Flow Cytometry: Applications Flashcards
Draw and label a diagram of the normal cell cycle.
Describe cell cycle analysis using flow cytometry, and some commonly used fluorochromes.
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Describe how flow cytometry can be used for assessment of cell viability, and some commonly used fluorochromes.
- Propidium iodide (PI) fluoresces when it binds to DNA
- PI can only cross the cell membrane of damaged or dead cells
- Thus PI can be used to distinguish between healthy and damaged/dead cells - i.e. it can be used to assess cell viability
What is apoptosis?
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Describe the techniques used to study apoptosis.
- Staining with the dye PI - cells fixed.
- Phosphatidyl serine can be detected by incubating the cells with fluorescein-labelled Annexin V and PI - FLAV binds to PS, which is only present on the extracellular membrane when a cell is undergoing apoptosis.
- Staining with 7-aminoactinomycin D - cells not fixed.
Describe how flow cytometry can be used for the quantitation of apoptosis, and some commonly used fluorochromes.
- Populations of live, early apoptotic and late apoptotic/necrotic cells can be quantitated at the same time using Annexin-V-FITC and PI.
- These 3 cell populations can be visualised on a dot-plot: live cells will be negative for both dyes, apoptotic will be positive for Annexin-V but not PI, and dead will be posititve for both.
Explain the reasons why different fluorochromes are used for cell cycle analysis, viability staining, and apoptosis quantitation.
- Cell cycle analysis - PI used to quantitate DNA
- Viability staining - cells that fluoresce with PI are damaged or dead
- Apoptosis quantitation - 3 methods: PI with fixed cells, Annexin V + PI (cells not fixed), 7-AAD (cells not fixed)
- Annexin V used to distinguish between early apoptotic, late apoptotic and dead cells
List some clinical and research aplications of flow cytometry.
- Immunophenotyping of leukaemias & lymphomas
- Detection of MRD
- Stem cell enumeration
- CD4/CD8 in HIV
- Measurement of intracellular cytokines
- Study of cell cycle, viability & apoptosis
- Measurement of cell proliferation
- Assessment of transfection efficiency
Outline the differences between flow cytometry and flow sorting.
- Flow cytometry used for comparing characteristics of different cell populations
- Flow sorting used to isolate highly purified (99% pure) populations of cells for analysis
Describe the basic instrumentation of a flow sorter.
Describe the principles of flow sorting.
- In flow sorting nozzle-tip vibrated at 1000s rpm
- This separates the stream containing cells into individual droplets which each contain one cell
- Electric charge is applied to the droplet containing the desired cells as they leave the stream
- Charged cells attracted to deflection plates and sorted into different tubes
- Flow sorting used to isolate purified cell populations
Explain when fluorescence-activated cell sorting (flow sorting) is used and describe some of its applications.
- Diagnostics - specific cell populations isolated for analysis, e.g. cancer cells, CD4/CD8 in HIV
- Allows immunophenotyping
- Stem cell enumeration - isolating and counting stem cells
What are the advantages of using 7-aminoactinomycin D (7-AAD) for quantitation of apoptotic cells?
- DNA-specific - intercalates in GC regions.
- Long emission wavelength - can easily be used with FITC and PE labelled Abs for simultaneous evaluation of DNA content and 2-colour immunofluorescence.
