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Published byClemence Wells Modified over 9 years ago
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FLOW CYTOMETRY Not as scary as it sounds!
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A BIT OF HOUSEKEEPING… About me! About you Institute Prior knowledge Core facility
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OVERVIEW Flow = fluid Cyto = cell Metry = measurement
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FORWARD SCATTER (FSC)
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SIDE SCATTER (SSC)
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FLUORESCENT MARKERS
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Size (FSC) Internal complexity (“granularity”) (SSC) Fluorescence intensity (“relative expression of marker”) {
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SAMPLE PREPARATION: PREWORK Choose your antibodies How many? Which fluorochromes? Will they need compensation? Which machine to use?
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BD FACSCANTO II FORTESSA X20
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Compensation? Nooooooo…
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Undercompensated Overcompensated Correctly compensated
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SAMPLE PREPARATION: STAINING a)Prepare FACS buffer b)Detach cells surface receptor? c)Resuspend cells min. 200,000 cells/tube, max 100 µl Unstained Isotype control (Compensation) Antibody/es d)Fc block
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e)Intracellular antigens only Fix: add 100 µl 4%PFA (30 min @ RT) 2x 1ml FACS wash Perm: 2x 2ml Permeabilisation buffer wash Resuspend 100 µl Perm buffer f)Antibody staining Add 10 µl Ab/10 6 cells Incubate 1h in the dark @ 4C (surface) or RT (intracellular) Wash 2x FACS buffer (surface) or 1x Perm buffer + 1x FACS buffer Resuspend in 200 µl FACS buffer g)(Beads) h)Analyse
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DATA ACQUISITION & ANALYSIS a)Set up experiment b)Acquire cells
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PE positive APC negative PE positive APC positive PE negative APC positive
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WHAT HAPPENED HERE? A) All cells are dead!
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B) Some of my cells are doublets Height Width Cells are growing / T-cell activation
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C) My cells are not displayed!
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D) Unstained and isotype weren’t fixed & permeabilised
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E) Cells are autofluorescent
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THIS IS BUT A SCRATCH… Cell identification Population sorting Cell proliferation Cell death Functional measurements (pH, Calcium) And more…
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THANK YOU! Questions?
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INTERESTED IN MORE? Theory behind flow: http://www.bdbiosciences.com/eu/s/training/e-learninghttp://www.bdbiosciences.com/eu/s/training/e-learning Design your experiment: https://fluorofinder.com/panels/newhttps://fluorofinder.com/panels/new http://m.bdbiosciences.com/us/s/spectrumviewer How to present flow data: http://www.ncbi.nlm.nih.gov/pubmed/18752282http://www.ncbi.nlm.nih.gov/pubmed/18752282
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