RBE of Cells Irradiated by Carbon Ions

LI Wen-Jian; ZHOU Guang-Ming; WEI Zeng-Quan; WANG Ju-Fang; DANG Bing-Rong; LI Qiang; XIE Hong-Mei

Chinese Physics C> 2002, Vol. 26> Issue(7) : 742-746

RBE of Cells Irradiated by Carbon Ions

Institute of Modern Physics, The Chinese Academy of Sciences, Lanzhou 730000, China

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Abstract：
The mouse melanoma cells (B16), human cervical squamous carcinoma cells (HeLa), Chinese hamster pulmonary cells V79, and human hepatoma cells (SMMC-7721) were collected for studing. The cells of 5×10⁵/ml were seeded in 35mm diameter petri dish and allowed to grow one day, and then the medium in petri dishes was removed away, the cells were washed once with phosphate-bufferd saline (PBS), petri dishes was covered with 4μm thickness Mylar film. The cells were irradiated by ¹²C ion beam with LETs of 125.5, 200, 700keV/μm in water generated from HIRFL (Heavy Ion Research Facility in Lanzhou). For ⁶⁰Co γ-ray experiment, the cells of 5×10⁴/ml were grown in 20ml culture flasks including 1.5ml cell suspension and directly used for irradiation. Following irradiation, the cells were trypsinized, counted, plated at appropriate densities in growth medium and then seeded in 60mm diameter culture dishes. Each dish was filled 4ml standard medium, and incubated for 8-12 days at 37℃ incubator containing 5% CO 2. The cultures were then rinsed with PBS buffer at pH6.8, fixed with Carnoy′s fluid, stained for 8min with Giemsa (1∶20,pH6.8), and colonies containing more than 50 cells were scored. Their relative biological effectivenesses (RBE) were investigated. The results show that RBE depends on cellular types and increases with increasing of cellular survival level when LET is at 125.5keV/μm, and decreases with increasing LET when LET≥125.5keV/μm.

References

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. Kraft G, Taucher-Scholz G, Heilmann J. LET- effects in DNA, in:Fuciarelli A F, Zimbrick J D. Radiation Damage in DNA, Battelle Press,1995,203—2142. ZHU Ren-Bao, LIU Yong, LUO Zu-Yu. Radiation Biology, Beijing:Science Press,1987,425—426(in Chinese)(朱任葆,刘永,罗祖玉编著.辐射生物学,北京:科学出版社,1987,425—426)3. YU Qing-Chang, LUO Zheng-Ming, AN Zhu et al. Base of Proton Therapy Technique, Beijing:Atomic Energy Press,1999,280—294(in Chinese)(郁庆长,罗正明,安竹等.质子治疗技术基础,北京:原子能出版社,1999,280—294)4. XIA Shou-Xuan, CHEN Jia-Pei, WEI Kang et al. Molecular Radiation Biology, Beijing:Atomic Energy Press,1992,46—48(in Chinese)(夏寿萱,陈家佩,魏康等.分子放射生物学,北京:原子能出版社,1992,46—48) 5. Butts J J, Katz R. Radiat. Res.,1967,30:855—871br6. Katz R. Radiat. Res.,1971,47:402—425

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LI Wen-Jian, ZHOU Guang-Ming, WEI Zeng-Quan, WANG Ju-Fang, DANG Bing-Rong, LI Qiang and XIE Hong-Mei. RBE of Cells Irradiated by Carbon Ions[J]. Chinese Physics C, 2002, 26(7): 742-746.

LI Wen-Jian, ZHOU Guang-Ming, WEI Zeng-Quan, WANG Ju-Fang, DANG Bing-Rong, LI Qiang and XIE Hong-Mei. RBE of Cells Irradiated by Carbon Ions[J]. Chinese Physics C, 2002, 26(7): 742-746. shu

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Received: 2001-07-24
Revised: 1900-01-01

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通讯作者: 陈斌, bchen63@163.com

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沈阳化工大学材料科学与工程学院沈阳 110142

RBE of Cells Irradiated by Carbon Ions

Corresponding author: LI Wen-Jian,

Institute of Modern Physics, The Chinese Academy of Sciences, Lanzhou 730000, China

Received Date: 2001-07-24

Accepted Date: 1900-01-01

Available Online: 2002-07-05

Abstract: The mouse melanoma cells (B16), human cervical squamous carcinoma cells (HeLa), Chinese hamster pulmonary cells V79, and human hepatoma cells (SMMC-7721) were collected for studing. The cells of 5×10⁵/ml were seeded in 35mm diameter petri dish and allowed to grow one day, and then the medium in petri dishes was removed away, the cells were washed once with phosphate-bufferd saline (PBS), petri dishes was covered with 4μm thickness Mylar film. The cells were irradiated by ¹²C ion beam with LETs of 125.5, 200, 700keV/μm in water generated from HIRFL (Heavy Ion Research Facility in Lanzhou). For ⁶⁰Co γ-ray experiment, the cells of 5×10⁴/ml were grown in 20ml culture flasks including 1.5ml cell suspension and directly used for irradiation. Following irradiation, the cells were trypsinized, counted, plated at appropriate densities in growth medium and then seeded in 60mm diameter culture dishes. Each dish was filled 4ml standard medium, and incubated for 8-12 days at 37℃ incubator containing 5% CO 2. The cultures were then rinsed with PBS buffer at pH6.8, fixed with Carnoy′s fluid, stained for 8min with Giemsa (1∶20,pH6.8), and colonies containing more than 50 cells were scored. Their relative biological effectivenesses (RBE) were investigated. The results show that RBE depends on cellular types and increases with increasing of cellular survival level when LET is at 125.5keV/μm, and decreases with increasing LET when LET≥125.5keV/μm.

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