[一种用于快速检测的荧光重组酶辅助扩增/CRISPR-Cas12a系统的建立及初步评估] (原文中检测对象缺失)
[Establishment and preliminary evaluation of a fluorescent recombinase-aided amplification/CRISPR-Cas12a system for rapid detection of ].
作者信息
Huang W, Wei H, Wang C, Wang J, Chen L, Chen W, Liu Y, Zheng Y, Lin M
机构信息
School of Laboratory Medicine, Youjiang Medical University for Nationalities, Baise, Guangxi 533000, China.
Department of Laboratory Medicine, The Affiliated Hospital of Youjiang Medical University for Nationalities, Baise, Guangxi 533000, China.
出版信息
Zhongguo Xue Xi Chong Bing Fang Zhi Za Zhi. 2023 Mar 13;35(1):38-43. doi: 10.16250/j.32.1374.2022240.
OBJECTIVE
To establish a fluorescent assay for rapid detection of based on recombinaseaided amplification (RAA) and CRISPR-Cas12a system,and to preliminarily evaluate the diagnostic efficiency of this system.
METHODS
The ribosomal RNA () gene of was selected as the target sequence, and three pairs of RAA primers and CRISPR-derived RNA (crRNA) were designed and synthesized. The optimal combination of RAA primers and crRNA was screened and the reaction conditions of the system were optimized to create a fluorescent RAA/CRISPR-Cas12a system. The plasmid containing gene of the strain 3D7 was generated, and diluted into concentrations of 1 000, 100, 10, 1 copy/μL for the fluorescent RAA/CRISPR-Cas12a assay, and its sensitivity was evaluated. The genomic DNA from , , , hepatitis B virus, human immunodeficiency virus and was employed as templates for the fluorescent RAA/CRISPR-Cas12a assay, and its specificity was evaluated. Fifty malaria clinical samples were subjected to the fluorescent RAA/CRISPR-Cas12a assay and nested PCR assay, and the consistency between two assays was compared. In addition, strain 3D7 was cultured . Then, the culture was diluted into blood samples with parasite densities of 1 000, 500, 200, 50, 10 parasites/μL with healthy volunteers' O-positive red blood cells for the RAA/CRISPR-Cas12a assay, and the detection efficiency was tested.
RESULTS
The Pf-F3/Pf-R3/crRNA2 combination, 2.5 μL as the addition amount of B buffer, 40 min as the RAA reaction time, 37 °C as the reaction temperature of the CRISPR-Cas12a system were employed to establish the fluorescent RAA/CRISPR-Cas12a system. Such a system was effective to detect the plasmid containing gene of the strain 3D7 at a concentration of 1 copy/μL, and presented fluorescent signals for detection of , but failed to detect , , , , hepatitis B virus or human immunodeficiency virus. The fluorescent RAA/CRISPR-Cas12a system and nested PCR assay showed completely consistent results for detection of 50 malaria clinical samples ( = 1.0, < 0.001). Following 6-day culture of the strain 3D7, 10 mL cultures were generated and the fluorescent RAA/CRISPR-Cas12a system showed the minimal detection limit of 50 parasites/μL.
CONCLUSIONS
The fluorescent RAA/CRISPR-Cas12a system is rapid, sensitive and specific for detection of , which shows promising value for rapid detection and risk monitoring of .
目的
建立一种基于重组酶辅助扩增(RAA)和CRISPR-Cas12a系统的荧光检测方法,用于快速检测疟原虫,并初步评估该系统的诊断效率。
方法
选择疟原虫核糖体RNA(rRNA)基因作为靶序列,设计并合成三对RAA引物和CRISPR衍生RNA(crRNA)。筛选RAA引物和crRNA的最佳组合,优化系统反应条件,构建荧光RAA/CRISPR-Cas12a系统。构建含恶性疟原虫3D7株基因的质粒,并将其稀释成浓度为1000、100、10、1拷贝/μL,用于荧光RAA/CRISPR-Cas12a检测,评估其灵敏度。以间日疟原虫、卵形疟原虫、三日疟原虫、乙型肝炎病毒、人类免疫缺陷病毒及弓形虫的基因组DNA作为荧光RAA/CRISPR-Cas12a检测的模板,评估其特异性。对50份疟疾临床样本进行荧光RAA/CRISPR-Cas12a检测和巢式PCR检测,比较两种检测方法的一致性。此外,培养恶性疟原虫3D7株。然后,将培养物与健康志愿者的O型阳性红细胞稀释成疟原虫密度为1000、500、200、50、10个/μL的血样,进行RAA/CRISPR-Cas12a检测,测试其检测效率。
结果
采用Pf-F3/Pf-R3/crRNA2组合、2.5 μL作为B缓冲液添加量、40 min作为RAA反应时间、37℃作为CRISPR-Cas12a系统反应温度,构建荧光RAA/CRISPR-Cas12a系统。该系统能有效检测浓度为1拷贝/μL的含恶性疟原虫3D7株基因的质粒,检测恶性疟原虫时呈现荧光信号,但未能检测到间日疟原虫、卵形疟原虫、三日疟原虫、弓形虫、乙型肝炎病毒或人类免疫缺陷病毒。荧光RAA/CRISPR-Cas12a系统和巢式PCR检测对50份疟疾临床样本的检测结果完全一致(Kappa值=1.0,P<0.001)。恶性疟原虫3D7株培养6天后,获得10 mL培养物,荧光RAA/CRISPR-Cas12a系统的最低检测限为50个/μL。
结论
荧光RAA/CRISPR-Cas12a系统检测疟原虫具有快速、灵敏、特异的特点,在疟疾快速检测和风险监测方面具有良好的应用价值。
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