首页> 外文期刊>Journal of Virological Methods >IDENTIFICATION OF CONSERVED NUCLEOTIDE SEQUENCES WITHIN THE GB VIRUS C 5'-UNTRANSLATED REGION - DESIGN OF PCR PRIMERS FOR DETECTION OF VIRAL RNA
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IDENTIFICATION OF CONSERVED NUCLEOTIDE SEQUENCES WITHIN THE GB VIRUS C 5'-UNTRANSLATED REGION - DESIGN OF PCR PRIMERS FOR DETECTION OF VIRAL RNA

机译:GB病毒C 5'-未转学区内保守核苷酸序列的鉴定PCR引物检测检测病毒RNA

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Recently, the discovery of a new human RNA virus, GB virus C (GBV-C), was reported. GBV-C was isolated from the serum of a West African individual using degenerate oligonucleotide PCR primers designed from a consensus sequence of the NS3 helicase genes of hepatitis C virus (HCV), GBV-A, and GBV-B. Seven other individuals were shown to be infected with GBV-C via RT-PCR using these primers. Subsequently, degenerate PCR primers based upon a consensus sequence of the eight original isolates were designed. These primers were shown to be superior to the original set. However, since they were derived from a region of the viral genome exhibiting up to 17% nucleotide sequence divergence, mismatch between the primers and template may result in an underestimation of the true GBV-C prevalence. To overcome this potential problem, we obtained the sequences at the 5'-untranslated region (UTR) of the GBV-C genome from 35 infected individuals and identified regions of high sequence conservation among the isolates. We describe the design and testing of PCR primers derived from conserved sequences within the 5'-UTR of the GBV-C genome. These primers were shown to be as effective as the helicase-derived primers in detecting GBV-C RNA in human sera.
机译:最近,据报道,发现新的人RNA病毒GB病毒C(GBV-C)。使用从丙型肝炎病毒(HCV),GBV-A和GBV-B的NS3 Helicase基因的共有序列设计的简并寡核苷酸PCR引物,从西非人的血清中分离出GBV-C。七种其他个体通过使用这些引物通过RT-PCR感染GBV-C。随后,设计了基于八个原始分离株的共有序列的简并PCR引物。这些引物显示出优于原始组。然而,由于它们来自表现出高达17%核苷酸序列发散的病毒基因组的区域,因此引物和模板之间的错配可能导致低估真正的GBV-C流行率。为了克服这种潜在的问题,我们在来自35个受感染的个体的GBV-C基因组的5'非翻译区(UTR)中获得了序列,并确定了分离株中的高序列保护区域。我们描述了GBV-C基因组5'-UTR中衍生自保守序列的PCR引物的设计和测试。显示这些引物作为检测人血清中的GBV-C RNA的螺旋酶衍生引物有效。

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