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Use of DOP-PCR for amplification and labeling of BAC DNA for FISH

机译:DOP-PCR用于扩增和标记F鱼的BAC DNA

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摘要

Fluorescence in situ hybridization (FISH) is a powerful molecular cytogenetic method that permits rapid detection of specific chromosomal rearrangements. It is based on the hybridization of fluorescent labeled probes to metaphase chromosomes or interphase nuclei. The DNA probes commonly are generated from cloned sources such as bacterial artificial chromosomes (BACs). The major disadvantage of this approach is that it requires laborious and time-consuming work. We used a degenerate oligonucleotide primed polymerase chain reaction (DOP-PCR) for both amplification and labeling of very small amounts of purified BAC DNA for FISH. The DOP-PCR reaction was processed in two steps: pre-amplification followed by simultaneous amplification and labeling of BAC DNA. The DOP-PCR probes obtained provided good hybridization signals and low background. Thus, DOP-PCR can be used to produce unlimited quantities of FISH probes with decreased cost and labor.
机译:原位杂交(鱼类)的荧光是一种强大的分子细胞遗传学方法,允许快速检测特异性染色体重排。 它基于荧光标记探针与中期染色体或间核的杂交。 通常由克隆来源(例如细菌人工染色体(BAC)产生的DNA探针。 这种方法的主要缺点是它需要艰苦的工作和耗时的工作。 我们使用了脱寡核苷酸引发的聚合酶链反应(DOP-PCR),用于扩增和标记非常少量的鱼类。 以两步加工DOP-PCR反应:预扩增,然后同时扩增和标记Bac DNA。 获得的DOP-PCR探针提供了良好的杂交信号和低背景。 因此,DOP-PCR可用于产生无限量的鱼探针,其成本和劳动力降低。

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