CX-5461 at Peter MacCallum Cancer Centre) (Khot et al., Cancer Discov 2019). CX-5461 has also been reported to exhibit synthetic lethality with BRCA1/2 deficiency through stabilization of G-quadruplex DNA (GQ) structures. Here, we investigate the efficacy of CX-5461 in treating HGSOC. Experimental Design: The mechanisms by which CX-5461 induces DNA damage response (DDR) and displays synthetic lethality in HR-deficient HGSOC cells are explored. We present in vivo data of mice bearing two functionally and genomically profiled HGSOC-patient-derived xenograft (PDX)s treated with CX-5461 and olaparib, alone and in combination. We also investigate CX-5461-sensitivity gene expression signatures in primary and relapsed HGSOC. Results: Utilizing ovarian cancer cell lines, we demonstrate that sensitivity to CX-5461 is associated with “BRCA1 mutation” and “MYC targets” gene expression signatures. In addition, sensitivity to CX-5461 is associated with high basal rates of Pol I transcription. Importantly, we demonstrate a novel mechanism for CX-5461 synthetic lethal interaction with HR deficiency mediated through the induction of replication stress at rDNA repeats. Our data reveal CX-5461-mediated DDR in HR-deficient cells does not involve stabilization of GQ structures as previously proposed. On the contrary, we show definitively that CX-5461 inhibits Pol I recruitment leading to rDNA chromatin defects including stabilization of R-loops, single-stranded DNA, and replic
- Published
- 2020