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Hepatitis C virus genotyping based on Core and NS5B regions in Cameroonian patients

机译:基于Core和NS5B区域的喀麦隆患者丙型肝炎病毒基因分型

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Current HCV treatments are genotype specific although potential pan-genotype treatments have recently been described. Therefore, genotyping is an essential tool for the therapeutic management of HCV infection and a variety of technologies have been developed for HCV genotypes determination. Sequences analysis of HCV sub-genomic regions is considered as gold standard and is widely used for HCV genotyping. Here, we compared HCV genotyping using core and NS5B regions in routine practice in HCV-positive Cameroonian patients. All plasma samples received at Centre Pasteur of Cameroon (CPC) in 2016 for HCV genotyping were included. Viral loads were determined using the Abbott Real Time assay. Further, genotyping was based on the amplification and sequencing of core and NS5B regions following by phylogenetic analysis of corresponding sequences. A total of 369 samples were received during the study period with high viral load values (median: 930,952?IU/ml; IQR: 281,833-2,861,179). Positive amplification was obtained in at least one genomic region (core or NS5B) for all the samples with similar amplification rate in the two genomic regions (p?=?0.34). Phylogenetic analysis showed that among the 369 samples, 146 (39.6%) were classified as genotype 4, 132 (35.8%) as genotype 1, 89 (24.1%) as genotype 2, in both core and NS5B regions. Interestingly, for two samples (0.54%) discordant genotypes were obtained in both regions with the core region classified as genotype 4 while the NS5B was identified as genotype 1 indicating the presence of putative HCV recombinant virus or multiple infections in these samples. Discrimination of HCV subtypes was most likely possible with NS5B compared to core region. We found high amplification rates of HCV in both core and NS5B regions, and a good concordance was obtained at genotype level using both regions except for two samples where putative 1–4 recombinants/multiple infections were detected. Therefore, HCV genotyping based on at least two genomic regions could help to identify putative recombinants and improve therapeutic management of HCV infection.
机译:尽管最近已经描述了潜在的泛基因型治疗,但是当前的HCV治疗是基因型特异性的。因此,基因分型是HCV感染的治疗管理的重要工具,并且已经开发出多种技术来确定HCV基因型。 HCV亚基因组区域的序列分析被认为是金标准,被广泛用于HCV基因分型。在这里,我们比较了在喀麦隆HCV阳性的喀麦隆患者常规实践中使用核心区和NS5B区进行的HCV基因分型。包括2016年在喀麦隆巴斯德中心(CPC)收到的用于HCV基因分型的所有血浆样品。使用雅培实时测定法测定病毒载量。此外,基因分型是基于核心和NS5B区的扩增和测序,随后是对相应序列的系统进化分析。在研究期间共收到369份病毒载量高的样品(中位数:930,952?IU / ml; IQR:281,833-2,861,179)。对于所有样品,在至少一个基因组区域(核心或NS5B)中获得了正扩增,在两个基因组区域中具有相似的扩增速率(p≥0.34)。系统发育分析表明,在369个样品中,在核心和NS5B区域中,有146个(39.6%)被归为基因型4,132个(35.8%)被归为基因型1,有89个(24.1%)被归为基因型2。有趣的是,对于两个样本(0.54%),在两个区域均获得了不一致的基因型,核心区域被分类为基因型4,而NS5B被鉴定为基因型1,表明这些样本中存在推定的HCV重组病毒或多种感染。与核心区域相比,NS5B最有可能区分HCV亚型。我们发现在核心和NS5B区域中HCV的扩增率都很高,并且在两个基因型水平上都获得了良好的一致性,除了两个样本中检测到推定的1-4个重组体/多重感染。因此,基于至少两个基因组区域的HCV基因分型可以帮助鉴定推定的重组体并改善HCV感染的治疗管理。

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