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结合多重多酶等温快速扩增、侧向流动试纸条和通用引物的生物样本简单且适用于现场的物种鉴定,用于无需标准PCR实验室的初始快速筛查。

Simple and field-adapted species identification of biological specimens combining multiplex multienzyme isothermal rapid amplification, lateral flow dipsticks, and universal primers for initial rapid screening without standard PCR laboratory.

作者信息

Sun Mao-Ling, Yang Ying, Hu Ran, Li Jia-Lun, Liu Shu-Han, Chen Yun-Zhou, Wang Dong-Yi, Wang Lan, Li Yu-Zhang, Zhong Yang, Yao Jun, Li Xiao-Na

机构信息

School of Forensic Medicine, China Medical University, No. 77 Puhe Road, Shenbei New District, Shenyang, 110122, People's Republic of China.

Key Laboratory of Forensic Bio-Evidence Sciences, Liaoning Province, Shenyang, People's Republic of China.

出版信息

Int J Legal Med. 2024 Mar;138(2):561-570. doi: 10.1007/s00414-023-03101-2. Epub 2023 Oct 6.

DOI:10.1007/s00414-023-03101-2
PMID:37801116
Abstract

Species identification of biological specimens can provide the valuable clues and accelerate the speed of prosecution material processing for forensic investigation, especially when the case scene is inaccessible and the physical evidence is cumbersome. Thus, establishing a rapid, simple, and field-adapted species identification method is crucial for forensic scientists, particularly as first-line technology at the crime scene for initial rapid screening. In this study, we established a new field-adapted species identification method by combining multiplex multienzyme isothermal rapid amplification (MIRA), lateral flow dipstick (LFD) system, and universal primers. Universal primers targeting COX I and COX II genes were used in multiplex MIRA-LFD system for seven species identification, and a dedicated MIRA-LFD system primer targeting CYT B gene was used to detect the human material. DNA extraction was performed by collecting DNA directly from the centrifuged supernatant. Our study found that the entire amplification process took only 15 min at 37 °C and the results of LFDs could be visually observed after 10 min. The detection sensitivity of human material could reach 10 pg, which is equivalent to the detection of single cell. Different common animal samples mixed at the ratio of 1 ng:1 ng, 10 ng:1 ng, and 1 ng:10 ng could be detected successfully. Furthermore, the damaged and degraded samples could also be detected. Therefore, the convenient, feasible, and rapid approach for species identification is suitable for popularization as first-line technology at the crime scene for initial rapid screening and provides a great convenient for forensic application.

摘要

生物样本的物种鉴定可为法医调查提供有价值的线索,并加快检材处理速度,尤其是在案发现场无法进入且物证繁杂的情况下。因此,建立一种快速、简便且适用于现场的物种鉴定方法对法医科学家至关重要,特别是作为犯罪现场的一线技术用于初步快速筛查。在本研究中,我们通过结合多重多酶等温快速扩增(MIRA)、侧向流动试纸条(LFD)系统和通用引物,建立了一种新的适用于现场的物种鉴定方法。针对COX I和COX II基因的通用引物用于多重MIRA-LFD系统以鉴定七种物种,而针对CYT B基因的专用MIRA-LFD系统引物用于检测人类样本。通过直接从离心后的上清液中收集DNA进行DNA提取。我们的研究发现,整个扩增过程在37℃下仅需15分钟,10分钟后即可肉眼观察到LFD的结果。人类样本的检测灵敏度可达10 pg,相当于单细胞检测。以1 ng:1 ng、10 ng:1 ng和1 ng:10 ng的比例混合的不同常见动物样本均可成功检测。此外,受损和降解的样本也能被检测到。因此,这种方便、可行且快速的物种鉴定方法适合作为犯罪现场的一线技术进行推广,用于初步快速筛查,为法医应用提供了极大便利。

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2
Development of a multienzyme isothermal rapid amplification and lateral flow dipstick combination assay for bovine coronavirus detection.用于牛冠状病毒检测的多酶等温快速扩增与侧向流动试纸条联合检测方法的开发。
Front Vet Sci. 2023 Jan 4;9:1059934. doi: 10.3389/fvets.2022.1059934. eCollection 2022.
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Development and evaluation of a rapid and sensitive multienzyme isothermal rapid amplification with a lateral flow dipstick assay for detection of in spiked blood specimens.
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