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运用Taqman一步法逆转录聚合酶链反应(RT-PCR)对儿童粪便中的诺如病毒进行检测及基因分型

Detection and genogrouping of noroviruses from children's stools by Taqman One-step RT-PCR.

作者信息

Apaza Sonia, Espetia Susan, Gilman Robert H, Montenegro Sonia, Pineda Susana, Herhold Fanny, Pomari Romeo, Kosek Margaret, Vu Nancy, Saito Mayuko

机构信息

Laboratorio de Investigación y Desarrollo, Universidad Peruana Cayetano Heredia.

出版信息

J Vis Exp. 2012 Jul 22(65):3232. doi: 10.3791/3232.

Abstract

Noroviruses (NoVs) are the leading cause of outbreaks of sporadic acute gastroenteritis worldwide in humans of all ages. They are important cause of hospitalizations in children with a public health impact similar to that of Rotavirus. NoVs are RNA viruses of great genetic diversity and there is a continuous appearance of new strains. Five genogroups are recognized; GI and GII with their many genotypes and subtypes being the most important for human infection. However, the diagnosis of these two genotypes remains problematic, delaying diagnosis and treatment. For RNA extraction from stool specimens the most commonly used method is the QIAmp Viral RNA commercial kit from Qiagen. This method combines the binding properties of a silica gel membrane, buffers that control RNases and provide optimum binding of the RNA to the column together with the speed of microspin. This method is simple, fast and reliable and is carried out in a few steps that are detailed in the description provided by the manufacturer. Norovirus is second only to rotavirus as the most common cause of diarrhea. Norovirus diagnosis should be available in all studies on pathogenesis of diarrhea as well as in outbreaks or individual diarrhea cases. At present however norovirus diagnosis is restricted to only a few centers due to the lack of simple methods of diagnosis. This delays diagnosis and treatment. In addition, due to costs and regulated transportation of corrosive buffers within and between countries use of these manufactured kits poses logistical problems. As a result, in this protocol we describe an alternative, economic, in-house method which is based on the original Boom et al. method which uses the nucleic acid binding properties of silica particles together with the anti-nuclease properties of guanidinium thiocyanate. For the detection and genogrouping (GI and GII) of NoVs isolates from stool specimens, several RT-PCR protocols utilizing different targets have been developed. The consensus is that an RT-PCR using TaqMan chemistry would be the best molecular technique for diagnosis, because it combines high sensitivity, specificity and reproducibility with high throughput and ease of use. Here we describe an assay targeting the open reading frame 1 (ORF1)-ORF2 junction region; the most conserved region of the NoV genome and hence most suitable for diagnosis. For further genetic analysis a conventional RT-PCR that targets the highly variable N-terminal-shell from the major protein of the capsid (Region C) using primers originally described by Kojima et al. is detailed. Sequencing of the PCR product from the conventional PCR enables the differentiation of genotypes belonging to the GI and GII genogroups.

摘要

诺如病毒(NoVs)是全球各年龄段人群散发性急性胃肠炎暴发的主要原因。它们是导致儿童住院的重要病因,对公共卫生的影响与轮状病毒类似。诺如病毒是具有高度遗传多样性的RNA病毒,新毒株不断出现。已识别出五个基因组;GI和GII及其众多基因型和亚型对人类感染最为重要。然而,这两种基因型的诊断仍然存在问题,延误了诊断和治疗。从粪便标本中提取RNA最常用的方法是使用Qiagen公司的QIAmp Viral RNA商业试剂盒。该方法结合了硅胶膜的结合特性、控制核糖核酸酶并使RNA与柱体实现最佳结合的缓冲液以及微量离心的速度。此方法简单、快速且可靠,按照制造商提供的说明分几步进行。诺如病毒是仅次于轮状病毒的最常见腹泻病因。在所有关于腹泻发病机制的研究以及暴发或个别腹泻病例中都应能够进行诺如病毒诊断。然而目前,由于缺乏简单的诊断方法,诺如病毒诊断仅限于少数几个中心。这延误了诊断和治疗。此外,由于成本以及各国境内和之间腐蚀性缓冲液的运输管制,使用这些成品试剂盒存在后勤问题。因此,在本方案中,我们描述了一种基于最初的Boom等人的方法的替代、经济的内部方法,该方法利用了二氧化硅颗粒的核酸结合特性以及硫氰酸胍的抗核酸酶特性。为了从粪便标本中检测诺如病毒分离株并进行基因组分类(GI和GII),已经开发了几种利用不同靶标的逆转录聚合酶链反应(RT-PCR)方案。共识是,使用TaqMan化学的RT-PCR将是诊断的最佳分子技术,因为它结合了高灵敏度、特异性和可重复性以及高通量和易用性。在这里,我们描述了一种针对开放阅读框1(ORF1)-ORF2连接区的检测方法;这是诺如病毒基因组中最保守的区域,因此最适合诊断。对于进一步的基因分析,详细介绍了一种传统的RT-PCR,该方法使用Kojima等人最初描述的引物,针对衣壳主要蛋白的高度可变N端壳(区域C)。

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