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首页> 外文期刊>Mutagenesis >Induction of chromosomal aberrations (unstable and stable) by inhibitors of topoisomerase II, m-AMSA and VP16, using conventional Giemsa staining and chromosome painting techniques.
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Induction of chromosomal aberrations (unstable and stable) by inhibitors of topoisomerase II, m-AMSA and VP16, using conventional Giemsa staining and chromosome painting techniques.

机译:拓扑异构酶II,m-AMSA和VP16的抑制剂使用常规的Giemsa染色和染色体涂染技术诱导染色体畸变(不稳定且稳定)。

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摘要

Frequencies of symmetrical and asymmetrical exchange aberrations induced by two inhibitors of topoisomerase II, namely, 4'-(9-acridinylamino) methanesulfon-m-anisidide (m-AMSA) and etoposide (VP16), were estimated in human peripheral blood lymphocytes. The aberrations were scored using conventional Giemsa staining and fluorescence in situ hybridization (FISH) techniques, using chromosome-specific DNA libraries. Stable aberrations (translocations) were detected using two cocktails of DNA libraries specific for three chromosomes, namely 1, 3 and X and 2, 4 and 8, representing approximately 40% of the whole human genome. The frequencies of dicentrics and translocations increased in a dose-dependent manner, however, m-AMSA was found to be a more potent inducer of chromosomal aberrations in comparison with VP16 (at concentrations at which comparable frequencies of aberrations were induced) by 20- to 30-fold. When corrected for DNA content of chromosomes in each cocktail, a higher frequency of translocations with the cocktail consisting of chromosomes 2, 4 and 8 in comparison with 1, 3 and X was evident. The genomic translocation frequency calculated from chromosome painting analysis for m-AMSA exceeded that estimated for dicentrics by approximately 2-fold. However, for VP16 almost equal frequencies of both types of chromosome exchange were found.
机译:估算了人类外周血淋巴细胞中两种拓扑异构酶II抑制剂(即4'-(9-ac啶基氨基)甲磺酰胺-间苯二胺(m-AMSA)和依托泊苷(VP16))引起的对称和不对称交换像差的频率。使用常规的吉姆萨染色和荧光原位杂交(FISH)技术,使用染色体特异的DNA文库对像差进行评分。使用两个特异于三个染色体(即1、3,X和2、4和8)的DNA库混合物检测到稳定的畸变(易位),占整个人类基因组的约40%。双着丝粒和易位的频率以剂量依赖的方式增加,但是,与VP16(在可比较的畸变频率下)相比,m-AMSA是更有效的染色体畸变诱导剂(在诱导可比畸变的浓度下)。 30倍。当校正每个混合物中染色体的DNA含量时,与1、3和X相比,由2、4和8号染色体组成的混合物的移位频率更高。从染色体涂漆分析得出的m-AMSA的基因组移位频率比双着丝粒估计的基因移位频率大约高2倍。但是,对于VP16,发现两种染色体交换的频率几乎相等。

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