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A method to determine the 5′ end of the binding site of primers included in a commercially available forensic human identification kit

机译:确定市售法医鉴定试剂盒中引物结合位点5'端的方法

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Analysis for short tandem repeat (STR) loci is widely performed in forensic laboratories for human identification that utilizes commercially available kits that employ fluorescently labeled primers and capillary electrophoresis. With only a few exceptions, the sequences of the primers included in a kit are not disclosed by the kit manufacturers. Therefore, we developed a simple method to determine the 5′ end of the binding site of the primers included in commercial kits. Our method requires only custom primers and human genome sequence data and routinely used equipment and consumables. One or two custom primers are added to the PCR reaction mixture containing kit primers and input human DNA prior to amplification, and PCR products are separated by capillary electrophoresis after amplification. With this method we can determine which primer of the pair is fluorescently labeled and the 5′ end of the binding site of primers based on the changes in an electropherogram that are caused by the addition of the custom primer(s), and the human genome sequence data. This method is also useful for the determination of the shortest possible lengths of labeled kit primers.
机译:短串联重复序列(STR)基因座的分析在法医实验室中进行了广泛的鉴定,以利用可利用荧光标记引物和毛细管电泳的市售试剂盒进行人类鉴定。除少数例外,试剂盒制造商未披露试剂盒中包含的引物序列。因此,我们开发了一种简单的方法来确定商业试剂盒中所包含引物结合位点的5'端。我们的方法仅需要定制引物和人类基因组序列数据,以及常规使用的设备和消耗品。在扩增之前,将一种或两种定制引物添加到含有试剂盒引物和输入人DNA的PCR反应混合物中,并在扩增后通过毛细管电泳分离PCR产物。通过这种方法,我们可以基于添加定制引物和人类基因组而引起的电泳图谱变化,确定该对引物中的哪个被荧光标记,以及引物结合位点的5'端。序列数据。该方法还可用于确定标记试剂盒引物的最短长度。

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