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首页> 外文期刊>Journal of Clinical Microbiology >Detection of adenovirus in clinical specimens by polymerase chain reaction and liquid-phase hybridization quantitated by time-resolved fluorometry.
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Detection of adenovirus in clinical specimens by polymerase chain reaction and liquid-phase hybridization quantitated by time-resolved fluorometry.

机译:通过聚合酶链反应和时间分辨荧光定量液相杂交技术检测临床标本中的腺病毒。

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In addition to tests for the group-specific hexon antigen of adenoviruses, adenoviruses can be detected in clinical specimens by hybridization assays utilizing the widely shared base sequences of the region of the hexon gene that codes for the group-reactive determinants. We have developed a liquid-phase hybridization system with biotin- and europium-labeled probes which are reacted after DNA amplification of a 161-bp region of the hexon gene and which are quantitated by time-resolved (TR) fluorometry in streptavidin-coated microtiter wells. Polymerase chain reaction (PCR)-TR fluorometry is not a rapid test in the usual sense, but it is highly useful for specimens with inherent toxicity or with low virus yield, such as organ minces and specimens obtained late in the course of an illness. In a survey of 103 specimens tested by this method, including urine, stool, and tissue suspensions, the agreement with the hexon-specific TR fluoroimmunoassay antigen test for positive specimens was 100% and the sensitivity compared with that of virus culture was 91%. The PCR-TR fluorometry system was also shown to be advantageous as a quantitative measure of PCR products.
机译:除了测试腺病毒的特定组六邻体抗原外,还可以利用六邻体基因编码组反应性决定簇的广泛共享碱基序列,通过杂交测定法在临床标本中检测腺病毒。我们已经开发了一种具有生物素和euro标记探针的液相杂交系统,该探针在六邻体基因的161 bp区域进行DNA扩增后会发生反应,并通过链霉亲和素包被的微量滴定仪中的时间分辨荧光(TR)进行定量井。聚合酶链反应(PCR)-TR荧光法不是通常意义上的快速测试,但对于具有固有毒性或病毒产量低的标本(例如器官碎屑和生病后期获得的标本)非常有用。在对通过这种方法测试的103个样本(包括尿液,粪便和组织悬液)进行的调查中,阳性样本与六邻体特异性TR荧光免疫测定抗原测试的一致性为100%,与病毒培养相比的敏感性为91%。还显示了PCR-TR荧光测定系统作为PCR产物定量方法的优势。

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