与纤维秃鹰细胞的吸附:加强病毒的自定义能力吗?

Gerhard Schmidt, Reinhard Wigand
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引用次数: 0

摘要

评估了两种改善临床材料中病毒培养的方法:用0.2 ml接种物强化吸附,在Bellco摇床上摇摇20小时,然后将材料低速离心到培养细胞上。采用终点滴定法对5个病毒科(腺病毒、单纯疱疹病毒、牛痘病毒、肠病毒、副流感病毒)的原型株和患者的原始标本(腺病毒、疱疹病毒、肠病毒)进行了研究,并与标准方法进行了比较。在腺病毒中,也进行了定量免疫荧光。在终点滴定中,与标准方法相比,离心法几乎从未导致病毒滴度升高。然而,在腺病毒的免疫荧光评价中,获得的值高出3- 4倍。另一方面,强化吸附法导致大多数腺病毒滴定的灵敏度增加,滴度增加4- 25倍,原型和原始材料。该方法对研究的所有其他病毒无效。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Intensiv-Adsorption von Viren an Gewebekulturzellen: Verbesserung der Virusisolierung?

Two procedures to improve virus cultivation from clinical material were evaluated: an intensified adsorption with 0.2 ml inoculum and 20 h rocking in a Bellco rocker and a low-speed centrifugation of the material onto the cultured cells. Prototype strains from 5 virus families (adenoviruses, herpes simplex virus, vaccinia virus, enteroviruses, para-influenza 2) as well as original specimens from patients (adenovirus, herpesvirus, enterovirus) were studied by endpoint titration in comparison with the standard procedure. In adenoviruses, a quantitative immunofluorescence was performed too.

In endpoint titrations, the centrifugation method did almost never lead to an increased virus titer, as compared with the standard method. However, in the immunofluorescence evaluation of adenoviruses the values attained were 3- to 4-fold higher. On the other hand, the intensified adsorption method led to an increased sensitivity in most adenovirus titrations with 4- to 25-fold titer increment, with prototype and original material. The procedure was ineffective in all other viruses studied.

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