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首页> 外文期刊>International journal of legal medicine >A proof of principal study on the use of direct PCR of semen and spermatozoa and development of a differential isolation protocol for use in cases of alleged sexual assault
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A proof of principal study on the use of direct PCR of semen and spermatozoa and development of a differential isolation protocol for use in cases of alleged sexual assault

机译:精液和精子直接PCR的主要研究证明以及在涉嫌性侵犯案件中使用差动隔离方案的发展

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摘要

Sexual assault samples are some of the most common samples encountered in forensic analysis. These samples can require a significant time investment due to differential extraction processes. We report on the first record of successful direct amplification of semen for STR analysis. Neat seminal fluid, dilutions ranging from 1:5 to 1:160 and GEDNAP samples were successfully amplified using a direct method. A mild differential isolation technique to enrich spermatozoa was developed and successfully implemented to separate and directly amplify a mixture of semen and female epithelial cells. Aliquots of samples subjected to the differential isolation protocol were stained with Haemotoxylin and Eosin for sperm scoring. Samples stained after PCR showed a complete lack of intact spermatozoa demonstrating that the cells are lysed during the PCR process. This paper demonstrates the potential to incorporate direct PCR in cases of sexual assault to more rapidly obtain results and achieve a higher sensitivity.
机译:性攻击样本是法医分析中遇到的一些最常见的样本。由于差分提取过程,这些样品可能需要大量的投资。我们报告了针对STR分析的精液成功直接扩增的第一次记录。用直接方法成功扩增了整齐的精液,从1:5至1:160和Gednap样品的稀释液。富含精子的温和差分分离技术被开发并成功地实施以分离并直接扩增精液和雌性上皮细胞的混合物。用差动分离方案进行的样品的样品用氧毒素和曙红染色,用于精子评分。在PCR后染色的样品显示出完全缺乏完整的精子,证明在PCR工艺期间细胞裂解细胞。本文展示了在性侵犯的情况下掺入更快地获得结果并达到更高的敏感性的可能性。

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