首页> 外文期刊>Canadian journal of microbiology >Simplified reverse transcription polymerase chain reaction procedure with detection by microplate hybridization for routine screening of hepatitis A virus.
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Simplified reverse transcription polymerase chain reaction procedure with detection by microplate hybridization for routine screening of hepatitis A virus.

机译:简化的逆转录聚合酶链反应程序,通过微孔板杂交检测,用于常规筛查甲型肝炎病毒。

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摘要

Reverse transcription polymerase chain reaction, using either nested or seminested primers, is used extensively for the detection of viruses in small quantities. However, existing methods are prone to false positive reactions. We report here an improved polymerase chain reaction technique based on the use of longer primers (39 nucleotides) with single-step amplification, applied to the detection of hepatitis A in low quantities. While the sensitivity of this technique (10 x the 50% tissue culture infective dose) is equivalent to that of existing methods, it is a simpler procedure, less time consuming, and less susceptible to contamination and therefore provides a more reliable tool for routine diagnosis. Finally, the development of a DNA enzyme immunoassay detection technique and the complete automation of the procedure allow a large number of samples to be processed in clinical laboratories.
机译:使用嵌套或晶的引物的逆转录聚合酶链反应广泛用于以少量检测病毒。 然而,现有方法容易发生误阳性反应。 在此报告基于使用具有单步扩增的更长引物(39个核苷酸)的改进的聚合酶链反应技术,其应用于甲型肝炎的低量。 虽然这种技术的敏感性(10 x 50%组织培养剂量)等同于现有方法的敏感性,但它是一种更简单的程序,耗时较少,较少易受污染的措施,因此为常规诊断提供更可靠的工具 。 最后,DNA酶免疫测定检测技术的发展和程序的完全自动化允许在临床实验室中加工大量样品。

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