Bender MedSystems FlowCytomix™ Technology

Bender MedSystems bead-based assays follow the same principle as a sandwich immunoassay.

Fluorescent polystyrol beads are coupled with antibodies specific to the analytes to be detected.
A mix of coupled beads is incubated with the samples to be tested.
Analytes in the sample bind to the antibodies coupled to the beads.
A biotin conjugated antibody mix is added, which binds to the analytes bound to the capture antibodies. Streptavidin-Phycoerythrin (PE) is added which binds to the biotin conjugates.
Beads are differentiated by their sizes and distinct spectral signature by flow cytometry. FlowCytomix Pro 2.3 Software enables calculation of analyte concentration in the tested samples.

Two sets of beads with different sizes (4 μm & 5 μm) are used in the FlowCytomix assay.
Each of the two sizes consists of bead populations which are differentiated by varying intensities of an internally fluorescent dye.
The dye can be excited with an Argon, He-Ne, or even UV laser, and emits in the far red (690 nm) which is detected in the FL-3/FL-4 channel.
The combination of the two different bead sizes and different internal dye intensities makes it possible to distinguish up to 20 bead sets in one fluorescent channel.
Streptavidin-PE, which binds to the biotin conjugate, emits at 578 nm and is detected in the FL-2 channel and allows the quantification of the analyte.

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