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首页> 外文期刊>Journal of clinical virology: The official publication of the Pan American Society for Clinical Virology >Development and evaluation of serological assays for detection of human hantavirus infections caused by Sin Nombre virus.
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Development and evaluation of serological assays for detection of human hantavirus infections caused by Sin Nombre virus.

机译:血清学检测方法的开发和评估,用于检测由罪恶诺贝尔病毒引起的人类汉坦病毒感染。

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BACKGROUND:: The hantavirus cardiopulmonary syndrome (HCPS) was first recognized in 1993 after a cluster of acute respiratory distress syndrome deaths in the southwestern of the United States. The major causative agent of HCPS in North America is the Sin Nombre virus (SNV) carried by the deer mouse Peromyscus maniculatus. The first HCPS case imported to Europe was reported in 2002. OBJECTIVES:: The objective of the study was to develop and evaluate ELISA and Western blot tests for the serological detection of human infections caused by SNV including those imported to Europe. STUDY DESIGN:: A polyhistidine (His)-tagged recombinant nucleocapsid (rN) protein of SNV was expressed in Saccharomyces cerevisiae and purified by nickel chelation chromatography. On the basis of the purified SNV rN protein mu-capture and indirect IgM and IgG ELISAs and an IgG Western blot were developed. The evaluation of the tests was performed using a negative serum panel and a blinded serum panel from the US containing acute-phase sera from HCPS patients. RESULTS:: Based upon the results obtained using a panel of negative control sera the specificity for SNV mu-capture and indirect IgM and IgG ELISAs were found to be 100%. All 33 sera from SNV-infected HCPS patients included in the blinded panel were detected by the SNV mu-capture and indirect IgM ELISAs. Twenty-nine out of the 33 SNV-IgM positive sera reacted also in the SNV-IgG ELISA. An SNV-IgG Western blot confirmed the data of the SNV-IgG ELISA. Although the majority of anti-SNV positive sera cross-reacted with rN proteins of Puumala virus and Dobrava virus, the lacking reactivity of a few sera with these heterologous rN antigens in the corresponding IgM and IgG ELISAs demonstrates the value of virus-specific test formats for acute-phase sera. CONCLUSIONS:: The novel SNV ELISA and Western blot tests represent a useful tool for the serological detection of SNV infections.
机译:背景:汉坦病毒性心肺综合征(HCPS)于1993年在美国西南部发生一系列急性呼吸窘迫综合征死亡后首次被发现。在北美,HCPS的主要病原体是由鹿小鼠Peromyscus maniculatus携带的Sin Nombre病毒(SNV)。 2002年报道了第一例进口到欧洲的HCPS病例。目的:该研究的目的是开发和评估ELISA和Western blot检测血清学检测由SNV引起的人类感染,包括进口到欧洲的SNV。研究设计:在酿酒酵母中表达了带有多组氨酸(His)标签的SNV重组核衣壳(rN)蛋白,并通过镍螯合色谱法纯化。基于纯化的SNV rN蛋白的mu-capture以及间接IgM和IgG,开发了ELISA和IgG Western印迹。使用阴性血清组和美国含HCPS患者急性期血清的盲法血清组进行测试评估。结果:基于使用一组阴性对照血清获得的结果,发现对SNV mu捕获以及间接IgM和IgG ELISA的特异性为100%。用SNV mu捕获和间接IgM ELISAs检测了所有SNV感染的HCPS患者的33份血清。在SNV-IgG ELISA中,33个SNV-IgM阳性血清中有29个也发生了反应。 SNV-IgG Western印迹证实了SNV-IgG ELISA的数据。尽管大多数抗SNV阳性血清与Puumala病毒和Dobrava病毒的rN蛋白发生交叉反应,但在相应的IgM和IgG ELISA中,一些血清与这些异源rN抗原缺乏反应性,这证明了病毒特异性测试格式的价值用于急性期血清。结论:新颖的SNV ELISA和Western blot检测代表了血清学检测SNV感染的有用工具。

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