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基于CRISPR/Cas12a的临床标本中HR-HPV快速检测及基因分型诊断试验的开发与评估

Development and evaluation of a CRISPR/Cas12a-based diagnostic test for rapid detection and genotyping of HR-HPV in clinical specimens.

作者信息

Yin Lijuan, Zhao Ziqian, Wang Chunhua, Zhou Caihong, Wu Xiuzhen, Gao Baoxue, Wang Liangyuan, Man Shuli, Cheng Xinkuan, Wu Qiankun, Hu Siqi, Fan Hongxia, Ma Long, Xing Hui, Shen Liang

机构信息

State Key Laboratory of Food Nutrition and Safety, Key Laboratory of Industrial Microbiology, Ministry of Education, Tianjin Key Laboratory of Industry Microbiology, National and Local United Engineering Lab of Metabolic Control Fermentation Technology, China International Science and Technology Cooperation Base of Food Nutrition/Safety and Medicinal Chemistry, College of Biotechnology, Tianjin University of Science & Technology, Tianjin, China.

Department of Clinical Laboratory, Xiangyang Central Hospital, Affiliated Hospital of Hubei University of Arts and Science, Xiangyang, Hubei Province, China.

出版信息

Microbiol Spectr. 2025 Jan 7;13(1):e0225324. doi: 10.1128/spectrum.02253-24. Epub 2024 Nov 21.

Abstract

Persistent infection with high-risk human papillomavirus (HR-HPV) is the principal etiological factor of cervical cancer. Considering the gradual progression of cervical cancer, the early, rapid, sensitive, and specific identification of HPV, particularly HR-HPV types, is crucial in halting the advancement of the illness. Here, we established a rapid, highly sensitive, and specific HR-HPV detection platform, leveraging the CRISPR/Cas12a assay in conjunction with multienzyme isothermal rapid amplification. Our platform enables the detection and genotyping of 14 types of HR-HPV by using type-specific crRNAs. The outcomes of the detection can be interpreted either through a fluorescence reader or visually. Furthermore, we achieved one-tube multiplex detection of 14 HR-HPV types through the use of multiple amplifications and a crRNA pool. The detection sensitivity of this method is 2 copies/μL with no cross-reactivity, and the results can be obtained within 30 minutes. This method exhibited 100% clinical sensitivity and 100% clinical specificity when applied to 258 clinical specimens. Based on these findings, our CRISPR/Cas-based HR-HPV detection platform holds promise as a novel clinical detection tool, offering a visually intuitive and expedited alternative to existing HPV infection diagnostics and providing fresh perspectives for clinical cervical cancer screening.IMPORTANCEThis study developed a novel high-risk human papillomavirus (HR-HPV) detection platform based on CRISPR/Cas12a technology. This platform not only enables the rapid, highly sensitive, and specific detection and genotyping of 14 types of HR-HPV but also achieves single-tube multiplex detection of 14 HR-HPV types through ingenious design. The outcomes of the detection can be interpreted either through a fluorescence reader or visually. To the best of our knowledge, this is the first paper to utilize CRISPR/Cas diagnostic technology for the simultaneous detection of 14 types of HPV and to evaluate its feasibility in clinical sample detection using a large number of clinical samples. We hope that this work will facilitate the rapid and accurate detection of HPV and promote the broader application of CRISPR/Cas diagnostic technology.

摘要

高危型人乳头瘤病毒(HR-HPV)的持续感染是宫颈癌的主要病因。鉴于宫颈癌的渐进性发展,早期、快速、灵敏且特异的HPV检测,尤其是HR-HPV类型的检测,对于阻止病情进展至关重要。在此,我们利用CRISPR/Cas12a检测法结合多酶等温快速扩增技术,建立了一个快速、高度灵敏且特异的HR-HPV检测平台。我们的平台通过使用型特异性crRNA能够检测14种HR-HPV类型并进行基因分型。检测结果既可以通过荧光读数仪解读,也可以直观地解读。此外,我们通过多次扩增和crRNA池实现了14种HR-HPV类型的一管多重检测。该方法的检测灵敏度为2拷贝/μL,无交叉反应,且可在30分钟内获得结果。当应用于258份临床标本时,该方法表现出100%的临床灵敏度和100%的临床特异性。基于这些发现,我们基于CRISPR的HR-HPV检测平台有望成为一种新型临床检测工具,为现有的HPV感染诊断提供直观且快速的替代方法,并为临床宫颈癌筛查提供新的视角。

重要性

本研究基于CRISPR/Cas12a技术开发了一种新型高危型人乳头瘤病毒(HR-HPV)检测平台。该平台不仅能够对14种HR-HPV类型进行快速、高度灵敏且特异的检测和基因分型,还通过巧妙设计实现了14种HR-HPV类型的单管多重检测。检测结果既可以通过荧光读数仪解读,也可以直观地解读。据我们所知,这是第一篇利用CRISPR/Cas诊断技术同时检测14种HPV类型并使用大量临床样本评估其在临床样本检测中可行性的论文。我们希望这项工作将有助于HPV的快速准确检测,并推动CRISPR/Cas诊断技术的更广泛应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/20cd/11705848/b7770520060e/spectrum.02253-24.f001.jpg

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