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Follow-Up on Diagnostic Proficiency of Laboratories Equipped To Perform Orthopoxvirus Detection and Quantification by PCR: the Second International External Quality Assurance Study

机译:通过PCR进行正痘病毒检测和定量的实验室诊断能力的后续研究:第二项国际外部质量保证研究

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摘要

Two years after the first external quality assurance study on bioterrorism-relevant viruses, we have conducted a follow-up study on orthopoxvirus detection by PCR. Thirty-three laboratories (27 European, 4 Austral-Asian, and 2 American) participated. Samples contained 0 to 40,000,000 DNA copies of lyophilized monkeypox, cowpox, and vaccinia virus per ml. Laboratories achieved a >80% detection chance above 56,234 copies per ml. Global sensitivity was not significantly improved over that of the first study. Twenty-seven and 9 participants, respectively, were able to genotype and quantify virus. Four of 27 genotyping results were incorrect. Quantification accuracy was significantly better for vaccinia virus than for the other viruses. False-positive results occurred in 22 (11.8%) of all 186 tests on negative samples, but 18 of these were contributed by only five laboratories. Fifty-five percent of laboratories could appropriately detect PCR inhibition. The use of either real-time PCR or commercial diagnostic kits had significant positive influence on laboratory performance.
机译:在首次对与生物恐怖主义有关的病毒进行外部质量保证研究之后的两年,我们对PCR检测正痘病毒进行了后续研究。有33个实验室(欧洲27个实验室,南亚4个实验室和美国2个实验室)参加了会议。样品每毫升含有0到40,000,000个冻干猴痘,牛痘和牛痘病毒的DNA拷贝。实验室在每毫升56,234份以上的样品中实现了> 80%的检测机会。与第一项研究相比,总体敏感性没有明显改善。分别有27名和9名参与者能够进行基因分型和量化病毒。 27个基因分型结果中有4个是错误的。牛痘病毒的定量准确性明显优于其他病毒。在186个阴性样本中,有22个(11.8%)出现假阳性结果,但其中18个仅由五个实验室提供。 55%的实验室可以适当地检测PCR抑制作用。实时PCR或商业诊断试剂盒的使用对实验室性能产生了显着的积极影响。

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