Rattanamas Khate, Taesuji Machimaporn, Kulthonggate Usakorn, Jantafong Tippawan, Mamom Thanongsak, Ruenphet Sakchai
Master of Science Program in Animal Biotechnology, Faculty of Veterinary Medicine, Mahanakorn University of Technology, Bangkok, Thailand.
Clinic for Horse, Faculty of Veterinary Medicine, Mahanakorn University of Technology, Bangkok, Thailand.
Vet World. 2022 Nov;15(11):2754-2759. doi: 10.14202/vetworld.2022.2754-2759. Epub 2022 Nov 30.
The flinders technology associates (FTA) card is a cotton-based cellulose membrane impregnated with a chaotropic agent that inactivates infectious microorganisms, lyses cellular material, and fixes DNA and/or RNA within the fiber matrix. However, little is known about the effectiveness of these cards for detecting RNA viruses in animals. This study aimed to evaluate the sensitivity of RNA virus detection using conventional reverse-transcription polymerase chain reaction (RT-PCR) on FTA cards.
A highly virulent Newcastle disease virus (NDV) and an avian influenza virus (AIV) with low pathogenicity were propagated using chicken embryonic eggs. Three days after inoculation, the allantoic fluid was harvested, stored at -80°C, and the stock virus was tested for virus titration. African horse sickness virus (AHSV) was obtained from a live attenuated vaccine that was dissolved and stored at -80°C. For sample preparation, each stock virus was 10-fold serially diluted and each dilution was inoculated onto an FTA card, followed by drying in a Class II safety cabinet. Both the stock virus and infected FTA card were genomically isolated using an extraction kit, FTA purification kit, and extraction kit with Tris-EDTA (TE) buffer. The target genome was then detected by one-step RT-PCR for NDV and AIV, and two-step RT-PCR for African horse sickness, including gel electrophoresis for the detection of specific nucleic acids.
The detection limit of stock AIV was compared on FTA cards, using the FTA purification kit, and with TE buffer with an extraction kit. The corresponding results were 1.47, 1.17, and 2.18 log EID, respectively, while for NDV the results were 4.13, 4.83, and 4.84 log ELD. Finally, detection limit of stock AHSV and AHSV on the FTA card extracted using TE buffer with an extraction kit were 4.30 and 4.01 log plaque-forming units, respectively.
This study demonstrated that the detection limit or sensitivity of all tested RNA viruses on FTA cards did not differ when compared with those of the stock virus and in both methods for RNA isolation on FTA cards. These cards are suitable for collecting and transporting samples infected with RNA viruses, particularly AIV, NDV, and AHSV. Flinders technology associates cards also provide hazard-free samples, a reliable source of RNA for molecular characterization, and sufficient quantity for diagnostic applications based on nucleic acid-based detection.
弗林德斯技术协会(FTA)卡是一种浸有离液剂的棉质纤维素膜,该离液剂可使感染性微生物失活、裂解细胞物质,并将DNA和/或RNA固定在纤维基质中。然而,关于这些卡在检测动物RNA病毒方面的有效性知之甚少。本研究旨在评估使用传统逆转录聚合酶链反应(RT-PCR)在FTA卡上检测RNA病毒的灵敏度。
使用鸡胚繁殖高致病性新城疫病毒(NDV)和低致病性禽流感病毒(AIV)。接种三天后,收集尿囊液,储存在-80°C,对储备病毒进行病毒滴定检测。非洲马瘟病毒(AHSV)获自一种减毒活疫苗,将其溶解并储存在-80°C。对于样品制备,将每种储备病毒进行10倍系列稀释,每种稀释液接种到一张FTA卡上,然后在二级安全柜中干燥。使用提取试剂盒、FTA纯化试剂盒以及含Tris-EDTA(TE)缓冲液的提取试剂盒对储备病毒和感染的FTA卡进行基因组分离。然后通过针对NDV和AIV的一步法RT-PCR以及针对非洲马瘟的两步法RT-PCR检测目标基因组,包括用于检测特定核酸的凝胶电泳。
在FTA卡上、使用FTA纯化试剂盒以及使用含提取试剂盒的TE缓冲液比较了储备AIV的检测限。相应结果分别为1.47、1.17和2.18 log EID,而对于NDV,结果分别为4.13、4.83和4.84 log ELD。最后,使用含提取试剂盒的TE缓冲液从FTA卡上提取的储备AHSV和AHSV的检测限分别为4.30和4.01 log蚀斑形成单位。
本研究表明,与储备病毒相比,以及在FTA卡上的两种RNA分离方法中,所有测试的RNA病毒在FTA卡上的检测限或灵敏度均无差异。这些卡适用于收集和运输感染RNA病毒的样品,特别是AIV、NDV和AHSV。弗林德斯技术协会卡还提供无危害的样品、用于分子特征分析的可靠RNA来源以及基于核酸检测的诊断应用所需的足够量。
Zotero 插件
