Intro to Flow Cytometry

Question 1

What is flow cytometry?

Answer 1

This is a technique which simultaneously measures several physical characteristics belonging to a single cell in suspension

Question 2

How are cells held in suspension and measured for flow cytometry?

Answer 2

This is done by light scatter and fluorescence

Question 3

What is the function of flow cytometry?

Answer 3

Flow Cytometry: Measuring properties of cells in flow

Question 4

What is the role of flow sorting?

Answer 4

Flow Sorting: Sorting (separating) cells based on properties measured in flow
Also called Fluorescence-Activated Cell Sorting (FACS)

Question 5

What information do we gain from a flow cytometer?

Answer 5

1. Its Relative Size
2. Its Relative Granularity/Internal Complexity
3. Its Relative Fluorescence Intensity

Question 6

What aspects of a cell can be measured using a flow cytometer?

Answer 6

Can measure anything on cell surface ie.

• receptors
• adhesion molecules etc.
• cytokines
• enzymes in cytoplasm

Can also interrogate cell DNA; cell cycle, cell viability & apoptosis

Question 7

What are the ways of visualising flow cytometer results?

Answer 7

• Fluorescence Microscopy

- Flow Cytometry

Question 8

Why is flow cytometery preferred over fluorescence microscopy?

Answer 8

• Flow cytometer is quick
• Quantitative
• Can find rare cells

Question 9

Why is fluorescence microscopy not a preferred method?

Answer 9

Can only view limited no. of cells in field view looking down a microscope

To find rare cells, need to interrogate thousands of field views

Microscopy not very quantitative as carried out by eye - subjective

Fluorescence varies in microscope marking - subjective

Question 10

What instrument is used to interrogate cells?

Answer 10

analyser used to interrogate cells

Question 11

What are the 3 compartments of the analysing machine?

Answer 11

The way the machine works is broken down into 3 compartments:

• Fluidics
• Optics
• Electronics

Question 12

Describe fluidics component of the analyser?

Answer 12

Fluidics

• Cells in suspension
• Flow in single-file through

Question 13

What are the optics in an analyser?

Answer 13

Optics

• an illuminated volume
• where they scatter light and emit fluorescence
• is collected, filtered

Question 14

Describe the electronic part of the analyser

Answer 14

Electronics

• converted to digital values
• that are stored on a computer

Question 15

How are cells required to be arranged in an analyser?

Answer 15

Need to have cells in suspension flow in single file

Question 16

How are cells kept in single file?

Answer 16

Accomplished by injecting sample into a sheath fluid as it passes through a small (50-300 µm) orifice

Question 17

Where in the analyser does the sample fluid flow?

Answer 17

Sample fluid flows in a central core that does not mix with the sheath fluid - Laminar flow

Question 18

What is hydrodynamic focusing?

Answer 18

Introduction of a large volume into a small volume

Question 19

Describe the flow of cells through the analyser

Answer 19

1. Cells flow through nozzle tip (small orifice)
   - forced to flow in single file due to sheath fluid flowing
   around sides: hydrodynamic focussing
2. Cells need to be single file for when laser hits
3. Laser hits, light scatters and picked up by the detectors

Question 20

What is a laser?

Answer 20

Single wavelength of light (a laser line) or (more rarely) a mixture of wavelengths

light source

Question 21

Describe the features of lasers

Answer 21

• can provide from milliwatts to watts of light
• can be inexpensive, air-cooled units or expensive, water-
  cooled units
• provide coherent light (Single frequency)

Question 22

What is the benefit of using laser as the light source?

Answer 22

Even without fluorescence and antibody marking, lasers provide a lot of info about the cells

Question 23

How does the laser provide cellular info?

Answer 23

Laser hits the cell and scatters light into 2 different directions:

• forward scatter
• side scatter

Question 24

What does forward light scatter tell us?

Answer 24

Forward light scatter = proportional to size of the cell

Question 25

What info do we gain from side scatter?

