首页> 外文期刊>Transfusion: The Journal of the American Association of Blood Banks >Evaluation of a new PCR assay with competitive internal control sequence for blood donor screening.
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Evaluation of a new PCR assay with competitive internal control sequence for blood donor screening.

机译:评估具有竞争性内部控制序列的新PCR分析用于献血者筛选。

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BACKGROUND: High-throughput nucleic acid testing for transfusion-relevant viruses by PCR requires contamination-proof methods with high sensitivity and validity. A new PCR reagent kit (TaqMan, PE BioSystems) reduces the risk of carry-over contamination by eliminating post-PCR processing. STUDY DESIGN AND METHODS: Oligonucleotide design was done with software specialized for designing the assays' (TaqMan) primers and probes. A template-derived competitive internal control sequence designed through site-directed mutagenesis was used to reveal failures in amplification. Assay sensitivity was determined for single-donor and single-patient testing and by spiking sample mini-pools. Three seroconversion panels were tested. RESULTS: Sensitivity is high, reaching 300 HBV genomes per mL of single-patient material on direct testing. A detection limit of 1000 HBV genome equivalents per mL of donor plasma is achieved for 96 pooled samples. The window period for HBV infection was reduced by 17, 10, and 63 days from that for HBsAg screening in three seroconverting donors. CONCLUSION: The assay provides sufficient sensitivity to be superior to HBsAg screening in transfusion medicine and will be useful in clinical laboratories because of its ease of handling.
机译:背景:通过PCR对输血相关病毒进行高通量核酸测试需要具有高灵敏度和有效性的防污染方法。一种新的PCR试剂盒(TaqMan,PE BioSystems)通过消除PCR后处理来降低残留污染的风险。研究设计和方法:寡核苷酸的设计是通过专门用于设计分析(TaqMan)引物和探针的软件完成的。通过定点诱变设计的模板来源的竞争性内部控制序列被用来揭示扩增失败。通过单样本供体和单样本加标池确定测定灵敏度,用于单供体和单患者测试。测试了三个血清转换面板。结果:敏感性很高,直接测试可达到每毫升单人病材料300 HBV基因组。对于96个合并样品,每毫升供体血浆的检测极限为1000 HBV基因组当量。与三个血清转化供体的HBsAg筛查相比,HBV感染的窗期缩短了17天,10天和63天。结论:该方法具有足够的灵敏度,优于输血医学中的HBsAg筛查,并且由于其易于操作,将在临床实验室中有用。

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