Lin Yu-Chih, Tsai Li-Chin, Liu Kuo-Lan, Huang Nu-En, Yang Lih-Jing, Su Chih-Wen, Lee James Chun-I, Linacre Adrian, Hsieh Hsing-Mei
Taichung City Government Police Department, No.500 Fengxing Road Section 1, Tanzi District, Taichung City, 427003, Taiwan, Republic of China.
Department of Forensic Science, Central Police University, 56 Shu-Jen Road, Kwei-San, Taoyuan, 33304, Taiwan, Republic of China.
Int J Legal Med. 2022 Jan;136(1):73-84. doi: 10.1007/s00414-021-02723-8. Epub 2021 Oct 29.
In alleged sexual assault cases, identification of the presence of spermatozoa at the crime scene, or on items of eventual significance, or associated with the body of the victim, is integral to the forensic investigation to support or refute the proposition that sexual act has occurred. A 3-plex MSRE-PCR (methylation-sensitive restriction enzyme-PCR) system has been developed previously to identify spermatozoa based on the presence or absence of DNA methylation. This assay showed that 0.1 ng of DNA from a semen extract was sufficient to identify the presence of spermatozoa even when there was excessively more DNA isolated from vaginal fluid than DNA from a semen extract (80 ng/0.1 ng) or a mix of the menstrual blood/semen DNA (5 ng/0.1 ng). In this study, we combine spermatozoa detection with co-amplification of 23 Y-STR loci. We perform standard validation steps to present a novel test that saves time and uses the same sample for both DNA typing and spermatozoa detection in the same reaction. The combined assay can identify Y-STR and spermatozoa simultaneously using just 0.1 ng semen DNA, even in the presence of 5 ng of DNA from a female (male/female:1/50). No other body fluid tested, such as saliva, gave a result for the presence of spermatozoa. A total of 9 non-probative forensic samples from 7 sexual assault cases were tested by this co-amplification system. In all cases, the same sperm-positive data were obtained, concordant with our previous study analyzed by only 3-plex MSRE-PCR, and the Y-STR results were also consistent with that analyzed by only PowerPlex® Y23 kit. The co-amplification will be beneficial for the limited samples in many criminal cases.
在涉嫌性侵犯案件中,在犯罪现场、或最终具有重要意义的物品上、或与受害者身体相关处鉴定出精子的存在,对于支持或反驳性行为已经发生这一论点的法医调查至关重要。此前已开发出一种三重MSRE-PCR(甲基化敏感限制性内切酶-PCR)系统,用于根据DNA甲基化的有无来鉴定精子。该检测方法表明,即使从阴道液中分离出的DNA比从精液提取物中分离出的DNA多得多(80 ng/0.1 ng),或者是月经血/精液DNA混合物(5 ng/0.1 ng),0.1 ng精液提取物中的DNA也足以鉴定出精子的存在。在本研究中,我们将精子检测与23个Y-STR基因座的共扩增相结合。我们执行标准验证步骤,以呈现一种新颖的检测方法,该方法节省时间,并且在同一反应中使用相同样本进行DNA分型和精子检测。这种联合检测方法仅使用0.1 ng精液DNA就能同时鉴定Y-STR和精子,即使存在5 ng女性DNA(男性/女性:1/50)时也是如此。所检测的其他体液,如唾液,均未得出存在精子的结果。通过这种共扩增系统对来自7起性侵犯案件的9份非验证性法医样本进行了检测。在所有案例中,均获得了相同的精子阳性数据,与我们之前仅通过三重MSRE-PCR分析的研究结果一致,并且Y-STR结果也与仅通过PowerPlex® Y23试剂盒分析的结果一致。这种共扩增方法将有利于许多刑事案件中有限样本的检测。
