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基于差异提取的雄性 DNA 分馏法推断法医样本中精子的存在。

Inferring the presence of spermatozoa in forensic samples based on male DNA fractionation following differential extraction.

机构信息

Centre of Forensic Sciences, Biology Section, 25 Morton Shulman Avenue, Toronto, Ontario M3M 0B1, Canada.

Centre of Forensic Science, Royal College Building, University of Strathclyde, 204 George Street, Glasgow, Scotland G1 1XW, United Kingdom.

出版信息

Forensic Sci Int Genet. 2018 Sep;36:225-232. doi: 10.1016/j.fsigen.2018.06.014. Epub 2018 Jul 9.

Abstract

To address sexual assault kit backlogs some laboratories in North America have implemented 'Direct to DNA' (DTD) approaches for the examination of relevant vaginal, oral, rectal and external genitalia swabs from sexual assault examination kits. Using this approach no preliminary serological screening for semen or spermatozoa is performed. Instead, swabs are directly subjected to differential extraction and quantitation using a dual quantification system. Decisions regarding the next steps in processing each sample are typically based on the quantity of male DNA detected, the fraction in which it is detected, and its ratio to the total human DNA in the sample. In the absence of serological results it remains of value in many cases to determine whether spermatozoa are present in the sample and whether the male DNA profile may be attributed to this body fluid. In this study we examine the distribution of male DNA from various body fluids between epithelial and spermatozoa fractions following differential extraction. Based on these results we identified criteria under which a DNA profile can be reliably attributed to spermatozoa. A total of 18 blood samples, 129 saliva samples, and 78 semen samples were processed. The maximum amount of male DNA observed in the sperm fraction of a spermatozoa-free sample was 10.4 ng and the maximum portion of total male DNA observed in the sperm fraction was 7.7%. In contrast, when a sample contained spermatozoa the minimum portion of total male DNA observed in the sperm fraction was 52.6%. This research supports a 50% threshold of male DNA in the sperm fraction following differential extraction as a conservative criterion under which the scientist at the Centre of Forensic Sciences (CFS) may infer that spermatozoa is present in a sample in the absence of serological results. This general threshold is applicable to all sample types (underwear, clothing, swabs, condoms) tested. We further demonstrate that, if the same male DNA profile is represented more prominently in the sperm fraction versus the epithelial fraction, the analyst should not fall into the intuitive trap of inferring the presence of spermatozoa in the sample. Instead, enrichment calculations must be based on the measured quantity of male and total DNA in each fraction and not the male:female DNA ratios observed in the DNA profiles.

摘要

为了解决性侵犯工具包积压的问题,北美的一些实验室已经实施了“直接到 DNA”(DTD)方法,用于检查性侵犯检查工具包中相关的阴道、口腔、直肠和外生殖器拭子。使用这种方法,不会对精液或精子进行初步的血清学筛查。相反,拭子直接使用双定量系统进行差异提取和定量。处理每个样本的下一步决策通常基于检测到的男性 DNA 的数量、检测到的部分及其与样本中总人类 DNA 的比例。在没有血清学结果的情况下,确定样本中是否存在精子以及男性 DNA 图谱是否归因于这种体液,在许多情况下仍然具有价值。在这项研究中,我们检查了差异提取后各种体液中的男性 DNA 在上皮细胞和精子部分之间的分布。基于这些结果,我们确定了可以可靠地将 DNA 图谱归因于精子的标准。共处理了 18 份血液样本、129 份唾液样本和 78 份精液样本。在没有精子的样本的精子部分观察到的最大男性 DNA 量为 10.4ng,在精子部分观察到的总男性 DNA 的最大部分为 7.7%。相比之下,当样本中含有精子时,在精子部分观察到的总男性 DNA 的最小部分为 52.6%。这项研究支持在差异提取后,精子部分的男性 DNA 含量达到 50%作为一个保守标准,在没有血清学结果的情况下,法医学中心的科学家可以据此推断样本中存在精子。这个一般标准适用于所有测试的样本类型(内衣、衣物、拭子、避孕套)。我们进一步证明,如果相同的男性 DNA 图谱在精子部分比上皮部分更突出,分析师不应陷入推断样本中存在精子的直观陷阱。相反,富集计算必须基于每个部分中测量到的男性和总 DNA 量,而不是 DNA 图谱中观察到的男性:女性 DNA 比值。

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