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电子显微镜下原位检测紫外线诱导的DNA断裂后的姐妹染色单体分化

Sister chromatid differentiation after in situ detection of ultraviolet-induced DNA breaks under electron microscopy.

作者信息

Fernández J L, Campos A, Goyanes V, Buño I, Gosálvez J

机构信息

Centro Oncológico de Galicia, Laboratorio de Dosimetría Biológica-Genética, Madrid, Spain.

出版信息

Biol Cell. 1994;82(1):33-7. doi: 10.1016/0248-4900(94)90063-9.

Abstract

Chinese hamster DON cells with 5-bromodeoxyuridine (BrdU)-substituted chromosomes were ultraviolet (UV)-exposed and processed for in situ detection of induced DNA breaks under electron microscopy. For this purpose, UV-induced breaks were amplified by an exonuclease III digestion to obtain single stranded DNA motifs which could hybridize with oligonucleotides of random sequences. These reannealed motifs could be used as primers which were extended by the Klenow polymerase, incorporating biotinylated-dUTP that was detected by a gold-tagged streptavidin. After processing, the chromatid whose DNA was BrdU-substituted in one strand showed a higher electron density than the chromatid substituted in both strands. In contrast, the unifilarly substituted chromatid showed about twice the labelling of DNA breaks as the bifilarly substituted one. This result could be the consequence of a greater loss of chromatin tracts in the bifilarly substituted chromatid, as implied by an X-ray microanalysis which showed that the amount of phosphorous lost by the bifilarly substituted chromatid was higher than that of the unifilarly substituted chromatid.

摘要

用5-溴脱氧尿苷(BrdU)替代染色体的中国仓鼠DON细胞经紫外线(UV)照射后,进行处理以在电子显微镜下原位检测诱导的DNA断裂。为此,通过核酸外切酶III消化扩增UV诱导的断裂,以获得可与随机序列的寡核苷酸杂交的单链DNA基序。这些重新退火的基序可用作引物,由Klenow聚合酶延伸,掺入通过金标记的链霉亲和素检测的生物素化-dUTP。处理后,单链中DNA被BrdU替代的染色单体比双链中被替代的染色单体显示出更高的电子密度。相反,单链替代的染色单体显示出的DNA断裂标记约为双链替代染色单体的两倍。这一结果可能是双链替代染色单体中染色质片段损失更大的结果,X射线微分析表明双链替代染色单体损失的磷量高于单链替代染色单体,这暗示了这一点。

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