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Comparison of the NucliSens Basic Kit (Nucleic Acid Sequence-Based Amplification) and the Argene Biosoft Enterovirus Consensus Reverse Transcription-PCR Assays for Rapid Detection of Enterovirus RNA in Clinical Specimens

机译:NucliSens基本试剂盒(基于核酸序列的扩增)和Argene Biosoft肠病毒共识逆转录PCR方法在临床标本中快速检测肠病毒RNA的比较

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摘要

Samples were tested for enterovirus by nucleic acid sequence-based amplification (NASBA) (NucliSens Basic kit; BioMerieux), reverse transcription-PCR (RT-PCR) (Enterovirus Consensus RT-PCR kit; Argene Biosoft), and virus isolation. Eighty-two samples were tested, and 44 were positive, 34 by both NASBA and RT-PCR and 5 each by NASBA or RT-PCR only. Two nasopharyngeal samples positive only by RT-PCR were determined to be rhinovirus. Of 42 enterovirus-positive samples, NASBA detected 39 (92.9%) and RT-PCR detected 37 (88.1%). The NucliSens Basic kit and the Argene Biosoft RT-PCR had comparable sensitivities for detection of enterovirus RNA, and both molecular methods were more sensitive than culture, which detected only 60.5% of positive samples. NASBA could be completed in 6.5 h versus 9 h for the Argene Biosoft RT-PCR kit.
机译:通过基于核酸序列的扩增(NASBA)(NucliSens Basic试剂盒; BioMerieux),逆转录PCR(RT-PCR)(肠病毒共识RT-PCR试剂盒; Argene Biosoft)和病毒分离测试了样品中的肠道病毒。测试了82个样品,其中44个为阳性,仅通过NASBA和RT-PCR分别为34个,仅通过NASBA或RT-PCR分别为5个。仅通过RT-PCR阳性的两个鼻咽样品被确定为鼻病毒。在42个肠病毒阳性样本中,NASBA检测到39个(92.9%),RT-PCR检测到37个(88.1%)。 NucliSens Basic试剂盒和Argene Biosoft RT-PCR在检测肠道病毒RNA方面具有可比的敏感性,并且两种分子方法都比培养更为灵敏,后者仅检测到阳性样本的60.5%。 NASBA可以在6.5小时内完成,而Argene Biosoft RT-PCR试剂盒则需要9小时。

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