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Differences in gamma-H2AX foci formation after irradiation with continuous; pulsed proton beams

机译:连续照射后γ-H2AX焦点形成的差异;脉冲质子梁

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Introduction: Classical particle accelerators offer proton pulses of some milliseconds duration. In contrast, the new technology of the high-intensity laser acceleration will produce ultimately shorter particle packages (up to one nanosecond) with substantially lower pulse frequency and higher pulse-dose achievement. Very little is known about the relative biological effectiveness (RBE) of this new beam quality, which could be a possible future application in radiation oncology. In our present study we investigate possible differences based on quantitative analysis of y-H2AX fluorescence - a known marker of DNA double strand breaks (DSBs). Methods: HeLa cells were irradiated with 1 Gy of 20 MeV protons at the Munich tandem accelerator, either at continuous mode (100 ms), or at pulsed mode with a single pulse of 1 ns duration. A dose-effect-curve based on five doses of 75 kV x-rays served for reference. The total number of y -H2AX foci per cell was determined using a self-developed macro (ImageJ, NIH, USA). Results: Quantitative analysis of y-H2AX fluorescence revealed no significant difference (p=0.16) in yield of foci formation after irradiation with pulsed or continuous proton beams. y-H2AX data for cell samples exposed to 1 Gy of 20 MeV protons at pulsed or continuous irradiation modes were 23.29 ± 2.04 and 26.54 ± 2.54 foci per cell, respectively. The corresponding RBE values for 20 MeV protons were 0.96 ±0.18 and 1.13 ±0.21 (p=0.2l) for pulsed and continuous irradiation modes. However, the percentage of foci smaller than 5-10 pixels was slightly decreased and foci tended to cluster after irradiation with pulsed protons. Conclusions: Based on y-H2AX foci formation no significant difference in the RBE between pulsed and continuous proton irradiation beams in HeLa cells has been detected so far. These results are well in line with our data on micronucleus induction in HeLa cells.
机译:简介:经典粒子加速器提供一些毫秒持续时间的质子脉冲。相反,高强度激光加速度的新技术将产生最终的粒子封装(最多一个纳秒),其脉冲频率和更高的脉冲剂量成就。很少熟悉这种新的光束质量的相对生物效果(RBE),这可能是辐射肿瘤学中可能的应用。在我们目前的研究中,我们研究了基于Y-H2AX荧光的定量分析的可能差异 - 一种已知的DNA双链突破(DSB)的标记。方法:在慕尼黑串联促进剂处用1GY的20meV质子,在连续模式(100ms)或脉冲模式下照射HeLa细胞,或者在脉冲模式下,具有1ns持续时间的单个脉冲。一种基于五剂量的75kV X射线的剂量效应曲线。使用自发宏(Imagej,NiH,USA)确定每个电池的Y-H2AX焦点的总数。结果:Y-H2AX荧光的定量分析显示在用脉冲或连续质子束照射后没有显着差异(P = 0.16)的焦焦形成产率。在脉冲或连续照射模式下暴露于20mEV质子的细胞样品的Y-H2AX数据分别为每种细胞23.29±2.04和26.54±2.54焦点。对于脉冲和连续照射模式,20meV质子的相应RBE值为20meV质子为0.96±0.18和1.13±0.21(p = 0.21)。然而,小于5-10像素的焦点的百分比略微降低,并且在用脉冲质子照射后倾向于簇的焦点。结论到目前为止,基于Y-H2AX焦点形成,迄今为止已经检测到HeLa细胞中脉冲和连续质子辐射束之间的RBE之间的显着差异。这些结果符合我们对HeLa细胞中微核感应的数据。

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