Application of nested PCR and mass spectrometry for DNA-based virus detection: HBV-DNA detected in the majority of isolated anti-HBc positive sera

Christian Jurinke , Bernhard Zöllner , Heinz-Hubert Feucht , Dirk van den Boom , Anette Jacob , Susanne Polywka , Rainer Laufs , Hubert Köster
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引用次数: 21

Abstract

DNA preparations from three different groups of serum samples were examined for HBV-DNA via a nested polymerase chain reaction assay (lower detection limit: 10 viral genomes in 100 μl serum): Group I consisted of 11 uninfected control sera, group II consisted of sera obtained from 11 HBV infected patients and group III consisted of 21 isolated anti-HBc positive samples. The 21 samples from group III were HBV-DNA negative according to a conventional non-nested PCR assay and hybridization with a 32P-labelled probe. Using nested PCR and mass spectrometry, HBV-DNA was detected in none of group I and in all of group II samples. In 11 out of 21 (52%) of the isolated anti-HBc positive sera from group III, HBV-DNA was detected. No correlation was observed between HBV-DNA positivity and anti-HBc titers. Matrix-assisted laser desorption/ionization time-of-flight (MALDI-TOF) mass spectrometry provided a fast, sensitive and non-radioactive assay for the detection of PCR products without the need for gel electrophoresis or hybridization with labelled probes.

巢式PCR和质谱法在基于dna的病毒检测中的应用:在大多数分离的抗hbc阳性血清中检测到HBV-DNA
采用巢式聚合酶链反应法检测三组血清样品的DNA制剂(最低检出限为100 μl血清中10个病毒基因组):第一组为11份未感染对照血清,第二组为11份HBV感染患者血清,第三组为21份分离抗hbc阳性样本。根据传统的非巢式PCR检测和32p标记探针杂交,III组的21份样本HBV-DNA阴性。采用巢式PCR和质谱法,在I组和II组的所有样本中均未检测到HBV-DNA。III组21例分离抗hbc阳性血清中有11例(52%)检测到HBV-DNA。HBV-DNA阳性与抗hbc滴度无相关性。基质辅助激光解吸/电离飞行时间(MALDI-TOF)质谱法为PCR产物的检测提供了一种快速、敏感和无放射性的检测方法,无需凝胶电泳或与标记探针杂交。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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