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1 Medicine, University of Maryland, Baltimore, Maryland, United States
2 Veterinary Medicine, Chungnam National University, Korea, Republic of
3 Pharmacology, University of Michigan, Ann Arbor, Michigan, United States
4 Radiation Oncology, University of Maryland, Baltimore, Maryland, United States
* To whom correspondence should be addressed. E-mail: skwoo{at}medicine.umaryland.edu.
When exposed to hypertonic conditions, cells accumulate double strand DNA breaks (DSBs) like they are exposed to ionizing radiation. It has been proposed that inactivation of MRN complex due to nuclear exit is responsible for the accumulation of DSBs as cells fail to repair DSBs produced during normal cellular activity. In this study, we examined MRN complex in cells switched to hypertonicity. Surprisingly, we found that the MRN complex stayed in the nucleus and remained intact in response to hypertonicity. In fact, MRN complex was dramatically activated after 4 hr of switch to hypertonicity in a dose-dependent manner as shown by formation of foci. Activation of ATM and MRN complex by hypertonicity and bleomycin was additive as was activation of their downstream targets including
H2AX and Chk2 indicating that the cellular response to DSB was intact in hypertonic conditions. Activation of Chk2 in response to hypertonicity was not observed in mutant cells with functionally impaired MRN complex confirming that they are in the same pathway. After 20 hr of switch to hypertonicity, MRN foci and
H2AX returned to control level suggesting that cells adapted to hypertonicity by repairing DNA. We conclude that cells respond normally to DSB and repair the DNA damages induced by hypertonicity.
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