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首页> 外文期刊>Journal of Clinical Microbiology >Clinical characterization of a competitive PCR assay for quantitative testing of hepatitis C virus.
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Clinical characterization of a competitive PCR assay for quantitative testing of hepatitis C virus.

机译:用于定量检测丙型肝炎病毒的竞争性PCR检测的临床表征。

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Rational clinical application of quantitative assessments of hepatitis C virus (HCV) RNA depends on an understanding of factors affecting the assay and its intrinsic variability. The effects of three types of blood collection tubes, two storage temperatures, five processing times, and two laboratories on a commercially available quantitative reverse transcriptase PCR assay (AMPLICOR HCV MONITOR) were evaluated. HCV RNA concentrations were assessed in 356 specimens representing 178 aliquots from nine patients. In a multivariate generalized linear model, HCV RNA concentrations decreased when centrifugation was delayed more than 6 h (P = 0.005) and were marginally different between laboratories (P = 0.06), but precentrifugation storage temperature (P = 1.00) and anticoagulation (P = 0.22) had no effect. After adjusting for other factors, the HCV concentration of 95% of a subject's samples were within 0.44 log. Specimens procured for reverse transcriptase PCR-based quantitative HCV testing should be centrifuged within 6 h of collection. Serial assessments should ideally be performed in the same laboratory, and changes in HCV RNA concentration of less than 0.44 log may not be biologically important.
机译:丙型肝炎病毒(HCV)RNA定量评估的合理临床应用取决于对影响分析及其内在变异性的因素的理解。评估了三种类型的血液采集管,两个存储温度,五个处理时间和两个实验室对市售定量逆转录酶PCR分析(AMPLICOR HCV MONITOR)的影响。评估了356份标本中的HCV RNA浓度,这些标本代表了9名患者的178等分试样。在多变量广义线性模型中,当离心延迟超过6 h(P = 0.005)时,HCV RNA浓度降低,并且实验室之间的差异很小(P = 0.06),但离心分离前的储存温度(P = 1.00)和抗凝(P = 0.22)无效。调整其他因素后,受试者样本中95%的HCV浓度在0.44 log之内。为进行基于逆转录酶PCR的定量HCV检测而采购的标本应在收集后6小时内离心。理想情况下,应在同一实验室进行系列评估,并且HCV RNA浓度变化小于0.44 log可能在生物学上并不重要。

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