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The use of fluorescence in situ hybridisation combined with premature chromosome condensation for the identification of chromosome damage.

机译:荧光原位杂交与染色体过早凝结相结合用于鉴定染色体损伤。

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摘要

The technique of fusing mitotic cells to interphase cells, thereby producing condensation of the chromosomes of the interphase cell (so-called 'premature chromosome condensation' or PCC), has allowed detection of the initial number of chromosome breaks and their repair following ionising radiation. However, the difficulty and tedium of scoring all the chromosome fragments, as well as the inability to readily detect exchange aberrations, has limited the use of PCC. We describe here the use of the recently developed technique of fluorescence in situ hybridisation with whole chromosome libraries to stain individual human chromosomes (also called 'chromosome painting') with the PCC's and show that this overcomes most of the limitations with the analysis of PCC's. First, by focusing on a single chromosome, scoring of breaks in the target chromosome is easy and rapid and greatly expands the radiation dose range over which the PCC technique can be used. Second, it allows the easy recognition of exchange type aberrations. A number of new applications of this technology, such as predicting the radiosensitivity of human tumours in situ, are feasible.
机译:将有丝分裂细胞融合至相间细胞,从而使相间细胞的染色体凝缩的技术(所谓的“过早染色体凝缩”或PCC),已使人们能够检测染色体断裂的初始数目并在电离辐射后对其进行修复。但是,对所有染色体片段进行评分的困难和繁琐,以及无法轻松检测交换像差,限制了PCC的使用。我们在这里描述了使用最近开发的与整个染色体库进行荧光原位杂交的技术,用PCC对单个人类染色体进行染色的方法(也称为``染色体绘画''),并显示通过PCC的分析可以克服大多数限制。首先,通过关注单个染色体,可以轻松,快速地对目标染色体的断裂进行评分,并大大扩展了可使用PCC技术的辐射剂量范围。其次,它可以轻松识别交换类型像差。该技术的许多新应用是可行的,例如在原位预测人类肿瘤的放射敏感性。

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