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用于从流式核型分析评估每个细胞辐射诱导的染色体畸变产额的算法。

Algorithms for the evaluation of radiation induced chromosome aberration yields per cell from flow karyotypes.

作者信息

Dietzel A H, Hain J, Virsik-Peuckert R P, Harder D

机构信息

Institute of Medical Physics and Biophysics, University of Goettingen, West Germany.

出版信息

Cytometry. 1990;11(6):708-15. doi: 10.1002/cyto.990110608.

Abstract

CHO-K1 cells were irradiated in G0/G1-phase with 150 kV X-rays. Single chromosomes isolated from metaphase cells and stained with DNA intercalating dye DAPI were analyzed in the ICP 22 with a modified flow chamber. In order to study dose-dependent changes in the flow karyotypes, they were split into peak- and background-portions by an iterative fit algorithm. As in a first approach, estimates of the frequencies of chromosome lesions were derived from an evaluation of the dose-dependent reduction in peak contents. The number of radiation-induced lesions per chromosome was found to be proportional to its length. As a second approach, the number of fluorescence events in the histogram background was corrected for non-chromosomal debris and evaluated interms of chromosome aberration frequency per cell, which was consistent with the yields of dicentric chromosomes and acentric fragments observed in microscopic investigations. As a third approach, lesion frequencies were calculated from the corrected background light sum in the karyotypes, utilizing a Monte Carlo model to simulate the effect of aberration formation on the flow histogram. The results indicate that the number of chromosome lesions observed by flow cytometry can be quantitatively related to the yield of structural chromosome aberrations detected by microscopic analysis. Dose-effect relations and split-dose kinetics are given as examples demonstrating the usefulness of this technique in radiobiology. Time saving compared to microscopic analysis was of the order of 90%.

摘要

将CHO-K1细胞在G0/G1期用150 kV X射线进行照射。从处于中期的细胞中分离出单条染色体,并用DNA嵌入染料DAPI染色,然后在配有改良流动腔的ICP 22中进行分析。为了研究流式核型中的剂量依赖性变化,通过迭代拟合算法将其分为峰部和背景部分。在第一种方法中,染色体损伤频率的估计值来自对峰含量剂量依赖性降低的评估。发现每条染色体上辐射诱导损伤的数量与其长度成正比。在第二种方法中,对直方图背景中的荧光事件数量进行非染色体碎片校正,并以每个细胞的染色体畸变频率进行评估,这与显微镜观察中观察到的双着丝粒染色体和无着丝粒片段的产率一致。在第三种方法中,利用蒙特卡罗模型模拟畸变形成对流动直方图的影响,从核型中校正后的背景光总和计算损伤频率。结果表明,通过流式细胞术观察到的染色体损伤数量可以与显微镜分析检测到的结构染色体畸变产率进行定量关联。给出了剂量效应关系和分次剂量动力学的例子,证明了该技术在放射生物学中的实用性。与显微镜分析相比,节省时间约为90%。

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