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  • Home
  • Knowledge Base
  • CellCountingSub Section
  • Direct Counting of Individual Infected Cells
Cell Counting and Image Cytometry

Direct Counting of Individual Infected Cells

Section
Modern Virology Assays
Celigo Applications
Cell Counting Method Selection
Cell Counting and Image Cytometry FAQs
Cell-based Assays for Bioprocessing
Cell-based Assays for Gene Therapy Development
Cellometer Applications
Modern Virology Assays
Sub Section
Viral Titre
Antibody Binding Inhibition
Antibody Neutralization
Cytopathic Effects
Viral Titre
Topic
Direct Counting of Individual Infected Cells
Direct Counting of Individual Infected Cells
High-Throughput Counting Of GFP-Expressing Influenza Viral Foci-1
Influenza Viral Titration With mKate2 Fluorescent Protein Reporter
Zika Viral Titration with mKate2 Fluorescent Protein Reporter
Automated Counting of Plaques

Direct counting of individual infected cells labeled with mKate2-expressing influenza virus

Researchers working with replication-incompetent viruses will require the use of fluorescent viral particles and fluorescent immunostaining to detect single infected cells. In order to quantify, the flow cytometry method is typically used to analyze 1000 – 2000 host cells in 96- or 384-well plates. First, these host cells require the lengthy process trypsinization which disturbs the host and virus interaction. Next, flow cytometry requires approximately 2 minutes per sample to analyze the infected cells, which is equivalent to 3 hours for 96 samples and around 12 hours for 384 samples.

The Celigo™ image cytometer can efficiently image and quantify individual infected cells, where the system can scan and analyze an entire 384-well plate in less than 10 min/plate in brightfield (HRP labeling) and fluorescence. The images below show individual infected MDCK cells with mKate2-expressing influenza virus. The plate imager was able to directly count the infected cells within a single well without trypsinization, calculate infection rate, and generate a highly linear viral titration plot using the equation:

Direct counting of individual infected cells-3
Direct counting of individual infected cells-1

Whole well brightfield and fluorescent overlay images for high (left) and low (right) viral concentrations

Direct counting of individual infected cells-2

Direct counting results of mKate2 positive infected MDCK cells, where the percentage infection was calculated from the total cell count

Direct counting of individual infected cells-3

Influenza viral infection rate in respect to dilution

For research use only. Not for use in diagnostic procedures.

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