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通过逆转录环介导等温扩增技术对法医样本中的唾液进行检测和鉴定。

The detection and identification of saliva in forensic samples by RT-LAMP.

作者信息

Tsai Li-Chin, Su Chih-Wen, Lee James Chun-I, Lu Yu-Sheng, Chen Hsuan-Chen, Lin Yu-Chih, Linacre Adrian, Hsieh Hsing-Mei

机构信息

Department of Forensic Science, Central Police University, 56 Shu-Jen Road, Kwei-San, Taoyuan, 33304, Taiwan, Republic of China.

Forensic Biology Division, Criminal Investigation Bureau, National Police Administration, No.5 Lane 553, Sec. 4, Zhongxiao E. RD., Xinyi District, Taipei, 11072, Taiwan, Republic of China.

出版信息

Forensic Sci Med Pathol. 2018 Dec;14(4):469-477. doi: 10.1007/s12024-018-0008-5. Epub 2018 Jul 30.

DOI:10.1007/s12024-018-0008-5
PMID:30058014
Abstract

We report on a novel method for saliva identification by reverse transcription-loop-mediated isothermal amplification (RT-LAMP). In our previous report, real-time RT-LAMP was used for blood identification by using HBB detection as a model but in this advanced study, this method was refined for the identification of the more challenging body fluid of saliva. Expression of the18S rRNA gene was used as the internal control and the Statherin (STATH) gene as the saliva-specific marker. A turbidimeter was used for real-time detection of the RT-LAMP products, and confirmation was obtained that the real products were generated using: agarose gel electrophoresis, calcein fluorescence detection and/or enzymatic digestion. The specificity of the test was performed using 42 samples including 7 different body fluids, and the expression of STATH was only observed in all the saliva samples (6) with a threshold time of 39.4 ± 2.9 min. Sensitivity testing showed that RT-LAMP products for STATH were stably detected when the RNA template was not less than 6.25 ng. When the primer concentrations for STATH were two times that of 18S rRNA, saliva could be identified in the body fluid mixtures even at a ratio (saliva:semen) of 1:3 (without loop primer)/1:5 (with loop primer). A multiplex RT-LAMP was established to simultaneously amplify the 18S rRNA and STATH genes, and applied to the identification of saliva on ten non-probative cigarette butts. A positive result for saliva was obtained from all ten butts, even for those that returned a negative or ambiguous result using the amylase test. A direct RT-LAMP test is also reported where the RNA extraction step was omitted to speed the collection of data and all tests using either the simplex or multiplex RT-LAMP resulted in a positive response if saliva was present. Our data provide a simple and effective means to detect the presence of saliva.

摘要

我们报告了一种通过逆转录环介导等温扩增(RT-LAMP)进行唾液鉴定的新方法。在我们之前的报告中,以HBB检测为模型,使用实时RT-LAMP进行血液鉴定,但在这项深入研究中,该方法经过改进,用于鉴定更具挑战性的唾液体液。使用18S rRNA基因的表达作为内部对照,使用Statherin(STATH)基因作为唾液特异性标志物。使用浊度仪实时检测RT-LAMP产物,并通过琼脂糖凝胶电泳、钙黄绿素荧光检测和/或酶切确认产生了真实产物。使用包括7种不同体液的42个样本进行检测特异性,仅在所有唾液样本(6个)中观察到STATH的表达,阈值时间为39.4±2.9分钟。灵敏度测试表明,当RNA模板不少于6.25 ng时,可稳定检测到STATH的RT-LAMP产物。当STATH的引物浓度是18S rRNA的两倍时,即使在体液混合物中唾液比例为1:3(无环引物)/1:5(有环引物)(唾液:精液)时也能鉴定出唾液。建立了多重RT-LAMP以同时扩增18S rRNA和STATH基因,并应用于十个非证据性烟蒂上唾液的鉴定。所有十个烟蒂均获得唾液阳性结果,即使对于那些使用淀粉酶测试返回阴性或模糊结果的烟蒂也是如此。还报告了一种直接RT-LAMP测试,其中省略了RNA提取步骤以加快数据收集,并且如果存在唾液,使用单重或多重RT-LAMP的所有测试均产生阳性反应。我们的数据提供了一种简单有效的方法来检测唾液的存在。

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