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两种转录介导扩增检测方法在献血者中检测乙型肝炎病毒、丙型肝炎病毒和人类免疫缺陷病毒 1 的头对头比较。

Head-to-head comparison of two transcription-mediated amplification assay versions for detection of hepatitis B virus, hepatitis C virus, and human immunodeficiency virus Type 1 in blood donors.

机构信息

Institute of Hematology and Transfusion Medicine, Warsaw, Poland; Biologicals Quality Control, DDL Diagnostic Laboratory, Rijswijk, the Netherlands; Regional Blood Center, Warsaw, Poland; Regional Blood Transfusion Center, Łódź, Poland; Regional Blood Transfusion Center, Krakow, Poland; National Health Service Blood and Transplant, Cambridge Blood Centre, Cambridge, United Kingdom; Lelie Research, Paris, France.

出版信息

Transfusion. 2013 Oct;53(10 Pt 2):2512-24. doi: 10.1111/trf.12190. Epub 2013 Apr 17.

DOI:10.1111/trf.12190
PMID:23590145
Abstract

BACKGROUND

The second triplex transcription-mediated amplification (TMA) assay version (Ultrio Plus, Novartis Diagnostics) uses an additional reagent enhancing the disruption of hepatitis B virus (HBV) particles and release of DNA for the target capture probe. This study compares the performance of this new assay version with the previous one (Ultrio).

STUDY DESIGN AND METHODS

For analytical sensitivity assessment the World Health Organization HBV, hepatitis C virus (HCV), and human immunodeficiency virus (HIV) international standards and various genotype dilution panels were used. Individual donations (IDs) from 9980 first-time donors were screened simultaneously by serology and both TMA assay versions.

RESULTS

The 50 and 95% limits of detection (LODs) for HBV using Ultrio Plus were 0.8 (0.6-1.0) and 4.6 (3.2-7.2) IU/mL, respectively, 2.4 (1.4-4.8)-fold more sensitive than Ultrio. The TMA assay versions had comparable LODs for HIV-1 and HCV. The improvement factors on analytical sensitivity panels of HBV Genotypes A to G ranged from 1.3 to 7.3 and 50% LODs (95% confidence interval) reduced from 12.5 (10-15) to 3.8 (3.2-4.4) copies/mL. One Ultrio Plus HBV Genotype D yield sample missed by the Ultrio assay in the donor screening study was detected with ninefold higher sensitivity. The specificities of ID nucleic acid test (ID-NAT) and serologic testing in a similar repeat test algorithm were 100 and 99.41%, respectively.

CONCLUSION

More efficient target capture chemistry in the new TMA assay version significantly improved sensitivity and diminished variability in detecting HBV strains of various genotypes. We recommend a triplicate ID-NAT repeat test strategy to eliminate discriminatory tests on false-non-repeat-reactive (anti-HBc-nonreactive) donations.

摘要

背景

第二代三重转录介导扩增(TMA)检测版本(罗氏诊断Ultrio Plus)采用了一种额外的试剂,可增强乙型肝炎病毒(HBV)颗粒的破坏和 DNA 的释放,以用于目标捕获探针。本研究比较了该新检测版本与上一代检测版本(Ultrio)的性能。

研究设计和方法

为了评估分析灵敏度,我们使用了世界卫生组织的乙型肝炎病毒、丙型肝炎病毒(HCV)和人类免疫缺陷病毒(HIV)国际标准以及各种基因型稀释板。我们同时使用血清学和两种 TMA 检测版本对 9980 名初次献血者的个体献血者样本(IDs)进行筛查。

结果

使用 Ultrio Plus 的 HBV 的 50%和 95%检测限(LOD)分别为 0.8(0.6-1.0)和 4.6(3.2-7.2)IU/mL,比 Ultrio 分别提高了 2.4(1.4-4.8)倍。两种 TMA 检测版本对 HIV-1 和 HCV 的 LOD 具有可比性。HBV 基因型 A 至 G 的分析灵敏度面板的改进因子范围为 1.3 至 7.3,50% LOD(95%置信区间)从 12.5(10-15)降低至 3.8(3.2-4.4)拷贝/mL。在献血者筛查研究中,Ultrio 检测漏检的一个 Ultrio Plus HBV 基因型 D 产量样本,用灵敏度提高 9 倍的方法检测到。在类似的重复测试算法中,ID-NAT 和血清学测试的特异性分别为 100%和 99.41%。

结论

新的 TMA 检测版本中更有效的目标捕获化学显著提高了灵敏度,并减少了检测各种基因型 HBV 菌株的变异性。我们建议采用三重复 ID-NAT 重复测试策略,以消除对假非重复反应(抗-HBc 无反应)献血者的鉴别测试。

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