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Cloning of deleted sequences (CODE): A genomic subtraction method for enriching and cloning deleted sequences

机译:缺失序列的克隆(CODE):一种基因组减法,用于富集和克隆缺失序列

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The deletion of specific genomic sequences is believed to influence the pathogenesis of certain diseases such as cancer. Identification of these sequences could provide novel therapeutic avenues for the treatment of disease. Here, we describe a simple and robust method called cloning of deleted sequences (CODE), which allows the selective cloning of deleted sequences from complex human genomes. Briefly, genomic DNA from two sources (human normal and tumor samples) was digested with restriction enzymes (e.g., BamHI, BglII, and BclI), then ligated to special linkers, and amplified by PCR. Tester (normal) DNA was amplified using a biotinylated primer and dNTPs. Driver (tumor) DNA was amplified using a non-biotinylated primer but with dUTP instead of dTTP. After denaturation and hybridization, all the driver DNA was destroyed with uracil-DNA glycosylase (UDG), and all imperfect hybrids were digested with mung bean nuclease. Sequences deleted from the driver DNA but present in the tester DNA were purified with streptavidin magnetic beads, and the cycle was repeated three more times. This procedure resulted in the rapid isolation and efficient cloning of genomic sequences homozygously deleted from the driver DNA sample, but present in the tester DNA fraction.
机译:据信特定基因组序列的缺失影响某些疾病例如癌症的发病机理。这些序列的鉴定可以为疾病的治疗提供新的治疗途径。在这里,我们描述了一种简单而健壮的方法,称为克隆缺失序列(CODE),它允许从复杂的人类基因组中选择性克隆缺失的序列。简而言之,用限制性内切酶(例如,BamHI,BglII和BclI)消化来自两种来源(人正常和肿瘤样品)的基因组DNA,然后连接至特殊的接头,并通过PCR扩增。使用生物素化的引物和dNTP扩增测试者(正常)DNA。使用非生物素化的引物,但用dUTP代替dTTP扩增了驱动程序(肿瘤)DNA。变性和杂交后,所有驱动DNA均被尿嘧啶-DNA糖基化酶(UDG)破坏,所有不完善的杂种均被绿豆核酸酶消化。用抗生蛋白链菌素磁珠纯化从驱动程序DNA中缺失但存在于测试者DNA中的序列,并将该循环再重复三遍。该过程导致快速分离和有效克隆从驱动器DNA样品中纯合缺失但存在于测试者DNA组分中的基因组序列。

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