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An Optimized Real-Time PCR to Avoid Species-/Tissue-Associated Inhibition for H5N1 Detection in Ferret and Monkey Tissues

机译:一种优化的实时PCR可避免在雪貂和猴子组织中检测H5N1的物种/组织相关抑制

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摘要

The real-time PCR diagnostics for avian influenza virus H5N1 in tissue specimens are often suboptimal, since naturally occurring PCR inhibitors present in samples, or unanticipated match of primer to unsequenced species' genome. With the principal aim of optimizing the SYBR Green real-time PCR method for detecting H5N1 in ferret and monkey (Chinese rhesus macaque) tissue specimens, we screened various H5N1 gene-specific primer pairs and tested their ability to sensitively and specifically detect H5N1 transcripts in the infected animal tissues, then we assessed RNA yield and quality by comparing Ct values obtained from the standard Trizol method, and four commonly used RNA isolation kits with small modifications, including Roche High Pure, Ambion RNAqueous, BioMIGA EZgene, and Qiagen RNeasy. The results indicated that a single primer pair exhibited high specificity and sensitivity for H5N1 transcripts in ferret and monkey tissues. Each of the four kits and Trizol reagent produced high-quality RNA and removed all or nearly all PCR inhibitors. No statistically significant differences were found between the Ct values from the isolation methods. So the optimized SYBR Green real-time PCR could avoid species- or tissue-associated PCR inhibition in detecting H5N1 in ferret and monkey tissues, including lung and small intestine.
机译:组织样本中禽流感病毒H5N1的实时PCR诊断通常不理想,因为样品中存在天然存在的PCR抑制剂,或者引物与未测序物种的基因组发生意外匹配。为了优化SYBR Green实时PCR方法以检测雪貂和猴子(猕猴)组织标本中的H5N1,我们筛选了各种H5N1基因特异性引物对,并测试了它们对H5N1转录本敏感和特异检测的能力。感染的动物组织,然后我们通过比较从标准Trizol方法获得的Ct值和四种经过细微修改的常用RNA分离试剂盒来评估RNA的产量和质量,其中包括Roche High Pure,Ambion RNAqueous,BioMIGA EZgene和Qiagen RNeasy。结果表明,单个引物对雪貂和猴子组织中的H5N1转录本表现出高特异性和敏感性。四种试剂盒和Trizol试剂均产生高质量的RNA,并去除了全部或几乎所有的PCR抑制剂。隔离方法的Ct值之间未发现统计学上的显着差异。因此,优化的SYBR Green实时PCR可以避免检测雪貂和猴子组织(包括肺和小肠)中的H5N1,从而避免物种或组织相关的PCR抑制。

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