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Rapid quantification of vesicular stomatitis virus in Vero cells using Laser Force Cytology

机译:使用激光致力细胞学快速定量VESO细胞中的脉络膜炎病毒

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The ability to rapidly and accurately determine viral infectivity can help improve the speed of vaccine product development and manufacturing. Current methods to determine infectious viral titers, such as the end-point dilution (50% tissue culture infective dose, TCID50) and plaque assays are slow, labor intensive, and often subjective. In order to accelerate virus quantification, Laser Force Cytology (LFC) was used to monitor vesicular stomatitis virus (VSV) infection in Vero (African green monkey kidney) cells. LFC uses a combination of optical and fluidic forces to interrogate single cells without the use of labels or antibodies. Using a combination of variables measured by the Radiance (TM) LFC instrument (LumaCyte), an infection metric was developed that correlates well with the viral titer as measured by TCID50 and shortens the timeframe from infection to titer determination from 3 days to 16 h (a 4.5 fold reduction). A correlation was also developed between in-process cellular measurements and the viral titer of collected supernatant, demonstrating the potential for real-time infectivity measurements. Overall, these results demonstrate the utility of LFC as a tool for rapid infectivity measurements throughout the vaccine development process. (C) 2018 The Authors. Published by Elsevier Ltd.
机译:快速准确地确定病毒感染性的能力可以有助于提高疫苗产品开发和制造的速度。目前的方法来确定传染性病毒滴度,例如终点稀释(50%组织培养感染剂量,TCID50)和斑块测定缓慢,劳动密集型和经常是主观的。为了加速病毒定量,使用激光力细胞学(LFC)监测Vero(非洲绿色猴肾脏)细胞中的囊泡口炎病毒(VSV)感染。 LFC使用光学和流体力的组合来询问单个细胞而不使用标签或抗体。利用由辐射(TM)LFC仪器(Lumacyte)测量的变量的组合,开发了一种感染率,其与TCID50测量的病毒滴度良好,并且从3天至16小时将时间框架从感染从感染缩短到滴度测定减少4.5倍)。在过程中的细胞测量和收集的上清液的病毒滴度之间也开发了相关性,证明了实时感染测量的可能性。总体而言,这些结果证明了LFC作为在整个疫苗开发过程中快速感染测量的工具的效用。 (c)2018年作者。 elsevier有限公司出版

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