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Integration of Fluorescence Detection and Image-Based Automated Counting Increases Speed Sensitivity and Robustness of Plaque Assays

机译:荧光检测和基于图像的自动计数的集成提高了噬斑测定的速度灵敏度和鲁棒性

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摘要

Plaque assays are used to measure the infectious titer of viral samples. These assays are multi-day and low-throughput and may be subject to analyst variability from biased or subjective manual plaque counting. Typically, on day 1, cells are adhered to plates overnight. On day 2, cells are infected with virus. After 3 additional days, plaques are fixed, stained with a horseradish peroxidase (HRP)-conjugated antibody and a HRP substrate, and counted by eye. Manual-based visual counting of plaques is time-consuming and laborious and may be subject to variability between analysts. Also, the assay must proceed for several days to allow the plaques to increase to sufficiently large sizes for manual identification. Here, we integrate fluorescent detection and automated plaque counting to increase the sensitivity and speed of the assay. First, we stain plaques with a fluorescent-labeled antibody. Second, we implement a plate-based cell imager to perform non-biased, non-subjective plaque counting. The integration of these two technologies decreases the assay length by 40%, from 5 days to 3 days, because plaque size, plaque signal to noise, and manual visualization are no longer limiting. This optimized plaque assay is sensitive, fast, and robust and expands the throughput and usage of this method for measuring plaque formation.
机译:噬斑测定法用于测量病毒样品的感染滴度。这些测定是多天且低通量的,并且可能由于有偏见的或主观的手动噬菌斑计数而导致分析者的差异。通常,在第1天,细胞会在平板上粘附过夜。在第二天,细胞被病毒感染。再过3天后,将噬菌斑固定,用辣根过氧化物酶(HRP)偶联的抗体和HRP底物染色,然后用肉眼计数。基于手动的噬菌斑肉眼计数非常耗时且费力,并且可能会因分析人员之间的差异而异。而且,测定必须进行几天,以使噬菌斑增加到足够大的尺寸以进行人工鉴定。在这里,我们整合了荧光检测和自动空斑计数功能,以提高检测的灵敏度和速度。首先,我们用荧光标记的抗体对噬菌斑进行染色。其次,我们实现了基于平板的细胞成像仪,以执行无偏见,非主观的斑块计数。两种技术的集成使检测长度从5天减少到3天减少了40%,因为噬菌斑大小,噬菌斑信噪比和手动可视化不再受到限制。这种优化的噬斑测定方法灵敏,快速且稳定,可扩展这种方法用于测量噬斑形成的通量和用途。

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