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作 者:王佶[1] 徐子乾[1] 张晨 牛培华 关丽[1] 段招军[1] 马学军[1]
机构地区:[1]中国疾病预防控制中心病毒病预防控制所,北京102206
出 处:《病毒学报》2014年第2期128-133,共6页Chinese Journal of Virology
基 金:传染病重大专项(2013ZX10004-001;2012ZX10004-215;2013ZX10004-202;2013ZX10004804-007)
摘 要:本研究建立了一种基于新型再测序芯片(Resequencing Pathogen Microarray,RPM)的腹泻症候群多病原检测方法,能同时检测14种轮状病毒,7种杯状病毒,8种星状病毒,28种肠道病毒,16种少见致泻病毒。选取已验证的阳性病毒样本为模板来评估该方法的特异性。用克隆质粒和体外转录的RNA梯度稀释液来检验RPM的灵敏度,在20~2000拷贝/gL水平时RPM仍能检测和分辨出相近的病毒亚型。通过调整参考品的浓度优化了阳性判定阈值,并改进了肠道病毒的检测流程以完成分型。对10份不明原因腹泻样品进行了筛查,从中检出6份腹泻病毒阳性样本。根据RPM结果对样品进行了单重PCR并且测序,RPM与测序结果一致。本研究建立了一种高通量,高特异性,灵敏度较高的RPM方法,对于不明原因腹泻病例的诊断和突发疫情的处理有巨大的应用价值。In this study, a novel resequencing pathogen microarray (RPM)-based multi-pathogen detection assay was developed to simultaneously detect 14 rotaviruses, 7 caliciviruses, 8 astroviruses, 28 enteroviruses, and 16 rare diarrhea viruses in patients with diarrhea syndrome. The specificity of the assay was examined using confirmed virus-positive specimens, and the sensitivity was evaluated by serial ten-fold dilu- tions of in vitro transcribed RNA. RPM assay could detect and differentiate virus types/subtypes at 20- 2000 copies/~tL. The detection threshold of RPM was determined by adjusting the reference concentration, and the detection steps were optimized to type Enterovirus. The nucleic acids of 10 stool samples from pa- tients with unexplained diarrhea were screened, and 6 of them showed positive results. The RPM results were further verified by singleplex PCR followed by sequencing, and no difference was found between the two assays. In conclusion, we have established a high-throughput RPM assay with high specificity and sensitivity, which demonstrates a great potential for the identification of pathogens in patients with unexplained diarrhea and the management of emerging epidemic.
分 类 号:R373.2[医药卫生—病原生物学]
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