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基于CRISPR-Cas13a纳米机器的甲型禽流感(H7N9)病毒现场检测简易技术

CRISPR-Cas13a Nanomachine Based Simple Technology for Avian Influenza A (H7N9) Virus On-Site Detection.

作者信息

Liu Yufeng, Xu Hongpan, Liu Chang, Peng Lijun, Khan Haroon, Cui Lunbiao, Huang Rui, Wu Chao, Shen Sisi, Wang Su, Liang Wenbiao, Li Zhiyang, Xu Benbo, He Nongyue

出版信息

J Biomed Nanotechnol. 2019 Apr 1;15(4):790-798. doi: 10.1166/jbn.2019.2742.

DOI:10.1166/jbn.2019.2742
PMID:30841971
Abstract

It is urgent to find an avian influenza A H7N9 detection simple method which is suitable for on-site detection. The Cas13a protein just likes a nanomachine, when specifically bound to target RNA by single-stranded RNA (crRNA), changes its protein structure and produces RNase activity, which degrades RNA non-specifically. Harnessing Cas13a, the paper aims to establish an underlying on-site H7N9 virus nucleic acid detection method. LwCas13a protein nanomachine was expressed in a prokaryotic expression system and purified by nickel column. transcribed RNA of H7N9 HA gene has been used as a target, to design a specific crRNA. The activity of Cas13a was verified with a single-stranded RNA-bound fluorescent group and a quenching fluorophore as signals. Using Cas13a, a room temperature H7N9 detection system was established. Detection of 1 nm of single-stranded RNA can be done within 5 min. When combined with the RT-RPA and T7 transcription system at room temperature, the detection limits of HA and NA are 1 fM and the reaction time is 50 min. Excellent specificity was achieved by comparison with subtype viruses such as H1N1 and H5N1. The rapid detection method based on CRISPR-Cas13a nanomachine H7N9 has been successfully established, which can detect H7N9 quickly and specifically. In the future, it can be quickly detected in the field with portable fluorescence detector.

摘要

寻找一种适用于现场检测的甲型H7N9禽流感检测简便方法迫在眉睫。Cas13a蛋白就像一台纳米机器,当通过单链RNA(crRNA)与靶RNA特异性结合时,会改变其蛋白质结构并产生核糖核酸酶活性,从而非特异性地降解RNA。利用Cas13a,本文旨在建立一种潜在的现场H7N9病毒核酸检测方法。LwCas13a蛋白纳米机器在原核表达系统中表达并通过镍柱纯化。以H7N9 HA基因的转录RNA为靶标,设计特异性crRNA。以结合有荧光基团的单链RNA和淬灭荧光团作为信号验证Cas13a的活性。利用Cas13a建立了室温下的H7N9检测系统。5分钟内可完成对1 nM单链RNA的检测。在室温下与RT-RPA和T7转录系统结合时,HA和NA的检测限为1 fM,反应时间为50分钟。通过与H1N1和H5N1等亚型病毒比较,实现了优异的特异性。基于CRISPR-Cas13a纳米机器的H7N9快速检测方法已成功建立,可快速、特异性地检测H7N9。未来,可使用便携式荧光检测仪在现场进行快速检测。

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