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RB loss sensitizes cells to replication-associated DNA damage after PARP inhibition by trapping

  • Luis Gregory Zamalloa
  • , Margaret M. Pruitt
  • , Nicole M. Hermance
  • , Himabindu Gali
  • , Rachel L. Flynn
  • , Amity L. Manning

Producción científica: Artículo CientíficoArtículo originalrevisión exhaustiva

7 Citas (Scopus)

Resumen

The retinoblastoma tumor suppressor protein (RB) interacts physically and functionally with a number of epigenetic modifying enzymes to control transcriptional regulation, respond to replication stress, promote DNA damage response and repair, and regulate genome stability. To better understand how disruption of RB function impacts epigenetic regulation of genome stability and determine whether such changes represent exploitable weaknesses of RB-deficient cancer cells, we performed an imaging-based screen to identify epigenetic inhibitors that promote DNA damage and compromise the viability of RB-deficient cells. We found that loss of RB alone leads to high levels of replication-dependent poly-ADP ribosylation (PARylation) and that preventing PARylation by trapping PARP enzymes on chromatin enables RB-deficient cells to progress to mitosis with unresolved replication stress. These defects contribute to high levels of DNA damage and compromised cell viability. We demonstrate this sensitivity is conserved across a panel of drugs that target both PARP1 and PARP2 and can be suppressed by reexpression of the RB protein. Together, these data indicate that drugs that target PARP1 and PARP2 may be clinically relevant for RB-deficient cancers.

Idioma originalInglés estadounidense
-e202302067
PublicaciónLife Science Alliance
Volumen6
N.º12
DOI
EstadoIndizado - dic. 2023
Publicado de forma externa

Nota bibliográfica

Publisher Copyright:
© 2023 Zamalloa et al.

ODS de las Naciones Unidas

Este resultado contribuye a los siguientes Objetivos de Desarrollo Sostenible

  1. ODS 3: Salud y bienestar
    ODS 3: Salud y bienestar

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