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首页> 外文期刊>Diseases of Aquatic Organisms >Development and evaluation of a one-step real-time reverse transcription polymerase chain reaction assay for the detection of salmonid alphaviruses in serum and tissues
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Development and evaluation of a one-step real-time reverse transcription polymerase chain reaction assay for the detection of salmonid alphaviruses in serum and tissues

机译:开发和评估用于检测血清和组织中鲑鱼甲型病毒的一步实时逆转录聚合酶链反应测定法

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摘要

We designed 4 primer pairs to amplify conserved regions of the E1 or nsP4 genes of salmonid alphavirus (SAV) and evaluated their performance in optimized 1-step SYBR green real-time RT-PCR (RRT-PCR) assays. A single primer pair, amplifying a 227 bp segment of E1 was then chosen for further study. This RRT-PCR was shown to be highly repeatable and reproducible over a wide range of RNA dilutions, with a linear relationship between cycle threshold (Ct) value and RNA concentration over a 10(7) dilution range. The limit of detection was calculated to be < or = 1.5 TCID50 ml(-1). When applied to sera previously screened by virus isolation for SAV viraemia, the RRT-PCR correctly identified all 13 culture-positive samples, as well as finding an additional 28 sera positive. Relative semi-quantitation of sera showed a very highly significant relationship between copy number and TCID50 (p < 0.001, R2 = 0.9563). Following experimental infection of salmon, heart samples were consistently positive until 21 d post infection (dpi), with (weak) positive signals still detectable in 50% of fish 70 dpi.
机译:我们设计了4对引物,以扩增鲑鱼甲病毒(SAV)的E1或nsP4基因的保守区,并在优化的1步SYBR绿色实时RT-PCR(RRT-PCR)分析中评估了它们的性能。然后选择单个引物对,扩增E1的227 bp片段进行进一步研究。该RRT-PCR在广泛的RNA稀释范围内显示出高度可重复性和可重复性,在10(7)稀释范围内循环阈值(Ct)值与RNA浓度之间具有线性关系。计算的检出限为<或= 1.5 TCID50 ml(-1)。当将RRT-PCR应用于先前通过病毒分离筛选出的SAV病毒血症的血清时,可以正确鉴定所有13个培养阳性样品,并另外发现28个阳性血清。血清的相对半定量显示拷贝数与TCID50之间的关系非常显着(p <0.001,R2 = 0.9563)。鲑鱼经过实验性感染后,心脏样品在感染后(dpi)直到21 d一直都是阳性的,在50 dpi的70 dpi鱼中仍可检测到(弱)阳性信号。

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