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Development of a quantitative pharmacodynamic assay for apoptosis in fixed tumor tissue and its application in distinguishing cytotoxic drug-induced DNA double strand breaks from DNA double strand breaks associated with apoptosis

  1. Author:
    Dull, Angie
    Wilsker, Deborah
    Hollingshead, Melinda
    Mazcko, Christina
    Annunziata, Christina M
    LeBlanc, Amy K
    Doroshow, James H
    Kinders, Robert
    Parchment, Ralph

  2. Author Address

    Clinical Pharmacodynamic Biomarkers Program, Applied/Developmental Research Directorate, Leidos Biomedical Research, Frederick National Laboratory for Cancer Research, Frederick, Maryland, USA., Biological Testing Branch, National Cancer Institute-Frederick, Frederick, Maryland, USA., Comparative Oncology Program, National Cancer Institute, Bethesda, Maryland, USA., Women 39;s Malignancies Branch, National Cancer Institute, Bethesda, Maryland, USA., Division of Cancer Treatment and Diagnosis and Center for Cancer Research, National Cancer Institute, Bethesda, Maryland, USA.,
    1. Year: 2018
    2. Date: Mar 30
    3. Epub Date: 2018 03 30
  2. Journal: Oncotarget
    1. 9
    2. 24
    3. Pages: 17104-17116
  4. Type of Article: Article
  1. Abstract:

    DNA double strand breaks (DSBs) induced by cancer therapeutic agents can lead to DNA damage repair or persistent DNA damage, which can induce apoptotic cell death; however, apoptosis also induces DSBs independent of genotoxic insult. ?H2AX is an established biomarker for DSBs but cannot distinguish between these mechanisms. Activated cleaved caspase-3 (CC3) promotes apoptosis by enhancing nuclear condensation, DNA fragmentation, and plasma membrane blebbing. Here, we describe an immunofluorescence assay that distinguishes between apoptosis and drug-induced DSBs by measuring coexpression of ?H2AX and membrane blebbing-associated CC3 to indicate apoptosis, and ?H2AX in the absence of CC3 blebbing to indicate drug-induced DNA damage. These markers were examined in xenograft models following treatment with topotecan, cisplatin, or birinapant. A topotecan regimen conferring tumor regression induced tumor cell DSBs resulting from both apoptosis and direct DNA damage. In contrast, a cisplatin regimen yielding tumor growth delay, but not regression, resulted in tumor cell DSBs due solely to direct DNA damage. MDA-MB-231 xenografts exposed to birinapant, which promotes apoptosis but does not directly induce DSBs, exhibited dose-dependent increases in colocalized ?H2AX/CC3 blebbing in tumor cells. Clinical feasibility was established using formalin-fixed, paraffin-embedded biopsies from a canine cancer clinical trial; ?H2AX/CC3 colocalization analysis revealed apoptosis induction by two novel indenoisoquinoline topoisomerase I inhibitors, which was consistent with pathologist-assessed apoptosis and reduction of tumor volume. This assay is ready for use in clinical trials to elucidate the mechanism of action of investigational agents and combination regimens intended to inflict DNA damage, apoptotic cell death, or both.

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External Sources

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  2. DOI: 10.18632/oncotarget.24936
  3. PMID: 29682208
  4. PMCID: PMC5908309
  5. PII : 24936

Library Notes

  1. Fiscal Year: FY2017-2018
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