Answer 25

Side scatter 90° = proportional to granularity / internal complexity of the cell

Question 26

What does a white cell dot plot show us?

Answer 26

Every dot represents ‘an event’ (cell)
The screen is refreshed every second to show 1000s of cells

Just on basis of forwards and side scatter we can see distinctions between populations

Question 27

What do the axis on a white cell dot plot show?

Answer 27

X axis - increase in forward scatter

Y axis - increase in side scatter

Question 28

Describe the basic pattern of peripheral blood seen on a white cell dot plot

Answer 28

RBCs and debris in bottom left corner

lymphocytes v. small and not very granular

monocytes are bigger and granular

a large pop of neutrophils

Question 29

Describe laser-based flow cytometry

Answer 29

Cells labelled with fluorescently labelled antibodies
Lasers hit cells emerging from nozzle tip

Light emitted from cells and picked up by PMTs after light has travelled through mirrors and filters

Question 30

What are electronics of flow cytometry?

Answer 30

Processing of signals from detectors

Analog-Digital Conversion

Question 31

When does fluorescence occur?

Answer 31

Fluorescence occurs when fluorochrome is excited by a laser and returns to unexcited state via emission
⇒ emits fluorescence at a higher wavelength

Question 32

What is stokes shift?

Answer 32

Stokes Shift is the energy difference between the lowest energy peak of absorbance and the highest energy of emission

Question 33

Give examples of common fluorochromes and dyes

Answer 33

Green: Fluorescein isothiocyanate (FITC)

Orange: Phycoerythrin (PE)

Red: Peridinin Chlorophyll Protein (PerCP)

Question 34

How can we investigate different parameters at once?

Answer 34

As these fluorochromes emit at different wavelengths we can detect them all at the same time to investigate 3 different parameters at once

Question 35

What is the purpose of filters and mirrors in flow cytometry?

Answer 35

The broad emission spectra overlap which is why we require filters and mirrors to separate them out

Question 36

Give examples of good samples to use in flow cytometry

Answer 36

The following are good samples to use in a flow cytometer:

• Peripheral blood
• Bone marrow
• Fine Needle Aspirate
• CSF and other fluids
• Fresh Tissue

Question 37

What are the 2 immunofluorescence labelling methods?

Answer 37

• Direct

- Indirect

Question 38

What is the direct method of immunofluorescence?

Answer 38

Monoclonal antibodies (MoAbs) are pre conjugated to fluorochromes (simplest and cleanest way)

Question 39

Describe the indirect way of immunofluorescence labelling

Answer 39

Unconjugated MoAbs, require secondary Abs with flurocohrome

Question 40

How can we display the data collected from flow cytometry?

Answer 40

> 2 ways of displaying data

• Dot plot
• Histogram

Question 41

What is the use of dot plots?

Answer 41

Dot plot allows the visualization of 2 parameters at the same time
(forward and side scatter)

Question 42

How are histograms used?

Answer 42

Histogram only looks at one parameter

fluorescence intensity

Question 43

What info do dot plots show us?

Answer 43

Using 2D dot plot can identify 4 populations of cells:

• Double -ve for both
• Single +ve for FITC
• Single +ve for PE
• Double +ve for both

Can quantitate cells

Question 44

What is gating?

Answer 44

A way of manipulating data and displaying it to analyse it

Question 45

What is a common use of gating?

Answer 45

Drawing a region around lymphocytes and using CPU visualised those specific cells on basis of their 2 fluorochromes (CD3 FITC and CD4 PE)

Question 46

How do we analyse flow cytometry data?

Answer 46

Put markers on histograms and CPU machines quantitate the no. of cells

Draw quadrants to analyse proportion of cells in each quadrant

Question 47

How does the no. of fluorochromes used enable broader data range?

Answer 47

By increasing no. of fluorochromes to 3 we can identify up to 8 populations:
-ve for all 3
+ve for all 3
Or combinations in between

By increasing colours we can increase populations to analyse