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An efficient chemical method to generate repetitive sequences depleted DNA probes.

机译:一种有效的化学方法来生成重复序列耗尽的DNA探针。

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We describe an efficient method to remove repetitive sequences from DNA of microdissected whole chromosomes, chromosome arms, locus specific probes, and specific bands. The chemical approach described removes human repetitive DNA sequences from a source DNA, eliminating the need for blocking such sequences when the source DNA used as a probe is hybridized with a target DNA. It employs subtracting hybridized biotin-labeled repetitive-sequence DNA complex with phenol and chloroform after incubation of hybridized products with avidin. The method produces unique products that are formed after such repetitive sequences have been removed from the DNA. We have applied our newly designed subtraction strategy to microdissected chromosomes in generating whole chromosome painting (e.g., chromosome 4), chromosome arm (e.g., 1q and 15q), and band (e.g., 3q26) specific probes, and we have demonstrated its utility using flow-sorted chromosome. FISH analyses using these probes show consistent strong signals with no cross-hybridization, and optimal hybridization results can be obtained relatively quickly.
机译:我们描述了一种有效的方法,可从显微解剖的整个染色体,染色体臂,基因座特异性探针和特定条带的DNA中去除重复序列。所描述的化学方法从源DNA中去除了人的重复DNA序列,当用作探针的源DNA与靶DNA杂交时,无需封闭此类序列。在将亲和素与杂交产物孵育后,采用与酚和氯仿的生物素标记的重复序列DNA复合体相减的方法。该方法产生独特的产物,该产物是在从DNA中去除了这些重复序列之后形成的。我们已将我们新设计的减法策略应用于显微解剖的染色体,以生成完整的染色体绘画(例如4号染色体),染色体臂(例如1q和15q)和条带(例如3q26)特定探针,并且我们已经证明了其实用性:流分类的染色体。使用这些探针进行的FISH分析显示出一致的强信号,没有交叉杂交,并且可以相对快速地获得最佳杂交结果。

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