ZIA BC 006140 (ZIA) | |||
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Title | Studies of Histone Functions in Chromatin; H2AX and DNA DSBs | ||
Institution | NCI, Bethesda, MD | ||
Principal Investigator | Bonner, William | NCI Program Director | N/A |
Cancer Activity | N/A | Division | CCR |
Funded Amount | $792,122 | Project Dates | 10/01/1976 - 00/00/0000 |
Fiscal Year | 2014 | Project Type | Intramural |
Research Topics w/ Percent Relevance | Cancer Types w/ Percent Relevance | ||
Aging (20.0%) Ataxia Telangiectasia (5.0%) Cancer (100.0%) Chemotherapy (20.0%) |
Nervous System (5.0%) | ||
Research Type | |||
Cancer Initiation: Alterations in Chromosomes Application of Model Systems |
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Abstract | |||
As mentioned in ""Goals and Objectives"", we have taken H2AX research into three areas. The first area is DNA DSB biodosimetry, the measurement of DNA levels in living systems, including humans, in response to disease and environmental insults. One of the overriding issues in radiation accidents is efficient triage, determination of which victims could benefit from medical intervention as opposed to those that do not need followup, the ""worried well"", and those whose exposure was too great to save. We are in the process of determining the limits of DSB detection after whole body exposure of animals to ionizing radiation using H2AX phosphorylation as a model for triage during a radiation-related emergency. With this biodosimeter, whole body irradiations above 2 Gy can be estimated up to four days post-exposure (Moroni et al., Int J Mol Sci. 14:14119-35 2013). We are also collaborating with Dr. Asako Nakamura, previously a visiting fellow in my group and now a researcher in Japan, to make the first biodosimetric measurements of radiation exposure after Fukashima. Also in the area of DNA DSB biodosimetry is the measurement of breaks induced during chemotherapy. Two recent developments have given considerable impetus to this project. The first development is the finding by us and others that H2AX is phosphorylated in tissue culture cells as a response not only to agents that directly cause DSBs but also to those that indirectly induce DSBs. As many of the agents used for cancer treatment fall into this latter category, this finding greatly increases possible roles for H2AX phosphorylation as a biomarker for drug responses. The second important development is the formation of a multi-disiplinary NCI team to expedite the clinical evaluation of new therapeutic and imaging agents, so-called phase zero trials. H2AX phosphorylation is being examined as a possible biodosimeter in these studies utilizing several possible surrogate tissues. We are also examining H2AX phosphorylation in mouse models and are involved in several clinical protocols either approved or being approved in the phase zero and phase one trials. This work is important because it will permit clinicians to obtain immediate feedback from the cells of an individual patient, feedback which can then be used to tailor the treatment to that patient, thereby improving their survival. The ultimate goal of this initiative is to develop gamma-H2AX detection into a useful tool for human health. Our second direction is to understand how H2AX levels and structures, particularly of the region surrounding the C-terminal serine residue, impact on cellular responses to DSBs, and we have several ongoing projects in this area. Our goal is to gain insight into the function of these foci both in terms of their growth and disappearance, and their roles in DSB repair. H2AX is essential for genome stability and the rapid phase of DNA DSB repair. We are working from a hypothesis that robust genome stability depends on the speed of the fast repair phase, which in turn depends on the rate of focal growth and accumulation of repair proteins at those foci. Thus measuring the kinetics of focal growth and protein accumulation when various proteins are absent or altered may open a novel window by which to gain insights into the mechanism of early DSB repair processes, and which proteins are rate limiting in this process. We are developing tools that will permit us to study focal substructure and how it changes with time. We have shown for example, that in yeast, Mre11 does not bind to the whole gamma-H2AX domain, but is concentrated next to the break site. Studies such as these will complement other findings concerning the interactions of various proteins with gamma-H2AX, leading to a greater understanding of DNA DSB repair and the maintenance of genome stability. This work is important as it will provide the basis for understanding the important parameters involved in utilizing gamma-H2AX foci as a bio" |