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一种用于在细胞培养中生产灭活虫媒病毒抗原的算法的开发。

Development of an algorithm for production of inactivated arbovirus antigens in cell culture.

作者信息

Goodman C H, Russell B J, Velez J O, Laven J J, Nicholson W L, Bagarozzi D A, Moon J L, Bedi K, Johnson B W

机构信息

Arboviral Diseases Branch, Division of Vector-borne Diseases, Centers for Disease Control and Prevention, 3156 Rampart Road, Fort Collins, CO 80521, USA.

Arboviral Diseases Branch, Division of Vector-borne Diseases, Centers for Disease Control and Prevention, 3156 Rampart Road, Fort Collins, CO 80521, USA.

出版信息

J Virol Methods. 2014 Nov;208:66-78. doi: 10.1016/j.jviromet.2014.07.030. Epub 2014 Aug 4.

Abstract

Arboviruses are medically important pathogens that cause human disease ranging from a mild fever to encephalitis. Laboratory diagnosis is essential to differentiate arbovirus infections from other pathogens with similar clinical manifestations. The Arboviral Diseases Branch (ADB) reference laboratory at the CDC Division of Vector-Borne Diseases (DVBD) produces reference antigens used in serological assays such as the virus-specific immunoglobulin M antibody-capture enzyme-linked immunosorbent assay (MAC-ELISA). Antigen production in cell culture has largely replaced the use of suckling mice; however, the methods are not directly transferable. The development of a cell culture antigen production algorithm for nine arboviruses from the three main arbovirus families, Flaviviridae, Togaviridae, and Bunyaviridae, is described here. Virus cell culture growth and harvest conditions were optimized, inactivation methods were evaluated, and concentration procedures were compared for each virus. Antigen performance was evaluated by the MAC-ELISA at each step of the procedure. The antigen production algorithm is a framework for standardization of methodology and quality control; however, a single antigen production protocol was not applicable to all arboviruses and needed to be optimized for each virus.

摘要

虫媒病毒是重要的医学病原体,可导致从轻度发热到脑炎等人类疾病。实验室诊断对于区分虫媒病毒感染与其他具有相似临床表现的病原体至关重要。美国疾病控制与预防中心媒介传播疾病司(DVBD)的虫媒病毒疾病分支(ADB)参考实验室生产用于血清学检测的参考抗原,如病毒特异性免疫球蛋白M抗体捕获酶联免疫吸附测定(MAC-ELISA)。细胞培养中的抗原生产在很大程度上已取代了乳鼠的使用;然而,这些方法无法直接转移。本文描述了一种针对黄病毒科、披膜病毒科和布尼亚病毒科这三个主要虫媒病毒科的九种虫媒病毒的细胞培养抗原生产算法。对每种病毒的细胞培养生长和收获条件进行了优化,评估了灭活方法,并比较了浓缩程序。在该程序的每个步骤通过MAC-ELISA评估抗原性能。抗原生产算法是方法标准化和质量控制的框架;然而,单一的抗原生产方案并不适用于所有虫媒病毒,需要针对每种病毒进行优化。

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