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首页> 外文期刊>Forensic science international. Genetics >Development of a rapid, 96-well alkaline based differential DNA extraction method for sexual assault evidence
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Development of a rapid, 96-well alkaline based differential DNA extraction method for sexual assault evidence

机译:快速的基于96孔碱性的差异DNA提取方法的开发,用于性攻击证据

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We present a rapid alkaline lysis procedure for the extraction of DNA from sexual assault evidence that generates purified sperm fraction extracts that yield STR typing results similar to those obtained from the traditional organic/dithiothreitol differential extraction. Specifically, a sodium hydroxide based differential extraction method has been developed in a single-tube format and further optimized in a 96-well format. The method yields purified extracts from a small sample set (~2-6 swabs) in approximately 2 h and from a larger sample set (up to 96 swabs) in approximately 4 h. While conventional differential extraction methods require vigorous sample manipulation to remove the spermatozoa from the substrate, the method described here exploits the propensity of sperm to adhere to a substrate and does not require any manipulation of the substrate after it is sampled. For swabs, sample handling is minimized by employing a process where the tip of the swab, including the shaft, is transferred to the appropriate vessel eliminating the need for potentially hazardous scalpels to separate the swab material from the shaft. The absence of multiple handling steps allows the process to be semi-automated, however the procedure as described here does not require use of a robotic system. This method may provide forensic laboratories a cost-effective tool for the eradication of backlogs of sexual assault evidence, and more timely service to their client agencies. In addition, we have demonstrated that a modification of the procedure can be used to retrieve residual sperm-cell DNA from previously extracted swabs.
机译:我们提出了一种快速的碱性裂解程序,用于从性侵犯证据中提取DNA,该证据产生纯化的精子馏分提取物,产生的STR分型结果与从传统有机/二硫苏糖醇差异提取法获得的结果相似。具体而言,已开发出了基于单管形式的氢氧化钠差分萃取方法,并进一步以96孔形式进行了优化。该方法可在约2小时内从少量样品(约2-6个棉签)中提取纯化的提取物,而在约4小时内从较大样品(约96个棉签)中提取纯化的提取物。尽管常规的差异提取方法需要大力进行样品处理才能从基质上去除精子,但此处描述的方法利用了精子粘附在基质上的倾向,并且在对基质进行采样后不需要对基质进行任何处理。对于棉签,通过采用将棉签的尖端(包括杆身)转移到适当的容器中的方法,可以最大程度地减少样品处理,而无需使用潜在危险的手术刀将棉签材料与杆身分离。由于没有多个处理步骤,因此该过程可以半自动化,但是此处所述的过程不需要使用机器人系统。这种方法可以为法医实验室提供一种经济有效的工具,以消除积压的性侵犯证据,并为客户机构提供更及时的服务。此外,我们已经证明,该程序的修改可用于从先前提取的拭子中检索残留的精子细胞DNA。

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