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用于诊断血清学检测的非感染性黄病毒重组抗原浓缩方法的比较。

A comparison of concentration methods applied to non-infectious flavivirus recombinant antigens for use in diagnostic serological assays.

作者信息

Russell Brandy J, Velez Jason O, Laven Janeen J, Johnson Alison J, Chang Gwong-Jen J, Johnson Barbara W

机构信息

Diagnostic and Reference Laboratory, Centers for Disease Control and Prevention, 3150 Rampart Rd., Fort Collins, CO 80521, United States.

出版信息

J Virol Methods. 2007 Oct;145(1):62-70. doi: 10.1016/j.jviromet.2007.05.008. Epub 2007 Jun 14.

DOI:10.1016/j.jviromet.2007.05.008
PMID:17570536
Abstract

Since the introduction of West Nile virus into the United States in 1999, there has been a greater awareness of arboviruses, consequently, diagnostic testing for West Nile virus and other arboviruses has increased both in U.S. and international public health laboratories. The Centers for Disease Control and Prevention/Division of Vector-Borne Infectious Diseases/Arbovirus Diagnostic and Reference Laboratory produces and provides the serodiagnostic reagents which are not available commercially. Reagents needed to conduct the enzyme-linked immunoassay (ELISA) include a virus-specific non-infectious antigen. Antigens for Japanese encephalitis and the four dengue virus serotypes have been developed from COS-1 transformed cells that secrete non-infectious, virus-like particles into the cell culture supernatant. Four methods for concentrating the supernatant are discussed here. The methods are ultracentrifugation, polyethylene glycol precipitation, and two ultrafiltration methods: the Stirred Cell (Millipore Corporation, Billerica, MA) and the Pellicon 2 (Millipore Corporation, Billerica, MA). Ultracentrifugation and the Pellicon 2 ultrafiltration system produced antigen at a sufficient concentration for use in the ELISA. Large volumes were concentrated in a shorter time in the Pellicon 2 ultrafiltration system. An additional filtration step was necessary to produce antigen of sufficient concentration for use in the microsphere-based immunoassay, which requires antigen concentrated an additional 10 times.

摘要

自1999年西尼罗河病毒传入美国以来,人们对虫媒病毒有了更高的认识,因此,美国和国际公共卫生实验室对西尼罗河病毒及其他虫媒病毒的诊断检测都有所增加。疾病控制与预防中心/媒介传播传染病司/虫媒病毒诊断与参考实验室生产并提供市售的血清学诊断试剂。进行酶联免疫吸附测定(ELISA)所需的试剂包括病毒特异性非感染性抗原。日本脑炎和四种登革病毒血清型的抗原是从COS-1转化细胞中开发出来的,这些细胞将非感染性、病毒样颗粒分泌到细胞培养上清液中。本文讨论了四种浓缩上清液的方法。这些方法是超速离心、聚乙二醇沉淀和两种超滤方法:搅拌细胞法(密理博公司,马萨诸塞州比勒里卡)和Pellicon 2法(密理博公司,马萨诸塞州比勒里卡)。超速离心和Pellicon 2超滤系统产生的抗原浓度足以用于ELISA。在Pellicon 2超滤系统中,大量样品能在更短时间内浓缩。为了生产出浓度足以用于基于微球的免疫测定的抗原,还需要额外的过滤步骤,这种免疫测定需要将抗原再浓缩10倍。

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