The role of DNA damage repair and Chk2 protein in hyper-radiosensitivity of lung adenocarcinoma A549 cells

Hongge Wu , Qitian Chen , Yong Zhang , Gang Wu , Rui Meng , Jing Cheng

Current Medical Science ›› 2012, Vol. 32 ›› Issue (5) : 750 -754.

PDF
Current Medical Science ›› 2012, Vol. 32 ›› Issue (5) : 750 -754. DOI: 10.1007/s11596-012-1029-z
Article

The role of DNA damage repair and Chk2 protein in hyper-radiosensitivity of lung adenocarcinoma A549 cells

Author information +
History +
PDF

Abstract

To explore the role of the Chk2 protein expression and DNA double strand breaks (DSBs) repair in low dose hyper-radiosensitivity (HRS)/increased radioresistance (IRR) of non-small cell lung cancer, A549 cells were subjected to irradiation at the dosage ranging from 0.05–2 Gy. Clonogenic survival was measured by using fluorescence-activated cell sorting (FACS) plating technique. Percentage of cells in M-phase after low doses of X-irradiation was evaluated by phospho-histone H3-FITC/PI and Western blotting was used to detect protein expression of Chk2 and phospo-Chk2. DNA DSBs repair efficiency was also measured by induction and persistence of γ-H2AX. The results showed that the killing ability of irradiation with A549 cells increased at low conditioning dose below 0.3 Gy. Within the dose of 0.3 to 0.5 Gy, A549 cells showed a certain extent of radiation resistance. And when the dose was more than 0.5 Gy, survival fraction exhibited a negative correlation with the dosage. There was no difference between the 0.1 or 0.2 Gy dosage groups and the un-irradiated group in terms of the percentage of cells in M phase. But in the high dosage group (0.3–1.0 Gy), the percentage of cells in M phase was decreased markedly. In addition, the percentage of cells in M phase began to decrease two hours after irradiation. One hour after irradiation, there was no conspicuous activation of Chk2 kinase in 0.1 or 0.2 Gy group, but when the irradiation dose reached 0.3 Gy or higher, Chk2 kinase started to be activated and the activation level showed no significant difference among high dosage groups (0.4, 0.5, 1.0 Gy). Within 1 to 6 h, the DNA DSBs repair efficiency was decreased at 0.2 Gy but increased at 0.5 Gy and 1.0 Gy, which was in line with Chk2 activation. We are led to conclude that the mechanism of HRS/IRR in A549 cell line was probably due to early G2/M checkpoint arrest and enhanced DNA DSBs repair. In this regard, Chk2 activation plays a key role in G2/M checkpoint activation.

Keywords

early G2/M checkpoint / Chk2 / HRS/IRR / DNA DSBs

Cite this article

Download citation ▾
Hongge Wu, Qitian Chen, Yong Zhang, Gang Wu, Rui Meng, Jing Cheng. The role of DNA damage repair and Chk2 protein in hyper-radiosensitivity of lung adenocarcinoma A549 cells. Current Medical Science, 2012, 32(5): 750-754 DOI:10.1007/s11596-012-1029-z

登录浏览全文

4963

注册一个新账户 忘记密码

References

Publishing order | Descend order by publishing year | Descend order by cited within
[1]

MarplesB., JoinerM.C.. The response of Chinese hamster V79 cells to low radiation doses: Evidence of enhanced sensitivity of the whole cell population. Radiat Res, 1993, 133(1): 41-51

[2]

MarplesB., CollisS.J.. Low-dose hyper-radiosensitivity: Past, present, and future. Int J Radiat Oncol Biol Phys, 2008, 70(5): 1310-1318

[3]

HonoreH.B., BentzenS.M.. A modeling study of the potential influence of low dose hypersensitivity on radiation treatment planning. Radiother Oncol, 2006, 79(1): 115-121

[4]

EnnsL., BogenK.T., WizniakJ., et al.. Low-dose radiation hyper-sensitivity is associated with p53-dependent apoptosis. Mol Cancer Res, 2004, 2(10): 557-566
[5]

ShortS.C., WoodcockM., MarplesB., et al.. The effects of cell cycle phase on low dose hyper-radiosensitivity. Int J Radiat Biol, 2003, 79(2): 99-105
[6]

MarplesB., WoutersB.G., JoinerM.C.. An association between the radiation-induced arrest of G 2 phase cells and low-dose hyper-radiosensitivity: A plausible underlying mechanism?. Radiat Res, 2003, 160(1): 38-45

[7]

XuB., KimS.T., LimD.S., et al.. Two molecularly distinct G2/Mcheckpoints are induced by ionizing irradiation. Mol Cell Biol, 2002, 22(4): 1049-1059

[8]

KruegerS.A., CollisS.J., JoinerM.C., et al.. The transition in survival from low-dose hyper-radiosensitivity to incressed radioresisitance is independent of activation of ATM SER1981 activity. Int J Radiat Oncol Biol Phys, 2007, 69(4): 1262-1271

[9]

KruegerS.A., WilsonG.D., PiasentinE., et al.. The effects of G2-phase enrichment and checkpoint abrogation on low-dose hyper-radiosensitivity. Int J Radiat Oncol Biol Phys, 2010, 77(5): 1509-1517

[10]

AhnJ., UristM.. Prives C: The Chk2 protein kinase. DNA Reipair, 2004, 3(8–9): 1039-1047

[11]

SchwarzJ.K., LovlyC.M., Piwnica-WormsH.. Regulation of the CHK2 protein by oligomerization-mediated cis- and trans-phosphorylation. Mol Cancer Res, 2003, 1(8): 598-609
[12]

RaineyM.D., BlackE.J., ZachosG., et al.. Chk2 is required for optimal mitotic delay in response to irradiation-induced DNA damage incurred in G2 phase. Oncogene, 2008, 27(7): 896-906

[13]

LandsverkK.S., PatzkeS., ReinI.D., et al.. Three independent mechanisms for arrest in G2 after ionizing radiation. Cell Cycle, 2011, 10(5): 819-829

[14]

SkoeK.A.. Radioresponsiveness at low doses: Hyper-radiosensitivity and increased radioresistance in mammalian cells. Mutat Res, 1999, 430(2): 241-253

[15]

MarplesB., JoinerM.C.. Modification of survival by DNA repair modifiers: A probable explanation for the phenomenon of increased radioresistance. Int J Radiat Biol, 2000, 76(3): 305-312

[16]

O’DriscollM., JeggoP.A.. The role of double-strand break repair-insights from human genetics. Nat Rev Genet, 2006, 7(1): 45-54

[17]

XueL., YuD., FurusawaY., et al.. ATM-dependent hyper-radiosensitivity in mammalian cells irradiated by heavy ions. Int J Radiat Oncol Biol Phys, 2009, 75(1): 235-243

AI Summary AI Mindmap
PDF

89

Accesses

0

Citation

Detail
Sections
Recommended

AI思维导图

/