首页> 美国卫生研究院文献>Nucleic Acids Research >Target Detection Assay (TDA): a versatile procedure to determine DNA binding sites as demonstrated on SP1 protein.
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Target Detection Assay (TDA): a versatile procedure to determine DNA binding sites as demonstrated on SP1 protein.

机译:靶标检测法(TDA):确定DNA结合位点的通用方法如SP1蛋白所示。

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摘要

We developed a rapid method designated Target Detection Assay (TDA) to determine DNA binding sites for putative DNA binding proteins. A purified, functionally active DNA binding protein and a pool of random double-stranded oligonucleotides harbouring PCR primer sites at each end are included the TDA cycle which consists of four separate steps: a DNA protein incubation step, a protein DNA complex separation step, a DNA elution step and a polymerase chain reaction (PCR) DNA amplification step. The stringency of selection can be increased in consecutive TDA cycles. Since tiny amounts of retained DNA can be rescued by PCR, buffer systems, salt concentrations and competitor DNA contents can be varied in order to determine high affinity binding sites for the protein of choice. To test the efficiency of the TDA procedure potential DNA binding sites were selected by the DNA binding protein SP1 from a pool of oligonucleotides with random nucleotides at 12 positions. Target sites selected by recombinant SP1 closely matched the SP1 consensus site. If DNA recognition sites have to be determined for known, mutated or putative DNA binding proteins, the Target Detection Assay (TDA) is a versatile and rapid technique for consideration.
机译:我们开发了一种称为目标检测测定(TDA)的快速方法,可以确定推定的DNA结合蛋白的DNA结合位点。 TDA循环包括纯化的,具有功能活性的DNA结合蛋白和在每个末端带有PCR引物位点的随机双链寡核苷酸库,该过程由四个独立的步骤组成:DNA蛋白质孵育步骤,蛋白质DNA复合物分离步骤, DNA洗脱步骤和聚合酶链反应(PCR)DNA扩增步骤。选择的严格性可以在连续的TDA周期中提高。由于可以通过PCR挽救极少量的保留DNA,因此可以改变缓冲液系统,盐浓度和竞争对手DNA的含量,以便确定所选蛋白质的高亲和力结合位点。为了测试TDA方法的效率,通过DNA结合蛋白SP1从具有12个位置的随机核苷酸的寡核苷酸池中选择潜在的DNA结合位点。重组SP1选择的目标位点与SP1共有位点紧密匹配。如果必须为已知的,突变的或推定的DNA结合蛋白确定DNA识别位点,则靶标检测测定(TDA)是一种通用且快速的技术。

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