Abstract

The long-term objective of this project is to continue development of probes and methodologies for analysis of individual cells by flow or image cytometry applicable to tumor diagnosis and prognosis and for studies of apoptosis, cell proliferation and antitumor drug screening.
The specific aims represent the continuation of four recently initiated projects: (1) DNA damage: Histone H2AX phosphorylation reveals the site of DNA double strand breaks (DSBs). We will: (a) design methods to distinguish antitumor drug induced (DI), primary DSBs from apoptosis-associated, secondary DSBs; (b) assess the kinetics of H2AX phosphorylation and dephosphorylation as a function of drug dose and treatment duration; (c) correlate the extent of H2AX phosphorylation with early events of apoptosis; (d) study how the rate of DNA replication and/or transcription affects the incidence of DI DSB; (e) explore whether phosphorylation of H2AX can provide a new, convenient marker of DNA-replicating cells; (f) reveal whether H2AX phosphorylation can serve as a marker of DNA repair, and (g) adapt the laser scanning cytometer (LSC) to quantify the number of DSBs per nucleus. (2) Activation of serine (Ser) proteases during apoptosis. Using fluorochrome-labeled inhibitors of Ser proteases (FLISP) as affinity ligands to active Ser proteases we will: (a) further characterize the specificity of these ligands; (b) correlate activation of Ser proteases with activation of initiator and effector caspases in intrinsic and extrinsic models of apoptosis; and (c) test fluorochrome-tagged phosphonate inhibitors of Ser proteases as alternative markers of protease activation. (3) Activation of transglutaminase (TGase 2) during apoptosis. A new cytometric assay of TGase 2 activation will be used to: (a) characterize the differences in morphology and in other physical/cytochemical attributes measured by cytometry of cells that undergo apoptosis with vs without TGase 2 activation; and (b) define conditions/causes under which apoptosis occurs with vs without TGase 2 activation. (4) Develop microtransponders (MTPs) as a platform for measuring cell viability with the goal of creating a high-content anticancer drug screening assay. Towards this goal: (a) the optimal conditions for growing cells attached to MTPs will be determined and cell growth and viability on these surfaces (by differential measurement of DNA and RNA content) will be compared with cell growth on standard solid-phase support; and (b) the ability to measure the cytostatic/cytotoxic effects of antitumor drugs on tumor cell lines will be tested and compared with the standard MTT cytotoxicity assay.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA028704-29
Application #
7340414
Study Section
Special Emphasis Panel (ZRG1-ISD (01))
Program Officer
Rasooly, Avraham
Project Start
1990-10-01
Project End
2010-01-31
Budget Start
2008-02-01
Budget End
2009-01-31
Support Year
29
Fiscal Year
2008
Total Cost
$328,522
Indirect Cost

  Institution

Name
New York Medical College
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
041907486
City
Valhalla
State
NY
Country
United States
Zip Code
10595

  Publications

Halicka, H Dorota; Garcia, Jorge; Li, Jiangwei et al. (2017) Synergy of 2-deoxy-D-glucose combined with berberine in inducing the lysosome/autophagy and transglutaminase activation-facilitated apoptosis. Apoptosis 22:229-238
Hanly, Elyse K; Bednarczyk, Robert B; Tuli, Neha Y et al. (2015) mTOR inhibitors sensitize thyroid cancer cells to cytotoxic effect of vemurafenib. Oncotarget 6:39702-13
Ferguson, Lynnette R; Chen, Helen; Collins, Andrew R et al. (2015) Genomic instability in human cancer: Molecular insights and opportunities for therapeutic attack and prevention through diet and nutrition. Semin Cancer Biol 35 Suppl:S5-S24
Block, Keith I; Gyllenhaal, Charlotte; Lowe, Leroy et al. (2015) Designing a broad-spectrum integrative approach for cancer prevention and treatment. Semin Cancer Biol 35 Suppl:S276-S304
Hanly, Elyse K; Darzynkiewicz, Zbigniew; Tiwari, Raj K (2015) Biguanides and targeted anti-cancer treatments. Genes Cancer 6:82-3
Zhao, Hong; Darzynkiewicz, Zbigniew (2014) Attenuation of replication stress-induced premature cellular senescence to assess anti-aging modalities. Curr Protoc Cytom 69:9.47.1-9.47.10
Darzynkiewicz, Zbigniew; Zhao, Hong; Halicka, H Dorota et al. (2014) In search of antiaging modalities: evaluation of mTOR- and ROS/DNA damage-signaling by cytometry. Cytometry A 85:386-99
Hanly, Elyse K; Rajoria, Shilpi; Darzynkiewicz, Zbigniew et al. (2014) Disruption of mutated BRAF signaling modulates thyroid cancer phenotype. BMC Res Notes 7:187
Tarnok, A; Darzynkiewicz, Z (2013) New insights into cell cycle and DNA damage response machineries through high-resolution AMICO quantitative imaging cytometry. Cell Prolif 46:497-500
Zhang, Sufang; Zhao, Hong; Darzynkiewicz, Zbiegniew et al. (2013) A novel function of CRL4(Cdt2): regulation of the subunit structure of DNA polymerase ? in response to DNA damage and during the S phase. J Biol Chem 288:29550-61

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