RNAi Screening Uncovers a Synthetic Sick Interaction between CtIP and the BARD1 Tumor Suppressor.
Hella A BolckSara PrzetockaRoger MeierChristine von AeschChristina ZurfluhKay HänggiVincent SpeggMatthias AltmeyerMichael SteblerSimon Flyvbjerg NørrelykkePeter HorvathAlessandro A SartoriAntonio PorroPublished in: Cells (2022)
Human CtIP is best known for its role in DNA end resection to initiate DNA double-strand break repair by homologous recombination. Recently, CtIP has also been shown to protect reversed replication forks from nucleolytic degradation upon DNA replication stress. However, still little is known about the DNA damage response (DDR) networks that preserve genome integrity and sustain cell survival in the context of CtIP insufficiency. Here, to reveal such potential buffering relationships, we screened a DDR siRNA library in CtIP-deficient cells to identify candidate genes that induce synthetic sickness/lethality (SSL). Our analyses unveil a negative genetic interaction between CtIP and BARD1, the heterodimeric binding partner of BRCA1. We found that simultaneous disruption of CtIP and BARD1 triggers enhanced apoptosis due to persistent replication stress-induced DNA lesions giving rise to chromosomal abnormalities. Moreover, we observed that the genetic interaction between CtIP and BARD1 occurs independently of the BRCA1-BARD1 complex formation and might be, therefore, therapeutical relevant for the treatment of BRCA-defective tumors.
Keyphrases
- stress induced
- dna damage response
- circulating tumor
- genome wide
- cell cycle arrest
- cell free
- dna repair
- single molecule
- induced apoptosis
- dna damage
- oxidative stress
- copy number
- endoplasmic reticulum stress
- risk assessment
- dna methylation
- drug delivery
- single cell
- combination therapy
- circulating tumor cells
- signaling pathway
- pi k akt
- human health
- pluripotent stem cells