Altered activation of the immune response causes radioresistance in HR-impaired breast cancer cells
OC-0263
Abstract
Altered activation of the immune response causes radioresistance in HR-impaired breast cancer cells
Authors: Sandra Classen1, Elena Rahlf1, Johannes Jungwirth2, Lena Poole1, Simon Gehre3, Michael Rückert3, Cordula Petersen4, Kai Rothkamm1, Udo Gaipl3, Helmut Pospiech2,5, Kerstin Borgmann1
1University Medical Center Hamburg-Eppendorf, Laboratory for Radiobiology and Experimental Radiooncology, Hamburg, Germany; 2Leibniz Institute on Aging - Fritz Lipmann Institute, Project group Biochemistry, Jena, Germany; 3Universitätsklinikum Erlangen, Translational Radiobiology, Department of Radiation Oncology, Erlangen, Germany; 4University Medical Center Hamburg-Eppendorf, Department of Radiotherapy and Radiation Oncology, Hamburg, Germany; 5University of Oulu, Faculty of Biochemistry and Molecular Medicine, Oulu, Finland
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Purpose or Objective
Turning immunologically cold tumors hot to sensitize
them to immune checkpoint inhibitors is a current clinical challenge. Defects
in DNA repair, especially in homologous recombination (HR), can trigger the intracellular
immune response by accumulation of cytosolic DNA due to an increase in the
number of DNA double strand breaks (DSBs). Thus, a combination of a HR-defect
and radiation, chemotherapeutics or DNA damage response inhibitors might
enhance the activation of the intracellular immune response, thereby maximizing
its anti-tumor activity. This project therefore aims to identify a new
combination of radio-chemotherapy in HR-impaired tumor cells to increase the
intracellular immune signaling, potentially creating a new synthetic lethality
effect.
Material and Methods
Isogenic MCF7 and MDA-MB231 clones with different BRCA1
status were generated using CRISPR/Cas9. The HR-capacities were determined by
plasmid-reconstruction assay and cell cycle distributions were analyzed by
propidium iodide staining. For determination of the radio- and chemoresistance a
colony formation assay was used. RPA and yH2AX foci formation was analyzed by
immunostaining. To analyze DNA replication, the DNA fiber assay was conducted.
Cytosolic DNA was measured using the PicoGreen Assay. PD-L1 expression on the
cell surface was analyzed by multicolor flow cytometry.
Results
All BRCA1 targeted
clones showed a significant reduction in the HR-capacity (p ≤0.001), while no changes
in the cell cycle were induced. Interestingly, the resistance to radiation (IR)
and mitomycin C varied. The MCF7 9.2 and MDA-MB231 9.11 clones were resistant
to both DNA damaging agents (D37 = 3.8 Gy; IC50 = 0.5 µg/mL),
while the MCF7 14.3 and MDA-MB231 7.22 clones were sensitive (D37 =
2 Gy; IC50 = 0.25 µg/mL). As this could not be explained by different
HR-capacities, we investigated whether there were variations in the DNA
replication stress (RS) level. And indeed, the resistant MCF7 9.2 clone showed
significantly lower level of RS (p = ≤0.01). Low level of RS might correlate
with fewer DSBs, which could be confirmed by low formation of RPA and yH2AX
foci. Strikingly, the resistant clones showed no increase in cytosolic DNA
after IR, thus no activation of the intracellular immune signaling, while the sensitive
clones did (p ≤0.001). It seems therefore likely that the resistance is
associated with the impaired activation of the intracellular immune response.
Additionally, we could observe a significantly increased PD-L1 surface expression
post IR in the resistant clones (p = ≤0.01), further suppressing the anti-tumor
effects of the immune system.
Conclusion
Our results indicate that radiochemoresistance in
HR-impaired cell lines might be associated with a reduced activation of the
intracellular immune signaling and active suppression of the anti-tumor effects.
Increasing the RS level and combining IR with immune checkpoint inhibitors might
offer a new therapeutic approach to treat tumors resistant to conventional
radiochemotherapy.