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首页> 外文期刊>Journal of Clinical Microbiology >Evaluation of the COBAS Amplicor HBV Monitor Assay and Comparison with the Ultrasensitive HBV Hybrid Capture 2 Assay for Quantification of Hepatitis B Virus DNA
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Evaluation of the COBAS Amplicor HBV Monitor Assay and Comparison with the Ultrasensitive HBV Hybrid Capture 2 Assay for Quantification of Hepatitis B Virus DNA

机译:评估COBAS Amplicor HBV监测仪分析并与超灵敏HBV Hybrid Capture 2分析法进行定量乙肝病毒DNA的比较

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摘要

Performance characteristics of the COBAS Amplicor HBV Monitor test (Roche Diagnostics), which measures hepatitis B virus (HBV) DNA quantitatively, were evaluated and compared with the Ultrasensitive HBV Hybrid Capture 2 (HC2; Digene Corporation) assay. Linearity and within-run precision were assessed for both methods by using eight HBV DNA-positive samples serially diluted to obtain a range of <100 to 500,000 HBV DNA copies/ml and run in triplicate. Agreement between the methods was studied with 100 clinical samples. HC2 assay performance near the limit of detection was investigated through repeat testing of 149 samples with HC2 and testing of 37 samples with HC2 results of <4,700 HBV DNA copies/ml by Amplicor assay and a qualitative PCR assay. The linearity experiment for Amplicor had regression of observed values compared to expected values (y = 1.073x ? 0.247; R2 = 0.993, n = 32; for HC2, y = 0.855x + 0.759, R2 = 0.729, n = 18). Within-run standard deviation of log HBV DNA copies/ml ranged from 0.003 to 0.348 (Amplicor) and 0.027 to 0.253 (HC2). Agreement assessed by Deming regression was poor [Amplicor = 1.197(HC2) ? 0.961; R2 = 0.799, standard error of the estimate (SEE) = 0.710, n = 94]. Near the lower limit of detection, 32 of 149 repeat HC2 results were <4,700 HBV DNA copies/ml. Of the 37 samples with HC2 results of <4,700 HBV DNA copies/ml, HBV DNA was not detected in 15 samples, while HBV DNA was detected by at least one PCR method in 12 samples. Amplicor is linear from 200 to 200,000 HBV DNA copies/ml with undiluted samples, and this range can be expanded through dilution. Inconsistent HC2 results near the limit of detection justify use of a grey zone.
机译:评估了COBAS Amplicor HBV Monitor测试(Roche Diagnostics)的性能特征,该测试定量测量了乙型肝炎病毒(HBV)DNA,并与超灵敏HBV Hybrid Capture 2(HC2; Digene Corporation)测定法进行了比较。通过使用八个连续稀释的HBV DNA阳性样品,获得范围<100至500,000 HBV DNA拷贝/ ml并一式三份运行,评估了两种方法的线性和批内精密度。方法之间的一致性研究了100个临床样品。通过重复测试149个样品中的HC2并测试37个样品中的HC2结果小于4,700 HBV DNA拷贝/ ml,通过Amplicor测定和定性PCR测定法研究了接近检测极限的HC2测定性能。与预期值相比,Amplicor的线性实验具有观察值的回归( y = 1.073 x = 0.247; R 2 = 0.993, n = 32;对于HC2, y = 0.855 x + 0.759, R 2 = 0.729, n = 18)。 log HBV DNA拷贝数/ ml的运行内标准偏差范围为0.003至0.348(扩增子)和0.027至0.253(HC2)。通过Deming回归评估的一致性差[放大器= 1.197(HC2)? 0.961; R 2 = 0.799,估算的标准误(SEE)= 0.710, n = 94]。在检测下限附近,149个重复的HC2结果中有32个结果<4,700 HBV DNA拷贝/ ml。在HC2结果低于4700 HBV DNA拷贝/ ml的37个样品中,有15个样品未检测到HBV DNA,而12个样品中至少通过一种PCR方法检测到HBV DNA。对于未稀释的样品,Amplicor在200至200,000 HBV DNA拷贝/毫升之间呈线性关系,可以通过稀释扩大此范围。接近检测极限的HC2结果不一致表明使用灰色区域是合理的。

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